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TIGER: A tdTomato in-vivo genome-editing reporter mouse for investigating precision-editor delivery approaches

Du, Samuel1; Palczewska, Grazyna1; Dong, Zhiqian1; Lauterborn, Julie1; Kaipa, Balasankara1; Yan, Alexander1; Holubowicz, Rafal1; Ha, Siyoung1; Chen, Paul2; Gall, Christine1; Zode, Gulab1; Liu, David2; Palczewski, Krzysztof1

Published Sep 03, 2025 on Dryad. https://doi.org/10.5061/dryad.866t1g23p

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Sep 03, 2025 version files 79.29 KB

Abstract

In vivo genome editing has the potential to address many inherited and environmental disorders. However, a major hurdle for the clinical translation of genome editing is safe, efficient delivery to disease-relevant tissues. A modality-agnostic reporter animal model that facilitates rapid, precise, and quantifiable assessment of functional delivery and editing could greatly enhance the evaluation and translation of delivery technologies. Here, we present the development of the TIGER (tdTomato in vivo genome-editing reporter) mouse, a reporter strain that harbors an integrated and constitutively expressed mutated tdTomato gene in the Polr2a locus. The mutations (Q115X, Q357X) abolish fluorescence, but successful adenine base editing (ABE) or prime editing (PE) restores tdTomato fluorescence. This mouse model facilitates the tissue- and cell-type-specific assessment of genome editing agent delivery. We describe several editing strategies validated in vitro and demonstrate efficient ABE and PE in vivo using viral and non-viral delivery vectors targeting four cell types within the mouse eye: the retinal pigment epithelium (RPE), photoreceptors, Müller glia, and the trabecular meshwork. We show direct editing characterization in the ocular tissues via in vivo and ex vivo two-photon confocal microscopy, and verify the spectral and fluorescence lifetime properties of tdTomato reporter in other mouse tissues. Additionally, we demonstrate successful AAV-mediated prime editing of extraocular tissues, including hepatocytes, skeletal muscle, and brain neurons, by intravenous injection. Thus, the TIGER mouse facilitates the direct development, comparison, and optimization of delivery platforms for efficient and productive ABE or PE broadly applicable in vivo across multiple tissues tested in this study.