Team:ZJU-China/Notebook/LabNotes/September

From 2013.igem.org

Revision as of 09:53, 27 September 2013 by Jinhuang (Talk | contribs)

(diff) ← Older revision | Latest revision (diff) | Newer revision → (diff)

Lab Notes

May June July August September

Protocol

Brainstorm

The "Elf"

Background Design Results Perspetives

Lab Notes: September

Date	Notes
Sept 1	PCR amplifications of lgt, DsbA-BLF1, DsbA-BLF2, addA stand, pSB1C3 linear backbone, GFP double terminator, and atrazine stand.
Sept 2	Cut BBa_K411003 with E+P. Make up new competent cells with LB and glycerin. Transformation with parts in iGEM kits (BBa_K091111, BBa_K091112 in 2012 distribution, and BBa_K091112 in 2011 distribution).
Sept 3	PCR amplification of theo-stand, atw-stand, DsbA-FA-lgt, DsbA-FB-lgt, and GFP with terminator.
Sept 4	Find that the transformation of lacIq and placIQ1 are both successful. Receive plasmids with TrzN degradation gene from NJU.
Sept 5	PCR amplification of RFP, antiholin, Trz N, holing, BLF1, and BLF2. Small-scale plasmid purification of cheZ and pSB1A3.
Sept 6	Small-scale plasmid purification of FA, ribo-cheZ, and atr riboswitch. Cut PE and kanamycin with X+P.
Sept 7	PCA of FB, BLF1, BLF2, and cheZ-RFP-antiholin. CPEC of DsbA-FA-lgt. Direct CPEC of DsbA-FA-lgt, DsbA-FB-lgt, DsbA-BLF1-lgt, DsbA-BLF2-lgt, and cheZ-RFP-antiholin.
Sept 8	PCR amplification of lgt and DsbA-BLF1. CPEC of ptactamaze-lgt complex.
Sept 9	PCR of holing, BLF2, theo, lact, and FB.
Sept 10	Pick up and test four colonies of the UC Davis strain, and inoculate to LB medium. PCR amplification of BLF1-pSB1C3 and FB.
Sept 11	New method: cover E. coli with calcium carbonate and calcium acid phosphate shell (safety issues). Find that E. coli in such shell can express GFP. PCR verification of anti-Dter, BLF1, BLF2.
Sept 12	Redo some steps of yesterday’s PCR.
Sept 13	Cut and link pluxR and cheZ; PCR clean-up. Small-scale plasmid purification of holin and K (mutant). Cut RFP with E+X, pluxR-cheZ with E+S.
Sept 14	PCR amplification of BLF1, PCA-theo, and PCA-addA. Cut pSB1CB and BLF1 with E+B.
Sept 15	Link pluxR-cheZ-RFP and BLH-pSB1C3. Transform addA, FA, FB, BLF1, BLF2, β-tactamase, and BLF1-1C3. Help UC Davis do transform works of three promoters in 2012 kit (BBa_J23108, BBa_J23109, and BBa_J23111).
Sept 16	Pick up monoxenie of B. subtilis and inoculate.
Sept 17	Find that the transformation of 2012 kit was failed. 3A assembly of luxR-cheZ, RFP, and pSB1A3.
Sept 18	Cut II with N+X, III with N+P. PCR amplification of cheZ, I, lgt, and lgt-RAW.
Sept 19	Mid-autumn festival. One-day holiday!
Sept 20	PCR amplification of lgt-RAW, BBa_K411003, lgt-S, and shrep-back.
Sept 21	Pick up five tubes of colonies and do PCR. Run gel, take photo (on computer). Transform K into BL21 (kanamycin resistance). Transform three parts again for UC Davis.
Sept 22	Pick up two tubes of Theo Ribo, Atra Ribo, and A+ each and put in shaker in 37°C. PCR amplification of FA, FB, I, and lgt-RAW.
Sept 23	Redo some steps of PCR yesterday.
Sept 24	Find that the transformation of FB2 was failed, and FB1 successful. Cut to verify FB1 and lgB1.
Sept 25	Measure the concentration curve of E. coli. Make up new Amp and Chl solution. Pick up three tubes of colonies with holin.

Previous: Lab Notes: August

Next: Protocol