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大鼠血红素加氧酶在大肠杆菌中的表达形式为具有催化活性的全长形式,且能与细菌膜结合。

Expression of rat heme oxygenase in Escherichia coli as a catalytically active, full-length form that binds to bacterial membranes.

作者信息

Ishikawa K, Sato M, Yoshida T

机构信息

Department of Molecular and Pathological Biochemistry, Yamagata University School of Medicine, Japan.

出版信息

Eur J Biochem. 1991 Nov 15;202(1):161-5. doi: 10.1111/j.1432-1033.1991.tb16357.x.

Abstract

A plasmid, pKK-RHO, was constructed by incorporating the coding sequence of a cDNA for rat heme oxygenase into the expression vector pKK233-2. Escherichia coli strain XL1-blue transformed with pKK-RHO produced a catalytically active, full-length heme oxygenase. The 32-kDa native enzyme expressed, was localized in the bacterial membranes, possibly due to the spontaneous membrane-binding properties of a hydrophobic segment in its C-terminal region. During cultivation, a few degraded forms of heme oxygenase that had lost their membrane-associative properties appeared. Probably, some bacterial proteases cut the native heme oxygenase at sites near its C-terminus and so release hydrophilic peptides of heme oxygenase from the membranes. A 30-kDa polypeptide, one of the degraded forms of heme oxygenase, retained ability to accept electrons from NADPH--cytochrome P450 reductase and also activity for catalyzing breakdown of heme to biliverdin. The cultured cells were pale green. From them we extracted green pigment(s), of which the absorption spectrum closely resembled that of biliverdin, suggesting that a large amount of the endogenous heme of E. coli was actually degraded to biliverdin by the expressed heme oxygenase.

摘要

通过将大鼠血红素加氧酶的cDNA编码序列整合到表达载体pKK233-2中构建了质粒pKK-RHO。用pKK-RHO转化的大肠杆菌XL1-blue菌株产生了具有催化活性的全长血红素加氧酶。所表达的32 kDa天然酶定位于细菌膜中,这可能是由于其C末端区域中疏水片段的自发膜结合特性所致。在培养过程中,出现了一些失去膜结合特性的血红素加氧酶降解形式。可能是一些细菌蛋白酶在其C末端附近的位点切割天然血红素加氧酶,从而从膜上释放出血红素加氧酶的亲水肽。30 kDa多肽是血红素加氧酶的降解形式之一,它保留了从NADPH-细胞色素P450还原酶接受电子的能力,以及催化血红素分解为胆绿素的活性。培养的细胞呈淡绿色。我们从它们中提取了绿色色素,其吸收光谱与胆绿素的吸收光谱非常相似,这表明大肠杆菌的大量内源性血红素实际上被表达的血红素加氧酶降解为胆绿素。

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