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Cloning and functional expression of a Na(+)-dependent phosphate co-transporter from human kidney: cDNA cloning and functional expression.

机译:来自人肾脏的Na(+)依赖性磷酸酯共转运蛋白的克隆和功能表达:cDNA克隆和功能表达。

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摘要

A cDNA clone encoding a protein 69% identical in amino acid sequence with that of the Na/P(i) co-transporter NaP(i)-1 was isolated from a human kidney cDNA library. The DNA sequence was identical with that of NPT-1 cDNA published by Chong, Kristjansson, Zoghbi and Hughe (1993) (Genomics, 18, 355-359). In the present study, we have characterized the function of the encoded protein and the tissue distribution of its mRNA. Injection of RNA transcribed from NPT-1 into Xenopus oocytes resulted in expression of Na/P(i) co-transport activity showing a high affinity for P(i) transport (Km 0.29 mM). Kinetic characterization ([P(i)], [Na+]) demonstrated that the expressed transport activity has properties similar to those displayed by oocytes injected with human kidney poly(A)+ RNA. Northern blotting demonstrated that NPT-1 mRNA is expressed in renal cortex, liver and brain but not in other tissues. Hybrid depletion with antisense oligonucleotides to NaP(i)-3 and NPT-1 completely inhibited poly(A)+ RNA-induced Na(+)-dependent P(i) uptake in oocytes. These findings indicate that two high-affinity Na/P(i) cotransporters (NaP(i)-3 and NPT-1) are present in human kidney cortex.
机译:从人肾脏cDNA文库中分离出cDNA克隆,该克隆编码与Na / P(i)共转运蛋白NaP(i)-1的氨基酸序列具有69%同一性的蛋白质。该DNA序列与Chong,Kristjansson,Zoghbi和Hughe(1993)发表的NPT-1 cDNA的序列相同(Genomics,18,355-359)。在本研究中,我们已经表征了编码蛋白的功能及其mRNA的组织分布。将从NPT-1转录的RNA注射到非洲爪蟾卵母细胞中,导致Na / P(i)共转运活性表达,显示对P(i)转运具有很高的亲和力(Km 0.29 mM)。动力学表征([P(i)],[Na +])表明,所表达的转运活性具有与注射人肾脏poly(A)+ RNA的卵母细胞所表现出的特性相似的特性。 Northern印迹表明,NPT-1 mRNA在肾皮质,肝和脑中表达,但在其他组织中不表达。与NaP(i)-3和NPT-1反义寡核苷酸的杂交耗竭完全抑制了卵母细胞中poly(A)+ RNA诱导的Na(+)依赖性P(i)摄取。这些发现表明在人类肾皮质中存在两个高亲和力的Na / P(i)共转运蛋白(NaP(i)-3和NPT-1)。

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