Paris/July 27

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Revision as of 17:48, 27 July 2007

PCR to perform

The following PCR reactions have been performed

P5
P6
P8
P9

Oligo design for Wanner deletion

We were for now on not able to perform the deletion of DapA through transduction. So we will try the deletion through the Wanner method. We will also attempt the deletion of FtsZ.

We will use the protocol of the keio collection: [http://ecoli.naist.jp/gb6/Resources/deletion/Del_construct.html]

20nt of upstream region of kan gene,

5'-ATTCCGGGGATCCGTCGACC-3' (P1)

20nt of kan downstream sequence,

5'-TGTAGGCTGGAGCTGCTTCG-3' (P2)

DapA deletion

50nt DapA upstream region

5'-CATACCAAACGTACCATTGAGACACTTGTTTGCACAGAGGATGGCCCATG-3' (P3)

50nt DapA downstream region (reverse complement)

5'-AAGCCATCAAATCTCCCTAAACTTTACAGCAAACCGGCATGCTTAAGCGC-3' (P4)

dDapA-F

CATACCAAACGTACCATTGAGACACTTGTTTGCACAGAGGATGGCCCATGATTCCGGGGATCCGTCGACC (P3 + P1)

dDapA-R

AAGCCATCAAATCTCCCTAAACTTTACAGCAAACCGGCATGCTTAAGCGCTGTAGGCTGGAGCTGCTTCG (P6 + P2)

FtsZ deletion

50nt FtsZ upstream region

5'-GACGATGATTACGGCCTCAGGCGACAGGCACAAATCGGAGAGAAACTATG-3' (P5)

50nt FtsZ downstream region (reverse complement)

5'-GAAACCCAAATTCCAGTCAATTCTTAATCAGCTTGCTTACGCAGGAATGC-3' (P6)

dFtsZ-F

GACGATGATTACGGCCTCAGGCGACAGGCACAAATCGGAGAGAAACTATGATTCCGGGGATCCGTCGACC (P5 + P1)

dFtsZ-R

GAAACCCAAATTCCAGTCAATTCTTAATCAGCTTGCTTACGCAGGAATGCTGTAGGCTGGAGCTGCTTCG (P6 + P2)

Ligations

Ligations
Number	Insert	Insert Volume (µL)	Vector	Vector Volume (µL)	Comments
Control 1			MP3.1 digested with EcoRI		control of ligation efficiency
Control 2			MP3.1 digested with EcoRI		without ligase in the mix: control of digestion efficiency
Control 3			D9.1 (J61002 ready for insertion of a FI)	2µl	control of D9.2 digestion
Control 3			D15.1 (B0030 BV)	2µl	control of D15.2 digestion
Control 3			D22.2 (pSB1A2 Eco, Pst)	2µl	control of D22.1 digestion
L1	D23.2 (AraC/pBad promoter FI)	8	D9.1 (J61002 ready for insertion of a FI)	2	construct with pBad promotor regulating expression of mRFP (in order to test activity of pBad)
L6	D14.2(Cre ORF)	8	D15.1 (B0030 BV)	2	construction of the biobrick strong RBS(B0030)-Cre ORF
L9	lox66 [O14+O15] (0.2µM)	2	D22.2 (pSB1A2 Eco, Pst)	2 (+6 H2O)	lox66 cloned as a biobrick in pSB1A2
L10	lox71 [O16+O17] (0.2µM)	2	D22.2 (pSB1A2 Eco, Pst)	2 (+6 H2O)	lox71 cloned as a biobrick

Ligation mix:

2µl TP
1µl Ligase
7µl H20

Reaction in 20µl

ON @ 4°C

Minipreps

minipreps were performed on the following ON cultures:

cultures of different clones of the ligation reactions of 25/07/07

L1.2 & L1.3
L2.1 & L2.2
L9
L10
L6.1, L6.2 & L6.3

for more detail on these ligation reactions, go to 25/07/07

no glycerol stocks of hese strains have been generated yet (the culyures are launched tonight in order to do this)

minipreps & glycerol stocks:

MP12.1 & MP12.2 (2 clones after transformation with biobrick BBa_P1003)

@@ Line 75: / Line 75: @@
 |
 |
-|D9.2 (J61002 ready for insertion of a FI)
+|D9.1 (J61002 ready for insertion of a FI)
 |2µl
 |control of D9.2 digestion
@@ Line 82: / Line 82: @@
 |
 |
-|D15.2 (B0030 BV)
+|D15.1 (B0030 BV)
 |2µl
 |control of D15.2 digestion
@@ Line 89: / Line 89: @@
 |
 |
-|D22.1 (pSB1A2 Eco, Pst)
+|D22.2 (pSB1A2 Eco, Pst)
 |2µl
 |control of D22.1 digestion
 |- style="background: #cccccc;"
 | style="background: #ccffcc;" |L1
-|D23.1 (AraC/pBad promoter FI)
+|D23.2 (AraC/pBad promoter FI)
 |8
 |D9.1 (J61002 ready for insertion of a FI)
@@ Line 101: / Line 101: @@
 |- style="background: #cccccc;"
 | style="background: #ccffcc;" |L6
-|D14.1 (Cre ORF)
+|D14.2(Cre ORF)
 |8
 |D15.1 (B0030 BV)
@@ Line 110: / Line 110: @@
 |lox66 [O14+O15] (0.2µM)
 |2
-|D22.1 (pSB1A2 Eco, Pst)
+|D22.2 (pSB1A2 Eco, Pst)
 |2 (+6 H2O)
 |lox66 cloned as a biobrick in pSB1A2
@@ Line 117: / Line 117: @@
 |lox71 [O16+O17] (0.2µM)
 |2
-|D22.1 (pSB1A2 Eco, Pst)
+|D22.2 (pSB1A2 Eco, Pst)
 |2 (+6 H2O)
 |lox71 cloned as a biobrick

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