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Characterization of pURB500 from the archaeon Methanococcus maripaludis and construction of a shuttle vector.

机译:从古细菌甲烷球菌中鉴定pURB500,并构建穿梭载体。

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摘要

The complete sequence of the 8,285-bp plasmid pURB500 from Methanococcus maripaludis C5 was determined. Sequence analysis identified 18 open reading frames as well as two regions of potential iterons and complex secondary structures. The shuttle vector, pDLT44, for M. maripaludis JJ was constructed from the entire pURB500 plasmid and pMEB.2, an Escherichia coli vector containing a methanococcal puromycin-resistance marker (P. Gernhardt, O. Possot, M. Foglino, L. Sibold, and A. Klein, Mol. Gen. Genet. 221:273-279, 1990). By using polyethylene glycol transformation, M. maripaludis JJ was transformed at a frequency of 3.3 x 10(7) transformants per microg of pDLT44. The shuttle vector was stable in E. coli under ampicillin selection but was maintained at a lower copy number than pMEB.2. Based on the inability of various restriction fragments of pURB500 to support maintenance in M. maripaludis JJ, multiple regions of pURB500 were required. pDLT44 did not replicate in Methanococcus voltae.
机译:确定了来自马氏甲烷球菌C5的8,285-bp质粒pURB500的完整序列。序列分析确定了18个开放阅读框以及两个潜在的迭代子和复杂的二级结构区域。 maripaludis JJ的穿梭载体pDLT44由完整的pURB500质粒和pMEB.2构建而成,pMEB.2是一种含有耐甲氧球菌嘌呤霉素标记的大肠杆菌载体(P. Gernhardt,O。Possot,M。Foglino,L。Sibold ,和A. Klein,分子遗传学杂志221:273-279,1990)。通过使用聚乙二醇转化,M。maripaludis JJ以每微克pDLT44 3.3 x 10(7)个转化子的频率转化。在氨苄青霉素选择下,穿梭载体在大肠杆菌中是稳定的,但维持在比pMEB.2更低的拷贝数上。基于pURB500的各种限制性片段无法支持M. maripaludis JJ的维护,需要pURB500的多个区域。 pDLT44在伏地甲烷球菌中不复制。

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