• Well 1 : 6µL DNA Ladder
• Well 2 : 5µL of BBa_K1155006 digested by EcoRI/SpeI+1µl of 6X loading dye
• Well 3 : 5µL of BBa_K1155005 digested by EcoRI/SpeI+1µl of 6X loading dye
• Well 4 : 5µL of BBa_K1155004 digested by EcoRI/SpeI+1µl of 6X loading dye
• Gel : 1%

We obtained NarK, NarG, NirB fragments at the right size but in very few quantity. We do it again but this time we will use more quantity of enzymes AND ADN ?!??????????

• Well 1 : 5µL of BBa_K1155000 digested by SpeI+1µl of 6X loading dye
• Well 2 : 5µL of BBa_K1155006 digested by SpeI+1µl of 6X loading dye
• Well 3 : 5µL of BBa_K1155005 digested by SpeI+1µl of 6X loading dye
• Well 4 : 5µL of BBa_K1155004 digested by SpeI+1µl of 6X loading dye
• Well 5 : 6µL DNA Ladder
• Well 6 : 5µL of BBa_K1155000 digested by EcoRI/SpeI+1µl of 6X loading dye
• Well 7 : 5µL of BBa_K1155006 digested by EcoRI/SpeI+1µl of 6X loading dye
• Well 8 : 5µL of BBa_K1155005 digested by EcoRI/SpeI+1µl of 6X loading dye
• Well 9 : 5µL of BBa_K1155004 digested by EcoRI/SpeI+1µl of 6X loading dye
• Gel : 1%

Well 1 : we have done one digestion so we have to obtain one fragment, we have two stripes, the digestion of Bba_K1155000 by SpeI wasn't good. Well 2, 3, 4, 6, 7 : we obtain NarG, NarK and NirB in PSB1C3 and Pfnr, NarK fragments at the right size, we can purify it. Well 8, 9 : we have done two digestions so we have to obtain two fragments, we have only one stripe, the digestion of Bba_K1155005 and Bba_K1155004 by EcoRI/SpeI wasn't good.

Picture : Electrophoresis gel of the digestion of Bba_K1155000, Bba_K1155004,Bba_K1155005, Bba_K1155006 by SpeI and EcoRI/SpeI The cutting for the gel purification was good.

CONCLUSION