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质粒 pFW213 的性质与构建,一种具有口腔链球菌复制起点的穿梭载体。

Properties and construction of plasmid pFW213, a shuttle vector with the oral Streptococcus origin of replication.

机构信息

Department of Microbiology and Immunology, College of Medicine, Chang Gung University, 259 Wen-Hwa 1st Road, Kwei-Shan, Tao-Yuan, Taiwan.

出版信息

Appl Environ Microbiol. 2011 Jun;77(12):3967-74. doi: 10.1128/AEM.02828-10. Epub 2011 Apr 29.

DOI:10.1128/AEM.02828-10
PMID:21531841
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3131664/
Abstract

Streptococcus parasanguinis is among the most successful colonizers of the human body. Strain FW213 harbors a 7.0-kb cryptic plasmid, pFW213, with a copy number at 5 to 10 per chromosome. Sequence and functional analyses of pFW213 revealed that the open reading frame (ORF) encoding the replication protein (Rep) is essential for the replication of pFW213, and the putative plasmid addiction system (RelB and RelE) and an ORF (ORF6) with no known function are required for its stability. The minimal replicon of pFW213 contains the rep gene and its 5'-flanking 390-bp region. Within the minimal replicon, an A/T-rich region followed by 5 contiguous 22-bp repeats was located 5' of the ATG of rep. No single-stranded replication intermediates were detected in the derivatives of pFW213, suggesting that pFW213 replicates via the theta replication mechanism. The minimal replicon was unstable in streptococcal hosts without selection, but the stability was greatly enhanced in derivatives containing the intact relBE genes. A Streptococcus-Escherichia coli shuttle vector, pCG1, was constructed with the pFW213 replicon. Plasmid pCG1 features a multiple cloning region and a spectinomycin resistance determinant that is expressed in both Streptococcus spp. and E. coli. Various streptococcal DNA fragments were cloned in pCG1, and the recombinant constructs were stably maintained in the streptococcal hosts. Since pCG1 is compatible with the most widely used streptococcal replicon, pVA380-1, pCG1 will provide a much needed tool allowing the cloning of two genes that work in concert in the same host.

摘要

副血链球菌是人体最成功的定植菌之一。菌株 FW213 含有一个 7.0kb 的隐秘质粒 pFW213,其拷贝数为每个染色体 5 到 10 个。对 pFW213 的序列和功能分析表明,编码复制蛋白(Rep)的开放阅读框(ORF)对于 pFW213 的复制是必需的,而假定的质粒成瘾系统(RelB 和 RelE)和一个具有未知功能的 ORF(ORF6)对于其稳定性是必需的。pFW213 的最小复制子包含 rep 基因及其 5'-侧翼 390bp 区域。在最小复制子中,位于 rep 的 ATG 上游的是一个 A/T 丰富区域,其后是 5 个连续的 22bp 重复序列。在 pFW213 的衍生物中没有检测到单链复制中间体,这表明 pFW213 通过θ复制机制进行复制。在没有选择的链球菌宿主中,最小复制子不稳定,但在包含完整 relBE 基因的衍生物中,其稳定性大大增强。构建了带有 pFW213 复制子的链球菌-大肠杆菌穿梭载体 pCG1。pCG1 质粒具有一个多克隆区域和一个壮观霉素抗性决定子,该决定子在链球菌属和大肠杆菌中都表达。将各种链球菌 DNA 片段克隆到 pCG1 中,重组构建体在链球菌宿主中稳定维持。由于 pCG1 与最广泛使用的链球菌复制子 pVA380-1 兼容,因此 pCG1 将提供一个急需的工具,允许在同一宿主中协同工作的两个基因的克隆。

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