Back to Golden Gate Protocols
Mix samples well by pipetting, then run the reaction on the thermocycler under the following conditions:
-- Main.KateElston - 29 Jan 2018
Second Stage Assembly
Second Stage assemblies are used to build plasmids out of multiple transcriptional units (Protocol found here). Occasionally this assembly can be used as a second step to building troublesome first stage plasmids - the first stage plasmid is assembled in a high copy/easier to work with backbone then moved to lower copy/more difficult to work with backbone. This assembly makes use of the BsmBI enzyme as described below.Assembly reaction
Access the old non-kit golden gate assembly protocols here Total volume will be 20 μL; you will need 10 fmol of each transcriptional unit plasmid for this assembly. Various backbones are regularly used in this step - if toxicity issues may be a factor, lower copy number vectors are recommended.- 10 fmol of each transcriptional unit/backbone
- 2 μL of 10× T4 DNA ligase buffer (Promega)
- 1 μL of BsmBI
- 1 μL of T4 DNA ligase
- x μL water up to 20 μL total.
Mix samples well by pipetting, then run the reaction on the thermocycler under the following conditions:
| Step | Temperature | Time |
|---|---|---|
| 1 | 42°C | 1.5 min |
| 2 | 16°C | 3 min |
| Cycles 1-2: | Repeat 25x | |
| 3 | 50°C | 5 min |
| 4 | 80°C | 10 min |
- Transform 2 μL assembly reaction and plate recovery on LB + Selective Antibiotic
-- Main.KateElston - 29 Jan 2018
Barrick Lab > BroadHostRangeToolkit > ProtocolsBTKAssembleMultipleTUPlasmid
Contributors to this topic 
KateElston, PatrickLariviere, SeanLeonard, VictorLi
KateElston, PatrickLariviere, SeanLeonard, VictorLiTopic revision: r6 - 2021-11-03 - 19:39:08 - Main.KateElston
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