Difference between revisions of "Team:KAIT Japan/Notebook"
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| − | < | + | <br><font size="5"> |
| − | </ | + | 6/22~7/24:PCR(Dronpa145N,Dronpa145K)<br> |
| + | 7/25~7/28:Digested PCR Product of Dronpa 145N,K(6/22) and pCold Vector<br> | ||
| + | 7/29~7/31:Ligation (Dronpa145N +pCold Vector),and transformation the ligation product.<br> | ||
| + | 8/1:Get three clonies that brite under UV light, pick up these colonies and incubate in liquide culuture<br> | ||
| + | 8/2:Miniprep the clones and digest plasmids to confirm we get correct clones<br> | ||
| + | 8/3:purified plasmid(Dronpa 145N+pCold)<br> | ||
| + | 8/4:transform RFP to Ecoli<br> | ||
| + | 8/5:Glycerol stock clones that have plasmid(Dronpa 145N+pcold)<br> | ||
| + | 8/6:digested PCR Product of Dronpa 145N,K(7/29) by EcorⅠand PstⅠ<br> | ||
| + | 8/7:After miniprep RFP clone, Digested the plasmid (RFP+pSB1C3) by EcoRⅠand PstⅠ,Ligation (pSB1C3+Dronpa 145N,K),transform the ligation product to Ecoli<br> | ||
| + | 8/8~8/12:incubated clones (pCold+Dronpa145N) to exprese Dronpa 145N<br> | ||
| + | 8/13~8/14:digested plasmid (pCold+Dronpa145N) by EcoRⅠ and XhoⅠ<br> | ||
| + | 8/15~8/18:digested Dronpa 145K by EcorⅠand PstⅠ,inserted into pCold vector by ligase,transform it into Ecoli<br> | ||
| + | 8/19~8/22:ligation (pCold vector+Dronpa145Nand Dronpa145N),and transformation the ligation product.<br> | ||
| + | 8/23:digested purifyide plsmid to check insert,we are not able to get good result ,try again<br> | ||
| + | 8/24~8/25:digested Dronpa145N by EcoRⅠ and, XhoⅠ,ligation (pCold vector+Dronpa145Nand Dronpa145N),and transformation the ligation product.<br> | ||
| + | 8/26:colony PCR<br> | ||
| + | 8/27:<br> | ||
| + | 8/28~8/29:<br> | ||
| + | 8/30:<br> | ||
| + | 8/31:<br> | ||
| + | 9/1:<br> | ||
| + | 9/2:<br> | ||
| + | 9/3:<br> | ||
| + | 9/4:<br> | ||
| + | 9/5:<br> | ||
| + | 9/6:<br> | ||
| + | 9/7:<br> | ||
| + | 9/8~9/10:<br> | ||
| + | <br> | ||
| + | <br> | ||
| + | <br> | ||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | </font> | ||
Revision as of 04:42, 18 September 2015
Lab note
6/22~7/24:PCR(Dronpa145N,Dronpa145K)
7/25~7/28:Digested PCR Product of Dronpa 145N,K(6/22) and pCold Vector
7/29~7/31:Ligation (Dronpa145N +pCold Vector),and transformation the ligation product.
8/1:Get three clonies that brite under UV light, pick up these colonies and incubate in liquide culuture
8/2:Miniprep the clones and digest plasmids to confirm we get correct clones
8/3:purified plasmid(Dronpa 145N+pCold)
8/4:transform RFP to Ecoli
8/5:Glycerol stock clones that have plasmid(Dronpa 145N+pcold)
8/6:digested PCR Product of Dronpa 145N,K(7/29) by EcorⅠand PstⅠ
8/7:After miniprep RFP clone, Digested the plasmid (RFP+pSB1C3) by EcoRⅠand PstⅠ,Ligation (pSB1C3+Dronpa 145N,K),transform the ligation product to Ecoli
8/8~8/12:incubated clones (pCold+Dronpa145N) to exprese Dronpa 145N
8/13~8/14:digested plasmid (pCold+Dronpa145N) by EcoRⅠ and XhoⅠ
8/15~8/18:digested Dronpa 145K by EcorⅠand PstⅠ,inserted into pCold vector by ligase,transform it into Ecoli
8/19~8/22:ligation (pCold vector+Dronpa145Nand Dronpa145N),and transformation the ligation product.
8/23:digested purifyide plsmid to check insert,we are not able to get good result ,try again
8/24~8/25:digested Dronpa145N by EcoRⅠ and, XhoⅠ,ligation (pCold vector+Dronpa145Nand Dronpa145N),and transformation the ligation product.
8/26:colony PCR
8/27:
8/28~8/29:
8/30:
8/31:
9/1:
9/2:
9/3:
9/4:
9/5:
9/6:
9/7:
9/8~9/10:
Link list
Sponsor
