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在视紫红质激活过程中,螺旋运动与第二个细胞外环的位移相关联。

Helix movement is coupled to displacement of the second extracellular loop in rhodopsin activation.

作者信息

Ahuja Shivani, Hornak Viktor, Yan Elsa C Y, Syrett Natalie, Goncalves Joseph A, Hirshfeld Amiram, Ziliox Martine, Sakmar Thomas P, Sheves Mordechai, Reeves Philip J, Smith Steven O, Eilers Markus

机构信息

Department of Physics and Astronomy, Stony Brook University, Stony Brook, New York 11794-5215, USA.

出版信息

Nat Struct Mol Biol. 2009 Feb;16(2):168-75. doi: 10.1038/nsmb.1549. Epub 2009 Feb 1.

Abstract

The second extracellular loop (EL2) of rhodopsin forms a cap over the binding site of its photoreactive 11-cis retinylidene chromophore. A crucial question has been whether EL2 forms a reversible gate that opens upon activation or acts as a rigid barrier. Distance measurements using solid-state (13)C NMR spectroscopy between the retinal chromophore and the beta4 strand of EL2 show that the loop is displaced from the retinal binding site upon activation, and there is a rearrangement in the hydrogen-bonding networks connecting EL2 with the extracellular ends of transmembrane helices H4, H5 and H6. NMR measurements further reveal that structural changes in EL2 are coupled to the motion of helix H5 and breaking of the ionic lock that regulates activation. These results provide a comprehensive view of how retinal isomerization triggers helix motion and activation in this prototypical G protein-coupled receptor.

摘要

视紫红质的第二个细胞外环(EL2)在其光反应性11-顺式视黄醛发色团的结合位点上形成一个帽状结构。一个关键问题是EL2是否形成一个在激活时打开的可逆门控,或者起到一个刚性屏障的作用。使用固态(13)C核磁共振光谱对视网膜发色团与EL2的β4链之间进行距离测量,结果表明该环在激活时从视网膜结合位点移位,并且在连接EL2与跨膜螺旋H4、H5和H6细胞外末端的氢键网络中存在重排。核磁共振测量进一步揭示,EL2中的结构变化与螺旋H5的运动以及调节激活的离子锁的断裂相关联。这些结果提供了关于视网膜异构化如何在这个典型的G蛋白偶联受体中触发螺旋运动和激活的全面观点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/86ea/2705779/f64104f977c9/nihms103234f1.jpg

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