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编码人肝脏开蓬还原酶的克隆cDNA的分离与鉴定

Isolation and characterization of cloned cDNAs encoding human liver chlordecone reductase.

作者信息

Winters C J, Molowa D T, Guzelian P S

机构信息

Department of Medicine, Medical College of Virginia, Richmond 23298.

出版信息

Biochemistry. 1990 Jan 30;29(4):1080-7. doi: 10.1021/bi00456a034.

Abstract

Chlordecone (Kepone), a toxic organochlorine pesticide, undergoes bioreduction to chlordecone alcohol in human liver. This reaction is controlled by a cytosolic enzyme, chlordecone reductase (CDR), which may be of the aldo-keto reductase family of xenobiotic metabolizing enzymes [Molowa et al. (1986) J. Biol. Chem. 261, 12624-12627]. To further investigate the primary structure and expression of CDR, we screened a library of human liver cDNAs cloned in the expression vector lambda gt11 and isolated an 800 bp cDNA that directed synthesis of a fusion protein recognized by polyclonal anti-CDR antibodies. Using this cDNA as a probe, we screened two human liver cDNA libraries and found several 1.2-kb cDNAs which would code for a polypeptide with 308 residues (35.8 kDa). However, a similar full-length cDNA, possibly the transcript of a pseudogene, contained an in-frame nonsense codon. The deduced protein sequence of CDR showed 65% similarity to the primary structure of human liver aldehyde reductase and 66% similarity to the inferred protein sequence of rat lens aldose reductase. A search of GenBank revealed significant nucleotide similarity to a cDNA coding for bovine lung prostaglandin f synthase and to a partial cDNA coding for frog lens rho-crystallin. Southern blot analysis of human genomic DNA displayed between 45 and 65 kilobases of DNA hybridizable to CDR cDNA and demonstrated several restriction fragment length polymorphisms among 26 individuals. Northern blot analysis of RNA from human, gerbil, rabbit, hamster, mouse, and rat livers disclosed hybridization with CDR cDNA only for the first three species.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

开蓬(十氯酮)是一种有毒的有机氯农药,在人肝脏中会通过生物还原作用转化为开蓬醇。该反应由一种胞质酶——开蓬还原酶(CDR)控制,CDR可能属于外源性物质代谢酶的醛酮还原酶家族[莫洛瓦等人(1986年)《生物化学杂志》261卷,12624 - 12627页]。为了进一步研究CDR的一级结构和表达情况,我们筛选了克隆于表达载体λgt11的人肝脏cDNA文库,分离出一个800 bp的cDNA,它能指导合成一种可被多克隆抗CDR抗体识别的融合蛋白。以该cDNA为探针,我们筛选了两个人肝脏cDNA文库,发现了几个1.2 kb的cDNA,它们编码的多肽含有308个氨基酸残基(35.8 kDa)。然而,一个类似的全长cDNA,可能是假基因的转录本,含有一个框内无义密码子。CDR推导的蛋白质序列与人类肝脏醛还原酶的一级结构有65%的相似性,与大鼠晶状体醛糖还原酶推导的蛋白质序列有66%的相似性。在GenBank中搜索发现,它与编码牛肺前列腺素f合酶的cDNA以及编码蛙晶状体rho - 晶体蛋白的部分cDNA有显著的核苷酸相似性。对人类基因组DNA的Southern印迹分析显示,有45至65千碱基的DNA可与CDR cDNA杂交,并在26个个体中显示出几种限制性片段长度多态性。对来自人、沙鼠、兔、仓鼠、小鼠和大鼠肝脏的RNA进行Northern印迹分析,结果显示仅前三个物种的RNA与CDR cDNA杂交。(摘要截短于250字)

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