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对绒毛蛋白头部结构域76个位置中的40个进行半胱氨酸扫描诱变,确定了F-肌动蛋白结合位点及该结构域的结构特征。

Cysteine scanning mutagenesis at 40 of 76 positions in villin headpiece maps the F-actin binding site and structural features of the domain.

作者信息

Doering D S, Matsudaira P

机构信息

Whitehead Institute for Biomedical Research, Massachusetts Institute of Technology, Cambridge 02142, USA.

出版信息

Biochemistry. 1996 Oct 1;35(39):12677-85. doi: 10.1021/bi9615699.

DOI:10.1021/bi9615699
PMID:8841111
Abstract

Villin headpiece, the 76 amino acid, C-terminal domain of villin, is one of the two F-actin binding sites in villin necessary for F-actin bundling activity. Expression and study of recombinant headpiece revealed the domain to be remarkably thermostable (Tm = 74 degrees C) for a non-disulfide-bonded domain. Forty independent point mutations to cysteine of headpiece have been purified and tested for their actin binding activity, cysteine reactivity, and thermal stability. These assays identify two segments of headpiece, near amino acids 38 and 70 of headpiece, in which mutations to cysteine significantly disrupt cosedimentation of headpiece with F-actin. Assay of the thermal stability of these mutants and assay of the reactivity of the introduced cysteine show that these amino acids are mutations at the protein surface that do not perturb the overall structure of the domain. The actin binding mutants are replacements to cysteine of Lys38, Glu39, Lys65, Lys70, Lys71, Leu75, and Phe76 of headpiece. We propose that these discontinuous segments of charged amino acids define the F-actin binding contacts of the headpiece domain. The assay of mutants for effects on the thermal stability of helical structure as well as the assay of reactivity of the introduced sulfhydryl group identify candidate positions that are involved in the stabilizing core and internal structure of the domain. The cysteine scanning mutagenesis also identifies an amino-terminal subdomain (Val1-Leu35) and a predominantly helical carboxy-terminal subdomain (Pro36-Phe76).

摘要

绒毛蛋白头部结构域是绒毛蛋白的76个氨基酸的C末端结构域,是绒毛蛋白中F-肌动蛋白成束活性所必需的两个F-肌动蛋白结合位点之一。重组头部结构域的表达和研究表明,对于一个非二硫键结合的结构域来说,该结构域具有显著的热稳定性(熔点=74摄氏度)。已经纯化了40个独立的头部结构域半胱氨酸点突变体,并测试了它们的肌动蛋白结合活性、半胱氨酸反应性和热稳定性。这些实验确定了头部结构域中靠近氨基酸38和70的两个片段,其中半胱氨酸突变显著破坏了头部结构域与F-肌动蛋白的共沉降。对这些突变体的热稳定性分析以及对引入的半胱氨酸的反应性分析表明,这些氨基酸是蛋白质表面的突变,不会干扰该结构域的整体结构。肌动蛋白结合突变体是头部结构域中赖氨酸38、谷氨酸39、赖氨酸65、赖氨酸70、赖氨酸71、亮氨酸75和苯丙氨酸76被半胱氨酸取代的突变体。我们提出,这些带电荷氨基酸的不连续片段定义了头部结构域的F-肌动蛋白结合位点。对突变体对螺旋结构热稳定性影响的分析以及对引入的巯基反应性的分析确定了参与该结构域稳定核心和内部结构的候选位置。半胱氨酸扫描诱变还确定了一个氨基末端亚结构域(缬氨酸1-亮氨酸35)和一个主要为螺旋的羧基末端亚结构域(脯氨酸36-苯丙氨酸76)。

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