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Bacteriophage lambda and plasmid vectors, allowing fusion of cloned genes in each of the three translational phases

机译:噬菌体λ和质粒载体,可在三个翻译阶段的每个阶段融合克隆的基因

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We have constructed vectors from bacteriophage lambda and from plasmid pBR322 having a single EcoRI restriction site which is immediatly downstream from the lac UV5 promotor. Each vector allows the fusion of a cloned gene to the lac Z gene in a different phase relative to the translation initiation codon of the lac Z gene. These vectors were constructed through modification of the initial EcoRI restriction site by S1 endonuclease treatment and then addition of octadeoxyribonucleotides (EcoRI linkers) , which shifted the restriction site by 2 or 4 nucleotides. Used in combination these vectors should allow translation of a cloned gene in any one of the three coding phases. The bacteriophages vectors are certified as B2 (EK2) safety level vectors by the French “recombinaison génétique in vitro” committee (D.G.R.S.T.).
机译:我们从噬菌体λ和质粒pBR322构建了载体,质粒pBR322具有单个EcoRI限制位点,该位点直接位于lac UV5 启动子的下游。每个载体都允许在相对于lac Z基因翻译起始密码子不同的阶段将克隆的基因与lac Z基因融合。这些载体是通过S1核酸内切酶处理修饰了最初的EcoRI限制性酶切位点,然后添加十八烷氧基核糖核苷酸(EcoRI接头)而构建的,该位点使限制性酶切位点移位了2个或4个核苷酸。这些载体组合使用时,应允许在三个编码阶段的任何一个中克隆基因的翻译。噬菌体载体被法国“体外重组基因”委员会(D.G.R.S.T.)认证为B2(EK2)安全水平载体。

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