Mechanism of R-loop formation and conformational activation of Cas9

Mapping Intimacies ◽

10.1101/2021.09.16.460614 ◽

2021 ◽

Author(s):

Martin Pacesa ◽

Martin Jinek

Keyword(s):

Dna Cleavage ◽

Structural Basis ◽

Seed Region ◽

Loop Formation ◽

Base Pairs ◽

Guide Rna ◽

Target Strand ◽

Target Dna ◽

Dna Strand ◽

Dna Substrate

Cas9 is a CRISPR-associated endonuclease capable of RNA-guided, site-specific DNA cleavage. The programmable activity of Cas9 has been widely utilized for genome editing applications. Despite extensive studies, the precise mechanism of target DNA binding and on-/off-target discrimination remains incompletely understood. Here we report cryo-EM structures of intermediate binding states of Streptococcus pyogenes Cas9 that reveal domain rearrangements induced by R-loop propagation and PAM-distal duplex positioning. At early stages of binding, the Cas9 REC2 and REC3 domains form a positively charged cleft that accommodates the PAM-distal duplex of the DNA substrate. Target hybridisation past the seed region positions the guide-target heteroduplex into the central binding channel and results in a conformational rearrangement of the REC lobe. Extension of the R-loop to 16 base pairs triggers the relocation of the HNH domain towards the target DNA strand in a catalytically incompetent conformation. The structures indicate that incomplete target strand pairing fails to induce the conformational displacements necessary for nuclease domain activation. Our results establish a structural basis for target DNA-dependent activation of Cas9 that advances our understanding of its off-target activity and will facilitate the development of novel Cas9 variants and guide RNA designs with enhanced specificity and activity.

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Structural basis for mismatch surveillance by CRISPR/Cas9

10.1101/2021.09.14.460224 ◽

2021 ◽

Author(s):

Jack PK Bravo ◽

Mu-Sen Liu ◽

Ryan S McCool ◽

Kyungseok Jung ◽

Kenneth A Johnson ◽

...

Keyword(s):

Dna Cleavage ◽

Molecular Mechanisms ◽

Structural Basis ◽

Guide Rna ◽

Flexible Loop ◽

Target Strand ◽

Target Dna ◽

Conformational Rearrangements ◽

Structural Mechanisms

The widespread use of CRISPR/Cas9 as a programmable genome editing tool has been hindered by off-target DNA cleavage (Cong et al., 2013; Doudna, 2020; Fu et al., 2013; Jinek et al., 2013). While analysis of such off-target editing events have enabled the development of Cas9 variants with greater discrimination against mismatches (Chen et al., 2017; Kleinstiver et al., 2016; Slaymaker et al., 2016), the underlying molecular mechanisms by which Cas9 rejects or accepts mismatches are poorly understood (Kim et al., 2019; Liu et al., 2020; Slaymaker and Gaudelli, 2021). Here, we used kinetic analysis to guide cryo-EM structure determination of Cas9 at different stages of mismatch surveillance. We observe a distinct, previously undescribed linear conformation of the duplex formed between the guide RNA (gRNA) and DNA target strand (TS), that occurs in the presence of PAM-distal mismatches, preventing Cas9 activation. The canonical kinked gRNA:TS duplex is a prerequisite for Cas9 activation, acting as a structural scaffold to facilitate Cas9 conformational rearrangements necessary for DNA cleavage. We observe that highly tolerated PAM- distal mismatches achieve this kinked conformation through stabilization of a distorted duplex conformation via a flexible loop in the RuvC domain. Our results provide molecular insights into the underlying structural mechanisms that may facilitate off- target cleavage by Cas9 and provides a molecular blueprint for the design of next- generation high fidelity Cas9 variants that selectively reduce off-target DNA cleavage while retaining efficient cleavage of on-target DNA.

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Mechanistic insights into the R-loop formation and cleavage in CRISPR-Cas12i1

Nature Communications ◽

10.1038/s41467-021-23876-5 ◽

2021 ◽

Vol 12 (1) ◽

Author(s):

Bo Zhang ◽

Diyin Luo ◽

Yu Li ◽

Vanja Perčulija ◽

Jing Chen ◽

...

Keyword(s):

Genome Editing ◽

Dna Cleavage ◽

Binary Complex ◽

Loop Formation ◽

Dna Duplex ◽

Target Dna ◽

Before And After ◽

Dna Strand ◽

Type V ◽

Functionally Diverse

AbstractCas12i is a newly identified member of the functionally diverse type V CRISPR-Cas effectors. Although Cas12i has the potential to serve as genome-editing tool, its structural and functional characteristics need to be investigated in more detail before effective application. Here we report the crystal structures of the Cas12i1 R-loop complexes before and after target DNA cleavage to elucidate the mechanisms underlying target DNA duplex unwinding, R-loop formation and cis cleavage. The structure of the R-loop complex after target DNA cleavage also provides information regarding trans cleavage. Besides, we report a crystal structure of the Cas12i1 binary complex interacting with a pseudo target oligonucleotide, which mimics target interrogation. Upon target DNA duplex binding, the Cas12i1 PAM-interacting cleft undergoes a remarkable open-to-closed adjustment. Notably, a zipper motif in the Helical-I domain facilitates unzipping of the target DNA duplex. Formation of the 19-bp crRNA-target DNA strand heteroduplex in the R-loop complexes triggers a conformational rearrangement and unleashes the DNase activity. This study provides valuable insights for developing Cas12i1 into a reliable genome-editing tool.

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DNA unwinding is the primary determinant of CRISPR-Cas9 activity

10.1101/205823 ◽

2017 ◽

Cited By ~ 1

Author(s):

Shanzhong Gong ◽

Helen Hong Yu ◽

Kenneth A. Johnson ◽

David W. Taylor

Keyword(s):

Genome Engineering ◽

Nuclease Activity ◽

Loop Formation ◽

Base Pairs ◽

Guide Rna ◽

Target Strand ◽

Primary Determinant ◽

Specificity Constant ◽

Rate Limiting

SummaryBacterial adaptive immunity utilizes RNA-guided surveillance complexes composed of CRISPR (clustered regularly interspaced short palindromic repeats)-associated (Cas) proteins together with CRISPR RNAs (crRNAs) to target foreign nucleic acids for destruction. Cas9, a type II CRISPR-Cas effector complex, can be programed with a single guide RNA that base-pairs with the target strand of dsDNA, displacing the non-target strand to create an R-loop, where the HNH and RuvC nuclease domains can cleave opposing strands. Cas9 has been repurposed for a variety of important genome engineering applications. While many structural and biochemical studies have shed light on the mechanism of Cas9 cleavage, a clear unifying model has yet to emerge. Our detailed kinetic characterization of the enzyme reveals that DNA binding is reversible, R-loop formation is rate-limiting, occurring in two steps, one for each of the nuclease domains. Although the HNH nuclease activity is stimulated by Mg2+ with a single measureable Kd, the RuvC activity requires two distinct Mg2+ binding events. The specificity constant for cleavage is determined through an induced-fit mechanism as the product of the equilibrium binding affinity for DNA and the rate of R-loop formation.

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Kinetic basis for DNA target specificity of CRISPR-Cas12a

10.1101/355917 ◽

2018 ◽

Author(s):

Isabel Strohkendl ◽

Fatema A. Saifuddin ◽

James R. Rybarski ◽

Ilya J. Finkelstein ◽

Rick Russell

Keyword(s):

Dna Cleavage ◽

Target Sequence ◽

Seed Region ◽

Target Specificity ◽

Loop Formation ◽

Guide Rna ◽

Dna Targeting ◽

Cas9 Nuclease ◽

Protospacer Adjacent Motif ◽

Late Transition

SUMMARYClass II CRISPR-Cas nucleases are programmable via a single guide RNA, enabling genome editing applications in nearly all organisms. However, DNA cleavage at off-target sites that resemble the target sequence is a pervasive problem that remains poorly understood mechanistically. Here, we use quantitative kinetics to dissect the reaction steps of DNA targeting by Acidaminococcus sp Cas12a (also known as Cpf1). We show that Cas12a binds DNA tightly in two kinetically-separable steps. Protospacer-adjacent motif (PAM) recognition is followed by rate-limiting R-loop propagation, leading to inevitable DNA cleavage of both strands. Despite the functionally irreversible binding, Cas12a discriminates strongly against mismatches along most of the DNA target sequence, implying substantial reversibility during R-loop formation –a late transition state– and the absence of a ‘seed’ region. Our results provide a quantitative underpinning for the DNA cleavage patterns measured in vivo and observations of greater reported target specificity of Cas12a than the Cas9 nuclease.

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The Effect of DNA Topology on Observed Rates of R-Loop Formation and DNA Strand Cleavage by CRISPR Cas12a

Genes ◽

10.3390/genes10020169 ◽

2019 ◽

Vol 10 (2) ◽

pp. 169 ◽

Cited By ~ 10

Author(s):

Kara van Aelst ◽

Carlos Martínez-Santiago ◽

Stephen Cross ◽

Mark Szczelkun

Keyword(s):

Single Molecule ◽

Dna Cleavage ◽

Streptococcus Thermophilus ◽

Dna Supercoiling ◽

Magnetic Tweezers ◽

Loop Formation ◽

Formation Kinetics ◽

Target Strand ◽

Dna Strand ◽

Type V

Here we explored the mechanism of R-loop formation and DNA cleavage by type V CRISPR Cas12a (formerly known as Cpf1). We first used a single-molecule magnetic tweezers (MT) assay to show that R-loop formation by Lachnospiraceae bacterium ND2006 Cas12a is significantly enhanced by negative DNA supercoiling, as observed previously with Streptococcus thermophilus DGCC7710 CRISPR3 Cas9. Consistent with the MT data, the apparent rate of cleavage of supercoiled plasmid DNA was observed to be >50-fold faster than the apparent rates for linear DNA or nicked circular DNA because of topology-dependent differences in R-loop formation kinetics. Taking the differences into account, the cleavage data for all substrates can be fitted with the same apparent rate constants for the two strand-cleavage steps, with the first event >15-fold faster than the second. By independently following the ensemble cleavage of the non-target strand (NTS) and target strand (TS), we could show that the faster rate is due to NTS cleavage, the slower rate due to TS cleavage, as expected from previous studies.

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Structural and functional insights into the bona fide catalytic state of Streptococcus pyogenes Cas9 HNH nuclease domain

eLife ◽

10.7554/elife.46500 ◽

2019 ◽

Vol 8 ◽

Cited By ~ 3

Author(s):

Zhicheng Zuo ◽

Ashwini Zolekar ◽

Kesavan Babu ◽

Victor JT Lin ◽

Hamed S Hayatshahi ◽

...

Keyword(s):

Streptococcus Pyogenes ◽

Dna Cleavage ◽

Ternary Complex ◽

Catalytic Triad ◽

Guide Rna ◽

Nuclease Domain ◽

Target Dna ◽

Bona Fide ◽

Experimental Approaches ◽

Dna Strand

The CRISPR-associated endonuclease Cas9 from Streptococcus pyogenes (SpyCas9), along with a programmable single-guide RNA (sgRNA), has been exploited as a significant genome-editing tool. Despite the recent advances in determining the SpyCas9 structures and DNA cleavage mechanism, the cleavage-competent conformation of the catalytic HNH nuclease domain of SpyCas9 remains largely elusive and debatable. By integrating computational and experimental approaches, we unveiled and validated the activated Cas9-sgRNA-DNA ternary complex in which the HNH domain is neatly poised for cleaving the target DNA strand. In this catalysis model, the HNH employs the catalytic triad of D839-H840-N863 for cleavage catalysis, rather than previously implicated D839-H840-D861, D837-D839-H840, or D839-H840-D861-N863. Our study contributes critical information to defining the catalytic conformation of the HNH domain and advances the knowledge about the conformational activation underlying Cas9-mediated DNA cleavage.

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Staring at the Naked Goddess: Unraveling the Structure and Reactivity of Artemis Endonuclease Interacting with a DNA Double Strand

Molecules ◽

10.3390/molecules26133986 ◽

2021 ◽

Vol 26 (13) ◽

pp. 3986

Author(s):

Cécilia Hognon ◽

Antonio Monari

Keyword(s):

Dna Cleavage ◽

Catalytic Mechanism ◽

Dna Lesions ◽

Cleavage Reaction ◽

Dynamic Simulations ◽

Important Target ◽

System Adaptation ◽

Dna Strands ◽

Dna Strand ◽

Dna Substrate

Artemis is an endonuclease responsible for breaking hairpin DNA strands during immune system adaptation and maturation as well as the processing of potentially toxic DNA lesions. Thus, Artemis may be an important target in the development of anticancer therapy, both for the sensitization of radiotherapy and for immunotherapy. Despite its importance, its structure has been resolved only recently, and important questions concerning the arrangement of its active center, the interaction with the DNA substrate, and the catalytic mechanism remain unanswered. In this contribution, by performing extensive molecular dynamic simulations, both classically and at the hybrid quantum mechanics/molecular mechanics level, we evidenced the stable interaction modes of Artemis with a model DNA strand. We also analyzed the catalytic cycle providing the free energy profile and key transition states for the DNA cleavage reaction.

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Dynamic mechanisms of CRISPR interference by Escherichia coli CRISPR-Cas3

10.1101/2021.07.18.452824 ◽

2021 ◽

Author(s):

Kazuto Yoshimi ◽

Kohei TAKESHITA ◽

Noriyuki Kodera ◽

Satomi Shibumura ◽

Yuko Yamauchi ◽

...

Keyword(s):

Escherichia Coli ◽

High Speed ◽

Dna Helicase ◽

Type I ◽

Loop Formation ◽

Force Microscopy ◽

Atomic Force ◽

Target Strand ◽

Target Dna

Type I CRISPR-Cas3 uses an RNA-guided multi Cas-protein complex, Cascade, which detects and degrades foreign nucleic acids via the helicase-nuclease Cas3 protein. Despite many studies using cryoEM and smFRET, the precise mechanism of Cas3-mediated cleavage and degradation of target DNA remains elusive. Here we reconstitute the CRISPR-Cas3 system in vitro to show how the Escherichia coli Cas3 (EcoCas3) with EcoCascade exhibits collateral non-specific ssDNA cleavage and target specific DNA degradation. Partial binding of EcoCascade to target DNA with tolerated mismatches within the spacer sequence, but not the PAM, elicits collateral ssDNA cleavage activity of recruited EcoCas3. Conversely, stable binding with complete R-loop formation drives EcoCas3 to nick the non-target strand (NTS) in the bound DNA. Helicase-dependent unwinding then combines with trans ssDNA cleavage of the target strand and repetitive cis cleavage of the NTS to degrade the target dsDNA substrate. High-speed atomic force microscopy demonstrates that EcoCas3 bound to EcoCascade repeatedly reels and releases the target DNA, followed by target fragmentation. Together, these results provide a revised model for collateral ssDNA cleavage and target dsDNA degradation by CRISPR-Cas3, furthering understanding of type I CRISPR priming and interference and informing future genome editing tools.

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Snapshots of a modified nucleotide moving through the confines of a DNA polymerase

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1811518115 ◽

2018 ◽

Vol 115 (40) ◽

pp. 9992-9997 ◽

Cited By ~ 16

Author(s):

Heike Maria Kropp ◽

Simon Leonard Dürr ◽

Christine Peter ◽

Kay Diederichs ◽

Andreas Marx

Keyword(s):

Dna Polymerase ◽

Dna Polymerases ◽

Ternary Complexes ◽

Structural Basis ◽

Modified Nucleotides ◽

Molecular Mechanics Calculations ◽

Modified Dna ◽

Substrate Properties ◽

Dna Strand ◽

Dna Substrate

DNA polymerases have evolved to process the four canonical nucleotides accurately. Nevertheless, these enzymes are also known to process modified nucleotides, which is the key to numerous core biotechnology applications. Processing of modified nucleotides includes incorporation of the modified nucleotide and postincorporation elongation to proceed with the synthesis of the nascent DNA strand. The structural basis for postincorporation elongation is currently unknown. We addressed this issue and successfully crystallized KlenTaq DNA polymerase in six closed ternary complexes containing the enzyme, the modified DNA substrate, and the incoming nucleotide. Each structure shows a high-resolution snapshot of the elongation of a modified primer, where the modification “moves” from the 3′-primer terminus upstream to the sixth nucleotide in the primer strand. Combining these data with quantum mechanics/molecular mechanics calculations and biochemical studies elucidates how the enzyme and the modified substrate mutually modulate their conformations without compromising the enzyme’s activity significantly. The study highlights the plasticity of the system as origin of the broad substrate properties of DNA polymerases and facilitates the design of improved systems.

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Structural basis for the dimerization-dependent CRISPR-Cas12f nuclease

10.1101/2020.12.22.424058 ◽

2020 ◽

Author(s):

Renjian Xiao ◽

Zhuang Li ◽

Shukun Wang ◽

Ruijie Han ◽

Leifu Chang

Keyword(s):

Genome Editing ◽

Conformational Changes ◽

Dna Cleavage ◽

Substrate Recognition ◽

Activation Mechanism ◽

Structural Basis ◽

Target Dna ◽

Type V ◽

Underlying Substrate

ABSTRACTCas12f, also known as Cas14, is an exceptionally small type V-F CRISPR-Cas nuclease that is roughly half the size of comparable nucleases of this type. To reveal the mechanisms underlying substrate recognition and cleavage, we determined the cryo-EM structures of the Cas12f-sgRNA-target DNA and Cas12f-sgRNA complexes at 3.1 Å and 3.9 Å, respectively. An asymmetric Cas12f dimer is bound to one sgRNA for recognition and cleavage of dsDNA substrate with a T-rich PAM sequence. Despite its dimerization, Cas12f adopts a conserved activation mechanism among the type V nucleases which requires coordinated conformational changes induced by the formation of the crRNA-target DNA heteroduplex, including the close-to-open transition in the lid motif of the RuvC domain. Only one RuvC domain in the Cas12f dimer is activated by substrate recognition, and the substrate bound to the activated RuvC domain is captured in the structure. Structure-assisted truncated sgRNA, which is less than half the length of the original sgRNA, is still active for target DNA cleavage. Our results expand our understanding of the diverse type V CRISPR-Cas nucleases and facilitate potential genome editing applications using the miniature Cas12f.

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