首页> 外文OA文献 >Characterization and mapping of regions encoding clindamycin resistance, tetracycline resistance, and a replication function on the Bacteroides R plasmid pCP1.
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Characterization and mapping of regions encoding clindamycin resistance, tetracycline resistance, and a replication function on the Bacteroides R plasmid pCP1.

机译:在拟杆菌R质粒pCP1上编码克林霉素抗性,四环素抗性和复制功能的区域的表征和作图。

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摘要

The Bacteroides drug resistance plasmid pCP1 encodes clindamycin resistance (Clr) and a cryptic tetracycline resistance (Tcr) determinant that is expressed in Escherichia coli cells grown aerobically, but not anaerobically, and is not expressed phenotypically in Bacteroides spp. Localization of genetic functions on pCP1 was facilitated by the construction of hybrid shuttle plasmids containing portions of pCP1 ligated to pDG5, a pBR322 derivative carrying the RK2 transfer origin. pDP1 delta 4 is a BglII deletion derivative of pCP1 linked to pDG5 and can be maintained in both E. coli and Bacteroides fragilis. By using Tn5 mutagenesis and subcloning, we localized the Clr and Tcr regions on the EcoRI B fragment between the 1.2-kilobase direct repeats of pCP1. The Clr and Tcr determinants are distinct and appear to be transcribed separately. Control of the Tcr phenotype is unusual in that expression is constitutive and is enhanced by a region encompassing the adjacent direct repeat. In addition, a region of pCP1 required for replication in Bacteroides spp. has been identified in the neighboring EcoRI A fragment.
机译:拟杆菌耐药质粒pCP1编码克林霉素抗性(Clr)和隐性四环素抗性(Tcr)决定簇,该决定簇在需氧生长但无厌氧的大肠杆菌细胞中表达,在拟杆菌属中不表型表达。通过构建包含与pDG5(带有RK2转移起点的pBR322衍生物)连接的pCP1部分的杂交穿梭质粒,可以促进遗传功能在pCP1上的定位。 pDP1 delta 4是与pDG5连接的pCP1的BglII缺失衍生物,可同时存在于大肠杆菌和脆弱拟杆菌中。通过使用Tn5诱变和亚克隆,我们在pCP1的1.2碱基对直接重复序列之间的EcoRI B片段上定位了Clr和Tcr区。 Clr和Tcr决定簇是截然不同的,似乎分别转录。 Tcr表型的控制是不寻常的,因为其表达是组成性的,并被包含相邻直接重复序列的区域增强。另外,在拟杆菌中复制需要的pCP1区域。在相邻的EcoRI A片段中已经鉴定出。

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  • 作者

    Matthews, B G; Guiney, D G;

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  • 年度 1986
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  • 原文格式 PDF
  • 正文语种 en
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