Difference between revisions of "Team:Paris Saclay/Notebook/August/25"
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| + | {{Team:Paris_Saclay/notebook_header}} | ||
=Tuesday 25th August= | =Tuesday 25th August= | ||
==Lab Work== | ==Lab Work== | ||
| − | |||
| − | |||
| − | |||
===Electrophoresis purification=== | ===Electrophoresis purification=== | ||
''by Audrey'' | ''by Audrey'' | ||
| − | |||
* BBa_K1707004 #5 (digested by SpeI and EcoRI) | * BBa_K1707004 #5 (digested by SpeI and EcoRI) | ||
* BBa_K1707022 #1 (digested by XbaI and PstI) | * BBa_K1707022 #1 (digested by XbaI and PstI) | ||
| Line 18: | Line 15: | ||
''by Audrey'' | ''by Audrey'' | ||
| − | |||
* BBa_K1707022 #1 | * BBa_K1707022 #1 | ||
* BBa_K1707023 #1 | * BBa_K1707023 #1 | ||
| Line 41: | Line 37: | ||
* BBa_K1707004 #5 (SpeI + PstI): 75 µg/µL | * BBa_K1707004 #5 (SpeI + PstI): 75 µg/µL | ||
* BBa_R0040 #1: 75 µg/µL | * BBa_R0040 #1: 75 µg/µL | ||
| − | |||
===PCR for the Gibson experiment=== | ===PCR for the Gibson experiment=== | ||
| Line 47: | Line 42: | ||
====Amplification Thermometer RNA BBa_K115017==== | ====Amplification Thermometer RNA BBa_K115017==== | ||
| − | |||
PCR mix for each tube: | PCR mix for each tube: | ||
* 36,75 µL H2O | * 36,75 µL H2O | ||
| Line 66: | Line 60: | ||
* 4°C for ever | * 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 | ||
PCR mix for each tube: | PCR mix for each tube: | ||
| Line 87: | Line 86: | ||
* 4°C for ever | * 4°C for ever | ||
| − | ====Amplification (reverse PCR) | + | ====Amplification (reverse PCR)==== |
| + | * BBa_K1707021 | ||
PCR mix for each tube: | PCR mix for each tube: | ||
| Line 107: | Line 107: | ||
* 4°C for ever | * 4°C for ever | ||
| − | ====Amplification (reverse PCR) | + | ====Amplification (reverse PCR)==== |
| + | * BBa_K1707027 | ||
PCR mix for each tube: | PCR mix for each tube: | ||
| Line 133: | Line 134: | ||
Agarose gel 1%, migration 90V | Agarose gel 1%, migration 90V | ||
| − | We load on gel 5μL of PCR product | + | 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. | We can conclude that we need to start over all PCR except BBa_K115017 which seems to be OK. | ||
| − | |||
'''Member present:''' | '''Member present:''' | ||
Revision as of 07:39, 15 September 2015
Contents
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
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
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
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.
Member present:
- Instructors: Claire
- Students: Audrey
Contact
eigem.parissaclay AT gmail DOT com
t@iGEMParisSaclay
aUniversité Paris Sud
a91405 Orsay, France
Copyright © 2015 iGEM Paris Saclay. All rights reserved All inspirations encouraged.
*This wiki was conceived during long nights of work and a great coffee experience in the beautiful Orsay, France.
eigem.parissaclay AT gmail DOT com
t@iGEMParisSaclay
aUniversité Paris Sud
a91405 Orsay, France
Copyright © 2015 iGEM Paris Saclay. *This wiki was conceived during long nights of work and a great coffee experience in the beautiful Orsay, France.