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利用来自α亚基的合成肽绘制G蛋白与视紫红质结合的位点。

Site of G protein binding to rhodopsin mapped with synthetic peptides from the alpha subunit.

作者信息

Hamm H E, Deretic D, Arendt A, Hargrave P A, Koenig B, Hofmann K P

机构信息

Department of Physiology and Biophysics, University of Illinois College of Medicine, Chicago 60680.

出版信息

Science. 1988 Aug 12;241(4867):832-5. doi: 10.1126/science.3136547.

Abstract

The interaction between receptors and guanine nucleotide binding (G) proteins leads to G protein activation and subsequent regulation of effector enzymes. The molecular basis of receptor-G protein interaction has been examined by using the ability of the G protein from rods (transducin) to cause a conformational change in rhodopsin as an assay. Synthetic peptides corresponding to two regions near the carboxyl terminus of the G protein alpha subunit, Glu311-Val328 and Ile340-Phe350, compete with G protein for interaction with rhodopsin. Amino acid substitution studies show that Cys321 is required for this effect. Ile340-Phe350 and a modified peptide, acetyl-Glu311-Lys329-amide, mimic G protein effects on rhodopsin conformation, showing that these peptides bind to and stabilize the activated conformation of rhodopsin.

摘要

受体与鸟嘌呤核苷酸结合(G)蛋白之间的相互作用导致G蛋白激活,进而调节效应酶。通过利用视杆细胞的G蛋白(转导素)使视紫红质发生构象变化的能力作为一种检测方法,研究了受体 - G蛋白相互作用的分子基础。与G蛋白α亚基羧基末端附近的两个区域相对应的合成肽,即Glu311 - Val328和Ile340 - Phe350,与G蛋白竞争与视紫红质的相互作用。氨基酸取代研究表明,Cys321是产生这种效应所必需的。Ile340 - Phe350和一种修饰肽,乙酰 - Glu311 - Lys329 - 酰胺,模拟了G蛋白对视紫红质构象的影响,表明这些肽结合并稳定了视紫红质的激活构象。

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