HELPER PHAGE PREPARATION

1. Grow an overnight of NM522 in NZCYM medium.

2. Dilute overnight 1:100 and grow to an A600 = 0.3 (@2.5 x 108 cells/ml).

3. Infect cells with VCS helper phage to a m.o.i. = 0.1 (phage:bacteria = 1:10). There should be a high-titer stock of VCS in the lab.

e.g., 40ml NM522 (@1010 cells) + 10ml VCS (@109phage from a stock = 1011 phage/ml)

4. Incubate/shake @ 37oC for 8h.

5. Centrifuge 10', 15krpm to remove bacterial cells.

6. Harvest supernatant and add 0.4% chloroform.

7. Store in aliquots @ 4oC. It is a good idea to titer the prep (expect >109 phage/ml).
acc 12/90