Dynamic behavior of GFP–CLIP-170 reveals fast protein turnover on microtubule plus ends

Author:

Dragestein Katharina A.1,van Cappellen Wiggert A.2,van Haren Jeffrey1,Tsibidis George D.3,Akhmanova Anna1,Knoch Tobias A.1,Grosveld Frank1,Galjart Niels1

Affiliation:

1. Department of Cell Biology and Genetics

2. Department of Reproduction and Development, Erasmus Medical Center, 3000 DR Rotterdam, Netherlands

3. Institute of Electronic Structure and Laser, Foundation for Research and Technology - Hellas, 71110 Heraklion, Crete, Greece

Abstract

Microtubule (MT) plus end–tracking proteins (+TIPs) specifically recognize the ends of growing MTs. +TIPs are involved in diverse cellular processes such as cell division, cell migration, and cell polarity. Although +TIP tracking is important for these processes, the mechanisms underlying plus end specificity of mammalian +TIPs are not completely understood. Cytoplasmic linker protein 170 (CLIP-170), the prototype +TIP, was proposed to bind to MT ends with high affinity, possibly by copolymerization with tubulin, and to dissociate seconds later. However, using fluorescence-based approaches, we show that two +TIPs, CLIP-170 and end-binding protein 3 (EB3), turn over rapidly on MT ends. Diffusion of CLIP-170 and EB3 appears to be rate limiting for their binding to MT plus ends. We also report that the ends of growing MTs contain a surplus of sites to which CLIP-170 binds with relatively low affinity. We propose that the observed loss of fluorescent +TIPs at plus ends does not reflect the behavior of single molecules but is a result of overall structural changes of the MT end.

Publisher

Rockefeller University Press

Subject

Cell Biology

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