Team:Caltech/Protocols/Titering
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#To begin infection, add appropriate amount of diluted phage to cell solution (10 ul usually works well for starters) and start the timer | #To begin infection, add appropriate amount of diluted phage to cell solution (10 ul usually works well for starters) and start the timer | ||
#During this 30 minute infection period, label the plates and place back in the 42 C oven | #During this 30 minute infection period, label the plates and place back in the 42 C oven | ||
- | #~3 minutes before the end of infection, can take 3 mL aliquots of the top medium in 13 mL falcon tubes or 5 mL round-bottom tubes and microwave till complete liquification has occurred. | + | #~3 minutes before the end of infection, can take 3 mL aliquots of the top medium in 13 mL falcon tubes or 5 mL round-bottom tubes and microwave till complete liquification has occurred. |
+ | #*Note that top agar is the same composition as is used to pour the plates, only with half the agar (so ~7g/L agar rather than 15 g/L). | ||
#Right before the end of infection, take out the plates and place on the bench with the cover on top. Have a flame close-by to prevent contamination. Also, set the pippette to the right volume of infected cell solution and have sterile pipette non-filter tips ready | #Right before the end of infection, take out the plates and place on the bench with the cover on top. Have a flame close-by to prevent contamination. Also, set the pippette to the right volume of infected cell solution and have sterile pipette non-filter tips ready | ||
#Very quickly with pipette in hand, pippette out infected cell solution, add to top medium, invert the tube at least 2 times, and pour the mixed contents onto the corresponding plate. | #Very quickly with pipette in hand, pippette out infected cell solution, add to top medium, invert the tube at least 2 times, and pour the mixed contents onto the corresponding plate. |
Latest revision as of 01:05, 30 October 2008
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Titering Bacteriophage
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