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The pyrimidine biosynthesis operon of the thermophile Bacillus caldolyticus includes genes for uracil phosphoribosyltransferase and uracil permease.

机译:嗜热芽孢杆菌的嘧啶生物合成操纵子包括尿嘧啶磷酸核糖基转移酶和尿嘧啶通透酶的基因。

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摘要

A 3-kb DNA segment of the Bacillus caldolyticus genome including the 5' end end of the pyr cluster has been cloned and sequenced. The sequence revealed the presence of two open reading frames, pyrR and pyrP, located immediately upstream of the previously sequenced pyrB gene encoding the pyrimidine biosynthesis enzyme aspartate transcarbamoylase. The pyrR and pyrP genes encoded polypeptides with calculated molecular masses of 19.9 and 45.2 kDa, respectively. Expression of these ORFs was confirmed by analysis of plasmid-encoded polypeptides in minicells. Sequence alignment and complementation analyses identified the pyrR gene product as a uracil phosphoribosyltransferase and the pyrP gene product as a membrane-bound uracil permease. By using promoter expression vectors, a 650-bp EcoRI-HincII fragment, including the 5' end of pyrR and its upstream region, was found to contain the pyr operon promoter. The transcriptional start point was located by primer extension at a position 153 bp upstream of the pyrR translation initiation codon, 7 bp 3' of a sequence resembling a sigma A-dependent Bacillus subtilis promoter. This established the following organization of the ten cistrons within the pyr operon: promoter-pyrR-pyrP-pyrB-pyrC-pyrAa-pyrA b-orf2-pyrD-pyrF-pyrE. The nucleotide sequences of the region upstream of pyrR and of the pyrR-pyrP and pyrP-pyrB intercistronic regions indicated that the transcript may form two mutually exclusive secondary structures within each of these regions. One of these structures resembled a rho-independent transcriptional terminator. The possible implication of these structures for pyrimidine regulation of the operon is discussed.
机译:已经克隆了解热芽孢杆菌基因组的3-kb DNA片段,包括pyr簇的5'末端。该序列显示存在两个开放阅读框pyrR和pyrP,它们位于编码嘧啶生物合成酶天冬氨酸转氨甲酰酶的先前测序的pyrB基因的紧邻上游。 pyrR和pyrP基因编码的多肽,其分子量分别为19.9和45.2 kDa。通过分析小细胞中质粒编码的多肽,证实了这些ORF的表达。序列比对和互补分析鉴定出pyrR基因产物为尿嘧啶磷酸核糖基转移酶,而pyrP基因产物为膜结合尿嘧啶通透酶。通过使用启动子表达载体,发现一个包含pyrR 5'端及其上游区域的650 bp EcoRI-HincII片段含有pyr操纵子启动子。转录起始点通过引物延伸定位在pyrR翻译起始密码子上游153 bp处,类似于σA依赖性枯草芽孢杆菌启动子的序列的7 bp 3'。这在pyr操纵子内建立了十个顺反子的以下组织:启动子-pyrR-pyrP-pyrB-pyrC-pyrAa-pyrA b-orf2-pyrD-pyrF-pyrE。在pyrR上游以及pyrR-pyrP和pyrP-pyrB间顺反子区域的上游的核苷酸序列表明,转录物可以在这些区域的每一个内形成两个互斥的二级结构。这些结构之一类似于不依赖rho的转录终止子。讨论了这些结构对操纵子的嘧啶调节的可能含义。

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  • 作者

    Ghim, S Y; Neuhard, J;

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  • 年度 1994
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  • 原文格式 PDF
  • 正文语种 en
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