Veyhl M, Spangenberg J, Püschel B, Poppe R, Dekel C, Fritzsch G, Haase W, Koepsell H
Max-Planck-Institut für Biophysik, Frankfurt am Main, Germany.
J Biol Chem. 1993 Nov 25;268(33):25041-53.
An expression library from porcine kidney cortex was screened with a monoclonal antibody (R4A6) which stimulates high-affinity phlorizin binding in kidney and intestine but does not react with the membrane protein (SGLT1) which mediates Na(+)-coupled transport of D-glucose (Hediger, M.A., Coady, M.J., Ikeda, T.S., and Wright, E.M. (1987) Nature 330, 379-381). A cDNA (RS1) was obtained which codes for a hydrophilic M(r) 66,832 polypeptide and contains a predicted hydrophobic alpha-helix at the COOH terminus. After expression in Xenopus oocytes RS1 protein was found associated with the plasma membrane. RS1-homologous mRNAs were detected in renal outer cortex and outer medulla, small intestine, liver, and LLCPK1 cells, but not in skeletal muscle, heart muscle, Madin-Darby canine kidney (MDCK) cells, renal inner medulla, and Xenopus oocytes. After nondenaturing gel electrophoresis of renal brush-border membranes comigration of RS1- and SGLT1-homologous proteins as a high molecular weight complex was demonstrated. RS1 altered the expression of Na(+)-glucose cotransport by SGLT1 in Xenopus oocytes. There was no effect on the expression of the nonhomologous transporters for Na(+)-gamma-aminobutyric acid cotransport and for Na(+)-independent glucose transport. However, RS1 also changed the expression of the SGLT1-homologous Na(+)-myo-inositol cotransporter from MDCK cells. The Vmax of methyl-alpha-D-glucopyranoside (AMG) transport expressed after injection of a small amount of SGLT1-cRNA was increased 40-fold when a stoichiometric amount of RS1-cRNA was coinjected. In addition the voltage and glucose dependence of expressed AMG uptake and the concentration dependence of transport inhibition by phlorizin were changed when stoichiometric amounts of RS1-cRNA were coinjected with SGLT1-cRNA. Thus with SGLT1 one apparent transport site (K0.5 about 100 microM) and one apparent phlorizin inhibition site (Ki about 5 microM) was observed whereas with SGLT1 plus RS1 two apparent transport sites (K0.5(1) about 20 microM, K0.5(2) about 1 mM) and two apparent phlorizin inhibition sites (Ki(1) about 0.3 microM, Ki(2) about 30 microM) were found as has been described in brush-border membrane vesicles of kidney and intestine (see e.g. Koepsell, H., Fritzsch, G., Korn, K., and Madrala, A. (1990) J. Membr. Biol. 114, 113-132). The data suggest that the Na(+)-D-glucose cotransporter and possibly also other SGLT1-type Na(+)-cotransporters contain RS1-type regulatory subunits.
用一种单克隆抗体(R4A6)筛选猪肾皮质的表达文库,该抗体可刺激肾脏和肠道中高亲和力的根皮苷结合,但不与介导D - 葡萄糖钠偶联转运的膜蛋白(SGLT1)反应(赫迪格,M.A.,科迪,M.J.,池田,T.S.,和赖特,E.M.(1987年)《自然》330,379 - 381)。获得了一个编码亲水性M(r)66,832多肽的cDNA(RS1),其COOH末端含有一个预测的疏水性α - 螺旋。在非洲爪蟾卵母细胞中表达后,发现RS1蛋白与质膜相关。在肾外皮质和外髓、小肠、肝脏和LLCPK1细胞中检测到RS1同源mRNA,但在骨骼肌、心肌、犬肾Madin - Darby细胞(MDCK)、肾内髓和非洲爪蟾卵母细胞中未检测到。对肾刷状缘膜进行非变性凝胶电泳后,证明RS1和SGLT1同源蛋白以高分子量复合物形式共迁移。RS1改变了非洲爪蟾卵母细胞中SGLT1介导的钠 - 葡萄糖共转运的表达。对钠 - γ - 氨基丁酸共转运和钠非依赖性葡萄糖转运的非同源转运体的表达没有影响。然而,RS1也改变了MDCK细胞中SGLT1同源的钠 - 肌醇共转运体的表达。当共注射化学计量的RS1 - cRNA时,注射少量SGLT 1 - cRNA后表达的甲基 - α - D - 吡喃葡萄糖苷(AMG)转运的Vmax增加了40倍。此外,当化学计量的RS1 - cRNA与SGLT 1 - cRNA共注射时,表达的AMG摄取的电压和葡萄糖依赖性以及根皮苷对转运的抑制浓度依赖性发生了变化。因此,对于SGLT 1,观察到一个明显的转运位点(K 0.5约100μM)和一个明显的根皮苷抑制位点(Ki约5μM),而对于SGLT 1加RS1,发现了两个明显的转运位点(K {0.5(1)}约20μM,K {0.5(2)}约1 mM)和两个明显的根皮苷抑制位点(Ki {(1)}约0.3μM,Ki {(2)}约30μM),这与在肾脏和肠道的刷状缘膜囊泡中所描述的情况一致(例如见克普塞尔,H.,弗里茨施,G.,科恩,K.,和马德拉拉,A.(1990年)《膜生物学杂志》114,113 - 132)。数据表明钠 - D - 葡萄糖共转运体以及可能其他SGLT1型钠共转运体含有RS1型调节亚基。
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