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两个不相邻的区域促使巢蛋白结合至层粘连蛋白γ1链的单个表皮生长因子样基序。

Two non-contiguous regions contribute to nidogen binding to a single EGF-like motif of the laminin gamma 1 chain.

作者信息

Pöschl E, Fox J W, Block D, Mayer U, Timpl R

机构信息

Max-Planck Connective Tissue Clinical Research Group for Rheumatology, Erlangen, Germany.

出版信息

EMBO J. 1994 Aug 15;13(16):3741-7. doi: 10.1002/j.1460-2075.1994.tb06683.x.

DOI:10.1002/j.1460-2075.1994.tb06683.x
PMID:8070402
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC395285/
Abstract

High affinity binding of nidogen to laminin is mediated by an EGF-like repeat gamma 1III4 of the mouse laminin gamma 1 chain and has now been restricted to two short noncontiguous regions of its 56 residue sequence by use of synthetic peptides and recombinant mutants. Disulfide loop a,b of the repeat and a modified loop a,c could completely inhibit binding, with a 5000-fold or 300-fold reduced affinity respectively. Synthetic loops c and d lacked inhibitory activity. Some binding contribution of Tyr819 in loop c was, however, shown by mutation and side chain modification. Together with studies of loop chimeras, this indicated a distinct cooperativity between the two binding sites. The major binding site of loop a was localized to the heptapeptide NIDPNAV (position 798-804). A change of Asp800 to Asn or Ala803 to Val caused a strong reduction in binding activity, while only small effects were observed for the changes Pro801 to Gln and Ile799 to Val. The latter replacement corresponds to the single substitution found in the same region of the Drosophila laminin gamma 1 chain. However, the changes Asn802 to Ser or Val804 to Ser, both known to exist in the laminin gamma 2 chain, were deleterious mutations. This demonstrated conservation of binding structures in laminins of distantly related species, but not between homologous chains of laminin isoforms.

摘要

巢蛋白与层粘连蛋白的高亲和力结合由小鼠层粘连蛋白γ1链的一个表皮生长因子样重复序列γ1III4介导,通过使用合成肽和重组突变体,现已将其限制在其56个残基序列的两个不连续的短区域内。该重复序列的二硫键环a、b以及一个修饰的环a、c可分别以5000倍或300倍降低的亲和力完全抑制结合。合成环c和d缺乏抑制活性。然而,通过突变和侧链修饰表明环c中的Tyr819有一定的结合贡献。连同环嵌合体的研究,这表明两个结合位点之间存在明显的协同作用。环a的主要结合位点定位于七肽NIDPNAV(第798 - 804位)。将Asp800突变为Asn或Ala803突变为Val会导致结合活性大幅降低,而将Pro801突变为Gln和Ile799突变为Val的变化仅观察到较小影响。后一种替换对应于果蝇层粘连蛋白γ1链同一区域中发现的单取代。然而,已知存在于层粘连蛋白γ2链中的Asn802突变为Ser或Val804突变为Ser的变化是有害突变。这证明了远缘物种层粘连蛋白中结合结构的保守性,但层粘连蛋白异构体的同源链之间不存在这种保守性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1274/395285/1d10c8b4045a/emboj00064-0093-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1274/395285/1d10c8b4045a/emboj00064-0093-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1274/395285/1d10c8b4045a/emboj00064-0093-a.jpg

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2
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The role of asparagine-32 in forming the receptor-binding epitope of human epidermal growth factor.天冬酰胺-32在形成人表皮生长因子受体结合表位中的作用。
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