枯草芽孢杆菌udp -葡萄糖焦磷酸化酶结构基因gtaB的序列分析。

B Soldo, V Lazarevic, P Margot, D Karamata
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引用次数: 42

摘要

核苷酸测序结果显示,udp -葡萄糖焦磷酸化酶(EC 2.7.7.9)的结构基因gtaB是一个分叉样遗传实体的一部分。后者由两个单顺反子操纵子gtaB和orfX组成,分别从245 bp的调控区转录,分别编码一个分子质量为33.0和42.6 kDa的酸性蛋白。gtaB转录自远端PA启动子和近端PB启动子,后者由Sin蛋白负调控。sin介导的PB和PD的转录减弱和增强表明这两个启动子控制着相互拮抗的功能。orfX的转录是由PA启动子介导的。调控区包括四个ATGAAA六聚体,以两个逆重复出现。蛋白质GtaB与类似的原核酶具有高度的同源性,而OrfX与大肠杆菌o389的产物具有55.4%的同源性,后者是参与糖加工的调节单元的一部分。对定义不同噬菌体吸附模式的突变gtaB515和gtaBg100进行了测序。它们是导致占据保守位置的氨基酸取代的过渡,因此可能是酶活性位点的一部分。讨论了缺陷噬菌体的可能受体PBSY和PBSZ的性质。
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Sequencing and analysis of the divergon comprising gtaB, the structural gene of UDP-glucose pyrophosphorylase of Bacillus subtilis 168.

Nucleotide sequencing revealed that gtaB, the structural gene of UDP-glucose pyrophosphorylase (EC 2.7.7.9), is part of a divergon-like genetic entity. The latter consists of two monocistronic operons gtaB and orfX, transcribed from a 245 bp regulatory region, each encoding an acidic protein with a molecular mass of 33.0 and 42.6 kDa, respectively. gtaB is transcribed from a distal PA promoter, and a proximal PB promoter which is negatively controlled by the Sin protein. Sin-mediated transcriptional attenuation and enhancement of PB and PD, respectively, suggest that these promoters control functions which antagonize each other. Transcription of orfX is mediated by a PA promoter. The regulatory region comprises four ATGAAA hexamers, present as two inverse repeats. Protein GtaB exhibits high homology to analogous prokaryotic enzymes, while OrfX shows 55.4% homology with the product of Escherichia coli o389, which is part of a regulatory unit involved in sugar processing. Mutations gtaB515 and gtaBg100, which define different bacteriophage adsorption patterns, were sequenced. They are transitions leading to substitution of amino acids which occupy conserved positions, and are thus likely to be part of an enzyme active site. The nature of the possible receptors for defective bacteriophages PBSY and PBSZ is discussed.

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