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猴RALDH1的克隆及猴肾近端小管细胞中视黄酸代谢的特征分析。

Cloning of monkey RALDH1 and characterization of retinoid metabolism in monkey kidney proximal tubule cells.

作者信息

Brodeur Helene, Gagnon Isabelle, Mader Sylvie, Bhat Pangala V

机构信息

Laboratory of Nutrition and Cancer, Universite de Montreal, Montreal, Quebec, Canada.

出版信息

J Lipid Res. 2003 Feb;44(2):303-13. doi: 10.1194/jlr.M200359-JLR200. Epub 2002 Nov 4.

DOI:10.1194/jlr.M200359-JLR200
PMID:12576512
Abstract

All-trans and 9-cis retinoic acids function as ligands for retinoic acid receptors (RARs and RXRs), which are ligand-dependent transcription factors and play important roles in development and cellular differentiation. Several retinal dehydrogenases are likely to contribute to the production of all-trans and 9-cis RAs in vivo, but their respective roles in different tissues are still poorly characterized. We have previously characterized and cloned from kidney tissues the rat retinal dehydrogenase type 1 (RALDH1), which oxidizes all-trans and 9-cis retinal with high efficiency but is inactive with 13-cis retinal. Here we have characterized the retinal-oxidizing activity in monkey JTC12 cells, which are derived from kidney proximal tubules. In vitro assay of cell lysates revealed the presence of a NAD+-dependent dehydrogenase that catalyzed the oxidation of all-trans, 9-cis, and 13-cis retinal. Northern blot analysis of JTC12 RNAs and cloning by reverse transcription-polymerase chain reaction demonstrated expression of a monkey homolog of RALDH1. Bacterially expressed JTC12 RALDH1 catalyzed conversion of all three retinal isomers, with a higher catalytic efficiency for 9-cis retinal than for all-trans and 13-cis retinal. Accordingly, live JTC12 produced 9-cis retinoic acid more efficiently than all-trans retinoic acid from their respective retinal precursors. Only metabolites corresponding to the same steric conformation were formed from 9-cis or all-trans retinal, indicating a lack of detectable isomerizing activity in JTC12 cells.

摘要

全反式视黄酸和9-顺式视黄酸作为视黄酸受体(RARs和RXRs)的配体发挥作用,视黄酸受体是依赖配体的转录因子,在发育和细胞分化中起重要作用。几种视网膜脱氢酶可能在体内全反式和9-顺式视黄酸的产生中起作用,但它们在不同组织中的各自作用仍未得到充分表征。我们之前已从肾组织中鉴定并克隆出大鼠视网膜脱氢酶1型(RALDH1),它能高效氧化全反式和9-顺式视黄醛,但对13-顺式视黄醛无活性。在此,我们对源自肾近端小管的猴JTC12细胞中的视黄醛氧化活性进行了表征。细胞裂解物的体外测定显示存在一种依赖NAD +的脱氢酶,它催化全反式、9-顺式和13-顺式视黄醛的氧化。对JTC12 RNA进行Northern印迹分析并通过逆转录-聚合酶链反应进行克隆,证实了RALDH1的猴同源物的表达。细菌表达的JTC12 RALDH1催化所有三种视黄醛异构体的转化,对9-顺式视黄醛的催化效率高于全反式和13-顺式视黄醛。因此,活的JTC12细胞从其各自的视黄醛前体产生9-顺式视黄酸的效率比全反式视黄酸更高。仅从9-顺式或全反式视黄醛形成了对应相同空间构象的代谢产物,表明JTC12细胞中缺乏可检测到的异构化活性。

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