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Team:HokkaidoU Japan/Notebook/September3
From 2010.igem.org
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| - | =1- | + | =PCR of 1-3A= |
| - | 1- | + | |
| - | + | Transformation of 1-3A part which is originaly on pSB1C3 was succesful<br> | |
| + | Thinking that linearized vector might gone bad we PCRed pSB1C3 from 1-3A | ||
| + | |||
{|style="text-align:center;" class="protocol" | {|style="text-align:center;" class="protocol" | ||
!Reagent | !Reagent | ||
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| - | * | + | * Extension was for120 sec |
| - | * YM- | + | * Purified via Microcon YM-10 |
| + | * Final volume was 43 uL | ||
Revision as of 17:34, 27 September 2010
since 13 Jul 2010
since 1 Aug 2010
Resultsof yesterdays trnsformation
- pSB1C3 uterly failed to produce colonies
- pUC119 produced 20 colonies
- colonies that should been red because of RFP insert wasn`t, so there is posibility that insert wasn`t there
Colony PCR on yesterdays E.coli
- Colony PCR was done acordig to protocol
- This day we did 20 samples
Electrophoresis
Concentration check of parts used for transformation yesterday
Confirmed that DNA solution concentration of parts for Ligation was as anticipated (good?)
| Lane | DNA |
| 1 | |
| 2 | Lambda/Hind III, EcoR I |
| 3 | |
| 4 | RFP |
| 5 | pUC119 |
| 6 | pSB1C3 |
PCR of 1-3A
Transformation of 1-3A part which is originaly on pSB1C3 was succesful
Thinking that linearized vector might gone bad we PCRed pSB1C3 from 1-3A
| Reagent | Amount |
|---|---|
| 1-3A | 1 |
| DW | 33 |
| 10x Buffer | 5 |
| 2 M 4dNTPs | 5 |
| 25 mM MgSO4 | 3 |
| Suffix-F | 1 |
| Prefix-R | 1 |
| KOD | 1 |
| Total | 50 uL |
- Extension was for120 sec
- Purified via Microcon YM-10
- Final volume was 43 uL
