Team:Paris Saclay/Notebook/August/8

From 2013.igem.org

(Difference between revisions)
(2 - Electrophoresis to check the colony PCR products : BBa_K1155007)
 
(39 intermediate revisions not shown)
Line 7: Line 7:
==='''A - Aerobic/Anaerobic regulation system'''===
==='''A - Aerobic/Anaerobic regulation system'''===
-
((((((===='''Obtaining the PSB3K3 backbone plasmid'''====
+
===='''Obtaining biobricks in pSB3K3'''====
-
====1 - Electrophoresis of BBa_J004450 digested by EcoRI/Pst1 to check if the digestion was right====
+
====1 - Digestion of BBa_J04450 by EcoRI/PstI====
 +
 
 +
Nadia
 +
 
 +
Used quantities :
 +
* DNA : 5µL
 +
* Buffer FD : 2µL
 +
* EcoRI FD : 1µL
 +
* PstI FD : 1µL
 +
* H2O : 11µL
 +
 
 +
We incubate our digestion  at 37°C for 1h30.
 +
 
 +
====2 - Electrophoresis of BBa_J004450 digested by EcoRI/Pst1 to check if the digestion====
Damir, Nadia
Damir, Nadia
{|
{|
-
| style="width:350px;border:1px solid black;" | IMAGE
+
| style="width:350px;border:1px solid black;" |[[File:Psgel10808.jpg]]
| style="width:350px;border:1px solid black;vertical-align:top;" |
| style="width:350px;border:1px solid black;vertical-align:top;" |
*Well 1 : 6µL DNA Ladder
*Well 1 : 6µL DNA Ladder
Line 22: Line 35:
Expected sizes :
Expected sizes :
-
*PSB3K3 : 2750kb
+
*pSB3K3 : 2750kb
*GFP : 1069kb
*GFP : 1069kb
-
We obtained fragments of the right size. Now we can purify the PSB3K3 plasmid.
+
{|
-
 
+
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
-
====2 - Gel purification of the PSB3K3 plasmid from BBa_J004450 digested by EcoRI/Pst1====
+
We obtained fragments at the right size. We will purify the highest band which contains the pSB3K3 plasmid.
 +
|}
-
''2.1 - Migration of the remaining 45µL of BBa_J004450 digested by EcoRI/Pst1''
+
====3 - Electrophoresis of BBa_J004450 digested by EcoRI/PstI====
Anaïs
Anaïs
{|
{|
-
| style="width:350px;border:1px solid black;" | [[File:PsNBa8_eelution.jpg|350px]]
+
| style="width:350px;border:1px solid black;" | [[File:Psgel20808.jpg]]
| style="width:350px;border:1px solid black;vertical-align:top;" |
| style="width:350px;border:1px solid black;vertical-align:top;" |
*Well 1 : 6µL DNA Ladder
*Well 1 : 6µL DNA Ladder
-
*Well 2 : 45µL of BBa_J004450 digested by EcoRI/Pst1
+
*Well 2 : 45µL of BBa_J004450 digested by EcoRI/Pst I
*Gel : 0.8%
*Gel : 0.8%
|}
|}
-
Now we can do a gel purification of the highest band which contains the PSB3K3 plasmid.
+
pSB3K3 : 2750bp
-
''2.2 - Electroelution of the highest band to extract the PSB3K3 plasmid from the gel''
+
{|
 +
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
 +
We obtained fragments at the right size. We will purify the highest band which contains the pSB3K3 plasmid.
 +
|}
 +
 
 +
==== 4- Electroelution of pSB3K3 digested by EcoRI/PstI====
Nadia
Nadia
-
Protocol : [[Team:Paris_Saclay/Protocols/Electroelution|Electroelution]]
+
Protocol : [[Team:Paris_Saclay/electro|Electroelution]]
-
We let the plasmid precipitate during the night.))))))))))))))))))))))
+
{|
 +
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
 +
We lost our plasmid. We will do the digestion again.
 +
|}
-
===='''Objective : obtaining Bba_K1155007'''====
+
===='''Objective : obtaining BBa_K1155007'''====
-
====1 - Colony PCR of Bba_K115007 in DH5α====
+
====1 - Colony PCR of BBa_K115007 in DH5α====
Anaïs
Anaïs
-
Colonie repiquée dans 10µL d'eau pour chaque tube ???????
+
{|
 +
| style="border:1px solid black;padding:5px;background-color:#DE;" |
 +
Transformation of 08/07/13 works. we will make a PCR Colony.
 +
|}
 +
 
 +
We took a single colony and resuspend in 10µL H2O. For each Biobrick, we did 25 PCR Colonies.
Used quantities :
Used quantities :
-
* DNA : 2µL
+
 
-
* Mix  : (it was divided in 25 tubes for each promotor with 23µL of mix in each on)
+
PCR preparation mix for 25 different colonies including:
-
** Oligo ... : 3.5µL
+
** Oligo 44 : 3.5µL
-
** Oligo ... : 3.5µL
+
** Oligo 45 : 3.5µL
** Buffer Dream Taq : 70µL
** Buffer Dream Taq : 70µL
** dNTP : 28µL
** dNTP : 28µL
** Dream Taq : 5µL
** Dream Taq : 5µL
-
** H2O : 590µL  
+
** H2O : 590µL  
 +
 
 +
PCR reaction: 
 +
* DNA : 2µL
 +
* Mix  :23µL
 +
Total volume: 25µL
PCR Program :
PCR Program :
Line 73: Line 105:
[[File:PsPcr808.jpg|400px]]
[[File:PsPcr808.jpg|400px]]
-
====2 - Electrophoresis to check the colony PCR products : Bba_K1155007====
+
====2 - Electrophoresis to check the colony PCR products : BBa_K1155007====
Anaïs, Damir
Anaïs, Damir
{|
{|
-
| style="width:350px;border:1px solid black;" | [[Team:350px|350px]]
+
| style="width:350px;border:1px solid black;" |[[File:Psgel30808.jpg]]
| style="width:350px;border:1px solid black;vertical-align:top;" |
| style="width:350px;border:1px solid black;vertical-align:top;" |
* Well 1 : 6µL DNA Ladder
* Well 1 : 6µL DNA Ladder
-
* Well 2 to 24 : 10µL of Bba_K1155007+2µL of 6X loading dye
+
* Well 2 to 24 : 10µL of BBa_K1155007 + 2µL of 6X loading dye
* Well 25 : 6µL DNA Ladder
* Well 25 : 6µL DNA Ladder
* Well 26 : 6µL DNA Ladder
* Well 26 : 6µL DNA Ladder
-
* Well 27 : 10µL of Bba_K1155007+2µL of 6X loading dye
+
* Well 27 : 6µL DNA Ladder
 +
* Well 28 : 10µL of BBa_K1155007 + 2µL of 6X loading dye
*Gel : 0.8%
*Gel : 0.8%
|}
|}
Expected size :  
Expected size :  
-
* Bba_K1155007 : 3583 bp
+
* BBa_K1155007 : 3583 bp
{|
{|
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
-
We obtain fragment at the right size for colonies 10, 14 and 15. We will extract BBa_K1155007.
+
We obtained fragments at the right size for colonies 10, 14 and 15. We will extract BBa_K1155007.
|}
|}
 +
===='''Objective : characterize BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006'''====
 +
===='''1 - Tranduction of Km in MG1655Z1 ====
 +
 +
Anaïs, Nadia
 +
 +
{|
 +
| style="border:1px solid black;padding:5px;background-color:#DE;" |
 +
We didn't obtain colonies from the transduction of 08/07/13. We will do it again.
 +
|}
 +
 +
Protocol : [[Team:Paris_Saclay/transduction|Transduction]]
 +
 +
Our Mutant strain is BW1328 (Δfnr::Km) and the wild type strain is MG1655Z1.
 +
 +
We did the first step of the protocol : bacteriophage stock on BW1328 (Δfnr::Km).
==='''A - Aerobic/Anaerobic regulation system / B - PCB sensor system'''===
==='''A - Aerobic/Anaerobic regulation system / B - PCB sensor system'''===
Line 102: Line 150:
===='''Objective : obtaining FNR and BphR2 proteins'''====
===='''Objective : obtaining FNR and BphR2 proteins'''====
-
====1 - Gel purification of PCR product : BphR2 Part I, BphR2 Part II, RBS-BphR2 Part I, FNR Part I, FNR Part II, RBS-FNR Part I====
+
====1 - Extraction of plasmid  pSB1C3 containing BphR2 ,FNR and RBS-FNR in competent cell DH5α====
Damir
Damir
-
Protocol : [[Team:Paris_Saclay/Protocols/Gel purification|Gel purification]]
+
{|
 +
| style="border:1px solid black;padding:5px;background-color:#DE;" |
 +
Transformation of 08/02/13 works. We will extract plasmids.
 +
|}
 +
 
 +
Protocol : [http://www.mn-net.com/tabid/1452/default.aspx Gel purification ]
{|
{|
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
-
CONCLUSION !!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!
+
We lost our plasmids. We will do the Gibson assembly again.
 +
|}
 +
 
 +
====2 - Gel purification of RBS-BphR2 Part I====
 +
 
 +
Nadia, XiaoJing
 +
 
 +
Protocol : [http://www.mn-net.com/tabid/1452/default.aspx Gel purification ]
 +
 
 +
{|
 +
| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
 +
We lost fragment. We will do the PCR again.
 +
|}
 +
 
 +
 
 +
{| border="1" align="center"
 +
|[[Team:Paris Saclay/Notebook/August/7|<big>Previous day</big>]]
 +
 
 +
|[[Team:Paris_Saclay/Notebook|<big>Back to calendar</big>]]
 +
 
 +
|[[Team:Paris Saclay/Notebook/August/9|<big>Next day</big>]]
|}
|}
{{Team:Paris_Saclay/incl_fin}}
{{Team:Paris_Saclay/incl_fin}}

Latest revision as of 01:26, 5 October 2013

Navigation Home Team Project Labwork Notebook Human practices

Contents

Notebook : August 8

Lab work

A - Aerobic/Anaerobic regulation system

Obtaining biobricks in pSB3K3

1 - Digestion of BBa_J04450 by EcoRI/PstI

Nadia

Used quantities :

  • DNA : 5µL
  • Buffer FD : 2µL
  • EcoRI FD : 1µL
  • PstI FD : 1µL
  • H2O : 11µL

We incubate our digestion at 37°C for 1h30.

2 - Electrophoresis of BBa_J004450 digested by EcoRI/Pst1 to check if the digestion

Damir, Nadia

Psgel10808.jpg
  • Well 1 : 6µL DNA Ladder
  • Well 2 : 5µL of BBa_J004450 digested by EcoRI/Pst1
  • Gel : 0.8%

Expected sizes :

  • pSB3K3 : 2750kb
  • GFP : 1069kb

We obtained fragments at the right size. We will purify the highest band which contains the pSB3K3 plasmid.

3 - Electrophoresis of BBa_J004450 digested by EcoRI/PstI

Anaïs

Psgel20808.jpg
  • Well 1 : 6µL DNA Ladder
  • Well 2 : 45µL of BBa_J004450 digested by EcoRI/Pst I
  • Gel : 0.8%

pSB3K3 : 2750bp

We obtained fragments at the right size. We will purify the highest band which contains the pSB3K3 plasmid.

4- Electroelution of pSB3K3 digested by EcoRI/PstI

Nadia

Protocol : Electroelution

We lost our plasmid. We will do the digestion again.

Objective : obtaining BBa_K1155007

1 - Colony PCR of BBa_K115007 in DH5α

Anaïs

Transformation of 08/07/13 works. we will make a PCR Colony.

We took a single colony and resuspend in 10µL H2O. For each Biobrick, we did 25 PCR Colonies.

Used quantities :

PCR preparation mix for 25 different colonies including:

    • Oligo 44 : 3.5µL
    • Oligo 45 : 3.5µL
    • Buffer Dream Taq : 70µL
    • dNTP : 28µL
    • Dream Taq : 5µL
    • H2O : 590µL

PCR reaction:

  • DNA : 2µL
  • Mix  :23µL

Total volume: 25µL

PCR Program :

PsPcr808.jpg

2 - Electrophoresis to check the colony PCR products : BBa_K1155007

Anaïs, Damir

Psgel30808.jpg
  • Well 1 : 6µL DNA Ladder
  • Well 2 to 24 : 10µL of BBa_K1155007 + 2µL of 6X loading dye
  • Well 25 : 6µL DNA Ladder
  • Well 26 : 6µL DNA Ladder
  • Well 27 : 6µL DNA Ladder
  • Well 28 : 10µL of BBa_K1155007 + 2µL of 6X loading dye
  • Gel : 0.8%

Expected size :

  • BBa_K1155007 : 3583 bp

We obtained fragments at the right size for colonies 10, 14 and 15. We will extract BBa_K1155007.

Objective : characterize BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006

1 - Tranduction of Km in MG1655Z1

Anaïs, Nadia

We didn't obtain colonies from the transduction of 08/07/13. We will do it again.

Protocol : Transduction

Our Mutant strain is BW1328 (Δfnr::Km) and the wild type strain is MG1655Z1.

We did the first step of the protocol : bacteriophage stock on BW1328 (Δfnr::Km).

A - Aerobic/Anaerobic regulation system / B - PCB sensor system

Objective : obtaining FNR and BphR2 proteins

1 - Extraction of plasmid pSB1C3 containing BphR2 ,FNR and RBS-FNR in competent cell DH5α

Damir

Transformation of 08/02/13 works. We will extract plasmids.

Protocol : [http://www.mn-net.com/tabid/1452/default.aspx Gel purification ]

We lost our plasmids. We will do the Gibson assembly again.

2 - Gel purification of RBS-BphR2 Part I

Nadia, XiaoJing

Protocol : [http://www.mn-net.com/tabid/1452/default.aspx Gel purification ]

We lost fragment. We will do the PCR again.


Previous day Back to calendar Next day

Retrieved from "http://2013.igem.org/Team:Paris_Saclay/Notebook/August/8"