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1. C5a anaphylatoxin as a product of complement activation up-regulates the complement inhibitory factor H in rat Kupffer cells

Author

Frauke Nitzki, Henrike L. Schieferdecker, Rüdiger Hardeland, G. Schlaf, Ines Heine, and Otto Götze

Subjects
Male, Kupffer Cells, Immunology, Complement C5a, Enzyme-Linked Immunosorbent Assay, Biology, Complement factor B, alpha-N-Acetylgalactosaminidase, Proinflammatory cytokine, 03 medical and health sciences, 0302 clinical medicine, Animals, Immunology and Allergy, RNA, Messenger, Rats, Wistar, Binding site, Antibodies, Blocking, Complement Activation, Decay-accelerating factor, 030304 developmental biology, 0303 health sciences, Reverse Transcriptase Polymerase Chain Reaction, Blotting, Northern, Molecular biology, Rats, Up-Regulation, Complement system, Liver, Biochemistry, Complement Factor H, 030220 oncology & carcinogenesis, Factor H, iC3b, Complement component 5a
Abstract

The 155-kDa complement regulator factor H (FH) is the predominant soluble regulatory protein of the complement system. It acts as a cofactor for the factor I-mediated conversion of the component C3b to iC3b, competes with factor B for a binding site on C3b and C3(H2O) and promotes the dissociation of the C3bBb complex. The primary site of synthesis is the liver, i.e. FH-specific mRNA and protein were identified in both hepatocytes (HC) and Kupffer cells (KC). Previous studies in rat primary HC and KC had shown that the proinflammatory cytokine IFN-gamma influences the balance between activation and inhibition of the complement system through up-regulation of the inhibitory FH. In this study we show that C5a, as a product of complement activation, stimulates the expression of FH-specific mRNA and protein in KC and thus induces a negative feedback. Quantitative-competitive RT-PCR showed an approximate threefold C5a-induced up-regulation of FH. ELISA analyses revealed a corresponding increase in FH protein in the supernatants of KC. The up-regulation of FH was completely inhibited by the C5a-blocking monoclonal antibody 6-9F. Furthermore, an involvement of LPS and IFN-gamma was excluded, which strongly indicates a direct effect of C5a on the expression of FH in KC.

Published
2004

2. Differences in the Involvement of Prostanoids from Kupffer Cells in the Mediation of Anaphylatoxin C5a-, Zymosan-, and Lipopolysaccharide-Dependent Hepatic Glucose Output and Flow Reduction

Author

Otto Götze, G. Schlaf, Sabine Pestel, Kurt Jungermann, and Henrike L. Schieferdecker

Subjects
Lipopolysaccharides, Male, medicine.medical_specialty, Lipopolysaccharide, Kupffer Cells, Thromboxane, Indomethacin, Prostaglandin, Complement C5a, Pathology and Forensic Medicine, chemistry.chemical_compound, Internal medicine, Escherichia coli, medicine, Animals, Anaphylatoxin, Rats, Wistar, Molecular Biology, Cells, Cultured, Phenylacetates, Sulfonamides, Kupffer cell, Zymosan, Hemodynamics, Thromboxanes, Prostanoid, hemic and immune systems, Cell Biology, Metabolism, respiratory system, musculoskeletal system, Rats, Perfusion, Glucose, medicine.anatomical_structure, Endocrinology, Liver, chemistry, Biochemistry, Hepatocytes, Prostaglandins, cardiovascular system, lipids (amino acids, peptides, and proteins)
Abstract

Various inflammatory stimuli such as anaphylatoxin C5a, zymosan, and lipopolysaccharides (LPSs) have been reported both to enhance glucose output in the perfused rat liver and to induce prostanoid (ie, prostaglandin and thromboxane) release from Kupffer cells, the resident liver macrophages. Because prostanoids can enhance glucose output from hepatocytes, it was the aim of this study to compare the possible roles of prostanoids released after C5a, zymosan, and LPS in the mediation of hepatic glucose output. In perfused livers both C5a and zymosan immediately enhanced glucose output, reduced flow, and induced prostanoid overflow into the hepatic vein, but with different quantities and kinetics. Only the C5a-induced but not the zymosan-induced effects were abrogated by inhibitors of prostanoid signaling as the prostanoid synthesis inhibitor indomethacin and the thromboxane receptor antagonist daltroban. In contrast to C5a and zymosan, LPS had no effect on glucose output, flow rate, or prostanoid overflow. In isolated Kupffer cells, C5a and zymosan induced maximal release of prostaglandins D(2) and E(2) and of thromboxane A(2) within a period of 0 to 2 minutes and 5 to 15 minutes, respectively. In pulse-chase experiments, maximal prostanoid release was already observed after 2 minutes of continuous stimulation with C5a, but only after 10 to 15 minutes of continuous stimulation with zymosan. LPS-dependent prostanoid release was not seen before 1 hour. Thus, even though C5a, zymosan, and LPS induced prostanoid release from Kupffer cells, only C5a quickly regulated hepatic glucose metabolism in a prostanoid-dependent manner (due to the kinetics and quantities of prostanoids released).

Published
2003

3. Rat Complement Factor H: Molecular Cloning, Sequencing and Quantification with a Newly Established ELISA

Author

Beatrix Pollok-Kopp, G. Schlaf, T Demberg, D. Gerke, and Otto Götze

Subjects
Untranslated region, chemistry.chemical_classification, 0303 health sciences, Messenger RNA, Immunology, Nucleic acid sequence, General Medicine, Biology, Molecular biology, 3. Good health, Complement system, 03 medical and health sciences, Open reading frame, 0302 clinical medicine, chemistry, Biochemistry, Factor H, Coding region, Nucleotide, 030304 developmental biology, 030215 immunology
Abstract

Factor H (FH) is the predominant soluble regulatory protein of the complement system. With a concentration of 300–600 µg/ml in human plasma it acts as a cofactor for the FI-mediated cleavage of the component C3b to iC3b. Furthermore, it competes with factor B for binding to C3b and C3(H2O) and promotes the dissociation of the C3bBb complex (i.e. it has decay accelerating activity). FH is a monomer of about 155 kDa which comprises 20 short consensus repeats (SCR), each of which is composed of nearly 60 amino acid residues. For the screening of a rat liver cDNA library, we used two hybridization probes which had been produced by polymerase chain reaction (PCR). The probes were generated using degenerated primers which corresponded to conserved parts of the human and the murine factor H nucleotide sequences. The entire rat sequence spanned 4240 nucleotides with an open reading frame of 3708 nucleotides. These were preceded by 23 nucleotides of the 5′ untranslated region, followed by a stop codon and a 3′ untranslated region of 478 nucleotides including the polyadenylation-signal up to the beginning of the poly A tail. Comparison of the rat cDNA-derived coding sequence revealed identities of 74% to the human and 87% to the mouse FH nucleotide sequence. The translation product of rat FH mRNA was 1236 aa in length (leader sequence included) with an identity of 63% to the human and 81.5% to the murine protein. The degree of glycosylation of rat FH-Mr is about 9.5%. To quantitate FH in rat serum and supernatants of primary cultures of rat hepatocytes (HC), a reliable and sensitive sandwich-enzyme-linked immunosorbent assay (ELISA) was established. The concentration of FH in rat serum was calculated to be 238 µg ± 21 µg/ml (mean ± SD). Its concentration in the culture supernatants of HC was upregulated about three-fold by interferon (IFN)-γ (100 U/ml).

Published
2002

4. Constitutive Expression and Regulation of Rat Complement Factor H in Primary Cultures of Hepatocytes, Kupffer Cells, and Two Hepatoma Cell Lines

Author

Beatrix Pollok-Kopp, G. Schlaf, Henrike L. Schieferdecker, T Demberg, Nadine Beisel, and Otto Götze

Subjects
Lipopolysaccharides, Male, medicine.medical_treatment, medicine.disease_cause, Polymerase Chain Reaction, Liver Neoplasms, Experimental, 0302 clinical medicine, Tumor Cells, Cultured, Interferon gamma, Cells, Cultured, 0303 health sciences, Kupffer cell, Up-Regulation, 3. Good health, Cell biology, Cytokine, medicine.anatomical_structure, Complement Factor H, Factor H, Hepatocyte, medicine.symptom, medicine.drug, medicine.medical_specialty, Kupffer Cells, Blotting, Western, Inflammation, Biology, Pathology and Forensic Medicine, Interferon-gamma, 03 medical and health sciences, Internal medicine, medicine, Animals, RNA, Messenger, Rats, Wistar, Molecular Biology, DNA Primers, 030304 developmental biology, Base Sequence, Dose-Response Relationship, Drug, Interleukin-6, Toxin, Cell Biology, Blotting, Northern, Rats, Endocrinology, Cell culture, Hepatocytes, Interleukin-1, 030215 immunology
Abstract

The 155-kd soluble complement regulator factor H (FH), which consists of 20 short consensus repeats, increases the affinity of complement factor I (FI) for C3b by about 15 times. In addition to its cofactor activity, it prevents factor B from binding to C3b and promotes the dissociation of the C3bBb complex. The primary site of synthesis of FH, as well as of FI, is the liver, but the cell types responsible for the hepatic synthesis of both factors have not yet been clearly identified. In contrast to FI-mRNA, which was detectable only in hepatocytes (HC), FH-specific mRNA was identified in both HC and Kupffer cells (KC). As calculated for equal amounts of mRNA isolated from both cell types, FH-specific mRNA was found to be nearly 10-fold higher in KC than in HC, leading to the conclusion that KC are an abundant source of FH. Of the investigated proinflammatory cytokines IL-6, TNF-alpha, IL-1beta, and IFN-gamma, only IFN-gamma up-regulated FH-specific mRNA up to 6-fold in both primary HC and KC. This was also demonstrable on the protein level. However, FH-specific mRNA was not inducible in the rat hepatoma cell line H4IIE, which did not express FH-specific mRNA and could not be up-regulated in FAO cells that constitutively expressed FH-specific mRNA. This demonstrates that transformed cell lines do not reflect FH regulation in isolated primary HC. In addition to IFN-gamma, the endotoxin lipopolysaccharide (LPS) up-regulated FH-specific mRNA nearly 10-fold in KC after stimulation at concentrations of 10 or 1 ng/ml. In contrast, concentrations of up to 2 microg LPS/ml did not show any effect on HC. Our data suggest that LPS does not regulate the expression of FH in HC.

Published
2002

5. Characterization of the human T cell response against the neuronal protein synapsin in patients with multiple sclerosis

Author

T. Polak, G. Schlaf, Frank Weber, C. Krome-Cesar, Klaus Felgenhauer, Ulrike Schöll, and Michael Mäder

Subjects
Multiple Sclerosis, CD3 Complex, T-Lymphocytes, T cell, Encephalomyelitis, Immunology, Dose-Response Relationship, Immunologic, Cell Line, Immunophenotyping, Interferon-gamma, 03 medical and health sciences, 0302 clinical medicine, medicine, Demyelinating disease, Humans, Immunology and Allergy, Lymphotoxin-alpha, 030304 developmental biology, 0303 health sciences, biology, Tumor Necrosis Factor-alpha, Multiple sclerosis, Encephalomyelitis, Acute Disseminated, Myelin Basic Protein, Synapsin, Synapsins, medicine.disease, Molecular biology, Interleukin-10, Myelin basic protein, medicine.anatomical_structure, Lymphotoxin, nervous system, Neurology, Acute Disease, CD4 Antigens, biology.protein, Interleukin-4, Neurology (clinical), 030217 neurology & neurosurgery, CD8
Abstract

Although multiple sclerosis (MS) is considered primarily as a demyelinating disease, neuronal damage is abundant and correlates with the neurological deficit. Therefore, we investigated the frequency and characteristics of human T cells specific for synapsin-a neuronal protein highly conserved among species. Synapsin specific T cell responses were detected at a frequency similar to that of MBP specific T cells in MS patients, one patient with acute demyelinating encephalomyelitis (ADEM) and controls. Long-term T cell lines specific for synapsin exhibited a CD3(+), CD4(+), CD8(-) phenotype and produced high amounts of tumor-necrosis-factor-alpha (TNF-alpha) and interferon-gamma (IFN-gamma) after antigen specific stimulation, whereas lymphotoxin (LT), interleukin-4 (IL-4) and interleukin-10 (IL-10) were detectable in smaller quantities.

Published
2001

6. Rat complement factor I: molecular cloning, sequencing and expression in tissues and isolated cells

Author

G. Schlaf, Otto Götze, Kurt Jungermann, E. Rothermel, Martin Oppermann, and Henrike L. Schieferdecker

Subjects
Untranslated region, 0303 health sciences, Messenger RNA, cDNA library, Immunology, Nucleic acid sequence, Complement factor I, Biology, Molecular biology, Complement system, 03 medical and health sciences, 0302 clinical medicine, Immunology and Allergy, Coding region, Peptide sequence, 030304 developmental biology, 030215 immunology
Abstract

Factor I (FI) is a regulatory serine protease of the complement system which cleaves three peptide bonds in the alpha-chain of C3b and two bonds in the alpha-chain of C4b thereby inactivating these proteins. The human protein and the recently characterized mouse factor I are heterodimers of about 88,000 MW which consist of a non-catalytic heavy chain of 50,000 MW which is linked to a catalytic light chain of 38,000 MW by a disulphide bond. For the screening of a rat liver cDNA library we used a hybridization probe produced by polymerase chain reaction (PCR) using degenerated primers which corresponded to conserved parts of the human and the murine factor I nucleotide sequences. One of the identified sequences, which had a length of 2243 base pairs (bp), contained the complete coding region and the whole 3' untranslated region. The length of the coding region in rat consisted of 1812 bp followed by a 3' untranslated region of 207 bp including the polyadenylation signal and the beginning of the poly A tail. Comparison of the rat cDNA-derived coding sequence revealed identities of 87% to the mouse and of 78% to the human FI nucleotide sequence. The translation product of rat FI mRNA was 604 amino acid residues (aa) in length with an identity of 85% to the mouse (603 aa) and 69% to the human protein (583 aa). The comparison of the molecular mass predicted by the primary structure and derived from rat FI isolated from rat serum as detected in immunoblot analyses suggested a glycosylation of more than 20% of the total mass of the FI protein. Expression studies using reverse transcription (RT)-PCR assays indicated that FI-specific mRNA could neither be identified in B cells, nor in T cells, monocytes or granulocytes from rat and human peripheral blood nor in rat peritoneal macrophages. These data were in agreement with the results of RT-PCR obtained with several human lymphoma cell lines (Jurkat, MOLT-4, HUT102, Wil 2-NS, Ramos, Raji, U937) all of which were devoid of FI-specific mRNA. In accord with our data from two rat hepatoma cell lines (FAO and H4IIE) and one from man (HepG2) only isolated rat hepatocytes (HC) but neither Kupffer cells (KC), hepatic stellate cells (HSC; Ito cells) nor sinusoidal endothelial cells (SEC) expressed FI-specific mRNA. FI mRNA was also detected in human umbilical vein endothelial cells (HUVEC) and in the uterus and small intestine of the rat. Spleen and lymph nodes did not contain any detectable FI-specific mRNA.

Published
1999

8. Complement Factor I Is Upregulated in Rat Hepatocytes by Interleukin-6 But Not by Interferon-γ , Interleukin-1β or Tumor Necrosis Factor-α

Author

G. Schlaf, Milena Koleva, T Demberg, Kurt Jungermann, and Otto Götze

Subjects
Lymphotoxin alpha, Blotting, Western, Molecular Sequence Data, Clinical Biochemistry, Complement factor I, Biochemistry, Proinflammatory cytokine, Interferon-gamma, 03 medical and health sciences, 0302 clinical medicine, medicine, Animals, Humans, Interferon gamma, Amino Acid Sequence, RNA, Messenger, Northern blot, B-cell activating factor, Molecular Biology, 030304 developmental biology, 0303 health sciences, Interleukin-6, Reverse Transcriptase Polymerase Chain Reaction, Tumor Necrosis Factor-alpha, Chemistry, Blotting, Northern, Molecular biology, Rats, Up-Regulation, Complement system, Gene Expression Regulation, Complement Factor I, Hepatocytes, Cytokines, Tumor necrosis factor alpha, Interleukin-1, 030215 immunology, medicine.drug
Abstract

Complement factor I (FI) is a regulatory serine protease of the complement system which cleaves three peptide bonds in the alpha-chain of C3b and two bonds in the alpha-chain of C4b and thus prevents the assembly of the C3 and C5 convertases. We have investigated the proinflammatory cytokines IL-6, IL-1beta, TNF-alpha and IFN-gamma for their potential role in the regulation of FI expression. Of the investigated cytokines, only IL-6 increased the FI-specific RT-PCR signal in isolated hepatocytes, in the two rat hepatoma-derived cell lines FAO and H4IIE or in HUVECs. Quantitative competitive RT-PCR showed an IL-6 induced upregulation of FI-specific mRNA by about ten-fold. These data are in accord with Northern blot analyses in which the FI-mRNA was upregulated by IL-6 between five- and seven-fold. IL-6, but not IL-1beta, TNF-alpha or IFN-gamma also increased FI-protein levels in cell culture supernatants by about five-fold as determined by a semiquantitative immunoblot using a novel monoclonal antibody specific for rat FI.

Published
2001

9. Analysis of the tissue distribution of the rat C5a receptor and inhibition of C5a-mediated effects through the use of two MoAbs

Author

S Zahn, G. Schlaf, E Rothermel, and Otto Götze

Subjects
medicine.drug_class, Immunology, Molecular Sequence Data, Complement C5a, Enzyme-Linked Immunosorbent Assay, Monoclonal antibody, C5a receptor, 03 medical and health sciences, Mice, 0302 clinical medicine, Antigens, CD, Acetylglucosaminidase, medicine, Animals, Amino Acid Sequence, Receptor, Receptor, Anaphylatoxin C5a, 030304 developmental biology, 0303 health sciences, Mice, Inbred BALB C, biology, Antibodies, Monoclonal, General Medicine, Transfection, Ligand (biochemistry), Molecular biology, Immunohistochemistry, Rats, Receptors, Complement, biology.protein, Calcium, Signal transduction, Antibody, 030215 immunology
Abstract

The C5-anaphylatoxin C5a is a protein of 74 (human) or 77 (rat) amino-acid residues, respectively, the generation of which may be induced by either the classical and/or the alternative pathways. C5a binds specifically to its receptor (C5aR/CD88) which belongs to the superfamily of G-protein-coupled receptors with seven transmembrane segments. In this study we describe the tissue distribution of the rat C5aR (rC5aR) and the blocking of its ligand by the application of two monoclonal antibodies (MoAbs). The first antibody (MoAb R63) which is directed against the amino-terminal domain Ex1 of the rat C5aR was generated in mice immunized with RBL-2H3 cells which had been stably transfected with the rat C5a receptor gene. Checking the rC5aR expression in various tissues bronchial epithelial cells stained positive only in tissue samples from animals with a mycoplasm infection indicating that the receptor may be induced in this cell type as a consequence of an inflammatory process. Using immunohistochemistry there was no evidence for nonmyeloid expression in the large or small intestine, heart, lung, kidney or liver of the normal rat. The MoAb R63 was found to be a reliable tool for the investigation of the expression of the receptor by FACS analyses or immunohistochemistry. Despite numerous attempts neutralizing antibodies could not be generated against the receptor. Therefore a C5a-ligand neutralizing MoAb was generated against the synthesized carboxyterminal 20mer peptide. This antibody (6-9F) recognized the carboxy terminus of C5a/C5a-FLUOS and prevented its binding at a three-fold molar excess as evidenced by FACS-analyses. It also blocked the C5a-mediated signal transduction as demonstrated by the inhibition of intracellular Ca2+-release (at a 16-fold molar excess) and the release of N-Acetyl-beta-D-glucosaminidase (at a 25-fold molar excess).

Published
2000

10. Large-scale purification of synaptophysin and quantification with a newly established enzyme-linked immunosorbent assay

Author

Joachim R. Wolff, Klaus Felgenhauer, Michael Mäder, G. Schlaf, and Matthias Göddecke

Subjects
Lysis, Swine, Immunoblotting, Synaptophysin, Enzyme-Linked Immunosorbent Assay, Biochemistry, Chromatography, Affinity, 03 medical and health sciences, 0302 clinical medicine, Affinity chromatography, Rosaniline Dyes, Animals, 030304 developmental biology, Antiserum, Gel electrophoresis, Brain Chemistry, 0303 health sciences, Chromatography, biology, Isoelectric focusing, Chromatofocusing, Chemistry, Hydrophilic interaction chromatography, Antibodies, Monoclonal, Molecular biology, Calibration, biology.protein, Chromatography, Gel, Synaptic Vesicles, Isoelectric Focusing, 030217 neurology & neurosurgery
Abstract

Synaptophysin (SYP I), an integral membrane protein, was purified on a large scale (0.55 - 2.7 mg) from isolated small synaptic vesicles (SSV) of porcine cortex. In order to achieve this, a conventional purification procedure which consists of size exlusion chromatography, hydrophobic interaction chromatography and chromatofocusing has been developed. This procedure was compared with purification of SYP I by immunoaffinity chromatography. The elution patterns of both procedures were monitored using sodium dodecylsulfate gel electrophoresis (SDS-PAGE) with subsequent Coomassie blue staining of proteins and simultaneous immunoblotting with SYP I-specific antibody. Contaminating proteins with relative molecular masses (M(r)) very similar to SYP I could be removed during the process of purification, demonstrating that the 38 kDa protein found after Triton X-100 lysis of enriched SSV does not exclusively represent SYP I. A specific antiserum was raised in rabbits using a highly purified preparation of SYP I. This antiserum was used in combination with a monoclonal antibody to establish a specific and sensitive enzyme-linked immunosorbent assay (ELISA) which allowed rapid and reliable quantification of this hydrophobic membrane protein in all purification steps, starting with Triton X-100-lysed brain homogenates. Using this ELISA, the concentration of SYP I in highly purified SSV was determined to be 5.8% of solubilized protein.

Published
1996

11. A novel enzyme-linked immunosorbent assay for determination of synaptophysin as compared with other quantification procedures

Author

G. Schlaf, Klaus Felgenhauer, Reinhild Poethke, Michael Mäder, and Claudia Salje

Subjects
Lysis, medicine.drug_class, Swine, Immunology, Blotting, Western, Immunoblotting, Synaptophysin, Enzyme-Linked Immunosorbent Assay, Biology, Monoclonal antibody, Synaptic vesicle, medicine, Immunology and Allergy, Animals, Humans, Antiserum, chemistry.chemical_classification, Molecular biology, Rats, Microscopy, Electron, Enzyme, nervous system, Neurology, chemistry, Rats, Inbred Lew, Reagent, biology.protein, Neurology (clinical), Rabbits, Synaptic Vesicles, Antibody
Abstract

A two-sided enzyme-linked immunosorbent assay (ELISA) has been established for reliable, specific and sensitive determination of synaptophysin (SYN), an intrinsic membrane protein of the small synaptic vesicles. This ELISA used a highly specific monoclonal antibody (SY 38) as capture reagent and a specific SYN antiserum in combination with a secondary peroxidase-conjugated antibody for detection. Calibration was carried out with immunoaffinity-purified SYN from porcine cortex. The sensitivity was found to be improved substantially when the ELISA was compared with previously used dot-immunobinding assays. This ELISA allowed rapid and reliable determination of SYN from detergent lysed homogenates, partially and highly purified preparations of rat, porcine and human brain. SYN was determined in highly purified small synaptic vesicles, and it was calculated to be 5.8% of total detergent solubilized protein.

Published
1996

12. Origin and immunoregulation of autoantibodies against intestinal alkaline phosphatase

Author

G. Schlaf, Michael Mäder, K. Felgenhauer, H. G. Nüsslein, W. Beuche, and N. Kolbus

Subjects
Adult, Male, Immunology, Phosphatase, Cross Reactions, Sepharose, Antigen-Antibody Reactions, chemistry.chemical_compound, Immunoglobulin Fab Fragments, Humans, Aged, Autoantibodies, Aged, 80 and over, biology, Chemistry, Isoelectric focusing, General Medicine, Bacterial Infections, Middle Aged, Alkaline Phosphatase, Isotype, Molecular biology, Blot, Immunoglobulin Isotypes, Intestines, Biochemistry, Immunoglobulin G, Acute Disease, biology.protein, Cyanogen bromide, Electrophoresis, Polyacrylamide Gel, Female, Antibody, Protein A
Abstract

In the sera of patients with acute bactetial infections specific autoantibodies (sIAPa) of the imtnuno-globulin class G (IgG) were found which bind to intestinal alkahne phosphatase (IAP) through the Fab portion. This was demonstrated using immunoaffinity (IA) isolation of sIAPa from patients' sera (particularly bacterial meningitis and ventriculitis) digestion with pepsin, purification of F(ab')2 fragments on protein A and subsequently binding on IAP coupled to CNBr (cyanogen bromide)-activated Sepharose. Immunoblots using specific anti-Fc and anti-Fab antibodies showed that the bulk of F(ab')2 fragments had bound. Additionally, binding of native IAP to the F(ab')2 fragments was observed after separation of F(ab')2 fragments using isoelectric focusing (IEF), blotting onto nitro cellulose and incubation with IAP. Moreover, we have demonstrated the occurrence of natural anti-IAP autoantibodies (nIAPa) which were isolated from sera of healthy individuals using IA chromatography. Investigation of isotype distribution revealed that IgG but not IgM or IgA were predominant even among nIAPa. The nIAPa fraction exhibited lower binding efficiencies on IEF blots than the sIAPa fraction, however, in contrast to sIAPa, cross-reactions with other autoantigens were observed for nIAPa. NIAPa and sIAPa did not show subclass restriction. As revealed by IEF the spectrotypes of sIAPa were found to be patient-specific, poly- to oligoclonal and stable during longer periods.

Published
1995

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