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Direct measurement of VDAC-actin interaction by surface plasmon resonance.

作者信息

Roman Inge, Figys Jurgen, Steurs Griet, Zizi Martin

机构信息

Molecular Membrane Biophysics and Neurophysiology, Dept. of Physiology, Faculty of Medicine and Pharmacy, Vrije Universiteit Brussel, 103 Laarbeeklaan, 1090 Brussels, Belgium.

出版信息

Biochim Biophys Acta. 2006 Apr;1758(4):479-86. doi: 10.1016/j.bbamem.2006.03.019. Epub 2006 Apr 7.

Abstract

VDAC--a mitochondrial channel involved in the control of aerobic metabolism and apoptosis--interacts in vitro and in vivo with a wide repertoire of proteins including cytoskeletal elements. A functional interaction between actin and Neurospora crassa VDAC was reported, excluding other VDAC isoforms. From a recent genome-wide screen of the VDAC interactome, we found that human actin is a putative ligand of yeast VDAC. Since such interaction may have broader implications for various mitochondrial processes, we probed it with Surface Plasmon Resonance (SPR) technology using purified yeast VDAC (YVDAC) and rabbit muscle G-actin (RGA). We show that RGA binds to immobilized YVDAC in a reversible and dose-dependent manner with saturating kinetics and an apparent K(D) of 50 microg/ml (1.2 microM actin). BSA does not bind VDAC regardless of the concentrations. Alternatively, VDAC binds similarly to immobilized RGA but without saturating kinetics. VDAC being known to interact with itself, this latter interaction was directly measured to interpret the RGA signals. VDAC could bind to VDAC without saturating kinetics as expected if higher order binding occurred, and could account for maximally 66% of the non-saturating behavior of VDAC binding onto RGA. Hence, actin-VDAC interactions are not a species-specific oddity and may be a more general phenomenon, the role of which ought to be further investigated.

摘要

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