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组织蛋白酶D中最小溶酶体酶识别结构域的鉴定

Identification of the minimal lysosomal enzyme recognition domain in cathepsin D.

作者信息

Steet Richard, Lee Wang-Sik, Kornfeld Stuart

机构信息

Department of Internal Medicine, Washington University School of Medicine, Saint Louis, Missouri 63110, USA.

出版信息

J Biol Chem. 2005 Sep 30;280(39):33318-23. doi: 10.1074/jbc.M505994200. Epub 2005 Aug 4.

Abstract

Specific recognition of lysosomal hydrolases by UDP-GlcNAc:lysosomal enzyme N-acetylglucosamine-1-phosphotransferase, the initial enzyme in the biosynthesis of mannose 6-phosphate residues, is governed by a common protein determinant. Previously, we generated a lysosomal enzyme recognition domain in the secretory protein glycopepsinogen by substituting in two regions (lysine 203 and amino acids 265-293 of the beta loop) from cathepsin D, a highly related lysosomal protease. Here we show that substitution of just two lysines (Lys-203 and Lys-267) stimulates mannose phosphorylation 116-fold. Substitution of additional residues in the beta loop, particularly lysines, increased phosphorylation 4-fold further, approaching the level obtained with intact cathepsin D. All the phosphorylation occurred at the carboxyl lobe glycan, indicating that additional elements are required for phosphorylation of the amino lobe glycan. These data support the proposal that as few as two lysines in the correct orientation to each other and to the glycan can serve as the minimal elements of the lysosomal enzyme recognition domain. However, our findings show that the spacing between lysines is flexible and other residues contribute to the recognition marker.

摘要

UDP-N-乙酰葡糖胺:溶酶体酶N-乙酰葡糖胺-1-磷酸转移酶对溶酶体水解酶的特异性识别是甘露糖6-磷酸残基生物合成中的起始酶,它受一个共同的蛋白质决定簇调控。此前,我们通过替换组织蛋白酶D(一种高度相关的溶酶体蛋白酶)的两个区域(赖氨酸203和β环的氨基酸265 - 293),在分泌蛋白糖胃蛋白酶原中生成了一个溶酶体酶识别结构域。在此我们表明,仅替换两个赖氨酸(Lys - 203和Lys - 267)就能使甘露糖磷酸化增加116倍。在β环中替换其他残基,尤其是赖氨酸,能使磷酸化进一步增加4倍,接近完整组织蛋白酶D所达到的水平。所有的磷酸化都发生在羧基叶聚糖上,这表明氨基叶聚糖的磷酸化还需要其他元件。这些数据支持了这样的提议,即彼此以及与聚糖呈正确方向排列的仅两个赖氨酸可作为溶酶体酶识别结构域的最小元件。然而,我们的研究结果表明,赖氨酸之间的间距是灵活的,其他残基也对识别标记有贡献。

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