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利用人红细胞带3重建葡萄糖转运

Reconstitution of glucose transport using human erythrocyte band 3.

作者信息

Shelton R L, Langdon R G

出版信息

Biochim Biophys Acta. 1983 Aug 24;733(1):25-33. doi: 10.1016/0005-2736(83)90087-1.

Abstract

Band 3 and the diffuse component of zone 4.5, designated band 4.5.B, have been separately prepared from human erythrocyte membranes and incorporated into the membranes of 150 nm 1-palmitoyl-2-oleoyl phosphatidylcholine vesicles. The rates of glucose influx into these vesicles were measured under zero-trans conditions. Both sets of vesicles exhibited substrate-saturable transport which was inhibited by phloretin. However, the specific activity of the band 3 vesicles, 292 mumol X min-1 X (mg protein)-1, was more than twice that of the band 4.5.B vesicles, and the turnover number of transporters in the band 3 vesicles was at least 4-fold greater than those in the 4.5.B vesicles. Very little background density was visible in the band 4.5 region of erythrocyte membranes protected from degradation. In unprotected membranes, band 4.5.B was abundantly present, could be purified, and had glucose transport activity. Previously we have shown (Biochemistry 19, 1205 (1980] that maltosyl isothiocyanate, an affinity label for the glucose transporter, labelled a single 100 000 Mr protein of the intact erythrocyte membrane. Based upon the results of both affinity labelling and reconstitution we suggest that the native glucose transporter is a component of band 3, and that band 4.5.B contains a partially active fragment of the native transporter.

摘要

带3以及4.5区的弥散成分(称为带4.5.B)已分别从人红细胞膜中制备出来,并整合到150 nm 1-棕榈酰-2-油酰磷脂酰胆碱囊泡的膜中。在零转运条件下测量了葡萄糖流入这些囊泡的速率。两组囊泡均表现出底物饱和转运,且这种转运受到根皮素的抑制。然而,带3囊泡的比活性为292 μmol·min⁻¹·(mg蛋白)⁻¹,是带4.5.B囊泡的两倍多,并且带3囊泡中转运体的周转数至少是4.5.B囊泡中转运体周转数的4倍。在免受降解的红细胞膜的4.5区几乎看不到背景密度。在未受保护的膜中,带4.5.B大量存在,可以被纯化,并且具有葡萄糖转运活性。此前我们已经表明(《生物化学》19, 1205 (1980)),麦芽基异硫氰酸酯是葡萄糖转运体的一种亲和标记物,它标记了完整红细胞膜上一个单一的100 000 Mr蛋白。基于亲和标记和重组的结果,我们认为天然葡萄糖转运体是带3的一个成分,并且带4.5.B包含天然转运体的一个部分活性片段。

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