Team:PKU Beijing/Notebook/AND Gate 1/Core/Min Lin

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2009.8.1

Transformation:
J23100-tetR-tetP and LuxR-LuxP-SupD

PCR assessment for the J23100-tetR- tetP and LuxR-LuxP-SupD
Overnight

2009.8.2

PCR product->GEL

Number2-6 J23100-tetR-tetP is correct.
Number1 of LuxR-LuxP-SupD is correct.

Digestion of the J23100-tetR-tetP
With EcoRI and SpeI overnight

2009.8.3

01:30
Help Zhangguosheng pick colonies and PCR

10:00
GEL

Enzyme Digest of the J23100-tetR-tetP with EcoRI and SpeI

GEL Purification.
Ligation:
J23100-tetR-tetP ES insert
E0840 EX vector and SupD-terminator EX vector

18:30
Transformation.

2009.8.4

PCR assessment

Shake the BL21 strain transformed with T7promoter-GFP by WangHao
Induce with IPTG.
The induced one has fluorescence

2009.8.5

Pick standard part I0500
Phusion PCR

GEL purification and then cut with EcoRI and SpeI.
Purify from digestion.

2009.8.6

Ligation of I0500(ES) to SupD-terminator and E0840 vector.

Transformation

In order to get a Kan resistant back bone, I transformed the pSB1K3 part from plate1-7A.

2009.8.7

Shake the 1-7A in the incubator.
PCR assessment of the I0500-GFP clone.

But it is no need to care about which is right, cause Gaorencheng has worked out a AraC and PBad promoter that works well.

2009.8.8

Miniprep the 1-7A plasmid.
Digest with EcoRI and PstI

GEL purification.
Store the backbone.

Ligation
T7promoter-GFP EP insert
pSB1K3 EP backbone

Transformation

2009.8.9

Pick colonies to do PCR assessment of the T7promoterpSB1K3

The 3 colonies are correct ones.

Induction of the LuxR-LuxP-GFP
A gradient of concentration:
5uM, 2uM, 100nM, 10nM, 1nM, 0
Use flocytometry to detect the fluorescence.

It shows a ten fold induction.
However the basal is very high.