Literature DB >> 23266704

Resolving multi-molecular protein interactions by photoactivated localization microscopy.

Eilon Sherman1, Valarie A Barr, Lawrence E Samelson.   

Abstract

Multi-molecular protein complexes are critical to many cellular functions, including signaling, DNA transcription and enzymatic reactions. In spite of their importance, current research techniques such as biochemistry and diffraction-limited microscopy cannot resolve the heterogeneity and nanoscale organization of protein complexes in intact cells. Here we describe a technique that enables the study of multi-molecular protein complexes at the single molecule level in intact cells. The technique uses photoactivated localization microscopy (PALM) to resolve individual proteins with a resolution down to 20nm in intact cells, and second-order statistics to study the spatial interactions of the proteins. We demonstrate the feasibility of this technique by studying signaling complexes that form in activated T cells. We first use single color PALM imaging and univariate second-order statistics to resolve the clustering of Linker for Activation of T cells (LAT) at the plasma membrane (PM) of the cells. We then use two color PALM and bivariate second-order statistics to resolve the interaction of LAT with key interacting proteins. We discuss potential caveats in studying molecular clustering and the robustness of the technique to study bimolecular interactions. Our proposed technique, combined with older techniques, could help shed new light on the nature of multimolecular protein complexes and their significance to cell function. Published by Elsevier Inc.

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Year:  2012        PMID: 23266704      PMCID: PMC3608816          DOI: 10.1016/j.ymeth.2012.12.002

Source DB:  PubMed          Journal:  Methods        ISSN: 1046-2023            Impact factor:   3.608


  30 in total

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  10 in total

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2.  Development of nanoscale structure in LAT-based signaling complexes.

Authors:  Valarie A Barr; Eilon Sherman; Jason Yi; Itoro Akpan; Alexandre K Rouquette-Jazdanian; Lawrence E Samelson
Journal:  J Cell Sci       Date:  2016-11-10       Impact factor: 5.285

Review 3.  Progress in quantitative single-molecule localization microscopy.

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Journal:  Histochem Cell Biol       Date:  2014-04-20       Impact factor: 4.304

4.  Hierarchical nanostructure and synergy of multimolecular signalling complexes.

Authors:  Eilon Sherman; Valarie A Barr; Robert K Merrill; Carole K Regan; Connie L Sommers; Lawrence E Samelson
Journal:  Nat Commun       Date:  2016-07-11       Impact factor: 14.919

5.  madSTORM: a superresolution technique for large-scale multiplexing at single-molecule accuracy.

Authors:  Jason Yi; Asit Manna; Valarie A Barr; Jennifer Hong; Keir C Neuman; Lawrence E Samelson
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6.  Nanoscale kinetic segregation of TCR and CD45 in engaged microvilli facilitates early T cell activation.

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Journal:  Nat Commun       Date:  2018-02-21       Impact factor: 14.919

7.  Gp41 dynamically interacts with the TCR in the immune synapse and promotes early T cell activation.

Authors:  Oren Yakovian; Roland Schwarzer; Julia Sajman; Yair Neve-Oz; Yair Razvag; Andreas Herrmann; Eilon Sherman
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8.  Adhering interacting cells to two opposing coverslips allows super-resolution imaging of cell-cell interfaces.

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9.  The L-type Voltage-Gated Calcium Channel co-localizes with Syntaxin 1A in nano-clusters at the plasma membrane.

Authors:  Julia Sajman; Michael Trus; Daphne Atlas; Eilon Sherman
Journal:  Sci Rep       Date:  2017-09-12       Impact factor: 4.379

10.  InterCells: A Generic Monte-Carlo Simulation of Intercellular Interfaces Captures Nanoscale Patterning at the Immune Synapse.

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  10 in total

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