Extra-viral DNA in adeno-associated viral vector preparations induces TLR9-dependent innate immune responses in human plasmacytoid dendritic cells

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作者
Kirsten Bucher
Eduardo Rodríguez-Bocanegra
Bernd Wissinger
Torsten Strasser
Simon J. Clark
Andreas L. Birkenfeld
Dorothea Siegel-Axel
M. Dominik Fischer
机构
[1] University Hospital Tübingen,University Eye Hospital, Centre for Ophthalmology
[2] University Hospital Tübingen,Institute for Ophthalmic Research, Centre for Ophthalmology
[3] University of Tübingen,Lydia Becker Institute of Immunology and Inflammation, Faculty of Biology, Medicine and Health
[4] University of Manchester,Division of Endocrinology, Diabetology and Nephrology, Department of Internal Medicine IV
[5] Institute of Diabetes Research and Metabolic Diseases (IDM) of the Helmholtz Center Munich,Oxford Eye Hospital
[6] German Center for Diabetes Research (DZD),Nuffield Laboratory of Ophthalmology, Department of Clinical Neurosciences
[7] University Hospital of Tübingen,undefined
[8] Oxford University NHS Foundation Trust,undefined
[9] University of Oxford,undefined
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摘要
Adeno-associated viral (AAV) vector suspensions produced in either human derived HEK cells or in Spodoptera frugiperda (Sf9) insect cells differ in terms of residual host cell components as well as species-specific post-translational modifications displayed on the AAV capsid proteins. Here we analysed the impact of these differences on the immunogenic properties of the vector. We stimulated human plasmacytoid dendritic cells with various lots of HEK cell-produced and Sf9 cell-produced AAV-CMV-eGFP vectors derived from different manufacturers. We found that AAV8-CMV-eGFP as well as AAV2-CMV-eGFP vectors induced lot-specific but not production platform-specific or manufacturer-specific inflammatory cytokine responses. These could be reduced or abolished by blocking toll-like receptor 9 signalling or by enzymatically reducing DNA in the vector lots using DNase. Successful HEK cell transduction by DNase-treated AAV lots and DNA analyses demonstrated that DNase did not affect the integrity of the vector but degraded extra-viral DNA. We conclude that both HEK- and Sf9-cell derived AAV preparations can contain immunogenic extra-viral DNA components which can trigger lot-specific inflammatory immune responses. This suggests that improved strategies to remove extra-viral DNA impurities may be instrumental in reducing the immunogenic properties of AAV vector preparations.
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