Purification of specific DNA species using the CRISPR system

AbstractIn 2013, we developed a new method of engineered DNA-binding molecule-mediated chromatin immunoprecipitation that incorporates the clustered regularly interspaced short palindromic repeats (CRISPR) system to purify specific DNA species. This CRISPR-mediated purification can be performed in-cell or in vitro; CRISPR complexes can be expressed to tag target DNA sequences in the cells to be analyzed, or a CRISPR ribonucleoprotein complex consisting of recombinant nuclease-dead Cas9 (dCas9) and synthetic guide RNA can be used to tag target DNA sequences in vitro. Both methods enable purification of specific DNA sequences in chromatin structures for subsequent identification of molecules (proteins, RNAs, and other genomic regions) associated with the target sequences. The in vitro method also enables enrichment of purified DNA sequences from a pool of heterogeneous sequences for next-generation sequencing or other applications. In this review, we outline the principle of CRISPR-mediated purification of specific DNA species and discuss recent advances in the technology.

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Cas12a trans-cleavage can be modulated in vitro and is active on ssDNA, dsDNA, and RNA

10.1101/600890 ◽

2019 ◽

Cited By ~ 8

Author(s):

Ryan T. Fuchs ◽

Jennifer Curcuru ◽

Megumu Mabuchi ◽

Paul Yourik ◽

G. Brett Robb

Keyword(s):

Dna Sequences ◽

Nuclease Activity ◽

Target Sequence ◽

Sequence Composition ◽

Guide Rna ◽

Dna Targeting ◽

Single Turnover ◽

Target Dna ◽

Buffer Composition

ABSTRACTCRISPR-Cas12a (Cpf1) are RNA-guided nuclease effectors of acquired immune response that act in their native organisms by cleaving targeted DNA sequences. Like CRISPR-Cas9 RNA-guided DNA targeting enzymes, Cas12a orthologs have been repurposed for genome editing in non-native organisms and for DNA manipulationin vitro. Recent studies have shown that activation of Cas12a via guide RNA-target DNA pairing causes multiple turnover, non-specific ssDNA degradation intrans, after single turnover on-target cleavage incis. We find that the non-specifictransnuclease activity affects RNA and dsDNA in addition to ssDNA, an activity made more evident by adjustment of reaction buffer composition. The magnitude of thetransnuclease activity varies depending on features of the guide RNA being used, specifically target sequence composition and length. We also find that the magnitude oftransnuclease activity varies between the three most well-studied Cas12a orthologs and that the Cas12a fromLachnospiraceaebacterium ND2006 appears to be the most active.

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In vitro Assay Revealed Mismatches between Guide RNA and Target DNA can Enhance Cas9 Nuclease Activity

Current Chinese Science ◽

10.2174/2210298101999200907161320 ◽

2020 ◽

Vol 1 (1) ◽

pp. 69-72

Author(s):

Ji Luan ◽

Zhen Li ◽

Hailong Wang ◽

Jun Fu ◽

Youming Zhang

Keyword(s):

Dna Sequences ◽

High Efficiency ◽

Nuclease Activity ◽

Ease Of Use ◽

Unexpected Finding ◽

Vitro Assay ◽

Guide Rna ◽

Cleavage Activity ◽

Target Dna

Background: CRISPR-Cas9 is a powerful technology that allows us to modify DNA sequences in a specific manner across a variety of organisms. Due to its high efficiency and specificity, and ease of use, it becomes a commonly used method for gene editing. Although many structural and biochemical studies have been carried out to understand the fundamental mechanism of CRISPR/Cas9, our understanding of CRISPR/Cas9 caused off-target effects is still lacking. Methods: The enhanced in vitro cleavage activity of Cas9 protein from Streptococcus pyogenes (SpCas9) was evaluated by both synthetic crRNA-tracrRNA duplexes and in vitro transcribed single guide RNAs. Results: Here, we report an unexpected finding that mismatches between the guide RNA and target DNA significantly enhanced the in vitro cleavage activity of SpCas9 by more than 2 folds. Conclusion: Our observation that mismatches between the guide RNA and target DNA can dramatically increase the in vitro cleavage of Cas9 suggests the potential sequence preference for the CRSIPR/Cas9 system.

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Efficient sequence-specific isolation of DNA fragments and chromatin by in vitro enChIP technology using recombinant CRISPR ribonucleoproteins

10.1101/033241 ◽

2015 ◽

Author(s):

Toshitsugu Fujita ◽

Miyuki Yuno ◽

Hodaka Fujii

Keyword(s):

Chromatin Immunoprecipitation ◽

Biochemical Characterization ◽

Target Dna ◽

Short Palindromic Repeat ◽

Downstream Analysis ◽

Genomic Regions ◽

Efficient Sequence ◽

Potential Use

The clustered regularly interspaced short palindromic repeat (CRISPR) system is widely used for various biological applications, including genome editing. We developed engineered DNA-binding molecule-mediated chromatin immunoprecipitation (enChIP) using CRISPR to isolate target genomic regions from cells for their biochemical characterization. In this study, we developed 'in vitro enChIP' using recombinant CRISPR ribonucleoproteins (RNPs) to isolate target genomic regions. in vitro enChIP has the great advantage over conventional enChIP of not requiring expression of CRISPR complexes in cells. We first demonstrate that in vitro enChIP using recombinant CRISPR RNPs can be used to isolate target DNA from mixtures of purified DNA in a sequence-specific manner. In addition, we show that this technology can be employed to efficiently isolate target genomic regions, while retaining their intracellular molecular interactions, with negligible contamination from irrelevant genomic regions. Thus, in vitro enChIP technology is of potential use for sequence-specific isolation of DNA, as well as for identification of molecules interacting with genomic regions of interest in vivo in combination with downstream analysis.

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Isolation of Specific Genomic Regions and Identification of Their Associated Molecules by Engineered DNA-Binding Molecule-Mediated Chromatin Immunoprecipitation (enChIP) Using the CRISPR System and TAL Proteins

International Journal of Molecular Sciences ◽

10.3390/ijms160921802 ◽

2015 ◽

Vol 16 (9) ◽

pp. 21802-21812 ◽

Cited By ~ 11

Author(s):

Hodaka Fujii ◽

Toshitsugu Fujita

Keyword(s):

Dna Binding ◽

Chromatin Immunoprecipitation ◽

Crispr System ◽

Genomic Regions

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Enhancement of target specificity of CRISPR–Cas12a by using a chimeric DNA–RNA guide

Nucleic Acids Research ◽

10.1093/nar/gkaa605 ◽

2020 ◽

Vol 48 (15) ◽

pp. 8601-8616 ◽

Cited By ~ 1

Author(s):

Hanseop Kim ◽

Wi-jae Lee ◽

Yeounsun Oh ◽

Seung-Hun Kang ◽

Junho K Hur ◽

...

Keyword(s):

Dna Sequences ◽

Genome Engineering ◽

Target Genes ◽

Target Sequence ◽

Energy Potential ◽

Guide Rna ◽

Sequence Recognition ◽

Protospacer Adjacent Motif ◽

Effective Manner ◽

Target Dna

Abstract The CRISPR–Cas9 system is widely used for target-specific genome engineering. CRISPR–Cas12a (Cpf1) is one of the CRISPR effectors that controls target genes by recognizing thymine-rich protospacer adjacent motif (PAM) sequences. Cas12a has a higher sensitivity to mismatches in the guide RNA than does Cas9; therefore, off-target sequence recognition and cleavage are lower. However, it tolerates mismatches in regions distant from the PAM sequence (TTTN or TTN) in the protospacer, and off-target cleavage issues may become more problematic when Cas12a activity is improved for therapeutic purposes. Therefore, we investigated off-target cleavage by Cas12a and modified the Cas12a (cr)RNA to address the off-target cleavage issue. We developed a CRISPR–Cas12a that can induce mutations in target DNA sequences in a highly specific and effective manner by partially substituting the (cr)RNA with DNA to change the energy potential of base pairing to the target DNA. A model to explain how chimeric (cr)RNA guided CRISPR–Cas12a and SpCas9 nickase effectively work in the intracellular genome is suggested. Chimeric guide-based CRISPR- Cas12a genome editing with reduced off-target cleavage, and the resultant, increased safety has potential for therapeutic applications in incurable diseases caused by genetic mutations.

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Enhancement of Target Specificity of CRISPR-Cas12a by Using a Chimeric DNA-RNA Guide

10.1101/2020.02.04.933614 ◽

2020 ◽

Author(s):

Hanseop Kim ◽

Wi-jae Lee ◽

Seung-Hun Kang ◽

Junho K. Hur ◽

Hyomin Lee ◽

...

Keyword(s):

Dna Sequences ◽

Genome Engineering ◽

Target Genes ◽

Genetic Mutation ◽

Target Sequence ◽

Energy Potential ◽

Guide Rna ◽

Sequence Recognition ◽

Effective Manner ◽

Target Dna

AbstractThe CRISPR-Cas9 system is widely used for target-specific genome engineering. Cpf1 is one of the CRISPR effectors that controls target genes by recognizing thymine-rich protospacer adjacent motif (PAM) sequences. Cpf1 has a higher sensitivity to mismatches in the guide RNA than does Cas9; therefore, off-target sequence recognition and cleavage are lower. However, it tolerates mismatches in regions distant from the PAM sequence (TTTN or TTN) in the protospacer, and off-target cleavage issues may become more problematic when Cpf1 activity is improved for therapeutic purposes. In our study, we investigated off-target cleavage by Cpf1 and modified the Cpf1 (cr)RNA to address the off-target cleavage issue. We developed a CRISPR-Cpf1 that can induce mutations in target DNA sequences in a highly specific and effective manner by partially substituting the (cr)RNA with DNA to change the energy potential of base pairing to the target DNA. A model to explain how chimeric (cr)RNA guided CRISPR-Cpf1 and SpCas9 nickase effectively work in the intracellular genome is suggested. In our results, CRISPR-Cpf1 induces less off-target mutations at the cell level, when chimeric DNA-RNA guide was used for genome editing. This study has a potential for therapeutic applications in incurable diseases caused by genetic mutation.

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A method to convert mRNA into a gRNA library for CRISPR/Cas9 editing of any organism

Science Advances ◽

10.1126/sciadv.1600699 ◽

2016 ◽

Vol 2 (8) ◽

pp. e1600699 ◽

Cited By ~ 11

Author(s):

Hiroshi Arakawa

Keyword(s):

Dna Sequences ◽

Genetic Screening ◽

Restriction Enzymes ◽

Mrna Sequence ◽

Complementary Sequence ◽

Complementary Dna ◽

Random Primer ◽

Guide Rna ◽

Protospacer Adjacent Motif ◽

Target Dna

The clustered regularly interspersed palindromic repeats (CRISPR)/Cas9 (CRISPR-associated protein 9) system is a powerful tool for genome editing that can be used to construct a guide RNA (gRNA) library for genetic screening. For gRNA design, one must know the sequence of the 20-mer flanking the protospacer adjacent motif (PAM), which seriously impedes experimentally making gRNA. I describe a method to construct a gRNA library via molecular biology techniques without relying on bioinformatics. Briefly, one synthesizes complementary DNA from the mRNA sequence using a semi-random primer containing a PAM complementary sequence and then cuts out the 20-mer adjacent to the PAM using type IIS and type III restriction enzymes to create a gRNA library. The described approach does not require prior knowledge about the target DNA sequences, making it applicable to any species.

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Universal microbial diagnostics using random DNA probes

Science Advances ◽

10.1126/sciadv.1600025 ◽

2016 ◽

Vol 2 (9) ◽

pp. e1600025 ◽

Cited By ~ 5

Author(s):

Amirali Aghazadeh ◽

Adam Y. Lin ◽

Mona A. Sheikh ◽

Allen L. Chen ◽

Lisa M. Atkins ◽

...

Keyword(s):

Dna Sequences ◽

Pathogenic Bacteria ◽

Disease Outbreaks ◽

Dna Probes ◽

Signal Recovery ◽

Human Pathogens ◽

Infectious Disease Outbreaks ◽

Target Dna ◽

Detection Schemes

Early identification of pathogens is essential for limiting development of therapy-resistant pathogens and mitigating infectious disease outbreaks. Most bacterial detection schemes use target-specific probes to differentiate pathogen species, creating time and cost inefficiencies in identifying newly discovered organisms. We present a novel universal microbial diagnostics (UMD) platform to screen for microbial organisms in an infectious sample, using a small number of random DNA probes that are agnostic to the target DNA sequences. Our platform leverages the theory of sparse signal recovery (compressive sensing) to identify the composition of a microbial sample that potentially contains novel or mutant species. We validated the UMD platform in vitro using five random probes to recover 11 pathogenic bacteria. We further demonstrated in silico that UMD can be generalized to screen for common human pathogens in different taxonomy levels. UMD’s unorthodox sensing approach opens the door to more efficient and universal molecular diagnostics.

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MSCV-based retroviral plasmids expressing 3xFLAG-Sp-dCas9 for enChIP analysis

10.21203/rs.2.16753/v4 ◽

2021 ◽

Author(s):

Miyuki Yuno ◽

Toshitsugu Fujita ◽

Hodaka Fujii

Keyword(s):

Dna Binding ◽

Streptococcus Pyogenes ◽

Chromatin Immunoprecipitation ◽

Genomic Region ◽

Target Cells ◽

Drug Selection ◽

Guide Rna ◽

Inactive Form ◽

Genomic Regions ◽

Selection Of

Abstract Engineered DNA-binding molecule–mediated chromatin immunoprecipitation (enChIP) is a technology for purifying specific genomic regions to facilitate identification of their associated molecules, including proteins, RNAs, and other genomic regions. In enChIP, the target genomic region is tagged with engineered DNA-binding molecules, e.g., a variant of the clustered regularly interspaced short palindromic repeats (CRISPR) system consisting of a guide RNA (gRNA) and a catalytically inactive form of Cas9 (dCas9). In this study, to increase the flexibility of enChIP and expand the range of target cells, we generated murine stem cell virus (MSCV)-based retroviral plasmids for expressing dCas9. We constructed MSCV-based retroviral plasmids expressing Streptococcus pyogenes dCas9 fused to a 3xFLAG-tag (3xFLAG-Sp-dCas9) and various drug resistance genes. We showed that by using these plasmids, it is feasible to purify target genomic regions with yields comparable to those reported using other systems. These systems might give enChIP users greater flexibility in choosing optimal systems for drug selection of transduced cells.

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In vitro analysis of site specific nuclease selectivity by NGS

AIMS Bioengineering ◽

10.3934/bioeng.2021020 ◽

2021 ◽

Vol 8 (4) ◽

pp. 235-242

Author(s):

Vincent Brondani ◽

Keyword(s):

Restriction Endonuclease ◽

Genome Engineering ◽

Direct Interaction ◽

Target Sequence ◽

Vitro Assay ◽

Guide Rna ◽

Phosphate Backbone ◽

Target Dna ◽

Vitro Analysis

<abstract> <p>Nucleases currently used in genome engineering induce hydrolysis of DNA phosphate backbone in a sequence-specific manner. The RNA guided nucleases describe today are recognizing a sequence with two distinct molecular interactions: first, like a restriction endonuclease, by direct interaction between the protein and the DNA; and second, by hybridization of the guide RNA with the target DNA sequence. Here we report an in vitro assay to assess the cleavage specificity and the selectivity of the nucleases. The assay is designed using a plasmid encompassing the DNA target site degenerated at positions determined on structural feature. The results demonstrate that the Cpf1 RNA guided nuclease is highly specific for the target sequence, nevertheless its substrate selectivity is low compare to a restriction endonuclease.</p> </abstract>

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