Membrane protein reconstitution in nanodiscs for luminescence spectroscopy studies

被引:7
|
作者
Zoghbi, Maria E. [1 ]
Altenberg, Guillermo A. [1 ]
机构
[1] Univ Calif, Sch Nat Sci, Merced,4225 N Hosp Rd, Atwater, CA 95301 USA
关键词
ATP-binding cassette; LRET; luminescence resonance energy transfer; MsbA; multidrug resistance; ABC TRANSPORTER MSBA; PHOSPHOLIPID-BILAYER NANODISCS; NUCLEOTIDE-BINDING DOMAIN; NANO-POSITIONING SYSTEM; ESCHERICHIA-COLI MSBA; ELECTRON-ELECTRON RESONANCE; MALEIC ACID COPOLYMER; BLOOD-BRAIN-BARRIER; ATP-BINDING; P-GLYCOPROTEIN;
D O I
10.1515/ntrev-2016-0078
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
ATP-binding cassette (ABC) exporters transport substrates across biological membranes using ATP hydrolysis by a process that involves switching between inward-and outward-facing conformations. Most of the structural studies of ABC proteins have been performed with proteins in detergent micelles, locked in specific conformations and/or at low temperature. In this article, we present recent data from our laboratories where we studied the prototypical ABC exporter MsbA during ATP hydrolysis, at 37 degrees C, reconstituted in a lipid bilayer. These studies were possible through the use of luminescence resonance energy transfer spectroscopy in MsbA reconstituted in nanodiscs. We found major differences between MsbA in these native-like conditions and in previous studies. These include a separation between the nucleotide-binding domains that was much smaller than previously thought, and a large fraction of molecules with associated nucleotide-binding domains in the nucleotide-free apo state. These studies stress the importance of studying membrane proteins in an environment that approaches physiological conditions.
引用
收藏
页码:33 / 46
页数:14
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