Your search keyword '"Terry W. Du Clos"' showing total 8 results

1. Analysis of Binding Sites in Human C-reactive Protein for FcγRI, FcγRIIA, and C1q by Site-directed Mutagenesis

Author

Kevin T. Du Clos, Mary-Pat Stein, Lorraine L. Marnell, Terry W. Du Clos, Carolyn Mold, Ranhy Bang, and Corinn Chivington-Buck

Subjects

Models, Molecular, CD32, Insecta, Recombinant Fusion Proteins, Mutant, Enzyme-Linked Immunosorbent Assay, Crystallography, X-Ray, Transfection, Biochemistry, Cell Line, law.invention, Antigen, Antigens, CD, Leucine, law, Animals, Humans, Receptors, Immunologic, Binding site, Site-directed mutagenesis, Receptor, Molecular Biology, Alleles, chemistry.chemical_classification, Binding Sites, Dose-Response Relationship, Drug, biology, Complement C1q, Lysine, Receptors, IgG, Cell Biology, Flow Cytometry, Molecular biology, Recombinant Proteins, Protein Structure, Tertiary, Amino acid, chemistry, Mutagenesis, Immunoglobulin G, COS Cells, Mutation, Mutagenesis, Site-Directed, biology.protein, Recombinant DNA, K562 Cells, Baculoviridae, Plasmids, Protein Binding

Abstract

Human C-reactive protein (CRP) is a classical, acute phase serum protein synthesized by the liver in response to infection, inflammation, or trauma. CRP binds to microbial antigens and damaged cells, opsonizes particles for phagocytosis and regulates the inflammatory response by the induction of cytokine synthesis. These activities of CRP depend on its ability to activate complement and to bind to Fcgamma receptors (FcgammaR). The goal of this study was to elucidate amino acid residues important for the interaction of CRP with human FcgammaRI (CD64) and FcgammaRIIa (CD32). Several mutations of the CRP structure were studied based on the published crystal structure of CRP. Mutant and wild-type recombinant CRP molecules were expressed in the baculovirus system and their interactions with FcgammaR and C1q were determined. A previous study by our laboratory identified an amino acid position, Leu(176), critical for CRP binding to FcgammaRI and work by others (Agrawal, A., Shrive, A. K., Greenhough, T. J., and Volanakis, J. E. (2001) J. Immunol. 166, 3998-4004) determined several residues important for C1q binding. The amino acid residues important to CRP binding to FcgammaRIIa were previously unknown. This study newly identifies residues Thr(173) and Asn(186) as important for the binding of CRP to FcgammaRIIa and FcgammaRI. Lys(114), like Leu(176), was implicated in binding to FcgammaRI, but not FcgammaRIIa. Single mutations at amino acid positions Lys(114), Asp(169), Thr(173), Tyr(175), and Leu(176) affected C1q binding to CRP. These results further identify amino acids involved in the binding sites on CRP for FcgammaRI, FcgammaRIIa, and C1q and indicate that these sites are overlapping.

Published

2005

2. Regulation of complement activation by C-reactive protein

Author

Henry Gewurz, Carolyn Mold, and Terry W. Du Clos

Subjects

Pharmacology, Binding Sites, Molecular Sequence Data, Acute-phase protein, Biology, Molecular biology, Complement system, Antibody opsonization, Classical complement pathway, C-Reactive Protein, Biochemistry, Lectin pathway, Alternative complement pathway, Animals, Humans, Amino Acid Sequence, Binding site, Complement Activation, Peptide sequence

Abstract

C-reactive protein (CRP) is an acute-phase serum protein and a mediator of innate immunity. CRP binds to microbial polysaccharides and to ligands exposed on damaged cells. Binding of CRP to these substrates activates the classical complement pathway leading to their uptake by phagocytic cells. Complement activation by CRP is restricted to C1, C4, C2 and C3 with little consumption of C5-9. Surface bound CRP reduces deposition of and generation of C5b-9 by the alternative pathway and deposition of C3b and lysis by the lectin pathway. These activities of CRP are the result of recruitment of factor H resulting in regulation of C3b on bacteria or erythrocytes. Evidence is presented for direct binding of H to CRP. H binding to CRP or C3b immobilized on microtiter wells was demonstrated by ELISA. Attachment of CRP to a surface was required for H binding. H binding to CRP was not inhibited by EDTA or phosphocholine, which inhibit ligand binding, but was inhibited by a 13 amino acid CRP peptide. The peptide sequence was identical to the region of CRP that showed the best alignment to H binding peptides from Streptococcus pyogenes (M6) and Neisseria gonorrhoeae (Por1A). The results suggest that CRP bound to a surface provides secondary binding sites for H resulting in greater regulation of alternative pathway amplification and C5 convertases. Complement activation by CRP may help limit the inflammatory response by providing opsonization with minimal generation of C5a and C5b-9.

Published

1999

3. Autoantibodies to Cryptic Epitopes of C-Reactive Protein and other Acute Phase Proteins in the Toxic Oil Syndrome

Author

Gus Khursigara, Terry W. Du Clos, Juan J. Picazo, Susanne A. Bell, and Robert L. Rubin

Subjects

Protein Denaturation, Immunology, Brassica, Cross Reactions, Biology, Fibrinogen, Autoantigens, Epitope, Autoimmune Diseases, Fatty Acids, Monounsaturated, Epitopes, medicine, Plant Oils, Immunology and Allergy, Autoantibodies, Autoimmune disease, Aniline Compounds, Poisoning, Autoantibody, Acute-phase protein, Ceruloplasmin, medicine.disease, C-Reactive Protein, Spain, alpha 1-Antitrypsin, Chronic Disease, Humoral immunity, biology.protein, Rapeseed Oil, Antibody, Toxic oil syndrome, Acute-Phase Proteins, medicine.drug

Abstract

Toxic oil syndrome (TOS) was caused by the consumption of rapeseed oil contaminated with derivatives of aniline. Many persons who survived the acute phase developed a puzzling, multi-year chronic disease considered to be inflammatory or autoimmune in nature. In attempting to characterize their autoantibodies, we found that 74% of TOS patients with chronic disease had IgG antibodies to C-reactive protein (CRP). This activity was detectable only when CRP was chemically or physically denatured and behaved like a previously described antibody produced by immunization with the CRP monomer. Significant antibody reactivities to other acute phase proteins, especially alpha 1-antitrypsin and fibrinogen (P0.025) and ceruloplasmin (P0.05) were also observed. IgG antibodies to cryptic epitopes in CRP and other major serum proteins that increase during the acute phase response may reflect an earlier toxin-mediated insult to the liver that included abnormal biosynthesis of and/or damage to acute phase proteins.

Published

1995

4. C-reactive protein (CRP) binding to the Sm-D protein of snRNPS. Identification of a short polypeptide binding region

Author

Lorraine L. Marnell, Luis A. Rokeach, Terry W. Du Clos, and Wendy S. Jewell

Subjects

Thymus extract, Binding Sites, SnRNP Core Proteins, Recombinant Fusion Proteins, Binding protein, Blotting, Western, Molecular Sequence Data, Immunology, Biology, Ribonucleoproteins, Small Nuclear, Autoantigens, environment and public health, Fusion protein, Molecular biology, snRNP Core Proteins, Histones, C-Reactive Protein, Biochemistry, Humans, snRNP, Amino Acid Sequence, Nuclear protein, Binding site, Molecular Biology, Ribonucleoprotein

Abstract

C-reactive protein (CRP) binds to chromatin, histones, and small nuclear ribonucleoproteins (snRNPs) through a phosphocholine (PC)-inhibitable, calcium-dependent binding site. snRNPs process pre-mRNA to mature mRNA and are composed of small uridine-rich RNAs (designated U1, U2, U5 and U4/U6) and associated proteins. We have shown that CRP binds to snRNPs in intact cells and to the U1 snRNP-specific 70 K protein in cell extracts. To determine whether CRP bound to other snRNP proteins, snRNPs were purified from rabbit thymus extract and CRP binding was assessed by blotting. CRP bound to a protein with the same mobility as Sm-D as well as to the 70 K protein. CRP specifically bound to and precipitated a fusion protein containing full-length Sm-D, confirming the binding of CRP to Sm-D. Binding was inhibited by PC and by EDTA. Binding studies using deletion mutants of the Sm-D fusion protein revealed that CRP binding was mediated by the C-terminal region of Sm-D, a region which binds autoantibodies and is proposed to bind to RNA. A comparison of the peptide regions on different autoantigens suggests that there is a shared motif to which CRP binds.

Published

1993

5. Hamster female protein binding to chromatin, histones and DNA

Author

Terry W. Du Clos, John E. Coe, Carolyn Mold, and Liliana Saunero-Nava

Subjects

biology, Pentraxins, Macromolecular Substances, Phosphorylcholine, Molecular Sequence Data, Immunology, DNA, Plasma protein binding, Molecular biology, DNA-binding protein, Chromatin, DNA-Binding Proteins, Histones, C-Reactive Protein, Histone, Biochemistry, Alpha-Globulins, biology.protein, Amino Acid Sequence, Binding site, Molecular Biology, Peptide sequence, Protein Binding, Histone binding

Abstract

Hamster female protein (FP) is a member of the family of proteins known as pentraxins which share amino acid sequence homology, cyclic pentameric structure and calcium-dependent binding to ligands. Other members of this family include C-reactive protein (CRP) and serum amyloid P component (SAP), and most species synthesize both CRP and SAP. FP is unusual in that it is apparently the only pentraxin produced in hamsters, it is under hormonal control and it shares binding characteristics with both CRP and SAP. CRP has been defined and isolated by its calcium-dependent binding to pneumococcal C-polysaccharide via phosphocholine (PC) residues. SAP has been isolated by calcium-dependent binding to agarose. FP binds to both PC and agarose. Recently, both SAP and CRP have been found to bind to chromatin in a calcium-dependent manner and involvement of these proteins in the clearance of nuclear material has been proposed. In this paper we test whether FP shares the ability to bind to chromatin and histones, and compare its relative avidities for these ligands. Similar to CRP, FP bound to histones H1 and H2A, and chromatin. FP shared with SAP the ability to bind to DNA. However, FP binding was inhibited by PC for all ligands, whereas SAP binding was not. FP and SAP also failed to compete with each other for binding to DNA. By cross-inhibition FP bound much less well to PC than CRP, but was a very effective inhibitor of CRP binding to H2A. These studies demonstrate that chromatin and histone binding are conserved among these pentraxins. The role of the proposed PC binding site in these binding reactions is discussed.

Published

1992

6. A new procedure for the separation of protein Z, prothrombin fragment 1.2 and calreticulin from human plasma

Author

Terry W. Du Clos, Lorraine L. Marnell, Tatsuya Sueyoshi, Walter Kisiel, and Brad A. McMullen

Subjects

chemistry.chemical_classification, Gel electrophoresis, biology, PROTHROMBIN FRAGMENT 1.2, Calcium-Binding Proteins, Molecular Sequence Data, Ion chromatography, Protein Z, Blood Proteins, Hematology, Peptide Fragments, Plasma, Biochemistry, chemistry, Affinity chromatography, Blood plasma, biology.protein, Humans, Prothrombin, Amino Acid Sequence, Calreticulin, Glycoprotein

Published

1991

7. Regulation of complement by direct binding of factor H to C-reactive protein

Author

Mary-Pat Stein, Terry W. Du Clos, and Carolyn Mold

Subjects

biology, Biochemistry, Chemistry, Factor H, Direct binding, Immunology, C-reactive protein, Protein A/G, biology.protein, Protein G, Complement factor I, Molecular Biology, Complement (complexity)

Published

1998

8. Monoclonal antibody for DNA measurement in biological fluids

Author

Robert L. Rubin, Terry W. Du Clos, and Eng M. Tan

Subjects

Detection limit, biology, Base pair, Chromogenic, medicine.drug_class, Immunology, Antibodies, Monoclonal, Enzyme-Linked Immunosorbent Assay, DNA, Monoclonal antibody, Binding, Competitive, Horseradish peroxidase, Molecular biology, Nucleosomes, Molecular Weight, chemistry.chemical_compound, chemistry, Biotinylation, medicine, biology.protein, Humans, Nucleic Acid Conformation, Immunology and Allergy, Antibody

Abstract

Two highly sensitive immunoassays for measuring soluble DNA are described. These methods employ a purified mouse monoclonal anti-DNA antibody in enzyme-linked immunoassays. One assay is an antigen capture method utilizing immobilized antibody. Bound DNA is subsequently detected with biotinylated monoclonal anti-DNA antibody, avidin-coupled horseradish peroxidase and a chromogenic substrate. The limit of detection of the assay was 2 ng/ml of DNA. A competition assay relying on immobilized heat-denatured DNA was also designed. In this assay the solution to be analyzed is mixed in equal proportions with monoclonal anti-DNA antibody and the mixture is incubated in the DNA-containing microtiter plates. The inhibition of antibody binding as detected with peroxidase-conjugated anti-mouse IgG was proportional to the concentration of DNA in the sample. The competition assay was tested for its ability to detect DNA in human plasma. The detection limit of DNA in plasma was approximately 150 ng/ml. The assays were compared in their ability to detect various size fragments of DNA. The competition assay was capable of detecting DNA fragments as small as 30 base pairs. In contrast, the capture assay failed to detect low molecular weight fragments up to 150 base pairs although its sensitivity for undigested DNA was comparable to the competition assay. The assay may be of use in the rapid quantitation of low levels of DNA, especially low molecular weight DNA and may also be useful in measuring DNA in human plasma.

Published

1986