GREATLY INCREASED EFFICIENCY OF RABIES VIRUS PRODUCTION FROM DNA
Massachusetts Institute of Technology
Presentation
Date TBA
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Poster Board
PS07-10AM-038
Poster
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Rescuing NNS viruses requires transfecting cells with plasmids expressing viral genes as well as an mRNA transcript containing the desired vector genome (or, more commonly, "antigenome", the genome's reverse complement), flanked by self-cleaving ribozymes to create authentic ends of the viral (anti)genome, allowing it to be packaged by the viral nucleoprotein. Recently, a novel family of highly-efficient ribozymes – the so-called "twister" ribozymes – was found to be widespread in eukaryotes and bacteria. Here we show that a "twister" ribozyme on the 3' end of the rabies viral antigenome increases rescue efficiency 37-fold over that of the most commonly-used 3' ribozyme (the standard hepatitis delta virus ribozyme) and 4.5-fold over that of the best previously-used 3' ribozyme (the "super cutter" hepatitis delta virus ribozyme). This increased efficiency should considerably increase the uniformity of barcode distribution in rabies virus preparations for multiplexed monosynaptic tracing.
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