Team:Cambridge/Gibson/Protocol
From 2010.igem.org
Gibson Assembly: Protocols
Step 1) Design Primers
- If you wish to ligate two pieces of DNA using Gibson they must be altered so as to have 40bp of overlap with respect to each other.
//Insert diagram of two pieces of DNA with overlap
- The standard way to do this is with PCR with specialised primers
- We have designed a tool to help you do this: [http://www.gibthon.org Gibthon]
Master mix
Volume/µl | |
Taq ligase (40u/µl) | 50 |
5x isothermal buffer | 100 |
T5 exonuclease (1u/µl) | 2 |
Phusion polymerase (2u/µl) | 6.25 |
Nuclease-free water | 216.75 |
=375 |