Your search keyword '"Klemens Löster"' showing total 38 results

1. PDGF-BB enhances α1β1 integrin-mediated activation of the ERK/AP-1 pathway involved in collagen matrix remodeling by rat mesangial cells

Author

Shoji Kagami, Yasuhiro Kuroda, Masanori Kitamura, Shuji Kondo, Akiko Kitamura, Klemens Löster, Werner Reutter, Maki Urushihara, and Tetsuhiro Hisayama

Subjects

MAPK/ERK pathway, medicine.medical_specialty, Physiology, Kinase, MEK inhibitor, Clinical Biochemistry, Integrin, Cell Biology, Biology, Cell biology, Blot, Endocrinology, Internal medicine, medicine, Extracellular, biology.protein, Electrophoretic mobility shift assay, Platelet-derived growth factor receptor

Abstract

Platelet-derived growth factor-BB (PDGF-BB) has been implicated in the pathogenesis of progressive glomerulonephritis (GN). Previous studies have reported that PDGF-BB stimulates mesangial cells (MCs)-induced collagen matrix remodeling through enhancement of alpha1beta1 integrin-dependent migratory activity. To determine the cell signaling pathway responsible for abnormal MC-related mesangial matrix remodeling in progressive GN, we studied the involvement of the extracellular signal-regulated kinase (ERK)/activator protein-1 (AP-1) pathway in PDGF-BB-enhanced collagen gel contraction. Western blotting and gel shift assay revealed that MC-induced gel contraction resulted in ERK activation in parallel with that of AP-1 binding, peaking at 4 h and lasting at least for 24 h. Application of the MEK inhibitor, U0126, and the c-jun/AP-1 inhibitor, curcumin, inhibited gel contraction and AP-1 activity, respectively, dose dependently. PDGF-BB enhanced not only gel contraction but ERK phosphorylation and AP-1 activity by MCs. Marked inhibitory effects on PDGF-BB-induced gel contraction and ERK/AP-1 activity were observed in the presence of either function blocking anti-alpha1- or anti-beta1-integrin antibody or U0126. Consistently, AP-1-inactive MCs expressing a dominant-negative mutant of c-jun showed a significant decrease of PDGF-BB-induced gel contraction as compared with mock-transfected MCs. Finally, migration assay showed that ERK/AP-1 activity is required for PDGF-BB-stimulated alpha1beta1 integrin-dependent MC migration to collagen I. These results indicated that PDGF-BB enhances alpha1beta1 integrin-mediated collagen matrix reorganization through the activation of the ERK/AP-1 pathway that is crucial for MC migration. We conclude that the ERK/AP-1 pathway plays an important role in PDGF-BB-induced alpha1beta1 integrin-dependent collagen matrix remodeling; therefore, the inhibition of its pathway may provide a novel approach to regulate abnormal collagen matrix remodeling in progressive GN.

Published

2003

2. Phospholipase Cγ Binds α1β1Integrin and Modulates α1β1 Integrin-specific Adhesion

Author

Kerstin Danker, Werner Hofmann, Dörte Vossmeyer, Werner Reutter, and Klemens Löster

Subjects

Integrin, Tyrosine phosphorylation, Cell Biology, Biology, Biochemistry, CD49c, Collagen receptor, Cell biology, chemistry.chemical_compound, chemistry, Integrin alpha M, biology.protein, Integrin, beta 6, Signal transduction, Cell adhesion, Molecular Biology

Abstract

Integrin adhesion receptors have been implicated in bidirectional signal transduction. The dynamic regulation of integrin affinity and avidity as well as post-ligand effects involved in outside-in signaling depends on the interaction of integrins with cytoskeletal and signaling proteins. In this study, we attempted to identify cytoplasmic binding partners of α1β1 integrin. We were able to show that cell adhesion to α1β1-specific substrates results in the association of phospholipase Cγ (PLCγ) with the α1β1 integrin independent of PLCγ tyrosine phosphorylation. Using peptide-binding assays, the membrane proximal sequences within the α1β1integrin subunits were identified as binding sites for PLCγ. In particular, the conserved sequence of β1 subunit binds the enzyme very efficiently. Because purified PLCγ also binds the integrin peptides, binding seems to be direct. Inhibition of PLC byU73122 leads to reduced cell adhesion on α1β1-specific substrates. Cells lacking the conserved domain of the α1 subunit fail to respond to the PLC inhibition, indicating that this domain is necessary for PLC-dependent adhesion modulation of α1β1 integrin.

Published

2002

3. α1 Integrin cytoplasmic domain is involved in focal adhesion formation via association with intracellular proteins

Author

Klemens LÖSTER, Dörte VOSSMEYER, Werner HOFMANN, Werner REUTTER, and Kerstin DANKER

Subjects

Cell Biology, Molecular Biology, Biochemistry

Abstract

Integrins are heterodimeric adhesion receptors consisting of α- and β-subunits capable of binding extracellular matrix molecules as well as other adhesion receptors on neighbouring cells. These interactions induce various signal transduction pathways in many cell types, leading to cytoskeletal reorganization, phosphorylation and induction of gene expression. Integrin ligation leads to cytoplasmic protein–protein interactions requiring both integrin cytoplasmic domains, and these domains are initiation points for focal adhesion formation and subsequent signal transduction cascades. In previous studies we have shown that the very short cytoplasmic α1 tail is required for post-ligand events, such as cell spreading as well as actin stress-fibre formation. In the present paper we report that cells lacking the cytoplasmic domain of the α1 integrin subunit are unable to form proper focal adhesions and that phosphorylation on tyrosine residues of focal adhesion components is reduced on α1β1-specific substrates. The α1 cytoplasmic sequence is a specific recognition site for focal adhesion components like paxillin, talin, α-actinin and pp125FAK. It seems to account for α1-specific signalling, since when peptides that mimic the cytoplasmic domain of α1 are transferred into cells, they influence α1β1-specific adhesion, presumably by competing for binding partners. For α1 integrin/protein binding, the conserved Lys-Ile-Gly-Phe-Phe-Lys-Arg motif and, in particular, the two lysine residues, are important.

Published

2001

4. Vitronectin in clotting factor IX concentrates

Author

Günter Iberer, Andrea Buchacher, Katharina Pock, Djuro Josic, Christoph Kannicht, and Klemens Löster

Subjects

Clotting factor, chemistry.chemical_classification, biology, business.industry, Thrombogenicity, Hematology, General Medicine, Heparin, Biochemistry, Affinity chromatography, chemistry, medicine, biology.protein, Vitronectin, Glycoprotein, business, Genetics (clinical), Factor IX, medicine.drug

Abstract

Highly purified, plasma-derived factor IX (FIX) concentrates are produced in large part by a combination of anion exchange and heparin affinity chromatography. However, the concentrates still contain some accompanying proteins. The main impurity has turned out to be the adhesive glycoprotein, vitronectin. It occurs in concentrates exclusively in its multimeric form, in contrast to the situation in plasma. The multimeric vitronectin can be removed either by nanofiltration with a crossflow system or by size-exclusion chromatography. When these FIX concentrates are used as therapeutic agents, the fact has to be taken into account that considerable amounts of multimeric vitronectin are given to the patient. The physiological consequences of the dosage of this protein have not yet been investigated. Although no thrombogenicity has been reported in connection with the above-mentioned FIX concentrates, we recommend that the impurity should be removed from the preparation with the methods described here.

Published

2001

5. Overexpression of α1β1 integrin directly affects rat mesangial cell behavior

Author

Takahiko Saijo, Yasuhiro Kuroda, Shoji Kagami, Shoko Kobayashi, Werner Reutter, Shuzi Kondo, Maki Urushihara, Klemens Löster, and Akiko Kitamura

Subjects

Integrins, medicine.medical_specialty, Glomerular Mesangial Cell, Integrin, Gene Expression, Cell Cycle Proteins, Biology, Transfection, Integrin alpha1beta1, Collagen receptor, Rats, Sprague-Dawley, Cicatrix, Laminin, Internal medicine, medicine, Animals, cell growth, scarring, Cloning, Molecular, Glomerulosclerosis, Focal Segmental, Cell adhesion molecule, Tumor Suppressor Proteins, progressive renal disease, collagen matrix, Flow Cytometry, Actins, Extracellular Matrix, Glomerular Mesangium, Rats, Cell biology, Fibronectin, Phenotype, Endocrinology, Integrin alpha M, Nephrology, COS Cells, biology.protein, Integrin, beta 6, Collagen, hypertrophy, Microtubule-Associated Proteins, Cell Division, Cyclin-Dependent Kinase Inhibitor p27, glomerulosclerosis

Abstract

Overexpression of α 1 β 1 integrin directly affects rat mesangial cell behavior. Background Glomerular mesangial cell (MC) proliferation, hypertrophy, and abnormal matrix remodeling characterized by increased expression of fibronectin, laminin and collagen type IV, and neoexpression of collagen I and III are the main biological features of progressive glomerulonephritis (GN). Especially, persistent pathological matrix remodeling may lead to glomerular scar formation (glomerular scarring). We reported recently that α 1 β 1 integrin, a major collagen receptor for MCs, may be a potential adhesion molecule for MC-mediated pathological collagen matrix remodeling in GN. Methods To address further the direct role of α 1 β 1 integrin in MC behavior, such as cell growth and matrix remodeling, α 1 β 1 integrin was overexpressed in MCs by transfecting an expression vector containing a full-length rat α 1 integrin cDNA. Flow cytometry and immunoprecipitation analysis were applied for selection of transfectants with a stable expression of the α 1 integrin subunit. The effect of α 1 β 1 integrin overexpression on MC biology was examined with a 3 H-thymidine incorporation assay, flow cytometric analysis of cell size and DNA content, Western blot analysis of a cyclin-dependent-kinase inhibitor, p27 Kip1 , α-smooth muscle actin expression, and a collagen gel contraction assay. Results The α 1 transfectants displayed a dramatic inhibition of 3 H-thymidine incorporation as compared with the mock transfectants. Increased expression of the α 1 subunit inversely correlated with cell cycle progression and paralleled the expression of p27 Kip1 and α-smooth muscle actin, as well as the cell size in MCs. In addition, the α 1 -transfectants were able to enhance collagen matrix reorganization effectively. Conclusion These results indicate that MC-α 1 β 1 integrin expression is a critical determinant of MC phenotypes, including cell growth, cell size, and collagen matrix remodeling ability, and thereby contributes to scar matrix remodeling (sclerosis) in GN.

Published

2000

6. The Cytoplasmic Domain of the α1 Integrin Subunit Influences Stress Fiber Formation via the Conserved GFFKR Motif

Author

Rüdiger Horstkorte, Kerstin Danker, Dörte Vossmeyer, Christine Kaufmann, Klemens Löster, Lothar Lucka, and Werner Reutter

Subjects

Cytoplasm, Integrins, Stress fiber, Protein subunit, Integrin alpha1, Integrin, CHO Cells, Biology, Transfection, CD49c, Antigens, CD, Cricetinae, Cell Adhesion, Animals, Amino Acid Sequence, Conserved Sequence, Actin, Sequence Deletion, Chemotaxis, Chinese hamster ovary cell, Cell Biology, Actin cytoskeleton, Actins, Recombinant Proteins, Rats, Cell biology, Integrin alpha M, biology.protein, Dimerization

Abstract

Integrins are heterodimeric transmembrane proteins that mediate substrate adhesion and migration but also the bidirectional transfer of information across the plasma membrane via their cytoplasmic domains. We addressed the question of whether the very short cytoplasmic tail of the alpha1 integrin subunit of alpha1beta1 integrin is required for alpha1beta1-specific adhesion, spreading, and migration. For this purpose we transfected the alpha1 integrin subunit and two cytoplasmically truncated alpha1 subunits into Chinese hamster ovary (CHO) cells. Elimination of the entire cytoplasmic domain of the alpha1 subunit does not affect adhesion but leads to inhibition of spreading and stress fiber formation. The defect in spreading could not be rescued by lysophosphatidic acid, which has been reported to stimulate actin stress fiber formation via Rho. Additionally, deletion of the entire cytoplasmic domain of the alpha1 subunit abolishes migration toward alpha1beta1-specific substrates. Migration and stress fiber formation are similar in CHO-alpha1 cells and CHO cells carrying an alpha1 subunit still containing the conserved GFFKR motif. So, the GFFKR motif of the alpha1 subunit is essential and sufficient for these processes.

Published

2000

7. α1β1 Integrin-Mediated Collagen Matrix Remodeling by Rat Mesangial Cells Is Differentially Regulated by Transforming Growth Factor-β and Platelet-Derived Growth Factor-BB

Author

Koji Yasutomo, Klemens Löster, Werner Reutter, Shoji Kagami, Shuji Kondo, Takashi Kuhara, and Yasuhiro Kuroda

Subjects

Integrins, medicine.medical_specialty, Platelet-derived growth factor, medicine.medical_treatment, Integrin, Integrin alpha1beta1, Collagen receptor, Rats, Sprague-Dawley, Extracellular matrix, chemistry.chemical_compound, Cell Movement, Reference Values, Transforming Growth Factor beta, Internal medicine, Cell Adhesion, medicine, Animals, Humans, Cell adhesion, Cells, Cultured, Platelet-Derived Growth Factor, biology, Mesangial cell, Growth factor, General Medicine, Blotting, Northern, Immunohistochemistry, Extracellular Matrix, Glomerular Mesangium, Rats, Cell biology, Disease Models, Animal, Endocrinology, chemistry, Nephrology, biology.protein, Collagen, Transforming growth factor

Abstract

Pathologic remodeling of mesangial matrix after glomerular injury is the central biologic feature of glomerular scarring (sclerosis). Transforming growth factor-beta (TGF-beta) and platelet-derived growth factor (PDGF)-BB have been implicated in the development of glomerular scarring in rat and human glomerulonephritis. To clarify molecular and cellular mechanisms involved in abnormal mesangial remodeling, this study focused on the role of alpha1beta1 integrin, a collagen/laminin receptor, in rat mesangial cells, using collagen gel contraction as an experimental model of in vivo collagen matrix remodeling and scar formation. In addition, the influence of TGF-beta and PDGF-BB on mesangial cell (MC)-mediated collagen gel contraction in association with the alpha1beta1 integrin expression was evaluated. Integrin function blocking studies using anti-alpha1, beta1 subunit antibodies indicated that MC-alpha1beta1 integrin is essentially required not only for collagen-dependent adhesion/migration, but also for gel contraction. Protein synthesis and mRNA analysis experiments demonstrated that TGF-beta, but not PDGF-BB, increases the expression of alpha1beta1 integrin in mesangial cells cultured on plastic surface and in collagen gels. The upregulation of alpha1beta1 integrin expression by TGF-beta correlated with increases in gel contraction and collagen-dependent adhesion but not migration of mesangial cells. On the other hand, PDGF-BB enhanced MC-mediated gel contraction and migration without affecting cell adhesion to collagen I. Growth factor-induced collagen-dependent adhesion, migration, and gel contraction were significantly attenuated by incubation with anti-alpha1, beta1 subunit antibodies. Thus, these data indicate that alpha1beta1 integrin-mediated collagen matrix remodeling can be modulated by TGF-beta and PDGF-BB via different mechanisms. Alpha1 integrin-mediated mesangial matrix remodeling induced by TGF-beta or PDGF-BB may be a pathogenic mechanism leading to glomerular scarring.

Published

1999

8. Electrophoretic analyses of clotting factor VIII concentrates

Author

Katharina Pock, Klemens Löster, Christoph Kannicht, Alois Jungbauer, Djuro Josic, and Andrea Buchacher

Subjects

Clotting factor, congenital, hereditary, and neonatal diseases and abnormalities, Chromatography, Two-dimensional gel electrophoresis, biology, Chemistry, Fibrinogen, Human serum albumin, Biochemistry, Blood proteins, Analytical Chemistry, Von Willebrand factor, Polyclonal antibodies, hemic and lymphatic diseases, Monoclonal, biology.protein, medicine, Environmental Chemistry, Plasma proteins, Clotting factor VIII, 2D-PAGE (two-dimensional electrophoresis), Proteomics, Spectroscopy, medicine.drug

Abstract

Preparations of clotting factor VIII (FVIII) are complex protein mixtures, regardless of whether they are made by genetically engineered cells or isolated from human plasma. Commercially available FVIII preparations contain either von Willebrand factor (vWF) or human serum albumin (HSA), both of which function as stabilizers. Apart from these, the preparations contain other plasma proteins as impurities. Such protein mixtures were analyzed with SDS–PAGE and 2D-electrophoresis. Single bands and spots were identified by immunoblot using monoclonal and polyclonal antibodies. The aim was to detect every preparation which has an increased level of FVIII cleavage products. Chromatographic methods and SDS–PAGE under reducing and non-reducing conditions usually do not show any differences between single preparations. Only by a combination of separations under non-reducing and increasingly reducing conditions cleavage products of FVIII can in some cases be detected in immunoblot. In 2D electrophoresis the detection of proteins with high molecular masses was achieved by applying a mixture of thiourea and urea. The spots in 2D-electrophoresis of plasma-derived FVIII preparations have been identified as FVIII and vWF, but also as impurities, chiefly from fibrinogen. It was shown that especially 2D-electrophoresis and immunoblot can be used for better characterization of FVIII concentrates. The 2D protein maps of FVIII concentrates will be an efficient tool for quality control of such products.

Published

1998

9. Analysis of protein aggregates by combination of cross-linking reactions and chromatographic separations

Author

Klemens Löster and Djuro Josic

Subjects

Integrins, Chromatography, Chemistry, Molecular cluster, Proteins, General Chemistry, Protein aggregation, Cross-Linking Reagents, Investigation methods, Covalent bond, Fructose-Bisphosphate Aldolase, Reagent, Heat-Shock Proteins, Chromatography, Liquid

Abstract

Chemical cross-linking provides a method that covalently bridges near-neighbour associations within proteins and protein aggregates. Combined with chromatographic separations and protein-chemical methods, it may be used to localize and to investigate three-dimensional relations as present under natural conditions. This paper reviews the chemistry and application of cross-linking reagents and the development of combination experimental approaches in view of chromatographic separations and cross-linking reactions. Investigations of homooligomeric and heterooligomeric protein associations as well as conformational analysis are presented.

Published

1997

10. Chemical Cross-Linking Detects Different Conformational Arrangements of Platelet Integrin αIIbβIII(gpIIb/IIIa)

Author

Werner Hofmann, Klemens Löster, Juan J. Calvete, and Werner Reutter

Subjects

chemistry.chemical_classification, biology, Protein Conformation, Fibrinogen receptor, Integrin, Biophysics, Succinimides, Platelet Glycoprotein GPIIb-IIIa Complex, Cell Biology, Biochemistry, Molecular Weight, Integrin Alpha-IIb, Cross-Linking Reagents, Membrane, chemistry, Covalent bond, Propionate, biology.protein, Humans, Platelet, Receptor, Molecular Biology

Abstract

Treatment of Triton X-100 solubilized platelet membrane with the homobifunctional cross-linker dithiobis(succinimidyl propionate) resulted in covalent cross-linking of the platelet integrin alpha IIb beta 3 (gpIIb/IIIa), the fibrinogen receptor, into three high-molecular-mass complexes with apparent M of 200, 220 and 240 k. Generation of these cross-linked alpha IIb beta 3 aggregates depended on the presence of a native receptor structure and was not influenced by Ca2+ ions and other experimental conditions. Immunoblotting analysis of purified 200/220/240 kDa aggregates revealed that they were made up exclusively by alpha IIb and beta 3 integrin chains in roughly stoichiometric amounts. We therefore conclude that alpha IIb beta 3 integrin occurs in different conformations in the platelet membrane that can be directly detected by chemical cross-linking.

Published

1996

11. Cell-Collagen Adhesion Is Inhibited by Monoclonal Antibody 33.4 against the Rat α1-Integrin Subunit

Author

Werner Reutter, Sebastian Voigt, Claudia Heidrich, Werner Hofmann, and Klemens Löster

Subjects

Integrins, medicine.drug_class, Protein subunit, Integrin alpha1, Integrin, Monoclonal antibody, Epitope, Integrin alpha1beta1, Liver Neoplasms, Experimental, Species Specificity, Affinity chromatography, Antibody Specificity, Laminin, Cell Adhesion, medicine, Animals, Tissue Distribution, biology, Integrin beta1, Antibodies, Monoclonal, Cell Biology, Molecular biology, Rats, Fibronectin, Liver, Biochemistry, biology.protein, Vitronectin, Collagen, Sequence Analysis

Abstract

A monoclonal antibody (mAb 33.4) is described which inhibits the adhesion and spreading of an adherent cell line (A-cells), established from Morris hepatoma 7777 and isolated hepatocytes on collagen IV but not on laminin, fibronectin, and vitronectin. mAb 33.4 retains its immunological activity after immobilization and covalent cross-linking to Protein G-Sepharose and is therefore a suitable tool for the preparative equimolar purification of two proteins with M(r) of 130 and 190 kDa from detergent-solubilized membrane fractions by immunoaffinity chromatography. The 190-kDa protein was identified as rat alpha 1-integrin subunit by N-terminal amino acid sequencing, while the 130-kDa protein was specifically stained by a beta 1-integrin subunit-specific antiserum. In immunoblot analysis mAb 33.4 recognized the 190-kDa band, suggesting that it is specific for the rat alpha 1-integrin subunit. The epitope recognized by mAb 33.4 is conformation-dependent because the staining in immunoblots was very strong if the SDS-PAGE was performed in the absence of reducing agents. The expression of alpha 1 beta 1-integrin in sinusoidal hepatocyte membrane domains of liver sections is shown by mAb 33.4 and antisera raised against the rat alpha 1- and beta 1-integrin subunits.

Published

1994

12. High-performance membrane chromatography of serum and plasma membrane proteins

Author

Oliver Baum, Klemens Löster, Djuro Josic, Joachim Reusch, and Werner Reutter

Subjects

Male, Glycidyl methacrylate, Detergents, Analytical chemistry, Disc diameter, Kidney, Biochemistry, High-performance liquid chromatography, Analytical Chemistry, chemistry.chemical_compound, Liver Neoplasms, Experimental, Animals, Porosity, Pressure drop, Chromatography, Chemistry, Organic Chemistry, Membrane Proteins, Rats, Inbred Strains, Blood Proteins, General Medicine, Plasma, Chromatography, Ion Exchange, Rats, Membrane, Liver, Membrane protein, Electrophoresis, Polyacrylamide Gel, Female

Abstract

Porous discs made of poly(glycidyl methacrylate) were used for high-performance membrane chromatography (HPMC) of proteins. In model experiments, separations of standard proteins by anion-exchange HPMC using a DEAE disc were carried out. The influences of sample distribution and disc diameter and thickness on separation performance were studied. The separation disc allowed a scaling-up from analytical (diameter 10 mm) to semi-preparative (diameter 50 mm) dimensions. In an application study, separations with anion-exchange and affinity HPMC were carried out using different complex samples such as rat serum and plasma membrane proteins. In all experiments the results on poly(glycidyl methacrylate) discs were comparable to those achieved on adequate high-performance liquid chromatographic (HPLC) columns. However, the separations on HPMC discs could be carried out faster than corresponding separations on HPLC columns. The pressure drop on the discs was low even at high flow-rates. The experiments show that the poly(glycidyl methacrylate) discs used are especially suitable for the isolation of proteins and other biopolymers which occur in a diluted state in complex mixtures.

Published

1992

13. Purification of Monoclonal Antibodies by Hydroxylapatite HPLC and Size Exclusion HPLC

Author

Rosemarie Kuhl, Klemens Löster, Joachim Reusch, Djuro Josic, and Franz Noll

Subjects

Quality Control, Chromatography, medicine.drug_class, Sodium, Fluorapatite, Size-exclusion chromatography, Antibodies, Monoclonal, chemistry.chemical_element, Buffers, Hydroxylapatite, Monoclonal antibody, Biochemistry, High-performance liquid chromatography, Electrophoresis, chemistry.chemical_compound, Immunoglobulin M, chemistry, Immunoglobulin G, Chromatography, Gel, medicine, Humans, Electrophoresis, Polyacrylamide Gel, Hydroxyapatites, Polyacrylamide gel electrophoresis, Chromatography, High Pressure Liquid

Abstract

Monoclonal antibodies of both the IgG and the IgM type were purified by hydroxylapatite HPLC (HA-HPLC) under very mild conditions. The IgM type antibodies, which were isolated from ascites fluid and separated from other proteins also by means of size exclusion HPLC. It was shown that the most frequently observed disadvantage of HA-HPLC, that is the relative short life of the columns (P. Steffen (1989) GIT Fachz. Lab., Suppl. 3/89 (Chromatogr.), 50-90), is due to microbial contamination rather than lower mechanical stability. In order to monitor column performance, a test was developed based on the use of standard proteins under isocratic separation conditions. This allows a direct comparison between the respective performances of columns made from different materials, hydroxylapatite or fluoroapatite, from different sources and with different particle sizes. A problem which often occurs with HA-HPLC in the case of IgM antibody isolation, namely precipitation of the antibodies at low salt concentrations at the beginning of a chromatographic run, was avoided by adding sodium chloride to both separation buffers.

Published

1991

14. 2-dimensional electrophoresis: detection of glycosylation and influence on spot pattern

Author

Klemens, Löster and Christoph, Kannicht

Subjects

Glycosylation, Blotting, Western, Electrophoresis, Gel, Two-Dimensional

Abstract

The detailed characterization of complex protein mixtures as in samples from biological sources cannot be sufficiently performed by separation of polypeptides according to their molecular weight as is done by conventional sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (1DE). For analysis of such samples, 2-dimensional gel electrophoresis (2DE) is the preferable methodological approach because it combines separation of polypeptides according to isoelectric properties and molecular weight as well. The resulting pattern of protein spots does not only provide information on composition of samples because of the complexity of a mixture of polypeptides. It delivers also a picture on the microheterogenity of polypeptides caused by post-translational modifications. These might be of natural or artificial type and occur during biosynthetic processing of a polypeptide or within industrial scale production. The presented method describes an experimental approach to investigate the influence of glycosylation in general and sialylation exclusively on spot pattern of proteins separated by 2DE.

Published

2008

15. 2-Dimensional Electrophoresis: Detection of Glycosylation and Influence on Spot Pattern

Author

Christoph Kannicht and Klemens Löster

Subjects

Gel electrophoresis, Electrophoresis, chemistry.chemical_compound, Glycosylation, Isoelectric point, Chromatography, chemistry, Complex protein, Industrial scale

Abstract

The detailed characterization of complex protein mixtures as in samples from biological sources cannot be sufficiently performed by separation of polypeptides according to their molecular weight as is done by conventional sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (1DE). For analysis of such samples, 2-dimensional gel electrophoresis (2DE) is the preferable methodological approach because it combines separation of polypeptides according to isoelectric properties and molecular weight as well. The resulting pattern of protein spots does not only provide information on composition of samples because of the complexity of a mixture of polypeptides. It delivers also a picture on the microheterogenity of polypeptides caused by post-translational modifications. These might be of natural or artificial type and occur during biosynthetic processing of a polypeptide or within industrial scale production. The presented method describes an experimental approach to investigate the influence of glycosylation in general and sialylation exclusively on spot pattern of proteins separated by 2DE.

Published

2008

16. PDGF-BB enhances alpha1beta1 integrin-mediated activation of the ERK/AP-1 pathway involved in collagen matrix remodeling by rat mesangial cells

Author

Shoji, Kagami, Maki, Urushihara, Akiko, Kitamura, Shuji, Kondo, Tetsuhiro, Hisayama, Masanori, Kitamura, Klemens, Löster, Werner, Reutter, and Yasuhiro, Kuroda

Subjects

Curcumin, Blotting, Western, Becaplermin, Electrophoretic Mobility Shift Assay, Transfection, Integrin alpha1beta1, Rats, Sprague-Dawley, Glomerulonephritis, Genes, jun, Cell Movement, Nitriles, Butadienes, Animals, Enzyme Inhibitors, Platelet-Derived Growth Factor, Dose-Response Relationship, Drug, Proto-Oncogene Proteins c-sis, Extracellular Matrix, Glomerular Mesangium, Rats, Enzyme Activation, Transcription Factor AP-1, Mutation, Collagen, Mitogen-Activated Protein Kinases, Signal Transduction

Abstract

Platelet-derived growth factor-BB (PDGF-BB) has been implicated in the pathogenesis of progressive glomerulonephritis (GN). Previous studies have reported that PDGF-BB stimulates mesangial cells (MCs)-induced collagen matrix remodeling through enhancement of alpha1beta1 integrin-dependent migratory activity. To determine the cell signaling pathway responsible for abnormal MC-related mesangial matrix remodeling in progressive GN, we studied the involvement of the extracellular signal-regulated kinase (ERK)/activator protein-1 (AP-1) pathway in PDGF-BB-enhanced collagen gel contraction. Western blotting and gel shift assay revealed that MC-induced gel contraction resulted in ERK activation in parallel with that of AP-1 binding, peaking at 4 h and lasting at least for 24 h. Application of the MEK inhibitor, U0126, and the c-jun/AP-1 inhibitor, curcumin, inhibited gel contraction and AP-1 activity, respectively, dose dependently. PDGF-BB enhanced not only gel contraction but ERK phosphorylation and AP-1 activity by MCs. Marked inhibitory effects on PDGF-BB-induced gel contraction and ERK/AP-1 activity were observed in the presence of either function blocking anti-alpha1- or anti-beta1-integrin antibody or U0126. Consistently, AP-1-inactive MCs expressing a dominant-negative mutant of c-jun showed a significant decrease of PDGF-BB-induced gel contraction as compared with mock-transfected MCs. Finally, migration assay showed that ERK/AP-1 activity is required for PDGF-BB-stimulated alpha1beta1 integrin-dependent MC migration to collagen I. These results indicated that PDGF-BB enhances alpha1beta1 integrin-mediated collagen matrix reorganization through the activation of the ERK/AP-1 pathway that is crucial for MC migration. We conclude that the ERK/AP-1 pathway plays an important role in PDGF-BB-induced alpha1beta1 integrin-dependent collagen matrix remodeling; therefore, the inhibition of its pathway may provide a novel approach to regulate abnormal collagen matrix remodeling in progressive GN.

Published

2004

17. 2D-Electrophoresis: Detection of Glycosylation and Influence on Spot Pattern

Author

Klemens Löster and Christoph Kannicht

Subjects

chemistry.chemical_compound, Glycosylation, Two-dimensional gel electrophoresis, Biochemistry, chemistry

Published

2003

18. Biochemical Engineering of Cell Surface Sialic Acids Stimulates Axonal Growth

Author

Klemens Löster, Werner Reutter, Sabine Nöhring, Christoph Kannicht, Carolin Schmidt, Bettina Büttner, Hye-Youn Lee, and Rüdiger Horstkorte

Subjects

Male, Neurite, Proteome, Glycoconjugate, Cell, Perforant Pathway, Stimulation, Biology, PC12 Cells, chemistry.chemical_compound, Mice, Transcription (biology), Cerebellum, medicine, Neurites, Animals, Electrophoresis, Gel, Two-Dimensional, ARTICLE, Cells, Cultured, chemistry.chemical_classification, Neurons, Mice, Inbred BALB C, Membrane Glycoproteins, General Neuroscience, Cell Membrane, Cell Differentiation, Hexosamines, Axons, Sialic acid, Nerve Regeneration, Rats, carbohydrates (lipids), Cytosol, medicine.anatomical_structure, Biochemistry, chemistry, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Sialic Acids, Female, Neuraminic Acids, Nucleus

Abstract

Sialylation is essential for development and regeneration in mammals. Using N-propanoylmannosamine, a novel precursor of sialic acid, we were able to incorporate unnatural sialic acids with a prolonged N-acyl side chain (e.g., N-propanoylneuraminic acid) into cell surface glycoconjugates. Here we report that this biochemical engineering of sialic acid leads to a stimulation of neuronal cells. Both PC12 cells and cerebellar neurons showed a significant increase in neurite outgrowth after treatment with this novel sialic acid precursor. Furthermore, also the reestablishment of the perforant pathway was stimulated in brain slices. In addition, we surprisingly identified several cytosolic proteins with regulatory functions, which are differentially expressed after treatment with N-propanoylmannosamine. Because sialic acid is the only monosaccharide that is activated in the nucleus, we hypothesize that transcription could be modulated by the unnatural CMP-N-propanoylneuraminic acid and that sialic acid activation might be a general tool to regulate cellular functions, such as neurite outgrowth.

Published

2002

19. Effects of anti-alpha1 integrin subunit antibody on anti-Thy-1 glomerulonephritis

Author

Shoji Kagami, Shuji Kondo, Werner Reutter, Yasuhiro Kuroda, Klemens Löster, Toshihiko Hayashi, Hiroko Yamano, Maki Urushihara, and Dörte Vossmeyer

Subjects

Male, medicine.medical_specialty, Integrins, Platelet-derived growth factor, Integrin, Matrix (biology), Pathology and Forensic Medicine, Collagen receptor, Integrin alpha1beta1, Extracellular matrix, Rats, Sprague-Dawley, chemistry.chemical_compound, Glomerulonephritis, Transforming Growth Factor beta, Internal medicine, medicine, Animals, Molecular Biology, Platelet-Derived Growth Factor, Wound Healing, biology, Mesangial cell, Antibodies, Monoclonal, Cell Biology, medicine.disease, Molecular biology, Extracellular Matrix, Glomerular Mesangium, Rats, Endocrinology, chemistry, biology.protein, Thy-1 Antigens, Collagen, Wound healing

Abstract

alpha1beta1 integrin is a potential collagen-binding extracellular matrix receptor that mediates collagen-dependent cell adhesion, proliferation, migration, and collagen matrix assembly and thereby may participate in the wound healing and pathologic scarring observed in some damaged organs. To clarify the role of alpha1beta1 integrin predominantly expressed on the mesangial cell (MC) surface in nephritic glomeruli, we investigated the involvement of MC-alpha1beta1 integrin in rat anti-Thy-1 glomerulonephritis (GN) by administering function-blocking monoclonal mouse anti-rat alpha1 integrin subunit antibody (anti-alpha1 Ab). Assay of collagen types I and IV mixed gel contraction, an in vitro model of pathologic collagen matrix remodeling, with function-blocking anti-alpha1 Ab and anti-beta1 Ab, revealed that collagen I and IV matrix reorganization is mediated by MC-alpha1beta1 integrin. In addition, conditioned medium from isolated Day 3 anti-Thy-1 nephritic glomeruli showed increased activity of MC-alpha1beta1 integrin-induced mixed collagen gel contraction as compared with that from isolated normal rat glomeruli. Treatment of Day 3 conditioned medium with anti-platelet-derived growth factor-BB antibody significantly inhibited conditioned media-induced gel contraction, whereas treatment with anti-transforming growth factor-beta antibody did not have a significant effect. Rats that received anti-alpha1 Ab from the left renal artery 3 days after anti-Thy-1 GN induction showed significant decreases of glomerular hypercellularity and mesangial matrix accumulation, including collagen I and IV in the left kidney, compared with those rats in which the left kidney received control mouse IgG1. These results suggest that MC-alpha1beta1 integrin is an important extracellular matrix receptor mediating mesangial remodeling characterized by MC proliferation and mesangial matrix reorganization in anti-Thy-1 GN. Platelet-derived growth factor-BB may be involved in early collagen matrix reorganization leading to pathologic mesangial remodeling in this GN model.

Published

2002

20. 2D-electrophoresis. Detection of glycosylation and influence on spot pattern

Author

Klemens, Löster and Christoph, Kannicht

Subjects

Glycosylation, Electrophoresis, Gel, Two-Dimensional, Glycoproteins

Published

2002

21. Development and applications of surface plasmon resonance-based von Willebrand factor-collagen binding assay

Author

Natalya M. Ananyeva, Klemens Löster, Midori Shima, Andrey Sarafanov, Christoph Kannicht, Alexey V. Khrenov, Gerhard Gruber, Horst Schwinn, Djuro Josic, Diana Kouiavskaia, and Evgueni L. Saenko

Subjects

congenital, hereditary, and neonatal diseases and abnormalities, Biophysics, Enzyme-Linked Immunosorbent Assay, Biosensing Techniques, Biochemistry, Extracellular matrix, Collagen Type III, Von Willebrand factor, Von Willebrand factor collagen binding assay, hemic and lymphatic diseases, von Willebrand Factor, Humans, Platelet, Binding site, Surface plasmon resonance, Molecular Biology, Binding Sites, Factor VIII, biology, Chemistry, Reproducibility of Results, Cell Biology, Surface Plasmon Resonance, Von Willebrand Factor, Collagen Binding Assay, Molecular biology, Kinetics, biology.protein, Biological Assay, Carrier Proteins, Biosensor, circulatory and respiratory physiology

Abstract

Von Willebrand factor (vWf) functions both as a carrier of factor VIII (fVIII) in plasma and as an adhesive protein providing the primary link between collagen of the extracellular matrix and platelets sequestered from blood flow. The functional activity of vWf correlates with the level of its binding to collagen, which is commonly measured in the enzyme-linked immunosorbent assay (ELISA). We developed an automated collagen-binding assay employing the surface plasmon resonance (SPR) phenomenon, which allows one to quantitatively measure the binding of purified vWf and vWf-containing therapeutic fVIII concentrates to collagen type III immobilized on a biosensor chip. The results of the SPR-based assay highly correlated (r = 0.987) with collagen-binding ELISA. The advantages of the SPR-based assay are its higher accuracy and reproducibility in comparison with ELISA. We applied the developed assay for monitoring structural changes in the vWf component of plasma-derived fVIII/vWf concentrates during a virus inactivation procedure performed by heat treatment. We determined the critical residual moisture content of 2% that can be present in lyophilized concentrates during heat-treatment procedures without causing deteriorative changes in vWf properties. Our data suggest that the SPR-based assay is a useful tool in the development of industrial virus-inactivation procedures, allowing one to preserve vWf activity and achieve the maximal therapeutic efficacy of fVIII/vWf concentrates.

Published

2002

22. Phospholipase Cgamma binds alpha1beta1 integrin and modulates alpha1beta1 integrin-specific adhesion

Author

Dörte, Vossmeyer, Werner, Hofmann, Klemens, Löster, Werner, Reutter, and Kerstin, Danker

Subjects

Cytoplasm, Integrins, Time Factors, Phosphodiesterase Inhibitors, Amino Acid Motifs, Blotting, Western, Molecular Sequence Data, CHO Cells, Transfection, Models, Biological, PC12 Cells, Integrin alpha1beta1, Cricetinae, Cell Adhesion, Animals, Amino Acid Sequence, Enzyme Inhibitors, Estrenes, Phosphorylation, Phosphoinositide-3 Kinase Inhibitors, Dose-Response Relationship, Drug, Phospholipase C gamma, Precipitin Tests, Pyrrolidinones, Protein Structure, Tertiary, Rats, Isoenzymes, Immunoglobulin G, Type C Phospholipases, Tyrosine, Electrophoresis, Polyacrylamide Gel, Collagen, Laminin, Peptides, Protein Binding

Abstract

Integrin adhesion receptors have been implicated in bidirectional signal transduction. The dynamic regulation of integrin affinity and avidity as well as post-ligand effects involved in outside-in signaling depends on the interaction of integrins with cytoskeletal and signaling proteins. In this study, we attempted to identify cytoplasmic binding partners of alpha(1)beta(1) integrin. We were able to show that cell adhesion to alpha(1)beta(1)-specific substrates results in the association of phospholipase Cgamma (PLCgamma) with the alpha(1)beta(1) integrin independent of PLCgamma tyrosine phosphorylation. Using peptide-binding assays, the membrane proximal sequences within the alpha(1)beta(1) integrin subunits were identified as binding sites for PLCgamma. In particular, the conserved sequence of beta(1) subunit binds the enzyme very efficiently. Because purified PLCgamma also binds the integrin peptides, binding seems to be direct. Inhibition of PLC by leads to reduced cell adhesion on alpha(1)beta(1)-specific substrates. Cells lacking the conserved domain of the alpha(1) subunit fail to respond to the PLC inhibition, indicating that this domain is necessary for PLC-dependent adhesion modulation of alpha(1)beta(1) integrin.

Published

2001

23. Requirement for tyrosine kinase-ERK1/2 signaling in alpha 1 beta 1 integrin-mediated collagen matrix remodeling by rat mesangial cells

Author

Klemens Löster, Maki Urushihara, Shoji Kagami, Masanori Yoshizumi, Toshiaki Tamaki, Shuji Kondo, Werner Reutter, and Yasuhiro Kuroda

Subjects

Integrins, Integrin, Collagen receptor, Integrin alpha1beta1, Oligodeoxyribonucleotides, Antisense, Extracellular matrix, Rats, Sprague-Dawley, Cell Movement, Physical Stimulation, Animals, Enzyme Inhibitors, Phosphorylation, Cell adhesion, Flavonoids, Mitogen-Activated Protein Kinase 1, Mitogen-Activated Protein Kinase 3, Mesangial cell, biology, Cell Biology, Molecular biology, Extracellular Matrix, Glomerular Mesangium, Rats, biology.protein, Collagen, Signal transduction, Mitogen-Activated Protein Kinases, Type I collagen, Signal Transduction

Abstract

Abnormal mesangial extracellular matrix remodeling by mesangial cells (MCs) is the hallmark of progressive glomerulonephritis (GN). We recently showed, using a type I collagen gel contraction assay, that alpha 1 beta 1 integrin-dependent MC adhesion and migration are necessary cell behaviors for collagen matrix remodeling. To further determine the mechanism of alpha 1 beta 1 integrin-mediated collagen remodeling, we studied the signaling pathways of MCs that participate in the regulation of collagen gel contraction. Immunoprecipitation and phosphotyrosine detection revealed that gel contraction is associated with the enhanced activity and phosphorylation of ERK1/2 by MCs. The tyrosine kinase inhibitors herbimycin and genistein inhibited collagen gel contraction dose dependently. Furthermore, targeting ERK1/2 activity with a MEK inhibitor, PD98059, and antisense ERK1/2 hindered gel contraction in a dose-dependent manner. Similar inhibitory effects on gel contraction and ERK1/2 phosphorylation were observed when MC-mediated gel contraction was performed in the presence of function-blocking anti-alpha1 or anti-beta1 integrin antibodies. However, cell adhesion and migration assays indicated that PD98059 and antisense ERK1/2 blocked alpha 1 beta 1 integrin-dependent MC migration, but did not interfere with collagen adhesion, although there was a marked decrease in ERK1/2 phosphorylation and ERK1/2 protein expression in cell adhesion on type I collagen. None of the above could affect membrane expression of alpha 1 beta 1 integrin. These results suggested that ERK1/2 activation is critical for the alpha 1 beta 1 integrin-dependent MC migration necessary for collagen matrix reorganization. We therefore conclude that ERK1/2 may serve as a possible target for pharmacological inhibition of pathological collagen matrix formation in GN.

Published

2001

24. Use of surface plasmon resonance for studies of protein–protein and protein–phospholipid membrane interactions

Author

Midori Shima, Andrey Sarafanov, Klemens Löster, Evgueni L. Saenko, N Greco, Djuro Josic, and Horst Schwinn

Subjects

Conformational change, congenital, hereditary, and neonatal diseases and abnormalities, Chromatography, Vesicle, Organic Chemistry, Synthetic membrane, Phospholipid, General Medicine, Phosphatidylserine, Biochemistry, Analytical Chemistry, Von Willebrand facto, Factor VIII, Membranes, Surface plasmon resonance detection, LC, chemistry.chemical_compound, Thrombin, chemistry, hemic and lymphatic diseases, medicine, Surface plasmon resonance, medicine.drug, C2 domain

Abstract

The surface plasmon resonance phenomenon is used for real time measurements of protein–protein and protein–membrane interactions. In the present study two surface plasmon resonance-based binding assays permitting study of the interaction of coagulation factor VIII (fVIII) with von Willebrand factor (vWf) and phospholipid have been developed. These interactions of fVIII are required for maintenance of fVIII concentration in circulation and for the assembly of the functional factor Xase complex, respectively. With these binding assays, the role of the light chain (LCh) in fVIII binding to vWf and to immobilized phospholipid monolayers and intact vesicles containing 25% phosphatidylserine (PS) and 4% PS was examined. The finding that Kd of LCh binding to vWf (3.8 nM) is 9.5 times higher than that of fVIII (0.4 nM), indicates that the heavy chain (HCh) is required for the maximal affinity of fVIII for vWf. In contrast, affinities of LCh for 25/75 PS/phosphatidylcholine (PC) monolayers and 4/76/20 PSPC-phosphatidylethanolamine (PE) vesicles are similar to that of fVIII, indicating that LCh is solely responsible for these interactions. It was also examined how removal of the acidic region affects the binding affinity of the remaining part of LCh for vWf and phospholipid. It was demonstrated that the loss of the LCh acidic region upon thrombin cleavage leads to an 11 and 160-fold increase in the dissociation rate constant (koff value) and a 165 and 1500-fold increase in the Kd value of the binding of fVIII fragment A3–C1–C2 to vWf compared to that of LCh and fVIII, respectively. In contrast, the binding affinity of A3–C1–C2 for PS-containing membranes was 8–11-fold higher than that of LCh. Possible conformational change(s) in C2 domain upon removal of the acidic region were studied using anti-fVIII monoclonal antibody NMC-VIII/5 with an epitope within the C2 domain of LCh as a probe. The determined lower binding affinity of A3–C1–C2 for NMC-VIII/5 immobilized to a sensor chip than that of LCh, indicates that these conformational changes do occur.

Published

1999

25. Effect of von Willebrand Factor and Its Proteolytic Fragments on Kinetics of Interaction between the Light and Heavy Chains of Human Factor VIII

Author

Djuro Josic, Klemens Löster, Evgueni L. Saenko, and Andrei G. Sarafanov

Subjects

congenital, hereditary, and neonatal diseases and abnormalities, Stereochemistry, Proteolysis, Kinetics, Immunoglobulin light chain, Dissociation (chemistry), Divalent, Reaction rate constant, Von Willebrand factor, hemic and lymphatic diseases, von Willebrand Factor, medicine, Humans, Binding site, Protein Structure, Quaternary, chemistry.chemical_classification, Manganese, Binding Sites, Factor VIII, biology, medicine.diagnostic_test, Chemistry, Hematology, von Willebrand factor, Subunits, Reconstitution, Molecular biology, Peptide Fragments, biology.protein, Calcium, Dimerization, Protein Binding

Abstract

It was previously shown that vWF increases the rate of divalent cation-mediated fVIII reconstitution from isolated light chain (LCh) and heavy chain (HCh) subunits. We examined the effect of vWF on kinetic parameters for interaction between LCh and HCh in the presence of Ca 2+ and Mn 2+ ions, the most effective mediators of fVIII reconstitution from isolated subunits, and determined the minimal structural portion of vWF able to enhance fVIII formation. We found that affinity (K d ) for LCh/HCh binding mediated by Ca 2+ and Mn 2+ was 91 and 34.9 nM in the absence of vWF and 15.5 and 5.6 nM in its presence. This decrease of K d resulted from a sixfold increase of the association rate constant (k on ) for this interaction. The value of the dissociation rate constant (k off ) for LCh/HCh complex was lower in the presence of Mn 2+ (k off 4.6×10 −6 s −1 ) than Ca 2+ (k off 8.4×10 −6 s −1 ) but in both cases vWF had no effect on k off . This indicates that at physiological concentration of 1 nM the rate of fVIII inactivation via dissociation to subunits would be entirely determined by the k off value, and it should not depend on the presence of vWF. Indeed, our experiments demonstrated that vWF did not have any effect on the rate of fVIII inactivation resulting from its dissociation to subunits at the physiological concentrations of the fVIII and vWF proteins. We identified the minimal portion of the vWF molecule, able to enhance reconstitution of fVIII from isolated subunits. Only vWF large proteolytic N-terminal homodimeric fragment SPIII (vWF residues 1–1365), but not small monomeric N-terminal fragment SPIII-T4 (1–272), both of which are known to contain a major fVIII binding site, was able to support reconstitution of fVIII activity from isolated LCh and HCh subunits in the presence of Mn 2+ or Ca 2+ . The effect of SPIII on the LCh/HCh association was similar to that of vWF, because both proteins identically increased of the value of k on and did not alter the k off value.

Published

1999

26. Collagen type I modulates the platelet-derived growth factor (PDGF) regulation of the growth and expression of beta1 integrins by rat mesangial cells

Author

Shoji Kagami, Yashuhiro Kuroda, Klemens Löster, Akiko Kitamura, Shuji Kondo, Werner Reutter, Shoko Kobayashi, and Maki Urushihara

Subjects

Platelet-derived growth factor, Cell, Integrin, Biophysics, Becaplermin, Biochemistry, Collagen receptor, Extracellular matrix, Rats, Sprague-Dawley, chemistry.chemical_compound, medicine, Animals, Molecular Biology, Cells, Cultured, Platelet-Derived Growth Factor, Mesangial cell, biology, Chemistry, Cell growth, Integrin beta1, Cell Biology, Proto-Oncogene Proteins c-sis, Molecular biology, Glomerular Mesangium, Rats, medicine.anatomical_structure, biology.protein, Collagen, Platelet-derived growth factor receptor, Cell Division

Abstract

Mesangial cell (MC) proliferation and the deposition of collagen type I (collagen I) are the major pathological features in many types of glomerulonephritis (GN). Recent work suggested that beta-integrins play a critical role in the cell proliferation and extracellular matrix (ECM) remodeling observed in tissue repair after injury. To examine the involvement of beta-integrins in MC proliferation in association with the interaction of MCs with pathological collagen I, we investigated the effect of a prominent mitogen, platelet-derived growth factor-BB (PDGF-BB) on the growth and expression of beta-integrins by MCs cultured on plastic or in a three-dimensional collagen I gel. Immunoprecipitation using 35S-metabolic labeling, flow cytometry and a 3H-thymidine-uptake analysis demonstrated that PDGF-BB stimulated the cell mitogenicity and the expression of alpha5beta1 integrin (a fibronectin receptor), but not alpha1beta1 integrin (a collagen and laminin receptor) of MCs on plastic, in a dose-dependent manner. In contrast, MCs in the collagen I gels showed no significant changes in mitogenicity or alpha1beta1 and alpha5beta1 integrin expression, but increased alpha1beta1 integrin-mediated gel contraction was observed after PDGF-BB stimulation. Thus, the parallel up-regulation of MC-mitogenicity and alpha5beta1 integrin expression by PDGF-BB suggested that alpha5beta1 integrin is an important ECM receptor involved in the proliferative phenotype of MC. A spatial interaction between MCs and pathological collagen I in GN may influence the PDGF regulation of the MC phenotype regarding the cell growth and the expression of beta1 integrins.

Published

1998

27. Cultured dermal papilla cells of the rat vibrissa follicle. Proliferative activity, adhesion properties and reorganization of the extracellular matrix in vitro

Author

Klemens Löster, Ulrike Blume-Peytavi, Constantin E. Orfanos, Margarete Schön, Michael P. Schön, Christian Sommer, and Brigitte Almond-Roesler

Subjects

Pathology, medicine.medical_specialty, Integrins, Integrin, Dermatology, Extracellular matrix, Hair cycle, Laminin, medicine, Cell Adhesion, Animals, reproductive and urinary physiology, Cells, Cultured, Skin, Basement membrane, integumentary system, biology, General Medicine, Fibroblasts, Hair follicle, Cell biology, Extracellular Matrix, Rats, Fibronectin, Dermal papillae, medicine.anatomical_structure, Vibrissae, embryonic structures, biology.protein, Collagen, Hair Follicle

Abstract

The dermal papilla of the mammalian hair follicle plays an important role in regulating and controlling the hair cycle. Distinct functional stages of dermal papilla cells (DPC) are involved in this process, thus suggesting that the dermal papilla is a highly specialized suborgan of the pilosebaceous unit. The aim of the present study was to investigate the functional properties of cultured DPC in various assays and to compare their functional properties with those of dermal fibroblasts (DFB). In monolayer cell cultures DPC showed an aggregative growth pattern, different to that of DFB, and lower proliferation rates, as compared to the controls. Adhesion assays performed using a 51[Cr]labeling method showed strong adhesion of both cell populations to collagen types I and IV, fibronectin and laminin, but DPC in vitro showed significantly higher adhesiveness to collagen type IV, a major component of the basement membrane of dermal papillae in vivo. The capacity of DPC to reorganize extracellular matrix components, as measured by gel contraction with three-dimensional collagen type I lattices, proved to be significantly lower than that of DFB and, moreover, DPC lysed the collagen lattices completely after 48 h in culture. The functional differences between DPC and DFB were paralleled by higher surface expression and synthesis levels of the beta 1, alpha 1, and alpha 5 chains of integrin adhesion receptors in DPC, as detected by fluorescence-activated cell-sorter analysis and radioimmunoprecipitation. These findings provide evidence that DPC are a highly specialized cell population, which clearly differs from another mesenchymal cell type, DFB. After their isolation and cultivation in vitro, DPC still preserve functional properties related to important steps of cell-matrix interaction involved in the hair cycle.

Published

1998

28. Quantification of cell-matrix and cell-cell adhesion using horseradish peroxidase

Author

Klemens Löster, Claudia Heidrich, Cora Schüler, Werner Reutter, and Rüdiger Horstkorte

Subjects

Cell, Biophysics, Phenylenediamines, Endocytosis, Biochemistry, Horseradish peroxidase, Sensitivity and Specificity, Extracellular matrix, chemistry.chemical_compound, medicine, Cell Adhesion, Tumor Cells, Cultured, Animals, Humans, Hydrogen peroxide, Cell adhesion, Molecular Biology, Horseradish Peroxidase, biology, Staining and Labeling, Chemistry, food and beverages, Antibodies, Monoclonal, Cell Biology, Adhesion, Chromium Radioisotopes, Rats, medicine.anatomical_structure, Cell culture, biology.protein, Collagen, Interleukin-1

Abstract

A simple, universal, and rapid enzymatic method for the quantitative determination of cell adhesion in 96-well cell culture plates has been established. The assay is based on cellular steady-state endocytosis, which is used to label cells with horseradish peroxidase (HRP) prior to adhesion. Subsequently, attached cells can be detected by a simple enzymatic reaction, in which the accumulated HRP catalyzes dye formation from a colorless hydrogen donor, e.g., o-phenylenediamine, in the presence of hydrogen peroxide. As demonstrated with different cell lines and test systems, the method can be used to quantify cell-matrix as well as cell-cell interactions and allows a very sensitive quantification of adherent cells. The HRP label is nontoxic and does not affect the adhesion properties of tested cell lines; the quantity of dye formed is proportional to the number of adherent cells. Furthermore, the assay represents an alternative method to isotopic cell labeling, e.g., with 51Cr, which is usually used for quantifying cell-cell interactions.

Published

1997

29. Transforming growth factor-beta (TGF-beta) stimulates the expression of beta1 integrins and adhesion by rat mesangial cells

Author

Werner Reutter, Kaname Okada, Klemens Löster, Shoji Kagami, Yasuhiro Kuroda, Takashi Kuhara, and Koji Yasutomo

Subjects

Transcription, Genetic, Integrin, Ligands, Collagen receptor, Rats, Sprague-Dawley, Laminin, Transforming Growth Factor beta, Cell Adhesion, Animals, Humans, Northern blot, RNA, Messenger, Cells, Cultured, Extracellular Matrix Proteins, biology, Cell adhesion molecule, Integrin beta1, Cell Biology, Adhesion, Molecular biology, Fibronectins, Glomerular Mesangium, Rats, Fibronectin, biology.protein, Collagen, Oligopeptides, Transforming growth factor

Abstract

Transforming growth factor-beta (TGF-beta) has been implicated in the pathogenesis of mesangial matrix (MM) accumulation in human and experimental glomerulonephritis. To clarify molecular mechanisms responsible for pathological MM deposition, we examined the effect of TGF-beta on the production of beta1 integrins and on adhesion function of rat mesangial cells (MC). In immunoprecipitation experiments using [35S]methionine-labeled MC, stimulation of MC with TGF-beta for 48 h resulted in an increase in the synthesis of alpha1beta1 (collagen/laminin receptor) and alpha5beta1 (fibronectin receptor) integrins accompanied by increases in the synthesis of their ligands, collagen type I (collagen I), and fibronectin. A time-dependent increase in beta1, alpha1 integrin subunit mRNA peaking 48 h after exposure to TGF-beta was shown by Northern blot analysis. After 48 h of treatment with TGF-beta, MC displayed significant increases in adhesion to fibronectin, collagen I, and laminin as compared to untreated MC. Anti-beta1 antiserum significantly inhibits MC adhesion to fibronectin, collagen I, and laminin. Anti-alpha1 subunit antibody very strongly inhibited adhesion to collagen I and laminin, but not to fibronectin. Synthetic peptides containing RGD sequences specifically blocked adhesion to fibronectin. These data suggest that TGF-beta may promote MM deposition by increasing MC synthesis of both matrix proteins and beta1 integrins which facilitate binding of these proteins to the MC surface and thus enhance their incorporation into MM.

Published

1996

30. The cysteine-rich region of dipeptidyl peptidase IV (CD 26) is the collagen-binding site

Author

Klemens Löster, Werner Reutter, K. Zeilinger, and Detlef Schuppan

Subjects

animal structures, Dipeptidyl Peptidase 4, Molecular Sequence Data, Biophysics, In Vitro Techniques, Ligands, Biochemistry, Epitope, Dipeptidyl peptidase, Catalysis, Mice, Laminin, Animals, Humans, Amino Acid Sequence, Cysteine, Binding site, Molecular Biology, chemistry.chemical_classification, Exopeptidase activity, Binding Sites, biology, Cell Membrane, Cell Biology, Ligand (biochemistry), Molecular biology, Rats, Fibronectin, chemistry, Liver, biology.protein, Collagen, Glycoprotein

Abstract

A remarkable property of the integral glycoprotein dipeptidyl peptidase IV (DPP IV, CD 26) is its affinity to proteins of the extracellular matrix (ECM). By in vitro binding assays we have shown that DPP IV binds to collagens; preferentially to the collagens I and III, which are both characterized by the formation of large triplehelical domains. No binding of DPP IV to laminin or fibronectin could be observed. Within collagen I, the αl(I) chain was found to be the most prominent binding ligand of DPP IV. A monoclonal anti DPP IV antibody (13.4) specifically inhibited the interaction of DPP IV with collagen I. Peptide mapping and N-terminal sequencing revealed that the corresponding epitope of mAb 13.4 is located in the cysteine-rich domain of DPP IV. We therefore conclude that the putative collagen binding site of DPP IV is different from the region of the catalytic site containing the exopeptidase activity, which is located at the C-terminal portion of the molecule.

Published

1995

31. Chemical cross-linking leads to two high molecular mass aggregates of rat alpha 1 beta 1 integrin differing in their conformation but not in their composition

Author

Klemens Löster, Werner Hofmann, Oliver Baum, and Werner Reutter

Subjects

Integrins, Octoxynol, Protein Conformation, Protein subunit, Dipeptidyl Peptidase 4, Integrin, Immunoblotting, Biophysics, Succinimides, Biochemistry, Chromatography, Affinity, Collagen receptor, Protein–protein interaction, Integrin alpha1beta1, Structural Biology, Genetics, Animals, Disulfides, Receptor, Molecular Biology, Rat α1β1 integrin, Molecular mass, biology, Chemistry, Cell Membrane, Membrane Proteins, Cell Biology, In vitro, Protein tertiary structure, Protein Structure, Tertiary, Rats, Molecular Weight, Dithiothreitol, Cross-Linking Reagents, Liver, Chemical cross-linking, biology.protein, Collagen

Abstract

In order to detect protein interactions of the collagen/laminin receptor alpha 1 beta 1 integrin, covalent chemical cross-linking was performed with the homo-bifunctional, amine reactive reagents DSS (disuccinimidylsuberate) and DSP (dithiobis(succinimidylpropionate)). After cross-linking of the 190 kDa rat alpha 1 integrin subunit, immunoblotting revealed two additional, immunoreactive, high molecular mass complexes (M(r) 240/290 k). Generation of the 240/290 kDa aggregates depended on the presence of the intact tertiary protein structure. As shown with immunoaffinity purified proteins, the 240/290 kDa aggregates consist exclusively of alpha 1 and beta 1 integrin subunits. No other cross-linked proteins associated with the alpha 1 or beta 1 subunit were detected. In contrast to the non-cross-linkable alpha 1 beta 1 integrin, the 240/290 kDa aggregates presumably represent active forms of the adhesion receptor, because both bound in vitro to collagen I and IV. This ability of alpha 1 beta 1 integrin to cross-link and produce two additional high molecular mass forms is shared by rat alpha 9 beta 1 integrin. Thus, the cross-linking approach directly indicates that beta 1 integrins occur in different conformations caused by variations in the folding and/or spatial arrangement of their subunits.

Published

1995

32. Characterization of molecular aggregates of alpha 1 beta 1-integrin and other rat liver membrane proteins by combination of size-exclusion chromatography and chemical cross-linking

Author

Werner Hofmann, Oliver Baum, Werner Reutter, and Klemens Löster

Subjects

Integrins, Protein Denaturation, Dipeptidyl Peptidase 4, Size-exclusion chromatography, Integrin, Protein aggregation, Biochemistry, Aminopeptidase, Analytical Chemistry, Integrin alpha1beta1, Antigens, CD, Animals, Cytoskeleton, Adenosine Triphosphatases, Chromatography, biology, Chemistry, Binding protein, Organic Chemistry, Membrane Proteins, General Medicine, Rats, Membrane, Cross-Linking Reagents, Membrane protein, Liver, biology.protein, Chromatography, Gel, Cell Adhesion Molecules

Abstract

Many membrane proteins display their biological activity in molecular aggregates of interacting counterparts. The analysis of these aggregates remains difficult; especially intermolecular complexes of membrane proteins tend to dissociate or artificially aggregate during detergent extraction out of membranes. Thus, the existence of protein aggregates was investigated by two approaches. First, after modest detergent extraction, the presence of three well characterized rat liver membrane proteins, α 1 β 1 -integrin, dipeptidyl aminopeptidase IV (DPP IV) and cell-CAM 105 (CAM = cell adhesion molecule), in aggregates could be demonstrated when investigated by size-exclusion chromatography (SEC) under non-denaturating conditions. However, the applied detergents partially influenced the resolution of the separation reducing the ability to discriminate between native and artificial protein aggregates. To circumvent these problems, a second approach based on covalent cross-linking of native protein complexes by dithiobis(succinimidylpropionate) was combined with the performance of denaturating SEC. Under such optimized conditions the expression of α 1 β 1 -integrin as heterodimer and DPP IV as homodimer was confirmed. In addition, some high-molecular-mass complexes of all model proteins consisting of unknown components could also be detected. Taken together, non-denaturating SEC and chemical cross-linking in combination with denaturating SEC represent methodological approaches for the characterization of protein aggregates.

Published

1995

33. Distribution and quantification of alpha1-integrin subunit in rat organs

Author

Sebastian Voigt, Klemens Löster, Werner Hofmann, Reinhart Gossrau, Oliver Baum, and Werner Reutter

Subjects

Male, Integrins, medicine.drug_class, Protein subunit, Immunoblotting, Integrin alpha1, Enzyme-Linked Immunosorbent Assay, Spleen, Monoclonal antibody, Antibody Specificity, Laminin, medicine, Animals, Rats, Wistar, Antiserum, biology, Antibodies, Monoclonal, Cell Biology, Epididymis, Immunohistochemistry, Molecular biology, Rats, medicine.anatomical_structure, Polyclonal antibodies, biology.protein, Female, Collagen, Anatomy

Abstract

The alpha 1 beta 1-integrin is known to be a receptor for collagen and laminin mediating cell-matrix interactions. A monoclonal antibody, 33.4, which specifically inhibits the alpha 1-integrin-mediated in vitro cell-collagen binding of rat hepatocytes and hepatoma-derived A-cells (Löster et al., 1994), was used to purify by immunoaffinity chromatography the alpha 1-integrin subunit from rat liver in large quantities for inducing a polyclonal antiserum. In immunoblot analysis on membrane extracts of several rat organs this polyclonal antiserum recognized only a 190 kDa-band, suggesting that it is highly specific for the alpha 1-integrin subunit. A sandwich-ELISA with monoclonal antibody 33.4 and the polyclonal antiserum against the alpha 1-integrin subunit, respectively, enabled the quantitative expression pattern of the alpha 1-integrin subunit to be studied in different rat organs. With the exceptions of brain (not detectable) and muscle (low concentration), the alpha 1-integrin subunit was detectable in almost all organs of the digestive, respiratory and urogenital system as well as in lymphatic organs. The highest relative concentrations of alpha 1-integrin subunit were found in uterus, lung and spleen, whereas in seminal vesicle, stomach, parotid gland, epididymis, kidney and liver only modest concentrations were evident. The organ distribution and localization of alpha 1-integrin subunit were studied by immunohistochemistry with monoclonal and polyclonal antibodies. Immunoreactivity was present in the plasma membranes of all smooth muscle cells, vascular endothelial cells of many organs and fibrocyte-fibroblast sheaths in the heart and kidney. Since these cells are in close contact with collagen-containing basal membranes as well as reticular fibrils, strong evidence exists that in rat tissues the alpha 1-integrin subunit is expressed at sites where collagen is present and might be involved in vivo in cell-collagen binding.

Published

1995

34. 034 Detection of different isoforms of monoclonal antibodies by hydroxylapatite HPLC

Author

Klemens Löster, J. Reusch, R. Kuhl, and Djuro Josic

Subjects

Gene isoform, chemistry.chemical_compound, Chromatography, Chemistry, medicine.drug_class, medicine, Physical Chemistry, Analytical Chemistry, HPLC, Monoclonal Antibody, Inorganic Chemistry, Hydroxylapatite, Monoclonal antibody, Biochemistry, High-performance liquid chromatography

Abstract

The application of monoclonal antibodies (mAbs) for biotechnological and diagnostical purposes needs well characterized antibody preparations with identical biochemical and antigen binding properties. Chromatography on hydroxylapatite is a suitable method for the purification of mAbs under very mild conditions. By using hydroxylapatite HPLC (HA- HPLC) we tried to characterize different mAbs.

Published

1992

35. Inhibition of urokinase activity and prevention of urokinase receptor binding by monoclonal antibodies

Author

Frank Schneider, Horst Will, Klemens Löster, Wilhelm Handschack, Franz Noll, Ute Zacharias, and Christel Kleitke

Subjects

medicine.drug_class, medicine.medical_treatment, Immunology, Blotting, Western, Antibody Affinity, Receptors, Cell Surface, In Vitro Techniques, Monoclonal antibody, Receptors, Urokinase Plasminogen Activator, Antigen, Antibody Specificity, medicine, Immunology and Allergy, Humans, Receptor, Urokinase, Protease, biology, Chemistry, Antibodies, Monoclonal, Molecular biology, Urokinase-Type Plasminogen Activator, Peptide Fragments, Urokinase receptor, Biochemistry, Tissue Plasminogen Activator, biology.protein, Antibody, Plasminogen activator, medicine.drug, Granulocytes

Abstract

Two murine monoclonal antibodies produced against human urokinase-type plasminogen activator were characterized with respect to their antigen-binding specificity and their effects on urokinase activity and urokinase receptor binding. One of the antibodies binds to the protease domain of urokinase (Kass = 2.1 X 10(7) M-1). Antibody binding inhibits catalysis of plasminogen activation. It does not, however, affect amidolytic activity of urokinase towards the chromogenic substrate D-Val-Leu-Arg-p-nitroanilide. The antibody thus appears to interfere with plasminogen binding without directly affecting catalytically active amino acid residues of the enzyme. The other antibody binds to the aminoterminal fragment of urokinase (Kass = 1.0 X 10(7) M-1) and prevents binding of the enzyme to high affinity receptors on human granulocytes. Binding of this antibody neither influences plasminogen activation nor the amidolytic activity of urokinase. Both antibodies are potentially useful for the further analysis and manipulation of urokinase function.

Published

1990

36. Erratum to: 'Use of surface plasmon resonance for studies of protein–protein and protein–phospholipid membrane interactions. Application to the binding of factor VIII to von Willebrand factor and to phosphatidylserine-containing membranes'

Author

Horst Schwinn, Klemens Löster, Evgueni L. Saenko, Andrey Sarafanov, Djuro Josic, N Greco, and Midori Shima

Subjects

Chromatography, biology, Protein protein, Organic Chemistry, Phospholipid, General Medicine, Phosphatidylserine, Biochemistry, Analytical Chemistry, chemistry.chemical_compound, Membrane, Von Willebrand factor, chemistry, biology.protein, Biophysics, Surface plasmon resonance

Published

2000

37. PDGF-BB enhances α1β1 integrin-mediated activation of the ERK/AP-1 pathway involved in collagen matrix remodeling by rat mesangial cells.

Author

Shoji Kagami, Maki Urushihara, Akiko Kitamura, Shuji Kondo, Tetsuhiro Hisayama, Masanori Kitamura, Klemens Löster, Werner Reutter, and Yasuhiro Kuroda

Subjects

BLOOD platelets, GROWTH factors, COLLAGEN, CARCINOGENESIS

Abstract

Platelet-derived growth factor-BB (PDGF-BB) has been implicated in the pathogenesis of progressive glomerulonephritis (GN). Previous studies have reported that PDGF-BB stimulates mesangial cells (MCs)-induced collagen matrix remodeling through enhancement of α1β1 integrin-dependent migratory activity. To determine the cell signaling pathway responsible for abnormal MC-related mesangial matrix remodeling in progressive GN, we studied the involvement of the extracellular signal-regulated kinase (ERK)/activator protein-1 (AP-1) pathway in PDGF-BB-enhanced collagen gel contraction. Western blotting and gel shift assay revealed that MC-induced gel contraction resulted in ERK activation in parallel with that of AP-1 binding, peaking at 4 h and lasting at least for 24 h. Application of the MEK inhibitor, U0126, and the c-jun/AP-1 inhibitor, curcumin, inhibited gel contraction and AP-1 activity, respectively, dose dependently. PDGF-BB enhanced not only gel contraction but ERK phosphorylation and AP-1 activity by MCs. Marked inhibitory effects on PDGF-BB-induced gel contraction and ERK/AP-1 activity were observed in the presence of either function blocking anti-α1- or anti-β1-integrin antibody or U0126. Consistently, AP-1-inactive MCs expressing a dominant-negative mutant of c-jun showed a significant decrease of PDGF-BB-induced gel contraction as compared with mock-transfected MCs. Finally, migration assay showed that ERK/AP-1 activity is required for PDGF-BB-stimulated α1β1 integrin-dependent MC migration to collagen I. These results indicated that PDGF-BB enhances α1β1 integrin-mediated collagen matrix reorganization through the activation of the ERK/AP-1 pathway that is crucial for MC migration. We conclude that the ERK/AP-1 pathway plays an important role in PDGF-BB-induced α1β1 integrin-dependent collagen matrix remodeling; therefore, the inhibition of its pathway may provide a novel approach to regulate abnormal collagen matrix remodeling in progressive GN. J. Cell. Physiol. 198: 470–478, 2004© 2003 Wiley-Liss, Inc. [ABSTRACT FROM AUTHOR]

Published

2004

38. Rat dipeptidyl peptidase IV (DPP IV) exhibits endopeptidase activity with specificity for denatured fibrillar collagens

Author

Klemens Löster, Oliver Baum, Werner Reutter, and Felix Bermpohl

Subjects

Proteases, Protein Denaturation, Kidney Cortex, animal structures, Dipeptidyl Peptidase 4, Biophysics, Biochemistry, Dipeptidyl peptidase, Substrate Specificity, Endopeptidase activity, Structural Biology, Endopeptidases, Genetics, medicine, Animals, Protease Inhibitors, Molecular Biology, Endopeptidase, Serine protease, Exopeptidase activity, Gelatin zymography, biology, Chemistry, Gelatinolytic integral membrane serine protease, Cell Membrane, Cell Biology, Exopeptidase, Molecular biology, Collagen degradation, Protease inhibitor (biology), Rats, Kinetics, Dipeptidyl peptidase IV, biology.protein, Electrophoresis, Polyacrylamide Gel, Collagen, medicine.drug

Abstract

Dipeptidyl peptidase IV (DPP IV, CD 26) is an integral membrane serine protease exhibiting a well characterized exopeptidase activity. The present study shows that DPP IV also possesses a novel gelatinase activity and therefore endopeptidase activity, which was directly demonstrated by gelatin zymography. Protease inhibitor profile analysis showed that the endo- and exopeptidase activities of DPP IV share a common active site. Substrate specificity was detected for denatured collagen types I, II, III and V suggesting that DPP IV might contribute to collagen trimming and metabolism. On the basis of these data we propose that DPP IV and the recently sequenced gelatinolytic seprase (FAPα) represent a new subfamily of gelatinolytic integral membrane serine proteases.