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SAAT1是一种低亲和力的钠/葡萄糖协同转运蛋白,而非氨基酸转运蛋白。一种重新诠释。

SAAT1 is a low affinity Na+/glucose cotransporter and not an amino acid transporter. A reinterpretation.

作者信息

Mackenzie B, Panayotova-Heiermann M, Loo D D, Lever J E, Wright E M

机构信息

Department of Physiology, UCLA School of Medicine 90024.

出版信息

J Biol Chem. 1994 Sep 9;269(36):22488-91.

PMID:8077195
Abstract

Recently a member of the Na+/glucose (SGLT1) gene family of cotransporters was isolated from a pig renal cell line and was thought to be the neutral amino acid transporter System A. This cDNA (Kong, C. T., Yet, S. F., and Lever, J. E. (1993) J. Biol. Chem. 268, 1509-1512) encodes a 660-amino acid protein with 76% identity to SGLT1. To confirm and extend the kinetic characterization of SAAT1, we have expressed this clone in Xenopus oocytes and measured transport using both radiotracer and electrophysiological techniques. SAAT1 did not stimulate either 50 microM 2-(methylamino)isobutyrate uptake or 2-(methylamino)isobutyrate-evoked inward Na+ currents, but instead stimulated 50 microM alpha MG (alpha-methyl-D-glucopyranoside) uptake 27-fold from 2 +/- 1 pmol.h-1/oocyte (n = 9) to 55 +/- 6 pmol.h-1/oocyte (n = 9) and alpha MG-evoked inward Na+ currents (I) by up to 1000 nA/oocyte. The apparent affinity constant for alpha MG (K alpha MG 0.5) was approximately 2 mM and was independent of membrane potential from -30 to -150 mV but was voltage-sensitive between -30 and +30 mV. The relative sugar specificity for the transporter was alpha MG > or = D-glucose >> D-galactose >>> 3-O-methyl-D-glucopyranose, L-glucose. The sugar-evoked currents were Na(+)-dependent (KNa 0.5 approximately 10 mM at -50 mV) and the Hill coefficient was 1. KNa 0.5 decreased with hyperpolarization of the membrane from -50 to -150 mV. Phlorizin inhibited the alpha MG-evoked current with apparent Ki of 18 microM at -50 mV. We conclude that the SAAT1 cDNA encodes a renal low affinity Na+(1)/glucose(1) cotransporter and propose that pig SAAT1 be renamed pSGLT2.

摘要

最近,从猪肾细胞系中分离出一种协同转运蛋白的Na⁺/葡萄糖(SGLT1)基因家族成员,它被认为是中性氨基酸转运体A系统。这个cDNA(Kong,C.T.,Yet,S.F.,和Lever,J.E.(1993)J.Biol.Chem.268,1509 - 1512)编码一个660个氨基酸的蛋白质,与SGLT1有76%的同源性。为了确认并扩展SAAT1的动力学特征,我们在非洲爪蟾卵母细胞中表达了这个克隆,并使用放射性示踪剂和电生理技术测量转运情况。SAAT1既不刺激50微摩尔2 - (甲基氨基)异丁酸的摄取,也不刺激2 - (甲基氨基)异丁酸诱发的内向Na⁺电流,而是刺激50微摩尔α - MG(α - 甲基 - D - 吡喃葡萄糖苷)的摄取,从2±1皮摩尔·小时⁻¹/卵母细胞(n = 9)增加27倍至55±6皮摩尔·小时⁻¹/卵母细胞(n = 9),并且将α - MG诱发的内向Na⁺电流(I)增加到高达1000纳安/卵母细胞。α - MG的表观亲和常数(KαMG 0.5)约为2毫摩尔,在 - 30至 - 150毫伏的膜电位范围内与膜电位无关,但在 - 30至 + 30毫伏之间对电压敏感。该转运体的相对糖特异性为α - MG≥D - 葡萄糖>>D - 半乳糖>>>3 - O - 甲基 - D - 吡喃葡萄糖,L - 葡萄糖。糖诱发的电流依赖于Na⁺(在 - 50毫伏时KNa 0.5约为10毫摩尔),希尔系数为1。随着膜从 - 50毫伏超极化到 - 150毫伏,KNa 0.5降低。根皮素在 - 50毫伏时以18微摩尔的表观Ki抑制α - MG诱发的电流。我们得出结论,SAAT1 cDNA编码一种肾低亲和力Na⁺(1)/葡萄糖(1)协同转运蛋白,并建议将猪SAAT1重新命名为pSGLT2。

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