基于CRISPR/neneneba CAS系统的基因组编辑:基因操作和遗传新时代的开始

J. S. Toledo
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引用次数: 0

摘要

2002年,乌得勒支大学的Ruud Jansen发现了21-37 bp的间隔短序列重复序列,在几种细菌中明显间隔,如鼠伤寒沙门氏菌(21bp)和化脓性链球菌(37bp)。Jansen的研究小组发现,crispr是某些原核生物所特有的,而不是病毒和真核生物。此外,他们在末端发现了一个共同序列GTT/AAC,在上游发现了一个没有开放阅读框的长同源序列,表明这是一个保守的ncRNA片段。他们的发现与Ishino和Mojica的发现相似,他们将这种现象称为聚集规则间隔短回文重复序列(CRISPR)。CRISPR的生物学意义一直不清楚,直到2005年,Pourcel、Mojica和Bolotin分别得出结论,CRISPR显然来自染色体外的DNA元件,其中大多数类似于噬菌体和质粒。值得注意的是,含有CRISPR元素的物种能够抵御相应的外来入侵者,并且没有残留的前噬菌体作为先前感染的证据
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Genome editing based on CRISPR/CAS systems: beginning of a new era of genetic manipulation and inheritance
In 2002, Ruud Jansen of Utrecht University found a 21-37 bp interspaced short sequence repeats distinctly spaced among several bacterial species, such as, Salmonella typhimurium (21bp) and Streptococcus pyogenes (37bp). Jansen’s team found that CRISPRs were unique to certain prokaryotes and not viruses and eukaryotes. Moreover, they identified a common sequence, GTT/AAC, at the ends and a long homologous sequence along the upstream without an open reading frame, indicating a conserved ncRNA segment. Their findings were similar to that of Ishino and Mojica, and they have referred the phenomenon as Clustered Regularly Interspaced Short Palindormic Repeats (CRISPR). The biological meaning of CRISPR remained obscure until 2005, when Pourcel, Mojica and Bolotin, independently, concluded that CRISPR were clearly derived from extrachromosomal DNA elements, with most being similar to bacteriophage and plasmids. Outstandingly, species containing CRISPR elements were protected against corresponding foreign invaders and had no residual prophage as evidence of prior infections.4‒6
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