Aav5 syn flex chrimsonr tdt

Viruses used in this study were either acquired commercially or produced locally. The following AAV plasmids were used and detailed sequence information is available as detailed or upon request: AAVDj-hSyn-flex-mGFP-2A-synaptophysin-mRuby^{57 (link)} (Stanford Vector Core Facility, reference AAV DJ GVVC-AAV-100), AAV5-CAG-DIO-COMET-tdTomato and AAV5CAG-COMET-GFP (a gift from M. Tuszynski), AAV5-Syn-flex-ChrimsonR-tdT (Addgene 62723), AAV5-CAG-flex-Jaws-KGC-GFP-ER2 (Addgene 84445), AAV5-hSyn-DIO-hm4D (Gi)-mCherry (Addgene 44362), AAV5-hSyn-DIO-hm3D (Gq)-mCherry (Addgene 44361), AAV5-CAG-flex-tdTomato (a gift from S. Arber), AAV5CAG-flex-human diphtheria toxin receptor (DTR) (a gift from S. Arber), AAV5-DIO-TC66T-2A-eGFP-2A-oG (GT3) (Salk Institute) and AAV5-hSyn-DIO-TVAP2A-EGFP-2A-oG (a gift from T. Karayannis). All floxed AAV vectors used in the present study showed transgene expression only upon Cre-mediated recombination. Trans-synaptic tracings were performed with EnvA-G-deleted rabies–mCherry (GT3) (Salk Institute 32646) or the cre-dependent PRV Ba2017 (expressing GFP; 4.9 × 10⁹ pfu per ml; Princeton University). Injection volumes, coordinates and experimental purpose are described below.