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构建用于结构研究的G蛋白偶联受体:稳定BLT1受体的基态。

Engineering a G protein-coupled receptor for structural studies: stabilization of the BLT1 receptor ground state.

作者信息

Martin Aimée, Damian Marjorie, Laguerre Michel, Parello Joseph, Pucci Bernard, Serre Laurence, Mary Sophie, Marie Jacky, Banères Jean-Louis

机构信息

Institut des Biomolécules Max Mousseron, UMR 5247 CNRS Universités Montpellier I et II, Faculté de Pharmacie, 15 Av. Ch. Flahault, BP14491, 34093 Montpellier Cedex 5, France.

出版信息

Protein Sci. 2009 Apr;18(4):727-34. doi: 10.1002/pro.55.

Abstract

Structural characterization of membrane proteins is hampered by their instability in detergent solutions. We modified here a G protein-coupled receptor, the BLT1 receptor of leukotriene B(4), to stabilize it in vitro. For this, we introduced a metal-binding site connecting the third and sixth transmembrane domains of the receptor. This modification was intended to restrain the activation-associated relative movement of these helices that results in a less stable packing in the isolated receptor. The modified receptor binds its agonist with low-affinity and can no longer trigger G protein activation, indicating that it is stabilized in its ground state conformation. Of importance, the modified BLT1 receptor displays an increased temperature-, detergent-, and time-dependent stability compared with the wild-type receptor. These data indicate that stabilizing the ground state of this GPCR by limiting the activation-associated movements of the transmembrane helices is a way to increase its stability in detergent solutions; this could represent a forward step on the way of its crystallization.

摘要

膜蛋白的结构表征因其在去污剂溶液中的不稳定性而受到阻碍。我们在此对一种G蛋白偶联受体——白三烯B4的BLT1受体进行了修饰,以使其在体外稳定。为此,我们在受体的第三和第六个跨膜结构域之间引入了一个金属结合位点。这种修饰旨在抑制这些螺旋在激活相关的相对运动,而这种运动导致分离的受体中堆积稳定性降低。修饰后的受体以低亲和力结合其激动剂,并且不再能触发G蛋白激活,这表明它在基态构象中是稳定的。重要的是,与野生型受体相比,修饰后的BLT1受体在温度、去污剂和时间依赖性方面表现出更高的稳定性。这些数据表明,通过限制跨膜螺旋的激活相关运动来稳定该GPCR的基态是提高其在去污剂溶液中稳定性的一种方法;这可能是其结晶道路上向前迈出的一步。

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