RBD11, a bioengineered Rab11-binding module for visualizing and analyzing endogenous Rab11

Author:

Osaki Futaba1,Matsui Takahide1,Hiragi Shu1,Homma Yuta1ORCID,Fukuda Mitsunori1ORCID

Affiliation:

1. Laboratory of Membrane Trafficking Mechanisms, Department of Integrative Life Sciences, Graduate School of Life Sciences, Tohoku University, Aobayama, Aoba-ku, Sendai, Miyagi 980-8578, Japan

Abstract

ABSTRACT The small GTPase Rab11 (herein referring to the Rab11A and Rab11B isoforms) plays pivotal roles in diverse physiological phenomena, including the recycling of membrane proteins, cytokinesis, neurite outgrowth and epithelial morphogenesis. One effective method of analyzing the function of endogenous Rab11 is to overexpress a Rab11-binding domain from one of its effectors, for example, the C-terminal domain of Rab11-FIP2 (Rab11-FIP2-C), as a dominant-negative construct. However, the drawback of this method is the broader Rab-binding specificity of the effector domain, because Rab11-FIP2-C binds to Rabs other than Rab11, for example, to Rab14 and Rab25. In this study, we bioengineered an artificial Rab11-specific binding domain, named RBD11. Expression of RBD11 allowed visualization of endogenous Rab11 without affecting its localization or function, whereas expression of a tandem RBD11, named 2×RBD11, inhibited epithelial morphogenesis and induced a multi-lumen phenotype characteristic of Rab11-deficient cysts. We also developed two tools for temporally and reversibly analyzing Rab11-dependent membrane trafficking – tetracycline-inducible 2×RBD11 and an artificially oligomerized domain (FM)-tagged RBD11.

Funder

Ministry of Education, Culture, Sports, Science and Technology

Kao Foundation for Arts and Sciences

Japan Science and Technology Agency

Publisher

The Company of Biologists

Subject

Cell Biology

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