Contents 1 208 lab 1.1 Main purposes today 1.2 who were in the lab 1.3 Procedure 1.4 Results 1.5 Conclusion from today

208 lab

---

Main purposes today

---

New PCR with x7-polymerase.

who were in the lab

---

Kristian

Procedure

---

Made PCRs on pZA21, GFP SF TAT, GFP SF Sec and RFP all samples where made in duplicates.

In tube 1+2+3+4+5+6 where pZA21. In 7+8+9+10+11+12 GFP SF TAT In 13+14+15+16+17+18 GFP SF Sec In 19+20+21+22+23+24 RFP

First program was 45°C annealing and 2:00 extension time with tube: 1+2, 7+8, 13+14, 19+20. Second program was ramp 68°C → 60°C annealing and 2:00 extension time with tube: 3+4, 9+10, 15+16, 21+22. Last program was a touch up program with 60°C annealing and 10 cycles with a temperature increment of 0.5°C per cycle this was looped 5 times so the final amount of annealing cycles was 50. Extension time was still 2:00 and this program was done on tube: 5+6, 11+12, 17+18, 23+24.

Purification was done by gel purification, see picture below.

After all PCR-products were purified the backbone was prepared for DpnI treatment and the right amount of each of the other PCR-products were mixed. Finally the DpnI treated backbone was added USER-enzyme and BSA, mixed with the appropriate PCR-products and set for reaction.

The constructs were transformed into chemical competent E.coli right after construction and incubated 2 hours in SOC before plated on Kana plates.

Results

---

Conclusion from today

---

All PCR-products have been made and the programs for each product have been determined. Navigate to the Previous or the Next Entry