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钙-myristoyl 牵拉是一种新的分子内调节钙敏感性和靶酶相互作用的机制,用于鸟苷酸环化酶激活蛋白 1:N-脂肪酸酰基和 EF 手之间的动态连接控制钙敏感性。

Calcium-myristoyl Tug is a new mechanism for intramolecular tuning of calcium sensitivity and target enzyme interaction for guanylyl cyclase-activating protein 1: dynamic connection between N-fatty acyl group and EF-hand controls calcium sensitivity.

机构信息

Department of Basic Sciences and Pennsylvania College of Optometry, Salus University, Elkins Park, Pennsylvania 19027, USA.

出版信息

J Biol Chem. 2012 Apr 20;287(17):13972-84. doi: 10.1074/jbc.M112.341883. Epub 2012 Mar 1.

Abstract

Guanylyl cyclase-activating protein 1 (GCAP1), a myristoylated Ca(2+) sensor in vision, regulates retinal guanylyl cyclase (RetGC). We show that protein-myristoyl group interactions control Ca(2+) sensitivity, apparent affinity for RetGC, and maximal level of cyclase activation. Mutating residues near the myristoyl moiety affected the affinity of Ca(2+) binding to EF-hand 4. Inserting Phe residues in the cavity around the myristoyl group increased both the affinity of GCAP1 for RetGC and maximal activation of the cyclase. NMR spectra show that the myristoyl group in the L80F/L176F/V180F mutant remained sequestered inside GCAP1 in both Ca(2+)-bound and Mg(2+)-bound states. This mutant displayed much higher affinity for the cyclase but reduced Ca(2+) sensitivity of the cyclase regulation. The L176F substitution improved affinity of myristoylated and non-acylated GCAP1 for the cyclase but simultaneously reduced the affinity of Ca(2+) binding to EF-hand 4 and Ca(2+) sensitivity of the cyclase regulation by acylated GCAP1. The replacement of amino acids near both ends of the myristoyl moiety (Leu(80) and Val(180)) minimally affected regulatory properties of GCAP1. N-Lauryl- and N-myristoyl-GCAP1 activated RetGC in a similar fashion. Thus, protein interactions with the central region of the fatty acyl chain optimize GCAP1 binding to RetGC and maximize activation of the cyclase. We propose a dynamic connection (or "tug") between the fatty acyl group and EF-hand 4 via the C-terminal helix that attenuates the efficiency of RetGC activation in exchange for optimal Ca(2+) sensitivity.

摘要

鸟苷酸环化酶激活蛋白 1(GCAP1)是一种在视觉中起作用的豆蔻酰化 Ca2+传感器,可调节视网膜鸟苷酸环化酶(RetGC)。我们表明,蛋白-豆蔻酰基相互作用控制 Ca2+敏感性、对 RetGC 的表观亲和力和环化酶激活的最大水平。突变豆蔻酰部分附近的残基会影响 EF 手型 4 对 Ca2+结合的亲和力。在豆蔻酰基团周围的腔中插入苯丙氨酸残基,会增加 GCAP1 与 RetGC 的亲和力和对环化酶的最大激活。NMR 谱表明,在 L80F/L176F/V180F 突变体中,豆蔻酰基团在 Ca2+结合和 Mg2+结合状态下仍被 GCAP1 隔离在内部。该突变体对环化酶显示出更高的亲和力,但降低了环化酶调节的 Ca2+敏感性。L176F 取代提高了豆蔻酰化和非酰化 GCAP1 对环化酶的亲和力,但同时降低了 Ca2+与 EF 手型 4 的结合亲和力和酰化 GCAP1 对环化酶调节的 Ca2+敏感性。豆蔻酰部分两端氨基酸的取代(Leu80 和 Val180)对 GCAP1 的调节性质影响最小。N-月桂酰基和 N-豆蔻酰基-GCAP1 以相似的方式激活 RetGC。因此,蛋白质与脂肪酸链中心区域的相互作用优化了 GCAP1 与 RetGC 的结合,并使环化酶的最大激活。我们提出了一种通过 C 端螺旋在脂肪酸基团和 EF 手型 4 之间的动态连接(或“拉”),通过降低 RetGC 激活效率来换取最佳的 Ca2+敏感性。

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