Revision as of 09:25, 1 July 2013

26 June 2013

208 lab

Main purposes today

helloworld-project

25 rxns including duplicates

34 rxna including duplicates with the following setup:

Tube 1-6 containing 5uL pZA21 plasmid template and 3uL of each primers for amplification of the backbone. Tube 7-10; 1uL g-Block from previous purification and 3uL of each Sec signal primers. Tube 11-14 containing same amount of g-Block and primers but now replaced with the TAT2 signal primers. Tube 15-18; 5uL GFP SF plasmid template and 3uL of each primers for GFP SF TAT. Tube 19-22; 5uL GFP SF plasmid template and 3uL of each primers for GFP SF Sec. Tube 23-26; 5uL RFP plasmid template and 3uL of each primer for RFP. Tube 27-30; 1uL g-Block purification and 3uL of each TAT3 primers. Tube 31-34; 0.5uL of the original g-Block and 3uL of each primers for amplifying the g-Block. All tube with less than 5uL template DNA was filled with MQ until final volume of 11uL(5+3+3).

First half of the samples where run on PCR with x7-polymerase and the second half where run with PHUSION-polymerase, with the exception of the g-Block where all reactions where run with PHUSION. This gives following setup: x7-poly in tube:

1-3, 7-8, 11-12, 15-16, 19-20, 23-24, 27-28

PHUSION in tube:

4-6, 9-10, 13-14, 17-18, 21-22, 25-26, 29-30, 31-34

A mastermix was made for both PCR with standard concentration setup and one additional volume for pipetting errors:

x7 mastermix for 16rxn

160uL HF buffer
16uL dNTP's 10mM
8uL x7 polymerase
440uL MQ

PHUSION mastermix for 20rxn

200uL HF buffer
20uL dNTP's 10mM
10uL x7 polymerase
5500uL MQ

The tubes were run on two programs simultaneously both where ramps. First program with the ramp going from 70°C → 60°C and another from 60°C → 50°C. The tubes in first program(70°C → 60°C) where tube 7-10, 15-26 and for second program(60°C → 50°C) tube 1-6, 11-14, 27-34.

Who was in the lab

Henrike, Jakob, Kristian, Gosia

Procedure

PCR for 7 fragments:

Conclusion from today

Inconsistent results from the first PCR where obtained with bands in some of the reactions but not in the duplicates. Even the g-Block was not seen though we have easily amplified that before with very bright bands. Something must have gone wrong and that's why we made the additional 34rxns which will be analyzed on gels tomorrow.

@@ Line 1: / Line 1: @@
+{{:Team:DTU-Denmark/Templates/StartPage|26 June 2013}}
+__TOC__
 =208 lab=
+<hr/>
 == Main purposes today ==
+<hr/>
 helloworld-project
 *25 rxns including duplicates
 *34 rxna including duplicates with the following setup:
@@ Line 16: / Line 20: @@
 A mastermix was made for both PCR with standard concentration [https://2013.igem.org/Team:DTU-Denmark/Methods/PCR-mix setup] and one additional volume for pipetting errors:
-=====x7 mastermix for 16rxn=====
+====x7 mastermix for 16rxn====
+<hr/>
 *160uL HF buffer
 *16uL dNTP's 10mM
@@ Line 22: / Line 27: @@
 *440uL MQ
-=====PHUSION mastermix for 20rxn=====
+====PHUSION mastermix for 20rxn====
+<hr/>
 *200uL HF buffer
 *20uL dNTP's 10mM
@@ Line 32: / Line 38: @@
 ==Who was in the lab==
+<hr/>
 Henrike, Jakob, Kristian, Gosia
 ==Procedure==
+<hr/>
 [[Team:DTU-Denmark/Methods/PCR|PCR]] for 7 fragments:
 == Conclusion from today ==
+<hr/>
 Inconsistent results from the first PCR where obtained with bands in some of the reactions but not in the duplicates. Even the g-Block was not seen though we have easily amplified that before with very bright bands. Something must have gone wrong and that's why we made the additional 34rxns which will be analyzed on gels tomorrow.
+{{:Team:DTU-Denmark/Templates/EndPage}}

Team:DTU-Denmark/Notebook/26 June 2013

From 2013.igem.org