Team:Hawaii/Notebook/2008-10- 9
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:* Restreaked original colonies #1, 3, 13, 18 on freshly made LB+sp<sub>100</sub>+sm<sub>100</sub> | :* Restreaked original colonies #1, 3, 13, 18 on freshly made LB+sp<sub>100</sub>+sm<sub>100</sub> | ||
::* Original colonies scraped w/ loop. Hopefully there's something there. | ::* Original colonies scraped w/ loop. Hopefully there's something there. | ||
+ | |||
+ | ===Made 5%LB+BG-11 and BG-11+sp<sub>2.5</sub>+sm<sub>2.5</sub> plates=== | ||
+ | :<strong>Grace and Krystle</strong> | ||
+ | |||
+ | ===Construction of plasmid=== | ||
+ | :<strong>margaret</strong> | ||
+ | [[Image:rep_aadA_purification_10_9.jpg|right|thumb|300px|plac/rbs/rep5 (E,S), plac/rbs/rep7 (E,S), plac/rbs/aada (ap32 E,S), plac/rbs/aada ap2 cut with X,P.]] | ||
+ | :* Gel purification of re-digest | ||
+ | ::*plac/rbs/aada (ap32 was cut with E,S), ap2 did not cut correctly | ||
+ | ::*plac/rbs/rep (7 was cut with E,S), rep5 did not cut correctly | ||
+ | :*Ligation, transformation (in DH5 alpha): | ||
+ | ::*oriT + plac/rbs/aada + pSB1A3 (dephosphorylated) | ||
+ | ::*oriV + plac/rbs/rep + pSB1A3 (dephosphorylated) | ||
+ | ::pSB1A3 (dephosphorylated) + self | ||
+ | ::*(+) control for transformation- pUC18 | ||
+ | ::*(-) control for transformation- no plasmid | ||
+ | |||
+ | ===OriV back-ups=== | ||
+ | :<strong>margaret</strong> | ||
+ | [[Image:oriv_verification_10_9.jpg|right|thumb|300px|Verification of oriV transformation.]] | ||
+ | :* two colonies were of correct size from yesterday's transformation, so i did a plasmid prep of them and I will store them in -20 C in TE | ||
= Discussion = | = Discussion = |
Latest revision as of 23:44, 11 October 2008
Projects | Events | Resources | ||
---|---|---|---|---|
Sponsors | Experiments | Milestones | Protocols | |
Notebook (t) | Meetings (t) |
Things we did today
Wetlab work
Construction of secretion device (cont.)
- Grace
- Ran RE digests on gel
- Extracted bands from gel
- Ligated:
- J33207 and pRL1383a
- nir and rbs+GFPf+tt #1 and pSB1A3
- plac and rbs+GFPf+tt #1 and pSB1A3
- nir+rbs and slr1+GFPf and pSB1A3
- nir+rbs and pilA+GFPf+tt and pSB1A3
- Used 5 μl ligation reaction to transform DH5α
Sequencing
- Grace
- Prepared and sent samples in for sequencing:
- pilA+GFPf+tt #21 (KS)
- nir+rbs+slr1+GFPf #15 (10/2 transformation)
- slr1+GFPf+tt (10/2 transformation)
- nir+rbs+slr1+GFPf #6 (10/8 transformation)
- plac+rbs+pilA+GFPf+tt #5, 7, 11 (10/8 transformation)
Triparental conjugtion
- Grace
- BBpRL #1, 18 cultures did not grow
- PCR of colonies (on Xgal plate) showed no insert present (?!?)
- PCR of colonies from non-Xgal plate) showed no insert present (?!?)
- Faint band for colonies #1, 13 at 400bp ???
- Restreaked original colonies #1, 3, 13, 18 on freshly made LB+sp100+sm100
- Original colonies scraped w/ loop. Hopefully there's something there.
Made 5%LB+BG-11 and BG-11+sp2.5+sm2.5 plates
- Grace and Krystle
Construction of plasmid
- margaret
- Gel purification of re-digest
- plac/rbs/aada (ap32 was cut with E,S), ap2 did not cut correctly
- plac/rbs/rep (7 was cut with E,S), rep5 did not cut correctly
- Ligation, transformation (in DH5 alpha):
- oriT + plac/rbs/aada + pSB1A3 (dephosphorylated)
- oriV + plac/rbs/rep + pSB1A3 (dephosphorylated)
- pSB1A3 (dephosphorylated) + self
- (+) control for transformation- pUC18
- (-) control for transformation- no plasmid
OriV back-ups
- margaret
- two colonies were of correct size from yesterday's transformation, so i did a plasmid prep of them and I will store them in -20 C in TE
Discussion
Quote of the Day
History is the only laboratory we have in which to test the consequences of thought. - Étienne Gilson
[http://manoa.hawaii.edu/ ][http://manoa.hawaii.edu/ovcrge/ ][http://www.ctahr.hawaii.edu ]