# Extracellular vesicle-mediated delivery of genetic material for transformation and CRISPR/Cas9-based gene editing in Pneumocystis murina

**Authors:** Steven G. Sayson, Alan Ashbaugh, Lillian C. Bauer, A. George Smulian

PMC · DOI: 10.1128/mbio.01825-25 · mBio · 2025-09-23

## TL;DR

Researchers developed a new method to edit the genome of Pneumocystis murina using extracellular vesicles, enabling genetic studies in this hard-to-manipulate fungus.

## Contribution

The first successful CRISPR/Cas9-based gene editing in Pneumocystis using extracellular vesicles for DNA delivery.

## Key findings

- Stable in vivo expression of reporter genes in Pneumocystis murina was achieved for up to 5 weeks.
- CRISPR/Cas9-mediated homologous recombination successfully introduced a DhpsARS mutation confirmed by sequencing.
- The method enables functional genomics and drug target validation in Pneumocystis.

## Abstract

Pneumocystis species are obligate fungal pathogens that cause severe pneumonia, particularly in immunocompromised individuals. The absence of robust genetic manipulation tools has impeded our mechanistic understanding of Pneumocystis biology and the development of novel therapeutic strategies. Herein, we describe a novel method for the stable transformation and CRISPR/Cas9-mediated genetic editing of Pneumocystis murina utilizing extracellular vesicles (EVs) as a delivery vehicle. Building upon our prior investigations demonstrating EV-mediated delivery of exogenous material to Pneumocystis, we engineered mouse lung EVs to deliver plasmid DNA encoding reporter genes and CRISPR/Cas9 components. Our initial findings demonstrated successful in vitro transformation and subsequent expression of mNeonGreen and DhpsARS in P. murina organisms. Subsequently, we established stable in vivo expression of mNeonGreen in mice infected with transformed P. murina for a duration of up to 5 weeks. Furthermore, we designed and validated a CRISPR/Cas9 system targeting the P. murina Dhps gene, confirming DNA cleavage efficiency in vitro. Ultimately, we achieved successful in vivo CRISPR/Cas9-mediated homologous recombination, precisely introducing a DhpsARS mutation into the P. murina genome, which was confirmed by Sanger sequencing across all tested animals. Here, we establish a foundational methodology for genetic manipulation in Pneumocystis, thereby opening avenues for functional genomics, drug target validation, and the generation of genetically modified strains for advanced research and potential therapeutic applications.

Pneumocystis species are obligate fungal pathogens and major causes of pneumonia in immunocompromised individuals. However, their strict dependence on the mammalian lung environment has precluded the development of genetic manipulation systems, limiting our ability to interrogate gene function, study antifungal resistance mechanisms, or validate therapeutic targets. Here, we report the first successful approach for stable transformation and CRISPR/Cas9-based genome editing of Pneumocystis murina, achieved through in vivo delivery of engineered extracellular vesicles containing plasmid DNA and encoding CRISPR/Cas9 components. We demonstrate sustained transgene expression and precise modification of the dhps locus via homology-directed repair. This modular, scalable platform overcomes a long-standing barrier in the field and establishes a foundation for functional genomics in Pneumocystis and other obligate, host-adapted microbes.

## Linked entities

- **Genes:** DHPS (deoxyhypusine synthase) [NCBI Gene 1725]
- **Diseases:** pneumonia (MONDO:0005249)
- **Species:** Pneumocystis murina (taxon 263815), Mus musculus (taxon 10090)

## Full-text entities

- **Diseases:** pneumonia (MESH:D011014), fungal (MESH:D009181)
- **Species:** Mus musculus (house mouse, species) [taxon 10090], Pneumocystis murina (species) [taxon 263815]

## Full text

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## Figures

5 figures with captions in the complete paper: https://tomesphere.com/paper/PMC12607567/full.md

## References

44 references — full list in the complete paper: https://tomesphere.com/paper/PMC12607567/full.md

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Source: https://tomesphere.com/paper/PMC12607567