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Characterization of CRISPR RNA processing in Clostridium thermocellum and Methanococcus maripaludis

机译:热纤梭菌和马氏甲烷球菌CRISPR RNA加工的表征

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摘要

The CRISPR arrays found in many bacteria and most archaea are transcribed into a long precursor RNA that is processed into small clustered regularly interspaced short palindromic repeats (CRISPR) RNAs (crRNAs). These RNA molecules can contain fragments of viral genomes and mediate, together with a set of CRISPR-associated (Cas) proteins, the prokaryotic immunity against viral attacks. CRISPR/Cas systems are diverse and the Cas6 enzymes that process crRNAs vary between different subtypes. We analysed CRISPR/Cas subtype I-B and present the identification of novel Cas6 enzymes from the bacterial and archaeal model organisms Clostridium thermocellum and Methanococcus maripaludis C5. Methanococcus maripaludis Cas6b in vitro activity and specificity was determined. Two complementary catalytic histidine residues were identified. RNA-Seq analyses revealed in vivo crRNA processing sites, crRNA abundance and orientation of CRISPR transcription within these two organisms. Individual spacer sequences were identified with strong effects on transcription and processing patterns of a CRISPR cluster. These effects will need to be considered for the application of CRISPR clusters that are designed to produce synthetic crRNAs.
机译:在许多细菌和大多数古细菌中发现的CRISPR阵列被转录成较长的前体RNA,然后将其加工成小的簇状规则间隔的短回文重复(CRISPR)RNA(crRNA)。这些RNA分子可以包含病毒基因组的片段,并与一组CRISPR相关(Cas)蛋白一起介导抗病毒攻击的原核免疫。 CRISPR / Cas系统是多种多样的,并且处理crRNA的Cas6酶在不同亚型之间也不同。我们分析了CRISPR / Cas I-B亚型,并提出了从细菌和古细菌生物体梭状芽胞杆菌和马氏甲烷球菌C5鉴定新型Cas6酶的方法。确定了马氏甲烷球菌Cas6b的体外活性和特异性。鉴定出两个互补的催化组氨酸残基。 RNA-Seq分析揭示了这两种生物体内的crRNA加工位点,crRNA丰度和CRISPR转录方向。鉴定出单个间隔区序列对CRISPR簇的转录和加工模式具有强烈影响。在设计产生合成crRNA的CRISPR簇的应用中,需要考虑这些影响。

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