4.8 Article

A programmable pAgo nuclease with universal guide and target specificity from the mesophilic bacterium Kurthia massiliensis

Journal

NUCLEIC ACIDS RESEARCH
Volume 49, Issue 7, Pages 4054-4065

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/nar/gkab182

Keywords

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Funding

  1. Russian Foundation for Basic Research [18-29-07086]
  2. Russian Science Foundation [19-14-00359]
  3. Russian Science Foundation [19-14-00359] Funding Source: Russian Science Foundation

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Argonaute proteins are programmable nucleases found in both eukaryotes and prokaryotes, with a newly discovered pAgo nuclease, KmAgo, showing unique properties of being able to cleave both DNA and RNA targets with no strict sequence specificity, making it potentially useful for highly specific nucleic acid detection and cleavage.
Argonaute proteins are programmable nucleases that are found in both eukaryotes and prokaryotes and provide defense against invading genetic elements. Although some prokaryotic argonautes (pAgos) were shown to recognize RNA targets in vitro, the majority of studied pAgos have strict specificity toward DNA, which limits their practical use in RNA-centric applications. Here, we describe a unique pAgo nuclease, KmAgo, from the mesophilic bacterium Kurthia massiliensis that can be programmed with either DNA or RNA guides and can precisely cleave both DNA and RNA targets. KmAgo binds 1620 nt long 5'-phosphorylated guide molecules with no strict specificity for their sequence and is active in a wide range of temperatures. In bacterial cells, KmAgo is loaded with small DNAs with no obvious sequence preferences suggesting that it can uniformly target genomic sequences. Mismatches between the guide and target sequences greatly affect the efficiency and precision of target cleavage, depending on the mismatch position and the nature of the reacting nucleic acids. Target RNA cleavage by KmAgo depends on the formation of secondary structure indicating that KmAgo can be used for structural probing of RNA. These properties of KmAgo open the way for its use for highly specific nucleic acid detection and cleavage.

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