AAV DNA Bacterial Growth

protocol

- Retrieve the agar plate and check to see if a single colony can be identified. You want to get a single spot of growth that isn’t touching any others and is of average size for the plate so groups, smudges, very large, or very small spots of growth should be avoided

• If you do not see a single colony because there is too much growth on the plate we suggest redoing the streaking the following afternoon and using less of the transformation than the previous time (may be helpful to plate multiple amounts to increase the chance of one working)

• If you do not see anything on the plate at all you can leave the plate at 37degC until the afternoon but be aware this introduces more risk to the plasmid. If there is still no colonies and you are confident that your transformation was done correctly then redo the transformation and lower the ampicillin concentration in the agar plate by half (this is rarely necessary but it may be worth trying).

- Prepare a 14mL round bottom tube with 3-5mL of LB broth and ampicillin at a 1:1000 ratio (3mL LB would need 3uL ampicillin)

- Now take a sterile toothpick or pipet tip and lightly scrape the tip over the colony. You don’t need to dig into the gel just roll it over, even if you can’t see bacteria on the tip there should be some picked up.

- Drop your tip into the LB/ampicillin and let that incubate all day (~8hrs) at 37℃ and 225rpm. Be sure that the tubes are secured into the incubator before shaking as it will create more movement of the broth and increase growth.

- Prepare a conical flask with LB and ampicillin at the same concentration as the starter growth (1:1000). The amount of LB/AMP that you use will depend on the size of growth you want to do. For a 250-300mL growth (a typical midi prep) we would use a 1L conical flask.

• Try to not to put too much LB in one flask as it will lower the amount of movement inside the flask and lower the growth efficiency.

- At the end of the 8 hour 3-5mL starter growth incubation, use the entire starter growth to inoculate the large 250mL growth and secure into a shaking incubator overnight (16 hours) at 37℃ and 225rpm.

- After the overnight large growth we take the OD600 of the large growth and then aliquot 1.5mL of the growth to mini prep with a ZymoPURE plasmid mini prep kit (VWR, 77001-480) before pelleting the large growth and holding the bacterial pellet at -20℃ until the quality control (QC) can be completed. 

- We use the purified DNA from the mini preps to QC the plasmids using full length sequencing at Plasmidsaurus. 

• Plasmidsaurus provides full length sequencing allowing us to check the structure of our plasmids and purity of DNA preps. Please check our AAV DNA QC guide for more information on how we judge our Plasmidsaurus results

- Once our plasmid sequences are verified, we purify the DNA using the Macherey Nagel NucleoBond Xtra Midi kit for transfection-grade plasmid DNA (Macherey Nagel, 740410.50). 

• We follow the kit instructions closely, however it is important to remember that the amount of each purification buffer you use in the kit should be adjusted to the amount of bacteria in the prep as measured in the OD600.