---
OA_type: closed access
_id: '21762'
abstract:
- lang: eng
  text: Bacteria, like eukaryotes, use conserved cytoskeletal systems for intracellular
    organization. The plasmid-encoded ParMRC system forms actin-like filaments that
    segregate low–copy number plasmids. In multicellular cyanobacteria such as Anabaena
    sp., we found that a chromosomally encoded ParMR system has evolved into a cytoskeletal
    system named CorMR with a function in cell shape control rather than DNA segregation.
    Live-cell imaging, in vitro reconstitution, and cryo–electron microscopy revealed
    that CorM formed dynamically unstable, antiparallel double-stranded filaments
    that were recruited to the membrane by CorR through an amphipathic helix conserved
    in multicellular cyanobacteria. CorMR filaments were regulated by MinC, which
    excluded them from the poles and division plane. Comparative genomics indicated
    that the repurposing of ParMR and Min systems coevolved with cyanobacterial multicellularity,
    highlighting the evolutionary plasticity of cytoskeletal systems in bacteria.
acknowledged_ssus:
- _id: Bio
- _id: ScienComp
- _id: EM-Fac
- _id: LifeSc
acknowledgement: "We thank all members of the Loose lab at ISTA for helpful discussions;
  M. Kojic for critical reading of the manuscript; A. Herrero (Sevilla University)
  for sharing her extensive BACTH plasmid library and other plasmids, as well as cyanobacterial
  strains; T. Dagan and F. Nies (both Kiel University) for sharing cyanobacterial
  strains and plasmids and for valuable discussions; N. Sapay and A. Michon for providing
  the Amphipaseek code, which enabled us to perform our large-scale amphipathic helix
  screen of cyanobacterial CorR proteins; V.-V. Hodirnau for support in cryo-ET data
  collection; and J. Hansen for advice about cryo-EM data processing.\r\nThis work
  was supported by the Scientific Service Units (SSU) of ISTA through resources provided
  by the Imaging & Optics Facility (IOF), the Scientific Computing (SciComp), the
  Electron Microscopy Facility (EMF), and the Lab Support Facility (LSF). This work
  was funded by the European Union’s Horizon 2020 research and innovation program
  (Marie Skłodowska-Curie grant 101034413 to B.L.S.); the European Research Council
  (ERC) of the European Union (grant ActinID 101076260 to F.K.M.S.); the Swiss National
  Science Foundation (starting grant TMSGI3_226208 to G.L.W.); and the Jean-Jacques
  et Letitia Lopez-Loreta Foundation (G.L.W.)."
article_number: eaea6343
article_processing_charge: No
article_type: original
author:
- first_name: Benjamin L
  full_name: Springstein, Benjamin L
  id: b4eb62ef-ac72-11ed-9503-ed3b4d66c083
  last_name: Springstein
  orcid: 0000-0002-3461-5391
- first_name: Manjunath
  full_name: Javoor, Manjunath
  id: 305ab18b-dc7d-11ea-9b2f-b58195228ea2
  last_name: Javoor
  orcid: 0000-0003-2311-2112
- first_name: Daniela
  full_name: Megrian, Daniela
  last_name: Megrian
- first_name: Roman
  full_name: Hajdu, Roman
  id: ffab949d-133f-11ed-8f02-94de21ace503
  last_name: Hajdu
- first_name: Dustin M.
  full_name: Hanke, Dustin M.
  last_name: Hanke
- first_name: Bettina
  full_name: Zens, Bettina
  id: 45FD126C-F248-11E8-B48F-1D18A9856A87
  last_name: Zens
  orcid: 0000-0002-9561-1239
- first_name: Gregor L.
  full_name: Weiss, Gregor L.
  last_name: Weiss
- first_name: Florian Km
  full_name: Schur, Florian Km
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Martin
  full_name: Loose, Martin
  id: 462D4284-F248-11E8-B48F-1D18A9856A87
  last_name: Loose
  orcid: 0000-0001-7309-9724
citation:
  ama: Springstein BL, Javoor M, Megrian D, et al. Repurposing of a DNA segregation
    machinery into a cytoskeletal system controlling cell shape. <i>Science</i>. 2026;392(6795).
    doi:<a href="https://doi.org/10.1126/science.aea6343">10.1126/science.aea6343</a>
  apa: Springstein, B. L., Javoor, M., Megrian, D., Hajdu, R., Hanke, D. M., Zens,
    B., … Loose, M. (2026). Repurposing of a DNA segregation machinery into a cytoskeletal
    system controlling cell shape. <i>Science</i>. AAAS. <a href="https://doi.org/10.1126/science.aea6343">https://doi.org/10.1126/science.aea6343</a>
  chicago: Springstein, Benjamin L, Manjunath Javoor, Daniela Megrian, Roman Hajdu,
    Dustin M. Hanke, Bettina Zens, Gregor L. Weiss, Florian KM Schur, and Martin Loose.
    “Repurposing of a DNA Segregation Machinery into a Cytoskeletal System Controlling
    Cell Shape.” <i>Science</i>. AAAS, 2026. <a href="https://doi.org/10.1126/science.aea6343">https://doi.org/10.1126/science.aea6343</a>.
  ieee: B. L. Springstein <i>et al.</i>, “Repurposing of a DNA segregation machinery
    into a cytoskeletal system controlling cell shape,” <i>Science</i>, vol. 392,
    no. 6795. AAAS, 2026.
  ista: Springstein BL, Javoor M, Megrian D, Hajdu R, Hanke DM, Zens B, Weiss GL,
    Schur FK, Loose M. 2026. Repurposing of a DNA segregation machinery into a cytoskeletal
    system controlling cell shape. Science. 392(6795), eaea6343.
  mla: Springstein, Benjamin L., et al. “Repurposing of a DNA Segregation Machinery
    into a Cytoskeletal System Controlling Cell Shape.” <i>Science</i>, vol. 392,
    no. 6795, eaea6343, AAAS, 2026, doi:<a href="https://doi.org/10.1126/science.aea6343">10.1126/science.aea6343</a>.
  short: B.L. Springstein, M. Javoor, D. Megrian, R. Hajdu, D.M. Hanke, B. Zens, G.L.
    Weiss, F.K. Schur, M. Loose, Science 392 (2026).
corr_author: '1'
date_created: 2026-04-26T22:01:46Z
date_published: 2026-04-16T00:00:00Z
date_updated: 2026-04-28T13:29:05Z
day: '16'
department:
- _id: MaLo
- _id: FlSc
- _id: GradSch
- _id: EM-Fac
doi: 10.1126/science.aea6343
ec_funded: 1
external_id:
  pmid:
  - '41990175'
intvolume: '       392'
issue: '6795'
language:
- iso: eng
month: '04'
oa_version: None
pmid: 1
project:
- _id: fc2ed2f7-9c52-11eb-aca3-c01059dda49c
  call_identifier: H2020
  grant_number: '101034413'
  name: 'IST-BRIDGE: International postdoctoral program'
- _id: bd980d18-d553-11ed-ba76-ceaa645c97eb
  grant_number: '101076260'
  name: A molecular atlas of Actin filament IDentities in the cell motility machinery
publication: Science
publication_identifier:
  eissn:
  - 1095-9203
  issn:
  - 0036-8075
publication_status: published
publisher: AAAS
quality_controlled: '1'
scopus_import: '1'
status: public
title: Repurposing of a DNA segregation machinery into a cytoskeletal system controlling
  cell shape
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 392
year: '2026'
...
---
DOAJ_listed: '1'
OA_place: publisher
OA_type: gold
PlanS_conform: '1'
_id: '20370'
abstract:
- lang: eng
  text: The Huntingtin protein (HTT), named for its role in Huntington’s disease,
    has been best understood as a scaffolding protein that promotes vesicle transport
    by molecular motors along microtubules. Here, we show that HTT also interacts
    with the actin cytoskeleton, and its loss of function disturbs the morphology
    and function of the axonal growth cone. We demonstrate that HTT organizes F-actin
    into bundles. Cryo–electron tomography (cryo-ET) and subtomogram averaging (STA)
    structural analyses reveal that HTT’s N-terminal HEAT and Bridge domains wrap
    around F-actin, while the C-terminal HEAT domain is displaced; furthermore, HTT
    dimerizes via the N-HEAT domain to bridge parallel actin filaments separated by
    ~20 nanometers. Our study provides the structural basis for understanding how
    HTT interacts with and organizes the actin cytoskeleton.
acknowledgement: 'We thank C. Cuveillier, J. Delaroche, T. Ferraro, and A. Zanchi
  for help with TIRF experiments, electron microscopy preparation, data analysis,
  and cell cultures, respectively; A. Antkowiak, C. Bosc, C. Fassier, A. Fourest-Lieuvin,
  and V. Brandt for helpful discussions. We acknowledge the contribution of the Photonic
  Imaging Center of Grenoble Institute Neuroscience which is part of the ISdV core
  facility and certified by the IBiSA label and ICM.Quant (RRID:SCR_026393) core facility
  of the Paris Brain Institute (ICM); the AniRA lentivector production facility from
  the CELPHEDIA Infrastructure and SFR Biosciences (UAR3444/CNRS, US8/Inserm, ENS
  de Lyon, UCBL); the Scientific Service Units (SSUs) of ISTA through resources provided
  by Scientific Computing (SciComp, A. Schloegl and S. Elefante); and the Electron
  Microscopy Facility (EMF, V.V. Hodirnau). The software programs used for the processing
  were supported by SBGrid (www.sbgrid.org). This work was supported by the Agence
  Nationale pour la Recherche (AXYON: ANR-18-CE16-0009-01, S.H.), Austrian Science
  Fund (FWF) grants (P33367, F.K.M.S.; E435, J.M.H.), ChanZuckerberg Initiative (CZI)
  grant (DAF2021-234754, F.K.M.S.), Hereditary Disease Foundation Research Grant (HDF
  990846, M.C.), European Union (ERC: ActinID 101076260, F.K.M.S.), Fondation pour
  la Recherche Médicale (FRM: équipe labellisée DEQ202203014675, S.H.; PhD fellowship,
  FDT202001010865, R.C.), Korea Health Industry Development Institute (KHIDI) (Korea-Switzerland
  global research support grant: RS-2023-00266300, J.-J.S.), National Research Foundation
  (NRF) of Korea (Korea-Austria collaborative grant NRF-2019K1A3A1A181160, J.-J.S.
  and F.K.M.S.; NRF-2020R1A2B5B03001517 and RS-2024-00333346 and RS-2024-00436173,
  J.-J.S.; 2021R1C1C1006700, D.K.).'
article_number: eadw4124
article_processing_charge: Yes
article_type: original
author:
- first_name: Rémi
  full_name: Carpentier, Rémi
  last_name: Carpentier
- first_name: Jaesung
  full_name: Kim, Jaesung
  last_name: Kim
- first_name: Mariacristina
  full_name: Capizzi, Mariacristina
  last_name: Capizzi
- first_name: Hyeongju
  full_name: Kim, Hyeongju
  last_name: Kim
- first_name: Florian
  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Jesse
  full_name: Hansen, Jesse
  id: 1063c618-6f9b-11ec-9123-f912fccded63
  last_name: Hansen
  orcid: 0000-0001-7967-2085
- first_name: Min Jeong
  full_name: Kim, Min Jeong
  last_name: Kim
- first_name: Eric
  full_name: Denarier, Eric
  last_name: Denarier
- first_name: Béatrice
  full_name: Blot, Béatrice
  last_name: Blot
- first_name: Marine
  full_name: Degennaro, Marine
  last_name: Degennaro
- first_name: Sophia
  full_name: Labou, Sophia
  last_name: Labou
- first_name: Isabelle
  full_name: Arnal, Isabelle
  last_name: Arnal
- first_name: Maria J.
  full_name: Marcaida, Maria J.
  last_name: Marcaida
- first_name: Matteo Dal
  full_name: Peraro, Matteo Dal
  last_name: Peraro
- first_name: Doory
  full_name: Kim, Doory
  last_name: Kim
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Ji-Joon
  full_name: Song, Ji-Joon
  last_name: Song
- first_name: Sandrine
  full_name: Humbert, Sandrine
  last_name: Humbert
citation:
  ama: Carpentier R, Kim J, Capizzi M, et al. Structure of the Huntingtin F-actin
    complex reveals its role in cytoskeleton organization. <i>Science Advances</i>.
    2025;11(38). doi:<a href="https://doi.org/10.1126/sciadv.adw4124">10.1126/sciadv.adw4124</a>
  apa: Carpentier, R., Kim, J., Capizzi, M., Kim, H., Fäßler, F., Hansen, J., … Humbert,
    S. (2025). Structure of the Huntingtin F-actin complex reveals its role in cytoskeleton
    organization. <i>Science Advances</i>. AAAS. <a href="https://doi.org/10.1126/sciadv.adw4124">https://doi.org/10.1126/sciadv.adw4124</a>
  chicago: Carpentier, Rémi, Jaesung Kim, Mariacristina Capizzi, Hyeongju Kim, Florian
    Fäßler, Jesse Hansen, Min Jeong Kim, et al. “Structure of the Huntingtin F-Actin
    Complex Reveals Its Role in Cytoskeleton Organization.” <i>Science Advances</i>.
    AAAS, 2025. <a href="https://doi.org/10.1126/sciadv.adw4124">https://doi.org/10.1126/sciadv.adw4124</a>.
  ieee: R. Carpentier <i>et al.</i>, “Structure of the Huntingtin F-actin complex
    reveals its role in cytoskeleton organization,” <i>Science Advances</i>, vol.
    11, no. 38. AAAS, 2025.
  ista: Carpentier R, Kim J, Capizzi M, Kim H, Fäßler F, Hansen J, Kim MJ, Denarier
    E, Blot B, Degennaro M, Labou S, Arnal I, Marcaida MJ, Peraro MD, Kim D, Schur
    FK, Song J-J, Humbert S. 2025. Structure of the Huntingtin F-actin complex reveals
    its role in cytoskeleton organization. Science Advances. 11(38), eadw4124.
  mla: Carpentier, Rémi, et al. “Structure of the Huntingtin F-Actin Complex Reveals
    Its Role in Cytoskeleton Organization.” <i>Science Advances</i>, vol. 11, no.
    38, eadw4124, AAAS, 2025, doi:<a href="https://doi.org/10.1126/sciadv.adw4124">10.1126/sciadv.adw4124</a>.
  short: R. Carpentier, J. Kim, M. Capizzi, H. Kim, F. Fäßler, J. Hansen, M.J. Kim,
    E. Denarier, B. Blot, M. Degennaro, S. Labou, I. Arnal, M.J. Marcaida, M.D. Peraro,
    D. Kim, F.K. Schur, J.-J. Song, S. Humbert, Science Advances 11 (2025).
corr_author: '1'
date_created: 2025-09-22T08:00:52Z
date_published: 2025-09-19T00:00:00Z
date_updated: 2026-02-16T11:45:54Z
day: '19'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.1126/sciadv.adw4124
external_id:
  isi:
  - '001575751700013'
  pmid:
  - '40971423'
file:
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  checksum: 4e2407bdabf8d53f399eb8a20d86218e
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  creator: dernst
  date_created: 2025-09-23T07:57:51Z
  date_updated: 2025-09-23T07:57:51Z
  file_id: '20372'
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  file_size: 3599137
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file_date_updated: 2025-09-23T07:57:51Z
has_accepted_license: '1'
intvolume: '        11'
isi: 1
issue: '38'
language:
- iso: eng
month: '09'
oa: 1
oa_version: Published Version
pmid: 1
project:
- _id: 9B954C5C-BA93-11EA-9121-9846C619BF3A
  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
- _id: 7bd318a1-9f16-11ee-852c-cc9217763180
  grant_number: E435
  name: In Situ Actin Structures via Hybrid Cryo-electron Microscopy
- _id: 62909c6f-2b32-11ec-9570-e1476aab5308
  grant_number: CZI01
  name: CryoMinflux-guided in-situ molecular census and structure determination
- _id: bd980d18-d553-11ed-ba76-ceaa645c97eb
  grant_number: '101076260'
  name: A molecular atlas of Actin filament IDentities in the cell motility machinery
publication: Science Advances
publication_identifier:
  issn:
  - 2375-2548
publication_status: published
publisher: AAAS
quality_controlled: '1'
scopus_import: '1'
status: public
title: Structure of the Huntingtin F-actin complex reveals its role in cytoskeleton
  organization
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 11
year: '2025'
...
---
APC_amount: 12348 EUR
OA_place: publisher
OA_type: hybrid
_id: '17884'
abstract:
- lang: eng
  text: Human T cell leukemia virus type 1 (HTLV-1) immature particles differ in morphology
    from other retroviruses, suggesting a distinct way of assembly. Here we report
    the results of cryo-electron tomography studies of HTLV-1 virus-like particles
    assembled in vitro, as well as derived from cells. This work shows that HTLV-1
    uses a distinct mechanism of Gag–Gag interactions to form the immature viral lattice.
    Analysis of high-resolution structural information from immature capsid (CA) tubular
    arrays reveals that the primary stabilizing component in HTLV-1 is the N-terminal
    domain of CA. Mutagenesis analysis supports this observation. This distinguishes
    HTLV-1 from other retroviruses, in which the stabilization is provided primarily
    by the C-terminal domain of CA. These results provide structural details of the
    quaternary arrangement of Gag for an immature deltaretrovirus and this helps explain
    why HTLV-1 particles are morphologically distinct.
acknowledged_ssus:
- _id: ScienComp
- _id: LifeSc
- _id: EM-Fac
acknowledgement: This work was funded by the Institute of Science and Technology Austria
  (ISTA) and the Austrian Science Fund (grant P31445 to F.K.M.S.). Access to high-resolution
  cryo-ET data acquisition at European Molecular Biology Laboratory (EMBL) Heidelberg
  was supported through the EMBL cryo-EM platform. We thank V.-V. Hodirnau at ISTA
  and W. Hagen and F. Weis at EMBL Heidelberg for support in cryo-ET data acquisition.
  This research was also supported by the scientific service units of ISTA through
  resources provided by Scientific Computing, the Life Science Facility, and the EM
  Facility. L.M.M. was supported by National Institutes of Health grants R01 GM151775
  and R21 DE032878 and by the University of Minnesota Masonic Cancer Center. D.P.
  was supported by the DOC doctoral fellowship program of the Austrian Academy of
  Sciences. R.A.D was supported by the National Institute of Allergy and Infectious
  Diseases (grant R01AI147890). The funders had no role in study design, data collection
  and analysis, decision to publish or preparation of the manuscript. Specifically,
  we also want to thank A. Schlögl for computational support and J. Hansen and V.
  Vogt for critical comments on the manuscript. We also thank the other members of
  the Schur lab for helpful discussions and experimental advice.
article_processing_charge: Yes (in subscription journal)
article_type: original
author:
- first_name: Martin
  full_name: Obr, Martin
  id: 4741CA5A-F248-11E8-B48F-1D18A9856A87
  last_name: Obr
  orcid: 0000-0003-1756-6564
- first_name: Mathias
  full_name: Percipalle, Mathias
  id: 4986e21c-eb97-11eb-a6c2-a4ef0b629971
  last_name: Percipalle
- first_name: Darya
  full_name: Chernikova, Darya
  id: 7dbaf460-fa9e-11eb-b0ca-bc7c7ff21ad0
  last_name: Chernikova
- first_name: Huixin
  full_name: Yang, Huixin
  last_name: Yang
- first_name: Andreas
  full_name: Thader, Andreas
  id: 3A18A7B8-F248-11E8-B48F-1D18A9856A87
  last_name: Thader
- first_name: Gergely
  full_name: Pinke, Gergely
  id: 4D5303E6-F248-11E8-B48F-1D18A9856A87
  last_name: Pinke
- first_name: Dario J
  full_name: Porley, Dario J
  id: 2FD6EA6C-F248-11E8-B48F-1D18A9856A87
  last_name: Porley
- first_name: Louis M.
  full_name: Mansky, Louis M.
  last_name: Mansky
- first_name: Robert A.
  full_name: Dick, Robert A.
  last_name: Dick
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Obr M, Percipalle M, Chernikova D, et al. Distinct stabilization of the human
    T cell leukemia virus type 1 immature Gag lattice. <i>Nature Structural &#38;
    Molecular Biology</i>. 2025;32:268-276. doi:<a href="https://doi.org/10.1038/s41594-024-01390-8">10.1038/s41594-024-01390-8</a>
  apa: Obr, M., Percipalle, M., Chernikova, D., Yang, H., Thader, A., Pinke, G., …
    Schur, F. K. (2025). Distinct stabilization of the human T cell leukemia virus
    type 1 immature Gag lattice. <i>Nature Structural &#38; Molecular Biology</i>.
    Springer Nature. <a href="https://doi.org/10.1038/s41594-024-01390-8">https://doi.org/10.1038/s41594-024-01390-8</a>
  chicago: Obr, Martin, Mathias Percipalle, Darya Chernikova, Huixin Yang, Andreas
    Thader, Gergely Pinke, Darío Porley Esteves, Louis M. Mansky, Robert A. Dick,
    and Florian KM Schur. “Distinct Stabilization of the Human T Cell Leukemia Virus
    Type 1 Immature Gag Lattice.” <i>Nature Structural &#38; Molecular Biology</i>.
    Springer Nature, 2025. <a href="https://doi.org/10.1038/s41594-024-01390-8">https://doi.org/10.1038/s41594-024-01390-8</a>.
  ieee: M. Obr <i>et al.</i>, “Distinct stabilization of the human T cell leukemia
    virus type 1 immature Gag lattice,” <i>Nature Structural &#38; Molecular Biology</i>,
    vol. 32. Springer Nature, pp. 268–276, 2025.
  ista: Obr M, Percipalle M, Chernikova D, Yang H, Thader A, Pinke G, Porley Esteves
    D, Mansky LM, Dick RA, Schur FK. 2025. Distinct stabilization of the human T cell
    leukemia virus type 1 immature Gag lattice. Nature Structural &#38; Molecular
    Biology. 32, 268–276.
  mla: Obr, Martin, et al. “Distinct Stabilization of the Human T Cell Leukemia Virus
    Type 1 Immature Gag Lattice.” <i>Nature Structural &#38; Molecular Biology</i>,
    vol. 32, Springer Nature, 2025, pp. 268–76, doi:<a href="https://doi.org/10.1038/s41594-024-01390-8">10.1038/s41594-024-01390-8</a>.
  short: M. Obr, M. Percipalle, D. Chernikova, H. Yang, A. Thader, G. Pinke, D. Porley
    Esteves, L.M. Mansky, R.A. Dick, F.K. Schur, Nature Structural &#38; Molecular
    Biology 32 (2025) 268–276.
corr_author: '1'
date_created: 2024-09-08T10:29:06Z
date_published: 2025-02-01T00:00:00Z
date_updated: 2026-03-16T12:55:18Z
day: '01'
ddc:
- '570'
department:
- _id: FlSc
- _id: LeSa
doi: 10.1038/s41594-024-01390-8
external_id:
  isi:
  - '001306564000001'
  oaworkid:
  - W4402316284
  pmid:
  - '39242978'
file:
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  checksum: c641ad94afb28917b20425db676fc3ee
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  creator: dernst
  date_created: 2025-04-23T07:02:33Z
  date_updated: 2025-04-23T07:02:33Z
  file_id: '19608'
  file_name: 2025_NatureStrucBio_Obr.pdf
  file_size: 13724041
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file_date_updated: 2025-04-23T07:02:33Z
has_accepted_license: '1'
intvolume: '        32'
isi: 1
language:
- iso: eng
month: '02'
oa: 1
oa_version: Published Version
oaworkid: 1
page: 268-276
pmid: 1
project:
- _id: 26736D6A-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: P31445
  name: Structural conservation and diversity in retroviral capsid
- _id: 9B9C98E0-BA93-11EA-9121-9846C619BF3A
  grant_number: '25762'
  name: Structural characterization of spumavirus capsid assemblies to understand
    conserved Ortervirales assembly mechanisms
publication: Nature Structural & Molecular Biology
publication_identifier:
  eissn:
  - 1545-9985
  issn:
  - 1545-9993
publication_status: published
publisher: Springer Nature
quality_controlled: '1'
scopus_import: '1'
status: public
title: Distinct stabilization of the human T cell leukemia virus type 1 immature Gag
  lattice
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 32
year: '2025'
...
---
DOAJ_listed: '1'
OA_place: publisher
OA_type: gold
_id: '19795'
abstract:
- lang: eng
  text: Super-resolution microscopy often entails long acquisition times of minutes
    to hours. Since drifts during the acquisition adversely affect data quality, active
    sample stabilization is commonly used for some of these techniques to reach their
    full potential. Although drifts in the lateral plane can often be corrected after
    acquisition, this is not always possible or may come with drawbacks. Therefore,
    it is appealing to stabilize sample position in three dimensions (3D) during acquisition.
    Various schemes for active sample stabilization have been demonstrated previously,
    with some reaching sub-nanometer stability in 3D. Here, we present a scheme for
    active drift correction that delivers the nanometer-scale 3D stability demanded
    by state-of-the-art super-resolution techniques and is straightforward to implement
    compared to previous schemes capable of reaching this level of stabilization precision.
    Using a refined algorithm that can handle various types of reference structure,
    without sparse signal peaks being mandatory, we stabilized sample position to
    ∼1 nm in 3D using objective lenses both with high and low numerical aperture.
    Our implementation requires only the addition of a simple widefield imaging path
    and we provide an open-source control software with graphical user interface to
    facilitate easy adoption of the module. Finally, we demonstrate how this has the
    potential to enhance data collection for diffraction-limited and super-resolution
    imaging techniques using single-molecule localization microscopy and cryo-confocal
    imaging as showcases.
acknowledged_ssus:
- _id: M-Shop
- _id: EM-Fac
- _id: LifeSc
acknowledgement: 'We acknowledge expert support by ISTA’s scientific service units,
  including the Miba Machine Shop, the Electron Microscopy Facility, and the Lab Support
  Facility. This work has been made possible in part by CZI grant DAF2021-234754 and
  grant DOI: https://doi.org/10.37921/812628ebpcwg from the Chan Zuckerberg Initiative
  DAF, an advised fund of Silicon Valley Community Foundation (funder DOI: https://doi.org/10.13039/100014989)
  (F.K.M.S. and J.G.D.). We further gratefully acknowledge funding by the following
  sources: Austrian Science Fund (FWF) grant DK W1232 (M.R.T. and J.G.D.); Austrian
  Academy of Sciences DOC fellowship 26137 (M.R.T.); Marie Skłodowska-Curie Actions
  Fellowship GA no. 665385 under the EU Horizon 2020 program (J.L.); ISTA postdoctoral
  fellowship IST fellow (A.W.); and Human Frontier Science Program postdoctoral fellowship
  LT000557/2018 (W.J.).'
article_number: '100211'
article_processing_charge: Yes
article_type: original
author:
- first_name: Jakob
  full_name: Vorlaufer, Jakob
  id: 937696FA-C996-11E9-8C7C-CF13E6697425
  last_name: Vorlaufer
  orcid: 0009-0000-7590-3501
- first_name: Nikolai
  full_name: Semenov, Nikolai
  id: e64d39c7-72ef-11ef-b75a-ee3046860d1b
  last_name: Semenov
- first_name: Caroline
  full_name: Kreuzinger, Caroline
  id: 382077BA-F248-11E8-B48F-1D18A9856A87
  last_name: Kreuzinger
- first_name: Manjunath
  full_name: Javoor, Manjunath
  id: 305ab18b-dc7d-11ea-9b2f-b58195228ea2
  last_name: Javoor
  orcid: 0000-0003-2311-2112
- first_name: Bettina
  full_name: Zens, Bettina
  id: 45FD126C-F248-11E8-B48F-1D18A9856A87
  last_name: Zens
  orcid: 0000-0002-9561-1239
- first_name: Nathalie
  full_name: Agudelo Duenas, Nathalie
  id: 40E7F008-F248-11E8-B48F-1D18A9856A87
  last_name: Agudelo Duenas
- first_name: Mojtaba
  full_name: Tavakoli, Mojtaba
  id: 3A0A06F4-F248-11E8-B48F-1D18A9856A87
  last_name: Tavakoli
  orcid: 0000-0002-7667-6854
- first_name: Marek
  full_name: Suplata, Marek
  id: EE8452B8-C26A-11E9-B157-E80CE6697425
  last_name: Suplata
- first_name: Wiebke
  full_name: Jahr, Wiebke
  id: 425C1CE8-F248-11E8-B48F-1D18A9856A87
  last_name: Jahr
  orcid: 0000-0003-0201-2315
- first_name: Julia
  full_name: Lyudchik, Julia
  id: 46E28B80-F248-11E8-B48F-1D18A9856A87
  last_name: Lyudchik
- first_name: Andreas
  full_name: Wartak, Andreas
  id: 60aaa06c-3de5-11eb-9e53-baa88e955dcb
  last_name: Wartak
- first_name: Florian Km
  full_name: Schur, Florian Km
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Johann G
  full_name: Danzl, Johann G
  id: 42EFD3B6-F248-11E8-B48F-1D18A9856A87
  last_name: Danzl
  orcid: 0000-0001-8559-3973
citation:
  ama: Vorlaufer J, Semenov N, Kreuzinger C, et al. Image-based 3D active sample stabilization
    on the nanometer scale for optical microscopy. <i>Biophysical Reports</i>. 2025;5(2).
    doi:<a href="https://doi.org/10.1016/j.bpr.2025.100211">10.1016/j.bpr.2025.100211</a>
  apa: Vorlaufer, J., Semenov, N., Kreuzinger, C., Javoor, M., Zens, B., Agudelo Duenas,
    N., … Danzl, J. G. (2025). Image-based 3D active sample stabilization on the nanometer
    scale for optical microscopy. <i>Biophysical Reports</i>. Elsevier. <a href="https://doi.org/10.1016/j.bpr.2025.100211">https://doi.org/10.1016/j.bpr.2025.100211</a>
  chicago: Vorlaufer, Jakob, Nikolai Semenov, Caroline Kreuzinger, Manjunath Javoor,
    Bettina Zens, Nathalie Agudelo Duenas, Mojtaba Tavakoli, et al. “Image-Based 3D
    Active Sample Stabilization on the Nanometer Scale for Optical Microscopy.” <i>Biophysical
    Reports</i>. Elsevier, 2025. <a href="https://doi.org/10.1016/j.bpr.2025.100211">https://doi.org/10.1016/j.bpr.2025.100211</a>.
  ieee: J. Vorlaufer <i>et al.</i>, “Image-based 3D active sample stabilization on
    the nanometer scale for optical microscopy,” <i>Biophysical Reports</i>, vol.
    5, no. 2. Elsevier, 2025.
  ista: Vorlaufer J, Semenov N, Kreuzinger C, Javoor M, Zens B, Agudelo Duenas N,
    Tavakoli M, Suplata M, Jahr W, Lyudchik J, Wartak A, Schur FK, Danzl JG. 2025.
    Image-based 3D active sample stabilization on the nanometer scale for optical
    microscopy. Biophysical Reports. 5(2), 100211.
  mla: Vorlaufer, Jakob, et al. “Image-Based 3D Active Sample Stabilization on the
    Nanometer Scale for Optical Microscopy.” <i>Biophysical Reports</i>, vol. 5, no.
    2, 100211, Elsevier, 2025, doi:<a href="https://doi.org/10.1016/j.bpr.2025.100211">10.1016/j.bpr.2025.100211</a>.
  short: J. Vorlaufer, N. Semenov, C. Kreuzinger, M. Javoor, B. Zens, N. Agudelo Duenas,
    M. Tavakoli, M. Suplata, W. Jahr, J. Lyudchik, A. Wartak, F.K. Schur, J.G. Danzl,
    Biophysical Reports 5 (2025).
corr_author: '1'
date_created: 2025-06-08T22:01:22Z
date_published: 2025-06-11T00:00:00Z
date_updated: 2026-04-07T11:48:07Z
day: '11'
ddc:
- '570'
department:
- _id: JoDa
- _id: GradSch
- _id: FlSc
- _id: EM-Fac
doi: 10.1016/j.bpr.2025.100211
ec_funded: 1
file:
- access_level: open_access
  checksum: 4018c833f25a3ad3b57e3577fed70334
  content_type: application/pdf
  creator: dernst
  date_created: 2025-06-10T07:24:46Z
  date_updated: 2025-06-10T07:24:46Z
  file_id: '19802'
  file_name: 2025_BiophysicalReports_Vorlaufer.pdf
  file_size: 7238179
  relation: main_file
  success: 1
file_date_updated: 2025-06-10T07:24:46Z
has_accepted_license: '1'
intvolume: '         5'
issue: '2'
language:
- iso: eng
month: '06'
oa: 1
oa_version: Published Version
project:
- _id: 62909c6f-2b32-11ec-9570-e1476aab5308
  grant_number: CZI01
  name: CryoMinflux-guided in-situ molecular census and structure determination
- _id: 6285a163-2b32-11ec-9570-8e204ca2dba5
  grant_number: '26137'
  name: Studying Organelle Structure and Function at Nanoscale Resolution with Expansion
    Microscopy
- _id: 2564DBCA-B435-11E9-9278-68D0E5697425
  call_identifier: H2020
  grant_number: '665385'
  name: International IST Doctoral Program
- _id: 26AA4EF2-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: W1232-B24
  name: Molecular Drug Targets
- _id: 2668BFA0-B435-11E9-9278-68D0E5697425
  grant_number: LT00057
  name: High-speed 3D-nanoscopy to study the role of adhesion during 3D cell migration
publication: Biophysical Reports
publication_identifier:
  eissn:
  - 2667-0747
publication_status: published
publisher: Elsevier
quality_controlled: '1'
related_material:
  record:
  - id: '20206'
    relation: dissertation_contains
    status: public
scopus_import: '1'
status: public
title: Image-based 3D active sample stabilization on the nanometer scale for optical
  microscopy
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 5
year: '2025'
...
---
_id: '15146'
abstract:
- lang: eng
  text: The extracellular matrix (ECM) serves as a scaffold for cells and plays an
    essential role in regulating numerous cellular processes, including cell migration
    and proliferation. Due to limitations in specimen preparation for conventional
    room-temperature electron microscopy, we lack structural knowledge on how ECM
    components are secreted, remodeled, and interact with surrounding cells. We have
    developed a 3D-ECM platform compatible with sample thinning by cryo-focused ion
    beam milling, the lift-out extraction procedure, and cryo-electron tomography.
    Our workflow implements cell-derived matrices (CDMs) grown on EM grids, resulting
    in a versatile tool closely mimicking ECM environments. This allows us to visualize
    ECM for the first time in its hydrated, native context. Our data reveal an intricate
    network of extracellular fibers, their positioning relative to matrix-secreting
    cells, and previously unresolved structural entities. Our workflow and results
    add to the structural atlas of the ECM, providing novel insights into its secretion
    and assembly.
acknowledged_ssus:
- _id: LifeSc
- _id: ScienComp
- _id: EM-Fac
- _id: M-Shop
acknowledgement: "Open Access funding provided by IST Austria. We thank Armel Nicolas
  and his team at the ISTA proteomics facility, Alois Schloegl, Stefano Elefante,
  and colleagues at the ISTA Scientific Computing facility, Tommaso Constanzo and
  Ludek Lovicar at the Electron Microsocpy Facility (EMF), and Thomas Menner at the
  Miba Machine shop for their support. We also thank Wanda Kukulski (University of
  Bern) as well as Darío Porley, Andreas Thader, and other members of the Schur group
  for helpful discussions. Matt Swulius and Jessica Heebner provided great support
  in using Dragonfly. We thank Dorotea Fracciolla (Art & Science) for support in figure
  illustration.\r\n\r\nThis research was supported by the Scientific Service Units
  of ISTA through resources provided by Scientific Computing, the Lab Support Facility,
  and the Electron Microscopy Facility. We acknowledge funding support from the following
  sources: Austrian Science Fund (FWF) grant P33367 (to F.K.M. Schur), the Federation
  of European Biochemical Societies (to F.K.M. Schur), Niederösterreich (NÖ) Fonds
  (to B. Zens), FWF grant E435 (to J.M. Hansen), European Research Council under the
  European Union’s Horizon 2020 research (grant agreement No. 724373) (to M. Sixt),
  and Jenny and Antti Wihuri Foundation (to J. Alanko). This publication has been
  made possible in part by CZI grant DAF2021-234754 and grant DOI https://doi.org/10.37921/812628ebpcwg
  from the Chan Zuckerberg Initiative DAF, an advised fund of Silicon Valley Community
  Foundation (to F.K.M. Schur)."
article_number: e202309125
article_processing_charge: Yes (via OA deal)
article_type: original
author:
- first_name: Bettina
  full_name: Zens, Bettina
  id: 45FD126C-F248-11E8-B48F-1D18A9856A87
  last_name: Zens
  orcid: 0000-0002-9561-1239
- first_name: Florian
  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Jesse
  full_name: Hansen, Jesse
  id: 1063c618-6f9b-11ec-9123-f912fccded63
  last_name: Hansen
  orcid: 0000-0001-7967-2085
- first_name: Robert
  full_name: Hauschild, Robert
  id: 4E01D6B4-F248-11E8-B48F-1D18A9856A87
  last_name: Hauschild
  orcid: 0000-0001-9843-3522
- first_name: Julia
  full_name: Datler, Julia
  id: 3B12E2E6-F248-11E8-B48F-1D18A9856A87
  last_name: Datler
  orcid: 0000-0002-3616-8580
- first_name: Victor-Valentin
  full_name: Hodirnau, Victor-Valentin
  id: 3661B498-F248-11E8-B48F-1D18A9856A87
  last_name: Hodirnau
  orcid: 0000-0003-3904-947X
- first_name: Vanessa
  full_name: Zheden, Vanessa
  id: 39C5A68A-F248-11E8-B48F-1D18A9856A87
  last_name: Zheden
  orcid: 0000-0002-9438-4783
- first_name: Jonna H
  full_name: Alanko, Jonna H
  id: 2CC12E8C-F248-11E8-B48F-1D18A9856A87
  last_name: Alanko
  orcid: 0000-0002-7698-3061
- first_name: Michael K
  full_name: Sixt, Michael K
  id: 41E9FBEA-F248-11E8-B48F-1D18A9856A87
  last_name: Sixt
  orcid: 0000-0002-6620-9179
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Zens B, Fäßler F, Hansen J, et al. Lift-out cryo-FIBSEM and cryo-ET reveal
    the ultrastructural landscape of extracellular matrix. <i>Journal of Cell Biology</i>.
    2024;223(6). doi:<a href="https://doi.org/10.1083/jcb.202309125">10.1083/jcb.202309125</a>
  apa: Zens, B., Fäßler, F., Hansen, J., Hauschild, R., Datler, J., Hodirnau, V.-V.,
    … Schur, F. K. (2024). Lift-out cryo-FIBSEM and cryo-ET reveal the ultrastructural
    landscape of extracellular matrix. <i>Journal of Cell Biology</i>. Rockefeller
    University Press. <a href="https://doi.org/10.1083/jcb.202309125">https://doi.org/10.1083/jcb.202309125</a>
  chicago: Zens, Bettina, Florian Fäßler, Jesse Hansen, Robert Hauschild, Julia Datler,
    Victor-Valentin Hodirnau, Vanessa Zheden, Jonna H Alanko, Michael K Sixt, and
    Florian KM Schur. “Lift-out Cryo-FIBSEM and Cryo-ET Reveal the Ultrastructural
    Landscape of Extracellular Matrix.” <i>Journal of Cell Biology</i>. Rockefeller
    University Press, 2024. <a href="https://doi.org/10.1083/jcb.202309125">https://doi.org/10.1083/jcb.202309125</a>.
  ieee: B. Zens <i>et al.</i>, “Lift-out cryo-FIBSEM and cryo-ET reveal the ultrastructural
    landscape of extracellular matrix,” <i>Journal of Cell Biology</i>, vol. 223,
    no. 6. Rockefeller University Press, 2024.
  ista: Zens B, Fäßler F, Hansen J, Hauschild R, Datler J, Hodirnau V-V, Zheden V,
    Alanko JH, Sixt MK, Schur FK. 2024. Lift-out cryo-FIBSEM and cryo-ET reveal the
    ultrastructural landscape of extracellular matrix. Journal of Cell Biology. 223(6),
    e202309125.
  mla: Zens, Bettina, et al. “Lift-out Cryo-FIBSEM and Cryo-ET Reveal the Ultrastructural
    Landscape of Extracellular Matrix.” <i>Journal of Cell Biology</i>, vol. 223,
    no. 6, e202309125, Rockefeller University Press, 2024, doi:<a href="https://doi.org/10.1083/jcb.202309125">10.1083/jcb.202309125</a>.
  short: B. Zens, F. Fäßler, J. Hansen, R. Hauschild, J. Datler, V.-V. Hodirnau, V.
    Zheden, J.H. Alanko, M.K. Sixt, F.K. Schur, Journal of Cell Biology 223 (2024).
corr_author: '1'
date_created: 2024-03-21T06:45:51Z
date_published: 2024-03-20T00:00:00Z
date_updated: 2025-09-04T13:17:16Z
day: '20'
ddc:
- '570'
department:
- _id: FlSc
- _id: MiSi
- _id: Bio
- _id: EM-Fac
doi: 10.1083/jcb.202309125
ec_funded: 1
external_id:
  isi:
  - '001264190100001'
  pmid:
  - '38506714'
file:
- access_level: open_access
  checksum: 90d1984a93660735e506c2a304bc3f73
  content_type: application/pdf
  creator: dernst
  date_created: 2024-03-25T12:52:04Z
  date_updated: 2024-03-25T12:52:04Z
  file_id: '15188'
  file_name: 2024_JCB_Zens.pdf
  file_size: 11907016
  relation: main_file
  success: 1
file_date_updated: 2024-03-25T12:52:04Z
has_accepted_license: '1'
intvolume: '       223'
isi: 1
issue: '6'
language:
- iso: eng
month: '03'
oa: 1
oa_version: Published Version
pmid: 1
project:
- _id: 9B954C5C-BA93-11EA-9121-9846C619BF3A
  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
- _id: 7bd318a1-9f16-11ee-852c-cc9217763180
  grant_number: E435
  name: In Situ Actin Structures via Hybrid Cryo-electron Microscopy
- _id: 25FE9508-B435-11E9-9278-68D0E5697425
  call_identifier: H2020
  grant_number: '724373'
  name: Cellular Navigation Along Spatial Gradients
- _id: 059B463C-7A3F-11EA-A408-12923DDC885E
  name: "NÃ\x96-Fonds Preis für die Jungforscherin des Jahres am IST Austria"
- _id: 2615199A-B435-11E9-9278-68D0E5697425
  grant_number: '21317'
  name: Spatiotemporal regulation of chemokine-induced signalling in leukocyte chemotaxis
- _id: 62909c6f-2b32-11ec-9570-e1476aab5308
  grant_number: CZI01
  name: CryoMinflux-guided in-situ visual proteomics and structure determination
publication: Journal of Cell Biology
publication_identifier:
  eissn:
  - 1540-8140
  issn:
  - 0021-9525
publication_status: published
publisher: Rockefeller University Press
quality_controlled: '1'
scopus_import: '1'
status: public
title: Lift-out cryo-FIBSEM and cryo-ET reveal the ultrastructural landscape of extracellular
  matrix
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 317138e5-6ab7-11ef-aa6d-ffef3953e345
volume: 223
year: '2024'
...
---
APC_amount: 11700 EUR
OA_place: publisher
OA_type: hybrid
_id: '14979'
abstract:
- lang: eng
  text: Poxviruses are among the largest double-stranded DNA viruses, with members
    such as variola virus, monkeypox virus and the vaccination strain vaccinia virus
    (VACV). Knowledge about the structural proteins that form the viral core has remained
    sparse. While major core proteins have been annotated via indirect experimental
    evidence, their structures have remained elusive and they could not be assigned
    to individual core features. Hence, which proteins constitute which layers of
    the core, such as the palisade layer and the inner core wall, has remained enigmatic.
    Here we show, using a multi-modal cryo-electron microscopy (cryo-EM) approach
    in combination with AlphaFold molecular modeling, that trimers formed by the cleavage
    product of VACV protein A10 are the key component of the palisade layer. This
    allows us to place previously obtained descriptions of protein interactions within
    the core wall into perspective and to provide a detailed model of poxvirus core
    architecture. Importantly, we show that interactions within A10 trimers are likely
    generalizable over members of orthopox- and parapoxviruses.
acknowledged_ssus:
- _id: ScienComp
- _id: LifeSc
- _id: EM-Fac
acknowledgement: "We thank A. Bergthaler (Research Center for Molecular Medicine of
  the Austrian Academy of Sciences) for providing VACV WR. We thank A. Nicholas and
  his team at the ISTA proteomics facility, and S. Elefante at the ISTA Scientific
  Computing facility for their support. We also thank F. Fäßler, D. Porley, T. Muthspiel
  and other members of the Schur group for support and helpful discussions. We also
  thank D. Castaño-Díez for support with Dynamo. We thank D. Farrell for his help
  optimizing the Rosetta protocol to refine the atomic model into the cryo-EM map
  with symmetry.\r\n\r\nF.K.M.S. acknowledges support from ISTA and EMBO. F.K.M.S.
  also received support from the Austrian Science Fund (FWF) grant P31445. This publication
  has been made possible in part by CZI grant DAF2021-234754 and grant https://doi.org/10.37921/812628ebpcwg
  from the Chan Zuckerberg Initiative DAF, an advised fund of Silicon Valley Community
  Foundation (funder https://doi.org/10.13039/100014989) awarded to F.K.M.S.\r\n\r\nThis
  research was also supported by the Scientific Service Units (SSUs) of ISTA through
  resources provided by Scientific Computing (SciComp), the Life Science Facility
  (LSF), and the Electron Microscopy Facility (EMF). We also acknowledge the use of
  COSMIC45 and Colabfold46."
article_processing_charge: Yes (in subscription journal)
article_type: original
author:
- first_name: Julia
  full_name: Datler, Julia
  id: 3B12E2E6-F248-11E8-B48F-1D18A9856A87
  last_name: Datler
  orcid: 0000-0002-3616-8580
- first_name: Jesse
  full_name: Hansen, Jesse
  id: 1063c618-6f9b-11ec-9123-f912fccded63
  last_name: Hansen
  orcid: 0000-0001-7967-2085
- first_name: Andreas
  full_name: Thader, Andreas
  id: 3A18A7B8-F248-11E8-B48F-1D18A9856A87
  last_name: Thader
- first_name: Alois
  full_name: Schlögl, Alois
  id: 45BF87EE-F248-11E8-B48F-1D18A9856A87
  last_name: Schlögl
  orcid: 0000-0002-5621-8100
- first_name: Lukas W
  full_name: Bauer, Lukas W
  id: 0c894dcf-897b-11ed-a09c-8186353224b0
  last_name: Bauer
- first_name: Victor-Valentin
  full_name: Hodirnau, Victor-Valentin
  id: 3661B498-F248-11E8-B48F-1D18A9856A87
  last_name: Hodirnau
  orcid: 0000-0003-3904-947X
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Datler J, Hansen J, Thader A, et al. Multi-modal cryo-EM reveals trimers of
    protein A10 to form the palisade layer in poxvirus cores. <i>Nature Structural
    &#38; Molecular Biology</i>. 2024;31:1114-1123. doi:<a href="https://doi.org/10.1038/s41594-023-01201-6">10.1038/s41594-023-01201-6</a>
  apa: Datler, J., Hansen, J., Thader, A., Schlögl, A., Bauer, L. W., Hodirnau, V.-V.,
    &#38; Schur, F. K. (2024). Multi-modal cryo-EM reveals trimers of protein A10
    to form the palisade layer in poxvirus cores. <i>Nature Structural &#38; Molecular
    Biology</i>. Springer Nature. <a href="https://doi.org/10.1038/s41594-023-01201-6">https://doi.org/10.1038/s41594-023-01201-6</a>
  chicago: Datler, Julia, Jesse Hansen, Andreas Thader, Alois Schlögl, Lukas W Bauer,
    Victor-Valentin Hodirnau, and Florian KM Schur. “Multi-Modal Cryo-EM Reveals Trimers
    of Protein A10 to Form the Palisade Layer in Poxvirus Cores.” <i>Nature Structural
    &#38; Molecular Biology</i>. Springer Nature, 2024. <a href="https://doi.org/10.1038/s41594-023-01201-6">https://doi.org/10.1038/s41594-023-01201-6</a>.
  ieee: J. Datler <i>et al.</i>, “Multi-modal cryo-EM reveals trimers of protein A10
    to form the palisade layer in poxvirus cores,” <i>Nature Structural &#38; Molecular
    Biology</i>, vol. 31. Springer Nature, pp. 1114–1123, 2024.
  ista: Datler J, Hansen J, Thader A, Schlögl A, Bauer LW, Hodirnau V-V, Schur FK.
    2024. Multi-modal cryo-EM reveals trimers of protein A10 to form the palisade
    layer in poxvirus cores. Nature Structural &#38; Molecular Biology. 31, 1114–1123.
  mla: Datler, Julia, et al. “Multi-Modal Cryo-EM Reveals Trimers of Protein A10 to
    Form the Palisade Layer in Poxvirus Cores.” <i>Nature Structural &#38; Molecular
    Biology</i>, vol. 31, Springer Nature, 2024, pp. 1114–23, doi:<a href="https://doi.org/10.1038/s41594-023-01201-6">10.1038/s41594-023-01201-6</a>.
  short: J. Datler, J. Hansen, A. Thader, A. Schlögl, L.W. Bauer, V.-V. Hodirnau,
    F.K. Schur, Nature Structural &#38; Molecular Biology 31 (2024) 1114–1123.
corr_author: '1'
date_created: 2024-02-12T09:59:45Z
date_published: 2024-07-01T00:00:00Z
date_updated: 2026-04-07T12:59:44Z
day: '01'
ddc:
- '570'
department:
- _id: FlSc
- _id: ScienComp
- _id: EM-Fac
doi: 10.1038/s41594-023-01201-6
external_id:
  isi:
  - '001158144600002'
  pmid:
  - '38316877'
file:
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  success: 1
file_date_updated: 2024-07-22T11:27:22Z
has_accepted_license: '1'
intvolume: '        31'
isi: 1
keyword:
- Molecular Biology
- Structural Biology
language:
- iso: eng
month: '07'
oa: 1
oa_version: Published Version
page: 1114-1123
pmid: 1
project:
- _id: 26736D6A-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: P31445
  name: Structural conservation and diversity in retroviral capsid
publication: Nature Structural & Molecular Biology
publication_identifier:
  eissn:
  - 1545-9985
  issn:
  - 1545-9993
publication_status: published
publisher: Springer Nature
quality_controlled: '1'
related_material:
  link:
  - description: News on ISTA Website
    relation: press_release
    url: https://ista.ac.at/en/news/down-to-the-core-of-poxviruses/
  record:
  - id: '18766'
    relation: dissertation_contains
    status: public
scopus_import: '1'
status: public
title: Multi-modal cryo-EM reveals trimers of protein A10 to form the palisade layer
  in poxvirus cores
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 317138e5-6ab7-11ef-aa6d-ffef3953e345
volume: 31
year: '2024'
...
---
_id: '14255'
abstract:
- lang: eng
  text: Toscana virus is a major cause of arboviral disease in humans in the Mediterranean
    basin during summer. However, early virus-host cell interactions and entry mechanisms
    remain poorly characterized. Investigating iPSC-derived human neurons and cell
    lines, we found that virus binding to the cell surface was specific, and 50% of
    bound virions were endocytosed within 10 min. Virions entered Rab5a+ early endosomes
    and, subsequently, Rab7a+ and LAMP-1+ late endosomal compartments. Penetration
    required intact late endosomes and occurred within 30 min following internalization.
    Virus entry relied on vacuolar acidification, with an optimal pH for viral membrane
    fusion at pH 5.5. The pH threshold increased to 5.8 with longer pre-exposure of
    virions to the slightly acidic pH in early endosomes. Strikingly, the particles
    remained infectious after entering late endosomes with a pH below the fusion threshold.
    Overall, our study establishes Toscana virus as a late-penetrating virus and reveals
    an atypical use of vacuolar acidity by this virus to enter host cells.
acknowledged_ssus:
- _id: EM-Fac
acknowledgement: "We acknowledge Elodie Chatre and the Imaging Platform Platim, SFR
  Biosciences, Lyon, as well as Vibor Laketa and the Infectious Diseases Imaging Platform
  (IDIP) at the Center for Integrative Infectious Disease Research (CIID) Heidelberg.
  The sand fly cell lines were supplied by the Tick Cell Biobank at the University
  of Liverpool. F.K.M.S. acknowledges support from the Scientific Service Units (SSUs)
  of ISTA through resources provided by the Electron Microscopy Facility (EMF).\r\nThis
  work was supported by CellNetworks Research Group funds and Deutsche Forschungsgemeinschaft
  (DFG) funding (LO-2338/3-1) and the Agence Nationale de la Recherche (ANR) funding
  (grant numbers ANR-21-CE11-0012 and ANR-22-CE15-0034), all awarded to P.-Y.L. This
  work was also supported by the LABEX ECOFECT (ANR-11-LABX-0048) of Université de
  Lyon (UDL), within the program “Investissements d’Avenir” (ANR-11-IDEX-0007) operated
  by the ANR and by the RESPOND program of the UDL (awarded to P.-Y.L) . C.A. was
  supported by the Chica and Heinz Schaller Research Group funds, NARSAD 2019 award,
  a Fritz Thyssen Research Grant, and the SFB1158-S02 grant. L.B-S. is supported by
  a United Kingdom Biotechnology and Biological Sciences Research Council grant (BB/P024270/1)
  and a Wellcome Trust grant (223743/Z/21/Z). F.K.M.S acknowledges support from the
  Austrian Science Fund (FWF, P31445). J.K. received a salary from the DFG (LO-2338/3-1)
  and then from the ANR (ANR-11-LABX-0048). The salary of Z.M.U. was partially covered
  by the DFG (LO-2338/3-1). S.K. received a salary from the DFG (SFB1129). We are
  grateful to the Chinese Scholarship Council (CSC; 201904910701), DAAD/ANID (57451854/62180003),
  the Rufus A. Kellogg fellowship program (Amherst College, Massachusetts, USA) for
  awarding fellowships to Q.X., J.C., and H.A.A., respectively."
article_number: e1011562
article_processing_charge: Yes
article_type: original
author:
- first_name: Jana
  full_name: Koch, Jana
  last_name: Koch
- first_name: Qilin
  full_name: Xin, Qilin
  last_name: Xin
- first_name: Martin
  full_name: Obr, Martin
  id: 4741CA5A-F248-11E8-B48F-1D18A9856A87
  last_name: Obr
  orcid: 0000-0003-1756-6564
- first_name: Alicia
  full_name: Schäfer, Alicia
  last_name: Schäfer
- first_name: Nina
  full_name: Rolfs, Nina
  last_name: Rolfs
- first_name: Holda A.
  full_name: Anagho, Holda A.
  last_name: Anagho
- first_name: Aiste
  full_name: Kudulyte, Aiste
  last_name: Kudulyte
- first_name: Lea
  full_name: Woltereck, Lea
  last_name: Woltereck
- first_name: Susann
  full_name: Kummer, Susann
  last_name: Kummer
- first_name: Joaquin
  full_name: Campos, Joaquin
  last_name: Campos
- first_name: Zina M.
  full_name: Uckeley, Zina M.
  last_name: Uckeley
- first_name: Lesley
  full_name: Bell-Sakyi, Lesley
  last_name: Bell-Sakyi
- first_name: Hans Georg
  full_name: Kräusslich, Hans Georg
  last_name: Kräusslich
- first_name: Florian Km
  full_name: Schur, Florian Km
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Claudio
  full_name: Acuna, Claudio
  last_name: Acuna
- first_name: Pierre Yves
  full_name: Lozach, Pierre Yves
  last_name: Lozach
citation:
  ama: Koch J, Xin Q, Obr M, et al. The phenuivirus Toscana virus makes an atypical
    use of vacuolar acidity to enter host cells. <i>PLoS Pathogens</i>. 2023;19(8).
    doi:<a href="https://doi.org/10.1371/journal.ppat.1011562">10.1371/journal.ppat.1011562</a>
  apa: Koch, J., Xin, Q., Obr, M., Schäfer, A., Rolfs, N., Anagho, H. A., … Lozach,
    P. Y. (2023). The phenuivirus Toscana virus makes an atypical use of vacuolar
    acidity to enter host cells. <i>PLoS Pathogens</i>. Public Library of Science.
    <a href="https://doi.org/10.1371/journal.ppat.1011562">https://doi.org/10.1371/journal.ppat.1011562</a>
  chicago: Koch, Jana, Qilin Xin, Martin Obr, Alicia Schäfer, Nina Rolfs, Holda A.
    Anagho, Aiste Kudulyte, et al. “The Phenuivirus Toscana Virus Makes an Atypical
    Use of Vacuolar Acidity to Enter Host Cells.” <i>PLoS Pathogens</i>. Public Library
    of Science, 2023. <a href="https://doi.org/10.1371/journal.ppat.1011562">https://doi.org/10.1371/journal.ppat.1011562</a>.
  ieee: J. Koch <i>et al.</i>, “The phenuivirus Toscana virus makes an atypical use
    of vacuolar acidity to enter host cells,” <i>PLoS Pathogens</i>, vol. 19, no.
    8. Public Library of Science, 2023.
  ista: Koch J, Xin Q, Obr M, Schäfer A, Rolfs N, Anagho HA, Kudulyte A, Woltereck
    L, Kummer S, Campos J, Uckeley ZM, Bell-Sakyi L, Kräusslich HG, Schur FK, Acuna
    C, Lozach PY. 2023. The phenuivirus Toscana virus makes an atypical use of vacuolar
    acidity to enter host cells. PLoS Pathogens. 19(8), e1011562.
  mla: Koch, Jana, et al. “The Phenuivirus Toscana Virus Makes an Atypical Use of
    Vacuolar Acidity to Enter Host Cells.” <i>PLoS Pathogens</i>, vol. 19, no. 8,
    e1011562, Public Library of Science, 2023, doi:<a href="https://doi.org/10.1371/journal.ppat.1011562">10.1371/journal.ppat.1011562</a>.
  short: J. Koch, Q. Xin, M. Obr, A. Schäfer, N. Rolfs, H.A. Anagho, A. Kudulyte,
    L. Woltereck, S. Kummer, J. Campos, Z.M. Uckeley, L. Bell-Sakyi, H.G. Kräusslich,
    F.K. Schur, C. Acuna, P.Y. Lozach, PLoS Pathogens 19 (2023).
date_created: 2023-09-03T22:01:14Z
date_published: 2023-08-14T00:00:00Z
date_updated: 2025-04-15T08:24:50Z
day: '14'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.1371/journal.ppat.1011562
external_id:
  isi:
  - '001050846300004'
  pmid:
  - '37578957'
file:
- access_level: open_access
  checksum: 47ca3bb54b27f28b05644be0ad064bc6
  content_type: application/pdf
  creator: dernst
  date_created: 2023-09-06T06:41:52Z
  date_updated: 2023-09-06T06:41:52Z
  file_id: '14269'
  file_name: 2023_PloSPathogens_Koch.pdf
  file_size: 4458336
  relation: main_file
  success: 1
file_date_updated: 2023-09-06T06:41:52Z
has_accepted_license: '1'
intvolume: '        19'
isi: 1
issue: '8'
language:
- iso: eng
month: '08'
oa: 1
oa_version: Published Version
pmid: 1
project:
- _id: 26736D6A-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: P31445
  name: Structural conservation and diversity in retroviral capsid
publication: PLoS Pathogens
publication_identifier:
  eissn:
  - 1553-7374
  issn:
  - 1553-7366
publication_status: published
publisher: Public Library of Science
quality_controlled: '1'
scopus_import: '1'
status: public
title: The phenuivirus Toscana virus makes an atypical use of vacuolar acidity to
  enter host cells
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 19
year: '2023'
...
---
_id: '14502'
abstract:
- lang: eng
  text: A precise quantitative description of the ultrastructural characteristics
    underlying biological mechanisms is often key to their understanding. This is
    particularly true for dynamic extra- and intracellular filamentous assemblies,
    playing a role in cell motility, cell integrity, cytokinesis, tissue formation
    and maintenance. For example, genetic manipulation or modulation of actin regulatory
    proteins frequently manifests in changes of the morphology, dynamics, and ultrastructural
    architecture of actin filament-rich cell peripheral structures, such as lamellipodia
    or filopodia. However, the observed ultrastructural effects often remain subtle
    and require sufficiently large datasets for appropriate quantitative analysis.
    The acquisition of such large datasets has been enabled by recent advances in
    high-throughput cryo-electron tomography (cryo-ET) methods. This also necessitates
    the development of complementary approaches to maximize the extraction of relevant
    biological information. We have developed a computational toolbox for the semi-automatic
    quantification of segmented and vectorized fila- mentous networks from pre-processed
    cryo-electron tomograms, facilitating the analysis and cross-comparison of multiple
    experimental conditions. GUI-based components simplify the processing of data
    and allow users to obtain a large number of ultrastructural parameters describing
    filamentous assemblies. We demonstrate the feasibility of this workflow by analyzing
    cryo-ET data of untreated and chemically perturbed branched actin filament networks
    and that of parallel actin filament arrays. In principle, the computational toolbox
    presented here is applicable for data analysis comprising any type of filaments
    in regular (i.e. parallel) or random arrangement. We show that it can ease the
    identification of key differences between experimental groups and facilitate the
    in-depth analysis of ultrastructural data in a time-efficient manner.
author:
- first_name: Georgi A
  full_name: Dimchev, Georgi A
  id: 38C393BE-F248-11E8-B48F-1D18A9856A87
  last_name: Dimchev
  orcid: 0000-0001-8370-6161
- first_name: Behnam
  full_name: Amiri, Behnam
  last_name: Amiri
- first_name: Florian
  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Martin
  full_name: Falcke, Martin
  last_name: Falcke
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Dimchev GA, Amiri B, Fäßler F, Falcke M, Schur FK. Computational toolbox for
    ultrastructural quantitative analysis of filament networks in cryo-ET data. 2023.
    doi:<a href="https://doi.org/10.15479/AT:ISTA:14502">10.15479/AT:ISTA:14502</a>
  apa: Dimchev, G. A., Amiri, B., Fäßler, F., Falcke, M., &#38; Schur, F. K. (2023).
    Computational toolbox for ultrastructural quantitative analysis of filament networks
    in cryo-ET data. Institute of Science and Technology Austria. <a href="https://doi.org/10.15479/AT:ISTA:14502">https://doi.org/10.15479/AT:ISTA:14502</a>
  chicago: Dimchev, Georgi A, Behnam Amiri, Florian Fäßler, Martin Falcke, and Florian
    KM Schur. “Computational Toolbox for Ultrastructural Quantitative Analysis of
    Filament Networks in Cryo-ET Data.” Institute of Science and Technology Austria,
    2023. <a href="https://doi.org/10.15479/AT:ISTA:14502">https://doi.org/10.15479/AT:ISTA:14502</a>.
  ieee: G. A. Dimchev, B. Amiri, F. Fäßler, M. Falcke, and F. K. Schur, “Computational
    toolbox for ultrastructural quantitative analysis of filament networks in cryo-ET
    data.” Institute of Science and Technology Austria, 2023.
  ista: Dimchev GA, Amiri B, Fäßler F, Falcke M, Schur FK. 2023. Computational toolbox
    for ultrastructural quantitative analysis of filament networks in cryo-ET data,
    Institute of Science and Technology Austria, <a href="https://doi.org/10.15479/AT:ISTA:14502">10.15479/AT:ISTA:14502</a>.
  mla: Dimchev, Georgi A., et al. <i>Computational Toolbox for Ultrastructural Quantitative
    Analysis of Filament Networks in Cryo-ET Data</i>. Institute of Science and Technology
    Austria, 2023, doi:<a href="https://doi.org/10.15479/AT:ISTA:14502">10.15479/AT:ISTA:14502</a>.
  short: G.A. Dimchev, B. Amiri, F. Fäßler, M. Falcke, F.K. Schur, (2023).
corr_author: '1'
date_created: 2023-11-08T19:40:54Z
date_published: 2023-11-21T00:00:00Z
date_updated: 2025-04-15T08:25:41Z
day: '21'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.15479/AT:ISTA:14502
file:
- access_level: open_access
  checksum: a8b9adeb53a4109dea4d5e39fa1acccf
  content_type: application/zip
  creator: fschur
  date_created: 2023-11-08T20:23:07Z
  date_updated: 2023-11-08T20:23:07Z
  file_id: '14503'
  file_name: Computational_Toolbox_v1.2.zip
  file_size: 347641117
  relation: main_file
  success: 1
- access_level: open_access
  checksum: 14db2addbfca61a085ba301ed6f2900b
  content_type: text/plain
  creator: dernst
  date_created: 2023-11-21T08:20:23Z
  date_updated: 2023-11-21T08:20:23Z
  file_id: '14586'
  file_name: Readme.txt
  file_size: 1522
  relation: main_file
  success: 1
file_date_updated: 2023-11-21T08:20:23Z
has_accepted_license: '1'
keyword:
- cryo-electron tomography
- actin cytoskeleton
- toolbox
license: https://choosealicense.com/licenses/agpl-3.0/
month: '11'
oa: 1
project:
- _id: 9B954C5C-BA93-11EA-9121-9846C619BF3A
  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
publisher: Institute of Science and Technology Austria
related_material:
  record:
  - id: '10290'
    relation: used_for_analysis_in
    status: public
status: public
title: Computational toolbox for ultrastructural quantitative analysis of filament
  networks in cryo-ET data
tmp:
  legal_code_url: https://www.gnu.org/licenses/agpl-3.0.html
  name: GNU Affero General Public License v3.0
  short: 'GNU AGPLv3  '
type: software
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
year: '2023'
...
---
_id: '14562'
abstract:
- lang: eng
  text: "Regulation of the Arp2/3 complex is required for productive nucleation of
    branched actin networks. An emerging aspect of regulation is the incorporation
    of subunit isoforms into the Arp2/3 complex. Specifically, both ArpC5 subunit
    isoforms, ArpC5 and ArpC5L, have been reported to fine-tune nucleation activity
    and branch junction stability. We have combined reverse genetics and cellular
    structural biology to describe how ArpC5 and ArpC5L differentially affect cell
    migration. Both define the structural stability of ArpC1 in branch junctions and,
    in turn, by determining protrusion characteristics, affect protein dynamics and
    actin network ultrastructure. ArpC5 isoforms also affect the positioning of members
    of the Ena/Vasodilator-stimulated phosphoprotein (VASP) family of actin filament
    elongators, which mediate ArpC5 isoform–specific effects on the actin assembly
    level. Our results suggest that ArpC5 and Ena/VASP proteins are part of a signaling
    pathway enhancing cell migration.\r\n"
acknowledged_ssus:
- _id: LifeSc
- _id: Bio
- _id: ScienComp
- _id: EM-Fac
acknowledgement: "We would like to thank K. von Peinen and B. Denker (Helmholtz Centre
  for Infection Research, Braunschweig, Germany) for experimental and technical assistance,
  respectively.\r\nFunding: This research was supported by the Scientific Service
  Units (SSUs) of ISTA through resources provided by Scientific Computing (SciComp),
  the Life Science Facility (LSF), the Imaging and Optics facility (IOF), and the
  Electron Microscopy Facility (EMF). We acknowledge support from ISTA and from the
  Austrian Science Fund (FWF) (P33367) to F.K.M.S., from the Research Training Group
  GRK2223 and the Helmholtz Society to K.R,. and from the Deutsche Forschungsgemeinschaft
  (DFG) to J.F. and K.R."
article_processing_charge: No
author:
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Schur FK. Research data of the publication “ArpC5 isoforms regulate Arp2/3
    complex-dependent protrusion through differential Ena/VASP positioning.” 2023.
    doi:<a href="https://doi.org/10.15479/AT:ISTA:14562">10.15479/AT:ISTA:14562</a>
  apa: Schur, F. K. (2023). Research data of the publication “ArpC5 isoforms regulate
    Arp2/3 complex-dependent protrusion through differential Ena/VASP positioning.”
    Institute of Science and Technology Austria. <a href="https://doi.org/10.15479/AT:ISTA:14562">https://doi.org/10.15479/AT:ISTA:14562</a>
  chicago: Schur, Florian KM. “Research Data of the Publication ‘ArpC5 Isoforms Regulate
    Arp2/3 Complex-Dependent Protrusion through Differential Ena/VASP Positioning.’”
    Institute of Science and Technology Austria, 2023. <a href="https://doi.org/10.15479/AT:ISTA:14562">https://doi.org/10.15479/AT:ISTA:14562</a>.
  ieee: F. K. Schur, “Research data of the publication ‘ArpC5 isoforms regulate Arp2/3
    complex-dependent protrusion through differential Ena/VASP positioning.’” Institute
    of Science and Technology Austria, 2023.
  ista: Schur FK. 2023. Research data of the publication ‘ArpC5 isoforms regulate
    Arp2/3 complex-dependent protrusion through differential Ena/VASP positioning’,
    Institute of Science and Technology Austria, <a href="https://doi.org/10.15479/AT:ISTA:14562">10.15479/AT:ISTA:14562</a>.
  mla: Schur, Florian KM. <i>Research Data of the Publication “ArpC5 Isoforms Regulate
    Arp2/3 Complex-Dependent Protrusion through Differential Ena/VASP Positioning.”</i>
    Institute of Science and Technology Austria, 2023, doi:<a href="https://doi.org/10.15479/AT:ISTA:14562">10.15479/AT:ISTA:14562</a>.
  short: F.K. Schur, (2023).
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  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
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  orcid: 0000-0003-4790-8078
corr_author: '1'
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date_updated: 2025-04-23T08:46:21Z
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  name: Structure and isoform diversity of the Arp2/3 complex
publisher: Institute of Science and Technology Austria
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title: Research data of the publication "ArpC5 isoforms regulate Arp2/3 complex-dependent
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type: research_data
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...
---
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abstract:
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  text: The actin cytoskeleton plays a key role in cell migration and cellular morphodynamics
    in most eukaryotes. The ability of the actin cytoskeleton to assemble and disassemble
    in a spatiotemporally controlled manner allows it to form higher-order structures,
    which can generate forces required for a cell to explore and navigate through
    its environment. It is regulated not only via a complex synergistic and competitive
    interplay between actin-binding proteins (ABP), but also by filament biochemistry
    and filament geometry. The lack of structural insights into how geometry and ABPs
    regulate the actin cytoskeleton limits our understanding of the molecular mechanisms
    that define actin cytoskeleton remodeling and, in turn, impact emerging cell migration
    characteristics. With the advent of cryo-electron microscopy (cryo-EM) and advanced
    computational methods, it is now possible to define these molecular mechanisms
    involving actin and its interactors at both atomic and ultra-structural levels
    in vitro and in cellulo. In this review, we will provide an overview of the available
    cryo-EM methods, applicable to further our understanding of the actin cytoskeleton,
    specifically in the context of cell migration. We will discuss how these methods
    have been employed to elucidate ABP- and geometry-defined regulatory mechanisms
    in initiating, maintaining, and disassembling cellular actin networks in migratory
    protrusions.
acknowledgement: 'We apologize for not being able to mention and cite additional excellent
  work that would have fit the scope of this review, due to space restraints. We thank
  Jesse Hansen for comments on the manuscript. We acknowledge support from the Austrian
  Science Fund (FWF): P33367 and the Institute of Science and Technology Austria.'
article_processing_charge: No
article_type: original
author:
- first_name: Florian
  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Manjunath
  full_name: Javoor, Manjunath
  id: 305ab18b-dc7d-11ea-9b2f-b58195228ea2
  last_name: Javoor
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Fäßler F, Javoor M, Schur FK. Deciphering the molecular mechanisms of actin
    cytoskeleton regulation in cell migration using cryo-EM. <i>Biochemical Society
    Transactions</i>. 2023;51(1):87-99. doi:<a href="https://doi.org/10.1042/bst20220221">10.1042/bst20220221</a>
  apa: Fäßler, F., Javoor, M., &#38; Schur, F. K. (2023). Deciphering the molecular
    mechanisms of actin cytoskeleton regulation in cell migration using cryo-EM. <i>Biochemical
    Society Transactions</i>. Portland Press. <a href="https://doi.org/10.1042/bst20220221">https://doi.org/10.1042/bst20220221</a>
  chicago: Fäßler, Florian, Manjunath Javoor, and Florian KM Schur. “Deciphering the
    Molecular Mechanisms of Actin Cytoskeleton Regulation in Cell Migration Using
    Cryo-EM.” <i>Biochemical Society Transactions</i>. Portland Press, 2023. <a href="https://doi.org/10.1042/bst20220221">https://doi.org/10.1042/bst20220221</a>.
  ieee: F. Fäßler, M. Javoor, and F. K. Schur, “Deciphering the molecular mechanisms
    of actin cytoskeleton regulation in cell migration using cryo-EM,” <i>Biochemical
    Society Transactions</i>, vol. 51, no. 1. Portland Press, pp. 87–99, 2023.
  ista: Fäßler F, Javoor M, Schur FK. 2023. Deciphering the molecular mechanisms of
    actin cytoskeleton regulation in cell migration using cryo-EM. Biochemical Society
    Transactions. 51(1), 87–99.
  mla: Fäßler, Florian, et al. “Deciphering the Molecular Mechanisms of Actin Cytoskeleton
    Regulation in Cell Migration Using Cryo-EM.” <i>Biochemical Society Transactions</i>,
    vol. 51, no. 1, Portland Press, 2023, pp. 87–99, doi:<a href="https://doi.org/10.1042/bst20220221">10.1042/bst20220221</a>.
  short: F. Fäßler, M. Javoor, F.K. Schur, Biochemical Society Transactions 51 (2023)
    87–99.
corr_author: '1'
date_created: 2023-01-27T10:08:19Z
date_published: 2023-02-01T00:00:00Z
date_updated: 2025-04-23T08:47:15Z
day: '01'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.1042/bst20220221
external_id:
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  pmid:
  - '36695514'
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keyword:
- Biochemistry
language:
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month: '02'
oa: 1
oa_version: Published Version
page: 87-99
pmid: 1
project:
- _id: 9B954C5C-BA93-11EA-9121-9846C619BF3A
  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
publication: Biochemical Society Transactions
publication_identifier:
  eissn:
  - 1470-8752
  issn:
  - 0300-5127
publication_status: published
publisher: Portland Press
quality_controlled: '1'
scopus_import: '1'
status: public
title: Deciphering the molecular mechanisms of actin cytoskeleton regulation in cell
  migration using cryo-EM
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
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  short: CC BY (4.0)
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 51
year: '2023'
...
---
_id: '12334'
abstract:
- lang: eng
  text: Regulation of the Arp2/3 complex is required for productive nucleation of
    branched actin networks. An emerging aspect of regulation is the incorporation
    of subunit isoforms into the Arp2/3 complex. Specifically, both ArpC5 subunit
    isoforms, ArpC5 and ArpC5L, have been reported to fine-tune nucleation activity
    and branch junction stability. We have combined reverse genetics and cellular
    structural biology to describe how ArpC5 and ArpC5L differentially affect cell
    migration. Both define the structural stability of ArpC1 in branch junctions and,
    in turn, by determining protrusion characteristics, affect protein dynamics and
    actin network ultrastructure. ArpC5 isoforms also affect the positioning of members
    of the Ena/Vasodilator-stimulated phosphoprotein (VASP) family of actin filament
    elongators, which mediate ArpC5 isoform–specific effects on the actin assembly
    level. Our results suggest that ArpC5 and Ena/VASP proteins are part of a signaling
    pathway enhancing cell migration.</jats:p>
acknowledged_ssus:
- _id: ScienComp
- _id: LifeSc
- _id: Bio
- _id: EM-Fac
acknowledgement: "We would like to thank K. von Peinen and B. Denker (Helmholtz Centre
  for Infection Research, Braunschweig, Germany) for experimental and technical assistance,
  respectively.\r\nThis research was supported by the Scientific Service Units (SSUs)
  of ISTA through resources provided by Scientific Computing (SciComp), the Life Science
  Facility (LSF), the Imaging and Optics facility (IOF), and the Electron Microscopy
  Facility (EMF). We acknowledge support from ISTA and from the Austrian Science Fund
  (FWF) (P33367) to F.K.M.S., from the Research Training Group GRK2223 and the Helmholtz
  Society to K.R,. and from the Deutsche Forschungsgemeinschaft (DFG) to J.F. and
  K.R."
article_number: add6495
article_processing_charge: No
article_type: original
author:
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  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Manjunath
  full_name: Javoor, Manjunath
  id: 305ab18b-dc7d-11ea-9b2f-b58195228ea2
  last_name: Javoor
  orcid: 0000-0003-2311-2112
- first_name: Julia
  full_name: Datler, Julia
  id: 3B12E2E6-F248-11E8-B48F-1D18A9856A87
  last_name: Datler
  orcid: 0000-0002-3616-8580
- first_name: Hermann
  full_name: Döring, Hermann
  last_name: Döring
- first_name: Florian
  full_name: Hofer, Florian
  id: b9d234ba-9e33-11ed-95b6-cd561df280e6
  last_name: Hofer
- first_name: Georgi A
  full_name: Dimchev, Georgi A
  id: 38C393BE-F248-11E8-B48F-1D18A9856A87
  last_name: Dimchev
  orcid: 0000-0001-8370-6161
- first_name: Victor-Valentin
  full_name: Hodirnau, Victor-Valentin
  id: 3661B498-F248-11E8-B48F-1D18A9856A87
  last_name: Hodirnau
  orcid: 0000-0003-3904-947X
- first_name: Jan
  full_name: Faix, Jan
  last_name: Faix
- first_name: Klemens
  full_name: Rottner, Klemens
  last_name: Rottner
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Fäßler F, Javoor M, Datler J, et al. ArpC5 isoforms regulate Arp2/3 complex–dependent
    protrusion through differential Ena/VASP positioning. <i>Science Advances</i>.
    2023;9(3). doi:<a href="https://doi.org/10.1126/sciadv.add6495">10.1126/sciadv.add6495</a>
  apa: Fäßler, F., Javoor, M., Datler, J., Döring, H., Hofer, F., Dimchev, G. A.,
    … Schur, F. K. (2023). ArpC5 isoforms regulate Arp2/3 complex–dependent protrusion
    through differential Ena/VASP positioning. <i>Science Advances</i>. American Association
    for the Advancement of Science. <a href="https://doi.org/10.1126/sciadv.add6495">https://doi.org/10.1126/sciadv.add6495</a>
  chicago: Fäßler, Florian, Manjunath Javoor, Julia Datler, Hermann Döring, Florian
    Hofer, Georgi A Dimchev, Victor-Valentin Hodirnau, Jan Faix, Klemens Rottner,
    and Florian KM Schur. “ArpC5 Isoforms Regulate Arp2/3 Complex–Dependent Protrusion
    through Differential Ena/VASP Positioning.” <i>Science Advances</i>. American
    Association for the Advancement of Science, 2023. <a href="https://doi.org/10.1126/sciadv.add6495">https://doi.org/10.1126/sciadv.add6495</a>.
  ieee: F. Fäßler <i>et al.</i>, “ArpC5 isoforms regulate Arp2/3 complex–dependent
    protrusion through differential Ena/VASP positioning,” <i>Science Advances</i>,
    vol. 9, no. 3. American Association for the Advancement of Science, 2023.
  ista: Fäßler F, Javoor M, Datler J, Döring H, Hofer F, Dimchev GA, Hodirnau V-V,
    Faix J, Rottner K, Schur FK. 2023. ArpC5 isoforms regulate Arp2/3 complex–dependent
    protrusion through differential Ena/VASP positioning. Science Advances. 9(3),
    add6495.
  mla: Fäßler, Florian, et al. “ArpC5 Isoforms Regulate Arp2/3 Complex–Dependent Protrusion
    through Differential Ena/VASP Positioning.” <i>Science Advances</i>, vol. 9, no.
    3, add6495, American Association for the Advancement of Science, 2023, doi:<a
    href="https://doi.org/10.1126/sciadv.add6495">10.1126/sciadv.add6495</a>.
  short: F. Fäßler, M. Javoor, J. Datler, H. Döring, F. Hofer, G.A. Dimchev, V.-V.
    Hodirnau, J. Faix, K. Rottner, F.K. Schur, Science Advances 9 (2023).
corr_author: '1'
date_created: 2023-01-23T07:26:42Z
date_published: 2023-01-20T00:00:00Z
date_updated: 2026-04-07T12:59:44Z
day: '20'
ddc:
- '570'
department:
- _id: FlSc
- _id: EM-Fac
doi: 10.1126/sciadv.add6495
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  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
publication: Science Advances
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  issn:
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publisher: American Association for the Advancement of Science
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title: ArpC5 isoforms regulate Arp2/3 complex–dependent protrusion through differential
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tmp:
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type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 9
year: '2023'
...
---
_id: '10639'
abstract:
- lang: eng
  text: With more than 80 members worldwide, the Orthobunyavirus genus in the Peribunyaviridae
    family is a large genus of enveloped RNA viruses, many of which are emerging pathogens
    in humans and livestock. How orthobunyaviruses (OBVs) penetrate and infect mammalian
    host cells remains poorly characterized. Here, we investigated the entry mechanisms
    of the OBV Germiston (GERV). Viral particles were visualized by cryo-electron
    microscopy and appeared roughly spherical with an average diameter of 98 nm. Labeling
    of the virus with fluorescent dyes did not adversely affect its infectivity and
    allowed the monitoring of single particles in fixed and live cells. Using this
    approach, we found that endocytic internalization of bound viruses was asynchronous
    and occurred within 30-40 min. The virus entered Rab5a+ early endosomes and, subsequently,
    late endosomal vacuoles containing Rab7a but not LAMP-1. Infectious entry did
    not require proteolytic cleavage, and endosomal acidification was sufficient and
    necessary for viral fusion. Acid-activated penetration began 15-25 min after initiation
    of virus internalization and relied on maturation of early endosomes to late endosomes.
    The optimal pH for viral membrane fusion was slightly below 6.0, and penetration
    was hampered when the potassium influx was abolished. Overall, our study provides
    real-time visualization of GERV entry into host cells and demonstrates the importance
    of late endosomal maturation in facilitating OBV penetration.
acknowledged_ssus:
- _id: EM-Fac
acknowledgement: This work  was  supported  by  INRAE  starter  funds, Project IDEXLYON  (University  of  Lyon)
  within  the  Programme  Investissements  d’Avenir  (ANR-16-IDEX-0005),  and  FINOVIAO14
  (Fondation  pour  l’Université  de  Lyon),  all  to  P.Y.L.  This  work  was  also  supported  by
  CellNetworks  Research  Group  funds  and  Deutsche  Forschungsgemeinschaft  (DFG)  funding
  (grant  numbers  LO-2338/1-1  and  LO-2338/3-1)  awarded  to  P.Y.L., Austrian  Science  Fund
  (FWF)  grant  P31445  to  F.K.M.S., a  Chinese  Scholarship  Council (CSC;no.  201904910701)
  fellowship  to   Q.X.,  and  a  ministére  de  l’enseignement  supérieur,  de  la  recherche  et  de
  l’innovation (MESRI) doctoral thesis grant to M.D.
article_number: e02146-21
article_processing_charge: No
article_type: original
author:
- first_name: Stefan
  full_name: Windhaber, Stefan
  last_name: Windhaber
- first_name: Qilin
  full_name: Xin, Qilin
  last_name: Xin
- first_name: Zina M.
  full_name: Uckeley, Zina M.
  last_name: Uckeley
- first_name: Jana
  full_name: Koch, Jana
  last_name: Koch
- first_name: Martin
  full_name: Obr, Martin
  id: 4741CA5A-F248-11E8-B48F-1D18A9856A87
  last_name: Obr
  orcid: 0000-0003-1756-6564
- first_name: Céline
  full_name: Garnier, Céline
  last_name: Garnier
- first_name: Catherine
  full_name: Luengo-Guyonnot, Catherine
  last_name: Luengo-Guyonnot
- first_name: Maëva
  full_name: Duboeuf, Maëva
  last_name: Duboeuf
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Pierre-Yves
  full_name: Lozach, Pierre-Yves
  last_name: Lozach
citation:
  ama: Windhaber S, Xin Q, Uckeley ZM, et al. The Orthobunyavirus Germiston enters
    host cells from late endosomes. <i>Journal of Virology</i>. 2022;96(5). doi:<a
    href="https://doi.org/10.1128/jvi.02146-21">10.1128/jvi.02146-21</a>
  apa: Windhaber, S., Xin, Q., Uckeley, Z. M., Koch, J., Obr, M., Garnier, C., … Lozach,
    P.-Y. (2022). The Orthobunyavirus Germiston enters host cells from late endosomes.
    <i>Journal of Virology</i>. American Society for Microbiology. <a href="https://doi.org/10.1128/jvi.02146-21">https://doi.org/10.1128/jvi.02146-21</a>
  chicago: Windhaber, Stefan, Qilin Xin, Zina M. Uckeley, Jana Koch, Martin Obr, Céline
    Garnier, Catherine Luengo-Guyonnot, Maëva Duboeuf, Florian KM Schur, and Pierre-Yves
    Lozach. “The Orthobunyavirus Germiston Enters Host Cells from Late Endosomes.”
    <i>Journal of Virology</i>. American Society for Microbiology, 2022. <a href="https://doi.org/10.1128/jvi.02146-21">https://doi.org/10.1128/jvi.02146-21</a>.
  ieee: S. Windhaber <i>et al.</i>, “The Orthobunyavirus Germiston enters host cells
    from late endosomes,” <i>Journal of Virology</i>, vol. 96, no. 5. American Society
    for Microbiology, 2022.
  ista: Windhaber S, Xin Q, Uckeley ZM, Koch J, Obr M, Garnier C, Luengo-Guyonnot
    C, Duboeuf M, Schur FK, Lozach P-Y. 2022. The Orthobunyavirus Germiston enters
    host cells from late endosomes. Journal of Virology. 96(5), e02146-21.
  mla: Windhaber, Stefan, et al. “The Orthobunyavirus Germiston Enters Host Cells
    from Late Endosomes.” <i>Journal of Virology</i>, vol. 96, no. 5, e02146-21, American
    Society for Microbiology, 2022, doi:<a href="https://doi.org/10.1128/jvi.02146-21">10.1128/jvi.02146-21</a>.
  short: S. Windhaber, Q. Xin, Z.M. Uckeley, J. Koch, M. Obr, C. Garnier, C. Luengo-Guyonnot,
    M. Duboeuf, F.K. Schur, P.-Y. Lozach, Journal of Virology 96 (2022).
date_created: 2022-01-18T10:04:18Z
date_published: 2022-03-01T00:00:00Z
date_updated: 2025-04-15T08:24:49Z
day: '01'
department:
- _id: FlSc
doi: 10.1128/jvi.02146-21
external_id:
  isi:
  - '000779305000033'
  pmid:
  - '35019710'
intvolume: '        96'
isi: 1
issue: '5'
keyword:
- virology
- insect science
- immunology
- microbiology
language:
- iso: eng
main_file_link:
- open_access: '1'
  url: https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8906410
month: '03'
oa: 1
oa_version: Published Version
pmid: 1
project:
- _id: 26736D6A-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: P31445
  name: Structural conservation and diversity in retroviral capsid
publication: Journal of Virology
publication_identifier:
  eissn:
  - 1098-5514
  issn:
  - 0022-538X
publication_status: published
publisher: American Society for Microbiology
quality_controlled: '1'
scopus_import: '1'
status: public
title: The Orthobunyavirus Germiston enters host cells from late endosomes
type: journal_article
user_id: 4359f0d1-fa6c-11eb-b949-802e58b17ae8
volume: 96
year: '2022'
...
---
_id: '11155'
abstract:
- lang: eng
  text: The potential of energy filtering and direct electron detection for cryo-electron
    microscopy (cryo-EM) has been well documented. Here, we assess the performance
    of recently introduced hardware for cryo-electron tomography (cryo-ET) and subtomogram
    averaging (STA), an increasingly popular structural determination method for complex
    3D specimens. We acquired cryo-ET datasets of EIAV virus-like particles (VLPs)
    on two contemporary cryo-EM systems equipped with different energy filters and
    direct electron detectors (DED), specifically a Krios G4, equipped with a cold
    field emission gun (CFEG), Thermo Fisher Scientific Selectris X energy filter,
    and a Falcon 4 DED; and a Krios G3i, with a Schottky field emission gun (XFEG),
    a Gatan Bioquantum energy filter, and a K3 DED. We performed constrained cross-correlation-based
    STA on equally sized datasets acquired on the respective systems. The resulting
    EIAV CA hexamer reconstructions show that both systems perform comparably in the
    4–6 Å resolution range based on Fourier-Shell correlation (FSC). In addition,
    by employing a recently introduced multiparticle refinement approach, we obtained
    a reconstruction of the EIAV CA hexamer at 2.9 Å. Our results demonstrate the
    potential of the new generation of energy filters and DEDs for STA, and the effects
    of using different processing pipelines on their STA outcomes.
acknowledged_ssus:
- _id: LifeSc
- _id: ScienComp
- _id: EM-Fac
acknowledgement: This work was funded by the Austrian Science Fund (FWF) grant P31445
  to F.K.M.S and the National Institute of Allergy and Infectious Diseases under awards
  R01AI147890 to R.A.D. This research was also supported by the Scientific Service
  Units (SSUs) of IST Austria through resources provided by Scientific Computing (SciComp),
  the Life Science Facility (LSF), and the Electron Microscopy Facility (EMF). We
  thank Dustin Morado for providing the software SubTOM for data processing. We also
  thank William Wan for critical reading of the manuscript and valuable feedback.
article_number: '107852'
article_processing_charge: Yes (via OA deal)
article_type: original
author:
- first_name: Martin
  full_name: Obr, Martin
  id: 4741CA5A-F248-11E8-B48F-1D18A9856A87
  last_name: Obr
  orcid: 0000-0003-1756-6564
- first_name: Wim J.H.
  full_name: Hagen, Wim J.H.
  last_name: Hagen
- first_name: Robert A.
  full_name: Dick, Robert A.
  last_name: Dick
- first_name: Lingbo
  full_name: Yu, Lingbo
  last_name: Yu
- first_name: Abhay
  full_name: Kotecha, Abhay
  last_name: Kotecha
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Obr M, Hagen WJH, Dick RA, Yu L, Kotecha A, Schur FK. Exploring high-resolution
    cryo-ET and subtomogram averaging capabilities of contemporary DEDs. <i>Journal
    of Structural Biology</i>. 2022;214(2). doi:<a href="https://doi.org/10.1016/j.jsb.2022.107852">10.1016/j.jsb.2022.107852</a>
  apa: Obr, M., Hagen, W. J. H., Dick, R. A., Yu, L., Kotecha, A., &#38; Schur, F.
    K. (2022). Exploring high-resolution cryo-ET and subtomogram averaging capabilities
    of contemporary DEDs. <i>Journal of Structural Biology</i>. Elsevier. <a href="https://doi.org/10.1016/j.jsb.2022.107852">https://doi.org/10.1016/j.jsb.2022.107852</a>
  chicago: Obr, Martin, Wim J.H. Hagen, Robert A. Dick, Lingbo Yu, Abhay Kotecha,
    and Florian KM Schur. “Exploring High-Resolution Cryo-ET and Subtomogram Averaging
    Capabilities of Contemporary DEDs.” <i>Journal of Structural Biology</i>. Elsevier,
    2022. <a href="https://doi.org/10.1016/j.jsb.2022.107852">https://doi.org/10.1016/j.jsb.2022.107852</a>.
  ieee: M. Obr, W. J. H. Hagen, R. A. Dick, L. Yu, A. Kotecha, and F. K. Schur, “Exploring
    high-resolution cryo-ET and subtomogram averaging capabilities of contemporary
    DEDs,” <i>Journal of Structural Biology</i>, vol. 214, no. 2. Elsevier, 2022.
  ista: Obr M, Hagen WJH, Dick RA, Yu L, Kotecha A, Schur FK. 2022. Exploring high-resolution
    cryo-ET and subtomogram averaging capabilities of contemporary DEDs. Journal of
    Structural Biology. 214(2), 107852.
  mla: Obr, Martin, et al. “Exploring High-Resolution Cryo-ET and Subtomogram Averaging
    Capabilities of Contemporary DEDs.” <i>Journal of Structural Biology</i>, vol.
    214, no. 2, 107852, Elsevier, 2022, doi:<a href="https://doi.org/10.1016/j.jsb.2022.107852">10.1016/j.jsb.2022.107852</a>.
  short: M. Obr, W.J.H. Hagen, R.A. Dick, L. Yu, A. Kotecha, F.K. Schur, Journal of
    Structural Biology 214 (2022).
corr_author: '1'
date_created: 2022-04-15T07:10:26Z
date_published: 2022-06-01T00:00:00Z
date_updated: 2025-04-15T08:24:50Z
day: '01'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.1016/j.jsb.2022.107852
external_id:
  isi:
  - '000790733600001'
  pmid:
  - '35351542'
file:
- access_level: open_access
  checksum: 0b1eb53447aae8e95ae4c12d193b0b00
  content_type: application/pdf
  creator: dernst
  date_created: 2022-08-02T11:07:58Z
  date_updated: 2022-08-02T11:07:58Z
  file_id: '11722'
  file_name: 2022_JourStructuralBiology_Obr.pdf
  file_size: 7080863
  relation: main_file
  success: 1
file_date_updated: 2022-08-02T11:07:58Z
has_accepted_license: '1'
intvolume: '       214'
isi: 1
issue: '2'
keyword:
- Structural Biology
language:
- iso: eng
month: '06'
oa: 1
oa_version: Published Version
pmid: 1
project:
- _id: 26736D6A-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: P31445
  name: Structural conservation and diversity in retroviral capsid
publication: Journal of Structural Biology
publication_identifier:
  issn:
  - 1047-8477
publication_status: published
publisher: Elsevier
quality_controlled: '1'
scopus_import: '1'
status: public
title: Exploring high-resolution cryo-ET and subtomogram averaging capabilities of
  contemporary DEDs
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 4359f0d1-fa6c-11eb-b949-802e58b17ae8
volume: 214
year: '2022'
...
---
_id: '11351'
abstract:
- lang: eng
  text: 'One hallmark of plant cells is their cell wall. They protect cells against
    the environment and high turgor and mediate morphogenesis through the dynamics
    of their mechanical and chemical properties. The walls are a complex polysaccharidic
    structure. Although their biochemical composition is well known, how the different
    components organize in the volume of the cell wall and interact with each other
    is not well understood and yet is key to the wall’s mechanical properties. To
    investigate the ultrastructure of the plant cell wall, we imaged the walls of
    onion (Allium cepa) bulbs in a near-native state via cryo-focused ion beam milling
    (cryo-FIB milling) and cryo-electron tomography (cryo-ET). This allowed the high-resolution
    visualization of cellulose fibers in situ. We reveal the coexistence of dense
    fiber fields bathed in a reticulated matrix we termed “meshing,” which is more
    abundant at the inner surface of the cell wall. The fibers adopted a regular bimodal
    angular distribution at all depths in the cell wall and bundled according to their
    orientation, creating layers within the cell wall. Concomitantly, employing homogalacturonan
    (HG)-specific enzymatic digestion, we observed changes in the meshing, suggesting
    that it is—at least in part—composed of HG pectins. We propose the following model
    for the construction of the abaxial epidermal primary cell wall: the cell deposits
    successive layers of cellulose fibers at −45° and +45° relative to the cell’s
    long axis and secretes the surrounding HG-rich meshing proximal to the plasma
    membrane, which then migrates to more distal regions of the cell wall.'
acknowledgement: This work was supported by the Howard Hughes Medical Institute (HHMI)
  and grant R35 GM122588 to G.J. and the Austrian Science Fund (FWF) P33367 to F.K.M.S.
  We thank Noé Cochetel for his guidance and great help in data analysis, discovery,
  and representation with the R software. We thank Hans-Ulrich Endress for graciously
  providing us with the purified citrus pectin and Jozef Mravec for generating and
  providing the COS488 probe. Cryo-EM work was done in the Beckman Institute Resource
  Center for Transmission Electron Microscopy at Caltech. This article is subject
  to HHMI’s Open Access to Publications policy. HHMI lab heads have previously granted
  a nonexclusive CC BY 4.0 license to the public and a sublicensable license to HHMI
  in their research articles. Pursuant to those licenses, the author accepted manuscript
  of this article can be made freely available under a CC BY 4.0 license immediately
  upon publication.
article_processing_charge: No
article_type: original
author:
- first_name: William J.
  full_name: Nicolas, William J.
  last_name: Nicolas
- first_name: Florian
  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Przemysław
  full_name: Dutka, Przemysław
  last_name: Dutka
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Grant
  full_name: Jensen, Grant
  last_name: Jensen
- first_name: Elliot
  full_name: Meyerowitz, Elliot
  last_name: Meyerowitz
citation:
  ama: Nicolas WJ, Fäßler F, Dutka P, Schur FK, Jensen G, Meyerowitz E. Cryo-electron
    tomography of the onion cell wall shows bimodally oriented cellulose fibers and
    reticulated homogalacturonan networks. <i>Current Biology</i>. 2022;32(11):P2375-2389.
    doi:<a href="https://doi.org/10.1016/j.cub.2022.04.024">10.1016/j.cub.2022.04.024</a>
  apa: Nicolas, W. J., Fäßler, F., Dutka, P., Schur, F. K., Jensen, G., &#38; Meyerowitz,
    E. (2022). Cryo-electron tomography of the onion cell wall shows bimodally oriented
    cellulose fibers and reticulated homogalacturonan networks. <i>Current Biology</i>.
    Elsevier. <a href="https://doi.org/10.1016/j.cub.2022.04.024">https://doi.org/10.1016/j.cub.2022.04.024</a>
  chicago: Nicolas, William J., Florian Fäßler, Przemysław Dutka, Florian KM Schur,
    Grant Jensen, and Elliot Meyerowitz. “Cryo-Electron Tomography of the Onion Cell
    Wall Shows Bimodally Oriented Cellulose Fibers and Reticulated Homogalacturonan
    Networks.” <i>Current Biology</i>. Elsevier, 2022. <a href="https://doi.org/10.1016/j.cub.2022.04.024">https://doi.org/10.1016/j.cub.2022.04.024</a>.
  ieee: W. J. Nicolas, F. Fäßler, P. Dutka, F. K. Schur, G. Jensen, and E. Meyerowitz,
    “Cryo-electron tomography of the onion cell wall shows bimodally oriented cellulose
    fibers and reticulated homogalacturonan networks,” <i>Current Biology</i>, vol.
    32, no. 11. Elsevier, pp. P2375-2389, 2022.
  ista: Nicolas WJ, Fäßler F, Dutka P, Schur FK, Jensen G, Meyerowitz E. 2022. Cryo-electron
    tomography of the onion cell wall shows bimodally oriented cellulose fibers and
    reticulated homogalacturonan networks. Current Biology. 32(11), P2375-2389.
  mla: Nicolas, William J., et al. “Cryo-Electron Tomography of the Onion Cell Wall
    Shows Bimodally Oriented Cellulose Fibers and Reticulated Homogalacturonan Networks.”
    <i>Current Biology</i>, vol. 32, no. 11, Elsevier, 2022, pp. P2375-2389, doi:<a
    href="https://doi.org/10.1016/j.cub.2022.04.024">10.1016/j.cub.2022.04.024</a>.
  short: W.J. Nicolas, F. Fäßler, P. Dutka, F.K. Schur, G. Jensen, E. Meyerowitz,
    Current Biology 32 (2022) P2375-2389.
date_created: 2022-05-04T06:22:06Z
date_published: 2022-06-06T00:00:00Z
date_updated: 2025-04-15T08:25:40Z
day: '06'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.1016/j.cub.2022.04.024
external_id:
  isi:
  - '000822399200019'
  pmid:
  - '35508170'
file:
- access_level: open_access
  checksum: af3f24d97c016d844df237abef987639
  content_type: application/pdf
  creator: dernst
  date_created: 2022-08-05T06:29:18Z
  date_updated: 2022-08-05T06:29:18Z
  file_id: '11730'
  file_name: 2022_CurrentBiology_Nicolas.pdf
  file_size: 12827717
  relation: main_file
  success: 1
file_date_updated: 2022-08-05T06:29:18Z
has_accepted_license: '1'
intvolume: '        32'
isi: 1
issue: '11'
keyword:
- General Agricultural and Biological Sciences
- General Biochemistry
- Genetics and Molecular Biology
language:
- iso: eng
month: '06'
oa: 1
oa_version: Published Version
page: P2375-2389
pmid: 1
project:
- _id: 9B954C5C-BA93-11EA-9121-9846C619BF3A
  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
publication: Current Biology
publication_identifier:
  issn:
  - 0960-9822
publication_status: published
publisher: Elsevier
quality_controlled: '1'
scopus_import: '1'
status: public
title: Cryo-electron tomography of the onion cell wall shows bimodally oriented cellulose
  fibers and reticulated homogalacturonan networks
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 4359f0d1-fa6c-11eb-b949-802e58b17ae8
volume: 32
year: '2022'
...
---
_id: '10103'
abstract:
- lang: eng
  text: The small cellular molecule inositol hexakisphosphate (IP6) has been known
    for ~20 years to promote the in vitro assembly of HIV-1 into immature virus-like
    particles. However, the molecular details underlying this effect have been determined
    only recently, with the identification of the IP6 binding site in the immature
    Gag lattice. IP6 also promotes formation of the mature capsid protein (CA) lattice
    via a second IP6 binding site, and enhances core stability, creating a favorable
    environment for reverse transcription. IP6 also enhances assembly of other retroviruses,
    from both the Lentivirus and the Alpharetrovirus genera. These findings suggest
    that IP6 may have a conserved function throughout the family Retroviridae. Here,
    we discuss the different steps in the viral life cycle that are influenced by
    IP6, and describe in detail how IP6 interacts with the immature and mature lattices
    of different retroviruses.
acknowledgement: We thank Volker M. Vogt for his critical comments in preparation
  of the review.
article_number: '1853'
article_processing_charge: Yes
article_type: original
author:
- first_name: Martin
  full_name: Obr, Martin
  id: 4741CA5A-F248-11E8-B48F-1D18A9856A87
  last_name: Obr
  orcid: 0000-0003-1756-6564
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Robert A.
  full_name: Dick, Robert A.
  last_name: Dick
citation:
  ama: Obr M, Schur FK, Dick RA. A structural perspective of the role of IP6 in immature
    and mature retroviral assembly. <i>Viruses</i>. 2021;13(9). doi:<a href="https://doi.org/10.3390/v13091853">10.3390/v13091853</a>
  apa: Obr, M., Schur, F. K., &#38; Dick, R. A. (2021). A structural perspective of
    the role of IP6 in immature and mature retroviral assembly. <i>Viruses</i>. MDPI.
    <a href="https://doi.org/10.3390/v13091853">https://doi.org/10.3390/v13091853</a>
  chicago: Obr, Martin, Florian KM Schur, and Robert A. Dick. “A Structural Perspective
    of the Role of IP6 in Immature and Mature Retroviral Assembly.” <i>Viruses</i>.
    MDPI, 2021. <a href="https://doi.org/10.3390/v13091853">https://doi.org/10.3390/v13091853</a>.
  ieee: M. Obr, F. K. Schur, and R. A. Dick, “A structural perspective of the role
    of IP6 in immature and mature retroviral assembly,” <i>Viruses</i>, vol. 13, no.
    9. MDPI, 2021.
  ista: Obr M, Schur FK, Dick RA. 2021. A structural perspective of the role of IP6
    in immature and mature retroviral assembly. Viruses. 13(9), 1853.
  mla: Obr, Martin, et al. “A Structural Perspective of the Role of IP6 in Immature
    and Mature Retroviral Assembly.” <i>Viruses</i>, vol. 13, no. 9, 1853, MDPI, 2021,
    doi:<a href="https://doi.org/10.3390/v13091853">10.3390/v13091853</a>.
  short: M. Obr, F.K. Schur, R.A. Dick, Viruses 13 (2021).
corr_author: '1'
date_created: 2021-10-07T09:13:29Z
date_published: 2021-09-17T00:00:00Z
date_updated: 2025-04-15T08:24:49Z
day: '17'
ddc:
- '616'
department:
- _id: FlSc
doi: 10.3390/v13091853
external_id:
  isi:
  - '000699841100001'
  pmid:
  - '34578434'
file:
- access_level: open_access
  checksum: bcfd72a12977d48e22df3d0cc55aacf1
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  date_created: 2021-10-08T10:38:15Z
  date_updated: 2021-10-08T10:38:15Z
  file_id: '10115'
  file_name: 2021_Viruses_Obr.pdf
  file_size: 4146796
  relation: main_file
  success: 1
file_date_updated: 2021-10-08T10:38:15Z
has_accepted_license: '1'
intvolume: '        13'
isi: 1
issue: '9'
keyword:
- virology
- infectious diseases
language:
- iso: eng
month: '09'
oa: 1
oa_version: Published Version
pmid: 1
project:
- _id: 26736D6A-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: P31445
  name: Structural conservation and diversity in retroviral capsid
publication: Viruses
publication_identifier:
  issn:
  - 1999-4915
publication_status: published
publisher: MDPI
quality_controlled: '1'
scopus_import: '1'
status: public
title: A structural perspective of the role of IP6 in immature and mature retroviral
  assembly
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 4359f0d1-fa6c-11eb-b949-802e58b17ae8
volume: 13
year: '2021'
...
---
_id: '10290'
abstract:
- lang: eng
  text: A precise quantitative description of the ultrastructural characteristics
    underlying biological mechanisms is often key to their understanding. This is
    particularly true for dynamic extra- and intracellular filamentous assemblies,
    playing a role in cell motility, cell integrity, cytokinesis, tissue formation
    and maintenance. For example, genetic manipulation or modulation of actin regulatory
    proteins frequently manifests in changes of the morphology, dynamics, and ultrastructural
    architecture of actin filament-rich cell peripheral structures, such as lamellipodia
    or filopodia. However, the observed ultrastructural effects often remain subtle
    and require sufficiently large datasets for appropriate quantitative analysis.
    The acquisition of such large datasets has been enabled by recent advances in
    high-throughput cryo-electron tomography (cryo-ET) methods. This also necessitates
    the development of complementary approaches to maximize the extraction of relevant
    biological information. We have developed a computational toolbox for the semi-automatic
    quantification of segmented and vectorized filamentous networks from pre-processed
    cryo-electron tomograms, facilitating the analysis and cross-comparison of multiple
    experimental conditions. GUI-based components simplify the processing of data
    and allow users to obtain a large number of ultrastructural parameters describing
    filamentous assemblies. We demonstrate the feasibility of this workflow by analyzing
    cryo-ET data of untreated and chemically perturbed branched actin filament networks
    and that of parallel actin filament arrays. In principle, the computational toolbox
    presented here is applicable for data analysis comprising any type of filaments
    in regular (i.e. parallel) or random arrangement. We show that it can ease the
    identification of key differences between experimental groups and facilitate the
    in-depth analysis of ultrastructural data in a time-efficient manner.
acknowledged_ssus:
- _id: ScienComp
- _id: LifeSc
- _id: Bio
- _id: EM-Fac
acknowledgement: 'This research was supported by the Scientific Service Units (SSUs)
  of IST Austria through resources provided by Scientific Computing (SciComp), the
  Life Science Facility (LSF), the BioImaging Facility (BIF), and the Electron Microscopy
  Facility (EMF). We also thank Victor-Valentin Hodirnau for help with cryo-ET data
  acquisition. The authors acknowledge support from IST Austria and from the Austrian
  Science Fund (FWF): M02495 to G.D. and Austrian Science Fund (FWF): P33367 to F.K.M.S.'
article_number: '107808'
article_processing_charge: Yes (via OA deal)
article_type: original
author:
- first_name: Georgi A
  full_name: Dimchev, Georgi A
  id: 38C393BE-F248-11E8-B48F-1D18A9856A87
  last_name: Dimchev
  orcid: 0000-0001-8370-6161
- first_name: Behnam
  full_name: Amiri, Behnam
  last_name: Amiri
- first_name: Florian
  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Martin
  full_name: Falcke, Martin
  last_name: Falcke
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Dimchev GA, Amiri B, Fäßler F, Falcke M, Schur FK. Computational toolbox for
    ultrastructural quantitative analysis of filament networks in cryo-ET data. <i>Journal
    of Structural Biology</i>. 2021;213(4). doi:<a href="https://doi.org/10.1016/j.jsb.2021.107808">10.1016/j.jsb.2021.107808</a>
  apa: Dimchev, G. A., Amiri, B., Fäßler, F., Falcke, M., &#38; Schur, F. K. (2021).
    Computational toolbox for ultrastructural quantitative analysis of filament networks
    in cryo-ET data. <i>Journal of Structural Biology</i>. Elsevier . <a href="https://doi.org/10.1016/j.jsb.2021.107808">https://doi.org/10.1016/j.jsb.2021.107808</a>
  chicago: Dimchev, Georgi A, Behnam Amiri, Florian Fäßler, Martin Falcke, and Florian
    KM Schur. “Computational Toolbox for Ultrastructural Quantitative Analysis of
    Filament Networks in Cryo-ET Data.” <i>Journal of Structural Biology</i>. Elsevier
    , 2021. <a href="https://doi.org/10.1016/j.jsb.2021.107808">https://doi.org/10.1016/j.jsb.2021.107808</a>.
  ieee: G. A. Dimchev, B. Amiri, F. Fäßler, M. Falcke, and F. K. Schur, “Computational
    toolbox for ultrastructural quantitative analysis of filament networks in cryo-ET
    data,” <i>Journal of Structural Biology</i>, vol. 213, no. 4. Elsevier , 2021.
  ista: Dimchev GA, Amiri B, Fäßler F, Falcke M, Schur FK. 2021. Computational toolbox
    for ultrastructural quantitative analysis of filament networks in cryo-ET data.
    Journal of Structural Biology. 213(4), 107808.
  mla: Dimchev, Georgi A., et al. “Computational Toolbox for Ultrastructural Quantitative
    Analysis of Filament Networks in Cryo-ET Data.” <i>Journal of Structural Biology</i>,
    vol. 213, no. 4, 107808, Elsevier , 2021, doi:<a href="https://doi.org/10.1016/j.jsb.2021.107808">10.1016/j.jsb.2021.107808</a>.
  short: G.A. Dimchev, B. Amiri, F. Fäßler, M. Falcke, F.K. Schur, Journal of Structural
    Biology 213 (2021).
corr_author: '1'
date_created: 2021-11-15T12:21:42Z
date_published: 2021-11-03T00:00:00Z
date_updated: 2025-04-15T08:25:41Z
day: '03'
ddc:
- '572'
department:
- _id: FlSc
doi: 10.1016/j.jsb.2021.107808
external_id:
  isi:
  - '000720259500002'
file:
- access_level: open_access
  checksum: 6b209e4d44775d4e02b50f78982c15fa
  content_type: application/pdf
  creator: cchlebak
  date_created: 2021-11-15T13:11:27Z
  date_updated: 2021-11-15T13:11:27Z
  file_id: '10291'
  file_name: 2021_JournalStructBiol_Dimchev.pdf
  file_size: 16818304
  relation: main_file
  success: 1
file_date_updated: 2021-11-15T13:11:27Z
has_accepted_license: '1'
intvolume: '       213'
isi: 1
issue: '4'
keyword:
- Structural Biology
language:
- iso: eng
month: '11'
oa: 1
oa_version: Published Version
project:
- _id: 9B954C5C-BA93-11EA-9121-9846C619BF3A
  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
- _id: 2674F658-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: M02495
  name: Protein structure and function in filopodia across scales
publication: Journal of Structural Biology
publication_identifier:
  issn:
  - 1047-8477
publication_status: published
publisher: 'Elsevier '
quality_controlled: '1'
related_material:
  record:
  - id: '14502'
    relation: software
    status: public
scopus_import: '1'
status: public
title: Computational toolbox for ultrastructural quantitative analysis of filament
  networks in cryo-ET data
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 213
year: '2021'
...
---
_id: '9431'
abstract:
- lang: eng
  text: Inositol hexakisphosphate (IP6) is an assembly cofactor for HIV-1. We report
    here that IP6 is also used for assembly of Rous sarcoma virus (RSV), a retrovirus
    from a different genus. IP6 is ~100-fold more potent at promoting RSV mature capsid
    protein (CA) assembly than observed for HIV-1 and removal of IP6 in cells reduces
    infectivity by 100-fold. Here, visualized by cryo-electron tomography and subtomogram
    averaging, mature capsid-like particles show an IP6-like density in the CA hexamer,
    coordinated by rings of six lysines and six arginines. Phosphate and IP6 have
    opposing effects on CA in vitro assembly, inducing formation of T = 1 icosahedrons
    and tubes, respectively, implying that phosphate promotes pentamer and IP6 hexamer
    formation. Subtomogram averaging and classification optimized for analysis of
    pleomorphic retrovirus particles reveal that the heterogeneity of mature RSV CA
    polyhedrons results from an unexpected, intrinsic CA hexamer flexibility. In contrast,
    the CA pentamer forms rigid units organizing the local architecture. These different
    features of hexamers and pentamers determine the structural mechanism to form
    CA polyhedrons of variable shape in mature RSV particles.
acknowledged_ssus:
- _id: ScienComp
- _id: LifeSc
- _id: EM-Fac
acknowledgement: This work was funded by the National Institute of Allergy and Infectious
  Diseases under awards R01AI147890 to R.A.D., R01AI150454 to V.M.V, R35GM136258 in
  support of J-P.R.F, and the Austrian Science Fund (FWF) grant P31445 to F.K.M.S.
  Access to high-resolution cryo-ET data acquisition at EMBL Heidelberg was supported
  by iNEXT (grant no. 653706), funded by the Horizon 2020 program of the European
  Union (PID 4246). We thank Wim Hagen and Felix Weis at EMBL Heidelberg for support
  in cryo-ET data acquisition. This work made use of the Cornell Center for Materials
  Research Shared Facilities, which are supported through the NSF MRSEC program (DMR-179875).
  This research was also supported by the Scientific Service Units (SSUs) of IST Austria
  through resources provided by Scientific Computing (SciComp), the Life Science Facility
  (LSF), and the Electron Microscopy Facility (EMF).
article_number: '3226'
article_processing_charge: No
article_type: original
author:
- first_name: Martin
  full_name: Obr, Martin
  id: 4741CA5A-F248-11E8-B48F-1D18A9856A87
  last_name: Obr
  orcid: 0000-0003-1756-6564
- first_name: Clifton L.
  full_name: Ricana, Clifton L.
  last_name: Ricana
- first_name: Nadia
  full_name: Nikulin, Nadia
  last_name: Nikulin
- first_name: Jon-Philip R.
  full_name: Feathers, Jon-Philip R.
  last_name: Feathers
- first_name: Marco
  full_name: Klanschnig, Marco
  last_name: Klanschnig
- first_name: Andreas
  full_name: Thader, Andreas
  id: 3A18A7B8-F248-11E8-B48F-1D18A9856A87
  last_name: Thader
- first_name: Marc C.
  full_name: Johnson, Marc C.
  last_name: Johnson
- first_name: Volker M.
  full_name: Vogt, Volker M.
  last_name: Vogt
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Robert A.
  full_name: Dick, Robert A.
  last_name: Dick
citation:
  ama: Obr M, Ricana CL, Nikulin N, et al. Structure of the mature Rous sarcoma virus
    lattice reveals a role for IP6 in the formation of the capsid hexamer. <i>Nature
    Communications</i>. 2021;12(1). doi:<a href="https://doi.org/10.1038/s41467-021-23506-0">10.1038/s41467-021-23506-0</a>
  apa: Obr, M., Ricana, C. L., Nikulin, N., Feathers, J.-P. R., Klanschnig, M., Thader,
    A., … Dick, R. A. (2021). Structure of the mature Rous sarcoma virus lattice reveals
    a role for IP6 in the formation of the capsid hexamer. <i>Nature Communications</i>.
    Nature Research. <a href="https://doi.org/10.1038/s41467-021-23506-0">https://doi.org/10.1038/s41467-021-23506-0</a>
  chicago: Obr, Martin, Clifton L. Ricana, Nadia Nikulin, Jon-Philip R. Feathers,
    Marco Klanschnig, Andreas Thader, Marc C. Johnson, Volker M. Vogt, Florian KM
    Schur, and Robert A. Dick. “Structure of the Mature Rous Sarcoma Virus Lattice
    Reveals a Role for IP6 in the Formation of the Capsid Hexamer.” <i>Nature Communications</i>.
    Nature Research, 2021. <a href="https://doi.org/10.1038/s41467-021-23506-0">https://doi.org/10.1038/s41467-021-23506-0</a>.
  ieee: M. Obr <i>et al.</i>, “Structure of the mature Rous sarcoma virus lattice
    reveals a role for IP6 in the formation of the capsid hexamer,” <i>Nature Communications</i>,
    vol. 12, no. 1. Nature Research, 2021.
  ista: Obr M, Ricana CL, Nikulin N, Feathers J-PR, Klanschnig M, Thader A, Johnson
    MC, Vogt VM, Schur FK, Dick RA. 2021. Structure of the mature Rous sarcoma virus
    lattice reveals a role for IP6 in the formation of the capsid hexamer. Nature
    Communications. 12(1), 3226.
  mla: Obr, Martin, et al. “Structure of the Mature Rous Sarcoma Virus Lattice Reveals
    a Role for IP6 in the Formation of the Capsid Hexamer.” <i>Nature Communications</i>,
    vol. 12, no. 1, 3226, Nature Research, 2021, doi:<a href="https://doi.org/10.1038/s41467-021-23506-0">10.1038/s41467-021-23506-0</a>.
  short: M. Obr, C.L. Ricana, N. Nikulin, J.-P.R. Feathers, M. Klanschnig, A. Thader,
    M.C. Johnson, V.M. Vogt, F.K. Schur, R.A. Dick, Nature Communications 12 (2021).
corr_author: '1'
date_created: 2021-05-28T14:25:50Z
date_published: 2021-05-28T00:00:00Z
date_updated: 2025-04-15T08:24:49Z
day: '28'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.1038/s41467-021-23506-0
external_id:
  isi:
  - '000659145000011'
file:
- access_level: open_access
  checksum: 53ccc53d09a9111143839dbe7784e663
  content_type: application/pdf
  creator: kschuh
  date_created: 2021-06-09T15:21:14Z
  date_updated: 2021-06-09T15:21:14Z
  file_id: '9538'
  file_name: 2021_NatureCommunications_Obr.pdf
  file_size: 6166295
  relation: main_file
  success: 1
file_date_updated: 2021-06-09T15:21:14Z
has_accepted_license: '1'
intvolume: '        12'
isi: 1
issue: '1'
keyword:
- General Biochemistry
- Genetics and Molecular Biology
- General Physics and Astronomy
- General Chemistry
language:
- iso: eng
month: '05'
oa: 1
oa_version: Published Version
project:
- _id: 26736D6A-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: P31445
  name: Structural conservation and diversity in retroviral capsid
publication: Nature Communications
publication_identifier:
  eissn:
  - 2041-1723
publication_status: published
publisher: Nature Research
quality_controlled: '1'
related_material:
  link:
  - description: News on IST Homepage
    relation: press_release
    url: https://ist.ac.at/en/news/how-retroviruses-become-infectious/
scopus_import: '1'
status: public
title: Structure of the mature Rous sarcoma virus lattice reveals a role for IP6 in
  the formation of the capsid hexamer
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 4359f0d1-fa6c-11eb-b949-802e58b17ae8
volume: 12
year: '2021'
...
---
_id: '9429'
abstract:
- lang: eng
  text: De novo loss of function mutations in the ubiquitin ligase-encoding gene Cullin3
    lead to autism spectrum disorder (ASD). In mouse, constitutive haploinsufficiency
    leads to motor coordination deficits as well as ASD-relevant social and cognitive
    impairments. However, induction of Cul3 haploinsufficiency later in life does
    not lead to ASD-relevant behaviors, pointing to an important role of Cul3 during
    a critical developmental window. Here we show that Cul3 is essential to regulate
    neuronal migration and, therefore, constitutive Cul3 heterozygous mutant mice
    display cortical lamination abnormalities. At the molecular level, we found that
    Cul3 controls neuronal migration by tightly regulating the amount of Plastin3
    (Pls3), a previously unrecognized player of neural migration. Furthermore, we
    found that Pls3 cell-autonomously regulates cell migration by regulating actin
    cytoskeleton organization, and its levels are inversely proportional to neural
    migration speed. Finally, we provide evidence that cellular phenotypes associated
    with autism-linked gene haploinsufficiency can be rescued by transcriptional activation
    of the intact allele in vitro, offering a proof of concept for a potential therapeutic
    approach for ASDs.
acknowledged_ssus:
- _id: PreCl
acknowledgement: We thank A. Coll Manzano, F. Freeman, M. Ladron de Guevara, and A.
  Ç. Yahya for technical assistance, S. Deixler, A. Lepold, and A. Schlerka for the
  management of our animal colony, as well as M. Schunn and the Preclinical Facility
  team for technical assistance. We thank K. Heesom and her team at the University
  of Bristol Proteomics Facility for the proteomics sample preparation, data generation,
  and analysis support. We thank Y. B. Simon for kindly providing the plasmid for
  lentiviral labeling. Further, we thank M. Sixt for his advice regarding cell migration
  and the fruitful discussions. This work was supported by the ISTPlus postdoctoral
  fellowship (Grant Agreement No. 754411) to B.B., by the European Union’s Horizon
  2020 research and innovation program (ERC) grant 715508 (REVERSEAUTISM), and by
  the Austrian Science Fund (FWF) to G.N. (DK W1232-B24 and SFB F7807-B) and to J.G.D
  (I3600-B27).
article_number: '3058'
article_processing_charge: No
article_type: original
author:
- first_name: Jasmin
  full_name: Morandell, Jasmin
  id: 4739D480-F248-11E8-B48F-1D18A9856A87
  last_name: Morandell
- first_name: Lena A
  full_name: Schwarz, Lena A
  id: 29A8453C-F248-11E8-B48F-1D18A9856A87
  last_name: Schwarz
- first_name: Bernadette
  full_name: Basilico, Bernadette
  id: 36035796-5ACA-11E9-A75E-7AF2E5697425
  last_name: Basilico
  orcid: 0000-0003-1843-3173
- first_name: Saren
  full_name: Tasciyan, Saren
  id: 4323B49C-F248-11E8-B48F-1D18A9856A87
  last_name: Tasciyan
  orcid: 0000-0003-1671-393X
- first_name: Georgi A
  full_name: Dimchev, Georgi A
  id: 38C393BE-F248-11E8-B48F-1D18A9856A87
  last_name: Dimchev
  orcid: 0000-0001-8370-6161
- first_name: Armel
  full_name: Nicolas, Armel
  id: 2A103192-F248-11E8-B48F-1D18A9856A87
  last_name: Nicolas
- first_name: Christoph M
  full_name: Sommer, Christoph M
  id: 4DF26D8C-F248-11E8-B48F-1D18A9856A87
  last_name: Sommer
  orcid: 0000-0003-1216-9105
- first_name: Caroline
  full_name: Kreuzinger, Caroline
  id: 382077BA-F248-11E8-B48F-1D18A9856A87
  last_name: Kreuzinger
- first_name: Christoph
  full_name: Dotter, Christoph
  id: 4C66542E-F248-11E8-B48F-1D18A9856A87
  last_name: Dotter
  orcid: 0000-0002-9033-9096
- first_name: Lisa
  full_name: Knaus, Lisa
  id: 3B2ABCF4-F248-11E8-B48F-1D18A9856A87
  last_name: Knaus
- first_name: Zoe
  full_name: Dobler, Zoe
  id: D23090A2-9057-11EA-883A-A8396FC7A38F
  last_name: Dobler
- first_name: Emanuele
  full_name: Cacci, Emanuele
  last_name: Cacci
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
- first_name: Johann G
  full_name: Danzl, Johann G
  id: 42EFD3B6-F248-11E8-B48F-1D18A9856A87
  last_name: Danzl
  orcid: 0000-0001-8559-3973
- first_name: Gaia
  full_name: Novarino, Gaia
  id: 3E57A680-F248-11E8-B48F-1D18A9856A87
  last_name: Novarino
  orcid: 0000-0002-7673-7178
citation:
  ama: Morandell J, Schwarz LA, Basilico B, et al. Cul3 regulates cytoskeleton protein
    homeostasis and cell migration during a critical window of brain development.
    <i>Nature Communications</i>. 2021;12(1). doi:<a href="https://doi.org/10.1038/s41467-021-23123-x">10.1038/s41467-021-23123-x</a>
  apa: Morandell, J., Schwarz, L. A., Basilico, B., Tasciyan, S., Dimchev, G. A.,
    Nicolas, A., … Novarino, G. (2021). Cul3 regulates cytoskeleton protein homeostasis
    and cell migration during a critical window of brain development. <i>Nature Communications</i>.
    Springer Nature. <a href="https://doi.org/10.1038/s41467-021-23123-x">https://doi.org/10.1038/s41467-021-23123-x</a>
  chicago: Morandell, Jasmin, Lena A Schwarz, Bernadette Basilico, Saren Tasciyan,
    Georgi A Dimchev, Armel Nicolas, Christoph M Sommer, et al. “Cul3 Regulates Cytoskeleton
    Protein Homeostasis and Cell Migration during a Critical Window of Brain Development.”
    <i>Nature Communications</i>. Springer Nature, 2021. <a href="https://doi.org/10.1038/s41467-021-23123-x">https://doi.org/10.1038/s41467-021-23123-x</a>.
  ieee: J. Morandell <i>et al.</i>, “Cul3 regulates cytoskeleton protein homeostasis
    and cell migration during a critical window of brain development,” <i>Nature Communications</i>,
    vol. 12, no. 1. Springer Nature, 2021.
  ista: Morandell J, Schwarz LA, Basilico B, Tasciyan S, Dimchev GA, Nicolas A, Sommer
    CM, Kreuzinger C, Dotter C, Knaus L, Dobler Z, Cacci E, Schur FK, Danzl JG, Novarino
    G. 2021. Cul3 regulates cytoskeleton protein homeostasis and cell migration during
    a critical window of brain development. Nature Communications. 12(1), 3058.
  mla: Morandell, Jasmin, et al. “Cul3 Regulates Cytoskeleton Protein Homeostasis
    and Cell Migration during a Critical Window of Brain Development.” <i>Nature Communications</i>,
    vol. 12, no. 1, 3058, Springer Nature, 2021, doi:<a href="https://doi.org/10.1038/s41467-021-23123-x">10.1038/s41467-021-23123-x</a>.
  short: J. Morandell, L.A. Schwarz, B. Basilico, S. Tasciyan, G.A. Dimchev, A. Nicolas,
    C.M. Sommer, C. Kreuzinger, C. Dotter, L. Knaus, Z. Dobler, E. Cacci, F.K. Schur,
    J.G. Danzl, G. Novarino, Nature Communications 12 (2021).
corr_author: '1'
date_created: 2021-05-28T11:49:46Z
date_published: 2021-05-24T00:00:00Z
date_updated: 2026-04-27T22:30:54Z
day: '24'
ddc:
- '572'
department:
- _id: GaNo
- _id: JoDa
- _id: FlSc
- _id: MiSi
- _id: LifeSc
- _id: Bio
doi: 10.1038/s41467-021-23123-x
ec_funded: 1
external_id:
  isi:
  - '000658769900010'
file:
- access_level: open_access
  checksum: 337e0f7959c35ec959984cacdcb472ba
  content_type: application/pdf
  creator: kschuh
  date_created: 2021-05-28T12:39:43Z
  date_updated: 2021-05-28T12:39:43Z
  file_id: '9430'
  file_name: 2021_NatureCommunications_Morandell.pdf
  file_size: 9358599
  relation: main_file
  success: 1
file_date_updated: 2021-05-28T12:39:43Z
has_accepted_license: '1'
intvolume: '        12'
isi: 1
issue: '1'
keyword:
- General Biochemistry
- Genetics and Molecular Biology
language:
- iso: eng
month: '05'
oa: 1
oa_version: Published Version
project:
- _id: 260C2330-B435-11E9-9278-68D0E5697425
  call_identifier: H2020
  grant_number: '754411'
  name: ISTplus - Postdoctoral Fellowships
- _id: 25444568-B435-11E9-9278-68D0E5697425
  call_identifier: H2020
  grant_number: '715508'
  name: Probing the Reversibility of Autism Spectrum Disorders by Employing in vivo
    and in vitro Models
- _id: 2548AE96-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: W1232
  name: Molecular Drug Targets
- _id: 05A0D778-7A3F-11EA-A408-12923DDC885E
  grant_number: F7807
  name: Stem Cell Modulation in Neural Development and Regeneration/ P07-Neural stem
    cells in autism and epilepsy
- _id: 265CB4D0-B435-11E9-9278-68D0E5697425
  call_identifier: FWF
  grant_number: I03600
  name: Optical control of synaptic function via adhesion molecules
publication: Nature Communications
publication_identifier:
  eissn:
  - 2041-1723
publication_status: published
publisher: Springer Nature
quality_controlled: '1'
related_material:
  link:
  - relation: press_release
    url: https://ist.ac.at/en/news/defective-gene-slows-down-brain-cells/
  record:
  - id: '19557'
    relation: dissertation_contains
    status: public
  - id: '7800'
    relation: earlier_version
    status: public
  - id: '12401'
    relation: dissertation_contains
    status: public
scopus_import: '1'
status: public
title: Cul3 regulates cytoskeleton protein homeostasis and cell migration during a
  critical window of brain development
tmp:
  image: /images/cc_by.png
  legal_code_url: https://creativecommons.org/licenses/by/4.0/legalcode
  name: Creative Commons Attribution 4.0 International Public License (CC-BY 4.0)
  short: CC BY (4.0)
type: journal_article
user_id: 4359f0d1-fa6c-11eb-b949-802e58b17ae8
volume: 12
year: '2021'
...
---
_id: '14592'
abstract:
- lang: eng
  text: Cryo-electron microscopy (cryo-EM) of cellular specimens provides insights
    into biological processes and structures within a native context. However, a major
    challenge still lies in the efficient and reproducible preparation of adherent
    cells for subsequent cryo-EM analysis. This is due to the sensitivity of many
    cellular specimens to the varying seeding and culturing conditions required for
    EM experiments, the often limited amount of cellular material and also the fragility
    of EM grids and their substrate. Here, we present low-cost and reusable 3D printed
    grid holders, designed to improve specimen preparation when culturing challenging
    cellular samples directly on grids. The described grid holders increase cell culture
    reproducibility and throughput, and reduce the resources required for cell culturing.
    We show that grid holders can be integrated into various cryo-EM workflows, including
    micro-patterning approaches to control cell seeding on grids, and for generating
    samples for cryo-focused ion beam milling and cryo-electron tomography experiments.
    Their adaptable design allows for the generation of specialized grid holders customized
    to a large variety of applications.
article_processing_charge: No
author:
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Schur FK. STL-files for 3D-printed grid holders described in  Fäßler F, Zens
    B, et al.; 3D printed cell culture grid holders for improved cellular specimen
    preparation in cryo-electron microscopy. 2020. doi:<a href="https://doi.org/10.15479/AT:ISTA:14592">10.15479/AT:ISTA:14592</a>
  apa: Schur, F. K. (2020). STL-files for 3D-printed grid holders described in  Fäßler
    F, Zens B, et al.; 3D printed cell culture grid holders for improved cellular
    specimen preparation in cryo-electron microscopy. Institute of Science and Technology
    Austria. <a href="https://doi.org/10.15479/AT:ISTA:14592">https://doi.org/10.15479/AT:ISTA:14592</a>
  chicago: Schur, Florian KM. “STL-Files for 3D-Printed Grid Holders Described in 
    Fäßler F, Zens B, et Al.; 3D Printed Cell Culture Grid Holders for Improved Cellular
    Specimen Preparation in Cryo-Electron Microscopy.” Institute of Science and Technology
    Austria, 2020. <a href="https://doi.org/10.15479/AT:ISTA:14592">https://doi.org/10.15479/AT:ISTA:14592</a>.
  ieee: F. K. Schur, “STL-files for 3D-printed grid holders described in  Fäßler F,
    Zens B, et al.; 3D printed cell culture grid holders for improved cellular specimen
    preparation in cryo-electron microscopy.” Institute of Science and Technology
    Austria, 2020.
  ista: Schur FK. 2020. STL-files for 3D-printed grid holders described in  Fäßler
    F, Zens B, et al.; 3D printed cell culture grid holders for improved cellular
    specimen preparation in cryo-electron microscopy, Institute of Science and Technology
    Austria, <a href="https://doi.org/10.15479/AT:ISTA:14592">10.15479/AT:ISTA:14592</a>.
  mla: Schur, Florian KM. <i>STL-Files for 3D-Printed Grid Holders Described in  Fäßler
    F, Zens B, et Al.; 3D Printed Cell Culture Grid Holders for Improved Cellular
    Specimen Preparation in Cryo-Electron Microscopy</i>. Institute of Science and
    Technology Austria, 2020, doi:<a href="https://doi.org/10.15479/AT:ISTA:14592">10.15479/AT:ISTA:14592</a>.
  short: F.K. Schur, (2020).
contributor:
- contributor_type: researcher
  first_name: Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- contributor_type: researcher
  first_name: Bettina
  id: 45FD126C-F248-11E8-B48F-1D18A9856A87
  last_name: Zens
- contributor_type: researcher
  first_name: Robert
  id: 4E01D6B4-F248-11E8-B48F-1D18A9856A87
  last_name: Hauschild
- contributor_type: researcher
  first_name: Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
corr_author: '1'
date_created: 2023-11-22T15:00:57Z
date_published: 2020-12-01T00:00:00Z
date_updated: 2025-06-12T07:35:28Z
day: '01'
ddc:
- '570'
department:
- _id: FlSc
doi: 10.15479/AT:ISTA:14592
file:
- access_level: open_access
  checksum: 0108616e2a59e51879ea51299a29b091
  content_type: application/zip
  creator: fschur
  date_created: 2023-11-22T14:58:44Z
  date_updated: 2023-11-22T14:58:44Z
  file_id: '14593'
  file_name: 3Dprint-files_download_v2.zip
  file_size: 49297
  relation: main_file
  success: 1
- access_level: open_access
  checksum: 4c66ddedee4d01c1c4a7978208350cfc
  content_type: text/plain
  creator: cchlebak
  date_created: 2023-12-01T10:39:59Z
  date_updated: 2023-12-01T10:39:59Z
  file_id: '14637'
  file_name: readme.txt
  file_size: 641
  relation: main_file
  success: 1
file_date_updated: 2023-12-01T10:39:59Z
has_accepted_license: '1'
license: https://creativecommons.org/licenses/by-nc-sa/4.0/
month: '12'
oa: 1
oa_version: Published Version
project:
- _id: 9B954C5C-BA93-11EA-9121-9846C619BF3A
  grant_number: P33367
  name: Structure and isoform diversity of the Arp2/3 complex
publisher: Institute of Science and Technology Austria
related_material:
  record:
  - id: '8586'
    relation: research_data
    status: public
status: public
title: STL-files for 3D-printed grid holders described in  Fäßler F, Zens B, et al.;
  3D printed cell culture grid holders for improved cellular specimen preparation
  in cryo-electron microscopy
tmp:
  image: /images/cc_by_nc_sa.png
  legal_code_url: https://creativecommons.org/licenses/by-nc-sa/4.0/legalcode
  name: Creative Commons Attribution-NonCommercial-ShareAlike 4.0 International (CC
    BY-NC-SA 4.0)
  short: CC BY-NC-SA (4.0)
type: research_data
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
year: '2020'
...
---
_id: '15286'
article_processing_charge: No
article_type: original
author:
- first_name: Florian
  full_name: Fäßler, Florian
  id: 404F5528-F248-11E8-B48F-1D18A9856A87
  last_name: Fäßler
  orcid: 0000-0001-7149-769X
- first_name: Georgi A
  full_name: Dimchev, Georgi A
  id: 38C393BE-F248-11E8-B48F-1D18A9856A87
  last_name: Dimchev
  orcid: 0000-0001-8370-6161
- first_name: Victor-Valentin
  full_name: Hodirnau, Victor-Valentin
  id: 3661B498-F248-11E8-B48F-1D18A9856A87
  last_name: Hodirnau
  orcid: 0000-0003-3904-947X
- first_name: Bettina
  full_name: Zens, Bettina
  id: 45FD126C-F248-11E8-B48F-1D18A9856A87
  last_name: Zens
  orcid: 0000-0002-9561-1239
- first_name: Christoph
  full_name: Möhl, Christoph
  last_name: Möhl
- first_name: Frank
  full_name: Bradke, Frank
  last_name: Bradke
- first_name: Florian KM
  full_name: Schur, Florian KM
  id: 48AD8942-F248-11E8-B48F-1D18A9856A87
  last_name: Schur
  orcid: 0000-0003-4790-8078
citation:
  ama: Fäßler F, Dimchev GA, Hodirnau V-V, et al. Cryo-electron tomography workflows
    for quantitative analysis of actin networks involved in cell migration. <i>Microscopy
    and Microanalysis</i>. 2020;26(S2):2518-2519. doi:<a href="https://doi.org/10.1017/s1431927620021881">10.1017/s1431927620021881</a>
  apa: Fäßler, F., Dimchev, G. A., Hodirnau, V.-V., Zens, B., Möhl, C., Bradke, F.,
    &#38; Schur, F. K. (2020). Cryo-electron tomography workflows for quantitative
    analysis of actin networks involved in cell migration. <i>Microscopy and Microanalysis</i>.
    Oxford University Press. <a href="https://doi.org/10.1017/s1431927620021881">https://doi.org/10.1017/s1431927620021881</a>
  chicago: Fäßler, Florian, Georgi A Dimchev, Victor-Valentin Hodirnau, Bettina Zens,
    Christoph Möhl, Frank Bradke, and Florian KM Schur. “Cryo-Electron Tomography
    Workflows for Quantitative Analysis of Actin Networks Involved in Cell Migration.”
    <i>Microscopy and Microanalysis</i>. Oxford University Press, 2020. <a href="https://doi.org/10.1017/s1431927620021881">https://doi.org/10.1017/s1431927620021881</a>.
  ieee: F. Fäßler <i>et al.</i>, “Cryo-electron tomography workflows for quantitative
    analysis of actin networks involved in cell migration,” <i>Microscopy and Microanalysis</i>,
    vol. 26, no. S2. Oxford University Press, pp. 2518–2519, 2020.
  ista: Fäßler F, Dimchev GA, Hodirnau V-V, Zens B, Möhl C, Bradke F, Schur FK. 2020.
    Cryo-electron tomography workflows for quantitative analysis of actin networks
    involved in cell migration. Microscopy and Microanalysis. 26(S2), 2518–2519.
  mla: Fäßler, Florian, et al. “Cryo-Electron Tomography Workflows for Quantitative
    Analysis of Actin Networks Involved in Cell Migration.” <i>Microscopy and Microanalysis</i>,
    vol. 26, no. S2, Oxford University Press, 2020, pp. 2518–19, doi:<a href="https://doi.org/10.1017/s1431927620021881">10.1017/s1431927620021881</a>.
  short: F. Fäßler, G.A. Dimchev, V.-V. Hodirnau, B. Zens, C. Möhl, F. Bradke, F.K.
    Schur, Microscopy and Microanalysis 26 (2020) 2518–2519.
corr_author: '1'
date_created: 2024-04-03T09:40:11Z
date_published: 2020-08-01T00:00:00Z
date_updated: 2024-10-09T21:08:43Z
day: '01'
department:
- _id: FlSc
- _id: EM-Fac
doi: 10.1017/s1431927620021881
intvolume: '        26'
issue: S2
keyword:
- Instrumentation
language:
- iso: eng
month: '08'
oa_version: None
page: 2518-2519
publication: Microscopy and Microanalysis
publication_identifier:
  eissn:
  - 1435-8115
  issn:
  - 1431-9276
publication_status: published
publisher: Oxford University Press
quality_controlled: '1'
status: public
title: Cryo-electron tomography workflows for quantitative analysis of actin networks
  involved in cell migration
type: journal_article
user_id: 2DF688A6-F248-11E8-B48F-1D18A9856A87
volume: 26
year: '2020'
...