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A combined in vitro / in vivo selection for polymerases with novel promoter specificities

机译:具有新颖启动子特异性的聚合酶的体外/体内联合选择

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摘要

BackgroundThe DNA-dependent RNA polymerase from T7 bacteriophage (T7 RNAP) has been extensively characterized, and like other phage RNA polymerases it is highly specific for its promoter. A combined in vitro / in vivo selection method has been developed for the evolution of T7 RNA polymerases with altered promoter specificities. Large (103 – 106) polymerase libraries were made and cloned downstream of variant promoters. Those polymerase variants that can recognize variant promoters self-amplify both themselves and their attendent mRNAs in vivo. Following RT / PCR amplification in vitro, the most numerous polymerase genes are preferentially cloned and carried into subsequent rounds of selection.
机译:背景技术已经广泛表征了来自T7噬菌体的DNA依赖性RNA聚合酶(T7 RNAP),并且像其他噬菌体RNA聚合酶一样,它对启动子具有高度特异性。已经开发了一种组合的体外/体内选择方法,用于进化具有改变的启动子特异性的T7 RNA聚合酶。制作了大的(10 3 – 10 6 )聚合酶文库,并将其克隆到变体启动子的下游。那些能够识别变体启动子的聚合酶变体会在体内自我扩增自身及其伴随的mRNA。在体外RT / PCR扩增后,优先克隆最多的聚合酶基因,并进行随后的选择。

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