Table 1.
Comparison of in vivo gene transfer and gene editing strategies.
| Gene transfer | Gene editing | |
|---|---|---|
|
| ||
| Principle | Deliver copy of functional gene | Restore or disrupt endogenous genes |
|
| ||
| Advantages | •Can treat any patient carrying any variants in a given gene • Does not require DNA breaks • Low risk of integrations with AAV-based vectors • Long-term efficacy • Longer experience in clinical development |
• Versatile technology, including base editing and prime editing • Editing of endogenous DNA, potentially conferring permanent efficacy • Can be delivered via viral or LNP systems • Transitory presence of editing machinery and delivery system (LNP) • Re-dosing may be possible when using LNPs |
|
| ||
| Limitations | • Cannot be “undone” • Current strategies require viral vectors • Adverse events include immune reactions caused by viral capsid • Re-dosing limited by development of neutralizing antibodies • Efficacy may dilute with time if AAV-delivered genetic information persists as episome • Possible development of autoantibodies against newly expressed proteins |
• Cannot be “undone” • Only patients with variant in specific target region can be treated • If viral vectors are used, adverse events include immune reactions caused by viral capsid • Possible development of autoantibodies against newly expressed proteins • Risk of off-target editing and unintended effect |
AAV, adeno-associated virus; LNP, lipid nanoparticle.