EPF-Lausanne/25 August 2009

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Revision as of 08:44, 4 September 2009

Wet Lab

Miniprep:

Made according to the protocol of Aisgen Miniprep Kit Elution in 50 ul. The RD2 #5 plasmids prep as some that have already been prepared will be sent for sequencing this afternoon.

Mediums

New medium were made to grow the double-transformed DH5 a (LovTap BB and RO2) -> should be without thy.

M9 was redone, pH adjusted with amino acid and filtred. for 1L:

5g glucose

6g Na2PO4

3g KH2PO4

1g NH4Cl

0.5g NaCl

0.12g MgSO4

0.01g CaCl2

Trp Operon synthesis

Using the Klenow fragments protocol and primers:

Trp operon Rev

Trp operon Fwd

**Trp Operon synthesis**
	2x Trp	1x Negative Control
NEB 2 (10x)	2ul each	2ul
dNTP	1ul each	1ul each
template primers	1ul (RV) + 1.5ul (FW) each	-
Klenow enzyme	1 ul each	1 ul
dH2O	18.5 ul each	21ul
total	25 ul each	25 ul

The primers volumes were directly taken from the original primer dilution (iGEM 09 primers box)

1. Running Klenow 1 file on thermal cycler to denature and slowlyy anneal primers (self-annealing) 2. Running Klenow file after adding the Klenow enzyme (for extension)

DNA preparation

For sending to sequencing

sample name	init concentration [ng/ul]	final volume [ul]	final concentration [ng/ul]	sample [ul]	H20
BB1	180.5	50	25	6.94	43.06
BB3	215.5	50	25	5.8	44.2
BB5	350.5	50	25	3.57	46.43
BB6	142.5	50	25	8.77	41.23
RD2 #5	81.5	50	25	15.34	34.66
LTT=LT5	326	50	25	3.83	46.17
LR2	92	50	25	13.59	36.41
LR5	47.5	50	25	26.32	23.68
LR7	113.5	50	25	11	39
RD2 #8	247	50	25	5.06	46.94
RD2 #4	226	50	25	5.53	46.47
RD2 #10	200	50	25	6.25	43.75
LT2	141	50	25	8.87	41.13
LT6	152	50	25	8.22	41.78
LT12	142	50	25	8.8	41.2

Double transformation

We made a double transformation of RO2#4/BB1, RO2#5/BB3, RO2#8/BB5 and RO2#10/BB6.

People in the lab

Basile, Rafael, Nicolas

@@ Line 320: / Line 320: @@
 ===Double transformation===
-,,,
+We made a double transformation of RO2#4/BB1, RO2#5/BB3, RO2#8/BB5 and RO2#10/BB6.
 ==People in the lab==