Your search keyword '"LamB protein"' showing total 2 results

1. Folding studies of purified LamB protein, the maltoporin from the Escherichia coli outer membrane: Trimer dissociation can be separated from unfolding

Author

Baldwin, Valerie, Bhatia, Mandeep, and Luckey, Mary

Subjects

*MEMBRANE proteins, *PROTEIN folding, *ESCHERICHIA coli, *DENATURATION of proteins, *POLYACRYLAMIDE gel electrophoresis, *BIOLOGICAL membranes, *CHEMICAL bonds, *OLIGOMERS

Abstract

Abstract: The folding mechanisms for β-barrel membrane proteins present unique challenges because acquisition of both secondary and tertiary structure is coupled with insertion into the bilayer. For the porins in Escherichia coli outer membrane, the assembly pathway also includes association into homotrimers. We study the folding pathway for purified LamB protein in detergent and observe extreme hysteresis in unfolding and refolding, as indicated by the shift in intrinsic fluorescence. The strong hysteresis is not seen in unfolding and refolding a mutant LamB protein lacking the disulfide bond, as it unfolds at much lower denaturant concentrations than wild type LamB protein. The disulfide bond is proposed to stabilize the structure of LamB protein by clasping together the two sides of Loop 1 as it lines the inner cavity of the barrel. In addition we find that low pH promotes dissociation of the LamB trimer to folded monomers, which run at about one third the size of the native trimer during SDS PAGE and are much more resistant to trypsin than the unfolded protein. We postulate the loss at low pH of two salt bridges between Loop 2 of the neighboring subunit and the inner wall of the monomer barrel destabilizes the quaternary structure. [Copyright &y& Elsevier]

Published

2011

2. Folding studies of purified LamB protein, the maltoporin from the Escherichia coli outer membrane: Trimer dissociation can be separated from unfolding

Author

Mandeep Bhatia, Valerie Baldwin, and Mary Luckey

Subjects

Protein Denaturation, Protein Folding, Protein subunit, Biophysics, Porins, Maltoporin, Trimer, Biochemistry, Article, 03 medical and health sciences, Escherichia coli, Oligomerization, Disulfides, Protein Structure, Quaternary, 030304 developmental biology, Folding β-barrel protein, 0303 health sciences, Disulfide bond, Dose-Response Relationship, Drug, Chemistry, Bilayer, 030302 biochemistry & molecular biology, Biological Transport, Cell Biology, Hydrogen-Ion Concentration, LamB protein, Protein tertiary structure, Crystallography, Outer membrane, Microscopy, Fluorescence, Membrane protein, Receptors, Virus, Electrophoresis, Polyacrylamide Gel, Protein quaternary structure, Bacterial outer membrane, Bacterial Outer Membrane Proteins, Peptide Hydrolases

Abstract

The folding mechanisms for β-barrel membrane proteins present unique challenges because acquisition of both secondary and tertiary structure is coupled with insertion into the bilayer. For the porins in Escherichia coli outer membrane, the assembly pathway also includes association into homotrimers. We study the folding pathway for purified LamB protein in detergent and observe extreme hysteresis in unfolding and refolding, as indicated by the shift in intrinsic fluorescence. The strong hysteresis is not seen in unfolding and refolding a mutant LamB protein lacking the disulfide bond, as it unfolds at much lower denaturant concentrations than wild type LamB protein. The disulfide bond is proposed to stabilize the structure of LamB protein by clasping together the two sides of Loop 1 as it lines the inner cavity of the barrel. In addition we find that low pH promotes dissociation of the LamB trimer to folded monomers, which run at about one third the size of the native trimer during SDS PAGE and are much more resistant to trypsin than the unfolded protein. We postulate the loss at low pH of two salt bridges between Loop 2 of the neighboring subunit and the inner wall of the monomer barrel destabilizes the quaternary structure.

Published

2011