Revision as of 14:02, 13 August 2013

12 August 2013

lab 208

Main purpose

Screening PCR on pZA21:RFP araBAD
PCR reaction in order to amplify backbone pZA21 containing araBAD and RFP
PCR reaction in order to amplify Nir1 and Nir2 fragments

Who was in the lab

Henrike, Kristian, Gosia, Julia

Procedure

Screening PCR on pZA21:araBAD:RFP spl

8 different conditions and 12 different annealing temperatures were screened.

PCR mix according to standard protocol with different amounts of water according to the amounts of DMSO and MgCl2 added to the reactions.

The conditions are: Row A -> 1% DMSO + 0.04mM MgCl2 + GC buffer Row B -> 3% DMSO + 0.04mM MgCl2 + GC buffer Row C -> 5% DMSO + 0.04mM MgCl2 + GC buffer Row D -> 5% DMSO + 0.5mM MgCl2 + GC buffer Row E -> 5% DMSO + 2mM MgCl2 + HF buffer Row F -> 3% DMSO + 1mM MgCl2 50mM + HF buffer Row G -> 5% DMSO + 1mM MgCl2 50mM + HF buffer Row H -> 5% DMSO + 0.04mM MgCl2 + HF buffer

Primers - 51a and 51b1
Template - "Ara" sample (plasmid isolation pZA21:araBAD:RFP).
Annealing temperature: each condition were run in the following 12 different annealing temperatures:

53.2 C
53.5 C
54.6 C
56 C
57.2 C
58.4 C
59.6 C
60.6 C
61.9 C
63.2 C
64.6 C
65 C

PCR mix for backbone

PCR mix - according to standard protocol.
Primers - 1an and 1b
Template - "Ara" sample (plasmid isolation pZA21:araBAD:RFP).
Program was based on standard program with 65 C of annealing temperature and 4 min of extension time.
Samples names: 1, 2, 3 and N (negative)

PCR for Nir1 and Nir2

PCR mix according to standar protocol with changes: addition of DMSO in 3 different final concentrations (2%, 3%, 5%); two different buffers (HF 5x and GC 5x), amount of added water was dependent on volume of added DMSO.
Primers for Nir1 - 39a, 39b
Primers for Nir2 - 40a, 40b
Templates - fragments Nir1 and Nir2 amplified with non-uracil primers, gel purified
Polymerase x7
Program (A99 - the same for Nir1 and Nir2) was based on standard PCR program with 50 C and 1 min of annealing parameters and 5 min of extension time.
Samples names:

Nir1, GC buffer, 2% DMSO
Nir1, GC buffer, 3% DMSO
Nir1, GC buffer, 5% DMSO
Nir1, HF buffer, 2% DMSO
Nir1, HF buffer, 3% DMSO
Nir1, HF buffer, 5% DMSO
Nir2, GC buffer, 2% DMSO
Nir2, GC buffer, 3% DMSO
Nir2, GC buffer, 5% DMSO
Nir2, HF buffer, 2% DMSO
Nir2, HF buffer, 3% DMSO
Nir2, HF buffer, 5% DMSO

Results

Conclusion

Navigate to the Previous or the Next Entry

@@ Line 19: / Line 19: @@
 * PCR mix according to [[Team:DTU-Denmark/Methods/PCR-mix| standard protocol]] with different amounts of water according to the amounts of DMSO and MgCl2 added to the reactions.
 The conditions are:
-# 1% DMSO + 40uM MgCl2 + GC buffer
+Row A -> 1% DMSO + 0.04mM MgCl2 + GC buffer
-# 3% DMSO + 1uL MgCl2 2mM + GC buffer
+Row B -> 3% DMSO + 0.04mM MgCl2 + GC buffer
-# 5% DMSO + 1uL MgCl2 2mM + GC buffer
+Row C -> 5% DMSO + 0.04mM MgCl2 + GC buffer
-# 5% DMSO + 0.5uL MgCl2 50mM + GC buffer
+Row D -> 5% DMSO + 0.5mM MgCl2 + GC buffer
-# 5% DMSO + 2uL MgCl2 50mM + HF buffer
+Row E -> 5% DMSO + 2mM MgCl2 + HF buffer
-# 3% DMSO + 1uL MgCl2 50mM + HF buffer
+Row F -> 3% DMSO + 1mM MgCl2 50mM + HF buffer
-# 5% DMSO + 1uL MgCl2 50mM + HF buffer
+Row G -> 5% DMSO + 1mM MgCl2 50mM + HF buffer
-# 5% DMSO + 1uL MgCl2 2mM + HF buffer
+Row H -> 5% DMSO + 0.04mM MgCl2 + HF buffer
 * Primers - 51a and 51b1
 * Template - "Ara" sample (plasmid isolation pZA21:araBAD:RFP).
-* Annealing temperature: each condition were run in 12 different annealing temperatures with constant interval within the range 51 C-65 C.
+* Annealing temperature: each condition were run in the following 12 different annealing temperatures:
+# 53.2 C
+# 53.5 C
+# 54.6 C
+# 56 C
+# 57.2 C
+# 58.4 C
+# 59.6 C
+# 60.6 C
+# 61.9 C
+# 63.2 C
+# 64.6 C
+# 65 C
 === PCR mix for backbone===

Team:DTU-Denmark/Notebook/12 August 2013

From 2013.igem.org