Refolding Record:
Protein | |
---|---|
Protein Name | HIV protease |
Abbreviated Name | HIV-PR |
SCOP Family | Retroviral protease (retropepsin) |
Structure Notes | |
Organism | HIV |
UniProt Accession | P03366 |
SCOP Unique ID | n/a |
Structure Solved | |
Class | Beta |
Molecularity | Dimer |
Construct | |
---|---|
Full Length | n |
Domain | n/a |
Chimera | tethered dimer: protease domains tethered head-to-tail |
Variants | D25G in first protease domain |
Chain Length | 273 |
Molecular Weight | 29646.3 |
Pi | 8.69067 |
Molecular Weight | 29646.3 |
Disulphides | 0 |
Full Sequence |
MEFMEDLAFL QGKAREFSSE QTRANSPTIS SEQTRANSPT RRELQVWGRD NNSPSEAGAD RQGTVSFNFP
VTLWQRPLV TIKIGGQLKE ALLGTGADDT VLEEMSLPGR
WKPKMIGGIG GFIKVRQYDQ ILIEICGHKA IGTVLVGPTP VNIIGRNLLT QIGCTLNFPI GGSSG VTLWQRPLV TIKIGGQLKE ALLDTGADDT VLEEMSLPGR WKPKMIGGIG GFIKVRQYDQ ILIEICGHKA IGTVLVGPTP VNIIGRNLLT QIGCTLNFPI
|
Notes | D25G mutation prevents autocleavage of leader sequence. |
Expression | |
---|---|
Report | Cheng YE, Yin FH, Foundling S, Blomstrom D, Kettner CA (1990) Proc. Natl. Acad. Sci. USA, 87, 9660-9664 |
Project Aim | Functional Studies |
Fusion | None |
Protein Expression and Production | Protein recombinantly expressed as and refolded from inclusion bodies. |
Expression Host | Escherichia coli |
Expression Strain | JM105 |
Expression Temp | 37.0 |
Expression Time | not stated |
Expression Vector | pET3 |
Expression Protocol | no details provided |
Method of Induction | Not Stated |
Cell Density at Induction | OD = |
Cell Disruption Method | French Press |
Lytic Agent | None |
Pre-Refolding Purification | None |
Solubility | insoluble |
Refolding | |
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Refolding Method | Dialysis |
Wash Buffer | n/a |
Solubilization Buffer | 67% acetic acid |
Refolding Buffer | 20mM Mes, 1mM DTT, 10% glycerol, pH 5.5 |
Pre-Refolding Purification | None |
Tag Cleaved | no tag |
Refolding pH | 5.5 |
Refolding Temperature | 25.0 |
Protein Concentration | |
Refolding Time | 2h |
Redox Agent | DTT |
Redox Agent Concentration | 1mM |
Refolding Protocol | After expression, cells were harvested and lysed using a French pressure cell. Inclusion bodies were extracted with 67% acetic acid, then diluted 33-fold with water. The extracts were then dialyzed against water overnight, then dialyzed for 2h at 25degC against refolding buffer. The refolded protein was then concentrated, loaded onto a Sephadex G-75 column and eluted with 0.1% acetic acid/1.0mM DTT/10% glycerol. |
Refolding Assay | Enzyme activity |
Refolding Chaperones | None |
Refolding Additives | None,Glycerol |
Additives Concentration | 10% |
Refolding Yield | |
Purity | |
Notes |