Your search keyword '"Cas9"' showing total 113 results

1. The Histone Chaperone FACT Induces Cas9 Multi-turnover Behavior and Modifies Genome Manipulation in Human Cells

Author

Wang, Alan S, Chen, Leo C, Wu, R Alex, Hao, Yvonne, McSwiggen, David T, Heckert, Alec B, Richardson, Christopher D, Gowen, Benjamin G, Kazane, Katelynn R, Vu, Jonathan T, Wyman, Stacia K, Shin, Jiyung J, Darzacq, Xavier, Walter, Johannes C, and Corn, Jacob E

Subjects

Biochemistry and Cell Biology, Biological Sciences, Human Genome, Genetics, 1.1 Normal biological development and functioning, Underpinning research, Generic health relevance, Animals, CRISPR-Associated Protein 9, CRISPR-Associated Proteins, Cell Line, DNA, DNA Breaks, Double-Stranded, DNA Repair, DNA-Binding Proteins, Epigenesis, Genetic, Gene Editing, Gene Knockdown Techniques, Genome, Human, High Mobility Group Proteins, Humans, Nucleosomes, Transcriptional Elongation Factors, Xenopus laevis, CRISPR, CRISPRa, CRISPRi, Cas9, FACT complex, SPT16, SSRP1, histone chaperone, Medical and Health Sciences, Developmental Biology, Biological sciences, Biomedical and clinical sciences, Health sciences

Abstract

Cas9 is a prokaryotic RNA-guided DNA endonuclease that binds substrates tightly in vitro but turns over rapidly when used to manipulate genomes in eukaryotic cells. Little is known about the factors responsible for dislodging Cas9 or how they influence genome engineering. Unbiased detection through proximity labeling of transient protein interactions in cell-free Xenopus laevis egg extract identified the dimeric histone chaperone facilitates chromatin transcription (FACT) as an interactor of substrate-bound Cas9. FACT is both necessary and sufficient to displace dCas9, and FACT immunodepletion converts Cas9's activity from multi-turnover to single turnover. In human cells, FACT depletion extends dCas9 residence times, delays genome editing, and alters the balance between indel formation and homology-directed repair. FACT knockdown also increases epigenetic marking by dCas9-based transcriptional effectors with a concomitant enhancement of transcriptional modulation. FACT thus shapes the intrinsic cellular response to Cas9-based genome manipulation most likely by determining Cas9 residence times.

Published

2020

2. Temperature-Responsive Competitive Inhibition of CRISPR-Cas9

Author

Jiang, Fuguo, Liu, Jun-Jie, Osuna, Beatriz A, Xu, Michael, Berry, Joel D, Rauch, Benjamin J, Nogales, Eva, Bondy-Denomy, Joseph, and Doudna, Jennifer A

Subjects

Biochemistry and Cell Biology, Biological Sciences, Infectious Diseases, Genetics, Emerging Infectious Diseases, Prevention, Underpinning research, 1.1 Normal biological development and functioning, Binding, Competitive, CRISPR-Associated Protein 9, CRISPR-Cas Systems, Cryoelectron Microscopy, DNA, Escherichia coli, Gene Editing, Gene Expression Regulation, Bacterial, Models, Molecular, Nucleic Acid Conformation, Protein Binding, Protein Conformation, Pseudomonas Phages, Pseudomonas aeruginosa, RNA, Guide, Kinetoplastida, Structure-Activity Relationship, Temperature, Viral Proteins, AcrIIA2, CRISPR-Cas, CRISPR-Cas9, Cas9, Cas9 inhibitors, PAM blockage, anti-CRISPR, bacteriophage, genome editing, temperature-dependent inhibition, RNA, Guide, Medical and Health Sciences, Developmental Biology, Biological sciences, Biomedical and clinical sciences, Health sciences

Abstract

CRISPR-Cas immune systems utilize RNA-guided nucleases to protect bacteria from bacteriophage infection. Bacteriophages have in turn evolved inhibitory "anti-CRISPR" (Acr) proteins, including six inhibitors (AcrIIA1-AcrIIA6) that can block DNA cutting and genome editing by type II-A CRISPR-Cas9 enzymes. We show here that AcrIIA2 and its more potent homolog, AcrIIA2b, prevent Cas9 binding to DNA by occluding protein residues required for DNA binding. Cryo-EM-determined structures of AcrIIA2 or AcrIIA2b bound to S. pyogenes Cas9 reveal a mode of competitive inhibition of DNA binding that is distinct from other known Acrs. Differences in the temperature dependence of Cas9 inhibition by AcrIIA2 and AcrIIA2b arise from differences in both inhibitor structure and the local inhibitor-binding environment on Cas9. These findings expand the natural toolbox for regulating CRISPR-Cas9 genome editing temporally, spatially, and conditionally.

Published

2019

3. A CRISPR Resource for Individual, Combinatorial, or Multiplexed Gene Knockout

Author

Erard, Nicolas, Knott, Simon RV, and Hannon, Gregory J

Subjects

Biological Sciences, Genetics, Biotechnology, Prevention, Algorithms, CRISPR-Associated Proteins, CRISPR-Cas Systems, Endonucleases, Gene Library, Gene Silencing, Gene Targeting, High-Throughput Nucleotide Sequencing, Humans, K562 Cells, Machine Learning, RNA, Guide, Kinetoplastida, Transfection, CRISPR, Cas9, algorithm, combinatorial, expression, lentivirus, library, prediction, screen, sgRNA, Medical and Health Sciences, Developmental Biology, Biological sciences, Biomedical and clinical sciences, Health sciences

Abstract

We have combined a machine-learning approach with other strategies to optimize knockout efficiency with the CRISPR/Cas9 system. In addition, we have developed a multiplexed sgRNA expression strategy that promotes the functional ablation of single genes and allows for combinatorial targeting. These strategies have been combined to design and construct a genome-wide, sequence-verified, arrayed CRISPR library. This resource allows single-target or combinatorial genetic screens to be carried out at scale in a multiplexed or arrayed format. By conducting parallel loss-of-function screens, we compare our approach to existing sgRNA design and expression strategies.

Published

2017

4. Mutations in Cas9 Enhance the Rate of Acquisition of Viral Spacer Sequences during the CRISPR-Cas Immune Response

Author

Heler, Robert, Wright, Addison V, Vucelja, Marija, Bikard, David, Doudna, Jennifer A, and Marraffini, Luciano A

Subjects

Medical Microbiology, Biomedical and Clinical Sciences, Biological Sciences, Immunology, Immunization, Genetics, Vaccine Related, Prevention, Aetiology, 2.1 Biological and endogenous factors, Infection, Adaptive Immunity, Bacterial Proteins, CRISPR-Associated Protein 9, CRISPR-Associated Proteins, CRISPR-Cas Systems, Clustered Regularly Interspaced Short Palindromic Repeats, DNA, Intergenic, DNA, Viral, Endonucleases, Genotype, High-Throughput Nucleotide Sequencing, Host-Pathogen Interactions, Mutation, Phenotype, Staphylococcus aureus, Substrate Specificity, Time Factors, CRISPR-Cas, Cas9, adaptation, adaptive immunity, bacteriophage, horizontal gene transfer, spacer acquisition, Medical and Health Sciences, Developmental Biology, Biological sciences, Biomedical and clinical sciences, Health sciences

Abstract

CRISPR loci and their associated (Cas) proteins encode a prokaryotic immune system that protects against viruses and plasmids. Upon infection, a low fraction of cells acquire short DNA sequences from the invader. These sequences (spacers) are integrated in between the repeats of the CRISPR locus and immunize the host against the matching invader. Spacers specify the targets of the CRISPR immune response through transcription into short RNA guides that direct Cas nucleases to the invading DNA molecules. Here we performed random mutagenesis of the RNA-guided Cas9 nuclease to look for variants that provide enhanced immunity against viral infection. We identified a mutation, I473F, that increases the rate of spacer acquisition by more than two orders of magnitude. Our results highlight the role of Cas9 during CRISPR immunization and provide a useful tool to study this rare process and develop it as a biotechnological application.

Published

2017

5. The Revolution Continues: Newly Discovered Systems Expand the CRISPR-Cas Toolkit.

Author

Murugan, Karthik, Sashital, Dipali G., Babu, Kesavan, Sundaresan, Ramya, and Rajan, Rakhi

Subjects

*CRISPRS, *ENDONUCLEASES, *GENOME editing, *DNA-binding proteins, *STREPTOCOCCUS pyogenes

Abstract

CRISPR-Cas systems defend prokaryotes against bacteriophages and mobile genetic elements and serve as the basis for revolutionary tools for genetic engineering. Class 2 CRISPR-Cas systems use single Cas endonucleases paired with guide RNAs to cleave complementary nucleic acid targets, enabling programmable sequence-specific targeting with minimal machinery. Recent discoveries of previously unidentified CRISPR-Cas systems have uncovered a deep reservoir of potential biotechnological tools beyond the well-characterized Type II Cas9 systems. Here we review the current mechanistic understanding of newly discovered single-protein Cas endonucleases. Comparison of these Cas effectors reveals substantial mechanistic diversity, underscoring the phylogenetic divergence of related CRISPR-Cas systems. This diversity has enabled further expansion of CRISPR-Cas biotechnological toolkits, with wide-ranging applications from genome editing to diagnostic tools based on various Cas endonuclease activities. These advances highlight the exciting prospects for future tools based on the continually expanding set of CRISPR-Cas systems. [ABSTRACT FROM AUTHOR]

Published

2017

6. The Anti-CRISPR Story: A Battle for Survival.

Author

Maxwell, Karen L.

Subjects

*BACTERIOPHAGES, *PSEUDOMONAS aeruginosa, *DNA-binding proteins, *HELICASE genetics, *NUCLEASE genetics

Abstract

The last decade has seen the fields of molecular biology and genetics transformed by the development of CRISPR-based gene editing technologies. These technologies were derived from bacterial defense systems that protect against viral invasion. Elegant studies focused on the evolutionary battle between CRISPR-encoding bacteria and the viruses that infect and kill them revealed the next step in this arms race, the anti-CRISPR proteins. Investigation of these proteins has provided important new insight into how CRISPR-Cas systems work and how bacterial genomes evolve. They have also led to the development of important biotechnological tools that can be used for genetic engineering, including off switches for CRISPR-Cas9 genome editing in human cells. [ABSTRACT FROM AUTHOR]

Published

2017

7. High-Throughput Approaches to Pinpoint Function within the Noncoding Genome.

Author

Montalbano, Antonino, Sanjana, Neville E., and Canver, Matthew C.

Subjects

*HUMAN genome, *NON-coding DNA, *NON-coding RNA, *NUCLEOTIDE sequence, *CRISPRS, *FUNCTIONAL genomics

Abstract

The clustered regularly interspaced short palindromic repeats (CRISPR)-Cas nuclease system is a powerful tool for genome editing, and its simple programmability has enabled high-throughput genetic and epigenetic studies. These high-throughput approaches offer investigators a toolkit for functional interrogation of not only protein-coding genes but also noncoding DNA. Historically, noncoding DNA has lacked the detailed characterization that has been applied to protein-coding genes in large part because there has not been a robust set of methodologies for perturbing these regions. Although the majority of high-throughput CRISPR screens have focused on the coding genome to date, an increasing number of CRISPR screens targeting noncoding genomic regions continue to emerge. Here, we review high-throughput CRISPR-based approaches to uncover and understand functional elements within the noncoding genome and discuss practical aspects of noncoding library design and screen analysis. [ABSTRACT FROM AUTHOR]

Published

2017

8. Unwinding the Role of FACT in Cas9-based Genome Editing

Author

Charles A. Gersbach and Brian D. Cosgrove

Subjects

0303 health sciences, Cas9, Cell Biology, Computational biology, Biology, Proteomics, Genome, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Histone, Genome editing, chemistry, Epigenome editing, biology.protein, Chaperone complex, Molecular Biology, 030217 neurology & neurosurgery, DNA, 030304 developmental biology

Abstract

In a recent issue of Molecular Cell, Wang et al. (2020) employ unbiased proteomics approaches and live-cell imaging to reveal a key role for the histone chaperone complex FACT (SPT16 and SSRP1) in governing Cas9 turnover at the DNA target site during genome and epigenome editing.

Published

2020

9. CRISPR Shields: Fending Off Diverse Cas Nucleases with Nucleus-like Structures

Author

Erik J. Sontheimer and Rodolphe Barrangou

Subjects

Host immunity, 0303 health sciences, Extramural, Cas9, RNA, Cell Biology, Computational biology, Biology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, medicine.anatomical_structure, chemistry, medicine, CRISPR, Molecular Biology, Nucleus, 030217 neurology & neurosurgery, DNA, 030304 developmental biology

Abstract

Two recent studies have uncovered a novel means by which bacteriophages thwart host immunity. Mendoza et al. (2020) and Malone et al. (2020) demonstrate that a nucleus-like proteinaceous structure shields phage DNA from CRISPR-associated nucleases encompassing Cascade-Cas3, Cas9, and Cas12.

Published

2020

10. Put on Your Para-spectacles: The Development of Optimized CRISPR-Cas13-Based Approaches to Image RNA Dynamics in Real Time

Author

Mitchell R. O’Connell and Brandon J. Davis

Subjects

RNA metabolism, 0303 health sciences, Cas9, Dynamics (mechanics), RNA, DNA, Cell Biology, Computational biology, Biology, 03 medical and health sciences, chemistry.chemical_compound, Eyeglasses, 0302 clinical medicine, chemistry, CRISPR, Clustered Regularly Interspaced Short Palindromic Repeats, CRISPR-Cas Systems, Molecular Biology, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Live-cell RNA imaging is a powerful approach to observe the real-time dynamics of RNA metabolism. Two recent papers describe an optimized fluorescence-based CRISPR-Cas13 approach to image colocalized or repeat-containing RNAs in real time, as well as demonstrate simultaneous RNA-DNA labeling by using Cas13 and Cas9 in tandem.

Published

2020

11. Discovery and Functional Characterization of Diverse Class 2 CRISPR-Cas Systems.

Author

Shmakov, Sergey, Abudayyeh, Omar O., Makarova, Kira S., Wolf, Yuri I., Gootenberg, Jonathan S., Semenova, Ekaterina, Minakhin, Leonid, Joung, Julia, Konermann, Silvana, Severinov, Konstantin, Zhang, Feng, and Koonin, Eugene V.

Subjects

*CRISPRS, *RIBONUCLEASES, *ENDONUCLEASES, *COMPARATIVE studies, *GENETIC recombination

Abstract

Summary Microbial CRISPR-Cas systems are divided into Class 1, with multisubunit effector complexes, and Class 2, with single protein effectors. Currently, only two Class 2 effectors, Cas9 and Cpf1, are known. We describe here three distinct Class 2 CRISPR-Cas systems. The effectors of two of the identified systems, C2c1 and C2c3, contain RuvC-like endonuclease domains distantly related to Cpf1. The third system, C2c2, contains an effector with two predicted HEPN RNase domains. Whereas production of mature CRISPR RNA (crRNA) by C2c1 depends on tracrRNA, C2c2 crRNA maturation is tracrRNA independent. We found that C2c1 systems can mediate DNA interference in a 5′-PAM-dependent fashion analogous to Cpf1. However, unlike Cpf1, which is a single-RNA-guided nuclease, C2c1 depends on both crRNA and tracrRNA for DNA cleavage. Finally, comparative analysis indicates that Class 2 CRISPR-Cas systems evolved on multiple occasions through recombination of Class 1 adaptation modules with effector proteins acquired from distinct mobile elements. [ABSTRACT FROM AUTHOR]

Published

2015

12. Building the Class 2 CRISPR-Cas Arsenal.

Author

Lewis, Kevin M. and Ke, Ailong

Subjects

*CRISPRS, *GENOME editing, *BIOLOGICAL adaptation, *BIOLOGICAL research, *BIOINFORMATICS

Abstract

Adaptation of CRISPR-Cas9 for genome-editing applications has revolutionized biomedical research. New single-component effector CRISPR systems are emerging from the bioinformatics pipeline. How can we best harness their power? Three new studies will no doubt facilitate this transition by generating the C2c1 and C2c2 structure snapshots in different functional states. [ABSTRACT FROM AUTHOR]

Published

2017

13. Genome oligopaint via local denaturation fluorescence in situ hybridization

Author

Yanbo Wang, Taekjip Ha, Scott Bailey, Haobo Wang, Xinyu Ashlee Feng, Wayne Taylor Cottle, John Mallon, and Momčilo Gavrilov

Subjects

Hot Temperature, Biology, Nucleic Acid Denaturation, Genome, DNA sequencing, Article, Cell Line, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, CRISPR-Associated Protein 9, medicine, CRISPR, Humans, Denaturation (biochemistry), Molecular Biology, In Situ Hybridization, Fluorescence, 030304 developmental biology, 0303 health sciences, medicine.diagnostic_test, Cas9, Cell Biology, Fibroblasts, genomic DNA, Biochemistry, chemistry, Female, CRISPR-Cas Systems, 030217 neurology & neurosurgery, DNA, Fluorescence in situ hybridization, RNA, Guide, Kinetoplastida

Abstract

Cas9 in complex with a programmable guide RNA targets specific double-stranded DNA for cleavage. By harnessing Cas9 as a programmable loader of superhelicase to genomic DNA, here we report a physiological-temperature DNA FISH method termed Genome Oligopaint via Local Denaturation Fluorescence in Situ Hybridization (GOLD FISH). Instead of global denaturation as in conventional DNA FISH, loading a superhelicase at a Cas9-generated nick allows for local DNA denaturation, reducing non-specific binding of probes and avoiding harsh treatments such as heat denaturation. GOLD FISH relies on Cas9 cleaving target DNA sequences and avoids the high nuclear background associated with other genome labeling methods that rely on Cas9 binding. The excellent signal brightness and specificity enable us to image non-repetitive genomic DNA loci and analyze the conformational differences between active and inactive X chromosomes. Finally, GOLD FISH could be used for rapid identification of HER2 gene amplification in a patient tissue.

Published

2020

14. Sequential Activation of Guide RNAs to Enable Successive CRISPR-Cas9 Activities

Author

Bradley J. Merrill, Matthew S. MacDougall, Alexander R. Terry, Hannah Pennington, Maureen Regan, Cody Hasty, and Ryan Clarke

Subjects

Streptococcus pyogenes, Green Fluorescent Proteins, Computational biology, Biology, Article, 03 medical and health sciences, Synthetic biology, Mice, 0302 clinical medicine, Genome editing, Genes, Reporter, CRISPR-Associated Protein 9, CRISPR, Animals, Humans, Clustered Regularly Interspaced Short Palindromic Repeats, Guide RNA, Promoter Regions, Genetic, Molecular Biology, Base Pairing, 030304 developmental biology, Gene Editing, 0303 health sciences, Base Sequence, Cas9, Mouse Embryonic Stem Cells, Cell Biology, HEK293 Cells, Proof of concept, Interfacing, Regulatory sequence, Nucleic Acid Conformation, CRISPR-Cas Systems, 030217 neurology & neurosurgery, Plasmids, RNA, Guide, Kinetoplastida

Abstract

Currently, either highly multiplexed genetic manipulations can be delivered to mammalian cells all at once, or extensive engineering of gene regulatory sequences can be used to conditionally activate a few manipulations. Here, we provide proof-of-principle for a new system enabling multiple genetic manipulations to be executed as a preprogrammed cascade of events. The system leverages the programmability of the S. pyogenes Cas9 and is based on flexible arrangements of individual modules of activity. The basic module consists of an inactive single guide RNA (sgRNA) -like component that is converted to an active state through the effects of another sgRNA. Modules can be arranged to bring about an algorithmic program of sequential genetic manipulations without the need for engineering cell type specific promoters or gene regulatory sequences. With the expanding diversity of available tools that utilize spCas9, this sgRNA-based system provides multiple levels of interfacing with mammalian cell biology.

Published

2020

15. Cleavage of viral DNA by restriction endonucleases stimulates the type II CRISPR-Cas immune response.

Author

Maguin, Pascal, Varble, Andrew, Modell, Joshua W., and Marraffini, Luciano A.

Subjects

*DNA restriction enzymes, *VIRAL DNA, *ENDONUCLEASES, *NUCLEOTIDE sequence, *CRISPRS, *IMMUNE response, *DNA modification & restriction

Abstract

Prokaryotic organisms have developed multiple defense systems against phages; however, little is known about whether and how these interact with each other. Here, we studied the connection between two of the most prominent prokaryotic immune systems: restriction-modification and CRISPR. While both systems employ enzymes that cleave a specific DNA sequence of the invader, CRISPR nucleases are programmed with phage-derived spacer sequences, which are integrated into the CRISPR locus upon infection. We found that restriction endonucleases provide a short-term defense, which is rapidly overcome through methylation of the phage genome. In a small fraction of the cells, however, restriction results in the acquisition of spacer sequences from the cleavage site, which mediates a robust type II-A CRISPR-Cas immune response against the methylated phage. This mechanism is reminiscent of eukaryotic immunity in which the innate response offers a first temporary line of defense and also activates a second and more robust adaptive response. [Display omitted] • Restriction nucleases generate free DNA ends and stop the viral lytic cycle • DNA repair nucleases degrade DNA ends to generate new ones • Type II CRISPR-Cas integrases acquire new spacers from free DNA ends • Bacteria are immunized to neutralize restriction escapers with methylated genomes Restriction and CRISPR-Cas nucleases cleave phage DNA. Maguin et al. show how these are coordinated to defend bacteria from infection. Restriction provides initial protection and also generates free dsDNA ends for the acquisition of spacers by CRISPR-Cas systems. Spacers guide CRISPR nucleases to destroy methylated phage DNA that bypasses restriction. [ABSTRACT FROM AUTHOR]

Published

2022

16. Improving the efficiency of CRISPR-Cas12a-based genome editing with site-specific covalent Cas12a-crRNA conjugates

Author

Bo Zhang, Jiazhi Hu, Xiaoqin Gao, Heqi Chen, Xinyu Ling, Jianhang Yin, Yujia Huang, Liying Chang, Tao Liu, and Yi Zuo

Subjects

CRISPR-Associated Proteins, Green Fluorescent Proteins, Computational biology, In Vitro Techniques, Mice, Bacterial Proteins, Genome editing, Tandem Mass Spectrometry, Gene knockin, Escherichia coli, Animals, Humans, CRISPR, Acidaminococcus, Multiplex, Gene Knock-In Techniques, Molecular Biology, Gene Editing, Trans-activating crRNA, Nuclease, Endodeoxyribonucleases, Receptors, Chimeric Antigen, biology, Cas9, RNA, DNA, Cell Biology, Endonucleases, HEK293 Cells, Genetic Techniques, Mutagenesis, biology.protein, CRISPR-Cas Systems, K562 Cells

Abstract

Summary The CRISPR-Cas12a system shows unique features compared with widely used Cas9, making it an attractive and potentially more precise alternative. However, the adoption of this system has been hindered by its relatively low editing efficiency. Guided by physical chemical principles, we covalently conjugated 5′ terminal modified CRISPR RNA (crRNA) to a site-specifically modified Cas12a through biorthogonal chemical reaction. The genome editing efficiency of the resulting conjugated Cas12a complex (cCas12a) was substantially higher than that of the wild-type complex. We also demonstrated that cCas12a could be used for precise gene knockin and multiplex gene editing in a chimeric antigen receptor T cell preparation with efficiency much higher than that of the wild-type system. Overall, our findings indicate that covalently linking Cas nuclease and crRNA is an effective approach to improve the Cas12a-based genome editing system and could potentially provide an insight into engineering other Cas family members with low efficiency as well.

Published

2021

17. Engineered miniature CRISPR-Cas system for mammalian genome regulation and editing

Author

Lei S. Qi, Augustine Chemparathy, Muneaki Nakamura, Hannah R. Kempton, Leiping Zeng, Stephen Shang, and Xiaoshu Xu

Subjects

Regulation of gene expression, Genome editing, Cas9, CRISPR, Cell Biology, Guide RNA, Protein engineering, Computational biology, Biology, Molecular Biology, Gene knockout, Genome engineering

Abstract

Summary Compact and versatile CRISPR-Cas systems will enable genome engineering applications through high-efficiency delivery in a wide variety of contexts. Here, we create an efficient miniature Cas system (CasMINI) engineered from the type V-F Cas12f (Cas14) system by guide RNA and protein engineering, which is less than half the size of currently used CRISPR systems (Cas9 or Cas12a). We demonstrate that CasMINI can drive high levels of gene activation (up to thousands-fold increases), while the natural Cas12f system fails to function in mammalian cells. We show that the CasMINI system has comparable activities to Cas12a for gene activation, is highly specific, and allows robust base editing and gene editing. We expect that CasMINI can be broadly useful for cell engineering and gene therapy applications ex vivo and in vivo.

Published

2021

18. Conformational control of Cas9 by CRISPR hybrid RNA-DNA guides mitigates off-target activity in T cells

Author

David B. Nyer, Lynda M. Banh, Megan van Overbeek, Tomer Rotstein, Elaine Lau, Kevin Baek, Chris R. Fuller, Martin Pacesa, Euan M. Slorach, Andrew May, Martin Jinek, Mckenzi S. Toh, B. Kohrs, Jason Gibson, Bastien Vidal, Matthew J. Irby, Arthur L.G. Owen, Paul Daniel Donohoue, and Peter Cameron

Subjects

T-Lymphocytes, CRISPR-Associated Proteins, Allosteric regulation, Molecular Conformation, Computational biology, Cleavage (embryo), Structure-Activity Relationship, 03 medical and health sciences, 0302 clinical medicine, Genome editing, CRISPR-Associated Protein 9, Humans, CRISPR, Molecular Biology, 030304 developmental biology, Gene Editing, 0303 health sciences, Nuclease, Genome, biology, Cas9, DNA–DNA hybridization, DNA, Genomics, Cell Biology, Endonucleases, Genetic Techniques, Duplex (building), Leukocytes, Mononuclear, biology.protein, CRISPR-Cas Systems, 030217 neurology & neurosurgery, RNA, Guide, Kinetoplastida

Abstract

Summary The off-target activity of the CRISPR-associated nuclease Cas9 is a potential concern for therapeutic genome editing applications. Although high-fidelity Cas9 variants have been engineered, they exhibit varying efficiencies and have residual off-target effects, limiting their applicability. Here, we show that CRISPR hybrid RNA-DNA (chRDNA) guides provide an effective approach to increase Cas9 specificity while preserving on-target editing activity. Across multiple genomic targets in primary human T cells, we show that 2′-deoxynucleotide (dnt) positioning affects guide activity and specificity in a target-dependent manner and that this can be used to engineer chRDNA guides with substantially reduced off-target effects. Crystal structures of DNA-bound Cas9-chRDNA complexes reveal distorted guide-target duplex geometry and allosteric modulation of Cas9 conformation. These structural effects increase specificity by perturbing DNA hybridization and modulating Cas9 activation kinetics to disfavor binding and cleavage of off-target substrates. Overall, these results pave the way for utilizing customized chRDNAs in clinical applications.

Published

2021

19. CRISPR-based peptide library display and programmable microarray self-assembly for rapid quantitative protein binding assays

Author

Stephen J. Elledge, Ellen Shrock, and Karl W. Barber

Subjects

Gene Editing, Cas9, Cell Biology, Computational biology, Biology, Epitopes, chemistry.chemical_compound, Epitope mapping, Genome editing, chemistry, Mutagenesis, Peptide Library, Protein microarray, Humans, CRISPR, Guide RNA, CRISPR-Cas Systems, Peptide library, Molecular Biology, DNA, Protein Binding, RNA, Guide, Kinetoplastida

Abstract

CRISPR-inspired systems have been extensively developed for applications in genome editing and nucleic acid detection. Here, we introduce a CRISPR-based peptide display technology to facilitate customized, high-throughput in vitro protein interaction studies. We show that bespoke peptide libraries fused to catalytically inactive Cas9 (dCas9) and barcoded with unique single guide RNA (sgRNA) molecules self-assemble from a single mixed pool to programmable positions on a DNA microarray surface for rapid, multiplexed binding assays. We develop dCas9-displayed saturation mutagenesis libraries to characterize antibody-epitope binding for a commercial anti-FLAG monoclonal antibody and human serum antibodies. We also show that our platform can be used for viral epitope mapping and exhibits promise as a multiplexed diagnostics tool. Our CRISPR-based peptide display platform and the principles of complex library self-assembly using dCas9 could be adapted for rapid interrogation of varied customized protein libraries or biological materials assembly using DNA scaffolding.

Published

2021

20. The Center Cannot Hold: NRF2 Battles Ferroptosis in the 3rd Dimension

Author

Thales Papagiannakopoulos and Warren L. Wu

Subjects

0303 health sciences, 03 medical and health sciences, 0302 clinical medicine, Extramural, Cas9, Ferroptosis, CRISPR, Cell Biology, Biology, Molecular Biology, Neuroscience, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Takahashi et al. (2020) conduct a focused CRISPR/Cas9 screen against NRF2 target and other redox regulatory genes in both 2D- and 3D-culture systems, uncovering a vulnerability of spheroid cancer cells deprived of extracellular matrix to undergo ferroptosis.

Published

2020

21. The Revolution Continues: Newly Discovered Systems Expand the CRISPR-Cas Toolkit

Author

Ramya Sundaresan, Dipali G. Sashital, Rakhi Rajan, Karthik Murugan, and Kesavan Babu

Subjects

Models, Molecular, 0301 basic medicine, Transcription, Genetic, Protein Conformation, Computational biology, Biology, Diagnostic tools, Article, 03 medical and health sciences, Endonuclease, Bacterial Proteins, Protein Domains, Genome editing, Humans, CRISPR, Bacteriophages, Clustered Regularly Interspaced Short Palindromic Repeats, Guide RNA, Molecular Biology, Gene Editing, Genetics, Genome, Bacteria, Cas9, Cell Biology, Endonucleases, eye diseases, humanities, 030104 developmental biology, embryonic structures, biology.protein, CRISPR-Cas Systems, Mobile genetic elements, Genetic Engineering, human activities, RNA, Guide, Kinetoplastida

Abstract

CRISPR–Cas systems defend prokaryotes against bacteriophages and mobile genetic elements and serve as the basis for revolutionary tools for genetic engineering. Class 2 CRISPR–Cas systems use single Cas endonucleases paired with guide RNAs to cleave complementary nucleic acid targets, enabling programmable sequence-specific targeting with minimal machinery. Recent discoveries of previously unidentified CRISPR–Cas systems have uncovered a deep reservoir of potential biotechnological tools beyond the well-characterized Type II Cas9 systems. Here we review the current mechanistic understanding of newly discovered single-protein Cas endonucleases. Comparison of these Cas effectors reveals substantial mechanistic diversity, underscoring the phylogenetic divergence of related CRISPR–Cas systems. This diversity has enabled further expansion of CRISPR–Cas biotechnological toolkits, with wide-ranging applications from genome editing to diagnostic tools based on various Cas endonuclease activities. These advances highlight the exciting prospects for future tools based on the continually expanding set of CRISPR–Cas systems.

Published

2017

22. Mutations in Cas9 Enhance the Rate of Acquisition of Viral Spacer Sequences during the CRISPR-Cas Immune Response

Author

Marija Vucelja, Addison V. Wright, Luciano A. Marraffini, Robert Heler, David Bikard, and Jennifer A. Doudna

Subjects

0301 basic medicine, Staphylococcus aureus, Time Factors, Genotype, CRISPR-Associated Proteins, 030106 microbiology, adaptation, Adaptive Immunity, Biology, Medical and Health Sciences, Article, Substrate Specificity, 03 medical and health sciences, chemistry.chemical_compound, Plasmid, bacteriophage, Bacterial Proteins, CRISPR-Associated Protein 9, CRISPR, Clustered Regularly Interspaced Short Palindromic Repeats, Viral, CRISPR-Cas, Cas9, Molecular Biology, Genetics, Trans-activating crRNA, CRISPR interference, Intergenic, High-Throughput Nucleotide Sequencing, DNA, Cell Biology, Biological Sciences, Endonucleases, Acquired immune system, Phenotype, 030104 developmental biology, chemistry, DNA, Viral, Host-Pathogen Interactions, Mutation, CRISPR Loci, horizontal gene transfer, DNA, Intergenic, spacer acquisition, CRISPR-Cas Systems, Developmental Biology

Abstract

Clustered regularly interspaced short palindromic repeat (CRISPR) loci and their associated (Cas) proteins encode a prokaryotic immune system that protects against viruses and plasmids. Upon infection, a low fraction of cells acquire short DNA sequences from the invader. These sequences (spacers) are integrated in between the repeats of the CRISPR locus and immunize the host against the matching invader. Spacers specify the targets of the CRISPR immune response through transcription into short RNA guides that direct Cas nucleases to the inavding DNA molecules. Here we performed random mutagenesis of the RNA-guided Cas9 nuclease to look for variants that provide enhanced immunity against viral infection. We identified a mutation, I473F, which increases the rate of spacer acquisition by more than two orders of magnitude. Our results highlight the role of Cas9 during CRISPR immunization and provide a useful tool to study this rare process and develop it as a biotechnological application.

Published

2017

23. Active Genetic Neutralizing Elements for Halting or Deleting Gene Drives

Author

Carissa Klanseck, Sara Sanz Juste, Stephanie R. Heimler, Valentino M. Gantz, Ankush Auradkar, John M. Marshall, Emily A. Bulger, Anna Buchman, Ethan Bier, Lauren Ashley Miller, Omar S. Akbari, Sarah Leahy, Jared B. Bennett, and Xiang-Ru S. Xu

Subjects

Transgene, Green Fluorescent Proteins, Inheritance Patterns, Computational biology, Target population, Biology, Chromosomes, 03 medical and health sciences, 0302 clinical medicine, CRISPR-Associated Protein 9, CRISPR, Animals, Transgenes, Molecular Biology, Gene, 030304 developmental biology, 0303 health sciences, Cas9, Gene Drive Technology, Cell Biology, Gene drive, Drosophila melanogaster, Mutagenesis, Female, Trans-acting, 030217 neurology & neurosurgery, Gene Deletion, RNA, Guide, Kinetoplastida

Abstract

CRISPR-Cas9-based gene drive systems possess the inherent capacity to spread progressively throughout target populations. Here we describe two self-copying (or active) guide RNA-only genetic elements, called e-CHACRs and ERACRs. These elements use Cas9 produced in trans by a gene drive either to inactivate the cas9 transgene (e-CHACRs) or to delete and replace the gene drive (ERACRs). e-CHACRs can be inserted at various genomic locations and carry two or more gRNAs, the first copying the e-CHACR and the second mutating and inactivating the cas9 transgene. Alternatively, ERACRs are inserted at the same genomic location as a gene drive, carrying two gRNAs that cut on either side of the gene drive to excise it. e-CHACRs efficiently inactivate Cas9 and can drive to completion in cage experiments. Similarly, ERACRs, particularly those carrying a recoded cDNA-restoring endogenous gene activity, can drive reliably to fully replace a gene drive. We compare the strengths of these two systems.

Published

2019

24. Harnessing the Power of Proteolysis for Targeted Protein Inactivation

Author

Dane Mohl, Rati Verma, and Raymond J. Deshaies

Subjects

Morpholino, Computational biology, Protein degradation, Biology, Protein Engineering, Morpholinos, 03 medical and health sciences, 0302 clinical medicine, CRISPR, Animals, Humans, Clustered Regularly Interspaced Short Palindromic Repeats, Molecular Biology, Gene, 030304 developmental biology, Gene Editing, 0303 health sciences, Gene knockdown, Cas9, RNA, Cell Biology, Transport protein, Protein Transport, Proteolysis, CRISPR-Cas Systems, Genetic Engineering, 030217 neurology & neurosurgery

Abstract

Two decades into the twenty-first century, a confluence of breakthrough technologies wielded at the molecular level is presenting biologists with unique opportunities to unravel the complexities of the cellular world. CRISPR/Cas9 allows gene knock-outs, knock-ins, and single-base editing at chromosomal loci. RNA-based tools such as siRNA, antisense oligos, and morpholinos can be used to silence expression of specific genes. Meanwhile, protein knockdown tools that draw inspiration from natural regulatory mechanisms and facilitate elimination of native or degron-tagged proteins from cells are rapidly emerging. The acute and reversible reduction in protein levels enabled by these methods allows for precise determination of loss-of-function phenotypes free from secondary effects or compensatory adaptation that can confound nucleic-acid-based methods that involve slow depletion or permanent loss of a protein. In this Review, we summarize the ingenious ways biologists have exploited natural mechanisms for protein degradation to direct the elimination of specific proteins at will. This has led to advancements not only in basic research but also in the therapeutic space with the introduction of PROTACs into clinical trials for cancer patients.

Published

2019

25. Plasticity of the Cullin-RING Ligase Repertoire Shapes Sensitivity to Ligand-Induced Protein Degradation

Author

Georg E. Winter, Matthias Brand, Sophie Bauer, Jörg Menche, Celine Sin, Martin G. Jaeger, André C. Mueller, Cristina Mayor-Ruiz, and Alexander Hanzl

Subjects

0303 health sciences, Effector, Cas9, COP9 Signalosome Complex, Chemical biology, Cell Biology, Protein degradation, Biology, Cullin Proteins, Small molecule, Cell biology, 03 medical and health sciences, 0302 clinical medicine, Proteolysis, biology.protein, CRISPR, Humans, COP9 signalosome, Molecular Biology, 030217 neurology & neurosurgery, Cullin, 030304 developmental biology, Transcription Factors

Abstract

Inducing protein degradation via small molecules is a transformative therapeutic paradigm. Although structural requirements of target degradation are emerging, mechanisms determining the cellular response to small-molecule degraders remain poorly understood. To systematically delineate effectors required for targeted protein degradation, we applied genome-scale CRISPR/Cas9 screens for five drugs that hijack different substrate receptors (SRs) of cullin RING ligases (CRLs) to induce target proteolysis. We found that sensitivity to small-molecule degraders is dictated by shared and drug-specific modulator networks, including the COP9 signalosome and the SR exchange factor CAND1. Genetic or pharmacologic perturbation of these effectors impairs CRL plasticity and arrests a wide array of ligases in a constitutively active state. Resulting defects in CRL decommissioning prompt widespread CRL auto-degradation that confers resistance to multiple degraders. Collectively, our study informs on regulation and architecture of CRLs amenable for targeted protein degradation and outlines biomarkers and putative resistance mechanisms for upcoming clinical investigation.

Published

2019

26. Structures of Neisseria meningitidis Cas9 Complexes in Catalytically Poised and Anti-CRISPR-Inhibited States

Author

Jizhong Lou, Jing Yang, Nadia Amrani, Gang Sheng, Kangkang Wang, Erik J. Sontheimer, Jiuyu Wang, Xue Huang, Liang Liu, Chao Liu, Min Wang, Zhi Cheng, Alireza Edraki, Yanhua Yang, Raed Ibraheim, Yanli Wang, and Wei Sun

Subjects

Stereochemistry, Protein domain, Neisseria meningitidis, Cleavage (embryo), Catalysis, Article, 03 medical and health sciences, Structure-Activity Relationship, Viral Proteins, 0302 clinical medicine, Genome editing, Protein Domains, CRISPR-Associated Protein 9, Escherichia coli, CRISPR, Bacteriophages, Clustered Regularly Interspaced Short Palindromic Repeats, Binding site, Molecular Biology, 030304 developmental biology, 0303 health sciences, Nuclease, Binding Sites, biology, Cas9, Active site, Cell Biology, DNA, biology.protein, CRISPR-Cas Systems, 030217 neurology & neurosurgery, Protein Binding, RNA, Guide, Kinetoplastida

Abstract

Summary High-resolution Cas9 structures have yet to reveal catalytic conformations due to HNH nuclease domain positioning away from the cleavage site. Nme1Cas9 and Nme2Cas9 are compact nucleases for in vivo genome editing. Here, we report structures of meningococcal Cas9 homologs in complex with sgRNA, dsDNA, or the AcrIIC3 anti-CRISPR protein. DNA-bound structures represent an early step of target recognition, a later HNH pre-catalytic state, the HNH catalytic state, and a cleaved-target-DNA-bound state. In the HNH catalytic state of Nme1Cas9, the active site is seen poised at the scissile phosphodiester linkage of the target strand, providing a high-resolution view of the active conformation. The HNH active conformation activates the RuvC domain. Our structures explain how Nme1Cas9 and Nme2Cas9 read distinct PAM sequences and how AcrIIC3 inhibits Nme1Cas9 activity. These structures provide insights into Cas9 domain rearrangements, guide-target engagement, cleavage mechanism, and anti-CRISPR inhibition, facilitating the optimization of these genome-editing platforms.

Published

2019

27. Impact of chromatin context on Cas9-induced DNA double-strand break repair pathway balance

Author

Bas van Steensel, René H. Medema, Ruben Schep, Ben Morris, Tom van Schaik, Robin H. van der Weide, Xabier Vergara, Roderick L. Beijersbergen, Jeroen van den Berg, Eva K. Brinkman, Daniel Peric-Hupkes, Stefano G. Manzo, Christ Leemans, and Cell biology

Subjects

DNA End-Joining Repair, DNA Repair, Euchromatin, DNA repair, Heterochromatin, Context (language use), Biology, Article, 03 medical and health sciences, 0302 clinical medicine, INDEL Mutation, Genome editing, CRISPR-Associated Protein 9, Humans, DNA Breaks, Double-Stranded, Molecular Biology, NHEJ, SSTR, 030304 developmental biology, Gene Rearrangement, 0303 health sciences, Base Sequence, Genome, Human, Cas9, reporter assay, fungi, Reproducibility of Results, Cell Biology, Chromatin Assembly and Disassembly, Chromatin, Double Strand Break Repair, Cell biology, Kinetics, CRISPR, MMEJ, double strand break, K562 Cells, nuclear lamina, 030217 neurology & neurosurgery, Protein Binding

Abstract

Summary DNA double-strand break (DSB) repair is mediated by multiple pathways. It is thought that the local chromatin context affects the pathway choice, but the underlying principles are poorly understood. Using a multiplexed reporter assay in combination with Cas9 cutting, we systematically measure the relative activities of three DSB repair pathways as a function of chromatin context in >1,000 genomic locations. This reveals that non-homologous end-joining (NHEJ) is broadly biased toward euchromatin, while the contribution of microhomology-mediated end-joining (MMEJ) is higher in specific heterochromatin contexts. In H3K27me3-marked heterochromatin, inhibition of the H3K27 methyltransferase EZH2 reverts the balance toward NHEJ. Single-stranded template repair (SSTR), often used for precise CRISPR editing, competes with MMEJ and is moderately linked to chromatin context. These results provide insight into the impact of chromatin on DSB repair pathway balance and guidance for the design of Cas9-mediated genome editing experiments., Graphical abstract, Highlights • Sequencing-based reporter detects activities of multiple DSB repair pathways • Multiplexing approach to integrate reporter in >1,000 genomic locations • Overlay with epigenome data reveals effects of chromatin context on pathway balance • Pathway balance differs between heterochromatin and euchromatin, Schep et al. designed a reporter to probe the activities of three DNA double-strand break repair pathways. Integration of this reporter in >1,000 genomic locations in a human cell line provided a detailed view of the impact of local chromatin context on the balance between the repair pathways.

Published

2021

28. Interrogation of the dynamic properties of higher-order heterochromatin using CRISPR-dCas9.

Author

Gao, Yuchen, Han, Mengting, Shang, Stephen, Wang, Haifeng, and Qi, Lei S.

Subjects

*HETEROCHROMATIN, *STRUCTURAL stability, *CHROMOSOMES, *DNA, *POLYMERS, *CHROMATIN

Abstract

Eukaryotic chromosomes feature large regions of compact, repressed heterochromatin hallmarked by Heterochromatin Protein 1 (HP1). HP1 proteins play multi-faceted roles in shaping heterochromatin, and in cells, HP1 tethering to individual gene promoters leads to epigenetic modifications and silencing. However, emergent properties of HP1 at supranucleosomal scales remain difficult to study in cells because of a lack of appropriate tools. Here, we develop CRISPR-engineered chromatin organization (EChO), combining live-cell CRISPR imaging with inducible large-scale recruitment of chromatin proteins to native genomic targets. We demonstrate that human HP1α tiled across kilobase-scale genomic DNA form novel contacts with natural heterochromatin, integrates two distantly targeted regions, and reversibly changes chromatin from a diffuse to compact state. The compact state exhibits delayed disassembly kinetics and represses transcription across over 600 kb. These findings support a polymer model of HP1α-mediated chromatin regulation and highlight the utility of CRISPR-EChO in studying supranucleosomal chromatin organization in living cells. [Display omitted] • CRISPR-dCas9 can be modified to tile chromatin proteins over large genomic regions • dCas9-HP1α tiling facilitates long-range chromatin interactions in cis and in trans • Polymers of HP1α impede distal transcription and confer structural stability • dCas9-HP1α tiling allows chromatin co-localization and compaction Technologies to manipulate and study 3D genome organization in living cells remain scarce. Gao et al. develop a CRISPR-dCas9-based approach for inducibly tiling chromatin proteins across kilobase-scale regions of the chromosome, uncovering the direct role of HP1α in dynamically mediating long-range chromatin interactions, chromatin compaction, and transcriptional repression. [ABSTRACT FROM AUTHOR]

Published

2021

29. CRISPR-based peptide library display and programmable microarray self-assembly for rapid quantitative protein binding assays.

Author

Barber, Karl W., Shrock, Ellen, and Elledge, Stephen J.

Subjects

*BINDING site assay, *CRISPRS, *PEPTIDE amphiphiles, *MONOCLONAL antibodies, *NUCLEIC acids, *BIOMATERIALS, *PROTEIN-protein interactions

Abstract

CRISPR-inspired systems have been extensively developed for applications in genome editing and nucleic acid detection. Here, we introduce a CRISPR-based peptide display technology to facilitate customized, high-throughput in vitro protein interaction studies. We show that bespoke peptide libraries fused to catalytically inactive Cas9 (dCas9) and barcoded with unique single guide RNA (sgRNA) molecules self-assemble from a single mixed pool to programmable positions on a DNA microarray surface for rapid, multiplexed binding assays. We develop dCas9-displayed saturation mutagenesis libraries to characterize antibody-epitope binding for a commercial anti-FLAG monoclonal antibody and human serum antibodies. We also show that our platform can be used for viral epitope mapping and exhibits promise as a multiplexed diagnostics tool. Our CRISPR-based peptide display platform and the principles of complex library self-assembly using dCas9 could be adapted for rapid interrogation of varied customized protein libraries or biological materials assembly using DNA scaffolding. [Display omitted] • dCas9-peptide fusions are barcoded with unique sgRNAs for peptide library studies • Peptides are directed to sgRNA-complementary sequences on a template DNA microarray • dCas9-peptide mixtures self-assemble on microarrays in a technique called PICASSO • PICASSO enables quantitative antibody binding characterization and epitope mapping To facilitate custom peptide library studies, Barber et al. fuse peptide collections to dCas9 barcoded with unique sgRNA sequences. They demonstrate that, from mixed pools, dCas9-peptide fusions self-assemble to positions on a DNA microarray surface complementary to their sgRNA barcodes and they use the resulting microarrays to characterize antibody-epitope binding. [ABSTRACT FROM AUTHOR]

Published

2021

30. Conformational control of Cas9 by CRISPR hybrid RNA-DNA guides mitigates off-target activity in T cells.

Author

Donohoue, Paul D., Pacesa, Martin, Lau, Elaine, Vidal, Bastien, Irby, Matthew J., Nyer, David B., Rotstein, Tomer, Banh, Lynda, Toh, Mckenzi S., Gibson, Jason, Kohrs, Bryan, Baek, Kevin, Owen, Arthur L.G., Slorach, Euan M., van Overbeek, Megan, Fuller, Christopher K., May, Andrew P., Jinek, Martin, and Cameron, Peter

Subjects

*T cells, *ALLOSTERIC regulation, *GENOME editing, *CRYSTAL structure, *CRISPRS

Abstract

The off-target activity of the CRISPR-associated nuclease Cas9 is a potential concern for therapeutic genome editing applications. Although high-fidelity Cas9 variants have been engineered, they exhibit varying efficiencies and have residual off-target effects, limiting their applicability. Here, we show that CRISPR hybrid RNA-DNA (chRDNA) guides provide an effective approach to increase Cas9 specificity while preserving on-target editing activity. Across multiple genomic targets in primary human T cells, we show that 2′-deoxynucleotide (dnt) positioning affects guide activity and specificity in a target-dependent manner and that this can be used to engineer chRDNA guides with substantially reduced off-target effects. Crystal structures of DNA-bound Cas9-chRDNA complexes reveal distorted guide-target duplex geometry and allosteric modulation of Cas9 conformation. These structural effects increase specificity by perturbing DNA hybridization and modulating Cas9 activation kinetics to disfavor binding and cleavage of off-target substrates. Overall, these results pave the way for utilizing customized chRDNAs in clinical applications. [Display omitted] • chRDNAs improve Cas9 specificity while preserving on-target editing efficiency • 2′-Deoxynucleotide positioning affects guide specificity in a target-dependent manner • chRDNAs cause distorted guide-target DNA duplex geometry and R-loop destabilization • chRDNAs slow Cas9 cleavage rates and promote dissociation of off-target substrates Cas9 off-target activity remains a concern for therapeutics. Donohoue, Pacesa, et al. demonstrate that selective 2′-deoxynucleotide modifications of the Cas9 guide reduce off-target activity in primary T cells. These CRISPR hybrid RNA-DNAs (chRDNAs) increase specificity by distorting the guide-substrate duplex, which disfavors the binding and cleavage of off-target substrates. [ABSTRACT FROM AUTHOR]

Published

2021

31. DNA Targeting by a Minimal CRISPR RNA-Guided Cascade

Author

David W. Taylor, Eva Nogales, Jack E. Kornfeld, Jennifer A. Doudna, and Megan L. Hochstrasser

Subjects

Models, Molecular, Protein Conformation, alpha-Helical, 0301 basic medicine, Amino Acid Motifs, Gene Expression, Computational biology, Biology, Article, Substrate Specificity, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Protein structure, Bacterial Proteins, Genome editing, Operon, Escherichia coli, CRISPR, Protein Interaction Domains and Motifs, Desulfovibrio vulgaris, Cloning, Molecular, Molecular Biology, Gene Editing, Genetics, Trans-activating crRNA, Binding Sites, Cas9, Cryoelectron Microscopy, RNA, DNA, Cell Biology, Endonucleases, Recombinant Proteins, Kinetics, RNA, Bacterial, 030104 developmental biology, chemistry, Nucleic acid, Nucleic Acid Conformation, CRISPR-Cas Systems, 030217 neurology & neurosurgery, Protein Binding, RNA, Guide, Kinetoplastida

Abstract

Bacteria employ surveillance complexes guided by CRISPR (clustered, regularly interspaced, short palindromic repeats) RNAs (crRNAs) to target foreign nucleic acids for destruction. Although most type I and type III CRISPR systems require four or more distinct proteins to form multi-subunit surveillance complexes, the type I-C systems use just three proteins to achieve crRNA maturation and double-stranded DNA target recognition. We show that each protein plays multiple functional and structural roles: Cas5c cleaves pre-crRNAs and recruits Cas7 to position the RNA guide for DNA binding and unwinding by Cas8c. Cryoelectron microscopy reconstructions of free and DNA-bound forms of the Cascade/I-C surveillance complex reveal conformational changes that enable R-loop formation with distinct positioning of each DNA strand. This streamlined type I-C system explains how CRISPR pathways can evolve compact structures that retain full functionality as RNA-guided DNA capture platforms.

Published

2016

32. DNA Repair Profiling Reveals Nonrandom Outcomes at Cas9-Mediated Breaks

Author

Scott Gradia, Matthew S. Thompson, Megan van Overbeek, Gregory R. Hoffman, Carsten Russ, Elizabeth Frias, Christopher D. Nye, Andrew May, John S. Reece-Hoyes, Daniel Capurso, Bastien Vidal, Chris R. Fuller, Jiashun Zheng, and Matthew Merrill Carter

Subjects

0301 basic medicine, DNA End-Joining Repair, Time Factors, DNA repair, Computational biology, Biology, Transfection, 03 medical and health sciences, chemistry.chemical_compound, Bacterial Proteins, Genome editing, CRISPR-Associated Protein 9, Humans, DNA Breaks, Double-Stranded, Molecular Biology, Gene, Gene Editing, Genetics, Cas9, Gene Expression Profiling, Cell Biology, Endonucleases, HCT116 Cells, HEK293 Cells, 030104 developmental biology, chemistry, RNA Interference, DNA mismatch repair, Human genome, CRISPR-Cas Systems, K562 Cells, DNA, RNA, Guide, Kinetoplastida

Abstract

Summary The repair outcomes at site-specific DNA double-strand breaks (DSBs) generated by the RNA-guided DNA endonuclease Cas9 determine how gene function is altered. Despite the widespread adoption of CRISPR-Cas9 technology to induce DSBs for genome engineering, the resulting repair products have not been examined in depth. Here, the DNA repair profiles of 223 sites in the human genome demonstrate that the pattern of DNA repair following Cas9 cutting at each site is nonrandom and consistent across experimental replicates, cell lines, and reagent delivery methods. Furthermore, the repair outcomes are determined by the protospacer sequence rather than genomic context, indicating that DNA repair profiling in cell lines can be used to anticipate repair outcomes in primary cells. Chemical inhibition of DNA-PK enabled dissection of the DNA repair profiles into contributions from c-NHEJ and MMEJ. Finally, this work elucidates a strategy for using "error-prone" DNA-repair machinery to generate precise edits.

Published

2016

33. Identifying and Visualizing Functional PAM Diversity across CRISPR-Cas Systems

Author

Kenneth R. Maksimchuk, Ryan T. Leenay, Rodolphe Barrangou, Rebecca A. Slotkowski, Alexandra E. Briner, Ahmed A. Gomaa, Roma N. Agrawal, and Chase L. Beisel

Subjects

0301 basic medicine, Protein family, CRISPR-Associated Proteins, Bacillus, Computational biology, Biology, medicine.disease_cause, Article, Microbiology, 03 medical and health sciences, 0302 clinical medicine, Escherichia coli, medicine, Streptococcus thermophilus, CRISPR, Francisella novicida, Francisella, Molecular Biology, Cas9, Extramural, Cell Biology, High-Throughput Screening Assays, Protein Structure, Tertiary, Protospacer adjacent motif, 030104 developmental biology, CRISPR-Cas Systems, 030217 neurology & neurosurgery

Abstract

CRISPR-Cas adaptive immune systems in prokaryotes boast a diversity of protein families and mechanisms of action, where most systems rely on protospacer-adjacent motifs (PAMs) for DNA target recognition. Here, we developed an in vivo, positive, and tunable screen termed PAM-SCANR (PAM screen achieved by NOT-gate repression) to elucidate functional PAMs as well as an interactive visualization scheme termed the PAM wheel to convey individual PAM sequences and their activities. PAM-SCANR and the PAM wheel identified known functional PAMs while revealing complex sequence-activity landscapes for the Bacillus halodurans I-C (Cascade), Escherichia coli I-E (Cascade), Streptococcus thermophilus II-A CRISPR1 (Cas9), and Francisella novicida V-A (Cpf1) systems. The PAM wheel was also readily applicable to existing high-throughput screens and garnered insights into SpyCas9 and SauCas9 PAM diversity. These tools offer powerful means of elucidating and visualizing functional PAMs toward accelerating our ability to understand and exploit the multitude of CRISPR-Cas systems in nature.

Published

2016

34. Structural Plasticity of PAM Recognition by Engineered Variants of the RNA-Guided Endonuclease Cas9

Author

Katja Bargsten, Martin Jinek, Carolin Anders, University of Zurich, and Jinek, Martin

Subjects

0301 basic medicine, 610 Medicine & health, medicine.disease_cause, Article, 1307 Cell Biology, 03 medical and health sciences, Endonuclease, chemistry.chemical_compound, Genome editing, Bacterial Proteins, parasitic diseases, 10019 Department of Biochemistry, 1312 Molecular Biology, medicine, Molecular Biology, chemistry.chemical_classification, Genetics, Mutation, biology, Cas9, RNA, Cell Biology, Endonucleases, Amino acid, Protospacer adjacent motif, 030104 developmental biology, chemistry, biology.protein, 570 Life sciences, DNA, Intergenic, CRISPR-Cas Systems, DNA, RNA, Guide, Kinetoplastida

Abstract

The RNA-guided endonuclease Cas9 from Streptococcus pyogenes (SpCas9) forms the core of a powerful genome editing technology. DNA cleavage by SpCas9 is dependent on the presence of a 5'-NGG-3' protospacer adjacent motif (PAM) in the target DNA, restricting the choice of targetable sequences. To address this limitation, artificial SpCas9 variants with altered PAM specificities have recently been developed. Here we report crystal structures of the VQR, EQR, and VRER SpCas9 variants bound to target DNAs containing their preferred PAM sequences. The structures reveal that the non-canonical PAMs are recognized by an induced fit mechanism. Besides mediating sequence-specific base recognition, the amino acid substitutions introduced in the SpCas9 variants facilitate conformational remodeling of the PAM region of the bound DNA. Guided by the structural data, we engineered a SpCas9 variant that specifically recognizes NAAG PAMs. Taken together, these studies inform further development of Cas9-based genome editing tools.

Published

2016

35. Structural Basis for the Altered PAM Specificities of Engineered CRISPR-Cas9

Author

Hiroshi Nishimasu, Seiichi Hirano, Ryuichiro Ishitani, and Osamu Nureki

Subjects

0301 basic medicine, Biology, Crystallography, X-Ray, Substrate Specificity, 03 medical and health sciences, chemistry.chemical_compound, Endonuclease, 0302 clinical medicine, Bacterial Proteins, Genome editing, CRISPR-Associated Protein 9, parasitic diseases, CRISPR, Guide RNA, Molecular Biology, Genetics, Cas9, RNA, DNA, Cell Biology, Endonucleases, Protospacer adjacent motif, 030104 developmental biology, chemistry, Mutation, biology.protein, DNA, Intergenic, CRISPR-Cas Systems, Genetic Engineering, 030217 neurology & neurosurgery, RNA, Guide, Kinetoplastida

Abstract

The RNA-guided endonuclease Cas9 cleaves double-stranded DNA targets bearing a PAM (protospacer adjacent motif) and complementarity to the guide RNA. A recent study showed that, whereas wild-type Streptococcus pyogenes Cas9 (SpCas9) recognizes the 5'-NGG-3' PAM, the engineered VQR, EQR, and VRER SpCas9 variants recognize the 5'-NGA-3', 5'-NGAG-3', and 5'-NGCG-3' PAMs, respectively, thus expanding the targetable sequences in Cas9-mediated genome editing applications. Here, we present the high-resolution crystal structures of the three SpCas9 variants in complexes with a single-guide RNA and its altered PAM-containing, partially double-stranded DNA targets. A structural comparison of the three SpCas9 variants with wild-type SpCas9 revealed that the multiple mutations synergistically induce an unexpected displacement in the phosphodiester backbone of the PAM duplex, thereby allowing the SpCas9 variants to directly recognize the altered PAM nucleotides. Our findings explain the altered PAM specificities of the SpCas9 variants and establish a framework for further rational engineering of CRISPR-Cas9.

Published

2016

36. A Therapeutic Double Whammy: Transcriptional or Post-transcriptional Suppression of Microsatellite Repeat Toxicity by Cas9

Author

Thomas A. Cooper and Ashish N. Rao

Subjects

0301 basic medicine, Genetics, chemistry.chemical_classification, Cas9, RNA, Cell Biology, Biology, Pathogenesis, 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, 0302 clinical medicine, chemistry, Tandem repeat, Microsatellite Repeat, Microsatellite, Nucleotide, Molecular Biology, 030217 neurology & neurosurgery, DNA

Abstract

Microsatellite expansion diseases are caused by unstable tandem repeats of 3–10 nucleotides that become pathogenic beyond a threshold number of copies. Two groups present different approaches to reduce pathogenesis by targeting deactivated Cas9 to either the DNA (Pinto et al., 2017) or the RNA (Batra et al., 2017) repeats with therapeutic potential for several diseases.

Published

2017

37. SAFB2 Enables the Processing of Suboptimal Stem-Loop Structures in Clustered Primary miRNA Transcripts

Author

Seymen Avci, Michael Lohmüller, Katharina Hutter, Almina Jukic, Sebastian Herzog, Simon M. Hoser, Tamas G. Szabo, Felix Eichin, Verena Labi, Alexander Huettenhofer, and Andreas Villunger

Subjects

DGCR8, Computational biology, Cleavage (embryo), Cell Line, Microprocessor complex, Mice, 03 medical and health sciences, 0302 clinical medicine, Nuclear Matrix-Associated Proteins, microRNA, Animals, Humans, CRISPR, RNA Processing, Post-Transcriptional, Molecular Biology, Drosha, 030304 developmental biology, Cell Nucleus, 0303 health sciences, biology, Cas9, Inverted Repeat Sequences, RNA-Binding Proteins, Matrix Attachment Region Binding Proteins, Cell Biology, Stem-loop, MicroRNAs, HEK293 Cells, Receptors, Estrogen, biology.protein, Nucleic Acid Conformation, 030217 neurology & neurosurgery

Abstract

Many microRNAs (miRNAs) are generated from primary transcripts containing multiple clustered stem-loop structures that are thought to be recognized and cleaved by the Microprocessor complex as independent units. Here, we uncover an unexpected mode of processing of the bicistronic miR-15a-16-1 cluster. We find that the primary miR-15a stem-loop is not processed on its own but that the presence of the neighboring primary miR-16-1 stem-loop on the same transcript can compensate for this deficiency in cis. Using a CRISPR/Cas9 screen, we identify SAFB2 (scaffold attachment factor B2) as an essential co-factor in this miR-16-1-assisted pri-miR-15 cleavage and describe SAFB2 as an accessory protein of the Microprocessor. Notably, SAFB2-mediated cleavage expands to other clustered pri-miRNAs, indicating a general mechanism. Together, our study reveals an unrecognized function of SAFB2 in miRNA processing and suggests a scenario in which SAFB2 enables the binding and processing of suboptimal Microprocessor substrates in clustered primary miRNA transcripts.

Published

2020

38. Diverse Mechanisms of CRISPR-Cas9 Inhibition by Type IIC Anti-CRISPR Proteins

Author

Yong Wang, Pu Gao, Songqing Liu, Ang Gao, Alexander Serganov, Han Feng, Yalan Zhu, Guangxia Gao, and Qi Zhan

Subjects

Biology, Neisseria meningitidis, medicine.disease_cause, Article, Bacterial protein, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Genome editing, Bacterial Proteins, CRISPR-Associated Protein 9, medicine, CRISPR, Humans, Molecular Biology, 030304 developmental biology, Hydrolase inhibitor, Gene Editing, 0303 health sciences, Cas9, Cell Biology, DNA, Cell biology, chemistry, Helix, CRISPR-Cas Systems, 030217 neurology & neurosurgery

Abstract

Summary Anti-CRISPR proteins (Acrs) targeting CRISPR-Cas9 systems represent natural “off switches” for Cas9-based applications. Recently, AcrIIC1, AcrIIC2, and AcrIIC3 proteins were found to inhibit Neisseria meningitidis Cas9 (NmeCas9) activity in bacterial and human cells. Here we report biochemical and structural data that suggest molecular mechanisms of AcrIIC2- and AcrIIC3-mediated Cas9 inhibition. AcrIIC2 dimer interacts with the bridge helix of Cas9, interferes with RNA binding, and prevents DNA loading into Cas9. AcrIIC3 blocks the DNA loading step through binding to a non-conserved surface of the HNH domain of Cas9. AcrIIC3 also forms additional interactions with the REC lobe of Cas9 and induces the dimerization of the AcrIIC3-Cas9 complex. While AcrIIC2 targets Cas9 orthologs from different subtypes, albeit with different efficiency, AcrIIC3 specifically inhibits NmeCas9. Structure-guided changes in NmeCas9 orthologs convert them into anti-CRISPR-sensitive proteins. Our studies provide insights into anti-CRISPR-mediated suppression mechanisms and guidelines for designing regulatory tools in Cas9-based applications.

Published

2018

39. Phage AcrIIA2 DNA Mimicry: Structural Basis of the CRISPR and Anti-CRISPR Arms Race

Author

Yanli Wang, Min Wang, Maolu Yin, and Liang Liu

Subjects

Models, Molecular, Protein Conformation, Computational biology, Biology, Binding, Competitive, 03 medical and health sciences, chemistry.chemical_compound, Structure-Activity Relationship, Viral Proteins, 0302 clinical medicine, Genome editing, CRISPR-Associated Protein 9, Escherichia coli, CRISPR, A-DNA, Bacteriophages, Clustered Regularly Interspaced Short Palindromic Repeats, Protein Interaction Domains and Motifs, Molecular Biology, 030304 developmental biology, Subgenomic mRNA, Gene Editing, 0303 health sciences, Binding Sites, Cas9, Molecular Mimicry, RNA, Cell Biology, DNA, Protospacer adjacent motif, chemistry, Nucleic Acid Conformation, CRISPR-Cas Systems, 030217 neurology & neurosurgery, Protein Binding, RNA, Guide, Kinetoplastida

Abstract

Summary CRISPR-Cas (clustered regularly interspaced short palindromic repeats-CRISPR-associated proteins) systems provide prokaryotic cells with adaptive immunity against invading bacteriophages. Bacteriophages counteract bacterial responses by encoding anti-CRISPR inhibitor proteins (Acr). However, the structural basis for their inhibitory actions remains largely unknown. Here, we report the crystal structure of the AcrIIA2-SpyCas9-sgRNA (single-guide RNA) complex at 3.3 A resolution. We show that AcrIIA2 binds SpyCas9 at a position similar to the target DNA binding region. More specifically, AcrIIA2 interacts with the protospacer adjacent motif (PAM) recognition residues of Cas9, preventing target double-stranded DNA (dsDNA) detection. Thus, phage-encoded AcrIIA2 appears to act as a DNA mimic that blocks subsequent dsDNA binding by virtue of its highly acidic residues, disabling bacterial Cas9 by competing with target dsDNA binding with a binding motif distinct from AcrIIA4. Our study provides a more detailed mechanistic understanding of AcrIIA2-mediated inhibition of SpyCas9, the most widely used genome-editing tool, opening new avenues for improved regulatory precision during genome editing.

Published

2018

40. A Compact, High-Accuracy Cas9 with a Dinucleotide PAM for In Vivo Genome Editing

Author

Yueying Cao, Judith Gallant, Raed Ibraheim, Ildar Gainetdinov, Aamir Mir, Jaime A. Rivera-Pérez, Erik J. Sontheimer, Alireza Edraki, Wen Xue, Chun-Qing Song, and Yeonsoo Yoon

Subjects

Zygote, Genetic Vectors, Computational biology, Biology, Neisseria meningitidis, medicine.disease_cause, Substrate Specificity, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Genome editing, CRISPR-Associated Protein 9, medicine, CRISPR, Animals, Humans, Clustered Regularly Interspaced Short Palindromic Repeats, Guide RNA, Nucleotide Motifs, Molecular Biology, Adeno-associated virus, 030304 developmental biology, Subgenomic mRNA, Gene Editing, 0303 health sciences, Cas9, Cell Biology, DNA, Dependovirus, Embryo Transfer, Mice, Inbred C57BL, Protospacer adjacent motif, HEK293 Cells, chemistry, Liver, Female, CRISPR-Cas Systems, Proprotein Convertase 9, K562 Cells, 030217 neurology & neurosurgery, RNA, Guide, Kinetoplastida

Abstract

Summary CRISPR-Cas9 genome editing has transformed biotechnology and therapeutics. However, in vivo applications of some Cas9s are hindered by large size (limiting delivery by adeno-associated virus [AAV] vectors), off-target editing, or complex protospacer-adjacent motifs (PAMs) that restrict the density of recognition sequences in target DNA. Here, we exploited natural variation in the PAM-interacting domains (PIDs) of closely related Cas9s to identify a compact ortholog from Neisseria meningitidis—Nme2Cas9—that recognizes a simple dinucleotide PAM (N4CC) that provides for high target site density. All-in-one AAV delivery of Nme2Cas9 with a guide RNA targeting Pcsk9 in adult mouse liver produces efficient genome editing and reduced serum cholesterol with exceptionally high specificity. We further expand our single-AAV platform to pre-implanted zygotes for streamlined generation of genome-edited mice. Nme2Cas9 combines all-in-one AAV compatibility, exceptional editing accuracy within cells, and high target site density for in vivo genome editing applications.

Published

2018

41. Precise and Predictable CRISPR Chromosomal Rearrangements Reveal Principles of Cas9-Mediated Nucleotide Insertion

Author

Yingbin Liu, Qiang Wu, Li Jinhuan, and Jia Shou

Subjects

0301 basic medicine, DNA End-Joining Repair, DNA repair, Computational biology, Biology, Cleavage (embryo), Genome, 03 medical and health sciences, CRISPR-Associated Protein 9, Gene Duplication, FANCD2, CRISPR, Humans, Nucleotide, Clustered Regularly Interspaced Short Palindromic Repeats, DNA Breaks, Double-Stranded, Molecular Biology, Sequence Deletion, Regulation of gene expression, chemistry.chemical_classification, Gene Editing, Endodeoxyribonucleases, Base Sequence, Cas9, Genome, Human, Sequence Inversion, Fanconi Anemia Complementation Group D2 Protein, Nuclear Proteins, Cell Biology, DNA, Mutagenesis, Insertional, 030104 developmental biology, HEK293 Cells, chemistry, CRISPR-Cas Systems, Carrier Proteins, RNA, Guide, Kinetoplastida

Abstract

Summary Chromosomal rearrangements including large DNA-fragment inversions, deletions, and duplications by Cas9 with paired sgRNAs are important to investigate genome structural variations and developmental gene regulation, but little is known about the underlying mechanisms. Here, we report that disrupting CtIP or FANCD2, which have roles in alternative non-homologous end joining, enhances precise DNA-fragment deletion. By analyzing the inserted nucleotides at the junctions of DNA-fragment editing of deletions, inversions, and duplications and characterizing the cleaved products, we find that Cas9 endonucleolytically cleaves the noncomplementary strand with a flexible scissile profile upstream of the −3 position of the PAM site in vivo and in vitro, generating double-strand break ends with 5′ overhangs of 1–3 nucleotides. Moreover, we find that engineered Cas9 nucleases have distinct cleavage profiles. Finally, Cas9-mediated nucleotide insertions are nonrandom and are equal to the combined sequences upstream of both PAM sites with predicted frequencies. Thus, precise and predictable DNA-fragment editing could be achieved by perturbing DNA repair genes and using appropriate PAM configurations.

Published

2018

42. Kinetics and Fidelity of the Repair of Cas9-Induced Double-Strand DNA Breaks

Author

Hanna Aleida Holland, Marcel de Haas, Bas van Steensel, Eva K. Brinkman, Tao Chen, and Waseem Akhtar

Subjects

0301 basic medicine, microhomology-mediated end-joining, DNA End-Joining Repair, media_common.quotation_subject, Kinetics, Fidelity, Biology, Article, non-homologous end-joining, 03 medical and health sciences, chemistry.chemical_compound, Genome editing, INDEL Mutation, CRISPR-Associated Protein 9, CRISPR, genome editing, Humans, Clustered Regularly Interspaced Short Palindromic Repeats, DNA Breaks, Double-Stranded, repair kinetics, CRISPR-Cas, Molecular Biology, media_common, Gene Editing, Models, Genetic, Cas9, Cell Biology, Cell biology, Non-homologous end joining, 030104 developmental biology, Microhomology-mediated end joining, chemistry, DNA double-strand break, CRISPR-Cas Systems, K562 Cells, DNA

Abstract

Summary The RNA-guided DNA endonuclease Cas9 is a powerful tool for genome editing. Little is known about the kinetics and fidelity of the double-strand break (DSB) repair process that follows a Cas9 cutting event in living cells. Here, we developed a strategy to measure the kinetics of DSB repair for single loci in human cells. Quantitative modeling of repaired DNA in time series after Cas9 activation reveals variable and often slow repair rates, with half-life times up to ∼10 hr. Furthermore, repair of the DSBs tends to be error prone. Both classical and microhomology-mediated end joining pathways contribute to the erroneous repair. Estimation of their individual rate constants indicates that the balance between these two pathways changes over time and can be altered by additional ionizing radiation. Our approach provides quantitative insights into DSB repair kinetics and fidelity in single loci and indicates that Cas9-induced DSBs are repaired in an unusual manner., Graphical Abstract, Highlights • Approach to measure single-locus DSB repair kinetics after Cas9-induced breaks • Multiple repair pathways can act on a single locus with distinct kinetics • Repair tends to be slow and error prone, although this depends on the locus, Brinkman et al. report a strategy to determine the rate and fidelity of double-strand break repair at single loci cut by Cas9. They also infer the contributions from different repair pathways. Cas9-induced breaks are repaired at variable but often slow rates, and the repair tends to be error prone.

Published

2018

43. CRISPR-Cas Systems Reduced to a Minimum

Author

Stan J. J. Brouns, Cristóbal Almendros, and Sebastian N. Kieper

Subjects

Gene Editing, 0303 health sciences, Cas9, Cell Biology, Computational biology, Biology, Microbiology, Article, 03 medical and health sciences, 0302 clinical medicine, Genome editing, Microbiologie, CRISPR, Life Science, CRISPR-Cas Systems, Molecular Biology, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

CRISPR-Cas9 genome editing has transformed biotechnology and therapeutics. However, in vivo applications of some Cas9s are hindered by large size [limiting delivery by adeno-associated virus (AAV) vectors], off-target editing, or complex protospacer adjacent motifs (PAMs) that restrict the density of recognition sequences in target DNA. Here, we exploited natural variation in the PAM Interacting Domains (PIDs) of closely related Cas9s to identify a compact ortholog from Neisseria meningitidis—Nme2Cas9—that recognizes a simple dinucleotide PAM (N(4)CC) that provides for high target site density. All-in-one AAV delivery of Nme2Cas9 with a guide RNA targeting Pcsk9 in adult mouse liver produces efficient genome editing and reduced serum cholesterol, with exceptionally high specificity. We further expand our single-AAV platform to pre-implanted zygotes for streamlined generation of genome-edited mice. Nme2Cas9 combines all-in-one AAV compatibility, exceptional editing accuracy within cells, and high target site density for in vivo genome editing applications.

Published

2019

44. Cas9 deactivation with photocleavable guide RNAs.

Author

Zou, Roger S., Liu, Yang, Wu, Bin, and Ha, Taekjip

Subjects

*RNA, *DNA damage, *GENOME editing, *MOIETIES (Chemistry), *CELL populations, *NUCLEASES, *DNA repair, *CRISPRS

Abstract

Precise control of CRISPR-Cas9 would improve its safety and applicability. Controlled CRISPR inhibition is a promising approach but is complicated by separate inhibitor delivery, incomplete deactivation, and slow kinetics. To overcome these obstacles, we engineered photocleavable guide RNAs (pcRNAs) that endow Cas9 nucleases and base editors with a built-in mechanism for light-based deactivation. pcRNA enabled the fastest (<1 min) and most complete (<1% residual indels) approach for Cas9 deactivation. It also exhibited significantly enhanced specificity with wild-type Cas9. Time-resolved deactivation revealed that 12–36 h of Cas9 activity or 2–4 h of base editor activity was sufficient to achieve high editing efficiency. pcRNA is useful for studies of the cellular response to DNA damage by abolishing sustained cycles of damage and repair that would otherwise desynchronize response trajectories. Together, pcRNA expands the CRISPR toolbox for precision genome editing and studies of DNA damage and repair. [Display omitted] • Light-mediated deactivation of Cas9 and base editors with a modified guide RNA • Deactivation occurs within seconds and approaches completeness • The modified guide RNA natively results in enhanced specificity • Facilitates DNA repair studies through synchronized termination of DNA damage Zou et al. developed light-mediated control over Cas9 and base editor deactivation by introducing a photocleavable moiety into guide RNA. Deactivation occurs within seconds and approaches completeness. This modification natively enhanced specificity. Timed deactivation facilitated studies of DNA repair by synchronizing the termination of DNA damage within a cell population. [ABSTRACT FROM AUTHOR]

Published

2021

45. CTCF Binding Polarity Determines Chromatin Looping

Author

Patrick J. Wijchers, E.S. Vos, Elzo de Wit, Marjon J.A.M. Verstegen, Peter H.L. Krijger, Sjoerd J B Holwerda, Wouter de Laat, Erik Splinter, Christian Valdes-Quezada, Hans Teunissen, and Hubrecht Institute for Developmental Biology and Stem Cell Research

Subjects

CCCTC-Binding Factor, Chromosomal Proteins, Non-Histone, Repressor, Cell Cycle Proteins, Plasma protein binding, Biology, Research Support, Cell Line, Mice, Journal Article, Animals, CRISPR, Binding site, Non-U.S. Gov't, Molecular Biology, Embryonic Stem Cells, Genetics, Binding Sites, Cohesin, Cas9, Research Support, Non-U.S. Gov't, Cell Biology, Chromatin, Cell biology, Repressor Proteins, CTCF, CRISPR-Cas Systems, Protein Binding

Abstract

CCCTC-binding factor (CTCF) is an architectural protein involved in the three-dimensional (3D) organization of chromatin. In this study, we assayed the 3D genomic contact profiles of a large number of CTCF binding sites with high-resolution 4C-seq. As recently reported, our data also suggest that chromatin loops preferentially form between CTCF binding sites oriented in a convergent manner. To directly test this, we used CRISPR/Cas9 genome editing to delete core CTCF binding sites in three loci, including the CTCF site in the Sox2 super-enhancer. In all instances, CTCF and cohesin recruitment were lost, and chromatin loops with distal, convergent CTCF sites were disrupted or destabilized. Re-insertion of oppositely oriented CTCF recognition sequences restored CTCF and cohesin recruitment, but did not re-establish chromatin loops. We conclude that CTCF binding polarity plays a functional role in the formation of higher-order chromatin structure.

Published

2015

46. Single-Stranded DNA Cleavage by Divergent CRISPR-Cas9 Enzymes

Author

Lucas B. Harrington, Kaihong Zhou, Enbo Ma, Mitchell R. O’Connell, and Jennifer A. Doudna

Subjects

Streptococcus pyogenes, DNA, Single-Stranded, Biology, Medical and Health Sciences, Article, Genome engineering, chemistry.chemical_compound, Bacterial Proteins, Genome editing, Single-Stranded, CRISPR, Guide RNA, Molecular Biology, Genetics, Cas9, Bacterial, RNA, DNA, Cell Biology, Biological Sciences, Endonucleases, RNA, Bacterial, Protospacer adjacent motif, chemistry, CRISPR-Cas Systems, Developmental Biology

Abstract

Double-stranded DNA (dsDNA) cleavage by Cas9 is a hallmark of type II CRISPR-Cas immune systems. Cas9–guide RNA complexes recognize 20-base-pair sequences in DNA and generate a site-specific double-strand break, a robust activity harnessed for genome editing. DNA recognition by all studied Cas9 enzymes requires a protospacer adjacent motif (PAM) next to the target site. We show that Cas9 enzymes from evolutionarily divergent bacteria can recognize and cleave single-stranded DNA (ssDNA) by an RNA-guided, PAM-independent recognition mechanism. Comparative analysis shows that in contrast to the type II-A S. pyogenes Cas9 that is widely used for genome engineering, the smaller type II-C Cas9 proteins have limited dsDNA binding and unwinding activity and promiscuous guide-RNA specificity. These results indicate that inefficiency of type II-C Cas9 enzymes for genome editing results from a limited ability to cleave dsDNA, and suggest that ssDNA cleavage was an ancestral function of the Cas9 enzyme family.

Published

2015

47. DNase H Activity of Neisseria meningitidis Cas9

Author

Yan Zhang, Rakhi Rajan, H. Steven Seifert, Alfonso Mondragón, and Erik J. Sontheimer

Subjects

DNA, Bacterial, Molecular Sequence Data, DNA, Single-Stranded, Neisseria meningitidis, Cleavage (embryo), medicine.disease_cause, Article, Genome engineering, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Bacterial Proteins, Cleave, medicine, Clustered Regularly Interspaced Short Palindromic Repeats, Nucleotide Motifs, Endodeoxyribonucleases, Molecular Biology, 030304 developmental biology, Genetics, Trans-activating crRNA, 0303 health sciences, biology, Cas9, Cell Biology, Biochemistry, chemistry, biology.protein, CRISPR-Cas Systems, 030217 neurology & neurosurgery, DNA, RNA, Guide, Kinetoplastida

Abstract

Type II CRISPR systems defend against invasive DNA by using Cas9 as an RNA-guided nuclease that creates double-stranded DNA breaks. Dual RNAs [CRISPR RNA (crRNA) and tracrRNA] are required for Cas9’s targeting activities observed to date. Targeting requires a protospacer adjacent motif (PAM) and crRNA-DNA complementarity. Cas9 orthologues [including Neisseria meningitidis Cas9 (NmeCas9)] have also been adopted for genome engineering. Here we examine the DNA cleavage activities and substrate requirements of NmeCas9, including a set of unusually complex PAM recognition patterns. Unexpectedly, NmeCas9 cleaves single-stranded DNAs in a manner that is RNA-guided but PAM- and tracrRNA-independent. Beyond the need for guide-target pairing, this “DNase H” activity has no apparent sequence requirements, and the cleavage sites are measured from the 5′ end of the DNA substrate’s RNA-paired region. These results indicate that tracrRNA is not strictly required for NmeCas9 enzymatic activation, and expand the list of targeting activities of Cas9 endonucleases.

Published

2015

48. Expanding the Biologist’s Toolkit with CRISPR-Cas9

Author

Samuel H. Sternberg and Jennifer A. Doudna

Subjects

Genetics, Genome, Models, Genetic, Cas9, CRISPR-Associated Proteins, Cell Biology, Computational biology, Biology, Genome engineering, Animals, Deoxyribonuclease I, Humans, CRISPR, Clustered Regularly Interspaced Short Palindromic Repeats, CRISPR-Cas Systems, Genetic Engineering, Molecular Biology, RNA, Guide, Kinetoplastida

Abstract

Few discoveries transform a discipline overnight, but biologists today can manipulate cells in ways never possible before, thanks to a peculiar form of prokaryotic adaptive immunity mediated by clustered regularly interspaced short palindromic repeats (CRISPR). From elegant studies that deciphered how these immune systems function in bacteria, researchers quickly uncovered the technological potential of Cas9, an RNA-guided DNA cleaving enzyme, for genome engineering. Here we highlight the recent explosion in visionary applications of CRISPR-Cas9 that promises to usher in a new era of biological understanding and control.

Published

2015

49. CRISPR RNA-Dependent Binding and Cleavage of Endogenous RNAs by the Campylobacter jejuni Cas9

Author

Sara K. Eisenbart, Ryan T. Leenay, Belinda U. Aul, Thorsten Bischler, Gaurav Dugar, Chase L. Beisel, Cynthia M. Sharma, and HIRI, Helmholtz-Institut für RNA-basierte Infektionsforschung, Josef-Shneider Strasse 2, 97080 Würzburg, Germany.

Subjects

0301 basic medicine, DNA, Bacterial, RNA Stability, RIP-seq, non-coding RNA, RNA-binding protein, Biology, Article, Campylobacter jejuni, 03 medical and health sciences, Protein Domains, CRISPR-Associated Protein 9, CRISPR, genome editing, RNA, Messenger, crRNA, Cas9, Molecular Biology, Trans-activating crRNA, RNA, Cell Biology, RNA cleavage, Non-coding RNA, Cell biology, RNA, Bacterial, 030104 developmental biology, RNA Cleavage, RNA binding proteins, CRISPR-Cas Systems, post-transcriptional regulation

Abstract

Cas9 nucleases naturally utilize CRISPR RNAs (crRNAs) to silence foreign double-stranded DNA. While recent work has shown that some Cas9 nucleases can also target RNA, RNA recognition has required nuclease modifications or accessory factors. Here, we show that the Campylobacter jejuni Cas9 (CjCas9) can bind and cleave complementary endogenous mRNAs in a crRNA-dependent manner. Approximately 100 transcripts co-immunoprecipitated with CjCas9 and generally can be subdivided through their base-pairing potential to the four crRNAs. A subset of these RNAs was cleaved around or within the predicted binding site. Mutational analyses revealed that RNA binding was crRNA- and tracrRNA-dependent, and that target RNA cleavage required the CjCas9 HNH domain. We further observed that RNA cleavage was PAM-independent, improved with greater complementarity between the crRNA and the RNA target, and was programmable in vitro. These findings suggest that C. jejuni Cas9 is a promiscuous nuclease that can coordinately target both DNA and RNA.

Published

2017

50. Polycomb-Dependent Chromatin Looping Contributes to Gene Silencing during Drosophila Development

Author

Yuki Ogiyama, Bernd Schuettengruber, Jia-Ming Chang, Giacomo Cavalli, Giorgio L. Papadopoulos, Institut de génétique humaine (IGH), and Université de Montpellier (UM)-Centre National de la Recherche Scientifique (CNRS)

Subjects

0301 basic medicine, [SDV]Life Sciences [q-bio], Polycomb-Group Proteins, Biology, Midblastula, 03 medical and health sciences, Hi-C, Gene silencing, CRISPR, Animals, Drosophila Proteins, Gene Silencing, TADs, Molecular Biology, Gene, Regulation of gene expression, Drosophila embryogenesis, [SDV.GEN]Life Sciences [q-bio]/Genetics, Cas9, Cell Biology, 3D genome, Chromatin, Cell biology, chromosome organization, looping interactions, 030104 developmental biology, Drosophila melanogaster, CRISPR-Cas Systems, polycomb

Abstract

International audience; Interphase chromatin is organized into topologically associating domains (TADs). Within TADs, chromatin looping interactions are formed between DNA regulatory elements, but their functional importance for the establishment of the 3D genome organization and gene regulation during development is unclear. Using high-resolution Hi-C experiments, we analyze higher order 3D chromatin organization during Drosophila embryogenesis and identify active and repressive chromatin loops that are established with different kinetics and depend on distinct factors: Zelda-dependent active loops are formed before the midblastula transition between transcribed genes over long distances. Repressive loops within polycomb domains are formed after the midblastula transition between polycomb response elements by the action of GAGA factor and polycomb proteins. Perturbation of PRE function by CRISPR/Cas9 genome engineering affects polycomb domain formation and destabilizes polycomb-mediated silencing. Preventing loop formation without removal of polycomb components also decreases silencing efficiency, suggesting that chromatin architecture can play instructive roles in gene regulation during development. VIDEO ABSTRACT.

Published

2017