PhiX:DsDNA isolation

Developed after Godson and Vapnek, 1973.

Step One: phage amplification

prepare ~20ml of high titre phage (I have tried this from chemostat where pfu = 10⁹/ml)

prepare 100ml LB + 200ul 1M CaCl₂ in a 250ml conical flask (~ 2mM CaCl₂)
add 2ml overnight C122 culture to each
shake at 37^oC and follow until 0.3 < OD_600nm < 0.4 (~1.5 hours)
add ~20ml phage - start timer
return to shaker for 9 minutes (within the time of a single burst)
remove from shaker and quickly add 88.2ul 34mg/ml chloramphenicol (~ 30ug/ml)
shake for 3 hours at 37^oC
aliquot culture into four 50ml centrifuge tubes
centrifuge @ 5000g for 20 minutes (4^oC to avoid overheating)
discard supernatent and leave tubes upside down on tissues
replace caps and store two tubes upside down at -20^oC as backup
miniprep remaining two using Qiagen miniprep kit (treat each as product of 2ml culture)
gel run and extract to isolate RFI DNA from chromosomal/RNA contamination