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编码锥虫硫醇还原酶的杜氏利什曼原虫基因的结构、组织及表达

The structure, organization, and expression of the Leishmania donovani gene encoding trypanothione reductase.

作者信息

Taylor M C, Kelly J M, Chapman C J, Fairlamb A H, Miles M A

机构信息

Department of Medical Parasitology, London School of Hygiene and Tropical Medicine, UK.

出版信息

Mol Biochem Parasitol. 1994 Apr;64(2):293-301. doi: 10.1016/0166-6851(94)00034-4.

Abstract

Trypanothione reductase (TR) is an NADPH-dependent flavoprotein oxidoreductase central to thiol metabolism in the trypanosomatids. We report here the cloning by expression of the Leishmania donovani gene. It is single copy, expresses a 2.6-kb transcript and a 52-kDa protein and is located on a 1.1-Mbp chromosome. The 491 amino acid sequence has 76% similarity to Crithidia fasciculata and 67% similarity to Trypanosoma cruzi, Trypanosoma congolense and Trypanosoma brucei TR. Residues recognising the adenosine pyrophosphate moiety of NADPH and FAD, and residues in the catalytic site segment (A47-A67) involving electron transfer from TR to trypanothione disulphide (T(S)2) were completely conserved. Thus inhibitors of TR are likely to be active against the enzyme from all the parasitic trypanosomatids. Two peptide inserts (39-47, 131-140) seen in other TR genes and a C-terminal extension of 19 residues were also present. When the gene was introduced back into L. donovani at high copy number using the pTEX expression vector, we detected elevated expression of TR RNA and a 14-fold increase in TR activity. Transfection and overexpression of the TR gene will facilitate studies of gene function and of the dependence of trypanosomatids on TR for protection against oxidative stress.

摘要

锥虫硫醇还原酶(TR)是一种依赖NADPH的黄素蛋白氧化还原酶,在锥虫的硫醇代谢中起核心作用。我们在此报告通过利什曼原虫基因的表达进行克隆。它是单拷贝的,表达一个2.6 kb的转录本和一个52 kDa的蛋白质,位于一条1.1 Mbp的染色体上。491个氨基酸序列与fasiculata克氏锥虫有76%的相似性,与克氏锥虫、刚果锥虫和布氏锥虫TR有67%的相似性。识别NADPH和FAD的腺苷焦磷酸部分的残基,以及催化位点片段(A47 - A67)中涉及从TR到锥虫硫醇二硫化物(T(S)2)电子转移的残基是完全保守的。因此,TR抑制剂可能对所有寄生锥虫的该酶都有活性。在其他TR基因中可见的两个肽插入片段(39 - 47,131 - 140)以及一个19个残基的C末端延伸也存在。当使用pTEX表达载体以高拷贝数将该基因重新导入杜氏利什曼原虫时,我们检测到TR RNA表达升高,TR活性增加了14倍。TR基因的转染和过表达将有助于研究基因功能以及锥虫对TR抵御氧化应激的依赖性。

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