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虹鳟(Oncorhynchus mykiss)诱导型一氧化氮合酶(iNOS)基因的分子克隆、基因结构及表达

Molecular cloning, gene organization and expression of rainbow trout (Oncorhynchus mykiss) inducible nitric oxide synthase (iNOS) gene.

作者信息

Wang T, Ward M, Grabowski P, Secombes C J

机构信息

Department of Zoology, University of Aberdeen, Aberdeen AB24 2TZ, UK.

出版信息

Biochem J. 2001 Sep 15;358(Pt 3):747-55. doi: 10.1042/0264-6021:3580747.

Abstract

A full-length inducible nitric oxide synthase (iNOS) gene has been sequenced for the first time outside the mammals, and the gene organization compared with that already determined for human iNOS. While there are some differences from the human gene, overall the exons show remarkable conservation in sequence and organization. As in human, the trout iNOS gene has 27 exons, with 18 of the trout exons being identical in size with the equivalent human exons. The cofactor-binding domains are found in the same exons and in some cases are absolutely conserved. Differences include the start of the ORF in exon 3 instead of exon 2, resulting in a deletion at the 5' end of the trout iNOS protein. Exon 27 also shows a large difference in size and although the trout exon is larger this is due to the length of the 3'-UTR. Several non-mammalian features are notable, and include a conserved potential glycosylation site in chicken and fish, and an insertion at the boundary of exons 20 and 21 in fish. The intron sizes in trout were generally much smaller than in human iNOS, making the trout iNOS gene approximately half the size of the human gene. Analysis of RNA secondary structure revealed two regions with complementarity, which could interfere with reverse transcription. Using a trout fibroblast cell line (RTG-2 cells), it was shown by reverse transcriptase (RT)-PCR that virus infection was a good inducer of iNOS expression. However, when using a combination of Superscripttrade mark II for reverse transcription and primers at the 5' end of the gene only very weak products were amplified, in contrast with the situation when primers at the 3' end of the gene were used, or ThermoScripttrade mark-derived cDNA was used. The impact of such results on RT-PCR analysis of iNOS expression in trout is discussed.

摘要

首次在哺乳动物以外的物种中对全长诱导型一氧化氮合酶(iNOS)基因进行了测序,并将该基因结构与已确定的人类iNOS基因结构进行了比较。虽然与人类基因存在一些差异,但总体而言,外显子在序列和结构上表现出显著的保守性。与人类一样,虹鳟鱼iNOS基因有27个外显子,其中18个虹鳟鱼外显子与相应的人类外显子大小相同。辅因子结合域位于相同的外显子中,在某些情况下是绝对保守的。差异包括开放阅读框(ORF)起始于外显子3而非外显子2,导致虹鳟鱼iNOS蛋白5'端出现缺失。外显子27在大小上也有很大差异,尽管虹鳟鱼外显子较大,但这是由于3'-非翻译区(3'-UTR)的长度所致。几个非哺乳动物的特征值得注意,包括鸡和鱼中一个保守的潜在糖基化位点,以及鱼中外显子20和21边界处的一个插入。虹鳟鱼的内含子大小通常比人类iNOS中的小得多,使得虹鳟鱼iNOS基因大小约为人类基因的一半。RNA二级结构分析揭示了两个具有互补性的区域,这可能会干扰逆转录。使用虹鳟鱼成纤维细胞系(RTG-2细胞),通过逆转录酶(RT)-PCR表明病毒感染是iNOS表达的良好诱导剂。然而,当使用Superscript™ II进行逆转录并仅使用基因5'端的引物时,仅扩增出非常弱的产物,这与使用基因3'端的引物或ThermoScript™衍生的cDNA时的情况形成对比。讨论了这些结果对虹鳟鱼iNOS表达的RT-PCR分析的影响。

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