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新型载体系统可随机、单步将多个 DNA 拷贝整合到红球菌基因组中。

New vector system for random, single-step integration of multiple copies of DNA into the Rhodococcus genome.

机构信息

Department of Food Hygiene and Control, Faculty of Veterinary Medicine, Mansoura University, Mansoura, Egypt.

出版信息

Appl Environ Microbiol. 2010 Apr;76(8):2531-9. doi: 10.1128/AEM.02131-09. Epub 2010 Feb 12.

Abstract

We designed a new vector system for creating a random mutant library with multiple integrations of DNA fragments into the Rhodococcus genome in a single step. For this, we cotransformed two vectors into Rhodococcus by electroporation: pTip-istAB-sacB regulates the expression of the transposase (IstA) and its helper protein (IstB) under the influence of a thiostrepton-inducible promoter, and pRTSK-sacB provides the transposable-marker DNA. Both are multicopy vectors that are stable in the host cells; transposition of the transposable-marker DNA occurs only after the induction of IstA/IstB expression. With the addition of thiostrepton, all cultured cells harboring the two vectors, irrespective of the volume, can be mutated by random insertion of the transposable-marker DNA into their genome. Among the generated mutants examined, 30% showed multiple (two to five) insertion copies. The multiple integrated DNA copies were stable in the genome for more than 80 generations of serial growth without the addition of any selective antibiotics. This system can also be used for integrating various copy numbers of stably maintained protein expression cassettes in the host cell genome to modulate the expression level of biologically active recombinant proteins. We successfully applied this system to integrate multiple copies of expression cassettes for proline iminopeptidase and vitamin D(3) hydroxylase into the Rhodococcus genome and verified that the clones containing double or multiple copies of the integrated cassettes produced higher levels and showed higher enzymatic activities of the target protein than clones with only a single copy of integration.

摘要

我们设计了一种新的载体系统,用于在单个步骤中将多个 DNA 片段随机整合到罗德里格斯氏菌基因组中,从而创建一个随机突变文库。为此,我们通过电穿孔将两个载体共转化到罗德里格斯氏菌中:pTip-istAB-sacB 在硫链丝菌素诱导型启动子的影响下调节转座酶(IstA)及其辅助蛋白(IstB)的表达,而 pRTSK-sacB 提供可转座标记 DNA。这两个载体都是多拷贝载体,在宿主细胞中稳定;只有在 IstA/IstB 表达被诱导后,可转座标记 DNA 才会发生转座。加入硫链丝菌素后,无论体积大小,所有含有这两个载体的培养细胞都可以通过可转座标记 DNA 随机插入其基因组而发生突变。在所检查的突变体中,有 30%表现出多个(两个到五个)插入拷贝。在没有添加任何选择性抗生素的情况下,多个整合的 DNA 拷贝在基因组中稳定存在超过 80 代的连续生长。该系统还可用于将各种拷贝数的稳定维持的蛋白质表达盒整合到宿主细胞基因组中,以调节生物活性重组蛋白的表达水平。我们成功地将脯氨酸亚氨基肽酶和维生素 D(3)羟化酶的表达盒的多个拷贝应用于该系统,并证实含有整合盒的双拷贝或多拷贝的克隆比只有单拷贝整合的克隆产生更高水平的目标蛋白,并显示出更高的酶活性。

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