Functionalized Bead Assay to Measure Three-dimensional Traction Forces during T-cell Activation

Morteza Aramesh; Simon Mergenthal; Marcel Issler; Birgit Plochberger; Florian Weber; Xiao Hua Qin; Robert Liska; Georg N. Duda; Johannes B. Huppa; Jonas Ries; Gerhard J. Schütz; Enrico Klotzsch

doi:10.1021/acs.nanolett.0c03964

Functionalized Bead Assay to Measure Three-dimensional Traction Forces during T-cell Activation

Morteza Aramesh, Simon Mergenthal, Marcel Issler, Birgit Plochberger, Florian Weber, Xiao Hua Qin, Robert Liska, Georg N. Duda, Johannes B. Huppa, Jonas Ries, Gerhard J. Schütz, Enrico Klotzsch

Research Center Linz

Publikation: Beitrag in Fachzeitschrift › Artikel › Begutachtung

33 Zitate (Scopus)

Abstract

When T-cells probe their environment for antigens, the bond between the T-cell receptor (TCR) and the peptide-loaded major histocompatibility complex (MHC) is put under tension, thereby influencing the antigen discrimination. Yet, the quantification of such forces in the context of T-cell signaling is technically challenging. Here, we developed a traction force microscopy platform which allows for quantifying the pulls and pushes exerted via T-cell microvilli, in both tangential and normal directions, during T-cell activation. We immobilized specific T-cell activating antibodies on the marker beads used to read out the hydrogel deformation. Microvilli targeted the functionalized beads, as confirmed by superresolution microscopy of the local actin organization. Moreover, we found that cellular components, such as actin, TCR, and CD45 reorganize upon interaction with the beads, such that actin forms a vortex-like ring structure around the beads and TCR is enriched at the bead surface, whereas CD45 is excluded from bead-microvilli contacts.

Originalsprache	Englisch
Seiten (von - bis)	507-514
Seitenumfang	8
Fachzeitschrift	Nano Letters
Jahrgang	21
Ausgabenummer	1
DOIs	https://doi.org/10.1021/acs.nanolett.0c03964
Publikationsstatus	Veröffentlicht - 13 Jän. 2021

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10.1021/acs.nanolett.0c03964

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title = "Functionalized Bead Assay to Measure Three-dimensional Traction Forces during T-cell Activation",

abstract = "When T-cells probe their environment for antigens, the bond between the T-cell receptor (TCR) and the peptide-loaded major histocompatibility complex (MHC) is put under tension, thereby influencing the antigen discrimination. Yet, the quantification of such forces in the context of T-cell signaling is technically challenging. Here, we developed a traction force microscopy platform which allows for quantifying the pulls and pushes exerted via T-cell microvilli, in both tangential and normal directions, during T-cell activation. We immobilized specific T-cell activating antibodies on the marker beads used to read out the hydrogel deformation. Microvilli targeted the functionalized beads, as confirmed by superresolution microscopy of the local actin organization. Moreover, we found that cellular components, such as actin, TCR, and CD45 reorganize upon interaction with the beads, such that actin forms a vortex-like ring structure around the beads and TCR is enriched at the bead surface, whereas CD45 is excluded from bead-microvilli contacts.",

keywords = "actin dynamics, microvilli, T-cell activation, traction force microscopy",

author = "Morteza Aramesh and Simon Mergenthal and Marcel Issler and Birgit Plochberger and Florian Weber and Qin, {Xiao Hua} and Robert Liska and Duda, {Georg N.} and Huppa, {Johannes B.} and Jonas Ries and Sch{\"u}tz, {Gerhard J.} and Enrico Klotzsch",

note = "Funding Information: We thank Wes Legant and Michael L. Smith for general discussions and helpful advice regarding TFM and Daniel Nieves for advice with surface functionalization. We thank M.Z. Lin for kindly providing the cyOFP tractin plasmid. E.K. is thankful for the financial support from the Human Frontiers Science Program (RGY0065/2017), a FEBS long-term fellowship throughout the onset of the project, and an ARC DECRA fellowship (DE160100282). M.A. is thankful for funding from SNF Spark. G.J.S. and J.B.H. acknowledge funding from the Vienna Science and Technology Fund (WWTF; project LS13-030). Publisher Copyright: {\textcopyright} Copyright: Copyright 2021 Elsevier B.V., All rights reserved.",

year = "2021",

month = jan,

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doi = "10.1021/acs.nanolett.0c03964",

language = "English",

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AU - Aramesh, Morteza

AU - Mergenthal, Simon

AU - Issler, Marcel

AU - Plochberger, Birgit

AU - Weber, Florian

AU - Qin, Xiao Hua

AU - Liska, Robert

AU - Duda, Georg N.

AU - Huppa, Johannes B.

AU - Ries, Jonas

AU - Schütz, Gerhard J.

AU - Klotzsch, Enrico

N1 - Funding Information: We thank Wes Legant and Michael L. Smith for general discussions and helpful advice regarding TFM and Daniel Nieves for advice with surface functionalization. We thank M.Z. Lin for kindly providing the cyOFP tractin plasmid. E.K. is thankful for the financial support from the Human Frontiers Science Program (RGY0065/2017), a FEBS long-term fellowship throughout the onset of the project, and an ARC DECRA fellowship (DE160100282). M.A. is thankful for funding from SNF Spark. G.J.S. and J.B.H. acknowledge funding from the Vienna Science and Technology Fund (WWTF; project LS13-030). Publisher Copyright: © Copyright: Copyright 2021 Elsevier B.V., All rights reserved.

PY - 2021/1/13

Y1 - 2021/1/13

N2 - When T-cells probe their environment for antigens, the bond between the T-cell receptor (TCR) and the peptide-loaded major histocompatibility complex (MHC) is put under tension, thereby influencing the antigen discrimination. Yet, the quantification of such forces in the context of T-cell signaling is technically challenging. Here, we developed a traction force microscopy platform which allows for quantifying the pulls and pushes exerted via T-cell microvilli, in both tangential and normal directions, during T-cell activation. We immobilized specific T-cell activating antibodies on the marker beads used to read out the hydrogel deformation. Microvilli targeted the functionalized beads, as confirmed by superresolution microscopy of the local actin organization. Moreover, we found that cellular components, such as actin, TCR, and CD45 reorganize upon interaction with the beads, such that actin forms a vortex-like ring structure around the beads and TCR is enriched at the bead surface, whereas CD45 is excluded from bead-microvilli contacts.

AB - When T-cells probe their environment for antigens, the bond between the T-cell receptor (TCR) and the peptide-loaded major histocompatibility complex (MHC) is put under tension, thereby influencing the antigen discrimination. Yet, the quantification of such forces in the context of T-cell signaling is technically challenging. Here, we developed a traction force microscopy platform which allows for quantifying the pulls and pushes exerted via T-cell microvilli, in both tangential and normal directions, during T-cell activation. We immobilized specific T-cell activating antibodies on the marker beads used to read out the hydrogel deformation. Microvilli targeted the functionalized beads, as confirmed by superresolution microscopy of the local actin organization. Moreover, we found that cellular components, such as actin, TCR, and CD45 reorganize upon interaction with the beads, such that actin forms a vortex-like ring structure around the beads and TCR is enriched at the bead surface, whereas CD45 is excluded from bead-microvilli contacts.

KW - actin dynamics

KW - microvilli

KW - T-cell activation

KW - traction force microscopy

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SP - 507

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JF - Nano Letters

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ER -

Functionalized Bead Assay to Measure Three-dimensional Traction Forces during T-cell Activation

Abstract

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