Team:Amsterdam/extra/diary

From 2012.igem.org

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<h1>Diary</h1>
<h1>Diary</h1>
-
11/05/2012
+
12/07/2012
-
Gel electrophoresis of the PCR reaction performed on 10/05/2012. Non-specific products obtained. Repeat PCR? Change annealing temperature?
+
Transformation of the plasmid containing the M.ScaI methyltransferase (pIDTSMART-AMP).
-
Ladder
+
11/07/2012
-
pET28a+ (1 ng for PCR)
+
Mini-prep BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320. Elution in 25µl.
-
pET28a+ (10 ng for PCR)
+
Restriction digestion of BBa_J63009+BBa_J04450 with DraI and RsaI/XbaI.
-
peGFP (1 ng for PCR)
+
Restriction digestion of pSB1AT3+BBa_J45320 with ScaI and xhoI.
-
peGFP (10 ng for PCR)
+
Something went wrong with the digestions.....
 +
Transformation:
 +
1)pSB3C5+ BBa_J04450 (2012 iGEM distribution kit plate 1 Well 3C)
 +
2)pSB4C5+ BBa_J04450 (2012 iGEM distribution kit plate 1 Well 3E)
-
Second PCR for peGFP and pET28a+. annealing temperature = 53˚C
+
10/07/2012
-
Same results obtained..... :(
+
Set overnight cultures for BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320 for mini-prep.
-
14/05/2012
+
09/07/2012
-
PCR of pET28a+ and peGFP -> annealing temperature 56˚C. non-specific DNA products obtained for the vector. Increase annealing temperature? Gel extract?
+
Symposium with all the dutch iGEM teams at Wageningen University.
 +
No plates for pSB1C3 again.... Noooooooooo!
-
Ladder
+
06/07/2012
-
Original pT28a+
+
Re-transform pSB1C3!
-
Transformed pET28a+ (200 pg DNA for PCR)
+
The overnight culture for BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320 turned pink! What is going on?
-
Transformed pET28a+ (1ng DNA for PCR)
+
At the end of the day -> BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320 both contain RFP......the colonies should be reddish..... Oops....already threw them away. Awwwww start again then!
-
Original peGFP
+
-
Transformed peGFP (200 pg DNA for PCR)
+
-
Transformed peGFP (1 ng DNA for PCR)
+
-
Gel extraction of pET28a+ from TAE gel + ethidium bromide. Elution in 25 µl miliQ water.
+
05/07/2012
-
PCR No. 2 -> pET28a+ and peGFP -> annealing temperature 60˚C.
+
Isolated colonies obtained for BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320.
 +
Set up overnight liquid LB culture for each plasmid for mini-prep.
-
16/05/2012
+
04/07/2012
 +
Plates show growth. Antibiotics are working! Swarming of bacteria. Unusable!
 +
Streak new plates with a single colony to obtain isolated colonies. Incubate overnight at 37˚C.
 +
Nothing grew on the pSB1C3 plate.
 +
 
 +
03/07/2012
 +
Prepared ampicillin and chloramphenicol stock solutions (50 mg/ml).
 +
Made LB/ampicillin and LB/chloramphenicol plates.
 +
Transformation:
 +
1)pSB1AT3+BBa_J45320 (2012 iGEM distribution kit plate 2 Well 5J)
 +
2)BBa_J63009+BBa_J04450 (2012 iGEM distribution kit plate 1 Well 1A)
 +
3)pSB1C3 (2012 iGEM distribution kit linearised plasmid)
 +
Incubate overnight at 37˚C.06/06/2012
 +
Mini-prep of the colony obtained from Gibson on 05/06. Elution in 25µl miliQ water.
 +
Digestion of extracted plasmid with NotI and BglII (double digest).
 +
 
 +
PICTUREEEEEEE
-
pET28a+ (gel extracted)
 
-
peGFP (gel extracted)
 
Ladder
Ladder
-
pET28a+ (PCR No.2 -> 14/05/2012)
+
Mini-prep colony digested with NotI and BglII
-
peGFP (PCR No.2 -> 14/05/2012)
+
-
Still non-specific products observed for the PCR. Possible inter-change during gel extraction; pET28a+ and peGFP got mixed up?
+
05/06/2012
 +
One colony obtained. Checked for fluorescence with GFP. No fluorescence.
 +
Prepared overnight culture with colony for mini-prep.
-
23/05/2012
+
01/06/2012
-
Repeat what was done on 14/05 (PCR Temp 60˚C + gel extraction.
+
Diewertje removed the plates from the incubator and put them at 4˚C for the weekend. Thank you Diewertje!
-
Two products obtained and concentration seems too low. Pfffffff.... Repeat again......And this is only a test, hope it will work better for the actual experiments
+
31/05/2012
-
:(
+
Prepared LB agar for LB plates + Kanamycin.
 +
Gibson assembly of peGFP and pET28a+ in equimolar amounts.
 +
Transformation of 5µl of Gibson reaction mix in DH5 alpha competent bacteria. Incubation overnight at 37˚C.
 +
30/05/2012
 +
Prepared TAE and TBE gels with ethidium bromide.
 +
Pooled all the PCR products for peGFP and gel extract the correct band. Elution in 25µl miliQ water.
-
24/05/2012
+
PICTUUUUREEEE
-
PCR pET28a+ -> annealing temperature 62˚C.
+
Ladder
Ladder
-
pET28a+
+
peGFP after gel extraction
-
 
+
Prepared the master mix for the Gibson assembly. Aliquoted 15µl in eppendorfs.
-
25/05/2012
+
Everything is ready! :)
-
Pooled all the PCR strips containing pET28a+ for DNA precipitation reaction.
+
29/05/2012
29/05/2012
Gel electrophoresis of precipitated DNA pET28a+ from 25/05/2012
Gel electrophoresis of precipitated DNA pET28a+ from 25/05/2012
 +
 +
PICTUUUURE
Ladder
Ladder
Line 69: Line 91:
The pET28a+ is ready for the one step isothermal gibson assembly reaction. peGFP should also be gel extracted.
The pET28a+ is ready for the one step isothermal gibson assembly reaction. peGFP should also be gel extracted.
 +
25/05/2012
 +
Pooled all the PCR strips containing pET28a+ for DNA precipitation reaction.
-
30/05/2012
+
24/05/2012
-
Prepared TAE and TBE gels with ethidium bromide.
+
PCR pET28a+ -> annealing temperature 62˚C.
-
Pooled all the PCR products for peGFP and gel extract the correct band. Elution in 25µl miliQ water.
+
-
 
+
 +
PICTUUUUUREEE
Ladder
Ladder
-
peGFP after gel extraction
+
pET28a+
-
Prepared the master mix for the Gibson assembly. Aliquoted 15µl in eppendorfs.
+
23/05/2012
-
Everything is ready! :)
+
Repeat what was done on 14/05 (PCR Temp 60˚C + gel extraction.
-
31/05/2012
+
PICTUUUUURE
-
Prepared LB agar for LB plates + Kanamycin.
+
-
Gibson assembly of peGFP and pET28a+ in equimolar amounts.
+
-
Transformation of 5µl of Gibson reaction mix in DH5 alpha competent bacteria. Incubation overnight at 37˚C.
+
-
01/06/2012
+
Two products obtained and concentration seems too low. Pfffffff.... Repeat again......And this is only a test, hope it will work better for the actual experiments
-
Diewertje removed the plates from the incubator and put them at 4˚C for the weekend. Thank you Diewertje!
+
:(
 +
16/05/2012
-
05/06/2012
+
PICTUUUURE
-
One colony obtained. Checked for fluorescence with GFP. No fluorescence.
+
-
Prepared overnight culture with colony for mini-prep.
+
-
 
+
-
06/06/2012
+
-
Mini-prep of the colony obtained from Gibson on 05/06. Elution in 25µl miliQ water.
+
-
Digestion of extracted plasmid with NotI and BglII (double digest).
+
 +
pET28a+ (gel extracted)
 +
peGFP (gel extracted)
Ladder
Ladder
-
Mini-prep colony digested with NotI and BglII
+
pET28a+ (PCR No.2 -> 14/05/2012)
 +
peGFP (PCR No.2 -> 14/05/2012)
-
03/07/2012
+
Still non-specific products observed for the PCR. Possible inter-change during gel extraction; pET28a+ and peGFP got mixed up?
-
Prepared ampicillin and chloramphenicol stock solutions (50 mg/ml).
+
-
Made LB/ampicillin and LB/chloramphenicol plates.
+
-
Transformation:
+
-
1)pSB1AT3+BBa_J45320 (2012 iGEM distribution kit plate 2 Well 5J)
+
-
2)BBa_J63009+BBa_J04450 (2012 iGEM distribution kit plate 1 Well 1A)
+
-
3)pSB1C3 (2012 iGEM distribution kit linearised plasmid)
+
-
Incubate overnight at 37˚C.
+
-
04/07/2012
+
14/05/2012
-
Plates show growth. Antibiotics are working! Swarming of bacteria. Unusable!
+
PCR of pET28a+ and peGFP -> annealing temperature 56˚C. non-specific DNA products obtained for the vector. Increase annealing temperature? Gel extract?
-
Streak new plates with a single colony to obtain isolated colonies. Incubate overnight at 37˚C.
+
-
Nothing grew on the pSB1C3 plate.
+
-
05/07/2012
+
PIIICTUUUUUREEEE
-
Isolated colonies obtained for BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320.
+
-
Set up overnight liquid LB culture for each plasmid for mini-prep.
+
-
06/07/2012
+
Ladder
-
Re-transform pSB1C3!
+
Original pT28a+
-
The overnight culture for BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320 turned pink! What is going on?
+
Transformed pET28a+ (200 pg DNA for PCR)
-
At the end of the day -> BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320 both contain RFP......the colonies should be reddish..... Oops....already threw them away. Awwwww start again then!
+
Transformed pET28a+ (1ng DNA for PCR)
 +
Original peGFP
 +
Transformed peGFP (200 pg DNA for PCR)
 +
Transformed peGFP (1 ng DNA for PCR)
-
09/07/2012
+
Gel extraction of pET28a+ from TAE gel + ethidium bromide. Elution in 25 µl miliQ water.
-
Symposium with all the dutch iGEM teams at Wageningen University.
+
PCR No. 2 -> pET28a+ and peGFP -> annealing temperature 60˚C.
-
No plates for pSB1C3 again.... Noooooooooo!
+
-
10/07/2012
+
11/05/2012
-
Set overnight cultures for BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320 for mini-prep.
+
Gel electrophoresis of the PCR reaction performed on 10/05/2012. Non-specific products obtained. Repeat PCR? Change annealing temperature?
-
11/07/2012
+
PICTUUUUUUREEEE
-
Mini-prep BBa_J63009+BBa_J04450 and pSB1AT3+BBa_J45320. Elution in 25µl.
+
-
Restriction digestion of BBa_J63009+BBa_J04450 with DraI and RsaI/XbaI.
+
-
Restriction digestion of pSB1AT3+BBa_J45320 with ScaI and xhoI.
+
-
Something went wrong with the digestions.....
+
-
Transformation:
+
-
1)pSB3C5+ BBa_J04450 (2012 iGEM distribution kit plate 1 Well 3C)
+
-
2)pSB4C5+ BBa_J04450 (2012 iGEM distribution kit plate 1 Well 3E)
+
-
12/07/2012
+
Ladder
-
Transformation of the plasmid containing the M.ScaI methyltransferase (pIDTSMART-AMP).
+
pET28a+ (1 ng for PCR)
 +
pET28a+ (10 ng for PCR)
 +
peGFP (1 ng for PCR)
 +
peGFP (10 ng for PCR)
 +
 
 +
Second PCR for peGFP and pET28a+. annealing temperature = 53˚C
 +
Same results obtained..... :(
</div>
</div>
</div>
</div>
{{Team:Amsterdam/Foot}}
{{Team:Amsterdam/Foot}}

Revision as of 11:04, 26 September 2012