Boyce Thompson Institute for Plant Research, Cornell University, Ithaca, NY 14853.
Proc Natl Acad Sci U S A. 1986 Dec;83(23):9080-4. doi: 10.1073/pnas.83.23.9080.
Two plasmid vectors pFIT001 and pPALE001, containing luxAB genes encoding bacterial luciferase [alkanal, reduced-FMN:oxygen oxidoreductase (1-hydroxylating, luminescing), EC 1.14.14.3] from Vibrio harveyi, have been constructed. Escherichia coli carrying derivatives of pFIT001 with DNA inserts in the unique EcoRI site located in luxB form "dark" colonies that can be readily distinguished from the bioluminescent or "bright" colonies. In contrast, promoterless pPALE001 is used as a promoter-search vector based on bioluminescence. The control and regulation of gene expression can be analyzed in vivo using promoter-luxAB fusions by a variety of simple methods, including a technique called "luxdot." As an example, we have introduced nitrogenase nifD and nifH promoter-luxAB fusions into the Bradyrhizobium japonicum chromosome and shown symbiotically regulated bioluminescence in soybean root nodules. B. japonicum transconjugants containing a single copy per genome of the nif promoter-controlled luciferase structural genes did not produce light in free-living cultures, but the same transconjugants did express bioluminescence in root nodules that was strong enough to be detected by the naked eye.
构建了两个质粒载体 pFIT001 和 pPALE001,它们含有来自 Harveyi 弧菌的 luxAB 基因,编码细菌荧光素酶[烷醇,还原-FMN:氧氧化还原酶(1-羟基化,发光),EC 1.14.14.3]。携带 pFIT001 衍生物的大肠杆菌,其 DNA 插入物位于 luxB 中的独特 EcoRI 位点,形成“暗”菌落,与生物发光或“亮”菌落很容易区分。相比之下,无启动子的 pPALE001 可作为基于生物发光的启动子搜索载体。通过多种简单方法,包括一种称为“luxdot”的技术,可在体内分析基因表达的控制和调节。作为一个例子,我们将固氮酶 nifD 和 nifH 启动子-luxAB 融合引入大豆根瘤中的日本根瘤菌染色体,并显示出共生调节的生物发光。含有单个基因组拷贝的 nif 启动子控制的荧光素酶结构基因的 B. japonicum 转导子在自由生活培养物中不发光,但相同的转导子在根瘤中表达的生物发光足够强,可以用肉眼检测到。
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