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用天然形式和突变形式的鸟苷酸环化酶激活蛋白1对光感受器鸟苷酸环化酶进行功能重建。

Functional reconstitution of photoreceptor guanylate cyclase with native and mutant forms of guanylate cyclase-activating protein 1.

作者信息

Otto-Bruc A, Buczylko J, Surgucheva I, Subbaraya I, Rudnicka-Nawrot M, Crabb J W, Arendt A, Hargrave P A, Baehr W, Palczewski K

机构信息

Department of Ophthalmology, School of Medicine, University of Washington, Seattle 98195, USA.

出版信息

Biochemistry. 1997 Apr 8;36(14):4295-302. doi: 10.1021/bi963000d.

DOI:10.1021/bi963000d
PMID:9100025
Abstract

In rod and cone photoreceptor cells, activation of particulate guanylate cyclase (retGC1) is mediated by a Ca2+-binding protein termed GCAP1, that detects changes in [Ca2+]free. In this study, we show that N-acylated GCAP1 restored Ca2+ sensitivity of native and recombinant photoreceptor retGC1. ATP increased the affinity of retGC1 for GCAP1 and accelerated catalysis. Using peptides derived from the GCAP1 sequence, we found that at least three regions, encompassing the N-terminus, the EF-1 motif, and the EF-3 motif, were likely involved in the interaction with retGC1. Mutation of 2Gly to Ala (GCAP1-G2A), which abolished myristoylation and a 25 amino acid truncation at the N-terminus (delta25-GCAP1) reduced retGC1-stimulating activity dramatically, while deletion of 10 amino acids (delta10-GCAP1) reduced the specific activity by only approximately 60% and modified the Ca2+ sensitivity. At 10(-6) M [Ca2+]free, in conditions that inactivated native GCAP1, retGC1 showed significant activity in the presence of delta10-GCAP1. Native and all three mutant forms of GCAP1 had similar affinities for Ca2+ as demonstrated by gel filtration and the changes in tryptophan fluorescence. All mutants bound to ROS membranes in a Ca2+-independent manner, except delta25-GCAP1, which was mostly soluble. These findings suggest that the N-terminal region is important in tethering of GCAP1 to the ROS membranes.

摘要

在视杆和视锥光感受器细胞中,颗粒型鸟苷酸环化酶(retGC1)的激活由一种名为GCAP1的Ca2+结合蛋白介导,该蛋白可检测游离[Ca2+]的变化。在本研究中,我们表明N-酰化的GCAP1恢复了天然和重组光感受器retGC1的Ca2+敏感性。ATP增加了retGC1对GCAP1的亲和力并加速了催化作用。使用源自GCAP1序列的肽段,我们发现至少三个区域,包括N端、EF-1基序和EF-3基序,可能参与与retGC1的相互作用。将2Gly突变为Ala(GCAP1-G2A)消除了肉豆蔻酰化,N端25个氨基酸的截短(delta25-GCAP1)显著降低了retGC1刺激活性,而缺失10个氨基酸(delta10-GCAP1)仅使比活性降低约60%并改变了Ca2+敏感性。在游离[Ca2+]为10(-6) M的条件下,即天然GCAP1失活的条件下,retGC1在存在delta10-GCAP1时显示出显著活性。通过凝胶过滤和色氨酸荧光变化证明,天然和所有三种突变形式的GCAP1对Ca2+具有相似的亲和力。除了大多可溶的delta25-GCAP1外,所有突变体均以Ca2+非依赖性方式与ROS膜结合。这些发现表明N端区域在将GCAP1 tether到ROS膜上很重要。 (注:tether这个词在文中可能是“ tether to”表示“附着到、系到”之类的意思,但单独这个词在生物学领域不太好直接准确翻译,可能需要结合上下文更准确理解其含义,这里保留英文以供参考)

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