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Team:Groningen/Notebook/Wetwork 23July2012
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| - | Plasmid isolation pSB1C3-alsT promoter + GFP | + | Tom and Arjan started with gas chromatography mass spectrometry. Test sample: 5gr. fresh meat incubated @ 37C for 3 houres. For both column (HP5 and CP wax) three runs on each column with different incubation and syringe temperature (1: 80C, 100C 2: 100C, 120C 3: 120C, 140C)<br> |
| - | + | <br> | |
| - | NanoDrop result (ng/ul): | + | <br> |
| - | + | Nisa<br> | |
| - | A1= 102.9 | + | <br> |
| - | + | Plasmid isolation pSB1C3-alsT promoter + GFP<br> | |
| - | A2= 96,6 | + | <br> |
| - | + | NanoDrop result (ng/ul):<br> | |
| - | B1= 118,1 | + | A1= 102.9<br> |
| - | + | A2= 96,6<br> | |
| - | B2= 113,7 | + | B1= 118,1<br> |
| - | + | B2= 113,7<br> | |
| - | C1= 122,8 | + | C1= 122,8<br> |
| - | + | C2= 88 Comment: gel picture OK!<br> | |
| - | C2= 88 Comment: gel picture OK! | + | D1= 124,9<br> |
| - | + | D2= 93,3<br> | |
| - | D1= 124,9 | + | <br> |
| - | + | Result:<br> | |
| - | D2= 93,3 | + | expected size: 3300bp for the pSB1C3 (2079bp)+ alsT (~500bp)+ GFP (800bp)<br> |
| - | + | <br> | |
| - | + | From the gel picture, only plasmid from colony C2 (promoter alsT300) showed the expected size. The other plasmids seem to be empty, probably due to self ligation.<br> | |
| - | Result: | + | <br> |
| - | + | Solution: Check plasmid from other white colony<br> | |
| - | expected size: 3300bp for the pSB1C3 (2079bp)+ alsT (~500bp)+ GFP (800bp) | + | <br> |
| - | + | re do transformation. Increase the ratio of plasmid backbone: insert gene<br> | |
| - | From the gel picture, only plasmid from colony C2 (promoter alsT300) showed the expected size. The other plasmids seem to be empty, probably due to self ligation. | + | <br> |
| - | + | <br> | |
| - | Solution: Check plasmid from other white colony | + | Building backbone biobrick for B.subtilis<br> |
| - | + | <br> | |
| - | re do transformation. Increase the ratio of plasmid backbone: insert gene | + | plasmid pSac-Cm: integration plasmid, double cross over in SacA region<br> |
| - | + | <br> | |
| - | + | add double terminator, BBa_B0015, and prefix-suffix: XbaI, SpeI, PstI<br> | |
| - | Building backbone biobrick for B.subtilis | + | <br> |
| - | + | <br> | |
| - | plasmid pSac-Cm: integration plasmid, double cross over in SacA region | + | How to? <br> |
| - | + | <br> | |
| - | add double terminator, BBa_B0015, and prefix-suffix: XbaI, SpeI, PstI | + | Cut backbone with HindIII and EcoRI<br> |
| - | + | <br> | |
| - | + | Cut BBa_B0015 with HindIII and EcoRI<br> | |
| - | How to? | + | <br> |
| - | + | Now we have separate parts ready to use for ligation into our biobrick device<br> | |
| - | Cut backbone with HindIII and EcoRI | + | <br> |
| - | + | <br> | |
| - | Cut BBa_B0015 with HindIII and EcoRI | + | |
| - | + | ||
| - | Now we have separate parts ready to use for ligation into our biobrick device | + | |
| - | + | ||
| - | + | ||
| - | < | + | |
<A HREF="https://2012.igem.org/Team:Groningen/Notebook"><FONT COLOR=#ff6700>Back to notebook</FONT></A> | <A HREF="https://2012.igem.org/Team:Groningen/Notebook"><FONT COLOR=#ff6700>Back to notebook</FONT></A> | ||
| - | </html> | + | <br><br></p></body></html> |
{{Template:SponsorsGroningen2012}} | {{Template:SponsorsGroningen2012}} | ||
Latest revision as of 21:20, 25 September 2012
Tom and Arjan started with gas chromatography mass spectrometry. Test sample: 5gr. fresh meat incubated @ 37C for 3 houres. For both column (HP5 and CP wax) three runs on each column with different incubation and syringe temperature (1: 80C, 100C 2: 100C, 120C 3: 120C, 140C)
Nisa
Plasmid isolation pSB1C3-alsT promoter + GFP
NanoDrop result (ng/ul):
A1= 102.9
A2= 96,6
B1= 118,1
B2= 113,7
C1= 122,8
C2= 88 Comment: gel picture OK!
D1= 124,9
D2= 93,3
Result:
expected size: 3300bp for the pSB1C3 (2079bp)+ alsT (~500bp)+ GFP (800bp)
From the gel picture, only plasmid from colony C2 (promoter alsT300) showed the expected size. The other plasmids seem to be empty, probably due to self ligation.
Solution: Check plasmid from other white colony
re do transformation. Increase the ratio of plasmid backbone: insert gene
Building backbone biobrick for B.subtilis
plasmid pSac-Cm: integration plasmid, double cross over in SacA region
add double terminator, BBa_B0015, and prefix-suffix: XbaI, SpeI, PstI
How to?
Cut backbone with HindIII and EcoRI
Cut BBa_B0015 with HindIII and EcoRI
Now we have separate parts ready to use for ligation into our biobrick device
Back to notebook
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