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人皮肤肥大细胞羧肽酶:功能特性、cDNA克隆及谱系研究

Human skin mast cell carboxypeptidase: functional characterization, cDNA cloning, and genealogy.

作者信息

Natsuaki M, Stewart C B, Vanderslice P, Schwartz L B, Natsuaki M, Wintroub B U, Rutter W J, Goldstein S M

机构信息

Department of Dermatology, University of California, San Francisco 94143-0536.

出版信息

J Invest Dermatol. 1992 Aug;99(2):138-45. doi: 10.1111/1523-1747.ep12616776.

DOI:10.1111/1523-1747.ep12616776
PMID:1629626
Abstract

We functionally characterized human skin mast cell carboxypeptidase A (MC-CPA), and explored its evolutionary relationship to other carboxypeptidases to understand further the structural basis for the substrate preferences of this enzyme. Purified human skin MC-CPA displayed more activity than did bovine pancreatic carboxypeptidase A (CPA) against carboxyl-terminal leucine residues, about equal activity with phenylalanine and tyrosine residues, and no activity with tryptophan or alanine. To correlate kinetic data with structure, we isolated and sequenced a cDNA encoding MC-CPA from human skin, and directly sequenced 30% of the purified protein. These sequences agreed with that of human lung MC-CPA, and further support the evidence for a single MC-CPA gene in humans. Four amino acid replacements, resulting in a net positive change in non-hydrogen atoms in the S1' subsite of MC-CPA, were associated with less alteration in substrate specificity, relative to bovine CPA, than might be expected from studies using rat CPA1 and CPA2. We noted two consensus N-linked glycosylation sites in human MC-CPA that are not found in rat and mouse MC-CPA, or in bovine CPA; that at least one of these sites is glycosylated in vivo was verified by N-glycosidase F treatment, lentil lectin binding, and Concanavalin A-Sepharose chromatography. Evolutionary trees constructed from the known carboxypeptidase sequences suggested that MC-CPA most likely evolved from a carboxypeptidase B-like enzyme, independent of the pancreatic CPA. Thus, in the carboxypeptidase gene family, MC-CPA displays a unique genealogy and several amino acid replacements in its S1' binding pocket that result in substrate specificity quite similar to bovine CPA.

摘要

我们对人皮肤肥大细胞羧肽酶A(MC-CPA)进行了功能表征,并探索了它与其他羧肽酶的进化关系,以进一步了解该酶底物偏好的结构基础。纯化的人皮肤MC-CPA对羧基末端亮氨酸残基的活性高于牛胰羧肽酶A(CPA),对苯丙氨酸和酪氨酸残基的活性大致相同,对色氨酸或丙氨酸则无活性。为了将动力学数据与结构相关联,我们从人皮肤中分离并测序了编码MC-CPA的cDNA,并直接对30%的纯化蛋白进行了测序。这些序列与人肺MC-CPA的序列一致,并进一步支持了人类中存在单个MC-CPA基因的证据。相对于牛CPA,MC-CPA的S1'亚位点中非氢原子净正变化的四个氨基酸替换与底物特异性变化较小有关,这与使用大鼠CPA1和CPA2的研究预期的情况相比有所不同。我们注意到人MC-CPA中有两个共有N-连接糖基化位点,在大鼠和小鼠MC-CPA或牛CPA中未发现;通过N-糖苷酶F处理、扁豆凝集素结合和伴刀豆球蛋白A-琼脂糖层析验证了这些位点中至少有一个在体内被糖基化。根据已知的羧肽酶序列构建的进化树表明,MC-CPA很可能从一种类羧肽酶B样酶进化而来,独立于胰CPA。因此,在羧肽酶基因家族中,MC-CPA显示出独特的谱系,并且其S1'结合口袋中有几个氨基酸替换,导致底物特异性与牛CPA非常相似。

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Human skin mast cell carboxypeptidase: functional characterization, cDNA cloning, and genealogy.人皮肤肥大细胞羧肽酶:功能特性、cDNA克隆及谱系研究
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