# Toward an all-in-one recombinant adeno-associated virus vector for functionally ablating the prion gene using CRISPR-Cas technology

**Authors:** Claire Verkuyl, Ari Belotserkovsky, Thomas Zerbes, Declan Williams, Medha R. Krishnan, Sabrina Zhu, Sophie Grunnesjӧ, Shehab Eid, Cunjie Zhang, Wenda Zhao, Leo Xu, Eleanore Lin, Teaghan O’Shea, Benjamin Draper, Andreas Jungman, Patrick Most, Gerold Schmitt-Ulms

PMC · DOI: 10.1371/journal.pone.0336578 · 2025-11-07

## TL;DR

Researchers developed a gene therapy vector to reduce prion protein in the brain, which could help treat prion diseases.

## Contribution

A first-generation all-in-one rAAV vector for prion gene editing using CRISPR-Cas technology was created and tested.

## Key findings

- A prion gene-specific guide RNA and Cas9 endonuclease were delivered via an rAAV vector with a cell-specific promoter.
- Prion gene editing rates of ~20% in human cells and ~5% in mice were achieved.
- The 9P31 capsid showed 7.5-fold higher gene expression than PHP.eB after injection.

## Abstract

Any strategy that can selectively and persistently lower the brain levels of the cellular prion protein (PrPC) is expected to extend survival in prion diseases. Recent advances in the virus-mediated delivery of gene therapies prompted us to explore if a recombinant adeno-associated virus (rAAV) vector delivering a CRISPR-Cas-based gene editor can be devised that induces a functional knockout of the prion gene. Whereas the eventual objective is to assess the therapeutic potency of an optimized vector in prion-infected mice, in this proof-of-concept study, we evaluated tools and methods that are suited to achieve this goal. The result of these efforts is a first-generation all-in-one rAAV vector that codes for a prion gene-specific guide RNA and a small Cas9 endonuclease, whose expression is controlled by a truncated neural cell adhesion molecule 1 (NCAM1) promoter that is active in PrPC expressing cells. We also constructed a second rAAV vector coding for a prion gene-specific ‘traffic light reporter’ (TLR). The TLR can be used to monitor prion gene-editing efficacy by coding for red and green fluorescent proteins separated by a segment of the prion gene that is targeted by the gene editor. For the purification of AAVs, we adopted a robust and scalable rAAV vector assembly pipeline and undertook proof-of-concept prion gene editing experiments in human cells and mice, which to date yielded prion gene editing rates of approximately 20% and 5%, respectively. Finally, we compared brain distributions of rAAV vectors following intrathalamic versus retro-orbital injection, and selected the 9P31 capsid for future studies based on a 7.5-fold higher heterologous gene expression level as compared to the PHP.eB capsid.

## Linked entities

- **Genes:** NCAM1 (neural cell adhesion molecule 1) [NCBI Gene 4684]
- **Proteins:** PRNP (prion protein (Kanno blood group))
- **Species:** Homo sapiens (taxon 9606), Mus musculus (taxon 10090)

## Full-text entities

- **Genes:** NCAM1 (neural cell adhesion molecule 1) [NCBI Gene 4684] {aka CD56, MSK39, NCAM}, PRNP (prion protein (Kanno blood group)) [NCBI Gene 5621] {aka ASCR, AltPrP, CD230, CJD, GSS, KURU}
- **Diseases:** prion (MESH:D017096)
- **Species:** Homo sapiens (human, species) [taxon 9606], Mus musculus (house mouse, species) [taxon 10090], Adeno-associated virus (species) [taxon 272636]

## Figures

10 figures with captions in the complete paper: https://tomesphere.com/paper/PMC12594398/full.md

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Source: https://tomesphere.com/paper/PMC12594398