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构建新型克隆载体,利用八氢番茄红素合成酶基因对嗜热栖热菌克隆 DNA 插入片段进行颜色筛选。

Construction of new cloning vectors that employ the phytoene synthase encoding gene for color screening of cloned DNA inserts in Thermus thermophilus.

机构信息

Health Research Institute, National Institute of Advanced Industrial Science and Technology (AIST), Midorigaoka, Ikeda, Osaka 563-8577, Japan.

出版信息

Gene. 2013 Sep 25;527(2):655-62. doi: 10.1016/j.gene.2013.06.069. Epub 2013 Jul 9.

DOI:10.1016/j.gene.2013.06.069
PMID:23845779
Abstract

Strains of Thermus thermophilus produce unique carotenoids called thermozeaxanthins and their colonies are light-yellow pigmented. Here, we developed a new cloning system allowing for the rapid and convenient detection of recombinants by color screening based on carotenoid production in T. thermophilus. We constructed two cloning vectors that overexpress the crtB gene encoding a phytoene synthase under the strong promoter of the slpA gene. Phytoene synthase is one of essential enzymes for the production of carotenoids. We also isolated a carotenoid-overproducing mutant that formed orange colonies. Because disruption of crtB in the carotenoid-overproducing mutant resulted in white colonies, we used the disruptant as a host strain. Whereas transformants carrying a new cloning vector, pTRK1-PRslpA-crtBcas, grew into unusual red-pigmented colonies probably because of the extreme accumulation of thermozeaxanthins, those carrying the vector with a foreign DNA inserts formed white colonies. Thus, recombinants can be detected easily by color screening (red/white screening) in T. thermophilus. This cloning system requires no additional chromogenic substrate in the medium. We also constructed a promoter-probe vector, pTRK1-crtBmcs-PP, employing the open reading frame of crtB with multiple cloning sites. Using this vector, a series of colony-color phenotypes is observed probably depending on promoter activities of foreign DNA inserts, which enables the rapid probing of promoters. These vectors are useful to simplify cloning procedures and to identify the promoters of different strengths in T. thermophilus.

摘要

嗜热栖热菌产生独特的类胡萝卜素,称为嗜热叶黄素,其菌落呈浅黄色。在这里,我们开发了一种新的克隆系统,通过基于嗜热栖热菌中类胡萝卜素生产的颜色筛选,快速方便地检测重组体。我们构建了两个克隆载体,在 slpA 基因的强启动子下过表达编码八氢番茄红素合酶的 crtB 基因。八氢番茄红素合酶是类胡萝卜素生产的必需酶之一。我们还分离到一个橙色菌落的类胡萝卜素高产突变体。由于在类胡萝卜素高产突变体中敲除 crtB 导致白色菌落,因此我们将该缺陷体用作宿主菌株。而携带新克隆载体 pTRK1-PRslpA-crtBcas 的转化体长成异常的红色着色菌落,可能是由于嗜热叶黄素的极度积累,而携带带有外源 DNA 插入的载体的转化体则形成白色菌落。因此,重组体可以通过颜色筛选(红色/白色筛选)在嗜热栖热菌中轻松检测到。该克隆系统不需要在培养基中添加额外的显色底物。我们还构建了一个启动子探针载体 pTRK1-crtBmcs-PP,该载体利用 crtB 的开放阅读框和多个克隆位点。使用该载体,可以观察到一系列菌落颜色表型,可能取决于外源 DNA 插入的启动子活性,这使得快速探测启动子成为可能。这些载体可用于简化克隆程序,并识别不同强度的嗜热栖热菌启动子。

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