Literature DB >> 22989304

Expression, purification, and reconstitution of the voltage-sensing domain from Ci-VSP.

Qufei Li1, Vishwanath Jogini, Sherry Wanderling, D Marien Cortes, Eduardo Perozo.   

Abstract

The voltage-sensing domain (VSD) is the common scaffold responsible for the functional behavior of voltage-gated ion channels, voltage sensitive enzymes, and proton channels. Because of the position of the voltage dependence of the available VSD structures, at present, they all represent the activated state of the sensor. Yet in the absence of a consensus resting state structure, the mechanistic details of voltage sensing remain controversial. The voltage dependence of the VSD from Ci-VSP (Ci-VSD) is dramatically right shifted, so that at 0 mV it presumably populates the putative resting state. Appropriate biochemical methods are an essential prerequisite for generating sufficient amounts of Ci-VSD protein for high-resolution structural studies. Here, we present a simple and robust protocol for the expression of eukaryotic Ci-VSD in Escherichia coli at milligram levels. The protein is pure, homogeneous, monodisperse, and well-folded after solubilization in Anzergent 3-14 at the analyzed concentration (~0.3 mg/mL). Ci-VSD can be reconstituted into liposomes of various compositions, and initial site-directed spin labeling and electron paramagnetic resonance (EPR) spectroscopic measurements indicate its first transmembrane segment folds into an α-helix, in agreement with the homologous region of other VSDs. On the basis of our results and enhanced relaxation EPR spectroscopy measurement, Ci-VSD reconstitutes essentially randomly in proteoliposomes, precluding straightforward application of transmembrane voltages in combination with spectroscopic methods. Nevertheless, these results represent an initial step that makes the resting state of a VSD accessible to a variety of biophysical and structural approaches, including X-ray crystallography, spectroscopic methods, and electrophysiology in lipid bilayers.

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Year:  2012        PMID: 22989304      PMCID: PMC3845960          DOI: 10.1021/bi300980q

Source DB:  PubMed          Journal:  Biochemistry        ISSN: 0006-2960            Impact factor:   3.162


  38 in total

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3.  Three-dimensional architecture and gating mechanism of a K+ channel studied by EPR spectroscopy.

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5.  Structural dynamics of the Streptomyces lividans K+ channel (SKC1): oligomeric stoichiometry and stability.

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7.  Sequence of a probable potassium channel component encoded at Shaker locus of Drosophila.

Authors:  B L Tempel; D M Papazian; T L Schwarz; Y N Jan; L Y Jan
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8.  Direct physical measure of conformational rearrangement underlying potassium channel gating.

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Review 9.  Hydrophobic mismatch between proteins and lipids in membranes.

Authors:  J A Killian
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10.  A spin label method for measuring internal volumes in liposomes or cells, applied to Ca-dependent fusion of negatively charged vesicles.

Authors:  A I Vistnes; J S Puskin
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  7 in total

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