Latest revision as of 23:15, 18 September 2015

Tuesday 25th August

Lab Work

Electrophoresis purification

by Audrey

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

Agarose gel 1%, migration 90V

Verification of gel purification, from left to right: 1. DNA Ladder, 2. BBa_K1707004#5, 3. BBa_K1707022#1, 4. Empty, 5. Empty

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

Quantification

by Audrey

Agarose gel 1%, migration 90V. For each sample:

5 µL plasmid
5 µL H2O
2 µL Ladder 6x

Quantification, from left to right: 1. DNA Ladder, 2. BBa_R0040 (EcoRI+XbaI), 3. BBa_K1707004#5 (SpeI+EcoRI), 4. BBa_K1707004#5 (SpeI+PstI), 5. BBa_K1707022, 6. BBa_K1707023, 7. Empty, 8. Empty, 9. Empty, 10. Empty

We can conclude:

BBa_K1707022 #1: nothing can be seen
BBa_K1707023 #1: nothing can be seen
BBa_K1707004 #5 (SpeI + EcoRI): 20 µg/µL
BBa_K1707004 #5 (SpeI + PstI): 75 µg/µL
BBa_R0040 #1: 75 µg/µL

PCR for the Gibson experiment

by Audrey

Amplification Thermometer RNA BBa_K115017

PCR mix for each tube:

36,75 µL H2O
10 µL Buffer Phusion
1 μL dNTP 10mM
0,5 μL Forward primer
0,5 μL Reverse primer
1μL plasmid BBa_K115017 v10
0,25 μL DNA Pol Phusion

PCR Cycle:

98°C - 30 seconds
30 cycles:
- 98°C - 5 seconds
- 69,8°C - 30 seconds
- 72°C - 10 seconds
72°C - 10 minutes
4°C for ever

Amplification (reverse PCR)

BioBricks with cI and cI857:

BBa_K1707013
BBa_K1707019
BBa_K1707020
BBa_K1707035
BBa_K1707036

PCR mix for each tube:

36,75 µL H2O
10 µL Buffer Phusion
1 μL dNTP 10mM
0,5 μL Forward primer
0,5 μL Reverse primer
1μL plasmid (dilution 1/10 or 1/100)
0,25 μL DNA Pol Phusion

PCR Cycle:

98°C - 30 seconds
30 cycles:
- 98°C - 5 seconds
- 65,6°C - 30 seconds
- 72°C - 3 minutes
72°C - 10 minutes
4°C for ever

Amplification (reverse PCR)

BBa_K1707021

PCR mix for each tube:

36,75 µL H2O
10 µL Buffer Phusion
1 μL dNTP 10mM
0,5 μL Forward primer
0,5 μL Reverse primer
1μL plasmid (dilution 1/10 or 1/100)
0,25 μL DNA Pol Phusion

PCR Cycle:

98°C - 30 seconds
30 cycles:
- 98°C - 5 seconds
- 65,6°C - 30 seconds
- 72°C - 3 minutes
72°C - 10 minutes
4°C for ever

Amplification (reverse PCR)

BBa_K1707027

PCR mix for each tube:

36,75 µL H2O
10 µL Buffer Phusion
1 μL dNTP 10mM
0,5 μL Forward primer
0,5 μL Reverse primer
1μL plasmid (dilution 1/10 or 1/100)
0,25 μL DNA Pol Phusion

PCR Cycle:

98°C - 30 seconds
30 cycles:
- 98°C - 5 seconds
- 62,6°C - 30 seconds
- 72°C - 2 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}}
 =Tuesday 25th August=
 ==Lab Work==
 ===Electrophoresis purification===
 ''by Audrey''
-Biobricks:
 * BBa_K1707004 #5 (digested by SpeI and EcoRI)
 * BBa_K1707022 #1 (digested by XbaI and PstI)
 Agarose gel 1%, migration 90V
+[[File:ParisSaclay 25.08.15-Purif sur gel.jpg|200px|center]]
+<html><p><i>Verification of gel purification, from left to right: 1. <a href="https://2015.igem.org/File:Paris_Saclay-Ladder.jpg" target="_blank">DNA Ladder</a>, 2. BBa_K1707004#5, 3. BBa_K1707022#1, 4. Empty, 5. Empty</i></p></html>
 We cut corresponding bands with a scalpel.
@@ Line 18: / Line 16: @@
 ''by Audrey''
-Biobricks:
 * BBa_K1707022 #1
 * BBa_K1707023 #1
@@ Line 34: / Line 31: @@
 * 5 µL H2O
 * 2 µL Ladder 6x
+[[File:ParisSaclay 25.08.15-quantif.jpg|300px|center]]
+<html><p><i>Quantification, from left to right: 1. <a href="https://2015.igem.org/File:Paris_Saclay-Ladder.jpg" target="_blank">DNA Ladder</a>, 2. BBa_R0040 (EcoRI+XbaI), 3. BBa_K1707004#5 (SpeI+EcoRI), 4. BBa_K1707004#5 (SpeI+PstI), 5. BBa_K1707022,  6. BBa_K1707023, 7. Empty, 8. Empty, 9. Empty, 10. Empty</i></p></html>
 We can conclude:
 * BBa_K1707022 #1: nothing can be seen
@@ Line 41: / Line 39: @@
 * BBa_K1707004 #5 (SpeI + PstI): 75 µg/µL
 * BBa_R0040 #1: 75 µg/µL
 ===PCR for the Gibson experiment===
@@ Line 47: / Line 44: @@
 ====Amplification Thermometer RNA BBa_K115017====
 PCR mix for each tube:
 * 36,75 µL H2O
@@ Line 66: / Line 62: @@
 * 4°C for ever
+====Amplification (reverse PCR)====
-====Amplification (reverse PCR) biobricks with cI and cI857: BBa_K1707013, BBa_K1707019, BBa_K1707020, BBa_K1707035, BBa_K1707036====
+BioBricks with cI and cI857:
+* BBa_K1707013
+* BBa_K1707019
+* BBa_K1707020
+* BBa_K1707035
+* BBa_K1707036
 PCR mix for each tube:
@@ Line 87: / Line 88: @@
 * 4°C for ever
-====Amplification (reverse PCR) biobrick: BBa_K1707021====
+====Amplification (reverse PCR)====
+* BBa_K1707021
 PCR mix for each tube:
@@ Line 107: / Line 109: @@
 * 4°C for ever
-====Amplification (reverse PCR) biobrick: BBa_K1707027====
+====Amplification (reverse PCR)====
+* BBa_K1707027
 PCR mix for each tube:
@@ Line 126: / Line 129: @@
 * 72°C - 10 minutes
 * 4°C for ever
-===Electrophoresis===
-''by Audrey''
-Agarose gel 1%, migration 90V
-We load on gel 5μL of PCR product
-We can conclude that we need to start over all PCR except BBa_K115017 which seems to be OK.

Difference between revisions of "Team:Paris Saclay/Notebook/August/25"

Latest revision as of 23:15, 18 September 2015

Contents

Tuesday 25th August

Lab Work

Electrophoresis purification

Purification

Quantification

PCR for the Gibson experiment

Amplification Thermometer RNA BBa_K115017

Amplification (reverse PCR)

Amplification (reverse PCR)

Amplification (reverse PCR)