Team:LCG-UNAM-Mexico/LauraJournal
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<br><span style="font-size:14px"> ''Burst size obtained with purification data.'' </span> | <br><span style="font-size:14px"> ''Burst size obtained with purification data.'' </span> | ||
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- | These results were used to obtain the “burst size” of T7 bacteriophages. I assumed a couple of things: all the phages are infecting a bacterium, all the cells were infected and almost all the bacteria died in the first round of infection. I calculated the bacteria number with the formula obtained from the growth curve which involves OD and UFC. So I calculated the burst size as the total number of phages produced divided by the total number of bacteria. The data from the first purification (1BS stock)indicate a burst size of 952 phages per bacterium. However the data from the 2BS stock indicate a burst size of 160,000 phages per bacterium and surprisingly the data from the 3BS stock indicate a bigger number. We | + | These results were used to obtain the “burst size” of T7 bacteriophages. I assumed a couple of things: all the phages are infecting a bacterium, all the cells were infected and almost all the bacteria died in the first round of infection. I calculated the bacteria number with the formula obtained from the growth curve which involves OD and UFC. So I calculated the burst size as the total number of phages produced divided by the total number of bacteria. The data from the first purification (1BS stock)indicate a burst size of 952 phages per bacterium. However the data from the 2BS stock indicate a burst size of 160,000 phages per bacterium and surprisingly the data from the 3BS stock indicate a bigger number. We know it is not possible because the phage production is limited by the amount of nucleotides available. For this reason, I designed other experiment to measure the burst size. From now I focused on T7 because I felt the time wasn't enough.<br> |
==October== | ==October== | ||
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<br> When I went over the plates I realized the results for the time 0 were inconsistent, however on time 5 plates I obtained 2 colonies for the 10^-3 T3 and T7 plates, 0 colonies for the 10^-5 T3 and T7 plates, for the control plates I almost got a bacteria monolayer in 10^-3 plate and non-countable bacteria in 10^-5. | <br> When I went over the plates I realized the results for the time 0 were inconsistent, however on time 5 plates I obtained 2 colonies for the 10^-3 T3 and T7 plates, 0 colonies for the 10^-5 T3 and T7 plates, for the control plates I almost got a bacteria monolayer in 10^-3 plate and non-countable bacteria in 10^-5. | ||
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+ | <br><span style="font-size:14px"> ''Second experiment to obtain the burst size.'' </span><br><br> | ||
+ | I did two replicates of this experiment. I did two 25ml cultures. When the culture had an OD around 0.8 (0.738 and 0.724, respectively)I put 100ul of some phage dilutions. I supposedly added seven and five phages, respectively. I waited for 20 minutes, it is supposed that the lysis lasts approximately 14 minutes. After this I follow the purification protocol adding 3ml of NaCl and 4ml of PEG 6000% in the right time. In the next step I did phage dilutions (10^-1, 10^-2 and 10^-3) and I followed the Titering Protocol. No one plaque was observed after three hours. I suppose the Purification Protocol was unsuccessful because the small amount of phages.<br> | ||
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+ | <br><span style="font-size:14px"> ''Third experiment to obtain the burst size.'' </span><br><br> | ||
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+ | I did two replicates of this experiment. I did a modified Titering Protocol. I took 500ul of cell with an OD of 0.8 and I added 100ul of phage dilution. The dilutios were made from the T7 original stock | ||
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Revision as of 01:43, 22 October 2009