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源自胞吐和胞吞途径的被膜小泡中的溶酶体酶前体。

Lysosomal enzyme precursors in coated vesicles derived from the exocytic and endocytic pathways.

作者信息

Lemansky P, Hasilik A, von Figura K, Helmy S, Fishman J, Fine R E, Kedersha N L, Rome L H

出版信息

J Cell Biol. 1987 Jun;104(6):1743-8. doi: 10.1083/jcb.104.6.1743.

Abstract

The molecular forms of two lysosomal enzymes, cathepsin C and cathepsin D, have been examined in lysosomes and coated vesicles (CVs) of rat liver. In addition, the relative proportion of these lysosomal enzymes residing in functionally distinct CV subpopulations was quantitated. CVs contained newly synthesized precursor forms of the enzymes in contrast to lysosomes where only the mature forms were detected. Exocytic and endocytic CV subpopulations were prepared by two completely different protocols. One procedure, a density shift method, uses cholinesterase to alter the density of CVs derived from exocytic or endocytic pathways. The other relies on electrophoretic heterogeneity to accomplish the CV subfractionation. Subpopulations of CVs prepared by either procedure showed similar results, when examined for their relative proportion of cathepsin C and cathepsin D precursors. Within the starting CV preparation, exocytic CVs contained approximately 80-90% of the total steady-state levels of these enzymes while the level in the endocytic population was approximately 10-13%. The implications of these findings are discussed with regard to lysosome trafficking.

摘要

在大鼠肝脏的溶酶体和被膜小泡(CVs)中,对两种溶酶体酶组织蛋白酶C和组织蛋白酶D的分子形式进行了检测。此外,还对这些溶酶体酶在功能不同的CV亚群中的相对比例进行了定量。与仅检测到成熟形式的溶酶体不同,CVs含有新合成的酶前体形式。通过两种完全不同的方案制备了胞吐和胞吞CV亚群。一种方法是密度转移法,利用胆碱酯酶改变源自胞吐或胞吞途径的CVs的密度。另一种方法则依靠电泳异质性来完成CV亚分级分离。当检测组织蛋白酶C和组织蛋白酶D前体的相对比例时,通过这两种方法制备的CV亚群显示出相似的结果。在起始的CV制剂中,胞吐CVs含有这些酶总稳态水平的约80 - 90%,而胞吞群体中的水平约为10 - 13%。就溶酶体运输而言,对这些发现的意义进行了讨论。

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