What is the best practice in propagating ITR-containing AAV transfer vector ?

30 January 2020 0 7K Report

I heard a lot of examples of troublesome ITR deletions in AAV vector propagation in bacteria. In general, people recommend using lower temperature (30oC) for culturing the bacteria or use some recombinase depleted bacterial strain to maximize the chance of getting intact plasmids. Yet screening of clones or cultures are still necessary in many cases. Does anyone have a better way to control this?

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