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两个质子化开关控制视紫红质在膜中的激活。

Two protonation switches control rhodopsin activation in membranes.

作者信息

Mahalingam Mohana, Martínez-Mayorga Karina, Brown Michael F, Vogel Reiner

机构信息

Biophysics Section, Institute of Molecular Medicine and Cell Research, Albert Ludwigs University, Hermann-Herder-Strasse 9, D-79104 Freiburg, Germany.

出版信息

Proc Natl Acad Sci U S A. 2008 Nov 18;105(46):17795-800. doi: 10.1073/pnas.0804541105. Epub 2008 Nov 7.

Abstract

Activation of the G protein-coupled receptor (GPCR) rhodopsin is initiated by light-induced isomerization of the retinal ligand, which triggers 2 protonation switches in the conformational transition to the active receptor state Meta II. The first switch involves disruption of an interhelical salt bridge by internal proton transfer from the retinal protonated Schiff base (PSB) to its counterion, Glu-113, in the transmembrane domain. The second switch consists of uptake of a proton from the solvent by Glu-134 of the conserved E(D)RY motif at the cytoplasmic terminus of helix 3, leading to pH-dependent receptor activation. By using a combination of UV-visible and FTIR spectroscopy, we study the activation mechanism of rhodopsin in different membrane environments and show that these 2 protonation switches become partially uncoupled at physiological temperature. This partial uncoupling leads to approximately 50% population of an entropy-stabilized Meta II state in which the interhelical PSB salt bridge is broken and activating helix movements have taken place but in which Glu-134 remains unprotonated. This partial activation is converted to full activation only by coupling to the pH-dependent protonation of Glu-134 from the solvent, which stabilizes the active receptor conformation by lowering its enthalpy. In a membrane environment, protonation of Glu-134 is therefore a thermodynamic rather than a structural prerequisite for activating helix movements. In light of the conservation of the E(D)RY motif in rhodopsin-like GPCRs, protonation of this carboxylate also may serve a similar function in signal transduction of other members of this receptor family.

摘要

G蛋白偶联受体(GPCR)视紫红质的激活是由视网膜配体的光诱导异构化引发的,这在向活性受体状态Meta II的构象转变中触发了2个质子化开关。第一个开关涉及跨膜结构域中从视网膜质子化席夫碱(PSB)到其反离子Glu-113的内部质子转移,从而破坏螺旋间盐桥。第二个开关包括螺旋3胞质末端保守的E(D)RY基序中的Glu-134从溶剂中摄取一个质子,导致pH依赖性受体激活。通过结合紫外可见光谱和傅里叶变换红外光谱,我们研究了视紫红质在不同膜环境中的激活机制,并表明这两个质子化开关在生理温度下会部分解偶联。这种部分解偶联导致约50%的熵稳定Meta II状态,其中螺旋间PSB盐桥被破坏,激活螺旋运动已经发生,但Glu-134仍未质子化。只有通过与溶剂中Glu-134的pH依赖性质子化偶联,这种部分激活才会转化为完全激活,通过降低其焓来稳定活性受体构象。因此,在膜环境中,Glu-134的质子化是激活螺旋运动的热力学而非结构先决条件。鉴于视紫红质样GPCR中E(D)RY基序的保守性,这种羧酸盐的质子化在该受体家族其他成员的信号转导中也可能发挥类似作用。

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本文引用的文献

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Structure of a beta1-adrenergic G-protein-coupled receptor.β1-肾上腺素能G蛋白偶联受体的结构
Nature. 2008 Jul 24;454(7203):486-91. doi: 10.1038/nature07101. Epub 2008 Jun 25.
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Sequence of late molecular events in the activation of rhodopsin.视紫红质激活过程中晚期分子事件的序列。
Proc Natl Acad Sci U S A. 2007 Dec 18;104(51):20290-5. doi: 10.1073/pnas.0710393104. Epub 2007 Dec 11.
9
Coupling of protonation switches during rhodopsin activation.视紫红质激活过程中质子化开关的偶联。
Photochem Photobiol. 2007 Mar-Apr;83(2):286-92. doi: 10.1562/2006-06-19-IR-937.
10
G protein coupled receptor structure and activation.G蛋白偶联受体的结构与激活
Biochim Biophys Acta. 2007 Apr;1768(4):794-807. doi: 10.1016/j.bbamem.2006.10.021. Epub 2006 Nov 15.

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