Composite

Part:BBa_K1412614:Experience

Designed by: Ruihua Zhang   Group: iGEM14_XMU-China   (2014-10-01)
Revision as of 05:58, 11 October 2014 by D (Talk | contribs) (Characterization stage)

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Protocol

Genetic link stage

1.As a skeleton, TT terminator link with target gene CheZ.

2.Then link the skeleton to target gene CheZ-TT.

3.Next, link RBS-CheZ-TT with promoter Plac.

Verification

Verification.png

Characterization stage

1. Transfer pBAD-RBS-CheZ-TTBBa_K1412624 into competent cell of E.coli (ΔCheZ) respectively.

2. Coated plates(LB solid medium with the antibiotic concentration 50ug/ml chloromycetin) and culture in 37℃ biochemical incubator

for 12h.

3. Select colony to culture in 5ml LB fluid medium, of which the antibiotic concentration is 50ug/ml chloromycetin.

4. Activation of bacterium: transfer 50uL bacterium medium into a new 5ml LB fluid medium, of which the antibiotic concentration is

50ug/ml chloromycetin.

5. Stab of bacterium: We draw three dots on a plate before, then stab 3ul bacterium medium into the M63 semisolid medium at the dots.

And culture the bacteria in constant temperature and humidity incubator at 37℃. Protocol of M63.jpg

6. The initial colony radius is recorded as R1, and the radius are measured at 12h, 24h, 30h, 36h, 42h... as R2, R3, R4, R5, R6, R7…

The chemotaxis rate grows higher over time, larger radius bringing less error. Each radius minus R1 is the net chemotaxis radius at

certain time. Plot the net chemotaxis radius versus time and set the radius of pLac-RBS (1.0)-CheZ-TT as RBS strength 1.0. Then we

can calculate the RBS efficiency (ΔR2L/ΔR2M) and (R2J/ΔR2M) and compare them with the official data.

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