Difference between revisions of "Team:Paris Saclay/Notebook/October/14"

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{{Team:Paris_Saclay/notebook_header}}
 
{{Team:Paris_Saclay/notebook_header}}
  
= Thursday 14<sup>th</sup> October=
+
= Friday 14<sup>th</sup> October=
  
 
===Visualization===
 
===Visualization===
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|}
 
|}
  
GEL SYLVIE 7
+
[[File:T--Paris Saclay--Gelsylvie7.png|400px|thumb|center|Result of the migration]]
  
 
No good clones were obtained for GFP 1.9 in pSB1C3 (pPS16_020).
 
No good clones were obtained for GFP 1.9 in pSB1C3 (pPS16_020).
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* 6 µL of water
 
* 6 µL of water
  
The mix were incubated for 30 minutes at 37°C.  
+
The mix were incubated for 30 minutes at 37°C. Then, 2 µL of digestion products and 15 µL of DNA ladder were placed in wells and migrated at 100V during 30 min.
 +
 
 +
[[File:T--Paris Saclay--Gelsylvie8.png|400px|thumb|center|Result of the migration]]
  
 
====Ligation of GFP 1.9 PCR product with PCR blunt====
 
====Ligation of GFP 1.9 PCR product with PCR blunt====
  
DNA ligase was used to join the sticky ends of the template and vector together:
+
DNA ligase was used to join the sticky ends of the template and vector together. For that purpose, two templates were used: GFP 1.9 PCR product obtained with pUC19 and GFP 1.9 PCR product obtained with gblock.
  
 
* 1 µL of vector
 
* 1 µL of vector
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* 3 µL of water
 
* 3 µL of water
  
The mix were incubated for 30 minutes at rooming temperature.  
+
The mix were incubated for 30 minutes at rooming temperature.
  
====Double transformation of DH5a cells with FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021) and GFP 1.9 in pUC19 (pPS16_009)====
+
====Transformation of DH5a cells with GFP 1.9 ligated to PCR blunt====
 
''By Sylvie''
 
''By Sylvie''
  
Dh5a cells were double transformed with pSB1C3 containing FRB - GFP 11 - FKBP - GFP 10 (pPS16_021) and with pUC19 containing GFP 1.9 (pPS16_009) using the usual [[Team:Paris_Saclay/Experiments#heat-shocktransformation|protocol]]. For that purpose, petri dishes used contained LB + Amp + Cm and two concentration of plasmids were used: 1 µL of plasmids not diluted and 1 µL of plasmids diluted 10X.
+
Dh5a cells were transformed with GFP 1.9 ligated to PCR blunt (two templates for GFP 1.9) or controls (digested plasmid) using the usual [[Team:Paris_Saclay/Experiments#heat-shocktransformation|protocol]].
 +
 
 +
====Co-transformation of DH5a cells with FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021) and GFP 1.9 in pUC19 (pPS16_009)====
 +
''By Sylvie''
 +
 
 +
Dh5a cells were co-transformed with pSB1C3 containing FRB - GFP 11 - FKBP - GFP 10 (pPS16_021) and with pUC19 containing GFP 1.9 (pPS16_009) using the usual [[Team:Paris_Saclay/Experiments#heat-shocktransformation|protocol]]. For that purpose, petri dishes used contained LB + Amp + Cm and two concentration of plasmids were used: 1 µL of plasmids not diluted and 1 µL of plasmids diluted 10X.
  
 
==== Glycerol stocks of clones containing FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021)====
 
==== Glycerol stocks of clones containing FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021)====
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The glycerol stock of the bacteria with the following plasmids were made.
 
The glycerol stock of the bacteria with the following plasmids were made.
 
*pPS16_021 (FRB - GFP 11 - FKBP - GFP 10)
 
*pPS16_021 (FRB - GFP 11 - FKBP - GFP 10)
 +
 +
{{Team:Paris_Saclay/notebook_footer}}

Latest revision as of 11:17, 19 October 2016

Friday 14th October

Visualization

PCR of GFP 1.9 in pUC19 (pPS16_009) and GFP 1.9 in gblock

By Sylvie

A new PCR was run in order to obtain a new GFP 1.9 PCR product. For each amplification, two matrix were used: GFP 1.9 in pUC19 (pPS16_009) and GFP 1.9 in gblock.

For each 50μl of reaction, mix the following reagents :

  • 1 µL of matrix (diluted 10X)
  • 1 µL of dNTPs (10mM)
  • 2.5 µL of each primer mix (10µM)
  • 10 µL of buffer (5X)
  • 0,5 µL of Phusion polymerase
  • 30 µL of nuclease free water
  • 1.5 µL of DMSO

Mix gently and aliquot 50 μl of the mix into the PCR tubes on ice. Perform PCR as follow:

Step Temperature Time
Initial denaturation 98°C 30sec
30 cycles 98°C 10sec
60°C 30sec
72°C 30 sec
Final Extension 72°C 5min
Hold 4°C $\infty$

Primers used were:

Matrix GFP 1.9 in pUC19 (pPS16_009) or GFP 1.9 in gblock
Primers iPS84 and iPS140

PCR of 24 extracted GFP 1.9 in pSB1C3 (pPS16_020) from the 13th October

By Sylvie

A PCR was run on 24 extracted plasmids pPS16_020 in order to verify if the clonage worked.

For each 50μl of reaction, mix the following reagents :

  • 1 µL of matrix
  • 1 µL of dNTPs (10mM)
  • 2.5 µL of each primer mix (10µM)
  • 10 µL of buffer (5X)
  • 0,5 µL of Phusion polymerase
  • 31.5 µL of nuclease free water

Mix gently and aliquot 50 μl of the mix into the PCR tubes on ice. Perform PCR as follow:

Step Temperature Time
Initial denaturation 95°C 5min
30 cycles 95°C 30sec
48°C 30sec
72°C 30 sec
Final Extension 72°C 5min
Hold 4°C $\infty$

Primers used were:

Matrix GFP 1.9 in pSB1C3 (pPS16_020) extracted the 13th October
Primers iPS168 and iPS169

Gel of PCR products

By Sylvie

5 µL of PCR products and 20 µL of DNA ladder were placed in wells and migrated at 100V during 30 min, in odrder to verify the DNA quantity.

PCR products expected were :

PCR products Expected band size (bp)
GFP 1.9 (iPS84 & iPS140) 862
GFP 1.9 (iPS168 & iPS169) 1135
Result of the migration

No good clones were obtained for GFP 1.9 in pSB1C3 (pPS16_020).

Digestion of FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021), GFP 1.9 PCR product and linearized pSB1C3

Linearized pSB1C3 was digested by restriction enzymes XbaI & PstI:

  • 4 µL of plasmid
  • 1 µL of buffer FD
  • 0.5 µL of restriction enzyme XbaI
  • 0.5 µL of restriction enzyme PstI
  • 2 µL of water

GFP 1.9 PCR product was digested by restriction enzymes XbaI & PstI:

  • 5 µL of GFP 1.9 PCR product
  • 1.5 µL of buffer FD
  • 1 µL of restriction enzyme XbaI
  • 1 µL of restriction enzyme PstI
  • 6.5 µL of water

FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021) was digested by restriction enzymes SpeI & PstI:

  • 10 µL plasmid
  • 2 µL of buffer FD
  • 1 µL of restriction enzyme SpeI
  • 1 µL of restriction enzyme PstI
  • 6 µL of water

The mix were incubated for 30 minutes at 37°C. Then, 2 µL of digestion products and 15 µL of DNA ladder were placed in wells and migrated at 100V during 30 min.

Result of the migration

Ligation of GFP 1.9 PCR product with PCR blunt

DNA ligase was used to join the sticky ends of the template and vector together. For that purpose, two templates were used: GFP 1.9 PCR product obtained with pUC19 and GFP 1.9 PCR product obtained with gblock.

  • 1 µL of vector
  • 3 µL of GFP 1.9 PCR product
  • 2 µL of Buffer T4 10X
  • 1 µL of ligase T4 enzyme
  • 3 µL of water

The mix were incubated for 30 minutes at rooming temperature.

Transformation of DH5a cells with GFP 1.9 ligated to PCR blunt

By Sylvie

Dh5a cells were transformed with GFP 1.9 ligated to PCR blunt (two templates for GFP 1.9) or controls (digested plasmid) using the usual protocol.

Co-transformation of DH5a cells with FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021) and GFP 1.9 in pUC19 (pPS16_009)

By Sylvie

Dh5a cells were co-transformed with pSB1C3 containing FRB - GFP 11 - FKBP - GFP 10 (pPS16_021) and with pUC19 containing GFP 1.9 (pPS16_009) using the usual protocol. For that purpose, petri dishes used contained LB + Amp + Cm and two concentration of plasmids were used: 1 µL of plasmids not diluted and 1 µL of plasmids diluted 10X.

Glycerol stocks of clones containing FRB - GFP 11 - FKBP - GFP 10 in pSB1C3 (pPS16_021)

By Sylvie

The glycerol stock of the bacteria with the following plasmids were made.

  • pPS16_021 (FRB - GFP 11 - FKBP - GFP 10)





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