Your search keyword '"Lipari F"' showing total 3 results

1. Single-well monitoring of protein-protein interaction and phosphorylation-dephosphorylation events.

Author

Arcand M, Roby P, Bossé R, Lipari F, Padrós J, Beaudet L, Marcil A, and Dahan S

Subjects

Adenosine Triphosphate metabolism, Binding, Competitive, Extracellular Signal-Regulated MAP Kinases metabolism, Mitogen-Activated Protein Kinase 3 metabolism, Mitogen-Activated Protein Kinases metabolism, Oxygen Consumption, Phosphorylation, Proteins chemistry, Proteins metabolism

Abstract

We combined oxygen channeling assays with two distinct chemiluminescent beads to detect simultaneously protein phosphorylation and interaction events that are usually monitored separately. This novel method was tested in the ERK1/2 MAP kinase pathway. It was first used to directly monitor dissociation of MAP kinase ERK2 from MEK1 upon phosphorylation and to evaluate MAP kinase phosphatase (MKP) selectivity and mechanism of action. In addition, MEK1 and ERK2 were probed with an ATP competitor and an allosteric MEK1 inhibitor, which generated distinct phosphorylation-interaction patterns. Simultaneous monitoring of protein-protein interactions and substrate phosphorylation can provide significant mechanistic insight into enzyme activity and small molecule action.

Published

2010

2. Purification and biophysical characterization of a minimal functional domain and of an N-terminal Zn2+-binding fragment from the human papillomavirus type 16 E6 protein.

Author

Lipari F, McGibbon GA, Wardrop E, and Cordingley MG

Subjects

Amino Acid Sequence, Carrier Proteins genetics, Cysteine chemistry, Escherichia coli genetics, Humans, Ligands, Molecular Sequence Data, Oncogene Proteins, Viral genetics, Papillomaviridae genetics, Peptide Fragments genetics, Protein Binding genetics, Protein Folding, Protein Structure, Tertiary genetics, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Sequence Deletion, Solubility, Carrier Proteins chemistry, Carrier Proteins isolation & purification, Oncogene Proteins, Viral chemistry, Oncogene Proteins, Viral isolation & purification, Papillomaviridae chemistry, Peptide Fragments chemistry, Peptide Fragments isolation & purification, Repressor Proteins, Zinc chemistry

Abstract

The E6 Zn(2+)-binding protein of high-risk human papillomaviruses (HPVs) is one of the major transforming proteins encoded by these tumor viruses. A bacterial system was used to express wild type and truncated forms of HPV-16 E6 linked to GST. The recombinant proteins were released from GST through cleavage of a factor Xa site. Functional analysis of these proteins demonstrated that amino acids 2--142 comprise the minimal domain of E6 required to promote the degradation of p53 in vitro in a rabbit reticulocyte lysate. This purified protein, E6(Delta 143--151), required a high salt concentration for maximum solubility, eluted as a monomer on gel filtration, and was shown to bind two Zn(2+) ions by atomic absorption analysis. An N-terminal subdomain of E6 (amino acids 2--77, E6-N) was similarly purified. Unlike E6(Delta 143--151), E6--N was very soluble in low-salt buffers and hence was highly amenable to biophysical characterization. E6-N was shown to bind one Zn(2+) ion by electrospray mass spectrometry and by atomic absorption analysis. UV--visible spectroscopic analysis of Co(2+)-substituted E6--N revealed that four cysteine residues coordinate the metal ion. Mutational studies of all the cysteine residues in E6--N substantiated a critical role for Cys 30, 33, 63, and 66 in Zn(2+) binding and in proper folding of the subdomain. Equilibrium sedimentation of E6-N demonstrated that it is a monomer, like E6(Delta 143--151), at low concentrations, but dimerization occurs at high concentrations (K(d) = 0.1 mM). Finally, circular dichroism studies revealed significant secondary structure for both E6(Delta 143--151) and E6--N. The results support a model of monomeric E6 possessing two functionally critical Zn(2+)-binding motifs.

Published

2001

3. Calcium binding to the class I alpha-1,2-mannosidase from Saccharomyces cerevisiae occurs outside the EF hand motif.

Author

Lipari F and Herscovics A

Subjects

Asparagine genetics, Asparagine metabolism, Aspartic Acid genetics, Aspartic Acid metabolism, Binding Sites genetics, Calcium physiology, Calcium-Binding Proteins chemistry, Calcium-Binding Proteins genetics, Catalysis, Enzyme Stability, Glutamic Acid genetics, Glutamic Acid metabolism, Glutamine genetics, Glutamine metabolism, Hot Temperature, Kinetics, Mannosidases chemistry, Mannosidases genetics, Mutagenesis, Site-Directed, Peptide Fragments chemistry, Peptide Fragments genetics, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Saccharomyces cerevisiae genetics, Calcium metabolism, Calcium-Binding Proteins metabolism, Mannosidases metabolism, Peptide Fragments metabolism, Saccharomyces cerevisiae enzymology

Abstract

Class I alpha-1,2-mannosidases are a family of Ca2+-dependent enzymes that have been conserved through eukaryotic evolution. These enzymes contain a conserved putative EF hand Ca2+-binding motif and nine invariant acidic residues. The catalytic domain of the alpha-1, 2-mannosidase from Saccharomyces cerevisiae was expressed in Pichia pastoris and was shown by atomic absorption and equilibrium dialysis to bind one Ca2+ ion with high affinity (KD = 4 x 10(-)7 M). Ca2+ protected the enzyme from thermal denaturation. Mutation of the 1st and 12th residues of the putative EF hand Ca2+ binding loop (D121N, D121A, E132Q, E132V, and D121A/E132V) had no effect on Ca2+ binding, demonstrating that the EF hand motif is not the site of Ca2+ binding. In contrast, three invariant acidic residue mutants (D275N, E279Q, and E438Q) lost the ability to bind 45Ca2+ following nondenaturing polyacrylamide gel electrophoresis whereas D86N, E132Q, E503Q, and E526Q mutants exhibited binding of 45Ca2+ similar to the wild-type enzyme. The wild-type enzyme had a Km and kcat of 0.5 mM and 12 s-1, respectively. The Km of E526Q was greatly increased to 4 mM with a small reduction in kcat to 5 s-1 whereas the kcat values of D86N and E132Q(V) were greatly reduced (0.005-0.007 s-1) with a decrease in Km (0.07-0.3 mM). The E503Q mutant is completely inactive. Asp275, Glu279, and Glu438 are therefore required for Ca2+ binding whereas Asp86, Glu132, and Glu503 are required for catalysis.

Published

1999