Imaging of adeno-associated viral capsids for purposes of gene editing using CEST NMR/MRI

Bonnie Lam; Mark Velasquez; Tomoko Ogiyama; Kevin Godines; Fan-Yun Szu; A J Velasquez-Mao; Wissam AlGhuraibawi; Jingshen Wang; Phillip B Messersmith; Moriel H Vandsburger

doi:10.1002/mrm.30058

Imaging of adeno-associated viral capsids for purposes of gene editing using CEST NMR/MRI

Magn Reson Med. 2024 Aug;92(2):792-806. doi: 10.1002/mrm.30058. Epub 2024 Apr 23.

Authors

Affiliations

¹ Department of Bioengineering, UC Berkeley, Berkeley, California, USA.
² Division of Biostatistics, UC Berkeley, Berkeley, California, USA.
³ Department of Materials Science and Engineering, UC Berkeley, Berkeley, California, USA.
⁴ Materials Sciences Division, Lawrence Berkeley National Laboratory, Berkeley, California, USA.

PMID: 38651648
PMCID: PMC11142879 (available on 2025-08-01)
DOI: 10.1002/mrm.30058

Abstract

Purpose: Gene therapy using adeno-associated virus (AAV) vector-mediated gene delivery has undergone substantial growth in recent years with promising results in both preclinical and clinical studies, as well as emerging regulatory approval. However, the inability to quantify the efficacy of gene therapy from cellular delivery of gene-editing technology to specific functional outcomes is an obstacle for efficient development of gene therapy treatments. Building on prior works that used the CEST reporter gene lysine rich protein, we hypothesized that AAV viral capsids may generate endogenous CEST contrast from an abundance of surface lysine residues.

Methods: NMR experiments were performed on isolated solutions of AAV serotypes 1-9 on a Bruker 800-MHz vertical scanner. In vitro experiments were performed for testing of CEST-NMR contrast of AAV2 capsids under varying pH, density, biological transduction stage, and across multiple serotypes and mixed biological media. Reverse transcriptase-polymerase chain reaction was used to quantify virus concentration. Subsequent experiments at 7 T optimized CEST saturation schemes for AAV contrast detection and detected AAV2 particles encapsulated in a biocompatible hydrogel administered in the hind limb of mice.

Results: CEST-NMR experiments revealed CEST contrast up to 52% for AAV2 viral capsids between 0.6 and 0.8 ppm. CEST contrast generated by AAV2 demonstrated high levels of CEST contrast across a variety of chemical environments, concentrations, and saturation schemes. AAV2 CEST contrast displayed significant positive correlations with capsid density (R² > 0.99, p < 0.001), pH (R² = 0.97, p = 0.01), and viral titer per cell count (R² = 0.92, p < 0.001). Transition to a preclinical field strength yielded up to 11.8% CEST contrast following optimization of saturation parameters. In vivo detection revealed statistically significant molecular contrast between viral and empty hydrogels using both mean values (4.67 ± 0.75% AAV2 vs. 3.47 ± 0.87% empty hydrogel, p = 0.02) and quantile analysis.

Conclusion: AAV2 viral capsids exhibit strong capacity as an endogenous CEST contrast agent and can potentially be used for monitoring and evaluation of AAV vector-mediated gene therapy protocols.

Keywords: AAV; CEST; MRI; gene therapy.

MeSH terms

Animals
Capsid* / chemistry
Contrast Media / chemistry
Dependovirus* / genetics
Gene Editing / methods
Genetic Therapy / methods
Genetic Vectors
Humans
Magnetic Resonance Imaging* / methods
Magnetic Resonance Spectroscopy / methods
Mice

Substances

Contrast Media

Abstract

MeSH terms

Substances

Grants and funding