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首页> 外文期刊>Biochemistry >The myristoylated amino terminus of G alpha(i1) plays a critical role in the structure and function of G alpha(i1) subunits in solution
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The myristoylated amino terminus of G alpha(i1) plays a critical role in the structure and function of G alpha(i1) subunits in solution

机译:G alpha(i1)的豆蔻酰化氨基末端在溶液中G alpha(i1)亚基的结构和功能中起关键作用

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摘要

To determine the role of the myristoylated amino terminus of Galpha in G protein activation, nine individual cysteine mutations along the myristoylated amino terminus of Galpha(i) were expressed in a functionally Cys-less background. Thiol reactive EPR and fluorescent probes were attached to each site as local reporters of mobility and conformational changes upon activation of Galpha(i)GDP by AlF4-, as well as binding to Gbetagamma. EPR and steady state fluorescence anisotropy are consistent with a high degree of immobility for labeled residues in solution all along the amino terminus of myristoylated Galpha(i). This is in contrast to the high mobility of this region in nonmyristoylated Galpha(i) [Medkova, M., et at. (2002) Biochemistry 41, 9962-9972]. Steady state fluorescence measurements revealed pronounced increases in fluorescence upon activation for residues 14-17 and 21 located midway through the 30-amino acid stretch comprising the amino-terminal region. Collectively, the data suggest that myristoylation is an important structural determinant of the amino terminus of Galpha(i) proteins. [References: 53]
机译:为了确定Galpha的豆蔻酰化氨基末端在G蛋白激活中的作用,沿功能性无Cys的背景表达了沿Galpha(i)的豆蔻酰化氨基末端的9个单独的半胱氨酸突变。硫醇反应性EPR和荧光探针作为Alf4-激活Galpha(i)GDP以及结合Gbetagamma时迁移率和构象变化的局部报告子,附着在每个位点上。 EPR和稳态荧光各向异性与豆蔻酰化Galpha(i)氨基末端的溶液中标记残基的高度固定性保持一致。这与该区域在非肉豆蔻酰化的Galpha(i)中的高迁移率形成对比[Medkova,M。,等人。 (2002)Biochemistry 41,9962-9972]。稳态荧光测量显示,激活位于包含氨基末端区域的30个氨基酸序列中间的14-17和21残基时,荧光显着增加。总体而言,数据表明肉豆蔻酰化是Galpha(i)蛋白质氨基末端的重要结构决定因素。 [参考:53]

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