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脯氨酰4-羟化酶及其蛋白质二硫键异构酶亚基。

Prolyl 4-hydroxylases and their protein disulfide isomerase subunit.

作者信息

Kivirikko K I, Myllyharju J

机构信息

Collagen Research Unit, University of Oulu, Finland.

出版信息

Matrix Biol. 1998 Feb;16(7):357-68. doi: 10.1016/s0945-053x(98)90009-9.

DOI:10.1016/s0945-053x(98)90009-9
PMID:9524356
Abstract

Prolyl 4-hydroxylases (EC 1.14,11.2) catalyze the formation of 4-hydroxyproline in collagens and other proteins with collagen-like sequences. The vertebrate type I and type II enzymes are [alpha (I)]2 beta 2 and [alpha (II)]2 beta 2 tetramers, respectively, whereas the enzyme from the nematode Caenorhabditis elegans is an alpha beta dimer. The type I enzyme is the major form in most but not all vertebrate tissues. The catalytic properties of the various enzyme forms are highly similar, but there are distinct, although small, differences in K(m) values for various peptide substrates between the enzyme forms and major differences in Ki values for the competitive inhibitor, poly(L-proline). Prolyl 4-hydroxylase requires Fe2+, 2-oxoglutarate, O2 and ascorbate. Kinetic studies and theoretical considerations have led to elucidation of the reaction mechanism, and recent extensive site-directed mutagenesis studies have identified five critical residues at the cosubstrate binding sites. A number of compounds have been characterized that inhibit it competitively with respect to some of the cosubstrates, and three groups of suicide inactivators have also been identified. The beta subunit in all forms of prolyl 4-hydroxylase is identical to protein disulfide isomerase (PDI), a multifunctional polypeptide that also serves as a subunit in the microsomal triglyceride transfer protein, as a chaperone-like polypeptide that probably assists folding of a number of newly synthesized proteins, and in several other functions. The main role of the PDI polypeptide as a protein subunit is probably related to its chaperone function. Recent expression studies of recombinant human prolyl 4-hydroxylase subunits in a yeast have indicated that the formation of a stable enzyme tetramer in vivo requires coexpression of collagen polypeptide chains.

摘要

脯氨酰4-羟化酶(EC 1.14,11.2)催化胶原蛋白及其他具有类胶原蛋白序列的蛋白质中4-羟脯氨酸的形成。脊椎动物的I型和II型酶分别是[α(I)]2β2和[α(II)]2β2四聚体,而来自线虫秀丽隐杆线虫的酶是αβ二聚体。I型酶是大多数但并非所有脊椎动物组织中的主要形式。各种酶形式的催化特性高度相似,但不同酶形式之间对于各种肽底物的米氏常数(Km)值存在明显但较小的差异,并且对于竞争性抑制剂聚(L-脯氨酸)的抑制常数(Ki)值存在较大差异。脯氨酰4-羟化酶需要Fe2+、2-氧代戊二酸、O2和抗坏血酸。动力学研究和理论思考已阐明了反应机制,最近广泛的定点诱变研究已确定了共底物结合位点的五个关键残基。已鉴定出一些化合物,它们相对于某些共底物具有竞争性抑制作用,并且还鉴定出了三组自杀性灭活剂。所有形式的脯氨酰4-羟化酶中的β亚基与蛋白质二硫键异构酶(PDI)相同,PDI是一种多功能多肽,它还作为微粒体甘油三酯转移蛋白的一个亚基、一种可能协助许多新合成蛋白质折叠的伴侣样多肽以及在其他几种功能中发挥作用。PDI多肽作为蛋白质亚基的主要作用可能与其伴侣功能有关。最近在酵母中对重组人脯氨酰4-羟化酶亚基的表达研究表明,体内稳定酶四聚体的形成需要胶原蛋白多肽链的共表达。

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