Transformation of 08/26/13 works. We will do a PCR Colony.

• Well 1 : 6µL DNA ladder
• Well 2 to 7 : 10µL of NirB with RBS-LacZ-Term in pSB1C3 +2µL of 6X loading dye
• Well 8 to 13 : 10µL of NirB with RBS-Amil CP-Term in pSB1C3 +2µL of 6X loading dye
• Well 14 to 19 : 10µL of Pfnr with RBS-LacZ-Term in pSB1C3 +2µL of 6X loading dye
• Well 20 to 25 : 10µL of Pfnr with RBS-Amil CP-Term in pSB1C3 +2µL of 6X loading dye
• Gel : 1%

We obtain fragments at the right size for NirB with RBS-Amil CP-Term in PSB1C3 in well 12, Pfnr with RBS-LacZ-Term in pSB1C3 in well 14, 15, 18 and 19 and Pfnr with RBS-Amil CP-Term in pSB1C3 in well 20, 22 and 25. Nevertheless, electrophoresis shows that these colonies weren't pure. We will purify them by streaking.

Gibson tranformation of the 08/27/13 didn't work. So we did an electrophoresis to check sizes and concentrations of Gibson parts.

• Well 1 : 6µL DNA ladder
• Well 2 : 5µL of PSB1C3+1µL of 6X loading dye
• Well 3 : 5µL of RBS-BphR2 Part I+1µL of 6X loading dye
• Well 4 : 5µL of RBS-FNR Part I+1µL of 6X loading dye
• Well 5 : 5µL of FNR Part I+1µL of 6X loading dye
• Well 6 : 5µL of FNR Part II+1µL of 6X loading dye
• Well 7 : 5µL of BphR2 Part II+1µL of 6X loading dye
• Gel : 1%

We obtain fragment at the right size for RBS-BphR2 Part I, BphR2 Part II, RBS-FNR Part I, FNR Part I, FNR Part II but not for PSB1C3. We will do a digestion of PSB1C3 by DnpI to clean it.

• Well 1 : 6µL DNA ladder
• Well 2 :
• Well 3 : 20µL of PSB1C3 digested by DnpI+4µL of 6X loading dye
• Gel : 1%

We obtain fragment at the right size for PSB1C3. We will purify it. We used an electronic eppendorf gun too fast, some product get up and fill from well 3 to well 4 and 5.