The TLR9-MyD88 pathway is critical for adaptive immune responses to adeno-associated virus gene therapy vectors in mice
Jiangao Zhu, … , Xiaopei Huang, Yiping Yang
Jiangao Zhu, … , Xiaopei Huang, Yiping Yang
Published July 1, 2009
Citation Information: J Clin Invest. 2009;119(8):2388-2398. https://doi.org/10.1172/JCI37607.
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Research Article Genetics

The TLR9-MyD88 pathway is critical for adaptive immune responses to adeno-associated virus gene therapy vectors in mice

Abstract

Recombinant adeno-associated viruses (AAVs) have been used widely for in vivo gene therapy. However, adaptive immune responses to AAV have posed a significant hurdle in clinical application of AAV vectors. Recent advances have suggested a crucial role for innate immunity in shaping adaptive immune responses. How AAV activates innate immunity, and thereby promotes AAV-targeted adaptive immune responses, remains unknown. Here we show that AAV activates mouse plasmacytoid DCs (pDCs) via TLR9 to produce type I IFNs. In vivo, the TLR9-MyD88 pathway was crucial to the activation of CD8+ T cell responses to both the transgene product and the AAV capsid, leading to loss of transgene expression and the generation of transgene product–specific and AAV-neutralizing antibodies. We further demonstrate that TLR9-dependent activation of adaptive immunity targeting AAV was mediated by type I IFNs and that human pDCs could be activated in vitro to induce type I IFN production via TLR9. These results reveal an essential role for the TLR9-MyD88–type I IFN pathway in induction of adaptive immune responses to AAV and suggest that strategies that interfere with this pathway may improve the outcome of AAV-mediated gene therapy in humans.

Authors

Jiangao Zhu, Xiaopei Huang, Yiping Yang

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Figure 8

Type I IFNs play a critical role in adaptive immune responses to AAV.

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Type I IFNs play a critical role in adaptive immune responses to AAV. AA...
AAV2-HA was injected intramuscularly into WT or Ifnr–/– mice. (A) After 12 and 36 days, the infected muscles were harvested and analyzed for HA expression by immunohistochemistry. Original magnification, ×100. (B) CD5+ T cells purified from splenocytes at day 36 after infection, along with uninfected WT splenocytes (naive), were restimulated with AAV2-HA at 0, 50, 500, or 5,000 vg/cell. Proliferation of AAV-specific T cells was analyzed by 3H-thymidine incorporation. Data reflect the mean ± SD of the stimulation index, which was calculated by dividing 3H counts in cpm in the presence of viral stimulation by those in the absence of stimulation, as a function of different virus doses. (C and D) Serum samples were harvested at day 36 for the measurement of anti-HA (C) and AAV-neutralizing (D) antibody titers. Data shown are representative of 2 independent experiments.