IGEM:Harvard/2006/Cyanobacteria/Notebook/2006-8-12: Difference between revisions
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==To-do== | |||
* RFP in low-copy plasmid (transformed in Top10 and Top10F') | |||
** Colony PCR the J04450 + pSB4A3 colonies with BB primers to test if our ligation worked | |||
** Inoculate liquid cultures with these colonies | |||
* GFP dev in low-copy plasmid (from digest assay) | |||
==Results of Restreak of J00450+PSB4A3== | ==Results of Restreak of J00450+PSB4A3== | ||
[[Image:Restreak 81206 zs.jpg]] | [[Image:Restreak 81206 zs.jpg]] | ||
Revision as of 12:58, 12 August 2006
To-do
- RFP in low-copy plasmid (transformed in Top10 and Top10F')
- Colony PCR the J04450 + pSB4A3 colonies with BB primers to test if our ligation worked
- Inoculate liquid cultures with these colonies
- GFP dev in low-copy plasmid (from digest assay)
Results of Restreak of J00450+PSB4A3
Although the colonies took two days to grow, the restreak of the plates on Carb worked; we will now verify the ligation via PCR while growing liquid culture from them.
PCR ligation test of J04450+PSB4A3
Following Perry's Protocol which worked pretty well, in order to check the ligation we will do a PCR using the PCR Supermix from the VF2 and VR areas of the plasmid;
From the above image, we will try 7 colonies:
- Top10 plate2 A (eg. 102)
- Top10 plate1 A (eg. 101)
- Top10F plate1 (eg. F1)
- Top10F plate2 1 (eg. F2-1)
- Top10F plate2 2 (eg. F2-2)
- Top10F plate2 3 (eg. F2-3)
- Top10F plate2 3 (eg. F2-4)
From Perry's Protocol, each will have:
- 8uL PCR supermix
- 1uL VF2 (2uM)
- 1uL VR (2uM)
Then, get a carb plate, pick the desired colony, streak it on the plate, and then dip it into the 10uL rxn.
