Revision as of 01:30, 27 September 2012

Labbook - TAL vector

08/08/12

1.) MutPCR for pSB1C3 vector backbone in order to remove restriction sites vor BsmBI
2.) Transformation of Sirt2 and HAT5
3.) GGC in order to produce our MammoBrick

1.) MutPCR:

	Tube 1 [µl]	Tube 2 [µl]
Primer MutPCR fo [10 mM]	1	0,25
Primer MutPCR re [10 mM]	1	0,25
dNTPs [10 mM]	1	1
Phusion Buffer HF	1,25	1,25
Phusion Polymerase	0,25	0,25
DMSO	1	1
MgCl2	1	1
Template	1	1
ddH2O	5	6,5

Program for Thermocycler (20 cycles)
1. 95°C 5min
2. 95°C 50s
3. 80°C 50s
4. 72°C 3min
5. 72°C 7min
6. 4°C //

2.) Transformation of Sirt2 and HAT5 in DH10B starin of E. coli using our standard protocol for transformation. Kanamycin resistance was used

3.) GGC in order to produce our Mammobrick:

Contens	[µl]
BsaI [10 U/µl]	1,5
NEB Buffer 4	1
ATP [10 mM]	1
BSA	1
TALEN fragment [40 ng]	2
exCMV promotor [20 ng]	0,5
PostORF [20 ng]	1,25
PuroORF [20 ng]	0,5
T7 Ligase	0,25
DTT [10 mM]	1
ddH2O	1

Program for Thermocycler (15 cycles)
1. 37°C 5min
2. 20°C 5min

08/09/12

1.) Gel-Run of MutPCR:

Gel-run without success (no plasmid containing) MutPCR needs to be repeated!!!

2.) Gel-Run of GGC for MammoBrick:

Gel-run without success!!! GGC needs to be repeated!!!

08/10/12

1.) Repeating GGC in order to produce our MammoBrick:

Contens	[µl]
BsaI [10 U/µl]	1,5
NEB Buffer 4	1
ATP [10 mM]	1
BSA	1
TALEN fragment [40 ng]	2
exCMV promotor [20 ng]	0,5
PostORF [20 ng]	1,25
PuroORF [20 ng]	0,5
T7 Ligase	0,25
DTT [10 mM]	1
ddH2O	1

One reaction was done with DTT as described above and one reaction was done without any DTT and was simply replaced with ddH2O
Thermocycler Program: as described on 08/08/12, but with 20 cycles instead of 15, afterwards heatkill with 80°C for 20min.

08/11/12

1.) Transformation of MammoBrick vector produced on day before
2.) Transformation of SUV
3.) Repeating MutPCR on pSB1C3 vector backbone

1.) and 2.)
Transformations were done using our standard protocol. DH10B strain of E.coli was used

3.) MutPCR of pSB1C3 vector backbone:
This time the following conditions were used. In comparison to the MutPCR done on 08/08/12 this time no MgCl2 and DMSO was used.

for 20µl	x1 [ul]
Primer MutPCR fow [10 mM]	1
Primer MutPCR rev [10 mM]	1
Phusion Buffer HF	4
Phusion	0,4
Template	0,2
ddH2O	12,3

Program for Thermocycler (15 cycles)
1. 98°C 30s
2. 98°C 10s
2. 65°C-80°C 15s
2. 72°C 45s
2. 72°C 7min
2. 4°C //

Thermocycler Program: a gradient was used between 65°C and 80°C as annealing temperature. This time we used 30 cycles.

@@ Line 8: / Line 8: @@
 <br>
 ==08/08/12==
+----
 .) MutPCR for pSB1C3 vector backbone in order to remove restriction sites vor BsmBI<br>
@@ Line 14: / Line 15: @@
 .) MutPCR:
+<html>
-<table border="0" style="background-color:transparent">
+<table border="0" align="left" style="background-color:transparent">
 <tr>
 <th></th><th>Tube 1 [µl]</th><th>Tube 2 [µl]</th>
@@ Line 38: / Line 39: @@
 </tr></table>
-<br>
-Program for Thermocycler (20 cycles)
-<table border="0" width="20%" style="background-color:transparent">
+<table border="0" width="20%" align="right" style="background-color:transparent; margin-right:180px">
 <tr>
-<td>1.</td><td>95°C</td><td>5min</td>
+<th>Program for Thermocycler (20 cycles)</th>
 </tr><tr>
-<td>2.</td><td>95°C</td><td>50s</td>
+<td>1. &nbsp;&nbsp;&nbsp;&nbsp; 95°C&nbsp;&nbsp;&nbsp;&nbsp;5min</td>
 </tr><tr>
-<td>3.</td><td>80°C</td><td>50s</td>
+<td>2. &nbsp;&nbsp;&nbsp;&nbsp; 95°C&nbsp;&nbsp;&nbsp;&nbsp;50s</td>
 </tr><tr>
-<td>4.</td><td>72°C</td><td>3min</td>
+<td>3. &nbsp;&nbsp;&nbsp;&nbsp; 80°C &nbsp;&nbsp;&nbsp;&nbsp;50s</td>
 </tr><tr>
-<td>5.</td><td>72°C</td><td>7min</td>
+<td>4. &nbsp;&nbsp;&nbsp;&nbsp; 72°C &nbsp;&nbsp;&nbsp;&nbsp;3min</td>
 </tr><tr>
-<td>6.</td><td>4°C</td><td>//</td>
+<td>5. &nbsp;&nbsp;&nbsp;&nbsp; 72°C &nbsp;&nbsp;&nbsp;&nbsp;7min</td>
-</tr></table><br><br>
+</tr><tr>
+<td>6. &nbsp;&nbsp;&nbsp;&nbsp; 4°C &nbsp;&nbsp;&nbsp;&nbsp; //</td>
+</tr></table><br><br><br><br><br><br><br><br><br><br><br><br><br><br>
 .) Transformation of Sirt2 and HAT5 in DH10B starin of E. coli using our standard protocol for transformation. Kanamycin resistance was used<br><br>
 .) GGC in order to produce our Mammobrick:<br><br>
-Program for Thermocycler (20 cycles)
 <table border="0" width="40%" style="background-color:transparent">
@@ Line 68: / Line 67: @@
 <td>BsaI [10 U/µl]</td><td>1,5</td>
 </tr><tr>
-<td>NEB Buffer 4</td><td>95°C</td><td>50s</td>
+<td>NEB Buffer 4</td><td>1</td>
 </tr><tr>
 <td>ATP [10 mM]</td><td>1</td>
@@ Line 96: / Line 95: @@
 </tr><tr>
 <td>2.	&nbsp;&nbsp;&nbsp;&nbsp; 20°C	&nbsp;&nbsp;&nbsp;&nbsp; 5min</td>
+</tr></table><br><br></html>
+== 08/09/12 ==
+----
+<html><br>
+.) Gel-Run of MutPCR:<br><br>
+Gel-run without success (no plasmid containing)
+MutPCR needs to be repeated!!!<br><br>
+.) Gel-Run of GGC for MammoBrick:<br><br>
+Gel-run without success!!! GGC needs to be repeated!!!<br>
+<br></html>
+==08/10/12==
+----
+<html><br>
+.) Repeating GGC in order to produce our MammoBrick:<br>
+<table border="0" width="40%" style="background-color:transparent">
+<tr>
+<th>Contens</th><th>[µl]</th>
+</tr><tr>
+<td>BsaI [10 U/µl]</td><td>1,5</td>
+</tr><tr>
+<td>NEB Buffer 4</td><td>1</td>
+</tr><tr>
+<td>ATP [10 mM]</td><td>1</td>
+</tr><tr>
+<td>BSA</td><td>1</td>
+</tr><tr>
+<td>TALEN fragment [40 ng]</td><td>2</td>
+</tr><tr>
+<td>exCMV promotor [20 ng]</td><td>0,5</td>
+</tr><tr>
+<td>PostORF [20 ng]</td><td>1,25</td>
+</tr><tr>
+<td>PuroORF [20 ng]</td><td>0,5</td>
+</tr><tr>
+<td>T7 Ligase</td><td>0,25</td>
+</tr><tr>
+<td>DTT [10 mM]</td><td>1</td>
+</tr><tr>
+<td>ddH2O</td><td>1</td>
+</tr></table><br><br>
+One reaction was done with DTT as described above and one reaction was done without any DTT and was simply replaced with ddH2O<br>
+Thermocycler Program: as described on 08/08/12, but with 20 cycles instead of 15, afterwards heatkill with 80°C for 20min.<br><br></html>
+==08/11/12==
+----
+<html><br>
+.) Transformation of MammoBrick vector produced on day before<br>
+.) Transformation of SUV<br>
+.) Repeating MutPCR on pSB1C3 vector backbone<br><br>
+.) and 2.) <br>
+Transformations were done using our standard protocol. DH10B strain of E.coli was used<br><br>
+.) MutPCR of pSB1C3 vector backbone:<br>
+This time the following conditions were used. In comparison to the MutPCR done on 08/08/12 this time no MgCl2 and DMSO was used.<br><br>
+<table border="0" width="40%" align="left" style="background-color:transparent">
+<tr>
+<th>for 20µl</th><th>x1 [ul]</th>
+</tr><tr>
+<td>Primer MutPCR fow [10 mM]</td><td>1</td>
+</tr><tr>
+<td>Primer MutPCR rev [10 mM]</td><td>1</td>
+</tr><tr>
+<td>Phusion Buffer HF</td><td>4</td>
+</tr><tr>
+<td>Phusion</td><td>0,4</td>
+</tr><tr>
+<td>Template</td><td>0,2</td>
+</tr><tr>
+<td>ddH2O</td><td>12,3</td>
 </tr></table>
+<table border="0" width="40%" align="right" style="background-color:transparent;">
+<tr>
+<th>Program for Thermocycler (15 cycles)</th>
+</tr><tr>
+<td>1.	&nbsp;&nbsp;&nbsp;&nbsp; 98°C	&nbsp;&nbsp;&nbsp;&nbsp; 30s</td>
+</tr><tr>
+<td>2.	&nbsp;&nbsp;&nbsp;&nbsp; 98°C	&nbsp;&nbsp;&nbsp;&nbsp; 10s</td>
+</tr><tr>
+<td>2.	&nbsp;&nbsp;&nbsp;&nbsp; 65°C-80°C	&nbsp;&nbsp;&nbsp;&nbsp; 15s</td>
+</tr><tr>
+<td>2.	&nbsp;&nbsp;&nbsp;&nbsp; 72°C	&nbsp;&nbsp;&nbsp;&nbsp; 45s</td>
+</tr><tr>
+<td>2.	&nbsp;&nbsp;&nbsp;&nbsp; 72°C	&nbsp;&nbsp;&nbsp;&nbsp; 7min</td>
+</tr><tr>
+<td>2.	&nbsp;&nbsp;&nbsp;&nbsp; 4°C	&nbsp;&nbsp;&nbsp;&nbsp; //</td>
+</tr></table><br><br><br><br><br><br><br><br><br>
+<div align="justified">Thermocycler Program: a gradient was used between 65°C and 80°C as annealing temperature. This time we used 30 cycles.<div>

Team:Freiburg/Notebook/TAL

From 2012.igem.org