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RNA-DIRECTED DNA CLEAVAGE BY THE CAS9-CRRNA COMPLEX

机译:CAS9-CRRNA复合物可进行RNA定向的DNA切割

摘要

Isolation or in vitro assembly of the Cas9-crRNA complex of the Streptococcus thermophilus CRISPR3/Cas system and use for cleavage of DNA bearing a nucleotide sequence complementary to the crRNA and a proto-spacer adjacent motif. Methods for site-specific modification of a target DNA molecule in vitro or in vivo using an RNA-guided DNA endonuclease comprising RNA sequences and at least one of an RuvC active site motif and an HNH active site motif; for conversion of Cas9 polypeptide into a nickase cleaving one strand of double-stranded DNA by inactivating one of the active sites (RuvC or HNH) in the polypeptide by at least one point mutation; for assembly of active polypeptide-polyribonucleotides complex in vivo or in vitro; and for re-programming a Cas9-crRNA complex specificity in vitro and using a cassette containing a single repeat-spacer-repeat unit.
机译:嗜热链球菌CRISPR3 / Cas系统的Cas9-crRNA复合物的分离或体外组装,并用于切割带有与crRNA和proto互补的核苷酸序列的DNA -间隔物相邻的主题。使用包含RNA序列和RuvC活性位点基序和HNH活性位点基序中的至少一个的RNA指导的DNA核酸内切酶在体外或体内对靶DNA分子进行位点特异性修饰的方法;通过至少一个点突变使多肽中的一个活性位点(RuvC或HNH)失活,从而将Cas9多肽转化为切口酶,从而切割一条双链DNA;用于在体内或体外组装活性多肽-多核糖核苷酸复合物;并在体外重新编程Cas9-crRNA复合物特异性,并使用包含单个重复间隔物-重复单元的盒式磁带。

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