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鉴定和比较锚蛋白重复域 1 小分子与 obscurin 的两个结合位点。

Characterization and comparison of two binding sites on obscurin for small ankyrin 1.

机构信息

Department of Biochemistry and Molecular Biology, University of Maryland, Baltimore,Baltimore, Maryland 21201, United States.

出版信息

Biochemistry. 2010 Nov 23;49(46):9948-56. doi: 10.1021/bi101165p. Epub 2010 Nov 1.

Abstract

Obscurin A, an ∼720 kDa modular protein of striated muscles, binds to small ankyrin 1 (sAnk1, Ank 1.5), an integral protein of the sarcoplasmic reticulum, through two distinct carboxy-terminal sequences, Obsc(6316-6436) and Obsc(6236-6260). We hypothesized that these sequences differ in affinity but that they compete for the same binding site on sAnk1. We show that the sequence within Obsc(6316-6436) that binds to sAnk1 is limited to residues 6316-6345. Comparison of Obsc(6231-6260) to Obsc(6316-6345) reveals that Obsc(6316-6345) binds sAnk1 with an affinity (133 ± 43 nM) comparable to that of the Obsc(6316-6436) fusion protein, whereas Obsc(6231-6260) binds with lower affinity (384 ± 53 nM). Oligopeptides of each sequence compete for binding with both sites at half-maximal inhibitory concentrations consistent with the affinities measured directly. Five of six site-directed mutants of sAnk1 showed similar reductions in binding to each binding site on obscurin, suggesting that they dock to many of the same residues of sAnk1. Circular dichroism (CD) analysis of the synthetic oligopeptides revealed a 2-fold greater α-helical content in Obsc(6316-6346), ∼35%, than Obsc(6231-6260,) ∼17%. Using these data, structural prediction algorithms, and homology modeling, we predict that Obsc(6316-6345) contains a bent α-helix of 12 amino acids, flanked by short disordered regions, and that Obsc(6231-6260) has a short, N-terminal α-helix of 4-5 residues followed by a long disordered region. Our results are consistent with a model in which both sequences of obscurin differ significantly in structure but bind to the ankyrin-like repeat motifs of sAnk1 in a similar though not identical manner.

摘要

obscurin A 是一种约 720 kDa 的横纹肌模块化蛋白,通过两个不同的羧基末端序列 obsc(6316-6436)和 obsc(6236-6260)与肌浆网的整合蛋白小锚蛋白 1 (sAnk1)结合。我们假设这些序列的亲和力不同,但它们竞争 sAnk1 上的相同结合位点。我们表明,与 sAnk1 结合的 obsc(6316-6436)内的序列仅限于残基 6316-6345。将 obsc(6231-6260)与 obsc(6316-6345)进行比较,结果表明 obsc(6316-6345)与 sAnk1 的结合亲和力 (133 ± 43 nM)与 obsc(6316-6436)融合蛋白相当,而 obsc(6231-6260)的结合亲和力较低 (384 ± 53 nM)。每个序列的寡肽以半最大抑制浓度与两个位点竞争结合,这与直接测量的亲和力一致。sAnk1 的六个位点定向突变体中的五个都显示出与 obscurin 上每个结合位点结合的相似降低,表明它们与 sAnk1 的许多相同残基结合。合成寡肽的圆二色性 (CD)分析表明,Obsc(6316-6346)的 α-螺旋含量增加了 2 倍,约为 35%,而 Obsc(6231-6260)的 α-螺旋含量约为 17%。利用这些数据、结构预测算法和同源建模,我们预测 Obsc(6316-6345)包含一个 12 个氨基酸的弯曲 α-螺旋,两侧是短的无序区域,而 Obsc(6231-6260)则有一个 4-5 个残基的短 N-端 α-螺旋,后面跟着一个长的无序区域。我们的结果与这样一个模型一致,即 obscurin 的两个序列在结构上有很大的不同,但以类似但不完全相同的方式与 sAnk1 的锚蛋白样重复基序结合。

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