Issue 17, 2011
From the journal:

Analyst

Single particle tracking as a method to resolve differences in highly colocalized proteins

Craig J. Szymanski,a   William H. Humphries, IVa  and  Christine K. Payne*a  

* Corresponding authors

a School of Chemistry and Biochemistry and Petit Institute for Bioengineering and Bioscience, Georgia Institute of Technology, 901 Atlantic Drive, Atlanta, Georgia, USA
E-mail: christine.payne@chemistry.gatech.edu
Fax: +1 404-385-6057
Tel: +1 404-385-3125

Abstract

Single particle tracking fluorescence microscopy was used to study two late endosomal proteins, Rab7 and LAMP1, that appear to be highly colocalized in static fluorescence microscopy images. Imaging these proteins simultaneously reveals that Rab7 and LAMP1 undergo periods of separation within the cell. Single particle tracking carried out during these periods of separation shows that Rab7-vesicles have greater velocities, but undergo less efficient transport than LAMP1-vesicles. This research demonstrates the use of single particle tracking as a tool to resolve functional differences in highly colocalized proteins in intact live cells.

Graphical abstract: Single particle tracking as a method to resolve differences in highly colocalized proteins

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Article information

DOI
https://doi.org/10.1039/C0AN00855A
Article type
Paper
Submitted
03 Nov 2010
Accepted
16 Dec 2010
First published
31 Jan 2011

Analyst, 2011,136, 3527-3533

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Single particle tracking as a method to resolve differences in highly colocalized proteins

C. J. Szymanski, W. H. Humphries, IV and C. K. Payne, Analyst, 2011, 136, 3527 DOI: 10.1039/C0AN00855A

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