Team:Paris Saclay/Notebook/August/30

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(Notebook : August 30)
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='''Notebook : August 23'''=
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=='''Lab work'''==
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==='''A - Aerobic/Anaerobic regulation system'''===
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===='''Objective : obtaining Pfnr, NarK, NarG or NirB and RBS-LacZ-Term or RBS-AmilCP-Term in PSB3K3'''====
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(((((((((((((((===='''1 - Electrophoresis to check the digestion of Bba_J04450 by EcoRI/PstI'''====
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{|
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| style="width:350px;border:1px solid black;" |]]
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| style="width:350px;border:1px solid black;vertical-align:top;" |
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* Well 1 : 6µL DNA Ladder
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* Well 2 : 5µL of Bba_J04450 digested by EcoRI/PstI+1µl of 6X loading dye
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* Gel : 1%
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Expect sizes :
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* PSB3K3 : 2750 bp
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{|
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| style="border:1px solid black;padding:5px;background-color:#DEDEDE;" |
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We can see anything. The digestion did work.
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Revision as of 00:55, 22 September 2013

Contents

Notebook : August 30

summary

  • check the size by Gel electrophoresis for PCR clonies on Gibson assembly and ligation promoter fnr(repressor) plus RBS_AmilCP+Term_PSB1C3 .
  • Do ligation for For promoter fnr(repressor)+ RBS_LacZ+Term_PSB1C3 , promoter fnr(activator)nirK + RBS_LacZ+Term_PSB3K3 and promoter fnr(repressor) + RBS_LacZ+Term_PSB3K3 and Transformation and

incubation.



lab work


  • A.aero/anaerobic regulation system


1 -Gel electrophoresis of PCR clonies on Gibson assembly .

[[]]
  • Well 1 : 6µL DNA Ladder
  • Well AA 1-8 : Clonies from Gibson FNR_part1, FNR part1 and plasmid PSB1C3
  • Well AB 1-8 : Clonies from Gibson FNR_part1, FNR part1 and plasmid PSB1C3 Concentrate3
  • Well AC 1-8 :Clonies from Gibson RBS_BphR2_part1, BphR2_part2 and plasmid PSB1C3
  • Well AD 1-8 :Clonies from Gibson RBS_FNR part1, FNR_part2 and plasmid PSB1C3
  • Well AE 1-8 :Clonies from Gibson RBS_FNR part1, FNR_part2 and plasmid PSB1C3 Concentrate
  • Well AF 1-8 :Clonies from Gibson RBS_BphR2_part1, BphR2_part2 and plasmid PSB1C3 Concentrate
  • Gel : 1.0%

2 -Gel electrophoresis of ligation promoter fnr(repressor) plus RBS_AmilCP+Term_PSB1C3 .

[[]]
  • Well 0: 6µL DNA Ladder
  • Well 1: clone1 of ligation promoter fnr(repressor) plus RBS_AmilCP+Term_PSB1C3
  • Well 2: clone2 of ligation promoter fnr(repressor) plus RBS_AmilCP+Term_PSB1C3
  • Well 3: clone3 of ligation promoter fnr(repressor) plus RBS_AmilCP+Term_PSB1C3
  • Well 4: clone4 of ligation promoter fnr(repressor) plus RBS_AmilCP+Term_PSB1C3
  • Gel : 1.0%



Ligation


For promoter fnr(repressor)+ RBS_LacZ+Term_PSB1C3  :
promoter fnr(repressor) 8µl
RBS_LacZ+Term 3µl
Ligation buffer 2µl
Ligation T4 enzyme 2µl
H2O 6µl

Transformation theligation and spread in LB plates with Chlorenphenicol and Xgal. incubated at 37°C in aerobic condition over night.

For promoter fnr(activator)nirK + RBS_LacZ+Term_PSB3K3  :


promoter fnr(activator)nirK 3µl
RBS_LacZ+Term 3µl
Plasmid PSB3K3 5µl
Ligation buffer 2µl
Ligation T4 enzyme 1µl
H2O 6µl

Transformation theligation and spread in LB plates with k and Xgal. incubated at 37°C in anaerobic condition over night.


For promoter fnr(repressor) + RBS_LacZ+Term_PSB3K3  :


promoter fnr(repressor) 3µl
RBS_LacZ+Term 3µl
Plasmid PSB3K3 5µl
Ligation buffer 2µl
Ligation T4 enzyme 1µl
H2O 6µl

Transformation theligation and spread in LB plates with k and Xgal. incubated at 37°C in aerobic condition over night.


Previous week Back to calendar Next day


Notebook : August 23

Lab work

A - Aerobic/Anaerobic regulation system

Objective : obtaining Pfnr, NarK, NarG or NirB and RBS-LacZ-Term or RBS-AmilCP-Term in PSB3K3

(((((((((((((((====1 - Electrophoresis to check the digestion of Bba_J04450 by EcoRI/PstI====

]]
  • Well 1 : 6µL DNA Ladder
  • Well 2 : 5µL of Bba_J04450 digested by EcoRI/PstI+1µl of 6X loading dye
  • Gel : 1%

Expect sizes :

  • PSB3K3 : 2750 bp

We can see anything. The digestion did work.

))))))))))))))))))))))