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小鼠46 kDa甘露糖6-磷酸受体的克隆、测序及功能特性分析

Cloning, sequencing, and functional characterization of the murine 46-kDa mannose 6-phosphate receptor.

作者信息

Ma Z M, Grubb J H, Sly W S

机构信息

Edward A. Doisy Department of Biochemistry and Molecular Biology, St. Louis University School of Medicine, Missouri 63104.

出版信息

J Biol Chem. 1991 Jun 5;266(16):10589-95.

PMID:1645352
Abstract

We have cloned and sequenced the 2175-nucleotide, full-length cDNA for the mouse 46-kDa Man 6-P receptor (46MPR) and studied its functional properties in stably transfected mouse L cells which do not express the insulin-like growth factor-II receptor/mannose 6-phosphate receptor (IGF-IIR/MPR). The 278-amino acid sequence deduced from the cDNA for the murine 46MPR shows 19 amino acid differences from that of the human 46MPR, none of which are found in the 68-amino acid cytoplasmic tail. Binding of ligand to the murine 46MPR in permeabilized cells showed a pH optimum of 6.5, was completely inhibited by Man 6-P, and was stimulated by divalent cations. Mn2+ was more effective than Ca2+ or Mg2+. Endocytosis was demonstrated at pH 6.5 and was stimulated 4-7-fold by Mn2+. In its responsiveness to divalent cations and its preference for Mn2+, the murine 46MPR resembled the bovine 46MPR more than the human 46MPR. It was even less efficient than the human receptor in its ability to mediate endocytosis in transfected murine cells. It was also no more efficient than the human 46MPR in correcting the sorting defect of IGF-IIR/MPR-deficient mouse L cells. We conclude that the previously observed relative inefficiency of the human 46MPR in sorting enzymes to lysosomes in murine cells is a property of the 46MPR itself and not a manifestation of studying its expression in a heterologous cell line.

摘要

我们已经克隆并测序了小鼠46 kDa甘露糖6-磷酸受体(46MPR)的2175个核苷酸的全长cDNA,并在稳定转染的不表达胰岛素样生长因子-II受体/甘露糖6-磷酸受体(IGF-IIR/MPR)的小鼠L细胞中研究了其功能特性。从小鼠46MPR的cDNA推导的278个氨基酸序列与人类46MPR的序列有19个氨基酸差异,其中在68个氨基酸的胞质尾部均未发现。在通透细胞中,配体与小鼠46MPR的结合显示最佳pH值为6.5,完全被甘露糖6-磷酸抑制,并受到二价阳离子的刺激。Mn2+比Ca2+或Mg2+更有效。在pH 6.5时证明有内吞作用,并且Mn2+可刺激4至7倍。在对二价阳离子的反应性及其对Mn2+的偏好方面,小鼠46MPR与牛46MPR的相似性超过人类46MPR。在转染的小鼠细胞中介导内吞作用的能力上,它甚至比人类受体效率更低。在纠正IGF-IIR/MPR缺陷的小鼠L细胞的分选缺陷方面,它也不比人类46MPR更有效。我们得出结论,先前观察到的人类46MPR在小鼠细胞中将酶分选到溶酶体中的相对低效是46MPR自身的特性,而不是在异源细胞系中研究其表达的表现。

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