Literature DB >> 12592025

Purification of correctly oxidized MHC class I heavy-chain molecules under denaturing conditions: a novel strategy exploiting disulfide assisted protein folding.

Henrik Ferré1, Emmanuel Ruffet, Thomas Blicher, Christina Sylvester-Hvid, Lise Lotte B Nielsen, Timothy J Hobley, Owen R T Thomas, Søren Buus.   

Abstract

The aim of this study has been to develop a strategy for purifying correctly oxidized denatured major histocompability complex class I (MHC-I) heavy-chain molecules, which on dilution, fold efficiently and become functional. Expression of heavy-chain molecules in bacteria results in the formation of insoluble cellular inclusion bodies, which must be solubilized under denaturing conditions. Their subsequent purification and refolding is complicated by the fact that (1). correct folding can only take place in combined presence of beta(2)-microglobulin and a binding peptide; and (2). optimal in vitro conditions for disulfide bond formation ( approximately pH 8) and peptide binding ( approximately pH 6.6) are far from complementary. Here we present a two-step strategy, which relies on uncoupling the events of disulfide bond formation and peptide binding. In the first phase, heavy-chain molecules with correct disulfide bonding are formed under non-reducing denaturing conditions and separated from scrambled disulfide bond forms by hydrophobic interaction chromatography. In the second step, rapid refolding of the oxidized heavy chains is afforded by disulfide bond-assisted folding in the presence of beta(2)-microglobulin and a specific peptide. Under conditions optimized for peptide binding, refolding and simultaneous peptide binding of the correctly oxidized heavy chain was much more efficient than that of the fully reduced molecule.

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Year:  2003        PMID: 12592025      PMCID: PMC2312438          DOI: 10.1110/ps.0233003

Source DB:  PubMed          Journal:  Protein Sci        ISSN: 0961-8368            Impact factor:   6.725


  22 in total

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Review 4.  Description and prediction of peptide-MHC binding: the 'human MHC project'.

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Journal:  Curr Opin Immunol       Date:  1999-04       Impact factor: 7.486

5.  Submit and disulfide structure of monomeric and dimeric forms of detergent-soluble HLA antigens.

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8.  Beta 2-microglobulin and calnexin can independently promote folding and disulfide bond formation in class I histocompatibility proteins.

Authors:  M Tector; Q Zhang; R D Salter
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9.  Cleavage of structural proteins during the assembly of the head of bacteriophage T4.

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  19 in total

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3.  A novel system for continuous protein refolding and on-line capture by expanded bed adsorption.

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4.  Recombinant chymosin used for exact and complete removal of a prochymosin derived fusion tag releasing intact native target protein.

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5.  Real-time, high-throughput measurements of peptide-MHC-I dissociation using a scintillation proximity assay.

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6.  The peptide-binding specificity of HLA-A*3001 demonstrates membership of the HLA-A3 supertype.

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7.  Measurement of MHC/peptide interactions by gel filtration or monoclonal antibody capture.

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9.  MHC-I peptide binding activity assessed by exchange after cleavage of peptide covalently linked to β2-microglobulin.

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10.  Characterization of binding specificities of bovine leucocyte class I molecules: impacts for rational epitope discovery.

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