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氯化汞使谷氨酸摄取与羟基当量的反向转运解偶联。

Mercuric chloride uncouples glutamate uptake from the countertransport of hydroxyl equivalents.

作者信息

Nagaraja T N, Brookes N

机构信息

Department of Pharmacology and Experimental Therapeutics, University of Maryland School of Medicine, Baltimore 21201, USA.

出版信息

Am J Physiol. 1996 Nov;271(5 Pt 1):C1487-93. doi: 10.1152/ajpcell.1996.271.5.C1487.

DOI:10.1152/ajpcell.1996.271.5.C1487
PMID:8944631
Abstract

The cotransport of sodium and glutamate by system X(AG)- is believed to be coupled to the countertransport of potassium and hydroxyl ion equivalents. Accordingly, the uptake of glutamate or D-aspartate in astrocytes is accompanied by an intracellular acidification. Here, we report that HgCl2 blocks the glutamate-induced acidification with an approximate 50% inhibitor concentration (IC50) of 55 nM, an order of magnitude below its IC50 for inhibition of glutamate uptake. At 100 nM HgCl2, glutamate-induced acidification was abolished, whereas glutamate uptake was unaffected. D-Aspartate-induced acidification was equally sensitive to HgCl2, indicating that HgCl2 blocked a transporter-mediated, rather than a receptor-mediated, acidification. Unaltered responses to acute acid and alkaline loads showed that HgCl2 was not acting indirectly via a change in pH regulation. We conclude that HgCl2 acted directly on the glutamate transporter to uncouple the uptake of glutamate from the export of hydroxyl equivalents. In contrast, two other sulfhydryl reagents, p-chloromercuribenzensulfonate and N-ethylmaleimide, failed to discriminate between glutamate-induced acidification and glutamate uptake. An additional effect of > or = 100 nM HgCl2, in this case shared by p-chlormercuribenzenesulfonate, was transient intracellular acidification. There is evidence that glutamate transport is regulated by intracellular pH. Mercuric mercury may disrupt the regulation of glutamate transport at lower concentrations than those that block transport.

摘要

X(AG)系统介导的钠和谷氨酸的协同转运被认为与钾和羟离子当量的反向转运相偶联。因此,星形胶质细胞对谷氨酸或D-天冬氨酸的摄取伴随着细胞内酸化。在此,我们报告HgCl2可阻断谷氨酸诱导的酸化,其约50%抑制浓度(IC50)为55 nM,比其抑制谷氨酸摄取的IC50低一个数量级。在100 nM HgCl2时,谷氨酸诱导的酸化被消除,而谷氨酸摄取不受影响。D-天冬氨酸诱导的酸化对HgCl2同样敏感,表明HgCl2阻断的是转运体介导的酸化,而非受体介导的酸化。对急性酸和碱负荷的反应未改变,表明HgCl2并非通过改变pH调节间接起作用。我们得出结论,HgCl2直接作用于谷氨酸转运体,使谷氨酸摄取与羟离子当量的输出解偶联。相比之下,另外两种巯基试剂,对氯汞苯磺酸盐和N-乙基马来酰亚胺未能区分谷氨酸诱导的酸化和谷氨酸摄取。≥100 nM HgCl2的另一个作用(在这种情况下对氯汞苯磺酸盐也有此作用)是短暂的细胞内酸化。有证据表明谷氨酸转运受细胞内pH调节。汞离子可能在低于阻断转运的浓度时就破坏谷氨酸转运的调节。

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