Team:Nevada/Week 13
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Contents |
August 13
- Joe:
- Primer stock- RFP f-anti
- PCR of [f]SBP-promoter to RFP anti
- Michelle:
- Transformation of Friday’s ligation of SBP (SpeI and PstI)-LRP (PstI and XbaI) digested with
- SpeI and PstI with Terminator (PstI and XbaI) and Promoter (TETrbs) (EcoRI and SpeI) into
- Top 10 competent cells onto KAN plates.
- Miniprep colony M2 from transformation of PCR Fusion SBP (SpeI and PstI)-LRP (PstI and XbaI) followed by PCR ::::purification with glass milk because of mistake in miniprep protocol.
- Nanodrop miniprep of colony M2 PCR Fusion SBP (SpeI and PstI)-LRP (PstI and XbaI) before transforming into BL21 ::::competent cells and onto AMP plates.
- Justin and Dafne
- Culture successful colonies from last weeks ligation in LB-amp until OD reaches 0.6
- Add IPTG in varying concentrations
- Tube 1: 0.01 uM Tube 2: 0.1 uM Tube 3: 1.0 uM Tube 4: 10.0 uM
- After 4 hrs, pellet, place in -80 freezer
- After 8 hrs, pellet, place in -80 freezer
- Transform SBP-B12 with L-arabinose promoter into BL21 cells
- Jeremiah & Chris:
- Miniprep colony 2
- Transform purified plasmid into BL21 expression cells
- Attempt to express the protein while in TOP10 cells using an IPTG gradient
- Took a 3 hour and overnight time point
- Jeremiah & Chris:
- Miniprep colony 2
- Transform purified plasmid into BL21 expression cells
- Attempt to express the protein while in TOP10 cells using an IPTG gradient
- Took a 3 hour and overnight time point
August 14
- Michelle:
- Check yesterday’s transformation of SBP (SpeI and PstI)-LRP (PstI and XbaI) digested
- with SpeI and PstI with Terminator (PstI and XbaI) and Promoter (TETrbs) (EcoRI and
- SpeI).
- Transformation yesterday of colony M2 from transformation of PCR Fusion SBP (SpeI and PstI)-LRP (PstI and XbaI) on :::AMP plates was wrong. Needed to be transformed onto Ampicillin-Chlorophenicol (AMP-CM) plates.
- Re-do transformation into BL21 competent cells onto AMP-CM plates.
- Justin and Dafne:
- Culture SBP-B12 in BL21 cells to an OD of 0.6
- Add concentrations of L-arabinose as done previously, also adding 5 nM Vitamin B-complex
- Take time samples as done above
- Jeremiah & Chris:
- Run the time points on a polyacrylamide gel
August 15
- Michelle:
- Check transformation of colony M2 from transformation PCR Fusion SBP (SpeI and
- PstI)-LRP (PstI and XbaI) with BL21 competent cells on AMP-CM plates.
- Culture smallest colony from this transformation, which we will call M2-BL21 with LB AMP-CM broth.
- Obtain pellet and supernatant preparation from 8ml of colony M2 from transformation of PCR
- Fusion SBP (SpeI and PstI)-LRP (PstI and XbaI) not IPTG induced for Western blot transfer.
- Justin and Dafne:
- Perform western blot analysis of both protein expression experiments
- IPTG unsuccessful, L-arabinose induced SBP-B12 in BL21 cells very successfull
- Jeremiah & Chris:
- Western blot protocol
- Cultured BL21 colony from transformation plate
August 16
- Michelle:
- Western blot transfer continued for pellet and supernatant samples of colony M2 from
- transformation of PCR Fusion SBP (SpeI and PstI)-LRP (PstI and XbaI) not induced with
- IPTG and membrane developed.
August 17
- Jeremiah & Chris:
- Developed western blot of expression in TOP10 cells
- No expression was detected (took pictures of the membranes on my iphone)
- Attempt to express the protein while in BL21 cells using an IPTG gradient
- Took a 3 hour and overnight time point
- Cultured same BL21 colony with thiamine supplement added
- Michelle:
- Western blot transfer of 8ml from culture to obtain pellet and supernatant samples of smallest
- colony from transformation of M2-BL21 from 8/15.
- Jeremiah & Chris:
- Run time points on a polyacrylamide gel (BL21 cells with no thiamine added)
- Attempt to express the protein while in BL21 cells using an IPTG gradient (BL21 cells with thiamine added)
- Took a 3 hour and overnight time point