Your search keyword '"Complement C3c"' showing total 555 results

101. Complement receptor expression and activation of the complement cascade on B lymphocytes from patients with systemic lupus erythematosus (SLE)

Author

Peter Junker, R. G. Q. Leslie, Anders Jørgen Svendsen, S E Svehag, J M Rasmussen, Claus Henrik Nielsen, and H. V. Marquart

Subjects

Adult, Male, Erythrocytes, Complement receptor 2, Complement Pathway, Alternative, Immunology, chemical and pharmacologic phenomena, Complement receptor, Biology, Complement C3d, Complement C3c, Leukocytes, medicine, Humans, Lupus Erythematosus, Systemic, Immunology and Allergy, B-Lymphocytes, Lupus erythematosus, Antibodies, Monoclonal, Complement C3, Middle Aged, medicine.disease, In vitro, Receptors, Complement, Complement system, Complement C3b, Alternative complement pathway, Female, Receptors, Complement 3d, Research Article

Abstract

It has previously been reported that the expression of the complement receptors, CR1 on erythrocytes and blood leucocytes and CR2 on B cells, is reduced in patients with SLE, and that the reduced expression of CR1 on erythrocytes is related to disease activity. We have earlier demonstrated that normal B cells are capable of activating the alternative pathway (AP) of complement in a CR2-dependent fashion. In this study we have investigated whether disturbances in this activity may be related to the altered phenotype of SLE B cells. Flow cytometry was used to measure expression of complement receptors and regulatory proteins on B cells from SLE patients, as well as the deposition of C3 fragments occurring in vivo or after in vitro AP activation. We have confirmed, for a proportion of the patients studied, reduced expression of CR1 and CR2 on B cells, and shown a consistency between low CR2 expression and reduced in vitro AP activation in the presence of homologous, normal serum. In addition, the B cells, like erythrocytes, bear raised levels of in vivo-deposited C3dg, but not C3b fragments, compared with normal B cells. The erythrocytes from SLE patients were unable to inhibit in vitro AP activation by B cells in homologous serum. Finally, we demonstrated an inverse relationship between SLE disease activity index (SLEDAI) and the expression of complement receptor 2 (CR2) on SLE B cells. Thus, determination of CR2 on B cells may emerge as an additional laboratory tool in the assessment of SLE activity. It has previously been reported that the expression of the complement receptors, CR1 on erythrocytes and blood leucocytes and CR2 on B cells, is reduced in patients with SLE, and that the reduced expression of CR1 on erythrocytes is related to disease activity. We have earlier demonstrated that normal B cells are capable of activating the alternative pathway (AP) of complement in a CR2-dependent fashion. In this study we have investigated whether disturbances in this activity may be related to the altered phenotype of SLE B cells. Flow cytometry was used to measure expression of complement receptors and regulatory proteins on B cells from SLE patients, as well as the deposition of C3 fragments occurring in vivo or after in vitro AP activation. We have confirmed, for a proportion of the patients studied, reduced expression of CR1 and CR2 on B cells, and shown a consistency between low CR2 expression and reduced in vitro AP activation in the presence of homologous, normal serum. In addition, the B cells, like erythrocytes, bear raised levels of in vivo-deposited C3dg, but not C3b fragments, compared with normal B cells. The erythrocytes from SLE patients were unable to inhibit in vitro AP activation by B cells in homologous serum. Finally, we demonstrated an inverse relationship between SLE disease activity index (SLEDAI) and the expression of complement receptor 2 (CR2) on SLE B cells. Thus, determination of CR2 on B cells may emerge as an additional laboratory tool in the assessment of SLE activity.

Published

1995

102. Laboratory Diagnosis and Clinical Profile of Anti-p200 Pemphigoid

Author

Marcel F. Jonkman, Joost M. Meijer, Gilles F. H. Diercks, Enno Schmidt, Hendri H. Pas, Translational Immunology Groningen (TRIGR), and Microbes in Health and Disease (MHD)

Subjects

Male, Pemphigoid, Pathology, Autoantigens, Basement Membrane, COEXISTENCE, 030207 dermatology & venereal diseases, 0302 clinical medicine, Pemphigoid, Bullous, Fluorescent Antibody Technique, Indirect, skin and connective tissue diseases, Aged, 80 and over, integumentary system, medicine.diagnostic_test, MICROSCOPY, Middle Aged, EPIDERMOLYSIS-BULLOSA ACQUISITA, DIFFERENTIATION, medicine.anatomical_structure, Complement C3c, 030220 oncology & carcinogenesis, Female, Bullous pemphigoid, Algorithms, Adult, Epidermolysis bullosa acquisita, VII COLLAGEN, medicine.medical_specialty, Collagen Type VII, Immunoblotting, ANTIGEN, IMMUNOFLUORESCENCE, Hand Dermatoses, Dermatology, Immunofluorescence, SUBEPIDERMAL BLISTERING DISEASE, Young Adult, 03 medical and health sciences, medicine, Humans, LAMINA-LUCIDA, Direct fluorescent antibody, Aged, Retrospective Studies, Foot Dermatoses, Basement membrane, business.industry, Autoantibody, medicine.disease, Lamina lucida, Immunoglobulin A, Immunoglobulin M, Immunoglobulin G, AUTOANTIBODIES, Laminin, business, Cell Adhesion Molecules

Abstract

IMPORTANCE Anti-p200 pemphigoid is a rare subepidermal autoimmune blistering disease characterized by autoantibodies against a 200-kDa protein in the basement membrane zone. Anti-p200 pemphigoid is probably often misdiagnosed because of low availability of diagnostic assays and expertise and classified as bullous pemphigoid or epidermolysis bullosa acquisita.OBJECTIVE To clinically characterize patients with anti-p200 pemphigoid, identified by using indirect immunofluorescence microscopy on skin substrates deficient in type VII collagen and laminin-332 (knockout analysis), to validate this technique by immunoblot with dermal extract, and to incorporate direct immunofluorescence serration pattern analysis in the diagnostic algorithm.DESIGN, SETTING, AND PARTICIPANTS This was a retrospective study performed from January 2014 to June 2015 with biobank patient materials and clinical data for the period 1998 to 2015 from the single national referral center on autoimmune bullous diseases. Patients were selected based on a dermal side binding on 1-mol/L salt (sodium chloride)-split human skin substrate by indirect immunofluorescence microscopy, not diagnosed epidermolysis bullosa acquisita or anti-laminin-332 mucous membrane pemphigoid.MAIN OUTCOMES AND MEASURES Indirect immunofluorescence microscopy knockout analysis was performed and diagnosis of anti-p200 confirmed by immunoblot with dermal extract. Clinical, histological, and immunological findings were registered. Autoantibodies against laminin Upsilon 1 were determined by immunoblot.RESULTS Twelve patients with anti-p200 pemphigoid (7 male and 5 female; mean age, 66.6 years) were identified using the indirect immunofluorescence microscopy knockout analysis. Direct immunofluorescence microscopy showed a linear n-serrated IgG deposition pattern along the basement membrane zone in 9 of 11 patients. The diagnosis was confirmed by immunoblot showing autoantibodies against 200-kDa protein in dermal extract in 12 of 12 patients. Autoantibodies against recombinant laminin Upsilon 1 were detected by immunoblot in 8 of 12 patients. Remarkable similarities were seen in clinical features with predominantly tense blisters on hands and feet, resembling dyshidrosiform pemphigoid. Mucosal involvement was seen in 6 (50%) of the patients.CONCLUSIONS AND RELEVANCE Predominance of blisters on hands and feet may be a clinical clue to the diagnosis of anti-p200 pemphigoid. Direct immunofluorescence microscopy serration pattern analysis and indirect immunofluorescence microscopy knockout analysis are valuable additional techniques to facilitate the diagnosis of anti-p200 pemphigoid.

Published

2016

103. The IgG 'Lupus-Band' Deposition Pattern of Pemphigus Erythematosus Association With the Desmoglein 1 Ectodomain as Revealed by 3 Cases

Author

Dyah Ayu Mira Oktarina, Gilles F. H. Diercks, Hendri H. Pas, Marcel F. Jonkman, Angelique Poot, Duco Kramer, Microbes in Health and Disease (MHD), and Translational Immunology Groningen (TRIGR)

Subjects

Male, Pathology, medicine.medical_specialty, Discoid lupus erythematosus, Dermatology, Desmoglein, Basement Membrane, immune system diseases, medicine, FOLIACEUS, Humans, Diagnostic Errors, skin and connective tissue diseases, PUVA Therapy, Pemphigus foliaceus, Aged, Aged, 80 and over, Lupus erythematosus, integumentary system, business.industry, Desmoglein 1, Pemphigus erythematosus, SENEAR-USHER-SYNDROME, General Medicine, medicine.disease, Ectodomain, Complement C3c, Immunoglobulin G, Antigens, Surface, Immunology, Female, Lamina densa, business, Pemphigus

Abstract

Background: Pemphigus foliaceus is an autoimmune skin disease characterized by subcorneal blistering and IgG antibodies directed against desmoglein 1. In the skin, these antibodies deposit intraepidermally. On rare occasions, an additional "lupus band" of granular depositions of IgG and complement is seen along the epidermal basement membrane zone. This combined pattern has been connected with a variant of pemphigus foliaceus named pemphigus erythematosus.Observations: We describe 3 pemphigus foliaceus cases in which phototherapy was administered after a misdiagnosis of psoriasis. This treatment resulted in a flare of skin lesions. Direct immunofluorescence of skin biopsy specimens that were obtained several weeks later demonstrated intraepidermal and granular basement membrane zone depositions. The basement membrane zone depositions consisted of IgG, complement, and the ectodomain of desmoglein 1 and were located below the lamina densa.Conclusions: High doses of UV light are likely to induce the cleaving of the desmoglein 1 ectoclomain. In patients with pemphigus foliaceus, the circulating anti desmoglein 1 antibodies precipitate this cleaved-off ectodomain along the basement membrane zone, resulting in a lupus band like appearance. In pemphigus erythematosus, a similar mechanism may be active, which might explain the lupus-band phenomenon. Arch Dermatol, 2012;148(10):1173-1178. Published online July 16, 2012. doi:10.1001/archdermatol.2012.1896

Published

2012

104. Complement factors in newly diagnosed Nigerian schizoprenic patients and those on antipsychotic therapy

Author

O B, Idonije, K S, Akinlade, O, Ihenyen, and O G, Arinola

Subjects

Adult, Male, Adolescent, Complement C1q, Complement C5, Nigeria, Complement C4, Complement C3, Middle Aged, Young Adult, Complement C3c, Schizophrenia, Humans, Female, Complement C1 Inhibitor Protein, Biomarkers, Antipsychotic Agents

Abstract

The role of Complement factors in the pathogenesis of psychiatric disorders is enormous, but the data on levels and functions of complement factors in patients with schizophrenia are scanty and conflicting. To address this issue, levels of Complement regulators (C1 inhibitor and C3 activator) and complement factors (C1q, C3c, C4 and C5) were determined in the serum of newly diagnosed drug free schizophrenic patients, schizophrenic patients on medication and healthy subjects using immune-plates. C1q was significantly reduced in newly diagnosed schizophrenic patients or schizophrenic patients on medication compared with the controls. C3c was significantly reduced in newly diagnosed schizophrenic patients compared with controls or schizophrenic patients on medication. The levels of C3 activators, C1 inhibitors and C4 were similar in the two groups of schizophrenic patients compared with the controls. It may be concluded from this study that C1q is deficient in schizophrenic patients; and that C3c may differentiate newly diagnosed schizophrenia from schizophrenic patients on medication.

Published

2012

105. Clinical and histological outcome predictors in renal limited pauci-immune crescentic glomerulonephritis: a single centre experience

Author

Antonietta Gigante, Maria Ludovica Gasperini, Francesco Pugliese, Italo Nofroni, Chiara Salviani, Felice Salsano, Rossella Cianci, Edoardo Rosato, Antonio Amoroso, Biagio Barbano, and Konstantinos Giannakakis

Subjects

Male, Pathology, medicine.medical_specialty, anca, pauci-immune crescentic necrotizing glomerulonephritis, renal limited vasculitis, renal vasculitis, vasculitis, Immunology, Renal function, Kidney, Antibodies, Antineutrophil Cytoplasmic, chemistry.chemical_compound, Glomerulonephritis, medicine, Immunology and Allergy, Rapidly progressive glomerulonephritis, Humans, Fibrinoid necrosis, Retrospective Studies, Pharmacology, Creatinine, medicine.diagnostic_test, business.industry, Retrospective cohort study, Middle Aged, medicine.disease, chemistry, Pauci-immune, Complement C3c, Female, Renal biopsy, medicine.symptom, business, Vasculitis

Abstract

Renal-limited vasculitis is a pauci-immune crescentic glomerulonephritis with no signs of systemic involvement, representing one of the most common causes of rapidly progressive glomerulonephritis. The study aims to examine clinical and histological features in twenty-four patients with RLV diagnosed by the Nephrology Department of Sapienza University of Rome, Italy, evaluating the role of these parameters in predicting renal survival. Patients details, clinical and histological features and outcomes were recorded at the time of renal biopsy and over a mean follow-up period of 36±6 months. In our study, serum creatinine at presentation was significantly higher in patients who had a poor outcome than in those who survived with independent renal function (6.3±2.47 mg/dl vs 2.84±2.01 mg/dl, P= 0.002). The presence of C3c was found in the area of glomerular fibrinoid necrosis and in small arteries and arterioles with fibrinoid necrosis in 17 patients (P= 0.018). In conclusion, serum creatinine at presentation and focal C3c depositions in areas of glomerular and arteriolar fibrinoid necrosis were the best determinants of poor renal outcome, maybe underlining the pathogenic role of alternative pathway activation of complement system but also demonstrating the focal distribution of necrotizing lesions.

Published

2012

106. Serum complement C4 in chronic hepatitis C: correlation with histopathologic findings and disease activity

Author

Banu Bayraktar, Beşir Kesici, Canan Alkim, Mehmet Sait Bugdaci, Cetin Karaca, and Mehmet Sokmen

Subjects

Liver Cirrhosis, medicine.medical_specialty, Pathology, Cirrhosis, Hepatitis C virus, Biopsy, Fine-Needle, Hepacivirus, Chronic liver disease, medicine.disease_cause, Complement C3c, Gastroenterology, Transaminase, Internal medicine, medicine, Humans, Aspartate Aminotransferases, Prospective Studies, medicine.diagnostic_test, business.industry, Alanine Transaminase, Complement C4, Hepatitis C, Complement C3, gamma-Glutamyltransferase, Hepatitis C, Chronic, Middle Aged, medicine.disease, Liver, Liver biopsy, Case-Control Studies, Coinfection, RNA, business

Abstract

BACKGROUND/AIMS Hepatitis C virus leads to chronic liver disease, cirrhosis and hepatocellular cancer. Viral markers and other laboratory tests used in the diagnosis and follow-up of chronic hepatitis C do not correlate well with disease activity and liver histopathology. Therefore, alternative tests that indicate disease activity and relate with liver biopsy findings are needed. We aimed to investigate the relationship between serum complement levels and biopsy findings in patients with chronic hepatitis C. METHODS One hundred cases (70 patients, 30 healthy controls) were included in the study. Patients were divided into two groups: chronic hepatitis C patients with high transaminase levels were evaluated as the first group and patients with normal transaminase levels as the second group. Patients with a high transaminase level were biopsied and activity scores were evaluated against complement C3c and C4 levels. In addition, demographic data and laboratory tests were evaluated. Patients with chronic hepatitis C without proteinuria, acute phase response, cirrhosis, or coinfection with another hepatitis virus were included in the prospective study. RESULTS Serum complement C3c (p

Published

2012

107. Detection of complement-fixing and non-fixing antibodies specific for endothelial precursor cells and lymphocytes using flow cytometry

Author

A, AlMahri, J, Holgersson, and M, Alheim

Subjects

Graft Rejection, Male, B-Lymphocytes, Complement C1q, T-Lymphocytes, Endothelial Cells, Cell Differentiation, Cytotoxicity Tests, Immunologic, Flow Cytometry, Kidney Transplantation, Sensitivity and Specificity, Peptide Fragments, Antibody Specificity, Complement C3d, HLA Antigens, Isoantibodies, Complement C3c, Immunoglobulin G, Complement C4b, Humans, Transplantation, Homologous

Abstract

Donor human leukocyte antigen (HLA)-specific antibodies (Abs) with the ability to activate complement are associated with an increased risk of early Ab-mediated rejection (AMR) of kidney allografts. In recent years, also non-HLA Abs-binding endothelial cells have been shown to elicit early AMR. Donor-specific anti-endothelial cell Abs escape detection in the pre-transplant evaluation if only lymphocytes are used as target cells in crossmatch tests. We addressed whether endothelial precursor cells (EPCs) could be used for detection of complement-fixing as well as non-fixing Abs and if complement factor and immunoglobulin G (IgG) deposition on co-purified T and B cells correlated to the outcome of the T- and B-cell complement-dependent cytotoxicity assay. Deposition of complement factors C3c and C3d, but not C1q nor C4d, were detected on EPCs and lymphocytes upon incubation with HLA Ab-positive sera. There was a correlation between the amount of C3c deposition and IgG binding on EPCs (R(2) = 0.71, P = 0.0012) and T cells (R(2) = 0.74, P = 0.0006) but not for B cells (R(2) = 0.34, P = 0.059). The specificity and sensitivity for C3d deposition on endothelial precursor cell crossmatch (EPCXM) T cells vs the T complement-dependent cytotoxicity (CDC) assay were 69% and 72%, respectively. The EPCXM B-cell C3d assay had considerably lower sensitivity (39%) than the B CDC assay. Altogether, this novel assay based on the detection of complements factors on EPCs and lymphocytes by flow cytometry may widen the diagnostic repertoire and thereby improve the clinical management of patients undergoing kidney transplantation.

Published

2012

108. In vitro Plasma protein adsorption and kallikrein formation on 3-mercaptopropionic acid,L-cysteine and glutathione immobilized onto gold

Author

Ingemar Lundström, Bo Liedberg, Magnus Lestelius, and Pentti Tengvall

Subjects

Surface Properties, Molecular Sequence Data, Biomedical Engineering, Complement C3c, Antibodies, Biomaterials, Contact angle, chemistry.chemical_compound, Adsorption, Spectroscopy, Fourier Transform Infrared, Amino Acid Sequence, Cysteine, 3-Mercaptopropionic Acid, Complement Activation, Chromatography, Blood Proteins, Kallikrein, Glutathione, Blood proteins, Complement system, chemistry, Kallikreins, Gold

Abstract

3-Mercaptopropionic acid (MPA), L-cysteine (L-cys), and glutathione (GSH) monolayers were immobilized onto gold and used in in vitro protein tests. The surfaces were characterized with ellipsometry, static contact angle measurements, atomic force microscopy, and Fourier transform infrared reflection absorption spectroscopy (FT-IRAS). After incubations in human plasma and antibody solutions, the surface antisera binding patterns were determined with ellipsometry. Using serum instead of plasma, complement activation was studied in the same fashion. Activated coagulation Factor XII and kallikrein formation on the surfaces and in the plasma were studied using a kallikrein-specific colorimetric assay. 3-Mercaptopropionic acid indicated contact activation of coagulation but L-cysteine did not. Glutathione displayed low deposition of plasma proteins, large deposition of proteins from serum, and did not promote kallikrein formation. None of the surfaces could be attributed complement activating properties, as determined by antibody deposition. The present study demonstrates that surface biology in complex model systems can be conveniently studied in vitro through systematic and well defined surface modifications.

Published

1994

109. Effect of gamma-interferon on the synthesis of the functional alternative and terminal comdement pathways by human umbilical vein endothelial cellsin vitro

Author

Egil Johnson, Viktor Berge, and M. Nazir

Subjects

Microbiology (medical), Umbilical Veins, medicine.medical_treatment, Complement Pathway, Alternative, Radioimmunoassay, Down-Regulation, Complement Membrane Attack Complex, Biology, Culture Media, Serum-Free, Umbilical vein, Pathology and Forensic Medicine, Interferon-gamma, Antibody Specificity, medicine, Humans, Immunology and Allergy, Interferon gamma, Cells, Cultured, General Medicine, Molecular biology, In vitro, Complement system, Endothelial stem cell, Cytokine, Complement C3c, Complement C3b, Immunology, Alternative complement pathway, Endothelium, Vascular, medicine.drug

Abstract

The cytokine gamma-interferon (gIFN) has been reported to modulate synthesis by endothelial cells (EC) of alternative pathway complement factors (H, I, and B). However, the net effect of gIFN on the synthesis and expression of the functional alternative and terminal pathways has not yet been reported. EC cultured under serum-free conditions were treated with different concentrations of gIFN and simultaneously co-incubated with agarose beads, which activate the alternative pathway. C3b and the terminal complement complex (TCC) bound to co-incubated beads were measured by radioimmunoassay using anti-human C3c and TCC antibodies. gIFN in concentrations 500-4000 U/ml increasingly reduced the amount of C3b and TCC detected on the beads. The down-regulating effect of gIFN on EC complement biosynthesis may be physiologically relevant by locally controlling complement activation.

Published

1994

110. Association of heart structure and function abnormalities with laboratory findings in patients with systemic lupus erythematosus

Author

Magdalena Kostkiewicz, Piotr Podolec, Krzysztof Gryga, Wojciech Płazak, Jacek Musiał, M Podolec, and Mamert Milewski

Subjects

Adult, Male, Technetium Tc 99m Sestamibi, medicine.medical_specialty, Systemic blood, Coronary artery disease, Young Adult, Rheumatology, immune system diseases, Internal medicine, Medicine, Humans, Lupus Erythematosus, Systemic, In patient, Young adult, skin and connective tissue diseases, Aged, Tomography, Emission-Computed, Single-Photon, Lupus erythematosus, business.industry, Myocardium, Complement C4, Heart, Middle Aged, medicine.disease, Prognosis, C-Reactive Protein, Echocardiography, beta 2-Glycoprotein I, Antibodies, Anticardiolipin, Complement C3c, Lupus Coagulation Inhibitor, Immunology, Hypertension, Cardiology, Female, Radiopharmaceuticals, business, Heart structure

Abstract

Conventional risk factors of coronary artery disease fail to explain the increased frequency of cardiovascular morbidity in patients with systemic lupus erythematosus (SLE). The study was conducted to determine possible association between the heart structure and function abnormalities with established prognostic value assessed by non-invasive imaging techniques and markers of autoimmune and inflammatory phenomena typical for SLE. Echocardiography and single photon emission computerized tomography (SPECT; Tc-99m-MIBI) at rest were performed in 60 SLE patients in a stable clinical condition of their disease. Laboratory evaluation included serum levels of C-reactive protein (CRP), complement C3c and C4 components and antiphospholipid antibodies (aPL). The latter included serum anticardiolipin (aCL) and anti-β2-glycoprotein I (antiβ2GPI) antibodies, both of IgG and IgM class, and lupus anticoagulant (LA) in plasma. Echocardiography revealed pathologic thickening of valvular leaflets and/or pericardium in more than 60% of patients. Right ventricular systolic pressure (RVSP) was elevated (>30 mmHg) in 16.7%. Myocardial perfusion defects were present in 36.7% of patients, despite normal ECG recordings and a lack of clinical symptoms of myocardial ischaemia. There was a significant association between thickening of valvular leaflets and/or pericardium and high CRP and low C3c and C4 concentrations. On the other hand, increased RVSP and the presence of myocardial perfusion defects were associated with the presence of anticardiolipin and antiβ2GPI antibodies of the IgG class. Increased anticardiolipin IgG levels predicted perfusion defects in SPECT study with 100% sensitivity and 68% specificity, whereas elevated antiβ2GPI IgG levels predicted RVSP elevation (>30 mmHg) with 100% sensitivity and 78% specificity. In stable SLE patients pericardial and valve abnormalities may be associated with markers of an ongoing inflammation. Also, pulmonary systolic pressure elevation and myocardial perfusion defects are combined with elevated levels of anticardiolipin and antiβ2GPI antibodies of the IgG class. These results indicate that even clinically silent pulmonary hypertension and myocardial perfusion defects in SLE patients could be causally related to the presence of antiphospholipid antibodies.

Published

2011

111. Isolation of the porcine complement activation fragments C3c and C3d and their use in the preparation of monospecific antibodies

Author

Ulf R. Nilsson and Karl-Erik Storm

Subjects

Immunodiffusion, Swine, Immunoblotting, Immunology, Antibodies, Immunoenzyme Techniques, Animal model, Biological fluids, Animals, Complement Activation, Immunoelectrophoresis, Polyacrylamide gel electrophoresis, General Veterinary, biology, Isolation (microbiology), Molecular biology, Complement (complexity), Complement system, Biochemistry, Complement C3d, Polyclonal antibodies, Complement C3c, Chromatography, Gel, biology.protein, Electrophoresis, Polyacrylamide Gel, Rabbits, Antibody

Abstract

The hemolytic test to date has been the sole analytic technique applied to study the complement reaction in the swine. To improve the analytical possibilities for this species we have developed polyclonal antibody reagents with specificities for the C3c and C3d activation fragments of swine C3. Access to these reagents, by which activation products can be analysed in tissues and biological fluids, will offer new possibilities for a more precise analysis of the complement reaction.

Published

1993

112. Serological findings in patients with allergic bronchopulmonary aspergillosis during remission

Author

Banani Banerjee, P.K. Bhatnagar, and P. Usha Sarma

Subjects

Male, Microbiology (medical), Allergy, Antigen-Antibody Complex, Aspergillosis, Immunoglobulin G, Serology, Immune system, Immunopathology, medicine, Humans, Mycosis, biology, business.industry, Aspergillosis, Allergic Bronchopulmonary, Remission Induction, medicine.disease, Infectious Diseases, Complement C3c, Acute Disease, Immunology, biology.protein, Female, Allergic bronchopulmonary aspergillosis, business

Abstract

The concentrations of total IgG, complement C3 and circulating immune complexes (CIC) were studied in 15 patients with allergic bronchopulmonary aspergillosis (ABPA) during remission and compared with those of 10 matched controls. The concentrations of complement and circulating immune complexes were similar to those of the controls but 33% of patients with ABPA in remission still had circulating immune complexes, mainly of IgG. Even so, the concentrations of IgG were significantly higher in patients during remission compared to controls but were lower than those observed during the acute stage of ABPA.

Published

1993

113. Specific interactions of polystyrene biomaterials with factor D of human complement

Author

Manuel Pascual, Denis Labarre, Béatrice Montdargent, Olivier Plastre, and Jürg A. Schifferli

Subjects

chemistry.chemical_classification, Proteases, biology, Biocompatibility, Chemistry, Complement Pathway, Alternative, Biophysics, Biocompatible Materials, Bioengineering, Complement system, Biomaterials, Serine, Enzyme, Coagulation, Biochemistry, Mechanics of Materials, Complement C3c, Ceramics and Composites, Alternative complement pathway, biology.protein, Humans, Polystyrenes, Complement Factor D, Electrophoresis, Polyacrylamide Gel, Factor D

Abstract

The contact of blood with some biomaterials results in complement activation, primarily by the alternative pathway (AP). Insoluble polystyrene derivatives bearing isolated sulphonate groups (PSSO3) deplete complement, whereas identical surfaces substituted with both sulphonate and hydroxymethyl groups (PSCH2OH-SO3) are non-activators. Polystyrene sulphonate derivatives possess high adsorptive properties, particularly for serine proteases of the coagulation cascade. Thus, we studied the interactions between polystyrene derivatives and factor D, an enzyme essential for AP activation. C3 was activated when normal human serum (NHS) was incubated with PSSO3, whereas PSCH2OH-SO3 did not induce any specific C3 activation. Both polymers adsorbed factor D from serum, as shown by the loss of haemolytic factor D from NHS incubated with the polymers and by the specific adsorption of radiolabelled factor D. When bound to the polymers, factor D was not functional. The disappearance of factor D was in contradiction to the observed complement activation induced by PSSO3. When other AP components were studied, it was evident that PSSO3 adsorbed factor H even more rapidly and efficiently than factor D. Thus, the net effect was an immediate deregulation of the AP resulting in C3 activation, followed by inhibition of the AP when factor D was finally depleted. Pre-exposure of PSSO3 to NHS prevented any complement activation because the polymer was saturated with factor H, but still adsorbed factor D. Such properties could be beneficial during haemodialysis with membranes for uremic patients who have increased levels of factor D in their serum.

Published

1993

114. Progesterone and dexamethasone inhibition of estrogen-induced synthesis of DNA and complement in rat uterine epithelium: Effects of antiprogesterone compounds

Author

Robert M. Bigsby

Subjects

medicine.medical_specialty, medicine.drug_class, Endocrinology, Diabetes and Metabolism, Clinical Biochemistry, Uterus, Biology, Biochemistry, Dexamethasone, Epithelium, chemistry.chemical_compound, Receptors, Glucocorticoid, Endocrinology, Glucocorticoid receptor, Internal medicine, medicine, Animals, Estrenes, Molecular Biology, Progesterone, Estradiol, DNA synthesis, Cell growth, Antiglucocorticoid, Epithelial Cells, Biological activity, DNA, Cell Biology, Rats, Mifepristone, medicine.anatomical_structure, chemistry, Estrogen, Complement C3c, Molecular Medicine, Electrophoresis, Polyacrylamide Gel, Female, Progestins, Cell Division, hormones, hormone substitutes, and hormone antagonists, Glucocorticoid, medicine.drug

Abstract

Progesterone (P) blocks estrogen induction of cell proliferation and synthesis of complement C3 in the epithelium of the immature rat uterus. Here it is shown that dexamethasone (Dex) exerts a similar inhibitory effect on these two parameters. Furthermore, analysis of the newly synthesized, secreted proteins produced during a 20 h explant culture period showed that not only does the uterus synthesize complement C3 but it is capable of proteolytically cleaving complement into its biologically active peptides. Since large doses of P are required for its inhibitory effects and since P can interact with the glucocorticoid receptor (GR), the role of the GR in mediating the P effect was questioned. Two antiprogesterone compounds with reportedly differing antiglucocorticoid activity, ZK98.734 and RU486, were tested for their ability to antagonize the inhibitory actions of P and Dex. Attenuation of estrogen-induced epithelial DNA synthesis by either P or Dex was fully overcome by concurrent administration of either ZK98.734 or RU486. On the other hand, while either antagonist was effective against the inhibitory action of P on estrogen-induced complement C3 synthesis, only ZK98.734 was fully effective in blocking inhibition by Dex. Thus, unlike its activity in rat hepatic cells, ZK98.734 is a potent antiglucocorticoid in the immature rat uterus. Because of this antiglucocorticoid activity, differential antagonism of the P response was not possible using these two steroid analogs. Although these observations support the notion of GR mediated inhibition of estrogen action in the uterus, they do not answer the question of whether P might act through a GR mediated pathway.

Published

1993

115. Antiandrogenic property of RU 486: Enhancement of estrogen-induced uterine peroxidase activity in the rat

Author

Anne-Marie Newcombe, C. Richard Lyttle, and Peter H. Jellinck

Subjects

medicine.medical_specialty, medicine.drug_class, Endocrinology, Diabetes and Metabolism, medicine.medical_treatment, Clinical Biochemistry, Uterus, Biochemistry, Steroid, Flutamide, Rats, Sprague-Dawley, chemistry.chemical_compound, Endocrinology, Internal medicine, medicine, Animals, Testosterone, Receptor, Molecular Biology, Progesterone, Estradiol, biology, Cell Biology, Mifepristone, Rats, medicine.anatomical_structure, Peroxidases, chemistry, Estrogen, Complement C3c, biology.protein, Molecular Medicine, Female, hormones, hormone substitutes, and hormone antagonists, medicine.drug, Peroxidase

Abstract

The contragestational steroid RU 486 enhanced the increase in peroxidase activity produced by estradiol in estrogen-primed immature rat uteri and, like the antiandrogen flutamide, RU 486 reversed the inhibitory effect of testosterone on this estrogen-induced response. It antagonized the inhibition produced by progesterone but had no effect on peroxidase induction by itself or in unprimed immature animals. RU 486 also enhanced the effect of estradiol on the synthesis of complement component C3 in the rat uterus. The results confirm that RU 486 possesses antiandrogenic as well as antiprogestational properties. They also suggest that, in normal adult animals, the increase in peroxidase activity in the uterus in response to estrogen is not expressed fully but held in check by other endogenous steroids acting through their individual receptors.

Published

1993

116. Complement activation in septic baboons detected by neoepitope-specific assays for C3b/iC3b/C3c, C5a and the terminal C5b-9 complement complex (TCC)

Author

Peter Garred, K Høgåsen, H Redl, G Schlag, T. Lea, Lars Speilberg, Anders Bengtsson, Tom Eirik Mollnes, Otto Götze, and Martin Oppermann

Subjects

Male, medicine.drug_class, Immunology, Complement C5a, Complement Membrane Attack Complex, Cross Reactions, Monoclonal antibody, Epitopes, Mice, Immune system, In vivo, biology.animal, medicine, Animals, Humans, Immunology and Allergy, Complement Activation, biology, Bacterial Infections, Complement system, Polyclonal antibodies, Complement C3c, Complement C3b, biology.protein, iC3b, Antibody, Papio, Research Article, Baboon

Abstract

SUMMARY We have investigated the cross-reactivity of various species in ncocpitope-specific methods for quantification of human complement aclivatlon products. In contrast to most other species examined, baboon showed a substantial cross-reactivity supporting a high degree of homology between human and bahoon complement. An assay for C3b, iC3b and C3c (MoAh bH6) showed moderately good reactivity, in contrast to a C3a assay which did not cross-react. Excellent reactivity was found for C5a using MoAbs C17/5 and G25/2. The reactivity of an established TCC assay (MoAb aEU to a C9 neoepitopc and polyclonal antibody to C5) was improved substantially by replacing the anti-C5 antibody with a new MoAb to C6 particularly selected on the basis of baboon cross-reactivity. Plasma samples from baboons receiving 2·5 · 109 and 1·0 ± 1·010 live Escherichia coli bacteria/kg were examined with the assays described. In vivo complement aetivation with the lowest dose was moderate and kept under control, in contrast to the highest dose, where an uncontrolled increase in all activation products continued throughout the infusion period. These results support the hypothesis that sufficiently high amounts of endotoxin lead to uncontrolled activation of complement as seen in irreversible septic shock. The results arc discussed with particular emphasis on activation of the terminal complement pathway.

Published

1993

117. Complement activation in stored platelet concentrates

Author

V. D. Miletic and O. Popovic

Subjects

Blood Platelets, Gel electrophoresis, Chemistry, Blotting, Western, Immunology, Fluorescent Antibody Technique, Complement C4, Hematology, Peptide Fragments, Immune complex, Complement system, Blot, Biochemistry, Blood product, Complement C3c, Complement C3b, Complement C4b, Alternative complement pathway, Humans, Immunology and Allergy, Platelet, Binding Sites, Antibody, Platelet activation, Complement Activation

Abstract

Activation of platelets during preparation and/or storage of platelet concentrates in plastic containers at room temperature has recently been recognized. Many different biologic causes of this activation have been postulated. Activated complement, as a multi-enzyme system, is one of the possible sources of molecules leading to platelet activation. To detect complement activation, functional complement activity and the generation of complement-derived ligands were investigated in platelet concentrate supernatant plasma during 5 days of storage at room temperature. Hemolytic tests for functional classical and alternative pathway activity were used, as was the kinetic test for complement-mediated inhibition of immune complex precipitation. The presence of C3 activation products (C3, C3c, C3dg) was investigated in plasma by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and Western blotting procedures and on platelets by immunofluorescence. Activation of complement was evident during storage, and C3c and C3d fragments were clearly demonstrated in plasma. The amount of C3d fragments on platelets gradually rose during the first 3 days of storage. At the end of 5 days of storage, the platelets became C3d negative. There are two possible mechanisms of C3d disappearance--shedding and/or further degradation of C3d fragments. Those results indicated that complement activation and the generation of complement-dependent ligand-receptor interaction may be mechanisms for platelet activation in concentrates stored at room temperature.

Published

1993

118. Estimation of the genetic variation in complement activity of common carp (Cyprinus carpio L.)

Author

W.B. van Muiswinkel, T. Yano, and Geert F. Wiegertjes

Subjects

Male, Carps, Erythrocytes, Lysis, Complement Pathway, Alternative, Immunology, Complement Hemolytic Activity Assay, Cyprinus, Hemolysin Proteins, Common carp, Genetic variation, Life Science, Animals, Carp, Immunoelectrophoresis, Experimental Animal Morphology and Cell Biology, General Veterinary, biology, Genetic Variation, Hemolysin, Biological activity, biology.organism_classification, Molecular biology, Experimentele diermorfologie en celbiologie, Complement C3c, Alternative complement pathway, Female

Abstract

The complement status of hybrid, laboratory raised carp was determined by an in vitro approach of the alternate complement activity (ACH50) and total haemolytic activity (CH50), and by measurement of serum C3 levels. The lysis of target sheep red blood cells (RBC) in the haemolytic assay for CH50 activity depended, amongst others, on the haemolysin concentration in the assay. Rocket electrophoresis showed a mean serum C3 concentration of 0.95 mg ml−1. The variation for both ACH50 and CH50 haemolytic activity was approximately 30%. The degree of genetic determination of the parameters was investigated by estimation of their repeatabilities, which were relatively high for CH50 (0.71) and ACH50 activity (0.72), but lower for C3 levels (0.54). Correlations between ACH50 values and C3 levels were significant, but moderate (0.54–0.58).

Published

1993

119. Regulation by sulphonate groups of complement activation induced by hydroxymethyl groups on polystyrene surfaces

Author

Marcel Jozefowicz, Denis Labarre, Béatrice Montdargent, Françoise Maillet, Marie Paule Carreno, and Michel Kazatchkinet

Subjects

Materials science, Biophysics, Biocompatible Materials, Bioengineering, Complement C3-C5 Convertases, In Vitro Techniques, Biomaterials, chemistry.chemical_compound, Adsorption, Polymer chemistry, Humans, Hydroxymethyl, Complement Activation, chemistry.chemical_classification, Benzenesulfonates, Blood Proteins, Polymer, C3-convertase, Complement system, Sulfonate, chemistry, Mechanics of Materials, Complement C3c, Ceramics and Composites, Alternative complement pathway, Polystyrenes, Polystyrene

Abstract

Reducing the complement-activating capacity of a polymer surface is important in improving its blood compatibility. Polystyrene surfaces bearing hydroxymethyl (CH 2 OH) groups activate the alternative pathway of complement. This activation depends strongly on the density of the groups. Polystyrene surfaces bearing sulphonate (SO 3 − ) groups adsorb proteins, resulting in an apparent activation. Polystyrene surfaces bearing both types of groups in close proportions are not activators in human serum, due to the adsorption of a protein of the alternative pathway, which has a protecting effect, not found when a polymer surface bearing hydroxyl groups is mixed in serum with another polymer surface bearing SO 3 − groups. In the presence of purified proteins of alternative pathway, C3 convertase activity can be created on each of these surfaces by deposition of C3b, but their susceptibility to inactivation by regulatory proteins H and I depends on the types of chemical groups present on the surface and whether the surfaces were passivated or not before C3b deposition.

Published

1993

120. Deposition of complement C3c, immunoglobulin (Ig)G4 and IgG at the basement membrane of pancreatic ducts and acini in autoimmune pancreatitis

Author

Detlefsen, S, Bräsen, Jh, Zamboni, Giuseppe, Capelli, Paola, and Klöppel, G.

Subjects

IgG4, Male, granulocytic epithelial lesions (GELs), Pancreatitis, Alcoholic, immune complex, Pancreatic Ducts, complement C3, Middle Aged, autoimmune pancreatitis, Immunohistochemistry, Basement Membrane, Autoimmune Diseases, Complement C3c, Immunoglobulin G, Pancreatitis, Chronic, immunopathology, Humans, Female, Aged

Abstract

Autoimmune pancreatitis (AIP) is a type of pancreatitis whose immunopathogenesis is still unknown. It has been reported that renal biopsy specimens from patients diagnosed with both AIP and tubulointerstitial nephritis reveal deposits containing complement C3, immunoglobulin (Ig)G and IgG4 at the tubular basement membranes (BMs). The aim was to investigate the deposition of complement and immunoglobulins in pancreatic tissue from AIP patients compared to non-AIP patients.Double immunofluorescence microscopy for C3c, IgG4 and IgG together with CK7, trypsin, collagen IV, CD31 and CD79a, as well as immunofluorescence microscopy for C1q, IgA and IgM, were performed on frozen pancreatic tissue from AIP and alcoholic chronic pancreatitis (ACP) patients.In AIP patients, complement C3c, IgG4 and IgG were deposited at the collagen IV-positive BMs of pancreatic and bile ducts and of acini. In a minority of the ACP patients, weak C3c-positive BM deposits were detected, but no IgG4- or IgG-positive BM deposits were present.The deposition of C3c, IgG4 and IgG at the BM of small- and medium-sized ducts and acini of the pancreas is characteristic of AIP. This suggests that immune complex-mediated destruction of ducts and acini play a role in the pathogenesis of AIP.

Published

2010

121. P1‐366: Microtubule destabilization leads to APP phosphorylation and processing: Implications for Alzheimer's disease pathogenesis

Author

Lisa Hornbeck, Jaya Padmanabhan, and Tina Fiorelli

Subjects

Pathology, medicine.medical_specialty, Amyloid, Microglia, biology, Epidemiology, animal diseases, Health Policy, Amyloidosis, medicine.disease, Complement C3c, nervous system diseases, Complement system, Psychiatry and Mental health, Cellular and Molecular Neuroscience, medicine.anatomical_structure, Developmental Neuroscience, Ubiquitin, mental disorders, medicine, biology.protein, Immunohistochemistry, Neurology (clinical), Cerebral amyloid angiopathy, Geriatrics and Gerontology

Abstract

However, also prion proteins produced by neurons, can form amyloid plaques in the brain. In variant Creutzfeldt Jakob disease (vCJD), sporadic CJD forms with a longer duration, hereditary CJD and Gerstmann Straussler Scheinker’s disease (GSS) prion amyloid plaques can be found. In the present immunohistochemical study we investigated the presence of amyloid associated proteins such as complement and alpha1-antichymotrypsin (ACT), microglia (HLADR), ubiquitin and tau in 4 different forms of prion diseases with prion amyloid plaques with or without prion cerebral amyloid angiopathy (CAA) and compared the results with the findings in classical AD. Methods: Cortical tissue obtained at autopsy was used from 3 vCJD (16, 37 and 49 y old), 2 sporadic CJD patients with longer duration (MM2, VV2 forms; resp. 55 y and 58 y) and 3 different GSS patients (57y, 57y, 45y) including 2 novel prion mutations, i.e. Y226X and Q227X stop codon mutations, and 5 AD cases (29y 76y). Immunohistochemistry was performed on formalin fixed tissue using antibodies against Abeta 1-17, prion proteins (3F4), complement C3b, HLADR, ubiquitin and Tau (AT8) and some sections were counterstained with Congo red. Cryostat sections were used for staining with antibodies against complement C3c and ACT. Results: Complement proteins were found in amyloid deposits both in AD and in prion diseases without Abeta. In a case with extensive prion CAA, complement was also detected in the amyloidotic vessel wall. Clustering of microglia was seen both in AD plaques and around prion plaques but also around prion CAA. Extensive neurofibrillary degeneration with numerous tangles throughout the cortex was found in the stopcodon Q227X patient (aged 45y) mimicking the AD cases. In the MM2 prion case (55 y) tau and ubiquitin was found especially near prion plaques. Prion CAA showed a mild tau and ubiquitin positivity around the vessel walls. No tau was found in the vCJD cases. Conclusions: Inflammatory changes and neurofibrillary degeneration seems to be related to cerebral amyloidosis irrespective the type of amyloid.

Published

2010

122. Generation of a C3c specific monoclonal antibody and assessment of C3c as a putative inflammatory marker derived from complement factor C3

Author

Børge Teisner, Yaseelan Palarasah, Claus Koch, Lars Vitved, Mikkel-Ole Skjoedt, Jette Brandt, and Karsten Skjødt

Subjects

Male, medicine.drug_class, Denmark, Immunology, Blood Donors, Enzyme-Linked Immunosorbent Assay, Complement factor I, Monoclonal antibody, Sensitivity and Specificity, Mice, Affinity chromatography, In vivo, Antibody Specificity, medicine, Immunology and Allergy, Animals, Humans, Complement Activation, Inflammation, Mice, Inbred BALB C, biology, Chemistry, Antibodies, Monoclonal, Molecular biology, In vitro, Complement system, Complement C3c, biology.protein, iC3b, Female, Antibody, Inflammation Mediators, Biomarkers

Abstract

There is a general need for markers of systemic inflammation in acute or chronic diseases, where complement activation is involved. Available methods to monitor complement activation are elaborate and of low sensitivity; they include haemolytic assays (CH50), quantification of fluid phase terminal complex (C5b-C9) and quantification of complement split products by precipitation-in-gel techniques (e.g. C3d). We have developed a mouse monoclonal antibody (mAb) that is able to detect fluid phase C3c without interference from other products generated from the complement component C3. The C3c specific mAb was tested in different ELISA combinations with various types of in vitro activated sera and with plasma or serum samples from factor I deficient patients. The specificity of the mAb was evaluated in immunoprecipitation techniques and by analysis of eluted fragments of C3 after immunoaffinity chromatography. The C3c mAb was confirmed to be C3c specific, as it showed no cross-reactivity with native (un-cleaved) C3, with C3b, iC3b, or with C3d. Also, no significant reaction was observed with C3 fragments in factor I deficient sera or plasma. This antibody forms the basis for the generation of a robust ELISA that allows for a quick and reliable evaluation of complement activation and consumption as a marker for inflammatory processes. We established the C3c plasma range in 100 healthy Danish blood donors with a mean of 3.47 μg/ml and a range of 2.12-4.92 μg/ml. We believe that such an antibody might be of potential value in the assessment of in vivo complement activity during the inflammatory processes.

Published

2010

123. Human intestinal ischemia-reperfusion-induced inflammation characterized: experiences from a new translational model

Author

Joep, Grootjans, Kaatje, Lenaerts, Joep P M, Derikx, Robert A, Matthijsen, Adriaan P, de Bruïne, Annemarie A, van Bijnen, Ronald M, van Dam, Cornelis H C, Dejong, and Wim A, Buurman

Subjects

Aged, 80 and over, Inflammation, Male, Interleukin-6, Tumor Necrosis Factor-alpha, Interleukin-8, Middle Aged, Immunohistochemistry, Tissue Culture Techniques, Complement C3c, Reperfusion Injury, Intestine, Small, Humans, Female, Aged, Regular Articles

Abstract

Human intestinal ischemia-reperfusion (IR) is a frequent phenomenon carrying high morbidity and mortality. Although intestinal IR-induced inflammation has been studied extensively in animal models, human intestinal IR induced inflammatory responses remain to be characterized. Using a newly developed human intestinal IR model, we show that human small intestinal ischemia results in massive leakage of intracellular components from ischemically damaged cells, as indicated by increased arteriovenous concentration differences of intestinal fatty acid binding protein and soluble cytokeratin 18. IR-induced intestinal barrier integrity loss resulted in free exposure of the gut basal membrane (collagen IV staining) to intraluminal contents, which was accompanied by increased arteriovenous concentration differences of endotoxin. Western blot for complement activation product C3c and immunohistochemistry for activated C3 revealed complement activation after IR. In addition, intestinal IR resulted in enhanced tissue mRNA expression of IL-6, IL-8, and TNF-alpha, which was accompanied by IL-6 and IL-8 release into the circulation. Expression of intercellular adhesion molecule-1 was markedly increased during reperfusion, facilitating influx of neutrophils into IR-damaged villus tips. In conclusion, this study for the first time shows the sequelae of human intestinal IR-induced inflammation, which is characterized by complement activation, production and release of cytokines into the circulation, endothelial activation, and neutrophil influx into IR-damaged tissue.

Published

2010

124. Unusual variants of pemphigoid: from pruritus to pemphigoid nodularis

Author

Hiroshi Shimizu, P. H. McKee, J. S. Ross, W. A. D. Griffiths, Martin M. Black, N. P. Smith, and Balbir S. Bhogal

Subjects

Pathology, medicine.medical_specialty, Pemphigoid, Histology, Immunoblotting, Fluorescent Antibody Technique, Dermatology, Pathology and Forensic Medicine, Blister, Antigen, Prurigo, Pemphigoid, Bullous, medicine, Humans, skin and connective tissue diseases, Direct fluorescent antibody, Aged, Skin, integumentary system, business.industry, Pruritus, Genetic Variation, Middle Aged, medicine.disease, Lamina lucida, Microscopy, Electron, Complement C3c, Immunoglobulin G, Pemphigoid nodularis, Female, Bullous pemphigoid, business

Abstract

We report three patients with pemphigoid nodularis. Patients were females aged 76, 71 and 50 years, and all had features of bullous pemphigoid together with prurigo-like lesions at some stage of their illness. In two cases, nodular lesions preceded the onset of blistering by some months. Blisters arose on normal skin and in one patients also at sites of prurigo lesions. Routine histology of bullous lesions revealed the presence of subepidermal blisters. Electron microscopy performed in two cases confirmed the level of split to be through the lamina lucida. Direct immunofluorescence in all cases was positive, with linear basement membrane zone deposition of IgG and C3. Circulating IgG anti-basement membrane antibody was also detected in all patients, and in two, immunoblotting revealed a single antigen of 220 kD.

Published

1992

125. Urticarial vasculitis: A histopathologic and clinical review of 72 cases

Author

Darius R. Mehregan, Lawrence E. Gibson, and Matthew J. Hall

Subjects

Male, Vasculitis, Abdominal pain, Pathology, medicine.medical_specialty, Urticaria, Biopsy, Immunoglobulins, Dermatology, Necrotizing Vasculitis, medicine, Humans, Urticarial vasculitis, Skin, Angioedema, medicine.diagnostic_test, business.industry, Middle Aged, medicine.disease, Neutrophilia, Purpura, Complement C3c, Female, medicine.symptom, business

Abstract

Background: Urticarial vasculitis is a subset of vasculitis characterized clinically by urticarial skin lesions and histologically by necrotizing vasculitis. Objective: A review of patients with urticarial vasculitis was undertaken to further characterize the clinical and histologic findings and to differentiate this disorder from urticaria and other types of cutaneous vasculitis. Methods: Seventy-two cases of biopsy-proven urticarial vasculitis were selected for a review of medical records, laboratory data, and histologic findings. Fifty cases of simple urticaria were also reviewed for purposes of comparison. Results: Systemic symptoms in patients with urticarial vasculitis included angioedema in 30 patients (42%), arthralgias in 35 (49%), pulmonary disease in 15 (21%), and abdominal pain in 12 (17%). Twenty-three patients (32%) had hypocomplementemia. Forty-six of 72 patients (64%) had lesions that lasted more than 24 hours, 23 of 72 (32%) had painful or burning lesions, and 25 of 72 (35%) had lesions that resolved with purpura. Sixteen biopsy specimens from the 23 patients with hypocomplementemia showed dermal neutrophilia in addition to the perivascular infiltrate. Of the 23 patients with hypocomplementernia, 20 (87%) had fluorescence of the blood vessels and 16 (70%) had fluorescence of the basement membrane zone as determined by routine direct immunofluorescence. Conclusion: Patients with hypocomplementemia were more likely to have systemic symptoms such as urticaria that resolved with purpura, arthralgias, abdominal pain, and chronic obstructive pulmonary disease. The histolog c pattern associated with hypocomplementemia is interstitial neutrophilic infiltrate of the dermis and an immunofluorescent pattern of immunoglobulins or C3 in the blood vessels and along the basement membrane zone.

Published

1992

126. Levels of Complement Receptor Type One (CR1, CD35) on Erythrocytes, Circulating Immune Complexes and Complement C3 Split Products C3d and C3c Are Not Changed by Short-Term Physical Exercise or Training

Author

B. S. Thomsen, Finn Rolsted Hansen, Bente Klarlund Pedersen, A. Rødgaard, J. Halkajoer Kristensen, N. Tvede, and J. Steensberg

Subjects

Adult, Male, medicine.medical_specialty, Erythrocytes, Physical fitness, Physical Therapy, Sports Therapy and Rehabilitation, Physical exercise, Antigen-Antibody Complex, Complement receptor, Immunoelectrophoresis, Biology, Complement C3c, Immune system, Internal medicine, medicine, Humans, Orthopedics and Sports Medicine, Exercise, Analysis of Variance, Physical Education and Training, medicine.diagnostic_test, business.industry, VO2 max, Immune complex, Receptors, Complement, Endocrinology, Physical Fitness, business

Abstract

The effect of heavy short-term physical exercise on the levels of complement receptor type one (CR1, CD35) on erythrocytes, the concentrations of circulating immune complexes (IC), and the complement C3 split products C3c and C3d were examined in young healthy males. Fourteen untrained volunteers underwent a 60-min bicycle exercise test at 75% of maximal oxygen uptake (VO2max). Six of the volunteers were exercised twice with an interval of at least one month. Before the second bicycle test they received oral indomethacin. With an interval of at least 1 week, 6 also went through a 60-min back-muscle exercise at up to 30% of VO2max. Blood samples were collected before and during the last few minutes of exercise as well as 2 h and 24 h afterwards. The same parameters were examined once in 29 highly trained racing cyclists. There were no consistent or significant exercise-induced changes in the levels of erythrocyte CR1, circulating IC, C3c nor C3d as measured by an enzyme-linked immunosorbent assay, polyethylene glycol precipitation complement consumption method, and by intermediate gel rocket immunoelectrophoresis, respectively. Neither did these parameters differ from controls in the highly trained group. The results indicate that CR1 on erythrocytes, circulating immune complexes and complement cleavage products C3c and C3d in healthy subjects remain unaffected by short-term heavy physical activity and training.

Published

1992

127. A long-term immunological study of childhood onset systemic lupus erythematosus

Author

Kue-Hsiung Hsieh and Cheng-Kai Ting

Subjects

Male, Interleukin 2, Systemic disease, Time Factors, Adolescent, Exacerbation, Immunology, CD4-CD8 Ratio, Asymptomatic, General Biochemistry, Genetics and Molecular Biology, Rheumatology, Complement C4b, medicine, Humans, Lupus Erythematosus, Systemic, Immunology and Allergy, Child, skin and connective tissue diseases, Autoimmune disease, Lupus erythematosus, business.industry, Lymphokine, Complement C4, Receptors, Interleukin-2, DNA, Prognosis, medicine.disease, Peptide Fragments, Antibodies, Antinuclear, Complement C3c, Interleukin-2, Female, medicine.symptom, Low Complement, business, Research Article, medicine.drug

Abstract

Immunological dysregulation is an important cause of the development of systemic lupus erythematosus (SLE). Serological evaluation has been useful in the clinical management of patients and as a prognostic indicator. Sixteen patients who developed SLE as children were followed up for more than three years and immunological data collected. The results showed that (a) complement C3 concentration was lower in the active stage of SLE, especially during a major clinical exacerbation, but rarely preceded a major flare up. The concentration was often normal during the mildly to moderately active stage. In contrast, a low complement C4 concentration often preceded a major clinical exacerbation and could be of longer duration, sometimes persisting regardless of disease activity. (b) A T cell subset distribution study showed persistently low CD4 positive T cells in the peripheral blood of patients with SLE during the long term follow up, strongly suggesting that the intrinsic defect is mainly localised in T helper/inducer cells. These abnormal cellular defects did not tend to return to normal even in long term remission. (c) The persistently higher serum interleukin 2 and interleukin 2 receptor concentrations in SLE strongly suggested that the T cells were preactivated in vivo and that these phenomena might persist even in remission. (d) The best single parameter for predicting active SLE was anti-dsDNA. It was highly correlated with disease activity in most patients, and the asymptomatic increase of anti-dsDNA (greater than or equal to 60 U/ml, radioimmunoassay) was often followed by a major clinical exacerbation, especially in patients with a simultaneously low complement C4 concentration, suggesting that it might be an important warning sign of a major flare up. High dose steroids are indicated in this group of patients.

Published

1992

128. Genetic associations of variants of the high affinity receptor for immunoglobulin E in Wegener's granulomatosis

Author

Marek Sanak, Jan Sznajd, Daniel P. Potaczek, Andrzej Szczeklik, and Jacek Musiał

Subjects

Male, Heterozygote, gene polymorphism, Genotype, Immunoglobulin E, Pathogenesis, Gene Frequency, Internal Medicine, Medicine, Humans, IgE receptor, Fc\varepsilonRI, Receptor, Gene, Genetic association, Polymorphism, Genetic, biology, business.industry, Receptors, IgE, Granulomatosis with Polyangiitis, hemic and immune systems, Complement C4, Middle Aged, FCER1A, Wegener's granulomatosis, C-Reactive Protein, Complement C3c, Immunology, biology.protein, Female, Antibody, business

Abstract

Immunoglobulin E (IgE) and the high affinity IgE receptor (FcepsilonRI) have been suggested to contribute to the pathogenesis of autoimmune disorders. Their role in Wegener's granulomatosis (WG) are, however, poorly recognized. We sought a genetic association between laboratory markers for the disease, i.e. anti-proteinase 3 antibodies (anti-PR3), anti-myeloperoxidase antibodies, anti-cyclic citrullinated peptide antibodies, C-reactive protein (CRP), C3c and C4 complement components, and total serum IgE levels in WG subjects with common genetic variants of FcepsilonRI subunits. Anti-PR3 and CRP and serum IgE levels showed significant associations, while complement components tended to be associated, with -18483A > C and/or -344C > T FCER1A (FcepsilonRI alpha-subunit gene) polymorphisms. Moreover, a correlation between -109T > C FCER1B (FcepsilonRI beta-subunit gene) genotypes and serum IgE was observed. Both WG specific auto-antibodies and other blood inflammatory markers displayed correlations with serum total IgE levels and genetic variants of the high affinity receptor for this immunoglobulin. This observation suggests a functional relantionship of FcepsilonRI in the regulation of autoimmune response observed in WG.

Published

2009

129. Synergistic effects of alpha-1,2-fucosyltransferase, DAF, and CD59 in suppression of xenogenic immunological responses

Author

Zhi-Fang Ma, Bing-Qian Liu, Tengxiang Ma, Yan-Chun Qu, Yue Zhang, Guangyou Wang, Rui-Fa Han, Sheng-zhi Li, and Mengsheng Qiu

Subjects

Genetically modified mouse, Graft Rejection, Fucosyltransferase, Transgene, Immunology, Transplantation, Heterologous, chemical and pharmacologic phenomena, Antibodies, Heterophile, CD59 Antigens, Mice, Transgenic, CD59, Biology, Flow cytometry, Mice, medicine, Animals, Humans, Decay-accelerating factor, Southern blot, Transplantation, medicine.diagnostic_test, CD55 Antigens, Myocardium, Complement C9, Fucosyltransferases, Molecular biology, Immunoglobulin M, Complement C3c, biology.protein, Heart Transplantation, Endothelium, Vascular

Abstract

Background: Previous studies showed that α-1,2-fucosyltransferase (HT), decay accelerating factor (DAF), and CD59 have an inhibitory effect on the immunological rejection of xenogenic transplantation. Methods: To investigate their possible synergistic effects in suppression of heterogeneic transplantation, we produced transgenic mouse lines expressing human HT, DAF, and/or CD59 by the standard pronuclear injection approach. PCR and Southern blot were used to identify the transgenic founder lines. Flow cytometry confirmed the high-level expression of HT, DAF, or CD59 in the transgenic mice. Results: The deposition of IgM, C3c, or C9 in the cardiac vascular endothelial cells of the HT, HT/CD59, and/or DAF multiple positive transgenic mice was markedly decreased. The survival time and function of the hearts of the co-transgenic mice were significantly longer and higher than that of the single HT-positive transgenic mice (P

Published

2009

130. Immunopathology of subcutaneous rheumatoid nodules

Author

T E Mollnes, O. J. Mellbye, Øystein Førre, and L Kvarnes

Subjects

Immunoglobulin A, Pathology, medicine.medical_specialty, medicine.drug_class, T-Lymphocytes, Immunology, Fluorescent Antibody Technique, Immunoglobulins, Monoclonal antibody, Autoantigens, General Biochemistry, Genetics and Molecular Biology, Immunoglobulin G, Arthritis, Rheumatoid, Rheumatology, Antigen, medicine, Humans, Immunology and Allergy, Fibrin, biology, business.industry, Macrophages, HLA-DR Antigens, Complement system, Immunoglobulin M, Complement C3c, biology.protein, Interdigitating Cells, Antibody, Rheumatoid Nodule, business, Research Article

Abstract

Nodules obtained from five patients with classical seropositive rheumatoid arthritis were studied by an immunofluorescence technique using polyclonal antibodies to IgG, IgA, IgM, C3c, and fibrin, and monoclonal antibodies to the terminal (C5b-9) complement complex (reaction with a neoantigen in C9 revealed during activation), DR antigens, T cells, macrophages, and interdigitating cells. In all instances the central necrotic areas stained strongly for fibrin and more weakly for IgG, IgA, IgM, C3, and terminal complement complex. The surrounding palisading cells reacted with antibodies to DR and macrophages. In the peripheral granulomatous tissue most of the lymphocytes reacted with the antibodies to T cells, whereas various amounts of the larger mononuclear cells were stained by antibodies to DR antigens, macrophages, and interdigitating cells. In all instances the walls of some of the smaller vessels in the granulomatous tissue stained for fibrin, C3, and terminal complement complex. Plasma cells were not seen except for scattered IgM cells in one nodule. These results support the view that the palisading cells are derived from macrophages, and indicate that there is vasculitis with activation of C3 and the terminal complement pathway in the granulomatous tissue.

Published

1991

131. Heparin reversal by protamine in humans--complement, prostaglandins, blood cells, and hemodynamics

Author

J. Hobbhahn, Peter Conzen, H. Habazettl, W. Kellermann, Klaus Peter, and R. Gutmann

Subjects

medicine.medical_specialty, Physiology, Hemodynamics, Blood Pressure, Prostacyclin, Cyclooxygenase pathway, Oxygen Consumption, Heart Rate, Physiology (medical), Internal medicine, medicine, Humans, Protamines, Pulmonary wedge pressure, Biotransformation, Aged, Arachidonic Acid, Blood Cells, biology, business.industry, Heparin Antagonists, Leukopenia, Heparin, Thrombocytopenia, Protamine, Blood Cell Count, Endocrinology, Blood pressure, Complement C3c, Anesthesia, Prostaglandins, biology.protein, Eicosanoids, lipids (amino acids, peptides, and proteins), Blood Gas Analysis, business, Transpulmonary pressure, medicine.drug

Abstract

Fourteen noncardiac surgical patients received heparin (10,000 IU), which was neutralized by 100 mg protamine injected within 2 min during steady-state anesthesia. After protamine application, plasma complement C3a, thromboxane B2 (TxB2), prostaglandin F2 alpha (PGF2 alpha) and KH2PGF2 alpha increased significantly, whereas prostacyclin (6-keto-PGF2 alpha) levels did not change. This mediator response was associated with transient leukopenia and thrombocytopenia. Arterial pressure, pulmonary arterial pressure, and transpulmonary pressure gradient increased significantly. Heart rate, cardiac output, pulmonary capillary wedge pressure, and arterial PO2 remained constant. Positive correlations of plasma C3a were observed with pulmonary leukosequestration and plasma TxB2. Inverse correlations of C3a were noted with the counts of leukocytes and of platelets. A positive correlation was found between TxB2 and pulmonary arterial pressure. Our results indicate that marked activation of the complement system and the cyclooxygenase pathway is common after heparin reversal by protamine in anesthetized patients. This is in contrast to previous human studies performed after cardiopulmonary bypass but agrees well with results obtained in animal experiments. The mediator response in our patients, however, was not accompanied by hemodynamic instability, suggesting appropriate compensatory mechanisms.

Published

1991

132. Elimination of immune precipitates from the rat corneal stroma: a histological study

Author

C. Verhagen, J. Klooster, A. C. Breebaart, René Den Heijer, and Aize Kijlstra

Subjects

Male, Pathology, medicine.medical_specialty, Inflammation, Antigen-Antibody Complex, Biology, Endoplasmic Reticulum, Cornea, Cellular and Molecular Neuroscience, Corneal Opacity, Immune system, Phagocytosis, Rats, Inbred BN, Immunopathology, medicine, Animals, Serum Albumin, Latex beads, MHC class II, Macrophages, Histocompatibility Antigens Class II, Molecular biology, Sensory Systems, Immune complex, Rats, Complement system, Microscopy, Electron, Ophthalmology, medicine.anatomical_structure, Complement C3c, biology.protein, Female, Rabbits, sense organs, medicine.symptom

Abstract

The pathogenesis of peripheral corneal lesions of immune aetiology, like Mooren's ulcer and catarrhal infiltrates, has been related to the formation or deposition of immune complexes. The present investigation was undertaken to study the mechanisms involved in the elimination of immune precipitates from the cornea. Immune precipitates were induced by injecting human serum albumin (HSA) and rabbit anti-HSA serum into opposite sites of the rat corneal stroma. This resulted in a line-shaped opacity in the stroma, which remained visible by slit-lamp for 7 days, and disappeared without clinical signs of keratitis and uveitis. At the ultrastructural level, the immune precipitates were clearly visible. Keratocytes in the vicinity of the immune precipitates appeared activated, as suggested by their less flattened appearance and well-developed rough endoplasmic reticulum. The arrangement of the collagen fibrils was not affected. Cells with a macrophage-like morphology were also present and contained electron-dense material, closely resembling the precipitate, suggesting phagocytosis. Separate corneas were injected with latex beads, which is known to induce migration of Langerhans cells into the cornea. Immunohistochemical analysis revealed that both latex beads and immune precipitates induced migration of macrophages (ED1+) into the rat corneal stroma. However, differences were observed with regard to the expression of MHC class II antigens by these ED1+ cells and the presence of complement deposits in the corneal stroma. ED1+ cells in corneas injected with latex beads were all MHC class II positive (OX4+), whereas most of the ED1+ cells at the site of the immune precipitates were negative (OX4−). Deposits of the complement activation product C3c were present in the immune complex model, but absent in the latex beads-induced reaction. These data demonstrate that immune precipitates induce migration of macrophages into the cornea, and that expression of MHC class II antigens by these cells is non-uniform. This variability may reflect the presence of subtypes of macrophages or different stages of maturation, or may be due to local stimuli like phagocytosis or complement activation.

Published

1991

133. A Functionally Active Complement System Is Present in Uterine Secretion of the Mouse Prior to Implantation

Author

Meishan Jin, Anders Larsson, and B. Ove Nilsson

Subjects

medicine.medical_specialty, Erythrocytes, Immunology, Uterus, Embryonic Development, Complement Membrane Attack Complex, Biology, Mice, Immune system, Pregnancy, Internal medicine, medicine, Animals, Immunology and Allergy, Secretion, Complement Activation, Sheep, Complement C1q, Complement C5, Obstetrics and Gynecology, Complement C4, Complement System Proteins, Cell biology, Complement system, Blot, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, Sephadex, Complement C3c, Female, Complement membrane attack complex, Immunostaining

Abstract

Sephadex beads were placed carefully in the uterus on days 2 and 3 and left for 6 to 8 h to absorb uterine secretion. The beads were then removed with volatile silicon oil and mounted on small pieces of nitrocellulose paper. Immunostaining of these bead blots showed they contained the complement components C1q, C3, C4, and C5. We demonstrated that complement component C3 in the uterine secretion could be activated and deposited on model immune complexes, and also that antibody-coated erythrocytes were lysed in utero, that is, a membrane attack complex was produced. Thus, the mouse uterine secretion at the preimplantation stage contains a functionally active complement system.

Published

1991

134. TEM immunogold staining of C3 from plasma onto titanium oxides

Author

E. S. Machlin, M. E. McAlarney, D. Neugroschl, R. Skalak, and S. Kim

Subjects

Titanium, Time Factors, Staining and Labeling, Biomedical Engineering, Oxide, Analytical chemistry, chemistry.chemical_element, Biocompatible Materials, Plasma, Immunogold labelling, Immunohistochemistry, Biomaterials, Microscopy, Electron, chemistry.chemical_compound, Colloid, Adsorption, Vroman effect, chemistry, Complement C3c, Grain boundary, Gold

Abstract

Immunogold staining in conjunction with TEM was used to observe C3 adsorption from plasma in relation to the underlying titanium structure of thermal, anodic, and electropolished oxides. Heat treatments and oxide thickness were found to have no significant effect on the adsorption behavior of C3, while surface oxide type possibly has. Surface concentration of C3 was found to be time- and plasma concentration-dependent. Evidence is given for the possible involvement of C3 in protein exchange, i.e., the Vroman effect. Diluted plasma resulted in a random distribution of gold colloids, whereas clustering occurred with undiluted plasma. Although C3 concentrations present on grain boundaries followed the same trend as that found on the surface, C3 was found to have a higher grain boundary than bulk concentration for 0.1% plasma.

Published

1991

135. Failure Co detect deposition of complement and immunoglobulin in allergen-induced late-phase skin reaction in atopic subjects

Author

A. J. Frew and A. B. Kay

Subjects

Hypersensitivity, Immediate, Pathology, medicine.medical_specialty, Allergy, Immunology, Fluorescent Antibody Technique, Immunoglobulins, Fibrinogen, Immunoglobulin E, medicine.disease_cause, Allergen, Immune system, Immunopathology, medicine, Humans, Immunology and Allergy, Skin, Skin Tests, biology, Chemistry, Complement C1q, Complement System Proteins, Allergens, medicine.disease, Immune complex, Immunoglobulin M, Complement C3c, Immunoglobulin G, biology.protein, Antibody, Research Article, medicine.drug

Abstract

SUMMARYThere still remains some controversy regarding the possible role of immune complexes in the pathogenesis of the late-phase skin reaction (LPSR). To assess this, skin biopsies were obtained from LPSR induced in atopic human subjects 6, 24 and 48 h after allergen challenge. Cryostat sections were stained by direct immunofluorescence for the presence of fibrinogen, immunoglobulin classes IgM and IgG and for the the complement components C1q and C3c. Complement components were observed in only two of the 29 biopsies studied. In both instances, only C3c was detected. One of these subjects also had unequivocal IgG staining at 6 h. IgM staining was detected in two out of 10 subjects at 6 h but no significant deposition of immunoglobulins could be found at 24 or 48 h. Fibrinogcn deposition was observed in about half of the biopsies at each time-point. This study suggests that substantial complement and immunoglobulin deposition arc not overt features of the allergen-induced LPSR. although the presence of small amounts of immune complexes, below the sensitivity of the method employed cannot be excluded. Fibrin deposition occurs in the LPSR but docs not appear to be a prerequisite for LPSR development.

Published

1991

136. Plasma C3c in immune-mediated neurological diseases: a preliminary report

Author

T. Hemachudha, Nuanthip Kamolvarin, Kammant Phanthumchinda, B. Ongpipattanakul, and Tada Sueblinvong

Subjects

Prednisolone, Polyradiculoneuropathy, Autoimmune Diseases, Immune system, Disease severity, Preliminary report, Immunopathology, Myasthenia Gravis, Blood plasma, medicine, Humans, Infusions, Intravenous, Neurologic Examination, Autoimmune disease, Plasma Exchange, Guillain-Barre syndrome, business.industry, General Medicine, medicine.disease, Myasthenia gravis, Neurology, Complement C3c, Immunology, bacteria, gamma-Globulins, Neurology (clinical), Nervous System Diseases, business, Follow-Up Studies

Abstract

Plasma C3c levels were examined in 56 patients with immune (27) and non-immune (29) mediated neurological diseases by crossed immunoelectrophoresis. Plasma samples were collected during the active phase of illness in both groups, usually within 7 days of admission. 11 patients (4 Guillain-Barré Syndrome-GBS, 3 chronic inflammatory demyelinating polyneuropathy-CIDP, 4 myasthenia gravis-MG) had their plasma saved sequentially during the active and the recovery phase. Plasma C3c levels were elevated in the group with immune mediated diseases when compared with those of non-immune mediated diseases. The sensitivity and specificity of C3c as a diagnostic test for immune mediated neurological diseases were 61.4 and 100% respectively with a positive and negative predictive value of 100 and 41%. the C3c levels in plasma correlated well with disease severity in MG and GBS patients. Such a correlation was also evident in all CIDP patients except one that had persistent elevation in the presence of clinical improvement. Results suggest that the plasma C3c level may be useful for differentiating immune from non-immune mediated neurological diseases. Plasma C3c may also be used for monitoring disease severity, particularly in myasthenia gravis.

Published

1991

137. LEVELS OF COMPLEMENT FACTOR C3 AND ITS ACTIVATED PRODUCT, C3a, IN OPERATIVELY SALVAGED BLOOD

Author

M. A. Goodman, Kishore Sieunarine, F. J. Prendergast, J. Wetherall, Michael Lawrence-Brown, and M. Hellings

Subjects

Blood Specimen Collection, business.industry, Contact system, Blood Loss, Surgical, chemical and pharmacologic phenomena, General Medicine, Plasma levels, Complement factor I, Aortic surgery, Transplantation, Autologous, Complement system, Andrology, Complement C3c, Anesthesia, Humans, Medicine, Surgery, business, Complement Activation, Autotransfusion

Abstract

In intra-operative blood salvage the collected blood is exposed to traumatized tissue and a synthetic circuit. Because of this exposure it was expected that the complement system, which is a contact system present in plasma, would be activated in salvaged blood. To determine whether this occurs, the plasma levels of the complement factor C3 and its activated fragment, C3a, were measured in intra-operative salvaged blood before and after washing. Samples were obtained from patients undergoing aortic surgery where intra-operative salvage was used. In the unwashed salvaged blood, the level of C3 fell (mean C3: 0.33 g/L) and the level of C3a increased (mean C3a: 1994 ng/mL) compared with the patient circulating levels of C3 and C3a (mean C3: 0.70 g/L, mean C3a: 855 ng/mL) respectively. Washing of the collected blood reduced the C3a level (mean: 346 ng/mL) to the patient's level and reduced C3 to the lower detection limit of the test (less than 0.2 g/L). The raised level of C3a and the reduced level of C3 confirm that the complement system is activated and imply that other complement factors are also activated.

Published

1991

138. Crosslinking with Diacrylylpiperazine (PIP) Reduces Activation of Complement by Polyacrylamide Microcapsules

Author

H. Gin, Ch. Cadic, Ch. Baquey, D. Ducassou, B. Dupuy, and A. Baquey

Subjects

Acrylamides, Biocompatibility, Polyacrylamide, Acrylic Resins, Zymosan, Biomaterial, Capsules, Complement C4, Complement C3, General Medicine, Piperazines, In vitro, Complement system, chemistry.chemical_compound, Cross-Linking Reagents, chemistry, Complement C3c, Polylysine, Materials Testing, Polymer chemistry, Diacrylylpiperazine, Biophysics, Complement Activation

Abstract

Activation of the complement system in vitro by a series of microcapsules based on polylysine, alginate or polyacrylamide was determined. Least activation was observed with microcapsules whose outer layer was composed of polyacrylamide. Activation was further reduced using diacrylylpiperazine instead of bisacrylamide as crosslinker.

Published

1991

139. Analysis of proteins eluted from hemodialysis membranes

Author

Patrice Deteix, Arlette Tridon, A.M. Françoise Gachon, and Jocelyne Mallet

Subjects

Acrylic Resins, Biomedical Engineering, Biophysics, Biocompatible Materials, Bioengineering, Chemical Fractionation, Complement C3d, Complement C3c, Dialysis tubing, Biomaterials, Hydrophobic effect, chemistry.chemical_compound, Renal Dialysis, Humans, Cellulose, Chromatography, Membranes, Artificial, Blood Proteins, Cellulose acetate, Blood proteins, Membrane, chemistry, Biochemistry, Electrophoresis, Polyacrylamide Gel, Kidneys, Artificial, Protein adsorption

Abstract

To further investigate the types of interactions occurring between blood and hemodialysis membranes, proteins were sequentially eluted from used dialysers. Four different membranes (cuprophan, hemophan, cellulose acetate and polyacrylonitrile) were successively treated with a hydrogen bond cleaving agent (10 M urea), an ionic detergent destabilizing the hydrophobic interactions between apolar groups (SDS solution), and a hydroxylamine solution at alkaline pH to release postulated covalently bound C3 fragments. The eluted proteins were analyzed by SDS-PAGE and immunological techniques. Total protein determinations demonstrate different behaviour of the membranes as regards the 'protein cake'. Electrophoretic analysis suggests that qualitative and quantitative differences in the binding of the blood proteins are related to the membrane material. Complement fragment studies indicate that the complement activating potential of the dialysis membrane may not be determined by the availability of potential binding sites for activated C3b. An attempt is made to correlate these results with the biocompatibility concept.

Published

1991

140. Activation of Rabbit C3: Studies of the Generation of Cleavage Products in vitro and of Their Metabolism in vivo

Author

J.A. Charlesworth, Philip W. Peake, and B. A. Pussell

Subjects

Complement Pathway, Alternative, Immunology, chemical and pharmacologic phenomena, In Vitro Techniques, Cleavage (embryo), In vivo, medicine, Animals, Humans, Trypsin, Complement Activation, Elapid Venoms, Catabolism, Chemistry, Complement C3, Hematology, Metabolism, In vitro, Immune complex, Biochemistry, Complement C3c, Complement C3b, Complement C3a, Autoradiography, iC3b, Electrophoresis, Polyacrylamide Gel, Rabbits, Half-Life, medicine.drug

Abstract

The cleavage of purified, functionally active rabbit C3 by cobra venom factor and trypsin was analysed by reducing and non-reducing sodium dodecyl sulphate electrophoresis and autoradiography. The specific aim of the study was to compare these reactions to those that occur with human C3. Analysis showed that the pattern of breakdown was very similar to that for the human protein: while the beta-chain remained intact, there was step-wise degradation of the alpha-chain to form C3a, C3b, iC3b and C3c, all of which could be identified by gel analysis. The metabolic behaviour of three of these cleavage products, C3a, C3b and iC3b, was then examined in vivo using dual isotope techniques. Rabbits were studied simultaneously with 131I-C3 and 125I-labelled C3 breakdown products. Analysis of plasma and urine radioactivity for the subsequent 72 h showed that all three breakdown proteins had rapid rates of catabolism in vivo compared to the native molecule. Specifically, 93 and 98% of C3b and iC3b, respectively, were eliminated from the plasma compartment within 10 h of injection. C3a was completely eliminated within 10 h. By comparison, native C3 showed a half-life of 29 +/- 3 h (mean +/- SD) and a fractional catabolic rate of 4.30 +/- 0.75%/h. The data support the use of this species in studies of complement behaviour in models of human immune disease and further clarify the basis for changes in plasma C3 concentration that accompany active immune complex- and antibody-mediated activity, in vivo.

Published

1991

141. Innate Immunity and Inflammation in Temporal Lobe Epilepsy: New Emphasis on the Role of Complement Activation

Author

Annamaria Vezzani

Subjects

Adult, Male, Adolescent, Complement C5b, Inflammation, Status epilepticus, Hippocampal formation, Epileptogenesis, Hippocampus, Rats, Sprague-Dawley, Classical complement pathway, Status Epilepticus, Basic Science, medicine, Animals, Humans, Gliosis, RNA, Messenger, Aged, Hippocampal sclerosis, business.industry, Complement C1q, Complement System Proteins, Middle Aged, Entorhinal cortex, medicine.disease, Complement system, Rats, Up-Regulation, Disease Models, Animal, nervous system, Epilepsy, Temporal Lobe, Complement C3d, Astrocytes, Complement C3c, Immunology, Encephalitis, Female, Neurology (clinical), Microglia, medicine.symptom, business, Neuroscience

Abstract

Complement Activation in Experimental and Human Temporal Lobe Epilepsy. Aronica E, Boer K, van Vliet EA, RedekerS, Baayen JC, Spliet WG, van Rijen PC, Troost D, da Silva FH, Wadman WJ, Gorter JA. Neurobiol Dis 2007;26(3):497–511. We investigated the involvement of the complement cascade during epileptogenesis in a rat model of temporal lobe epilepsy (TLE), and in the chronic epileptic phase in both experimental as well as human TLE. Previous rat gene expression analysis using microarrays indicated prominent activation of the classical complement pathway which peaked at 1 week after SE in CA3 and entorhinal cortex. Increased expression of C1q, C3 and C4 was confirmed in CA3 tissue using quantitative PCR at 1 day, 1 week and 3–4 months after status epilepticus (SE). Upregulation of C1q and C3d protein expression was confirmed mainly to be present in microglia and in a few hippocampal neurons. In human TLE with hippocampal sclerosis, astroglial, microglial and neuronal (5/8 cases) expression of C1q, C3c and C3d was observed particularly within regions where neuronal cell loss occurs. The membrane attack protein complex (C5b-C9) was predominantly detected in activated microglial cells. The persistence of complement activation could contribute to a sustained inflammatory response and could destabilize neuronal networks involved.

Published

2008

142. Direct Immunofluorescence and Immunohistochemistry in Diagnostics of Glomerulonephritis

Author

Jasminka Mustedanagić Mujanović, Zinaida Karasalihović, Elmir Cickusic, Ermina Iljazovic, Dušan Ferluga, J. Stahov, and Ina Skaljić

Subjects

Immunoglobulin A, Pathology, medicine.medical_specialty, Fluorescent Antibody Technique, immunoperoxidase (IP), immune deposits, Immunofluorescence, Kidney, Sensitivity and Specificity, Article, Immunoenzyme Techniques, Glomerulonephritis, immunofluorescence (IF), Biopsy, Medicine, Humans, Prospective Studies, Direct fluorescent antibody, Complement C1q, Retrospective Studies, lcsh:R5-920, biology, medicine.diagnostic_test, Immunoperoxidase, business.industry, Biopsy, Needle, General Medicine, Immunoglobulin M, Complement C3c, Immunoglobulin G, renal biopsies, biology.protein, Antibody, business, lcsh:Medicine (General)

Abstract

The needle biopsies from 60 transplanted and native kidneys have been processed and a prospective analysis of pattern, intensity and distribution of immunoglobulin deposits (IgA, IgG and IgM) and complement components (C3c and C1q) identified in these lesions has been carried out by immunohistochemistry with three step immunoperoxidase, in the period from 2000 to 2004. Those deposits were previously detected and analyzed by immunofluorescence. The samples consisted of 30 renal biopsies, previously diagnosed with glomerulonephritis and positive immunofluorescence and 30 renal biopsies without morphologic changes and deposits on immunofluorescence. 78,7% of the analyzed samples showed the identical results of the deposits of immunoglobulin and components of the complement with both, immunohistochemistry and immunofluorescence method. Sensitivity of the immunohistochemistry method with three step immunoperoxidase for all analyzed immunoglobulin and complement components is high (0,93), while specificity for the same method is 0,79. Standardized method of the three step immunoperoxidase on the paraffin embedded, formalin fixed needle renal biopsies could successfully replace the immunofluorescence method in diagnostic of GN, with the emphasis on a follow up and control of each single step in the procedure of the method.

Published

2008

143. Biomarker identification in human pancreatic cancer sera

Author

Rushie J. Hanas, Stan Lightfoot, Brenda J. Smith, Russell G. Postier, Daniel J. Brackett, Jay S. Hanas, Kent D. Denson, Daniel L. Morgan, Kristi C Prejeant, James R. Hocker, Yuiry Gusev, John Y. Cheung, Jason L. Larabee, and Megan R. Lerner

Subjects

Adult, Male, Spectrometry, Mass, Electrospray Ionization, Endocrinology, Diabetes and Metabolism, Molecular Sequence Data, Inflammation, Adenocarcinoma, Endocrinology, Pancreatic cancer, Internal Medicine, medicine, Biomarkers, Tumor, Humans, Trypsin, alpha-Macroglobulins, Amino Acid Sequence, Aged, Neoplasm Staging, Gel electrophoresis, Hepatology, biology, business.industry, Histocytochemistry, Cancer, Ceruloplasmin, Middle Aged, medicine.disease, Macroglobulin, Pancreatic Neoplasms, Complement C3c, Immunology, biology.protein, Electrophoresis, Polyacrylamide Gel, Female, medicine.symptom, business, medicine.drug

Abstract

Objective The aim of this study is to identify biomarkers in sera of pancreatic cancer patients using mass spectrometry (MS) approaches. Methods Sera from patients diagnosed with pancreatic adenocarcinoma and sera from normal volunteers were subjected to gel electrophoresis to resolve and quantify differences in protein levels. Protein bands that differed quantitatively were digested with trypsin, and peptides were identified by electrospray ionization (ESI) ion-trap tandem MS. Mass spectra were also collected directly from pancreatic cancer sera as well as healthy control sera using ESI-MS. Results Three large-mass proteins were found to be elevated in pancreatic cancer sera versus normal sera, alpha-2 macroglobulin, ceruloplasmin, and complement 3C. Complement 3C is a major regulator of inflammatory responses. The ESI-MS of human pancreatic cancer sera versus normal sera revealed greater heterogeneity in cancer sera than control sera, especially in the low-mass region. Bootstrapping statistical analysis identified 20 low-mass serum peaks that correlated with control sera and 20 different peaks that correlated with pancreatic cancer sera. Conclusions The fact that inflammation-sensitive proteins were identified as increased in pancreatic cancer sera supports the hypothesis that inflammatory-driven processes are involved in pancreatic carcinogenesis. Liquid ESI-MS analyses of sera hold promise for future pancreatic cancer blood tests as well as for understanding mechanisms of pancreatic carcinogenesis. The variability observed between the low-mass regions of normal versus pancreatic cancer spectra may aid in diagnosis and therapy.

Published

2008

144. Expression of complement alternative pathway proteins by endothelial cells. Differential regulation by interleukin 1 and glucocorticoids

Author

Jean Ripoche, Denyse Ozanne, Nathalie Julen, Hélène Dauchel, Marc Fontaine, Claudie Lemercier, and Maryvonne Daveau

Subjects

medicine.medical_specialty, medicine.medical_treatment, Complement Pathway, Alternative, Immunology, Enzyme-Linked Immunosorbent Assay, Complement factor I, In Vitro Techniques, Biology, Complement factor B, Dexamethasone, Internal medicine, Complement C3b Inactivator Proteins, medicine, Humans, Immunology and Allergy, Endothelium, Glucocorticoids, Serine Endopeptidases, Interleukin, Complement system, Endothelial stem cell, Endocrinology, Cytokine, Gene Expression Regulation, Complement Factor I, Complement C3c, Complement Factor H, Factor H, Alternative complement pathway, Complement Factor B, Interleukin-1

Abstract

We have studied the secretion of proteins of the alternative pathway of complement C3, factor B and factor H by human umbilical vein endothelial cells (HUVEC). Results showed that factor H and factor B are quantitatively secreted in abundance whereas C3 could only be detected when the cells are maintained in culture during long periods of time. Interferon-gamma stimulated factor H, factor B and, to a lesser extent, C3 secretions. Interleukin (IL) 1 had a differential effect on spontaneous C3, factor B and factor H secretions. In the presence of IL 1, there was a significant secretion of C3 occurring within a short period of culture. IL 1 also stimulated factor B secretion. There was a synergistic stimulating effect between IL 1 and interferon-gamma to bring C3 and factor B productions by HUVEC to very high levels. In contrast, factor H secretion was consistently inhibited by IL 1. Local increase in C3 and factor B secretions by endothelial cells in the presence of IL 1 may have important implications in the inflammatory reaction. In striking contrast, the glucocorticoid dexamethasone (DXM) had modulatory effects which are consistent with its anti-inflammatory properties. DXM, at therapeutic concentrations, decreased C3 and factor B secretions and increased factor H secretion. Local modulation of complement protein secretion by DXM appears to be a new mechanism by which this glucocorticoid may control inflammation.

Published

1990

145. The level of mannan-binding protein regulates the binding of complement-derived opsonins to mannan and zymosan at low serum concentrations

Author

R. J. Levinsky, Malcolm W. Turner, and Michael Super

Subjects

Chemistry, Binding protein, Immunology, Zymosan, Complement C4, chemical and pharmacologic phenomena, Opsonin Proteins, Complement factor B, Molecular biology, Collectins, Complement system, Mannans, Classical complement pathway, Biochemistry, Complement C3c, Complement C3b, Alternative complement pathway, Humans, Immunology and Allergy, Properdin, Carrier Proteins, Immunoglobulin binding, Research Article, Mannan

Abstract

SUMMARY When sera diluted to 5% in a buffer containing calcium and magnesium were incubated with mannancoated ELISA plates, C4 fragments, properdin and factor B were bound to the plates as well as the expected opsonic C3 fragments, C3b and C3bi. The calcium-dependent lectin mannan-binding protein, which is structurally similar to C1q, was also shown to bind in this assay and analysis of sera from 179 healthy blood donors revealed that the binding levels of all these proteins were highly significantly correlated. Results obtained with a previously described C3b opsonic assay using zymosan also correlated with the mannan-binding levels. When the sera were diluted to 5% in the presence of Mg-EGTA there was no detectable binding of complement proteins to the mannan surface, confirming that no alternative pathway activation occurred at this serum concentration. When sera were diluted to 5% in a buffer containing EDTA in order to study immunoglobulin binding in the absence of complement activation, the levels of bound IgG1, IgG2, IgG3, IgA and IgM antibodies were found to be completely unrelated to the C3bi binding levels previously observed. The results suggest that in this experimental system using low concentrations of serum, mannan-binding protein initiates an antibody-independent mechanism of cleavage of the classical pathway component C4, which subsequently regulates the degree of cleavage of C3 and recruitment of alternative pathway proteins.

Published

1990

146. Identification of specific serum proteins synthesized de novo by monolayer cultures of glandular cells of gestational endometrium

Author

J.G. Grudzinskas, T.N. Fay, Børge Teisner, S. Lindenberg, J.G. Westergaard, and L.G. Westergaard

Subjects

Orosomucoid, Immunoelectrophoresis, In Vitro Techniques, Endometrium, chemistry.chemical_compound, Pregnancy, medicine, Humans, alpha-Macroglobulins, Cells, Cultured, Serum Albumin, Methionine, biology, medicine.diagnostic_test, Rehabilitation, Albumin, Ceruloplasmin, Obstetrics and Gynecology, Complement C4, Blood Proteins, Molecular biology, Blood proteins, Fibronectins, Lipoproteins, LDL, De novo synthesis, Pregnancy Trimester, First, medicine.anatomical_structure, Reproductive Medicine, chemistry, Complement C3c, alpha 1-Antitrypsin, biology.protein, Female

Abstract

Monolayer cell cultures (n = 3) of glandular epithelium of gestational endometrium obtained from three apparently healthy women undergoing elective termination of pregnancy (7-9 weeks gestation) were established. De novo synthesis of eight serum proteins (albumin, alpha 1-antitrypsin, ceruloplasmin, beta-lipoprotein, alpha 2-macroglobulin, fibronectin and complement factors C3 and C4) was demonstrated by the incorporation of radiolabelled substrate ([35S]methionine) employing autoradiography (AR) in combination with crossed immunoelectrophoresis (XIE), referred to as ARXIE, and line immunoelectrophoresis (LIE), referred to as ARLIE. By contrast, there was no evidence for de novo synthesis of IgA, haptoglobin and orosomucoid. Our findings suggest that the gestational endometrium may contribute to the production of several proteins considered to be synthesized and secreted mainly by the liver and reticulo-endothelial system. The simple techniques used here to identify the de novo synthesis of human serum proteins could be applied to investigate protein synthesis by a wide range of tissues and cells.

Published

1990

147. Multicentre physiological reference intervals for serum concentrations of immunoglobulins A, G and M, complement C3c and C4 measured with Tina-Quant reagents systems

Author

Santiago Juvé-Cuxart, Carmen Mar-Medina, Lluís Coca-Fábregas, Pedro La-Torre-Marcellán, Julián Díaz-Fernández, Pilar Herrero-Bernal, María del Señor López-Vélez, Eduardo Alonso-Gregorio, María del Mar Larrea-Ortiz-Quintana, Adolfo Sicilia-Enríquez-de-Salamanca, Xavier Fuentes-Arderiu, Cándido Serrano-López, Javier Martín-Oncina, María Pilar Pinel-Julián, Beatriz Gutiérrez-Cecchini, Marta Cruz-Placer, Francisca García-Caballero, María Victoria Romero-Sotomayor, Carmen Ambrós-Marigómez, María Victoria Rodríguez-Hernández, Ana María Velasco-Romero, Marcos Sempere-Alcocer, and Virtudes Álvarez-Funes

Subjects

Immunoglobulin A, medicine.medical_specialty, Clinical Biochemistry, Complement C3c, Immunoglobulin G, Reference Values, medicine, Humans, Gynecology, Complement (group theory), biology, business.industry, Biochemistry (medical), Complement C4, General Medicine, Complement C3, Serum concentration, Reference intervals, Immunoglobulin M, Spain, Immunology, biology.protein, Indicators and Reagents, Antibody, business

Abstract

Background: Clinical laboratories seeking accreditation for compliance with ISO 15189:2003 need to demonstrate that the physiological reference intervals communicated to all users of the laboratory service are appropriate for the patient population served and for the measurement systems used. In the case of immunological quantities, few articles have been published in peer-reviewed journals. Methods: A total of 21 clinical laboratories in different regions of Spain collaborated in identifying reference individuals and determining adult reference intervals for some immunological quantities measured using RD/Hitachi Modular Analytics analysers and Tina-Quant® reagent systems. These immunological quantities are the mass concentrations of immunoglobulin A, immunoglobulin G, immunoglobulin M, complement C3c and complement C4 in serum. All the logistic work was carried out in co-operation with the supplier of the reagents and analysers (Roche Diagnostics Espana, S.L., Sant Cugat del Valles, Catalonia, Spain). From the set of reference values obtained by each laboratory, multicentre reference limits were estimated non-parametrically. Results and conclusions: The reference intervals estimated in this study for concentrations of serum components under consideration are: complement C3c, 0,62-1,64 g/L for women and men; complement C4, 0,14-0,72 g/L for women and men; immunoglobulin A, 0,89-4,80 g/L for women and men; immunoglobulin G, 6,5-14,3 g/L for women and men; and immunoglobulin M, 0,48-3,38 g/L for women and 0,41-2,46 g/L for men. (According to ISO, IUPAC and IFCC recommendations, the comma is used as the decimal sign.)

Published

2007

148. Glomerular C3c deposition and intravascular macrophage accumulation in early humoral renal allograft rejection signifies a poor short-term outcome

Author

I. Blohmé, Gudrun Nyberg, Christian Svalander, Johan Mölne, Michael E. Breimer, and Lennart Rydberg

Subjects

Microbiology (medical), Adult, Graft Rejection, Male, Pathology, medicine.medical_specialty, Adolescent, Biopsy, Antigens, Differentiation, Myelomonocytic, Biology, Kidney, Peritubular capillaries, Pathology and Forensic Medicine, Leukocyte Count, Antigens, CD, medicine, Cadaver, Immunology and Allergy, Macrophage, Humans, Transplantation, Homologous, Kidney transplantation, Aged, Retrospective Studies, medicine.diagnostic_test, CD68, Macrophages, General Medicine, Middle Aged, medicine.disease, Prognosis, Immunohistochemistry, Kidney Transplantation, Capillaries, medicine.anatomical_structure, Kidney Tubules, Treatment Outcome, Complement C3c, Humoral immunity, Female, Biomarkers

Abstract

C4d deposition in the walls of peritubular capillaries is considered the key phenomenon in the histopathological diagnosis of humoral, i.e. antibody-mediated, allograft rejection. We have earlier proposed that deposition of C3c in glomerular capillaries and simultaneous intravascular accumulation of macrophages in allografts with immediate or early humoral rejection indicates a potentially serious condition with very poor prognosis. The clinical outcome of 45 cadaveric grafts with this phenomenon among 1960 renal allografts transplanted at our centre during 1984-1999, and the recipients of the contralateral kidneys, was retrospectively evaluated. Graft failure occurred in 44/45 grafts within 3 weeks, with graft loss in 33/45 (77%) within 4 months and 37/45 (82%) within 1 year. From the contralateral kidneys, 5/33 (15%) were lost within 1 year. In a recent series of early biopsies, we recognised that of 13 cases showing C4d positivity in peritubular capillaries but lacking C3c in glomeruli, 10/13 (77%) were still functioning after 4 months. The mean number of CD68(+) macrophages per glomerular profile, i.e. the glomerular macrophage index, shows a significant difference between C4d(+)C3c(-) and C4d(+)C3c(+) cases (p

Published

2006

149. The ontogeny and extrahepatic expression of complement factor C3 in Atlantic salmon (Salmo salar)

Author

Hanne Johnsen, J. Oriol Sunyer, Hani Boshra, Jarl Bøgwald, Roy A. Dalmo, and Marie Løvoll

Subjects

Embryo, Nonmammalian, Hot Temperature, Ontogeny, Salmo salar, Complement factor I, Aquatic Science, Hemolysis, Notochord, medicine, Environmental Chemistry, Animals, RNA, Messenger, Salmo, Edetic Acid, Chelating Agents, Innate immune system, biology, Reverse Transcriptase Polymerase Chain Reaction, Antibodies, Monoclonal, Gene Expression Regulation, Developmental, Embryo, Chemotaxis, General Medicine, biology.organism_classification, Immunohistochemistry, Complement system, Cell biology, medicine.anatomical_structure, Complement C3c, Immunology

Abstract

Fish embryos and hatchlings are exposed to pathogens long before maturation of their lymphoid organs. Little is known about defence mechanisms during the earliest stages of life, but innate mechanisms may be essential for survival. The complement system in fish is well developed and represents a major part of innate immunity. Complement factor 3 (C3) is central subsequent to activation of all pathways of the complement system, leading to inflammatory reactions, such as chemotaxis, opsonisation and lysis of pathogens. Hepatocytes represent the major source of C3, but modern molecular biological methods have confirmed that C3 is synthesised at multiple sites. Our main objective was to study the ontogeny of C3 in Atlantic salmon by mapping the commencement of synthesis and localisation of proteins. Eggs, embryos, hatchlings and adult fish were analysed for the presence of C3 mRNA and proteins. From immunohistochemical studies, C3 proteins were detected at several extrahepatic sites, such as the skeletal muscle, developing notochord and chondrocytes of the gill arch. Immunoblotting revealed presence of C3 proteins in the unfertilised egg, but C3 mRNA was only detected after fertilisation by real-time RT-PCR. Taken together, the results implicated the maternal transfer of C3 proteins as well as novel non-immunological functions during development.

Published

2006

150. Proteomic analysis of recurrent spontaneous abortion: Identification of an inadequately expressed set of proteins in human follicular fluid

Author

Bum-Chae Choi, Sook-Hwan Lee, Kwang Yul Cha, Jeong Mook Lim, Myung-Sun Kim, Kwang-Hyun Baek, and Yong-Soo Kim

Subjects

Adult, Proteomics, medicine.medical_specialty, Abortion, Habitual, Population, Angiotensinogen, Down-Regulation, Biology, Biochemistry, Antithrombins, Follicle, Western blot, Hemopexin, Internal medicine, medicine, Humans, Electrophoresis, Gel, Two-Dimensional, RNA, Messenger, education, Molecular Biology, education.field_of_study, Complement component 3, medicine.diagnostic_test, Reverse Transcriptase Polymerase Chain Reaction, Antithrombin, Fibrinogen, Follicular fluid, Follicular Fluid, medicine.anatomical_structure, Endocrinology, Complement C3c, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Chorionic villi, Female, Chorionic Villi, medicine.drug

Abstract

Recurrent spontaneous abortion (RSA), defined as the loss of three or more consecutive pregnancies prior to the 20th week of gestation, affects up to 5% of the child-bearing population. To investigate the proteins associated with RSA, the protein expression in human follicular fluid was analyzed using 2-DE. Follicular fluid contains a variety of biologically important proteins for oocyte fertilization and follicle maturation in the mammalian reproductive process. Therefore, it can be used as a provisional source for identifying proteins involved in RSA. In this study, we identified five aberrantly expressed proteins (complement component C3c chain E, fibrinogen gamma, antithrombin, angiotensinogen, and hemopexin precursor) in follicular fluid from RSA patients with MALDI-TOF-MS and nano-LC MS/MS. Western blot analysis confirmed that the protein expression level of fibrinogen gamma and antithrombin was less in follicular fluid from RSA patients than those from normal controls. Semiquantitative RT-PCR and real-time PCR analyses revealed that mRNA level of these coagulation factors was also decreased significantly in chorionic villi of RSA patients compared with normal samples. Taken all together, it is likely that coagulation factors (fibrinogen gamma and antithrombin) play an important role in maintaining the normal pregnancy.

Published

2006