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膜蛋白的表面等离子体共振光谱研究:在薄膜中监测视紫红质对视神经转导蛋白的结合与激活。

Surface plasmon resonance spectroscopy studies of membrane proteins: transducin binding and activation by rhodopsin monitored in thin membrane films.

作者信息

Salamon Z, Wang Y, Soulages J L, Brown M F, Tollin G

机构信息

Department of Biochemistry, University of Arizona, Tucson 85721, USA.

出版信息

Biophys J. 1996 Jul;71(1):283-94. doi: 10.1016/S0006-3495(96)79224-X.

Abstract

Surface plasmon resonance (SPR) spectroscopy can provide useful information regarding average structural properties of membrane films supported on planar solid substrates. Here we have used SPR spectroscopy for the first time to monitor the binding and activation of G-protein (transducin or Gt) by bovine rhodopsin incorporated into an egg phosphatidylcholine bilayer deposited on a silver film. Rhodopsin incorporation into the membrane, performed by dilution of a detergent solution of the protein, proceeds in a saturable manner. Before photolysis, the SPR data show that Gt binds tightly (Keq approximately equal to 60 nM) and with positive cooperativity to rhodopsin in the lipid layer to form a closely packed film. A simple multilayer model yields a calculated average thickness of about 57 A, in good agreement with the structure of Gt. The data also demonstrate that Gt binding saturates at a Gt/rhodopsin ratio of approximately 0.6. Moreover, upon visible light irradiation, characteristic changes occur in the SPR spectrum, which can be modeled by a 6 A increase in the average thickness of the lipid/protein film caused by formation of metarhodopsin II (MII). Upon subsequent addition of GTP, further SPR spectral changes are induced. These are interpreted as resulting from dissociation of the alpha-subunit of Gt, formation of new MII-Gt complexes, and possible conformational changes of Gt as a consequence of complex formation. The above results clearly demonstrate the ability of SPR spectroscopy to monitor interactions among the proteins associated with signal transduction in membrane-bound systems.

摘要

表面等离子体共振(SPR)光谱能够提供有关支撑在平面固体基质上的膜的平均结构性质的有用信息。在这里,我们首次使用SPR光谱来监测结合在沉积于银膜上的卵磷脂双层中的牛视紫红质对G蛋白(转导素或Gt)的结合和激活。通过稀释蛋白质的去污剂溶液将视紫红质掺入膜中,此过程以饱和方式进行。在光解之前,SPR数据表明Gt紧密结合(平衡常数约等于60 nM),并且以正协同性与脂质层中的视紫红质结合,形成紧密堆积的膜。一个简单的多层模型计算得出的平均厚度约为57埃,与Gt的结构非常吻合。数据还表明,Gt结合在Gt/视紫红质比约为0.6时达到饱和。此外,在可见光照射下,SPR光谱会发生特征性变化,这可以通过视紫红质II(MII)的形成导致脂质/蛋白质膜平均厚度增加6埃来模拟。随后加入GTP时,会诱导进一步的SPR光谱变化。这些变化被解释为是由于Gt的α亚基解离、新的MII-Gt复合物形成以及复合物形成导致的Gt可能的构象变化所致。上述结果清楚地证明了SPR光谱监测膜结合系统中与信号转导相关蛋白质之间相互作用的能力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ca24/1233479/6c961267ec4e/biophysj00045-0285-a.jpg

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