Literature DB >> 25268018

Quantitative measurement of intracellular protein dynamics using photobleaching or photoactivation of fluorescent proteins.

Tomoki Matsuda1, Takeharu Nagai2.   

Abstract

Unlike in vitro protein dynamics, intracellular protein dynamics are intricately regulated by protein-protein interactions or interactions between proteins and other cellular components, including nucleic acids, the plasma membrane and the cytoskeleton. Alteration of these dynamics plays a crucial role in physiological phenomena such as gene expression and cell division. Live-cell imaging via microscopy with the inherent properties of fluorescent proteins, i.e. photobleaching and photoconversion, or fluorescence correlation spectroscopy, provides insight into the movement of proteins and their interactions with cellular components. This article reviews techniques based on photo-induced changes in the physicochemical properties of fluorescent proteins to measure protein dynamics inside living cells, and it also discusses the strengths and weaknesses of these techniques.
© The Author 2014. Published by Oxford University Press on behalf of The Japanese Society of Microscopy. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.

Keywords:  FDAP; FRAP; diffusion coefficient; fluorescent protein; photoactivation; photobleaching

Mesh:

Substances:

Year:  2014        PMID: 25268018     DOI: 10.1093/jmicro/dfu033

Source DB:  PubMed          Journal:  Microscopy (Oxf)        ISSN: 2050-5698            Impact factor:   1.571


  7 in total

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5.  Dynamic microtubule association of Doublecortin X (DCX) is regulated by its C-terminus.

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6.  Genetically encoded fluorescent tags.

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7.  Determination of diffusion coefficients in live cells using fluorescence recovery after photobleaching with wide-field fluorescence microscopy.

Authors:  Akira Kitamura; Masataka Kinjo
Journal:  Biophys Physicobiol       Date:  2018-01-19
  7 in total

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