Harnessing CRISPR-Cas system diversity for gene editing technologies

Alexander McKay; Gaetan Burgio

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Harnessing CRISPR-Cas system diversity for gene editing technologies

机译：利用基因编辑技术的CRISPR-CAS系统多样性

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The discovery and utilization of RNA-guided surveillance complexes,such as CRISPR-Cas9,for sequencespecific DNA or RNA cleavage,has revolutionised the process of gene modification or knockdown.To optimise the use of this technology,an exploratory race has ensued to discover or develop new RNA-guided endonucleases with the most flexible sequence targeting requirements,coupled with high cleavage efficacy and specificity.Here we review the constraints of existing gene editing and assess the merits of exploiting the diversity of CRISPR-Cas effectors as a methodology for surmounting these limitations.

机译：RNA引导的监测复合物的发现和利用，如CRISPR-CAS9，用于序列性DNA或RNA切割，已彻底改变了基因改性或击倒的过程。为了优化这种技术的使用，探索性比赛已经发现或开发具有最灵活的序列靶向要求的新的RNA引导的内切核酸酶，再加上具有高分性疗效和特异性。我们审查了现有基因编辑的约束，并评估利用CRIP-CAS效应的多样性作为超越这些方法的优点限制。

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来源
《生物医学研究杂志：英文版》 |2021年第002期|P.91-106|共16页
作者
Alexander McKay; Gaetan Burgio;
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作者单位

Department of Immunology and Infectious Diseases John Curtin School of Medical Research Australian National University Canberra ACT 2601 Australia;

Department of Immunology and Infectious Diseases John Curtin School of Medical Research Australian National University Canberra ACT 2601 Australia;

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原文格式 PDF
正文语种 chi
中图分类基因工程的应用;
关键词
CRISPR-Cas systems; gene editing; biological evolution; DNA repair; classification; DNA transposable elements;

机译：CRISPR-CAS系统;基因编辑;生物进化;DNA修复;分类;DNA转换元素;

Harnessing CRISPR-Cas system diversity for gene editing technologies

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