Team:Macquarie Australia/Protocols/GibsonAssembly

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Gibson Assembly Protocol

Before beginning Gibson assembly, all agar plate requirements, concentration calculations and equipment requirements were prepared. Once the gBlocks had arrived Gibson assembly was performed on all fragments.

Each Gene Block fragment was supplied as 200ng and before use it was dissolved in 20µl of TE buffer. The table below shows each tube with vector & volume, volume of Gibson Master Mix, water volume & volume of each gBlock fragment. After incubation, these were transformed into Top10 cells using the Transformation Protocol found here - Transformation Protocol.

5. After addition of all components (shown in table) incubation was preformed at 50°C for 60 min followed.

Element	ChlM	ChlI1	CTH1	POR	ChlG	DVR1	ChlP	ChlI2	Gene	Gene
Fragment 1	3.3uL Gblock1	5.0uL Gblock1	2.3uL Gblock1	4.8uL Gblock1
Fragment 2	3.3uL Gblock2	3.3uL Gblock2	3.2uL Gblock2	3.0uL Gblock2
Fragment 3			3.1uL Gblock3
10X T4 DNA ligase buffer	2 µL
Vector (0.05pmol)	2.7uL	2.7uL	2.7uL	2.7uL	2.7uL	2.7uL	2.7uL	2.7uL	2.7uL	2.7uL
H2O	0.7uL
Gibson Master Mix	10 uL	11 uL	11.3 uL	10.5 uL

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