Regulation of purE transcription in a purE::lac fusion strain of Escherichia coli.

机译：大肠杆菌purE :: lac融合菌株中purE转录的调控。

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摘要

A purE::lac fusion strain was isolated by using a special Mu phage developed by M. Casadaban. In the presence of adenine (100 micrograms/ml), beta-galactosidase synthesis was repressed by greater than 90%. beta-Galactosidase activity could be detected 6 to 8 min after the removal of adenine and increased linearly for at least 20 min. purR- mutants were isolated and synthesized 1.7- to 1.8-fold-higher levels of beta-galactosidase compared with purR+ cells. Azaserine derepressed purE transcription approximately 1.7-fold by lowering purine nucleotide pools. Glutamine and pyrimidine supplementation or starvation had no effect on purE transcription. A comparison of the rate of de novo purine biosynthesis and purE transcription indicated that the in vivo rate of de novo purine biosynthesis was more sensitive to the inhibitory effects of adenine than was transcription at the purE locus.

机译：通过使用M. Casadaban开发的特殊Mu噬菌体分离出purE :: lac融合菌株。在腺嘌呤（100微克/毫升）存在下，β-半乳糖苷酶的合成被抑制了90％以上。去除腺嘌呤后6至8分钟可以检测到β-半乳糖苷酶活性，并且线性增加至少20分钟。分离了purR-突变体，与purR +细胞相比，其合成的β-半乳糖苷酶水平高1.7-1.8倍。 Azaserine通过降低嘌呤核苷酸库降低了purE转录约1.7倍。谷氨酰胺和嘧啶的补充或饥饿对purE转录没有影响。从头嘌呤生物合成和purE转录的速率的比较表明，从头体内嘌呤生物合成的体内速率对腺嘌呤的抑制作用比在purE基因座处的转录更加敏感。

著录项

期刊名称 Journal of Bacteriology
作者
R A Levine; M W Taylor;
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作者单位

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年(卷),期 1982(149),3
年度 1982
页码 1041–1049
总页数 9
原文格式 PDF
正文语种
中图分类微生物学;
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机译：使用生物-lac融合菌株研究大肠杆菌中生物素生物合成的调控。
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8. Regulation of purE transcription in a purE::lac fusion strain of Escherichia coli [O] . R A Levine, M W Taylor 1982

机译：纯:: Lac融合应变纯转录的调节大肠杆菌
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机译：“在大肠杆菌结合过程中转移的遗传物质的性质研究。”和“在大肠杆菌中无色素形成色氨酸合成酶的遗传和生化研究”。

Regulation of purE transcription in a purE::lac fusion strain of Escherichia coli.

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