- I've got a clone called M15-pQEC1 (Escherichia coli M15 as a host, pQE-30 as expression vector that carried phaC1 gene). Then I continued with optimization of protein expression condition as below :
(midexponential phase), before induction of 0.01 mM IPTG.
| INCUBATION TEMPERATURE | INDUCTION PERIOD | SAMPLES COLLECTION |
| 37°C | 4 hours | Every hour |
| 30°C | 8 hours | Every 2 hours |
| 28°C | 4 hours | Every hour |
| 24°C | 12 hours | Every 3 hours |
| 20°C | 24 hours | Every 6 hours |
| 15°C | 24 hours | Every 6 hours |
~Extraction of expressed total protein and also solubility test was done in order to determine at
which condition the protein expressed give more soluble form.
2. Co-transformation with chaperon plasmid, pGro7 ( Chloramphenicol for plasmid selection and
L-arabinose for induction of chaperone expression ) in order to improve protein solubility. I've
called this clone as M15-pQEC1/pGro7. Optimization of protein expression was done with same
condition as above.
~I found that induction at 28°C give more soluble form compared with other induction temperature.
While M15-pQEC1/pGro7 give better result than M15-pQEC1
3. Purification using Metal Affinity Chromatography - only done with soluble fraction of the protein.
4. Bovine Serum Albumin (BSA) Standard Curve was done for determination of protein
concentration . Based on the standard curve..I managed to get about 0.6 mg/ml protein.
This concentration of protein did not good enough for crystallization screening.
*Current work : Optimising the process to obtain sufficient sample to be screened for crystallisation conditions
p/s:I'll update more.......
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