Engineered pegRNAs improve prime editing efficiency

Nelson, Jelani; Randolph, Peyton B.; Shen, Simon P.; Everette, Kelcee A.; Chen, Peter J.; Anzalone, Andrew V.; An, Meirui; Newby, Gregory A.; Chen, Jonathan C.; Hsu, Alvin; Liu, David R.

doi:10.1038/s41587-021-01039-7

Cited by 428 publications

(405 citation statements)

References 61 publications

Supporting

Mentioning

389

Contrasting

Unclassified

Order By: Relevance

“…In vitro transcription of prime editor and MLH1dn mRNA used in iPSC and T cell experiments As described previously (Nelson et al, 2021), plasmids were cloned to encode an inactivated T7 promoter followed by a 5 0 untranslated region (UTR), Kozak sequence, coding sequences of PE2 or MLH1dn, and a 3 0 UTR. T7 promoter inactivation prevents potential transcription from circular plasmid template during mRNA generation.…”

Section: Prime Editing Of Therapeutically Relevant Locimentioning

confidence: 99%

“…Strategic installation of additional silent mutations nearby an intended edit can also improve prime editing efficiency by evading MMR recognition, even in the absence of MLH1dn. Finally, we engineered an optimized “PEmax” prime editor architecture that further increased editing efficiency in synergy with PE4, PE5, and engineered pegRNAs (epegRNAs) ( Nelson et al, 2021 ). These findings deepen our understanding of prime editing and establish prime editing systems with substantially improved efficiency and outcome purity across 191 different edits at 20 loci in seven mammalian cell types.…”

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Enhanced prime editing systems by manipulating cellular determinants of editing outcomes

Chen

Hussmann

Yan

et al. 2021

Cell

Self Cite

478

576

View full text Add to dashboard Cite

While prime editing enables precise sequence changes in DNA, cellular determinants of prime editing remain poorly understood. Using pooled CRISPRi screens, we discovered that DNA mismatch repair (MMR) impedes prime editing and promotes undesired indel byproducts. We developed PE4 and PE5 prime editing systems in which transient expression of an engineered MMR-inhibiting protein enhances the efficiency of substitution, small insertion, and small deletion prime edits by an average 7.7-fold and 2.0-fold compared to PE2 and PE3 systems, respectively, while improving edit/indel ratios by 3.4-fold in MMR-proficient cell types. Strategic installation of silent mutations near the intended edit can enhance prime editing outcomes by evading MMR. Prime editor protein optimization resulted in a PEmax architecture that enhances editing efficacy by 2.8-fold on average in HeLa cells. These findings enrich our understanding of prime editing and establish prime editing systems that show substantial improvement across 191 edits in seven mammalian cell types. ll

show abstract

Section: Prime Editing Of Therapeutically Relevant Locimentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Enhanced prime editing systems by manipulating cellular determinants of editing outcomes

Chen

Hussmann

Yan

et al. 2021

Cell

Self Cite

478

576

View full text Add to dashboard Cite

show abstract

“…To determine if coselection could streamline the production of homozygous cell lines for functional studies, we designed pegRNAs to install well-characterized and clinically relevant MTOR hyperactivating mutations 49,50,52,53 or rapamycin resistance mutations [54][55][56] . While the design and screening of several pegRNAs remains a critical aspect of successful PE 1,7,12 , we designed and tested only one pegRNA per target based on previously established rules 1,5 for this proof-of-concept experiment.…”

Section: Installation Of Clinically Relevant Mutations At Mtormentioning

confidence: 99%

“…Thus, the optimal PE strategy to adopt varies according to the context and there is a need to develop methods to consistently improve its success rate.To circumvent these limitations several approaches have been implemented including editing with purified ribonucleoprotein complexes (RNPs) 10 , mRNA-based delivery 7,11 , engineered pegRNAs (epegRNAs) 12 , NLS-and codon-optimized prime editors 7,9,13 , enrichment with puromycin, and fluorescent reporter-based selection [14][15][16] . Nevertheless, these improvements are still dependent on extensive pegRNA optimization, absolute activity remains low, and the streamlined production of homozygous cell lines has yet to be achieved 1,12 . Hence, further refinements to these approaches are needed to boost the efficiency of PE in human cells 2,3,7,12 .We previously reported a robust coselection method for CRISPR nucleases that relies on cotargeting a gene of interest (GOI) and the ATP1A1 locus to confer dominant cellular resistance to ouabain 17 , a plant-derived inhibitor of the ubiquitous and essential Na + /K + ATPase 18,19 .…”

mentioning

confidence: 99%

“…Nevertheless, these improvements are still dependent on extensive pegRNA optimization, absolute activity remains low, and the streamlined production of homozygous cell lines has yet to be achieved 1,12 . Hence, further refinements to these approaches are needed to boost the efficiency of PE in human cells 2,3,7,12 .We previously reported a robust coselection method for CRISPR nucleases that relies on cotargeting a gene of interest (GOI) and the ATP1A1 locus to confer dominant cellular resistance to ouabain 17 , a plant-derived inhibitor of the ubiquitous and essential Na + /K + ATPase 18,19 . Such an approach derives from the observation that simultaneous targeting of two different loci results in double-editing events that are not statistically independent 17,[20][21][22][23][24][25] .…”

mentioning

confidence: 99%

See 1 more Smart Citation

Marker-free coselection for successive rounds of prime editing in human cells

Levesque

Mayorga

Fiset

et al. 2021

Preprint

View full text Add to dashboard Cite

Prime editing enables the introduction of precise point mutations, small insertions, or short deletions without requiring donor DNA templates. However, editing efficiency remains a key challenge in a broad range of cell types. We designed a robust coselection strategy to perform successive rounds of genetic changes in human cells using CRISPR-Cas nucleases and prime editors. Through coediting, the recovery of cells modified at a target gene of interest is coupled to selection for dominant alleles of the ubiquitous and essential sodium/potassium pump (Na+/K+ ATPase). The method improves prime editing efficiency 1.5–10-fold in K562 and HeLa cells, reaching up to 83% of desired alleles in cell populations, for previously optimized prime editing guide RNAs (pegRNAs). Using pegRNAs designed de novo, we readily engineered homozygous cell lines with cancer-associated or drug resistant MTOR mutations displaying altered mTORC1 signaling. Our approach streamlines the production of cell lines with multiple genetic modifications to create cellular models for biological research and lays the foundation for the development of cell-type specific coselection strategies.

show abstract

Engineered CRISPR RNA improves the RNA cleavage efficiency of hfCas13X

Liu,

Zhang,

Wang

et al. 2024

FEBS Letters

View full text Add to dashboard Cite

As the most compact variant in the Cas13 family, CRISPR‐Cas13X holds considerable promise for gene therapy applications. The development of high‐fidelity Cas13X (hfCas13X) mutants has enhanced the safety profile for in vivo applications. However, a notable reduction in on‐target cleavage efficiency accompanies the diminished collateral cleavage activity in hfCas13X. In this study, we obtained two engineered crRNA mutants that notably enhance the on‐target cleavage efficiency of hfCas13X. Furthermore, we have identified a novel crRNA structure that consistently augments the on‐target cleavage efficiency of hfCas13X across various cellular environments, without significant enhancement of its collateral activity. These findings collectively enrich the gene‐editing toolkit, presenting a more effective hfCas13X system for future research and application.

show abstract

Engineered pegRNAs improve prime editing efficiency

Cited by 428 publications

References 61 publications

Enhanced prime editing systems by manipulating cellular determinants of editing outcomes

Enhanced prime editing systems by manipulating cellular determinants of editing outcomes

Marker-free coselection for successive rounds of prime editing in human cells

Engineered CRISPR RNA improves the RNA cleavage efficiency of hfCas13X

Contact Info

Product

Resources

About