Part:BBa_K4630114:Experience
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how you used this part and how it worked out.
Applications of BBa_K4630114
This part is the more integrated form that contains three cassettes. Using this part, we can verify the concept of multi-level recording and gain comprehensive data.
General Induction Protocol
- Pick a colony from the verified plate, cultivate in 5ml liquid LB media for 12 hours.
- Transfer 100µl bacteria solution to 3ml new liquid LB media. Cultivate to an OD600 of 0.3~0.5.
- Add L-Arabinose and IPTG to final concentrations of 2g/L and 3g/L, and induce for 22 hours and 5 hours, respectively.
- Spread the diluted solution to plates with appropriate antibiotics and cultivate for 12 hours.
- Pick the colonies and test the editing result.
Result
Proof-of-Concept
We implement induction over the part, and it is successfully knock-out.
Fig 1 The successful knock-out of the stgRNA-cassette (1+2+3)
Time-Gradient Test
Also, according to our PI's advice, IPTG induction do harm to the cells. However, refractory phase is a key parameter of the multi-level recorder. So, we performed time-gradient tests over the part (tbl 1).
All of the samples achieve full knock-out, at a rate of 100% (fig 2). However, the time-gradient within 2 hours did not really set up, because of inconsistency with the time-gradient tes in BBa_K4630100. Not surprisingly, the test carried out on stgRNA-cassette (1+2+3) showed some kind of leakage expression. More experiments of different promoters should be taken.
Table 1 Time-gradient test
Fig 2 Time-gradient test over the part
User Reviews
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