Molecular Therapy: Methods & Clinical Development (Mar 2024)

Improving cell-specific recombination using AAV vectors in the murine CNS by capsid and expression cassette optimization

  • Hayato Kawabata,
  • Ayumu Konno,
  • Yasunori Matsuzaki,
  • Yumika Sato,
  • Mika Kawachi,
  • Ryo Aoki,
  • Saki Tsutsumi,
  • Shota Togai,
  • Ryosuke Kobayashi,
  • Takuro Horii,
  • Izuho Hatada,
  • Hirokazu Hirai

Journal volume & issue
Vol. 32, no. 1
p. 101185

Abstract

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The production of cell-type– and age-specific genetically modified mice is a powerful approach for unraveling unknown gene functions. Here, we present a simple and timesaving method that enables adeno-associated virus (AAV)–mediated cell-type– and age-specific recombination in floxed mice. To achieve astrocyte-specific recombination in floxed Ai14 reporter mice, we intravenously injected blood-brain barrier–penetrating AAV-PHP.eB vectors expressing Cre recombinase (Cre) using the astrocyte-specific mouse glial fibrillary acidic protein (mGfaABC1D) promoter. However, we observed nonspecific neuron-predominant transduction despite the use of an astrocyte-specific promoter. We speculated that subtle but continuous Cre expression in nonastrocytic cells triggers recombination, and that excess production of Cre in astrocytes inhibits recombination by forming Cre-DNA aggregates. Here, we resolved this paradoxical event by dividing a single AAV into two mGfaABC1D-promoter-driven AAV vectors, one expressing codon-optimized flippase (FlpO) and another expressing flippase recognition target–flanked rapidly degrading Cre (dCre), together with switching the neuron-tropic PHP.eB capsid to astrocyte-tropic AAV-F. Moreover, we found that the FlpO-dCre system with a target cell-tropic capsid can also function in neuron-targeting recombination in floxed mice.

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