A new family of CRISPR‐type V nucleases with C‐rich PAM recognition |
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| Authors: | Tomas Urbaitis Giedrius Gasiunas Joshua K Young Zhenglin Hou Sushmitha Paulraj Egle Godliauskaite Mantvyda M Juskeviciene Migle Stitilyte Monika Jasnauskaite Megumu Mabuchi G Brett Robb Virginijus Siksnys |
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| Affiliation: | 1. CasZyme, Vilnius Lithuania ; 2. Institute of Biotechnology, Vilnius University, Vilnius Lithuania ; 3. Genomics Technologies, Corteva Agriscience™, Johnston IA, USA ; 4. Farming Solutions & Digital, Corteva Agriscience™, Johnston IA, USA ; 5. New England Biolabs, Ipswich MA, USA ;6.Present address: LSC‐EMBL Partnership Institute for Genome Technologies Editing, Life Sciences Center, Vilnius University, Vilnius Lithuania |
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| Abstract: | ![]()
Most CRISPR‐type V nucleases are stimulated to cleave double‐stranded (ds) DNA targets by a T‐rich PAM, which restricts their targeting range. Here, we identify and characterize a new family of type V RNA‐guided nuclease, Cas12l, that exclusively recognizes a C‐rich (5''‐CCY‐3′) PAM. The organization of genes within its CRISPR locus is similar to type II‐B CRISPR‐Cas9 systems, but both sequence analysis and functional studies establish it as a new family of type V effector. Biochemical experiments show that Cas12l nucleases function optimally between 37 and 52°C, depending on the ortholog, and preferentially cut supercoiled DNA. Like other type V nucleases, it exhibits collateral nonspecific ssDNA and ssRNA cleavage activity that is triggered by ssDNA or dsDNA target recognition. Finally, we show that one family member, Asp2Cas12l, functions in a heterologous cellular environment, altogether, suggesting that this new group of CRISPR‐associated nucleases may be harnessed as genome editing reagents. |
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| Keywords: | CRISPR‐ Cas, genome editing, nucleic acid detection, PAM, RNA‐ guided nuclease |
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