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大鼠肾脏胆绿素还原酶cDNA的表达与特性分析。有证据表明肝脏和肾脏中的该酶是同一转录产物。

Expression and characterization of a cDNA for rat kidney biliverdin reductase. Evidence suggesting the liver and kidney enzymes are the same transcript product.

作者信息

Fakhrai H, Maines M D

机构信息

Department of Biophysics, University of Rochester School of Medicine, New York 14642.

出版信息

J Biol Chem. 1992 Feb 25;267(6):4023-9.

PMID:1371282
Abstract

Biliverdin reductase is a unique dual cofactor- and pH-dependent enzyme that converts biliverdin to bilirubin and displays extensive inter-organ pI and molecular weight microheterogeneity. Presently we have explored the molecular basis for these properties. The amino acid composition and the sequences of NH2 termini plus five tryptic fragments of purified rat liver and kidney enzymes were obtained. A 62-nucleotide DNA probe was designed and in combination with antibody was used to screen a rat kidney cDNA library. A cDNA sequence of 1108 base pairs (bp) containing an 885-bp open reading frame was generated. The cloned cDNA probe detected a single mRNA of approximately 1500 bp in liver and kidney. The open reading frame encodes a 295 amino acid protein. Methionine and aspartic acid residues at positions 1 and 2 of the deduced protein are removed during processing. The deduced amino acid composition of the mature protein closely matched that of the purified rat liver and kidney enzymes. All liver peptides were found in the deduced amino acid sequence of kidney enzyme and the NH2 termini of both enzymes were identical. The expressed protein co-migrated with purified reductase and was recognized by antiserum to the enzyme. The expressed reductase displayed two distinct pH optima using a different cofactor at each pH: NADH at the lower pH 6.7-6.9 range and NADPH at pH 8.5-8.7. The findings suggest that the liver and kidney enzymes are the products of the same transcript(s) and that their microheterogeneity may reflect tissue-specific post-translational modifications.

摘要

胆绿素还原酶是一种独特的双辅助因子和pH依赖性酶,可将胆绿素转化为胆红素,并表现出广泛的器官间等电点和分子量微不均一性。目前我们已经探究了这些特性的分子基础。获得了纯化的大鼠肝脏和肾脏酶的氨基酸组成以及氨基末端序列和五个胰蛋白酶片段的序列。设计了一个62个核苷酸的DNA探针,并与抗体结合用于筛选大鼠肾脏cDNA文库。生成了一个1108个碱基对(bp)的cDNA序列,其中包含一个885bp的开放阅读框。克隆的cDNA探针在肝脏和肾脏中检测到一条约1500bp的单一mRNA。开放阅读框编码一个295个氨基酸的蛋白质。在加工过程中,推导蛋白质第1和第2位的甲硫氨酸和天冬氨酸残基被去除。成熟蛋白质推导的氨基酸组成与纯化的大鼠肝脏和肾脏酶的氨基酸组成紧密匹配。在肾脏酶推导的氨基酸序列中发现了所有肝脏肽段,并且两种酶的氨基末端相同。表达的蛋白质与纯化的还原酶共迁移,并被该酶的抗血清识别。使用不同的辅助因子时,表达的还原酶在每个pH值下显示出两个不同的最适pH值:在较低的pH 6.7 - 6.9范围内为NADH,在pH 8.5 - 8.7时为NADPH。这些发现表明肝脏和肾脏中的酶是同一转录本的产物,并且它们的微不均一性可能反映了组织特异性的翻译后修饰。

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