Revision as of 07:41, 15 September 2015

Wednesday 26th August

Lab Work

PCR on colony

by Audrey

BBa_K1707037 #1 to #9

PCR mix for each tube:

9,75 µL H2O
5 µL Buffer Taq 10x
1 μL dNTP 10mM
0,5 μL Forward primer iPS43
0,5 μL Reverse primer iPS44
3 μL 25mM MgCl2
0,25 μL Taq Pol

PCR Cycle:

95°C - 6 + 2 min
30 cycles:
- 95°C - 30 seconds
- 51,8°C - 30 seconds
- 72°C - 2 minutes
72°C - 10 minutes
4°C for ever

Electrophoresis

by Audrey

Agarose gel 1%, migration 90V

PCR Products of BBa_K1707037

We can't conclude anything because we can't see any positive result. So we choose arbitrary 5 clones for different extractions.

Electrophoresis purification

by Audrey

PCR product of BBa_K175017 from the 08/25/2015

In each weel of the agarose gel, we put 45μL of PCR Product + 15 μL Ladder 6x

Agarose gel 1%, Migration 90V

We cut bands with a scalpel and purificate them by the Macherey-Nagel gel purification kit

Plasmid extraction

by Audrey

BBa_K1707022 #1
BBa_K1707023 #2
BBa_K1707037 #5 to #9
BBa_K1707004 #2 (from two different cultures)

With Macherey-Nagel Extraction kit

BBa_K1707004 #5 (digested by SpeI and EcoRI)
BBa_K1707022 #1 (digested by XbaI and PstI)

Agarose gel 1%, migration 90V

We cut corresponding bands with a scalpel.

Purification

by Audrey

BBa_K1707022 #1
BBa_K1707023 #1
BBa_K1707004 #5
BBa_R0040 #1

With Macherey Nagel purification kit

Reverse PCR

by Audrey

1

BBa_K1707013
BBa_K1707019
BBa_K1707020
BBa_K1707030
BBa_K1707035
BBa_K1707036

PCR mix for each tube:

36,75 µL H2O
10 µL Buffer Phusion 5x
1 μL dNTP 10mM
0,5 μL Forward primer insertion cI
0,5 μL Reverse primer RV
1μL plasmid
0,25 μL DNA Pol Phusion
With and without DMSO 1,5μL

2

BBa_K1707021
BBa_K1707027

PCR mix for each tube:

36,75 µL H2O
10 µL Buffer Phusion 5x
1 μL dNTP 10mM
0,5 μL Forward primer insertion CFP or GFP
0,5 μL Reverse primer insertion RV
1μL plasmid
0,25 μL DNA Pol Phusion
With and without DMSO 1,5μL

Control (-) for primers:

PCR mix for each tube:

36,75 µL H2O
10 µL Buffer Phusion 5x
1 μL dNTP 10mM
0,5 μL Forward primer insertion CFP/GFP/cI + 0,5μL iPS44 or 0,5 μL Reverse primer insertion RV + 0,5μL iPS43
1μL plasmid BBa_K1707013 or BBa_K1707021 or BBa_K1707027
0,25 μL DNA Pol Phusion
With and without DMSO 1,5μL

PCR Cycle:

98°C - 30 seconds
3 cycles:
- 98°C - 5 seconds
- 55°C - 30 seconds
- 72°C - 3 minutes
27 cycles:
- 98°C - 5 seconds
- 65°C - 30 seconds
- 72°C - 3 minutes
72°C - 10 minutes
4°C for ever

Member present:

Instructors: Claire
Students: Audrey

Back to the calendar

@@ Line 1: / Line 1: @@
+{{Team:Paris_Saclay/notebook_header}}
 =Wednesday 26th August=
 ==Lab Work==
@@ Line 5: / Line 6: @@
 ''by Audrey''
-Biobrick: BBa_K1707037 #1 to #9
+* BBa_K1707037 #1 to #9
 PCR mix for each tube:
@@ Line 51: / Line 52: @@
 ''by Audrey''
-Biobricks:
 * BBa_K1707022 #1
 * BBa_K1707023 #2
@@ Line 59: / Line 59: @@
 With Macherey-Nagel Extraction kit
-Biobricks:
 * BBa_K1707004 #5 (digested by SpeI and EcoRI)
 * BBa_K1707022 #1 (digested by XbaI and PstI)
@@ Line 71: / Line 69: @@
 ''by Audrey''
-Biobricks:
 * BBa_K1707022 #1
 * BBa_K1707023 #1
@@ Line 82: / Line 79: @@
 '' by Audrey''
-Biobricks:
+#1
 * BBa_K1707013
 * BBa_K1707019
@@ Line 100: / Line 97: @@
 * With and without DMSO 1,5μL
+#2
-Biobricks:
 * BBa_K1707021
 * BBa_K1707027
@@ Line 115: / Line 110: @@
 * 0,25 μL DNA Pol Phusion
 * With and without DMSO 1,5μL
@@ Line 142: / Line 136: @@
 * 72°C - 10 minutes
 * 4°C for ever
 '''Member present:'''

Difference between revisions of "Team:Paris Saclay/Notebook/August/26"

Revision as of 07:41, 15 September 2015

Contents

Wednesday 26th August

Lab Work

PCR on colony

Electrophoresis

Electrophoresis purification

Plasmid extraction

Purification

Reverse PCR