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FLUORESCENCE-BASED REPORTERS FOR MUTAGENESIS DETECTION IN E. COLI

机译:基于荧光的大肠杆菌中致突变检测报告

摘要

Direct detection of mutagenesis in prokaryotes by reversion of an inactivating mutation (reversion mutation assay), producing a quantitative signal for in vivo mutagenesis, may greatly reduce the amount of test chemicals and labor involved in these assays. Further, transcriptional coupling of β-lactamase reversion and GFP, translational fusion between β-lactamase and GFP with stop codon in GFP, and a novel dual reporter to monitor continuous mutagenesis may be used in methods described herein.
机译:通过失活突变的回复(回复突变测定)直接检测原核生物中的诱变,产生体内诱变的定量信号,可以大大减少这些测定中涉及的测试化学品和工作量。此外,可以在本文所述的方法中使用β-内酰胺酶回复和GFP的转录偶联,β-内酰胺酶和GFP之间的翻译融合以及GFP中的终止密码子,以及用于监测连续诱变的新型双重报告基因。

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