Refolding Record:
Protein | |
---|---|
Protein Name | Ribonuclease A |
Abbreviated Name | RNase A |
SCOP Family | Ribonuclease A-like |
Structure Notes | |
Organism | Human |
UniProt Accession | P07998 |
SCOP Unique ID | n/a |
Structure Solved | |
Class | Alpha+Beta |
Molecularity | Monomer |
Construct | |
---|---|
Full Length | n |
Domain | HuS, aa.18-125 |
Chimera | n/a |
Variants | P19A, S20A |
Chain Length | 109 |
Molecular Weight | 12299.9 |
Pi | 8.85 |
Molecular Weight | 12299.9 |
Disulphides | 4 |
Full Sequence |
MSAASS STYCNQMMRR RNMTQGRCKP VNTFVHEPLV DVQNVCFQEK VTCKNGQGNC YKSNSSMHIT DCRLTNGSRY PNCAYRTSPK ERHIIVACEG SPYVPVHFDA SVE
|
Notes | P19A and S20A mutations to increase protein yield |
Expression | |
---|---|
Report | Backer MV, Gaynutdinov TI, Gorshkova II, Crouch RJ, Hu T, Aloise R, Arab M, Przekop K, Backer JM (2003) J Controlled Release, 89, 499-511 |
Project Aim | Drug Studies |
Fusion | None |
Protein Expression and Production | Protein recombinantly expressed as and refolded from inclusion bodies. |
Expression Host | Escherichia coli |
Expression Strain | OrigamiB(DE3)pLacI |
Expression Temp | 37.0 |
Expression Time | 12-16h |
Expression Vector | pET29a(+) |
Expression Protocol | Cells were grown in Circle Grow medium (Q-Biogen), expression was induced with 1mM IPTG when OD600 reached 0.5-0.7. Cells were grown overnight at 37degC then harvested by centrifugation (15min x 5000g). |
Method of Induction | IPTG |
Cell Density at Induction | OD 600 = 0.5-0.7 |
Cell Disruption Method | Sonication |
Lytic Agent | None |
Pre-Refolding Purification | None |
Solubility | not stated |
Refolding | |
---|---|
Refolding Method | Dilution |
Wash Buffer | BugBuster (Novagen)/CelLytic B (Sigma), HisBind buffer (Novagen) |
Solubilization Buffer | 20mM TrisHCl, 100mM NaCl, 8M Urea pH 8.0 |
Refolding Buffer | 100mM Tris-Acetate, 100mM NaCl, 0.5M arginine, 1mM GSH, 0.4mM GSSG pH 8.6 |
Pre-Refolding Purification | None |
Tag Cleaved | yes |
Refolding pH | 8.6 |
Refolding Temperature | 25.0 |
Protein Concentration | n/a |
Refolding Time | n/a |
Redox Agent | GSH/GSSG |
Redox Agent Concentration | 1mM/0.4mM |
Refolding Protocol | The cells were lysed using BugBuster reagent according to the manufacturer instructions of the manufacturer. The inclusion bodies were were centrifuged and washed with BugBuster reagent, followed by CelLytic B reagent (Sigma) diluted 1:10 with water, and then finally 1x HisBind buffer (Novagen). The concentration of protein was determined by RP HPLC. Synthetic peptide (aa.18-125 or was aa.18-127) was added to the solubilized inclusion bodies at a molar ratio of 2:1 peptide:protein. The protein/peptide mixture was then refolded in refolding buffer and then purified using ion-exchange chromatography and RP HPLC. |
Refolding Assay | Bioactivity |
Refolding Chaperones | None |
Refolding Additives | None,L-Arginine |
Additives Concentration | 0.5M |
Refolding Yield | n/a |
Purity | n/a |
Notes | n/a |