Team:Wash U/Protocol
From 2009.igem.org
(Difference between revisions)
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:1. Begin by thawing the upstream, downstream, and destination plasmid parts along with the NEBuffer 2 and BSA.<br> | :1. Begin by thawing the upstream, downstream, and destination plasmid parts along with the NEBuffer 2 and BSA.<br> | ||
:2. In three separate PCR microcentrifuge tubes labeled upstream, downstream, and destination, add 500ng of the respective dried DNA and dilute with dH20 to 42.5 uL.<br> | :2. In three separate PCR microcentrifuge tubes labeled upstream, downstream, and destination, add 500ng of the respective dried DNA and dilute with dH20 to 42.5 uL.<br> | ||
- | :3. Add 5 uL of NEBuffer 2 and 0.5 uL of BSA to | + | :3. Add 5 uL of NEBuffer 2 and 0.5 uL of BSA to each tube.<br> |
:4. Add 1 uL of the first appropriate enzyme to each tube. Then add 1 uL of the second appropriate enzyme.<br> | :4. Add 1 uL of the first appropriate enzyme to each tube. Then add 1 uL of the second appropriate enzyme.<br> | ||
:5. Flick each tube to mix reagents and incubate at 37C for 15 minutes.<br> | :5. Flick each tube to mix reagents and incubate at 37C for 15 minutes.<br> |
Revision as of 16:18, 6 July 2009