CRISPR-Cpf1 mediates efficient homology-directed repair and temperature-controlled genome editing

Moreno-Mateos, Miguel A.; Fernández, Juan Pablo; Rouet, Romain; Vejnar, Charles E.; Lane, Maura; Mis, Emily K; Khokha, Mustafa K.; Doudna, Jennifer A.; Giráldez, Antonio J.

doi:10.1038/s41467-017-01836-2

Cited by 247 publications

(277 citation statements)

References 37 publications

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“…Therefore, we tested whether LbCas12a (Zetsche et al ., ), with its thymine rich PAM (TTTV), which occurs also more frequent, can serve as an efficient alternative nuclease for in planta GT. In addition, testing Cas12a variant was especially interesting as other reports, unfortunately based on very small numbers of GT events, claimed that the use of Cas12a as a nuclease might result in higher GT frequencies than the use of Cas9 (Begemann et al ., ; Ferenczi et al ., ; Moreno‐Mateos et al ., ).…”

Section: Introductionmentioning

confidence: 97%

In planta gene targeting can be enhanced by the use of CRISPR/Cas12a

Wolter

Puchta

2019

The Plant Journal

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The controlled change of plant genomes by homologous recombination (HR) is still difficult to achieve. We previously developed the in planta gene targeting (ipGT) technology which depends on the simultaneous activation of the target locus by a double-strand break and the excision of the target vector. Whereas the use of SpCas9 resulted in low ipGT frequencies in Arabidopsis, we were recently able to improve the efficiency by using egg cell-specific expression of the potent but less broadly applicable SaCas9 nuclease. In this study, we now tested whether we could improve ipGT further, by either performing it in cells with enhanced intrachromosomal HR efficiencies or by the use of Cas12a, a different kind of CRISPR/Cas nuclease with an alternative cutting mechanism. We could show before that plants possess three kinds of DNA ATPase complexes, which all lead to instabilities of homologous genomic repeats if lost by mutation. As these proteins act in independent pathways, we tested ipGT in double mutants in which intrachromosomal HR is enhanced 20-80-fold. However, we were not able to obtain higher ipGT frequencies, indicating that mechanisms for gene targeting (GT) and chromosomal repeat-induced HR differ. However, using LbCas12a, the GT frequencies were higher than with SaCas9, despite a lower non-homologous end-joining (NHEJ) induction efficiency, demonstrating the particular suitability of Cas12a to induce HR. As SaCas9 has substantial restrictions due to its longer GC rich PAM sequence, the use of LbCas12a with its AT-rich PAM broadens the range of ipGT drastically, particularly when targeting in CG-deserts like promoters and introns.

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Section: Introductionmentioning

confidence: 97%

In planta gene targeting can be enhanced by the use of CRISPR/Cas12a

Wolter

Puchta

2019

The Plant Journal

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“…CRISPR-Cas12a (formerly known as Cpf1) is a class 2 type V CRISPR system that has been adopted for genome engineering in several organisms (Zetsche et al 2015;Moreno-Mateos et al 2017;Malzahn et al 2019;Chow et al 2019). Cas12a is a RNA-guided DNA endonuclease with a number of attributes distinct from Cas9, making it an interesting candidate to complement the CRISPR toolbox also in Drosophila.…”

Section: Introductionmentioning

confidence: 99%

“…We previously assessed Cas12a performance in Drosophila focused exclusively on AsCas12a and reported low activity compared to SpCas9 (Port and Bullock 2016). A subsequent study in zebrafish and Xenopus demonstrated that Cas12a activity is strongly temperature-dependent and showed that AsCas12a has low activity at temperatures below 30°C (Moreno-Mateos et al 2017). This is likely to limit the utility of AsCas12a in Drosophila, which do not tolerate long-term exposure to temperatures above 30°C.…”

Section: Introductionmentioning

confidence: 99%

“…This is likely to limit the utility of AsCas12a in Drosophila, which do not tolerate long-term exposure to temperatures above 30°C. However, in fish and frogs LbCas12a was found to have higher activity at low temperatures, raising the possibility that LbCas12a might efficiently function as RNA-guided DNA endonuclease also in flies (Moreno-Mateos et al 2017).…”

Section: Introductionmentioning

confidence: 99%

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Multiplexed conditional genome editing with Cas12a inDrosophila

Port

Starostecka

Boutros

2020

Preprint

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CRISPR-Cas genome engineering has revolutionised biomedical research by enabling targeted genome modification with unprecedented ease. In the popular model organism Drosophila melanogaster gene editing has so far relied exclusively on the prototypical CRISPR nuclease Cas9. The availability of additional CRISPR systems could expand the genomic target space, offer additional modes of regulation and enable the independent manipulation of genes in different cell populations of the same animal. Here we describe a platform for efficient Cas12a gene editing in Drosophila. We show that Cas12a from Lachnospiraceae bacterium, but not Acidaminococcus spec., can mediate robust gene editing in vivo. In combination with most crRNAs, LbCas12a activity is strongly suppressed at lower temperatures, enabling control of gene editing by simply modulating temperature. LbCas12a can directly utilize compact crRNAs arrays that are substantially easier to construct than Cas9 sgRNA arrays, facilitating multiplex genome engineering of several target sites in parallel. Targeting genes with arrays of three crRNAs results in the induction of loss-of function phenotypes with comparable efficiencies than a state-of-the-art Cas9 system. Lastly, we show that cell type-specific expression of LbCas12a is sufficient to mediate tightly controlled gene editing in a variety of tissues, allowing detailed analysis of gene function in this multicellular organism. Cas12a gene editing substantially expands the genome engineering toolbox in this organism and will be a powerful method for the functional annotation of the Drosophila genome. This work also lays out principles for the development of multiplexed transgenic Cas12a genome engineering systems in other genetically tractable organisms.

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“…Furthermore, the protospacer-adjacent motif (PAM) of Cas12a is Trich in comparison to the G-rich PAM of Cas9 which identifies more possible target sequences near STOP codons of mammalian cells (Buchmuller et al, 2019). In addition, Cas9 induces DSBs close to the PAM site while Cas12a cuts further away from it, which might increase targeting efficiency as the target sequence is not as easily destroyed by indel formation and may be re-cleaved after repair (Zetsche et al, 2015;Moreno-Mateos et al, 2017).…”

Section: Introductionmentioning

confidence: 99%

CRISPR-Cas12a-assisted PCR tagging of mammalian genes

Fueller

Herbst

Meurer

et al. 2018

Preprint

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AbstractHere we describe a time-efficient strategy for endogenous C-terminal gene tagging in mammalian tissue culture cells. An online platform is used to design two long gene-specific oligonucleotides for PCR with generic template cassettes to create linear dsDNA donors, termed PCR cassettes. PCR cassettes encode the tag (e.g. GFP), a Cas12a CRISPR RNA for cleavage of the target locus and short homology arms for directed integration via homologous recombination. The integrated tag is coupled to a generic terminator shielding the tagged gene from the co-inserted auxiliary sequences. Co-transfection of PCR cassettes with a Cas12a-encoding plasmid leads to robust endogenous expression of tagged genes, with tagging efficiency of up to 20% without selection, and up to 60% when selection markers are used. We used target-enrichment sequencing to investigate all potential sources of artefacts. Our work outlines a quick strategy particularly suitable for exploratory studies using endogenous expression of fluorescent protein tagged genes

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CRISPR-Cpf1 mediates efficient homology-directed repair and temperature-controlled genome editing

Cited by 247 publications

References 37 publications

In planta gene targeting can be enhanced by the use of CRISPR/Cas12a

In planta gene targeting can be enhanced by the use of CRISPR/Cas12a

Multiplexed conditional genome editing with Cas12a inDrosophila

CRISPR-Cas12a-assisted PCR tagging of mammalian genes

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