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克隆的大鼠脑L-谷氨酸/L-天冬氨酸转运体GLAST-1的N-糖基化位点定位及碳水化合物单元的功能作用

Localization of N-glycosylation sites and functional role of the carbohydrate units of GLAST-1, a cloned rat brain L-glutamate/L-aspartate transporter.

作者信息

Conradt M, Storck T, Stoffel W

机构信息

Institute of Biochemistry, Medical Faculty, University of Cologne, Germany.

出版信息

Eur J Biochem. 1995 May 1;229(3):682-7. doi: 10.1111/j.1432-1033.1995.tb20514.x.

DOI:10.1111/j.1432-1033.1995.tb20514.x
PMID:7758463
Abstract

The L-glutamate transporter GLAST-1 belongs to the newly discovered family of Na(+)-dependent, high-affinity glutamate transporters, which are involved in the regulation of synaptic excitatory neurotransmitter concentration in mammalian brain. The members of this family have a similar topological organisation with at least six transmembrane helices (TMHs) and two putative N-glycosylation sites located in the extracellular loop connecting TMH 3 and TMH 4. Besides these two conserved N-glycosylation motifs at Asn206 and Asn216, GLAST-1 possesses an additional one at Asn35. The putative N-glycosylation consensus motifs (Asn-Xaa-Ser/Thr) were deleted by replacement of Asn206 and/or Asn216 by Thr using site-directed mutagenesis (mutants N206T, N216T and N206,216T). The cDNAs encoding wild-type GLAST-1 and the three glycosylation-defective transport proteins were expressed in the Xenopus laevis oocyte system. Immunoprecipitation of the [35S]methionine-labeled and glycopeptidase-F-treated transporter molecules indicates that GLAST-1 is glycosylated at Asn206 and Asn216, whereas Asn35 remains unglycosylated. To assess a possible functional role of the two glycosylation sites wild-type and glycosylation-deficient GLAST-1 were expressed in Xenopus oocytes and characterized functionally by using the whole-cell voltage-clamp technique. The results prove that N-glycosylation has no impact on the transport activity of GLAST-1.

摘要

L-谷氨酸转运体GLAST-1属于新发现的Na⁺依赖性高亲和力谷氨酸转运体家族,该家族参与调节哺乳动物大脑中突触兴奋性神经递质的浓度。这个家族的成员具有相似的拓扑结构,至少有六个跨膜螺旋(TMH),以及位于连接TMH 3和TMH 4的细胞外环中的两个假定的N-糖基化位点。除了在Asn206和Asn216处的这两个保守的N-糖基化基序外,GLAST-1在Asn35处还有一个额外的N-糖基化位点。通过定点诱变(突变体N206T、N216T和N206,216T)将Asn206和/或Asn216替换为Thr,从而删除假定的N-糖基化共有基序(Asn-Xaa-Ser/Thr)。编码野生型GLAST-1和三种糖基化缺陷转运蛋白的cDNA在非洲爪蟾卵母细胞系统中表达。对[³⁵S]甲硫氨酸标记且经糖肽酶F处理的转运体分子进行免疫沉淀表明,GLAST-1在Asn206和Asn216处被糖基化,而Asn35未被糖基化。为了评估这两个糖基化位点可能的功能作用,将野生型和糖基化缺陷型GLAST-1在非洲爪蟾卵母细胞中表达,并使用全细胞膜片钳技术进行功能表征。结果证明,N-糖基化对GLAST-1的转运活性没有影响。

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