27: ENVLPE+: Shuttling VLPs that load functional CRISPR RNPs episode artwork

EPISODE · May 21, 2025 · 16 MIN

27: ENVLPE+: Shuttling VLPs that load functional CRISPR RNPs

from Base by Base · host Gustavo Barra

Geilenkeuser J et al., Cell - A Cell paper describing ENVLPE/ENVLPE+, virus-like particles engineered with nucleocytosolic-shuttling Gag-PCP to recruit aptamer-tagged (pe)gRNAs and preferentially package fully assembled CRISPR RNPs. Csy4-mediated 3' protection of pegRNAs and modular minimal budding modules boost prime and base editing in cells and restore gene function in retinal mouse models. Key terms: VLP, prime editing, pegRNA stabilization, Csy4, gene delivery. Study Highlights:The authors engineered nucleocytosolic-shuttling Gag-PCP VLPs (ENVLPE) that retrieve assembled Cas effector RNPs via PP7-aptamer-tagged (pe)gRNAs, increasing the fraction of functional cargo. Co-expression of Csy4 stabilizes pegRNA 3' ends and markedly improves prime editing rates during RNP delivery. A minimal homomeric “miniENVLPE” and an enhanced ENVLPE+ with GCN4 coiled coils achieve high per-particle loading of Cas9 and pegRNA. ENVLPE+ outperforms prior eVLP systems ex vivo in primary T cells and in vivo in two mouse retinal disease models, restoring protein expression and visual function. Conclusion:ENVLPE+ is a modular VLP platform that preferentially packages intact RNP editors via aptamer-tagged (pe)gRNAs and uses Csy4 to protect pegRNA 3' ends, producing higher per-particle editing efficiency and demonstrating therapeutic potential in ex vivo and in vivo models. QC:This episode was checked against the original article PDF and publication metadata for the episode release published on 2025-05-21. QC Scope:- article metadata and core scientific claims from the narration- excludes analogies, intro/outro, and music QC Summary:- factual score: 10/10- metadata score: 10/10- supported core claims: 8- claims flagged for review: 0- metadata checks passed: 4- metadata issues found: 0 Metadata Audited:- article_doi- article_title- article_journal- license Factual Items Audited:- ENVLPE enables loading of fully assembled editor RNPs by recruiting PP7-tagged gRNAs via Gag-PCP, rather than fusing Cas9 to Gag.- Csy4/Cas6f protection fortifies the pegRNA 3' end, increasing prime editing efficiency in ENVLPE.- ENVLPE+ improves per-particle loading and editing efficacy via GCN4 coiled-coil enhancement.- ENVLPE+ particles carry high cargo per particle (around 78 Cas9 and 77 pegRNAs) and outperform prior VLPs per particle.- In hiPSC-derived cortical neurons, ENVLPE/ENVLPE+ achieve about 90% base editing at the B2M locus.- ENVLPE+ enables in vivo prime editing in inherited retinal disease models, restoring gene function and improving visual outcomes. QC result: Pass.

Geilenkeuser J et al., Cell - A Cell paper describing ENVLPE/ENVLPE+, virus-like particles engineered with nucleocytosolic-shuttling Gag-PCP to recruit aptamer-tagged (pe)gRNAs and preferentially package fully assembled CRISPR RNPs. Csy4-mediated 3' protection of pegRNAs and modular minimal budding modules boost prime and base editing in cells and restore gene function in retinal mouse models. Key terms: VLP, prime editing, pegRNA stabilization, Csy4, gene delivery. Study Highlights:The authors engineered nucleocytosolic-shuttling Gag-PCP VLPs (ENVLPE) that retrieve assembled Cas effector RNPs via PP7-aptamer-tagged (pe)gRNAs, increasing the fraction of functional cargo. Co-expression of Csy4 stabilizes pegRNA 3' ends and markedly improves prime editing rates during RNP delivery. A minimal homomeric “miniENVLPE” and an enhanced ENVLPE+ with GCN4 coiled coils achieve high per-particle loading of Cas9 and pegRNA. ENVLPE+ outperforms prior eVLP systems ex vivo in primary T cells and in vivo in two mouse retinal disease models, restoring protein expression and visual function. Conclusion:ENVLPE+ is a modular VLP platform that preferentially packages intact RNP editors via aptamer-tagged (pe)gRNAs and uses Csy4 to protect pegRNA 3' ends, producing higher per-particle editing efficiency and demonstrating therapeutic potential in ex vivo and in vivo models. QC:This episode was checked against the original article PDF and publication metadata for the episode release published on 2025-05-21. QC Scope:- article metadata and core scientific claims from the narration- excludes analogies, intro/outro, and music QC Summary:- factual score: 10/10- metadata score: 10/10- supported core claims: 8- claims flagged for review: 0- metadata checks passed: 4- metadata issues found: 0 Metadata Audited:- article_doi- article_title- article_journal- license Factual Items Audited:- ENVLPE enables loading of fully assembled editor RNPs by recruiting PP7-tagged gRNAs via Gag-PCP, rather than fusing Cas9 to Gag.- Csy4/Cas6f protection fortifies the pegRNA 3' end, increasing prime editing efficiency in ENVLPE.- ENVLPE+ improves per-particle loading and editing efficacy via GCN4 coiled-coil enhancement.- ENVLPE+ particles carry high cargo per particle (around 78 Cas9 and 77 pegRNAs) and outperform prior VLPs per particle.- In hiPSC-derived cortical neurons, ENVLPE/ENVLPE+ achieve about 90% base editing at the B2M locus.- ENVLPE+ enables in vivo prime editing in inherited retinal disease models, restoring gene function and improving visual outcomes. QC result: Pass.

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27: ENVLPE+: Shuttling VLPs that load functional CRISPR RNPs

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Geilenkeuser J et al., Cell - A Cell paper describing ENVLPE/ENVLPE+, virus-like particles engineered with nucleocytosolic-shuttling Gag-PCP to recruit aptamer-tagged (pe)gRNAs and preferentially package fully assembled CRISPR RNPs. Csy4-mediated 3'...

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