Structural insight into multistage inhibition of CRISPR-Cas12a by AcrVA4

Prokaryotes possess CRISPR-Cas systems to exclude parasitic predators, such as phages and mobile genetic elements (MGEs). These predators, in turn, encode anti-CRISPR (Acr) proteins to evade the CRISPR-Cas immunity. Recently, AcrVA4, an Acr protein inhibiting the CRISPR-Cas12a system, was shown to diminish Lachnospiraceae bacterium Cas12a (LbCas12a)-mediated genome editing in human cells, but the underlying mechanisms remain elusive. Here we report the cryo-EM structures of AcrVA4 bound to CRISPR RNA (crRNA)-loaded LbCas12a and found AcrVA4 could inhibit LbCas12a at several stages of the CRISPR-Cas working pathway, different from other characterized type I/II Acr inhibitors which target only 1 stage. First, it locks the conformation of the LbCas12a-crRNA complex to prevent target DNA-crRNA hybridization. Second, it interacts with the LbCas12a-crRNA-dsDNA complex to release the bound DNA before cleavage. Third, AcrVA4 binds the postcleavage LbCas12a complex to possibly block enzyme recycling. These findings highlight the multifunctionality of AcrVA4 and provide clues for developing regulatory genome-editing tools.

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Cas12a is a dynamic and precise RNA-guided nuclease without off-target activity on λ-DNA

10.1101/2021.06.09.447528 ◽

2021 ◽

Author(s):

Bijoya Paul ◽

Loic Chaubet ◽

Emma Verver ◽

Guillermo Montoya

Keyword(s):

Dna Binding ◽

Genome Editing ◽

Optical Tweezers ◽

Target Site ◽

Target Dna ◽

Multiple Binding ◽

Target Sites ◽

Dna Binding And Cleavage ◽

Target Activity ◽

Insight Into

Cas12a is an RNA-guided endonuclease that is emerging as a powerful genome-editing tool. Here we combined optical tweezers with fluorescence to monitor Cas12a binding onto λ-DNA, providing insight into its DNA binding and cleavage mechanisms. At low forces Cas12a binds DNA specifically with two off-target sites, while at higher forces numerous binding events appear driven by the mechanical distortion of the DNA and partial matches to the crRNA. Despite the multiple binding events, cleavage is only observed on the target site at low forces, when the DNA is flexible. Activity assays show that the preferential off-target sites are not cleaved, and the λ-DNA is severed at the target site. This precision is also observed in Cas12a variants where the specific dsDNA and the unspecific ssDNA cleavage are dissociated or nick the target DNA. We propose that Cas12a and its variants are precise endonucleases that efficiently scan the DNA for its target but only cleave the selected site in the λ-DNA.

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Efficient target cleavage by Type V Cas12a effector programmed with split CRISPR RNA

10.1101/2020.12.21.423781 ◽

2020 ◽

Author(s):

Regina Tkach ◽

Natalia Nikitchina ◽

Nikita Shebanov ◽

Vladimir Mekler ◽

Egor Ulashchik ◽

...

Keyword(s):

Genome Editing ◽

Dna Cleavage ◽

Target Recognition ◽

Human Cells ◽

Stable Complex ◽

Slight Effect ◽

Target Dna ◽

Type V

ABSTRACTCRISPR RNAs (crRNAs) directing target DNA cleavage by type V-A Cas12a nucleases consist of repeat-derived 5’-scaffold moiety and 3’-spacer moiety. We demonstrate that removal of most of the 20-nucleotide scaffold has only a slight effect on in vitro target DNA cleavage by Cas12a ortholog from Acidaminococcus sp (AsCas12a). In fact, residual cleavage was observed even in the presence of a 20-nucleotide crRNA spacer part only, while crRNAs split into two individual moieties (scaffold and spacer RNAs) catalyzed highly specific and efficient cleavage of target DNA. Our data also indicate that AsCas12a combined with split crRNA forms a stable complex with the target. These observations were also confirmed in lysates of human cells expressing AsCas12a. The ability of the AsCas12a nuclease to be programmed with split crRNAs opens new lines of inquiry into the mechanisms of target recognition and cleavage and will further facilitate genome editing techniques based on Cas12a nucleases.

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Disabling a Type I-E CRISPR-Cas Nuclease with a Bacteriophage-Encoded Anti-CRISPR Protein

mBio ◽

10.1128/mbio.01751-17 ◽

2017 ◽

Vol 8 (6) ◽

Cited By ~ 31

Author(s):

April Pawluk ◽

Megha Shah ◽

Marios Mejdani ◽

Charles Calmettes ◽

Trevor F. Moraes ◽

...

Keyword(s):

Pseudomonas Aeruginosa ◽

Transcriptional Repressor ◽

Mobile Genetic Elements ◽

Type I ◽

Genetic Studies ◽

Genetic Elements ◽

Crispr System ◽

Mechanistic Insight ◽

Resistance To Invasion ◽

Insight Into

ABSTRACT CRISPR (clustered regularly interspaced short palindromic repeat)-Cas adaptive immune systems are prevalent defense mechanisms in bacteria and archaea. They provide sequence-specific detection and neutralization of foreign nucleic acids such as bacteriophages and plasmids. One mechanism by which phages and other mobile genetic elements are able to overcome the CRISPR-Cas system is through the expression of anti-CRISPR proteins. Over 20 different families of anti-CRISPR proteins have been described, each of which inhibits a particular type of CRISPR-Cas system. In this work, we determined the structure of type I-E anti-CRISPR protein AcrE1 by X-ray crystallography. We show that AcrE1 binds to the CRISPR-associated helicase/nuclease Cas3 and that the C-terminal region of the anti-CRISPR protein is important for its inhibitory activity. We further show that AcrE1 can convert the endogenous type I-E CRISPR system into a programmable transcriptional repressor. IMPORTANCE The CRISPR-Cas immune system provides bacteria with resistance to invasion by potentially harmful viruses, plasmids, and other foreign mobile genetic elements. This study presents the first structural and mechanistic insight into a phage-encoded protein that inactivates the type I-E CRISPR-Cas system in Pseudomonas aeruginosa. The interaction of this anti-CRISPR protein with the CRISPR-associated helicase/nuclease proteins Cas3 shuts down the CRISPR-Cas system and protects phages carrying this gene from destruction. This interaction also allows the repurposing of the endogenous type I-E CRISPR system into a programmable transcriptional repressor, providing a new biotechnological tool for genetic studies of bacteria encoding this type I-E CRISPR-Cas system. IMPORTANCE The CRISPR-Cas immune system provides bacteria with resistance to invasion by potentially harmful viruses, plasmids, and other foreign mobile genetic elements. This study presents the first structural and mechanistic insight into a phage-encoded protein that inactivates the type I-E CRISPR-Cas system in Pseudomonas aeruginosa. The interaction of this anti-CRISPR protein with the CRISPR-associated helicase/nuclease proteins Cas3 shuts down the CRISPR-Cas system and protects phages carrying this gene from destruction. This interaction also allows the repurposing of the endogenous type I-E CRISPR system into a programmable transcriptional repressor, providing a new biotechnological tool for genetic studies of bacteria encoding this type I-E CRISPR-Cas system.

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Structural basis for inhibition of the type I-F CRISPR–Cas surveillance complex by AcrIF4, AcrIF7 and AcrIF14

Nucleic Acids Research ◽

10.1093/nar/gkaa1199 ◽

2020 ◽

Author(s):

Clinton Gabel ◽

Zhuang Li ◽

Heng Zhang ◽

Leifu Chang

Keyword(s):

Genome Editing ◽

Conformational Changes ◽

Structural Basis ◽

Type I ◽

Structural Detail ◽

Immune Systems ◽

Helical Bundle ◽

Adaptive Immune ◽

Target Dna ◽

Adaptive Immune Systems

Abstract CRISPR–Cas systems are adaptive immune systems in bacteria and archaea to defend against mobile genetic elements (MGEs) and have been repurposed as genome editing tools. Anti-CRISPR (Acr) proteins are produced by MGEs to counteract CRISPR–Cas systems and can be used to regulate genome editing by CRISPR techniques. Here, we report the cryo-EM structures of three type I-F Acr proteins, AcrIF4, AcrIF7 and AcrIF14, bound to the type I-F CRISPR–Cas surveillance complex (the Csy complex) from Pseudomonas aeruginosa. AcrIF4 binds to an unprecedented site on the C-terminal helical bundle of Cas8f subunit, precluding conformational changes required for activation of the Csy complex. AcrIF7 mimics the PAM duplex of target DNA and is bound to the N-terminal DNA vise of Cas8f. Two copies of AcrIF14 bind to the thumb domains of Cas7.4f and Cas7.6f, preventing hybridization between target DNA and the crRNA. Our results reveal structural detail of three AcrIF proteins, each binding to a different site on the Csy complex for inhibiting degradation of MGEs.

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Thermodynamic and structural insight into the underlying mechanisms of the phosphatidylcholine liposomes – casein associates co-assembly and functionality

Food & Function ◽

10.1039/c2fo10185h ◽

2012 ◽

Vol 3 (3) ◽

pp. 271 ◽

Cited By ~ 12

Author(s):

M. G. Semenova ◽

A. S. Antipova ◽

M. S. Anokhina ◽

L. E. Belyakova ◽

Yu. N. Polikarpov ◽

...

Keyword(s):

Phosphatidylcholine Liposomes ◽

Structural Insight ◽

Underlying Mechanisms ◽

Insight Into

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Decision letter: Structural insight into the activation of a class B G-protein-coupled receptor by peptide hormones in live human cells

10.7554/elife.27711.024 ◽

2017 ◽

Keyword(s):

G Protein ◽

Peptide Hormones ◽

Human Cells ◽

G Protein Coupled Receptor ◽

Class B ◽

Structural Insight ◽

G Protein Coupled ◽

Insight Into

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Genome editing in plants using CRISPR type I-D nuclease

Communications Biology ◽

10.1038/s42003-020-01366-6 ◽

2020 ◽

Vol 3 (1) ◽

Author(s):

Keishi Osakabe ◽

Naoki Wada ◽

Tomoko Miyaji ◽

Emi Murakami ◽

Kazuya Marui ◽

...

Keyword(s):

Genome Editing ◽

First Generation ◽

Genome Engineering ◽

Targeted Mutagenesis ◽

Plant Genome ◽

Type I ◽

Crispr System ◽

Target Dna ◽

Short Indels

Abstract Genome editing in plants has advanced greatly by applying the clustered regularly interspaced short palindromic repeats (CRISPRs)-Cas system, especially CRISPR-Cas9. However, CRISPR type I—the most abundant CRISPR system in bacteria—has not been exploited for plant genome modification. In type I CRISPR-Cas systems, e.g., type I-E, Cas3 nucleases degrade the target DNA in mammals. Here, we present a type I-D (TiD) CRISPR-Cas genome editing system in plants. TiD lacks the Cas3 nuclease domain; instead, Cas10d is the functional nuclease in vivo. TiD was active in targeted mutagenesis of tomato genomic DNA. The mutations generated by TiD differed from those of CRISPR/Cas9; both bi-directional long-range deletions and short indels mutations were detected in tomato cells. Furthermore, TiD can be used to efficiently generate bi-allelic mutant plants in the first generation. These findings indicate that TiD is a unique CRISPR system that can be used for genome engineering in plants.

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Structural insight into Pichia pastoris fatty acid synthase

Scientific Reports ◽

10.1038/s41598-021-89196-2 ◽

2021 ◽

Vol 11 (1) ◽

Author(s):

Joseph S. Snowden ◽

Jehad Alzahrani ◽

Lee Sherry ◽

Martin Stacey ◽

David J. Rowlands ◽

...

Keyword(s):

Fatty Acid ◽

Protein Production ◽

Fatty Acid Synthase ◽

Acyl Carrier Protein ◽

Expression System ◽

Model Organism ◽

Type I ◽

Structural Insight ◽

Fatty Acid Synthases ◽

Insight Into

AbstractType I fatty acid synthases (FASs) are critical metabolic enzymes which are common targets for bioengineering in the production of biofuels and other products. Serendipitously, we identified FAS as a contaminant in a cryoEM dataset of virus-like particles (VLPs) purified from P. pastoris, an important model organism and common expression system used in protein production. From these data, we determined the structure of P. pastoris FAS to 3.1 Å resolution. While the overall organisation of the complex was typical of type I FASs, we identified several differences in both structural and enzymatic domains through comparison with the prototypical yeast FAS from S. cerevisiae. Using focussed classification, we were also able to resolve and model the mobile acyl-carrier protein (ACP) domain, which is key for function. Ultimately, the structure reported here will be a useful resource for further efforts to engineer yeast FAS for synthesis of alternate products.

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Genome editing in mammals using CRISPR type I-D nuclease

10.1101/2020.03.14.991976 ◽

2020 ◽

Cited By ~ 1

Author(s):

Keishi Osakabe ◽

Naoki Wada ◽

Emi Murakami ◽

Yuriko Osakabe

Keyword(s):

Genome Editing ◽

Genomic Dna ◽

Genome Engineering ◽

Dna Degradation ◽

Targeted Mutagenesis ◽

Eukaryotic Cells ◽

Type I ◽

Effector Pathway ◽

Target Dna ◽

Target Effects

SUMMARYAdoption of the CRISPR-Cas system has revolutionized genome engineering in recent years; however, application of genome editing with CRISPR type I—the most abundant CRISPR system in bacteria—has been less developed. Type I systems in which Cas3 nuclease degrades the target DNA are known; in contrast, for the sub-type CRISPR type I-D (TiD), which lacks a typical Cas3 nuclease in its cascade, the mechanism of target DNA degradation remains unknown. Here, we found that Cas10d—a nuclease in TiD—is multi-functional in PAM recognition, stabilization and target DNA degradation. TiD can be used for targeted mutagenesis of genomic DNA in human cells, directing both bi-directional long-range deletions and short insertions/deletions. TiD off-target effects, which were dependent on the mismatch position in the protospacer of TiD, were also identified. Our findings suggest TiD as a unique effector pathway in CRISPR that can be repurposed for genome engineering in eukaryotic cells.

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CRISPR-Cas3 induces broad and unidirectional genome editing in human cells

Nature Communications ◽

10.1038/s41467-019-13226-x ◽

2019 ◽

Vol 10 (1) ◽

Cited By ~ 27

Author(s):

Hiroyuki Morisaka ◽

Kazuto Yoshimi ◽

Yuya Okuzaki ◽

Peter Gee ◽

Yayoi Kunihiro ◽

...

Keyword(s):

Genome Editing ◽

Dna Cleavage ◽

Exon Skipping ◽

Nuclease Activity ◽

Human Cells ◽

Eukaryotic Cells ◽

Type I ◽

Crispr System ◽

Class 1 ◽

Component Class

AbstractAlthough single-component Class 2 CRISPR systems, such as type II Cas9 or type V Cas12a (Cpf1), are widely used for genome editing in eukaryotic cells, the application of multi-component Class 1 CRISPR has been less developed. Here we demonstrate that type I-E CRISPR mediates distinct DNA cleavage activity in human cells. Notably, Cas3, which possesses helicase and nuclease activity, predominantly triggered several thousand base pair deletions upstream of the 5′-ARG protospacer adjacent motif (PAM), without prominent off-target activity. This Cas3-mediated directional and broad DNA degradation can be used to introduce functional gene knockouts and knock-ins. As an example of potential therapeutic applications, we show Cas3-mediated exon-skipping of the Duchenne muscular dystrophy (DMD) gene in patient-induced pluripotent stem cells (iPSCs). These findings broaden our understanding of the Class 1 CRISPR system, which may serve as a unique genome editing tool in eukaryotic cells distinct from the Class 2 CRISPR system.

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