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首页> 外文期刊>Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems >Characterization of a small cryptic plasmid pK50-2 isolated from Lactobacillus reuteri K50
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Characterization of a small cryptic plasmid pK50-2 isolated from Lactobacillus reuteri K50

机译:从罗伊氏乳杆菌K50分离的小型隐性质粒pK50-2的表征

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摘要

The complete nucleotide sequence of a cryptic plasmid, pK50-2, from Lactobacillus reuteri K50 had been determined. It consisted of an 1866. bp circular molecule with a G. +. C content of 35%, from which two putative open reading frames (orfs) could be predicted. Based on sequence similarity, the orf1 was not homologous to any known protein, while the N-terminus of the orf2 shared 56% and 64% identities with RepB proteins of plasmid pAR141 and an unnamed plasmid in L. reuteri strain PA-16, members of the rolling-circle replication (RCR) pMV158 family, respectively. Downstream of orf2, a sequence containing two conserved regions (i.e., bind and nick), possibly involved in the binding and nicking of Rep protein, similar to the dso (double strand origin) of RCR-pMV158 family was also identified. Furthermore, a sequence capable of forming the characteristic secondary structure of ssoT (single-strand origin type T) was subsequently determined upstream of the orf2 gene. Thus, the three elements essential for a RCR plasmid (i.e., dso, sso, and rep gene) were all deducible in the pK50-2. Noteworthy was that a conserved alpha helix-turn-alpha helix (HTH) motif, thus far only seen in theta-type plasmids, was for the first time identified in Rep protein of RCR plasmid, pK50-2. To estimate the pK50-2 could be an expression vector to deliver exogenous antigens, a shuttle vector pK50-S containing both pK50-2 and pUE80 (-) was used to analyze the segregational stability and copy-number, which were shown that pK50-S in L. reuteri DSM 20016 were estimated to be 98%, 77%, and 75% after 36, 72, and 100 generations and about 50 copies per chromosome equivalent by real-time PCR.
机译:已经确定了来自罗伊氏乳杆菌K50的密码质粒pK50-2的完整核苷酸序列。它由一个带G. +的1866 bp环状分子组成。 C含量为35%,由此可以预测两个推定的开放阅读框(orfs)。基于序列相似性,orf1与任何已知蛋白都不同源,而orf2的N端与罗伊氏乳杆菌菌株PA-16中的质粒pAR141和一个未命名质粒的RepB蛋白共享56%和64%的同一性,分别为滚环复制(RCR)pMV158系列。在orf2的下游,还发现了一个包含两个保守区域(即结合和切口)的序列,可能与Rep蛋白的结合和切口有关,类似于RCR-pMV158家族的dso(双链起源)。此外,随后在orf2基因的上游确定了能够形成ssoT的特征性二级结构(单链起源类型T)的序列。因此,在pK50-2中可以推断出RCR质粒必需的三个要素(即dso,sso和rep基因)。值得注意的是,迄今仅在θ型质粒中可见的保守α螺旋-转-α螺旋(HTH)基序首次在RCR质粒pK50-2的Rep蛋白中鉴定。为了评估pK50-2可能是传递外源抗原的表达载体,使用同时包含pK50-2和pUE80(-)的穿梭载体pK50-S分析了分离稳定性和拷贝数,结果表明pK50-通过实时PCR,在36、72和100代后,罗伊氏乳杆菌DSM 20016中的S估计为98%,77%和75%,每条染色体当量约50个拷贝。

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