Refolding Record:
Protein | |
---|---|
Protein Name | Human Leukocyte Antigen DR2 |
Abbreviated Name | HLA DR2 |
SCOP Family | C1 set domains (antibody constant domain-like) |
Structure Notes | |
Organism | Human |
UniProt Accession | P01903 |
SCOP Unique ID | n/a |
Structure Solved | |
Class | Beta |
Molecularity | Dimer |
Construct | |
---|---|
Full Length | n |
Domain | n/a |
Chimera | n/a |
Variants | Alpha Polypeptide Chain Lacking Transmembrane Domain |
Chain Length | 216 |
Molecular Weight | 24705.2 |
Pi | 4.66 |
Molecular Weight | 24705.2 |
Disulphides | 1 |
Full Sequence |
MAISGVPVLGFFIIAVLMSAQESWAIKEEHVIIQAEFYLNPDQSGEFMFDFDGDEIFHVDMAKKETVWRLEEFGRFASFEAQGALANIAVDKANLEIMTKRSNYTPITNVPPEVTVLTNSPVELREPNVLICFIDKFTPPVVNVTWLRNGKPVTTGVSETVFLPREDHLFRKFHYLPFLPSTEDVYDCRVEHWGLDEPLLKHWEFDAPSPLPETTE
|
Notes | n/a |
Expression | |
---|---|
Report | Arimilli, S., Cardoso, C., Mukku, P, Baichwal, V., Nag, B. (1995) J Biol Chem, 270, 971-977 |
Project Aim | Folding,Functional Studies |
Fusion | None |
Protein Expression and Production | Protein recombinantly expressed as and refolded from inclusion bodies. |
Expression Host | Escherichia coli |
Expression Strain | W3310/D3 |
Expression Temp | 37.0 |
Expression Time | 2h |
Expression Vector | p27313 |
Expression Protocol | Vector pET-11a was used to construct the expression vector by modifications to cloning site. Insert |
Method of Induction | IPTG |
Cell Density at Induction | OD n/a = n/a |
Cell Disruption Method | Osmotic shock |
Lytic Agent | None |
Pre-Refolding Purification | Ion-exchange chromatography |
Solubility | insoluble |
Refolding | |
---|---|
Refolding Method | Dialysis |
Wash Buffer | n/a |
Solubilization Buffer | 25 mM phosphate buffer, pH 7.4, 8 M urea, 20 mM DTT |
Refolding Buffer | 12.5 mM phosphate buffer, pH 7.4, 4 M urea, 10 mM DTT, 1.0 M NaCI |
Pre-Refolding Purification | Ion-exchange chromatography |
Tag Cleaved | no |
Refolding pH | 7.4 |
Refolding Temperature | 37.0 |
Protein Concentration | n/a |
Refolding Time | n/a |
Redox Agent | DTT |
Redox Agent Concentration | 30 mM |
Refolding Protocol | Inclusion bodies solubilized in solubilization buffer. Pellet broken up by mild sonication and allowed to sit at 36degC overnight. Preparation then centriguged (100 000g, 1 hr). Supernatant removed and filtered through 2-pm filter. Recombinant chain purified and refolded by ion exchange chromatography. Which was preformed as follows: 100mg of crude solution was loaded onto 50-ml High Q-50 column. The column was washed subsequently with 90% buffer 12.5 mM phosphate buffer, pH 7.4, 4 M urea, 10 mm DTT) for 60 min at a flow rate of 2.5 m/min. A gradient was run at a flow rate of 2.0 min as follows: 60-180 min 10-30% B refolding buffer, 180-200 min 30%-100%B . Fractions (6.5 ml) were collected and analyzed by SDS-PAGE. |
Refolding Assay | SDS-PAGE |
Refolding Chaperones | None |
Refolding Additives | None |
Additives Concentration | n/a |
Refolding Yield | n/a |
Purity | n/a |
Notes | n/a |