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| | Both plates had lawns on them however the plate containing the colony (along with some lawn and labelled Isolate) was green which was weird<br> | | Both plates had lawns on them however the plate containing the colony (along with some lawn and labelled Isolate) was green which was weird<br> |
| | <br> | | <br> |
| − | Took plate from 3/8/16 and streaked on a plate divided in 3 a single colony, the lawn, and for the last portion, 10 uL of the B subtilis solution in the fridge was diluted in 200 uL of LB before streaking it. | + | Took plate from 3/8/16 and streaked on a plate divided in 3 a single colony, the lawn, and for the last portion, 10 uL of the B subtilis solution in the fridge was diluted in 200 uL of LB before streaking it.<br> |
| | The rest of B subtilis solution in the fridge was spinned, diluted in 10ml LB and divided in 2 x 50 mL tubes, 5 uL of Kan was added in each. Both were put back in the fridge<br> | | The rest of B subtilis solution in the fridge was spinned, diluted in 10ml LB and divided in 2 x 50 mL tubes, 5 uL of Kan was added in each. Both were put back in the fridge<br> |
| | <br> | | <br> |
| | Tris HCl made by Kevin<br> | | Tris HCl made by Kevin<br> |
| | <br> | | <br> |
| − | All streaks grew well so we put them in fridge<br> | + | All streaks grew well so we put them in fridge<br> </p> |
| | | | |
| | </div> | | </div> |
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| | <div align="center" style="margin: 10px 0px 10px;" onClick="ShowHide(week3)"><h3>Week 3 :</h3><img src="aaa" width=600px" height="200px"/></div> | | <div align="center" style="margin: 10px 0px 10px;" onClick="ShowHide(week3)"><h3>Week 3 :</h3><img src="aaa" width=600px" height="200px"/></div> |
| | <div id="week3" style="display: none;"> | | <div id="week3" style="display: none;"> |
| − | | + | <p> |
| | <u>Tris-EDTA preparation (Sofiane):</u><br> | | <u>Tris-EDTA preparation (Sofiane):</u><br> |
| | <ol> | | <ol> |
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| | <li>➟1M Tris : 30,285g + 205 mL H2O. Ajust pH 7.5 with HCl. </li><br> | | <li>➟1M Tris : 30,285g + 205 mL H2O. Ajust pH 7.5 with HCl. </li><br> |
| | </ol> | | </ol> |
| − | <i>Note :</i> pH ajustment failed, I add 25mL of 12% HCl and 12 mL of 20% HCl to have a pH 7,6. <br> Concentration is not good anymore. We have to make this solution again. Maybe buy TE Buffer? Verification of TE we have is needed! <br> | + | <p><i>Note :</i> pH ajustment failed, I add 25mL of 12% HCl and 12 mL of 20% HCl to have a pH 7,6. <br> Concentration is not good anymore. We have to make this solution again. Maybe buy TE Buffer? Verification of TE we have is needed! <br> |
| | <br> | | <br> |
| | <u><b>Competency test (Djamila/Zinebe)</b></u> | | <u><b>Competency test (Djamila/Zinebe)</b></u> |
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| | Made SpII-EGTA solution (solutions made yesterday by Sofiane) <br> | | Made SpII-EGTA solution (solutions made yesterday by Sofiane) <br> |
| | <br> | | <br> |
| − | <u>T base 200 ml :</u><br> | + | <u>T base 200 ml :</u><br></p> |
| | <ol> | | <ol> |
| | <li>➟50% (w/v) glucose 2 ml<br> | | <li>➟50% (w/v) glucose 2 ml<br> |
| Line 126: |
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| | <li>➟4 ml EGTA (0.1 M, pH 8.0) <br> | | <li>➟4 ml EGTA (0.1 M, pH 8.0) <br> |
| | </ol> | | </ol> |
| − | Aliquots put at -20°C<br> | + | <p>Aliquots put at -20°C<br> |
| | <br> | | <br> |
| | After thawing competent BSU9716 at 37C in incubator (water bath had issues), added 500 uL of SpII-EGTA and mixed up and down. <br> | | After thawing competent BSU9716 at 37C in incubator (water bath had issues), added 500 uL of SpII-EGTA and mixed up and down. <br> |
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| | <u>Note: </u><br> | | <u>Note: </u><br> |
| | Should have spread the transformed bacteria on Cm and Kan plates<br> | | Should have spread the transformed bacteria on Cm and Kan plates<br> |
| − | Competency test kit contains five vials of purified DNA from BBa_J04450 (RFP construct) in plasmid backbone pSB1C3 (cm resistant). Each vial contains DNA at a different concentration: 50pg/ul, 20pg/ul, 10pg/ul, 5pg/ul, 0.5pg/ul. <br> | + | Competency test kit contains five vials of purified DNA from BBa_J04450 (RFP construct) in plasmid backbone pSB1C3 (cm resistant). Each vial contains DNA at a different concentration: 50pg/ul, 20pg/ul, 10pg/ul, 5pg/ul, 0.5pg/ul. <br> </p> |
| | | | |
| | </div> | | </div> |
Week 1 :
Competence of Bsu9716:
Bacteria from 2/8/16 in fridge (Dj)
50 ml LB and 10 uL Kan added (so total 150 mL and 15 uL Kan) and cells back in incubator
Spin (4000 rpm 10 min) 50 ml X 2 and used pellet for competency
Spinned again same way after pulling both pellet together
Changed medium (50 mL LB + 5 uL Kan) and put it back at 4 degrees
Stock solutions (Dj)
Name Mass (g) Total Volume (mL)
1.2% MgSO4 0.1023 12.5
10% (w/v) Bacto yeast extract 1.0096 10
1% (w/v) casamino acids 0.1039 10
0.1 M CaCl2 (110.98 g/mol) 0.1792 15
SpC medium made by Djamila
T base 20 ml
50% (w/v) filtered glucose 0.2 ml
1.2% (w/v) MgSO4 0.3 ml
10% (w/v) Bacto yeast extract 0.4 ml
1% (w/v) casamino acids 0.5 ml
ODi 0.5 and put back at 37 degrees with shaking
ODf 0.8
SpII medium made by Sofiane
T base 200 ml
50% (w/v) filtered glucose 2 ml
1.2% (w/v) MgSO4 14 ml
10% (w/v) Bacto yeast extract 2 ml
1% (w/v) casamino acids 2 ml
0.1 M CaCl2 1 ml
2 mL of SpC BSU in SpII and 90 min incubation 37 degrees with shaking
Note:
Originally 1.2% of the dihydrate form so made the calculations in function of that; and Sofiane had to make a second batch
50% (w/v) glucose was filtered
No tryptophan added for the cell growth
Plates from 03/08/2016 (Zinebe)
Contains lawn and colonies ⇒ Not sure which are the B. subtilis.
Diluted some of the lawn and the colony each in 200 uL LB and plated it on LB-Kan then 37 degrees overnight
Note:
LB used for dilution was contaminated
When picking the colony with a tip some of the lawn was scraped with it
Pick primers and autoclaved MilliQ at school
Plates (from 04/08/16) (DJ)
Both plates had lawns on them however the plate containing the colony (along with some lawn and labelled Isolate) was green which was weird
Took plate from 3/8/16 and streaked on a plate divided in 3 a single colony, the lawn, and for the last portion, 10 uL of the B subtilis solution in the fridge was diluted in 200 uL of LB before streaking it.
The rest of B subtilis solution in the fridge was spinned, diluted in 10ml LB and divided in 2 x 50 mL tubes, 5 uL of Kan was added in each. Both were put back in the fridge
Tris HCl made by Kevin
All streaks grew well so we put them in fridge
Week 2 :
Nothing done at the bench this week because of material issues
Week 3 :
Tris-EDTA preparation (Sofiane):
- ➟10mL 1M Tris pH 7.5 + 2mL 0,5M EDTA pH 8.0
- ➟0,5M EDTA : 18,6g EDTA + 100 mL H2O. Ajuste pH 8.0 with solid NaOH (2,6g)
- ➟1M Tris : 30,285g + 205 mL H2O. Ajust pH 7.5 with HCl.
Note : pH ajustment failed, I add 25mL of 12% HCl and 12 mL of 20% HCl to have a pH 7,6.
Concentration is not good anymore. We have to make this solution again. Maybe buy TE Buffer? Verification of TE we have is needed!
Competency test (Djamila/Zinebe)
Chloramphenicol (cm 25 mg/mL) preparation:
0.25 g diluted in 10 mL EtOH 95%; aliquots at -20
Note: first dilution in milliQ water by mistake; got rid of water and tried to let it dry but without success so will probably just add directly EtOH in to make more Cm
Cm (Cf = 5 ug/mL) LB plates:
70 mL melted LB agar + 14 uL cm
Note: agar cooled too much before pouring plate (only got 3 plates) so made more
100 mL melted LB agar + 20 uL cm
Competency test (CT)
Made SpII-EGTA solution (solutions made yesterday by Sofiane)
T base 200 ml :
- ➟50% (w/v) glucose 2 ml
- ➟1.2% (w/v) MgSO4·3H2O 14 ml
- ➟10% (w/v) Bacto yeast extract 2 ml
- ➟1% (w/v) casamino acids 2 ml
- ➟4 ml EGTA (0.1 M, pH 8.0)
Aliquots put at -20°C
After thawing competent BSU9716 at 37C in incubator (water bath had issues), added 500 uL of SpII-EGTA and mixed up and down.
Added 50 uL bacteria in 5 eppendorf tubes after spinning CT plasmids, added 1 uL of DNA in the appropriate tube (50pg/ul, 20pg/ul, 10pg/ul, 5pg/ul, 0.5pg/ul).
Bacteria+DNA mixture incubated at 37°C with shaking (150 rpm) for an hour
Spreaded the bacteria on Cm LB agar plate then put at 37°C overnight
At this point from the rest of competent bacteria, 100 uL spread on Kan plates
Note:
Should have spread the transformed bacteria on Cm and Kan plates
Competency test kit contains five vials of purified DNA from BBa_J04450 (RFP construct) in plasmid backbone pSB1C3 (cm resistant). Each vial contains DNA at a different concentration: 50pg/ul, 20pg/ul, 10pg/ul, 5pg/ul, 0.5pg/ul.
Week 4 :
Ca me soule toujours autant
- Benjamin : Il s'est fait chier
- Nassim : Il a cassé les couilles
- Sofiane : Il a tout fait cramer
- Wilhelm : Il est reparti
- Kévin : Il est pas venu
- Perwin : Continuation de la quête chez les RG
- Zinebe : Elle a volé le PLA
- Djamila : Comme d'hab, le quota
- Les autres : Vacances
Week 5 :
Ca me soule toujours autant
- Benjamin : Il s'est fait chier
- Nassim : Il a cassé les couilles
- Sofiane : Il a tout fait cramer
- Wilhelm : Il est reparti
- Kévin : Il est pas venu
- Perwin : Continuation de la quête chez les RG
- Zinebe : Elle a volé le PLA
- Djamila : Comme d'hab, le quota
- Les autres : Vacances
Week 6 :
Ca me soule toujours autant
- Benjamin : Il s'est fait chier
- Nassim : Il a cassé les couilles
- Sofiane : Il a tout fait cramer
- Wilhelm : Il est reparti
- Kévin : Il est pas venu
- Perwin : Continuation de la quête chez les RG
- Zinebe : Elle a volé le PLA
- Djamila : Comme d'hab, le quota
- Les autres : Vacances
Week 7 :
Ca me soule toujours autant
- Benjamin : Il s'est fait chier
- Nassim : Il a cassé les couilles
- Sofiane : Il a tout fait cramer
- Wilhelm : Il est reparti
- Kévin : Il est pas venu
- Perwin : Continuation de la quête chez les RG
- Zinebe : Elle a volé le PLA
- Djamila : Comme d'hab, le quota
- Les autres : Vacances
Week 8 :
Ca me soule toujours autant
- Benjamin : Il s'est fait chier
- Nassim : Il a cassé les couilles
- Sofiane : Il a tout fait cramer
- Wilhelm : Il est reparti
- Kévin : Il est pas venu
- Perwin : Continuation de la quête chez les RG
- Zinebe : Elle a volé le PLA
- Djamila : Comme d'hab, le quota
- Les autres : Vacances
