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溶酶体硫酸盐转运依赖于巯基。

Lysosomal sulphate transport is dependent upon sulphydryl groups.

作者信息

Chou H F, Passage M, Jonas A J

机构信息

Division of Medical Genetics, E4, Department of Pediatrics, Harbor-UCLA Medical Center, 1124 W. Carson St., Torrance, CA 90502, USA.

出版信息

Biochem J. 1998 Mar 1;330 ( Pt 2)(Pt 2):713-7. doi: 10.1042/bj3300713.

Abstract

Using thiol blocking agents, we examined the role of sulphydryl groups for function of the lysosomal sulphate transport system. Monothiol binding reagents, p-hydroxymercuribenzoic acid (p-HMB) and p-chloromercuribenzene sulphonic acid (p-CMBS), dithiol binding reagents such as CuCl2, the alkylating agent, N-ethylmaleimide (NEM), and NADH all inhibited lysosomal sulphate transport. The inhibitory effects of NEM and Cu2+ were not additive, suggesting that they both act upon the same critical sulphydryl group(s). Unlike the case for NEM, the inhibitory effects of Cu2+ were reversed by the reducing agent, dithiothreitol. Exposure to NEM resulted in a seven-fold increase in Km to 867 microM versus a control value of 126 microM and a modest decrease in Vmax to 99 pmolperunit beta-hexosaminidase per 30 s versus a control value of 129 pmolperunit beta-hexosaminidase per 30 s. Similar although somewhat less dramatic results were obtained using Cu2+ with an increase of Km to 448 microM and a Vmax of 77 pmolperunit beta-hexosaminidase per 30 s. The sulphate transport activity of detergent solubilized lysosomal membranes could be bound to a p-chloromercuribenzoic acid (p-CMB)-Sepharose sulphydryl affinity resin and eluted with mercaptoethanol. Sulphydryl groups thus appear to play a role in sulphate transport through effects on substrate affinity. Sulphydryl-binding appears to be a strategy that may be useful for purification of the transporter.

摘要

我们使用硫醇阻断剂研究了巯基在溶酶体硫酸盐转运系统功能中的作用。单硫醇结合试剂对羟基汞苯甲酸(p-HMB)和对氯汞苯磺酸(p-CMBS)、二硫醇结合试剂如氯化铜、烷基化剂N-乙基马来酰亚胺(NEM)以及NADH均抑制溶酶体硫酸盐转运。NEM和Cu²⁺的抑制作用并非相加性的,这表明它们作用于同一个关键巯基。与NEM不同,Cu²⁺的抑制作用可被还原剂二硫苏糖醇逆转。暴露于NEM导致Km增加7倍至867微摩尔,而对照值为126微摩尔,Vmax适度降低至每30秒每单位β-己糖胺酶99皮摩尔,而对照值为每30秒每单位β-己糖胺酶129皮摩尔。使用Cu²⁺时获得了类似但不太显著的结果,Km增加至448微摩尔,Vmax为每30秒每单位β-己糖胺酶77皮摩尔。去污剂溶解的溶酶体膜的硫酸盐转运活性可与对氯汞苯甲酸(p-CMB)-琼脂糖巯基亲和树脂结合,并用巯基乙醇洗脱。因此,巯基似乎通过影响底物亲和力在硫酸盐转运中发挥作用。巯基结合似乎是一种可能有助于转运体纯化的策略。

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