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| Date | Member | Experiment | Result |
|---|---|---|---|
| 2022/3/19 | L.X.R. | (1) Transfer MP6 to S2060;
(2) Measure the concentrarion of phage. |
(1) No single colonies existed for the concentration of plasmids was a little bit high;
(2) Phage plaques were not obvious. |
| 2022/3/20 | C.Q.Y. | Assemble the PACE units; validate the operation of the units. | |
| 2022/3/23 | C.Q.Y. | Make 10 L of solution A and 1 L of solution B of DRM; autoclave the solution A; sterilize the solution B by using bacterial filter membranes and syringes; autoclave all instruments used to construct the PACE units. | |
| 2022/3/24 | C.Q.Y. | Autoclave and dispense 1 L of DRM liquid media. | |
| 2022/3/26 | C.Q.Y. | Pick the single colonies cultured by G.P.Z. and 8 gradient dilution cultures were performed in the DRM media with required antibiotics according to the protocol. | |
| 2022/3/27 | L.X.R. | (1) PCR: M13 backbone, artificial sytheic section T7RNAP; (2) Electrophoresis and gel extraction; (3) Transfer MP6 into S2060. |
The results of gel extraction were normal; the results of transformation were not ideal for the sizes of colonies were not the same. |
| C.Q.Y. | (1) Measure OD600 of gradient dilution bacterial solution by microplate reader. Take proper concentration of bacterial solution to the conical flask and culture it for 2.5 h and transfer it to chemostat;
(2) Make 10 L of DRM liquid media with antibiotics by using solution A and solution B. Construct the units. Run the chemostat in the light incubator at the first floor; (3) Dealing with a number of abnormal unit operations. | Time and results of OD600: 0.595(22:09), 0.284(23:09). | |
| 2022/3/28 | C.Q.Y. | Take a number of samples from the chemostat to measure the OD600; adjust the setting of the units | Time and results of OD600: 0.139(11:09), 0.195(16:00), 0.925(21:05). |
| 2022/3/29 | L.J.J. | Transfer MP into the bacteria. Paint the bacterial solution onto the plates and put them in the biological shaker at 220 rpm, 37℃ for 12 h. | No colonies grew on the plates til 9:00 p.m. |
| Z.Y.H., N.X.H., T.W.H. | PCR | Wrong section. | |
| L.X.R. | Transfer MP6 into S2060 (3 repetitions). | The bacterial colonies appeared after 24 h. Colony morphology was normal, but it was contaminated with other bacterial. | |
| C.Q.Y. | (1) Anomalous floating of tubes in a constant calorifier substrate bottle. Readjust the units;
(2) Set the input speed of chemostat at 1 unit volume per hour. Set the light incubator at 40℃; (3) Take samples from chemostat to measure the OD600. |
Time and results of OD600: 0.500(13:46), 0.636(14:39), 0.529(15:35), 0.680(16:47), 0.611(17:57); the constantiser is basically considered to be in stable operation. | |
| 2022/3/30 | Z.Y.H., L.J. | PCR | Wrong section. |
| L.X.R. | (1) Homologous recombination of the purified fragment in March, 27th. Operate the phage infection experiment;
(2) Take the S2060 bacterial solution into the tubes and put them in the biological shaker. It was prepared to estimate the mutation ratio of MP6; (3) Make the arabinose solution and glucose solution and were sent to be sterilised in a high temperature. |
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| 2022/3/31 | L.X.R. | (1) Dilute the bacterial solution 1000 times. Take the bacterial solution into basic media or 2xYT media respectively until the OD600 became 0.5~0.7. Divide the samples into two conical flasks and
take 25 mL of bacterial solution into every flask;
(2) 100 mM D-Glucose was added into one of the flasks. The same quantity of 100 mM L-Arabinose was added into another flask. Put them in the biological shaker at 37℃ for 24 h. |
Put the bacterial solution in the biological shaker for 7 h. |
| C.Q.Y. | Paint the plates with new SP made by G.P.Z.; operate the PCR for the phage; culture the bacteria in the biological shaker; electrophoresis. | The results did not match the theory. |
