Difference between revisions of "Team:Paris Saclay/Notebook/July/28"

(Tuesday 28th July)
(Tuesday 28th July)
 
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{{Team:Paris_Saclay/notebook_header}}
 
=Tuesday 28th July=
 
=Tuesday 28th July=
 
==Lab Work==
 
==Lab Work==
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Purification on agarose gel 1%, migration 100V
 
Purification on agarose gel 1%, migration 100V
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[[File:ParisSaclay 28.07.15-purif.jpg|300px|center]]
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<html><i><p>Verification of gel purification, from left to right: 1. Empty, 2. Empty, 3. Empty, 4. <a href="https://2015.igem.org/File:Paris_Saclay-Ladder.jpg" target="_blank">DNA Ladder</a>, 5. BBa_K1707006, 6. BBa_K1707007, 7. BBa_K1399019, 8. BBa_K1399023, 9. Empty, 10. Empty, 11. Empty, 12. Empty</p></i></html>
 
Cut with a scalpel
 
Cut with a scalpel
 
Purification with the PCR Clean up kit from Macherey-Nagel
 
Purification with the PCR Clean up kit from Macherey-Nagel
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Agarose gel 1%
 
Agarose gel 1%
 
Migration 100V
 
Migration 100V
 
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[[File:ParisSaclay 28.07.15-quantif2.jpg|300px|center]]
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<html><i><p>Quantification, from left to right: 1. <a href="https://2015.igem.org/File:Paris_Saclay-Ladder.jpg" target="_blank">DNA Ladder</a>, 2. BBa_B0030, 3. BBa_R0051, 4. BBa_J23117#1, 5. BBa_J23117#2, 6. BBa_K1399019, 7. BBa_K1399023, 8. BBa_K1707006, 9. BBa_K1707007, 10. BBa_K1707003#4</p></i></html>
  
 
===Interlab study===
 
===Interlab study===
 
''by Johan''
 
''by Johan''
  
 
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https://2015.igem.org/Team:Paris_Saclay/Measurement#28th_July
Tecan utilisation :
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we use only LB without chloramphenicol and we suspect a contamination of our samples.
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We depose in inch well 300µL
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We analyse the OD and fluorescence's variation (the excitation and emission wave lenght were choose after a scan in the process to obtain the best results)
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For each sample, we depose twelve time (12x8 plate)
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*LB
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*Competent cells
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*Cells with J23101
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*Cells with J23101 + GFP
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*Cells with J23106
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*Cells with J23106 + GFP
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*Cells with J23117
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*Cells with J23117 + GFP
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We let's run for 20 cycles of 1 hour
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We create new culture of BBa_J23101/BBa_J23106/BBa_J23117 + BBa_I13504.
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Latest revision as of 21:20, 18 September 2015


Tuesday 28th July

Lab Work

Plasmid extraction

by Coralie

Biobricks:

  • BBa_K1707005 #1 and #2
  • BBa_K1707006 #1 and #2
  • BBa_K1707007 #1 and #2

With Macherey-Nigel Nucleospin kit


Digestion

by Coralie

  • BBa_B0030 and BBa_R0051
    • 2µL Buffer FastDigest 10x
    • 1µL SpeI
    • 1µL PstI
    • 10µL Plasmid
    • 6µL H2O
  • BBa_K1707007, BBa_K1707006, BBa_K1399019 and BBa_K1399023
    • 2µL Buffer FastDigest 10x
    • 1µL XbaI
    • 1µL PstI
    • 10µL Plasmid
    • 6µL H2O
  • BBa_J23117
    • 1µL Buffer FastDigest 10x
    • 1µL XbaI
    • 1µL PstI
    • 2µL Plasmid
    • 5µL H2O

Incubation 1h30, 37°C

Purification gel

by Pauline, Audrey and Coralie

Biobricks:

  • BBa_K1707006
  • BBa_K1707007
  • BBa_K1399019
  • BBa_K1399023


Purification on agarose gel 1%, migration 100V

ParisSaclay 28.07.15-purif.jpg

Verification of gel purification, from left to right: 1. Empty, 2. Empty, 3. Empty, 4. DNA Ladder, 5. BBa_K1707006, 6. BBa_K1707007, 7. BBa_K1399019, 8. BBa_K1399023, 9. Empty, 10. Empty, 11. Empty, 12. Empty

Cut with a scalpel Purification with the PCR Clean up kit from Macherey-Nagel Observation: BBa_K1399019 and BBa_K1399023 weren't on the right length on the gel

Soil experiment

by Audrey, Johan and Coralie

Soil

We put 100µL of each culture on MacConkey plate with specific antbiotic (Control +):

  • 1696: Tetracyclin
  • 1693: Spectinomycine
  • 1320: Chloramphenicol

We put 30 mL of each culture in 60g of non sterile soil in a pot.

  • 1696: 3 pots
  • 1693: 3 pots
  • 1320: 3 pots

We put 30 mL of clean LB in 60g of non sterile soil in a pot (Control -)

  • LB: 3 pots

After this contamination, we take 1g of each pot to make the J0 measurement. We dilute it in 5mL of sterile H2O, and shake it during 5 min. Then, we let it to decant during 15 min. We take 50µL of the supernatant, and dilute it in 950µL of Sterile H2O (complete dilution from the soil is now at 10-2) We put 100µL of this previous dilution on plates that fits. We incubate plates over night at 37°C

Pots are placed in trays: 1 strain by tray. Trays are covered by a shrink-wrap, and we let them in room temperature

Water

We test two different water: seawater, from the Atlantic ocean, and stagnant water from Orsay's pool. For each water, we make dilutions: 10-1, 10-2, 10-3 and 10-4 We 100µL of different dilution on each type of plate:

  • LB without antibiotic
  • LB + Spectinomycin
  • LB + tetracyclin
  • LB + Chloramphenicol
  • MacConkey without antibiotic
  • MacConkey + Spectinomycin
  • MacConkey + Tetracyclin
  • MacConkey + Chloramphenicol

We incubate plates over night at 37°C

New culture

by Pauline

Biobricks:

  • BBa_K1707008
  • BBa_K1707010

We take 2 colony of each, and put it in 5mL of LB + 20µg/mL Chloramphenicol Incubation 37°C, 250 rpm

Purification

by Audrey

Biobricks:

  • BBa_B0030
  • BBa_R0051
  • BBa_J23117 #1 and #2
  • BBa_K1399019
  • BBa_K1399023
  • BBa_K1707006
  • BBa_K1707007

With PCR CLean-up/Gel extraction kit from Macherey-Nigel

Quantification

by Audrey

Agarose gel 1% Migration 100V

ParisSaclay 28.07.15-quantif2.jpg

Quantification, from left to right: 1. DNA Ladder, 2. BBa_B0030, 3. BBa_R0051, 4. BBa_J23117#1, 5. BBa_J23117#2, 6. BBa_K1399019, 7. BBa_K1399023, 8. BBa_K1707006, 9. BBa_K1707007, 10. BBa_K1707003#4

Interlab study

by Johan

https://2015.igem.org/Team:Paris_Saclay/Measurement#28th_July


Member present:

  • Instructors: Alice
  • Students: Coralie, Audrey, Pauline, Johan and Seong-Koo

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