One-step generation of modular CAR-T cells with AAV–Cpf1

Dai, Xiaoyun; Park, Jonathan J.; Du, Yaying; Kim, Hyunu R; Wang, Guangchuan; Errami, Youssef; Chen, Sidi

doi:10.1038/s41592-019-0329-7

Cited by 124 publications

(126 citation statements)

References 36 publications

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“…Cas12a can be programmed to induce DNA doublestrand breaks (DSBs) at specific genomic loci in vivo [14,15,17,18,20,25,26]. To test if CeCas12a and BfCas12a could be harnessed for gene editing in mammalian cells, we optimized the codons of two genes and attached a Cterminal and an N-terminal nuclear localization signals (NLS) for optimal expression and nuclear targeting in human cells.…”

Section: Gene Editing With Cecas12a and Bfcas12a In Human Cellsmentioning

confidence: 99%

A Cas12a ortholog with stringent PAM recognition followed by low off-target editing rates for genome editing

et al. 2020

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Background: AsCas12a and LbCas12a nucleases are reported to be promising tools for genome engineering with protospacer adjacent motif (PAM) TTTV as the optimal. However, the C-containing PAM (CTTV, TCTV, TTCV, etc.) recognition by Cas12a might induce extra off-target edits at these non-canonical PAM sites. Results: Here, we identify a novel Cas12a nuclease CeCas12a from Coprococcus eutactus, which is a programmable nuclease with genome-editing efficiencies comparable to AsCas12a and LbCas12a in human cells. Moreover, CeCas12a is revealed to be more stringent for PAM recognition in vitro and in vivo followed by very low off-target editing rates in cells. Notably, CeCas12a renders less off-target edits located at C-containing PAM at multiple sites compared to LbCas12a and AsCas12a, as assessed by targeted sequencing methods. Conclusions: Our study shows that CeCas12a nuclease is active in human cells and the stringency of PAM recognition could be an important factor shaping off-target editing in gene editing. Thus, CeCas12a provides a promising candidate with distinctive characteristics for research and therapeutic applications.

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Section: Gene Editing With Cecas12a and Bfcas12a In Human Cellsmentioning

confidence: 99%

A Cas12a ortholog with stringent PAM recognition followed by low off-target editing rates for genome editing

et al. 2020

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“…Applying CRISPR‐Cas9 under ex vivo conditions may be technically less challenging but equally valuable for disease therapy. For instance, ex vivo genome editing in hematopoietic stem cells (HSCs) could potentially provide a cure for patients carrying sickle cell disease (SCD) and β‐thalassaemia, and targeted insertions via CRISPR strategies may provide a valuable alternative to T‐cell engineering for cancer immunotherapy . A proof‐of‐concept study by Dewitt et al has reported an efficient correction of the E6V mutation at sickle alleles in patients' HSCs, through CRISPR‐HDR‐based replacement with the assistance of oligonucleotide donors.…”

Section: High‐efficiency Genome Editing and New Applications Enabled mentioning

confidence: 99%

“…A proof‐of‐concept study by Dewitt et al has reported an efficient correction of the E6V mutation at sickle alleles in patients' HSCs, through CRISPR‐HDR‐based replacement with the assistance of oligonucleotide donors. Using AAV‐delivered Cpf1, Dai et al built stable CAR‐T cells with immune‐checkpoint knockout (KIKO CAR‐T cells) via the HDR‐based strategy in one step.…”

Section: High‐efficiency Genome Editing and New Applications Enabled mentioning

confidence: 99%

“…For instance, ex vivo genome editing in hematopoietic stem cells (HSCs) could potentially provide a cure for patients carrying sickle cell disease (SCD) and β-thalassaemia, 85 and targeted insertions via CRISPR strategies may provide a valuable alternative to T-cell engineering for cancer immunotherapy. 86 which identified TOP2A and CDK6 as new genes responsible for the drug resistance to purine analogue 6-thioguanine. 93 Subsequent screenings also discovered other genes critical to cancer development and treatment, [94][95][96] such as BCR and ABL, which could be potentially regarded as new therapeutic targets in leukaemia and colorectal carcinoma.…”

Section: Genome Editing For Disease Therapymentioning

confidence: 99%

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The rapidly advancing Class 2 CRISPR‐Cas technologies: A customizable toolbox for molecular manipulations

Wang

Zhang

Feng

2020

J Cellular Molecular Medi

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The CRISPR‐Cas technologies derived from bacterial and archaeal adaptive immune systems have emerged as a series of groundbreaking nucleic acid‐guided gene editing tools, ultimately standing out among several engineered nucleases because of their high efficiency, sequence‐specific targeting, ease of programming and versatility. Facilitated by the advancement across multiple disciplines such as bioinformatics, structural biology and high‐throughput sequencing, the discoveries and engineering of various innovative CRISPR‐Cas systems are rapidly expanding the CRISPR toolbox. This is revolutionizing not only genome editing but also various other types of nucleic acid‐guided manipulations such as transcriptional control and genomic imaging. Meanwhile, the adaptation of various CRISPR strategies in multiple settings has realized numerous previously non‐existing applications, ranging from the introduction of sophisticated approaches in basic research to impactful agricultural and therapeutic applications. Here, we summarize the recent advances of CRISPR technologies and strategies, as well as their impactful applications.

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“…The Sadelain group inserted a CAR into the TRAC locus by electroporating T cells with Cas9/gRNA RNPs and delivering the CAR transgene using rAAV6 (Eyquem et al 2017). The Chen group also recently generated CAR-T cells by electroporating Cpf1 mRNA while delivering gRNA and donor DNA sequences via AAV, a method which enabled genetic disruption of a second location (Dai et al 2019). The Marson lab similarly delivered Cas9/gRNA RNP into T cells and used high-output PCR products as donor templates to correct a pathological IL2RA defect and replace endogenous TCR genes with a cancer antigen-specific transgenic TCR (Roth et al 2018).…”

Section: Introductionmentioning

confidence: 99%

Self-cutting and integrating CRISPR plasmids (SCIPs) enable targeted genomic integration of genetic payloads for rapid cell engineering

Bloemberg

Sosa-Miranda

Nguyen

et al. 2020

Preprint

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Since observations that CRISPR nucleases function in mammalian cells, many strategies have been devised to adapt them for genetic engineering. Here, we investigated self-cutting and integrating Cas9/CRISPR plasmids (SCIPs) as easy-to-use gene editing tools that insert themselves at CRISPR-guided locations. SCIPs demonstrated similar expression kinetics and gene disruption efficiency in mouse (EL4) and human (Jurkat) cells, with stable integration in 3-6% of transfected cells. Clonal sequencing analysis indicated that integrants showed bi-or mono-allelic integration of entire CRISPR plasmids in predictable orientations with approximately half of clones showing indel formation. Interestingly, including longer homology arms (HAs) (up to 500 bp) in varying orientations only modestly increased knock-in efficiency (~2-fold), indicating that SCIP integration primarily occurs through homology-independent mechanisms.Using a SCIP-payload design (SCIPay) which liberates a promoter-less sequence flanked by HAs thereby requiring perfect homology-directed repair (HDR) for expression, longer HAs resulted in higher integration efficiency but did not affect integration efficiency for the remaining plasmid sequence. As proofs-ofconcept, we used SCIPay to 1) insert a gene fragment encoding tdTomato into the CD69 locus of Jurkat cells, thereby creating a novel cell line that reports T cell activation, and 2) insert a chimeric antigen receptor (CAR) gene into the T cell receptor alpha constant (TRAC) locus. Here, we demonstrate that SCIPs function as simple, efficient, and programmable tools useful for generating gene knockout/knock-in cell lines and suggest future utility in knock-in site screening/optimization, unbiased off-target site identification, and multiplexed, iterative, and/or library-scale automated genome engineering.

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One-step generation of modular CAR-T cells with AAV–Cpf1

Cited by 124 publications

References 36 publications

A Cas12a ortholog with stringent PAM recognition followed by low off-target editing rates for genome editing

A Cas12a ortholog with stringent PAM recognition followed by low off-target editing rates for genome editing

The rapidly advancing Class 2 CRISPR‐Cas technologies: A customizable toolbox for molecular manipulations

Self-cutting and integrating CRISPR plasmids (SCIPs) enable targeted genomic integration of genetic payloads for rapid cell engineering

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