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枯草芽孢杆菌天冬氨酸转氨甲酰酶基因(pyrB)的克隆与结构

Cloning and structure of the Bacillus subtilis aspartate transcarbamylase gene (pyrB).

作者信息

Lerner C G, Switzer R L

出版信息

J Biol Chem. 1986 Aug 25;261(24):11156-65.

PMID:3015959
Abstract

The Bacillus subtilis gene (pyrB), which encodes aspartate transcarbamylase (ATCase), was cloned on a HindIII restriction endonuclease fragment inserted into the pUC13 plasmid vector. B. subtilis pyrB was expressed in Escherichia coli, as judged by complementation of E. coli pyrB mutants and production of enzyme that was specifically inhibited by antibody directed against B. subtilis ATCase. The extent of expression was strongly dependent on the orientation of the inserted DNA in the vector, which suggested that transcription was initiated from vector-borne (rather than B. subtilis) promoters. The entire 1098-base pair HindIII fragment of B. subtilis DNA was sequenced by the Maxam-Gilbert method. The amino acid sequence of B. subtilis ATCase was deduced from a 305-codon open reading frame and agreed very well with analyses of the purified enzyme. Comparison of the sequence of B. subtilis ATCase with that of E. coli ATCase catalytic subunit, for which the three-dimensional structure is known, revealed many homologous residues of probable importance in catalysis and structural folding of ATCases. The significance of homology to E. coli ornithine transcarbamylases was also analyzed. The sequences of the 5' and 3' flanking regions to pyrB encode open reading frames in both cases which overlap with pyrB by eight and six codons, respectively. It is probable that these open reading frames encode other enzymes of a coordinately regulated unit. The sequence 5' to pyrB also encodes an mRNA bearing a pyrimidine-rich sequence followed by a typical sequence for a rho-independent transcription terminator. The presence of these elements and the 5' open reading frame suggest that B. subtilis pyrB, like E. coli pyrBI, is regulated by an attenuation mechanism.

摘要

编码天冬氨酸转氨甲酰酶(ATCase)的枯草芽孢杆菌基因(pyrB),被克隆到插入pUC13质粒载体的HindIII限制性内切酶片段上。通过对大肠杆菌pyrB突变体的互补作用以及产生被针对枯草芽孢杆菌ATCase的抗体特异性抑制的酶来判断,枯草芽孢杆菌pyrB在大肠杆菌中表达。表达程度强烈依赖于插入载体中的DNA的方向,这表明转录是从载体携带的(而非枯草芽孢杆菌的)启动子起始的。枯草芽孢杆菌DNA的整个1098碱基对的HindIII片段通过Maxam-Gilbert方法进行测序。从一个305密码子的开放阅读框推导出枯草芽孢杆菌ATCase的氨基酸序列,并且与纯化酶的分析结果非常吻合。将枯草芽孢杆菌ATCase的序列与已知三维结构的大肠杆菌ATCase催化亚基的序列进行比较,揭示了许多在ATCase的催化和结构折叠中可能重要的同源残基。还分析了与大肠杆菌鸟氨酸转氨甲酰酶同源性的意义。pyrB两侧5'和3'区域的序列在两种情况下都编码开放阅读框,它们分别与pyrB重叠8个和6个密码子。这些开放阅读框很可能编码一个协同调节单元的其他酶。pyrB 5'端的序列还编码一个带有富含嘧啶序列的mRNA,其后是一个典型的不依赖ρ因子的转录终止子序列。这些元件和5'开放阅读框的存在表明,枯草芽孢杆菌pyrB与大肠杆菌pyrBI一样,受衰减机制调节。

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