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Use of bacterial luciferase to establish a promoter probe vehicle capable of nondestructive real-time analysis of gene expression in Bacillus spp.

机译:使用细菌荧光素酶建立能够对芽孢杆菌属基因表达进行非破坏性实时分析的启动子探针载体。

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摘要

We report the construction and use of a new promoter probe vehicle capable of allowing extremely sensitive measurements of transcriptional activity promoted from random, chromosomal DNA fragment inserts. Coupled with the advantage of sensitivity, the detection system is noninvasive, nondestructive, and provides real-time reportage of expression potential. These latter aspects make it an especially valuable system for a continuing analysis of the complex transcriptional regulation patterns now recognized as a dominant control feature during the differentiation and morphogenesis characteristic of the sporulation cycle in Bacillus species. In this respect we describe the isolation of DNA fragments from B. megaterium and B. subtilis capable of initiating transcription in both the respective parent organisms and, in certain instances, also in Escherichia coli. Detailed luminescence studies showed that several promoter regions which are entirely or substantially developmentally controlled were isolated.
机译:我们报告了一种新型启动子探针载体的构建和使用,该载体能够对来自随机,染色体DNA片段插入片段的转录活性进行极其灵敏的测量。加上灵敏度高的优势,该检测系统是无创,无损的,并提供表达潜力的实时报告。后面的这些方面使它成为一个特别有价值的系统,用于继续分析复杂的转录调控模式,这些模式现在已被认为是芽孢杆菌属物种芽孢形成周期的分化和形态发生特征中的主要控制特征。在这方面,我们描述了从巨大芽孢杆菌和枯草芽孢杆菌分离DNA片段的方法,该片段能够在各自的亲代生物体中以及在某些情况下也在大肠杆菌中引发转录。详细的发光研究表明,分离了几个完全或基本受发育控制的启动子区域。

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