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内质网伴侣蛋白GRP94的亚基组装通过一个特定的寡聚化结构域进行调控。

Endoplasmic reticulum chaperone GRP94 subunit assembly is regulated through a defined oligomerization domain.

作者信息

Wearsch P A, Nicchitta C V

机构信息

Department of Cell Biology, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Biochemistry. 1996 Dec 24;35(51):16760-9. doi: 10.1021/bi962068q.

DOI:10.1021/bi962068q
PMID:8988013
Abstract

GRP94 is an abundant, resident glycoprotein of the mammalian endoplasmic reticulum lumen and member of the hsp90 family of molecular chaperones. To identify the structure/function relationships which define the molecular basis of GRP94 activity, we have performed a structural analysis of native GRP94 and identified a discrete domain, representing amino acids 676-719, which regulates dimerization and displays autonomous oligomerization activity. Velocity sedimentation and gel filtration chromatography were used to identify native GRP94 as a dimer with an extended, rod-like shape. Limited proteolysis resulted in the loss of approximately 16 kDa from the C-terminus and disassembly into monomers, implicating the C-terminus as the site of assembly. An assembly function for the C-terminal domain was established by analysis of the quaternary structure of C-terminal constructs synthesized either in vitro or through recombinant expression. In vitro translation was used to demonstrate that a C-terminal 20 kDa domain was both necessary and sufficient for dimerization. Structural studies of recombinant fusion protein constructs yielded identification of a 44 amino acid domain that displayed autonomous dimerization activity and conferred a highly elongated structure, characteristic of native GRP94, to the fusion protein. These data, combined with molecular dimensions obtained from rotary shadowing electron microscopy, provide a structural model of GRP94 and identify the molecular basis of GRP94 self-assembly.

摘要

GRP94是一种丰富的驻留于哺乳动物内质网腔的糖蛋白,也是分子伴侣hsp90家族的成员。为了确定定义GRP94活性分子基础的结构/功能关系,我们对天然GRP94进行了结构分析,并鉴定出一个离散结构域,该结构域代表氨基酸676 - 719,它调节二聚化并显示出自主寡聚化活性。通过速度沉降和凝胶过滤色谱法鉴定出天然GRP94为具有延长的杆状形状的二聚体。有限的蛋白水解导致C末端约16 kDa的丢失并分解为单体,这表明C末端是组装位点。通过分析体外合成或通过重组表达产生的C末端构建体的四级结构,确定了C末端结构域的组装功能。体外翻译用于证明C末端20 kDa结构域对于二聚化既必要又充分。重组融合蛋白构建体的结构研究鉴定出一个44个氨基酸的结构域,该结构域显示出自主二聚化活性,并赋予融合蛋白以天然GRP94特有的高度延长结构。这些数据与通过旋转阴影电子显微镜获得的分子尺寸相结合,提供了GRP94的结构模型,并确定了GRP94自组装的分子基础。

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