11/16/12
- ---Karmella 13:51, 16 November 2012 (EST): Here is my suggested procedure for trying the PcTF fusion cloning...
Assemblies: Shown as Part/cuts/purified fragment size
- KAH109/pT7CFE1-CHis: KAH109/(E/P)/1132 + pT7CFE1-CHis/(E/P)/3600
- KAH111/pT7CFE1-CHis: KAH184/(E/S)/1123 + "
- KAH112/pT7CFE1-CHis: KAH187/(E/S)/1123 + "
- KAH115/pT7CFE1-CHis: KAH188/(E/S)/931 + "
- KAH148/pT7CFE1-CHis: KAH189/(E/S)/967 + "
- KAH150/pT7CFE1-CHis: KAH190/(E/S)/967 + "
- KAH151/pT7CFE1-CHis: KAH191/(E/S)/967 + "
Note: KAH109 is being re-done as an internal control to trouble-shoot the ligation
Note: KAH111-KAH151 are all cut and purified already
> Digest (Fermentas FD)
- pT7CFE1-CHis, E/P
| Reagent | Volume |
|
|
| DNA (plasmid) | 25.0 μL
|
| 10x buffer | 3.0
|
| EcoRI | 1.0
|
| PstI | 1.0
|
| dH2O | 0
|
| | 30 μL --> 37°C/ ~30 min.
|
> Measure concentration(s)
| Sample | OD260 | 260/280 | ng/μL
|
| 1. pT7CFE1-CHis (E/P) | --- | --- | ---
|
> Ligations (trouble shooting suggestions)
- Note: Use 50 ng of vector this time (instead of 20)
- Note: Use a 3:1 ratio of insert to vector... x μL insert = 3 * (bp of insert/ bp of vector) * 50 ng vector / (concentration of insert ng/μL)
| | 1 | 2 |
|
| Insert DNA | 3.5 | --- |
|
| Vector DNA | 0.5 | 0.5 |
|
| 2x lgn buf (Roche) | 5.0 | 5.0 |
|
| T4 ligase (NEB) | 1.0 | 1.0 |
|
| dH2O | --- | 3.5 |
|
| | 10 μL | 10 μL |
|
|
PcTF Subcloning in E. coli
Main project page
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