39 results on '"Kresse, H."'
Search Results
2. A dielectric study of nematogen 4-n-hexyloxyphenyl 4-n-methoxybenzoate, C1O/OC6
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Kresse, H., primary and Mościcki, J.K., additional
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- 1981
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3. Sulfatase Deficiencies in Mucopolysaccharidoses
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KRESSE, H., primary and VON FIGURA, K., additional
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- 1975
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4. Specificity of Pinocytosis of α-N-acetylglucosaminidase by Fibroblasts
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VON FIGURA, K., primary and KRESSE, H., additional
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- 1975
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5. Dielectric investigations of 4-n-pentylphenyl-4-n-heptyloxythiobenzoate (7S5)
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Chruσciel, J., primary, Wröbel, S., additional, Janik, J.A., additional, Janik, J.M., additional, and Kresse, H., additional
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- 1981
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6. A physiologic three-dimensional cell culture system to investigate the role of decorin in matrix organisation and cell survival.
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Seidler DG, Schaefer L, Robenek H, Iozzo RV, Kresse H, and Schönherr E
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- Animals, Apoptosis, Ascorbic Acid metabolism, Caspase 3, Caspase 8, Caspases metabolism, Cell Communication, Cell Line, Cell Proliferation, Cell Survival, Cells, Cultured, Collagen chemistry, Collagen Type I chemistry, Collagen Type V chemistry, Decorin, Extracellular Matrix Proteins, Fibroblasts metabolism, Humans, Mice, Mice, Transgenic, Microscopy, Electron, Pepsin A chemistry, Phenotype, Proteoglycans chemistry, Proteoglycans metabolism, Ascorbic Acid analogs & derivatives, Proteoglycans physiology
- Abstract
In vivo cells exist in a three-dimensional environment generated and maintained by multiple cell-cell and cell-matrix interactions. Proteoglycans, like decorin, affect these complex interactions. Thus, we sought to investigate the role of decorin in a three-dimensional environment where the matrix was generated over time by decorin-deficient fibroblasts in the presence of L-ascorbic acid 2-phosphate. The cells were viable and proliferated in response to FGF2. Decorin was incorporated in the matrix and caused a approximately 2 nm shift in the average diameter of the collagen fibrils, and the range and distribution of the fibrils became narrower and more uniform. Although there were no appreciable changes in collagen composition, we found that exogenous decorin induced the de novo synthesis of collagen I and V and cross-linked beta(I). In the early phases of the three-dimensional culture, decorin reduced apoptosis. However, following the establishment of a three-dimensional matrix, the cells did not require decorin for their survival.
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- 2005
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7. Expression of transcription factors and matrix genes in response to serum stimulus in vascular smooth muscle cells.
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Markmann A, Rauterberg J, Vischer P, Robenek H, Echtermeyer F, Will H, Seidler DG, Young MF, and Kresse H
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- Adenoviridae growth & development, Animals, Arteriosclerosis metabolism, Arteriosclerosis pathology, Cells, Cultured, Cloning, Molecular, Culture Media pharmacology, Culture Media, Serum-Free pharmacology, Culture Techniques, DNA-Binding Proteins genetics, Decorin, Down-Regulation, Extracellular Matrix Proteins, GATA6 Transcription Factor, Gene Expression Regulation drug effects, Homeodomain Proteins genetics, Host Cell Factor C1, Immunohistochemistry, In Situ Hybridization, Integrin alpha2 genetics, Kinetics, Laminin genetics, Muscle Proteins genetics, Muscle, Smooth, Vascular cytology, Muscle, Smooth, Vascular virology, Octamer Transcription Factor-1, Osteopontin, Proteoglycans genetics, Sialoglycoproteins genetics, Swine, Up-Regulation, Extracellular Matrix metabolism, Muscle, Smooth, Vascular metabolism, Transcription Factors genetics
- Abstract
During atherogenesis vascular smooth muscle cells are converted from a contractile into a synthetic phenotype characterized by enhanced matrix production. The transcription factors Gax and GATA-6 are considered negative, and Oct-1 positive regulators of the synthetic phenotype. Since the phenotype transition can be induced by culturing the cells with serum, we followed the expression of Gax, GATA-6 and Oct-1, integrins and matrix genes in quiescent porcine vascular smooth muscle cells after serum application. Comparisons were made between enzymatically released primary smooth muscle cells and cells grown out from explants of the medial layer of porcine aorta. The serum-mediated down-regulation of Gax was more intense than that of GATA-6, and stronger in explant-derived than in primary cells. Serum was without influence on the expression of Oct-1. Changes in the expression of the transcription factors preceded the induction of integrin alpha2 and the down-regulation of decorin, while mRNAs for laminin beta1 and osteopontin rose immediately after serum stimulation. Primary cells reacted more rapidly than explant cells with respect to changes in laminin isoforms. Studies with a Gax-expressing adenovirus indicated that among all the gene products tested only the expression of integrin alpha2 responded to Gax induction. Thus, our data show that i) Gax should be considered a transcription factor being directly responsible for only few aspects of the phenotypic conversion of smooth muscle cells and that ii) explant cells may represent a subpopulation of smooth muscle cells, which differ from the total population of smooth muscle cells, as obtained in primary culture, in their response to serum stimuli.
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- 2003
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8. Absence of decorin adversely influences tubulointerstitial fibrosis of the obstructed kidney by enhanced apoptosis and increased inflammatory reaction.
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Schaefer L, Macakova K, Raslik I, Micegova M, Gröne HJ, Schönherr E, Robenek H, Echtermeyer FG, Grässel S, Bruckner P, Schaefer RM, Iozzo RV, and Kresse H
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- Animals, Decorin, Extracellular Matrix Proteins, Fibrosis, Gene Deletion, Kidney pathology, Mice, Apoptosis genetics, Disease Models, Animal, Kidney Diseases genetics, Kidney Diseases pathology, Proteoglycans genetics
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Decorin, a small dermatan-sulfate proteoglycan, participates in extracellular matrix assembly and influences directly and indirectly cell behavior via interactions with signaling membrane receptors and transforming growth factor (TGF)-beta. We have therefore compared the development of tubulointerstitial kidney fibrosis in wild-type (WT) and decorin-/- mice in the model of unilateral ureteral obstruction. Without obstruction, kidneys from decorin-/- mice did not differ in any aspect from their WT counterparts. However, already 12 hours after obstruction decorin-/- animals showed lower levels of p27(KIP1) and soon thereafter a more pronounced up-regulation and activation of initiator and effector caspases followed by enhanced apoptosis of tubular epithelial cells. Later, a higher increase of TGF-beta1 became apparent. After 7 days, there was an up to 15-fold transient up-regulation of the related proteoglycan biglycan, which was mainly caused by the appearance of biglycan-expressing mononuclear cells. Other small proteoglycans showed no similar response. Because of enhanced degradation of type I collagen, end-stage kidneys from decorin-/- animals were more atrophic than WT kidneys. These data suggest that decorin exerts beneficial effects on tubulointerstitial fibrosis, primarily by influencing the expression of a key cyclin-dependent kinase inhibitor and by limiting the degree of apoptosis, mononuclear cell infiltration, tubular atrophy, and expression of TGF-beta1.
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- 2002
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9. Influence of decorin expression on transforming growth factor-beta-mediated collagen gel retraction and biglycan induction.
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Markmann A, Hausser H, Schönherr E, and Kresse H
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- Biglycan, Decorin, Extracellular Matrix Proteins, Gels, Gene Expression Regulation, Humans, Proteoglycans genetics, Proteoglycans pharmacology, Transforming Growth Factor beta antagonists & inhibitors, Tumor Cells, Cultured, Collagen metabolism, Proteoglycans biosynthesis, Proteoglycans metabolism, Transforming Growth Factor beta metabolism
- Abstract
Complex formation of transforming growth factor-beta (TGF-beta) with the small proteoglycan decorin has been considered to inactivate the cytokine. However, neither the TGF-beta-mediated stimulation of the retraction of collagen lattices in culture nor the enhanced transcription of biglycan were influenced by an excess of native decorin in the culture medium. In contrast, when MG-63 osteosarcoma cells were transfected with sense- or antisense-decorin-cDNA, which led to an over- or under-expression of the proteoglycan, they responded to TGF-beta differently. An inverse correlation between decorin expression and the TGF-beta-mediated stimulation of collagen gel retraction and biglycan induction, respectively, was found. These results are best explained by assuming that decorin is not inactivating but sequestering TGF-beta in the extracellular matrix.
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- 2000
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10. Lipoprotein lipase-mediated interactions of small proteoglycans and low-density lipoproteins.
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Schönherr E, Zhao B, Hausser H, Müller M, Langer C, Wagner WD, Goldberg IJ, and Kresse H
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- Biglycan, Chromatography, Gel, Decorin, Dose-Response Relationship, Drug, Endocytosis, Extracellular Matrix Proteins, Fibroblasts metabolism, Heparin metabolism, Humans, Lipoproteins, LDL pharmacokinetics, Protein Binding, Lipoprotein Lipase metabolism, Lipoproteins, LDL metabolism, Proteoglycans metabolism
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According to numerous studies low-density lipoproteins (LDL) are supposed to interact with the glycosaminoglycan chain(s) of proteoglycans, e.g. with decorin and biglycan, which themselves are subject to receptor-mediated endocytosis. We tested, therefore, whether complexes of LDL and small proteoglycans can be endocytosed by either the LDL- or the small proteoglycan uptake mechanism. However, neither was the endocytosis of LDL significantly influenced by proteoglycans nor that of proteoglycans by LDL. This negative result could be explained by the observation that in vitro complex formation takes place only in buffers of low ionic strength. Under physiological conditions additional molecules may be necessary for complex stabilization. Lipoprotein lipase (LpL) which binds LDL was also able to interact with high affinity with decorin and its glycosaminoglycan-free core protein, both interactions being heparin-sensitive. Regardless of the presence or absence of LDL, LpL stimulated the endocytosis of decorin 1.5-fold, whereas LpL mediated a 4-fold stimulation of LDL uptake in the absence of decorin. No significant additional effect was seen in the presence of small concentrations of proteoglycans whereas in the presence of 1 microM decorin the endocytosis of [125I]LDL was reduced in normal as well as in LDL receptor-deficient fibroblasts. These observations could best be explained by assuming that LpL/LDL complexes are internalized upon binding to membrane-associated heparan sulphate and that small proteoglycans interfere with this process. It could not be ruled out, however, that a small proportion of the complexes is also taken up by the small proteoglycan receptor.
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- 2000
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11. Small proteoglycans of normal adult human kidney: distinct expression patterns of decorin, biglycan, fibromodulin, and lumican.
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Schaefer L, Gröne HJ, Raslik I, Robenek H, Ugorcakova J, Budny S, Schaefer RM, and Kresse H
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- Adult, Arterioles chemistry, Arterioles metabolism, Basement Membrane chemistry, Basement Membrane metabolism, Basement Membrane ultrastructure, Biglycan, Biopsy, Carrier Proteins analysis, Chondroitin Sulfate Proteoglycans analysis, Decorin, Endocytosis physiology, Epithelial Cells chemistry, Epithelial Cells metabolism, Epithelial Cells ultrastructure, Female, Fibromodulin, Gene Expression physiology, Glomerular Mesangium chemistry, Glomerular Mesangium cytology, Glomerulonephritis, Membranous metabolism, Glomerulonephritis, Membranous pathology, Humans, In Situ Hybridization, Keratan Sulfate analysis, Kidney Cortex cytology, Kidney Cortex metabolism, Kidney Tubules, Distal chemistry, Kidney Tubules, Distal cytology, Lumican, Male, Microscopy, Immunoelectron, Middle Aged, Proteoglycans analysis, Proteoglycans urine, RNA, Messenger analysis, Carrier Proteins genetics, Chondroitin Sulfate Proteoglycans genetics, Extracellular Matrix Proteins, Glomerular Mesangium metabolism, Keratan Sulfate genetics, Kidney Tubules, Distal metabolism, Proteoglycans genetics
- Abstract
Background: Among the members of the small leucine-rich proteoglycan family, decorin, biglycan, and fibromodulin have been proposed to be potent modulators of transforming growth factor-beta (TGF-beta) activity, thereby playing an important role in the pathogenesis of fibrotic kidney diseases. Furthermore, decorin expression influences the expression of p21WAF1/CIP1, which has been related to kidney hypertrophy and hyperplasia. However, none of the members of this proteoglycan family have been investigated in normal adult human kidney cortex, thus making it impossible to correlate disease-mediated alterations of their expression with the normal situation in vivo., Methods: The chondroitin/dermatan sulfate proteoglycans, decorin and biglycan, and the keratan sulfate proteoglycans, fibromodulin and lumican, were investigated in normal human adult renal cortex by immunohistochemistry on the light and electron microscopic level and by in situ hybridization. Northern blot and reverse transcription-polymerase chain reaction (RT-PCR) methods were used to get an estimate of their expression in isolated glomeruli. Decorin excretion with the urine was measured by Western blotting., Results: Two bands of decorin and a single band of biglycan mRNA were identified in Northern blots of isolated glomeruli. Amplification by RT-PCR was required to detect the signals for fibromodulin and lumican. All four proteoglycans were preferentially expressed in the renal interstitium with accumulations around tubules. Weak expression was found in the mesangial matrix. Biglycan was expressed by glomerular endothelial cells and, together with fibromodulin, was synthesized and deposited in distal tubular cells and collecting ducts. Immunogold labeling indicated the presence of the proteoglycans in the glomerular basement membrane, which was interpreted as a result of glomerular filtration. Indirect evidence suggested tubular reuptake of decorin after glomerular filtration., Conclusion: The data indicate that the different cells of the adult human kidney are characterized by a distinct expression pattern of the four small proteoglycans. It is suggested that these proteoglycans may have distinct pathophysiological roles depending upon whether they are expressed by mesangial cells, endothelial cells, epithelial cells, or cells of the tubulointerstitium.
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- 2000
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12. Alternative exon usage of rat septins.
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Jackisch BO, Hausser H, Schaefer L, Kappler J, Müller HW, and Kresse H
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- Amino Acid Sequence, Animals, Base Sequence, Cloning, Molecular, Cytoskeletal Proteins chemistry, Fibroblasts, GTP-Binding Proteins chemistry, GTP-Binding Proteins genetics, In Situ Hybridization, Kidney metabolism, Molecular Sequence Data, Oligonucleotides, Antisense, Protein Isoforms chemistry, Protein Isoforms genetics, RNA, Messenger analysis, RNA, Messenger genetics, Rats, Septins, Sequence Homology, Amino Acid, Alternative Splicing genetics, Cytoskeletal Proteins genetics, Exons genetics, GTP Phosphohydrolases
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Septins represent a family of phylogenetically conserved proteins required for cytokinesis. Their presence in pre- and postsynaptic neuronal membranes suggests a general function as scaffolds for membrane reorganization. The transcriptional regulation of all septins examined so far is complex, resulting in alternatively spliced variants. We focus here on the rat homologue of the gene for the human septin MSF, a truncated form of which, designated eseptin, had been described previously. It will be shown here that there is an alternative usage of the first exon by two forms, named exon r1a and r1b, respectively. Exon r1a, but not exon r1b, contains a part of the coding sequence while the start of translation for the remaining coding sequence resides in the second exon. The complete genomic organization was resolved and data on the temporal and spatial expression of this septins are presented., (Copyright 2000 Academic Press.)
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- 2000
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13. Synthesis of proteoglycans is augmented in dystrophic mdx mouse skeletal muscle.
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Cáceres S, Cuellar C, Casar JC, Garrido J, Schaefer L, Kresse H, and Brandan E
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- Age Factors, Animals, Chromatography, Ion Exchange, Decorin, Diaphragm metabolism, Electrophoresis, Polyacrylamide Gel, Extracellular Matrix Proteins, In Situ Hybridization, Mice, Mice, Inbred C57BL, Mice, Inbred mdx, Regeneration, Up-Regulation, Muscle, Skeletal metabolism, Muscular Dystrophy, Animal metabolism, Proteoglycans biosynthesis
- Abstract
Mdx mice uniquely recover from degenerative dystrophic lesions through an intense myoproliferative response. The onset and progression of this process are controlled by a complex set of interactions between myoblasts and their environment. The presence of the extracellular matrix is essential for normal myogenesis. Proteoglycans are abundant components of the extracellular matrix. The synthesis of proteoglycans in mdx mice during skeletal muscle regeneration was evaluated. Incorporation of radioactive sulfate demonstrated a significant increase in the synthesis of several types of proteoglycans in mdx animals compared to age-matched controls. The size and charge of proteoglycans synthesized by the mdx mice remained unchanged. In particular, one of the up-regulated proteoglycans, the small chondroitin/dermatan sulfate proteoglycan decorin which is known to bind and to sequester transforming growth factor-beta, was investigated. Immunocytolocalization and in situ hybridization studies showed that decorin mainly accumulated in the endomysium, i.e. around individual skeletal muscle fibers from M. tibialis anterior and diaphragm.
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- 2000
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14. Paracrine or virus-mediated induction of decorin expression by endothelial cells contributes to tube formation and prevention of apoptosis in collagen lattices.
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Schönherr E, O'Connell BC, Schittny J, Robenek H, Fastermann D, Fisher LW, Plenz G, Vischer P, Young MF, and Kresse H
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- Adenoviridae, Animals, Biglycan, Blotting, Northern, Cell Line, Chondroitin metabolism, Decorin, Dermatan Sulfate metabolism, Dose-Response Relationship, Drug, Extracellular Matrix Proteins, Fibroblasts metabolism, Fibroblasts ultrastructure, Genetic Vectors, Humans, Immunohistochemistry, In Situ Nick-End Labeling, Microscopy, Electron, Proteoglycans metabolism, Rats, Reverse Transcriptase Polymerase Chain Reaction, Time Factors, Tissue Distribution, Transfection, Apoptosis physiology, Collagen metabolism, Endothelium metabolism, Paracrine Communication, Proteoglycans biosynthesis
- Abstract
Resting endothelial cells express the small proteoglycan biglycan, whereas sprouting endothelial cells also synthesize decorin, a related proteoglycan. Here we show that decorin is expressed in endothelial cells in human granulomatous tissue. For in vitro investigations, the human endothelium-derived cell line, EA.hy 926, was cultured for 6 or more days in the presence of 1% fetal calf serum on top of or within floating collagen lattices which were also populated by a small number of rat fibroblasts. Endothelial cells aligned in cord-like structures and developed cavities that were surrounded by human decorin. About 14% and 20% of endothelial cells became apoptotic after 6 and 12 days of co-culture, respectively. In the absence of fibroblasts, however, the extent of apoptosis was about 60% after 12 days, and cord-like structures were not formed nor could decorin production be induced. This was also the case when lattices populated by EA.hy 926 cells were maintained under one of the following conditions: 1) 10% fetal calf serum; 2) fibroblast-conditioned media; 3) exogenous decorin; or 4) treatment with individual growth factors known to be involved in angiogenesis. The mechanism(s) by which fibroblasts induce an angiogenic phenotype in EA.hy 926 cells is (are) not known, but a causal relationship between decorin expression and endothelial cell phenotype was suggested by transducing human decorin cDNA into EA.hy 926 cells using a replication-deficient adenovirus. When the transduced cells were cultured in collagen lattices, there was no requirement of fibroblasts for the formation of capillary-like structures and apoptosis was reduced. Thus, decorin expression seems to be of special importance for the survival of EA.hy 926 cells as well as for cord and tube formation in this angiogenesis model.
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- 1999
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15. Decorin, biglycan and their endocytosis receptor in rat renal cortex.
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Schaefer L, Hausser H, Altenburger M, Ugorcakova J, August C, Fisher LW, Schaefer RM, and Kresse H
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- Animals, Biglycan, Decorin, Extracellular Matrix Proteins, Glomerular Mesangium metabolism, Glomerulonephritis, Membranoproliferative metabolism, Immunohistochemistry, Male, Proteoglycans genetics, Proteoglycans metabolism, RNA, Messenger analysis, Rats, Rats, Sprague-Dawley, Transforming Growth Factor beta physiology, Endocytosis, Kidney Cortex chemistry, Proteoglycans analysis
- Abstract
Background: Among the small proteoglycans, biglycan and decorin have been proposed to be potent modulators of TGF-beta-mediated inflammatory kidney diseases. They were considered to become induced during glomerulonephritis and to subsequently inactivate the cytokine., Methods: Decorin and biglycan as well as their endocytosis receptor were investigated in normal rat renal cortex, in anti-Thy-1 glomerulonephritis, in polycystic kidneys, in the remnant kidney following 5/6-nephrectomy, and in kidneys from the Milan normotensive strain by immunohistochemistry and in situ hybridization. Northern blots were used for the detection of mRNA expression for decorin and biglycan in isolated glomeruli. Functional aspects of the endocytosis of decorin and biglycan were studied in cultured mesangial cells., Results: In the normal adult rat kidney decorin was expressed preferentially by Bowman's capsule and by interstitial connective tissue cells, but only in trace amounts by mesangial cells. In contrast, biglycan was found in tubular epithelial cells, in association with glomerular capillaries, podocytes and occasionally in the mesangium. In the tubulointerstitium of diseased kidneys (polycystic kidneys, 5/6-nephrectomy, kidneys from the Milan normotensive strain) there was a general up-regulation of decorin expression, while biglycan was localized only in distinct foci of fibrotic lesions. Glomerulosclerosis (5/6-nephrectomy, Milan normotensive strain) was associated with an increased staining for both decorin and biglycan within glomeruli. However, even in the anti-Thy-1 model of an acute mesangioproliferative glomerulonephritis where the greatest accumulation of decorin was found there was only a slight enhancement of decorin mRNA in isolated glomeruli. Decorin and biglycan become degraded upon receptor-mediated endocytosis. Immunohistochemical investigations indicated that the pattern of expression of the receptor protein correlated well with the immunolocalization of both decorin and biglycan. In vitro experiments with cultured mesangial cells provided direct evidence for the expression of the receptor and for the cell's capability to endocytose decorin as well as biglycan., Conclusions: Decorin and biglycan are characterized by a distinct expression pattern in the normal rat kidney, whereas the presence of their endocytosis receptor protein correlates with the expression of both proteoglycans. Decorin is almost completely absent in the normal mesangium. Both proteoglycans become up-regulated in various models of renal disease. The mesangial accumulation of decorin in the anti-Thy-1 glomerulonephritis that is observed in spite of the only slightly enhanced mRNA expression could result from decreased decorin turnover and/or increased mesangial retention.
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- 1998
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16. Decorin core protein fragment Leu155-Val260 interacts with TGF-beta but does not compete for decorin binding to type I collagen.
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Schönherr E, Broszat M, Brandan E, Bruckner P, and Kresse H
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- Binding Sites, Binding, Competitive, Chromatography, Gel, Decorin, Extracellular Matrix Proteins, Humans, Immune Sera pharmacology, Immunoglobulin Fab Fragments metabolism, Immunoglobulin Fab Fragments pharmacology, Leucine metabolism, Monocytes, Peptide Fragments immunology, Peptide Fragments metabolism, Protein Binding, Proteoglycans genetics, Recombinant Proteins metabolism, Tumor Cells, Cultured, Valine metabolism, Collagen metabolism, Proteoglycans metabolism, Transforming Growth Factor beta metabolism
- Abstract
It has been shown that small proteoglycans containing leucine-rich repeats in their core proteins can form complexes with TGF-beta. Decorin, a ubiquitously found molecule of the extracellular matrix, is the best-studied example. Therefore, binding domains on its core protein were investigated using recombinant decorin fragments generated as fusion proteins in prokaryotes. The peptide Leu155-Val260 immobilized by the polyhistidine tag on a nickel chelate column bound TGF-beta1 and -beta2 almost as effectively as the largest fragment (Asp45-Lys359) studied. Other peptides were less effective. For the two peptides Asp45-Lys359 and Leu155-Val260 dissociation constants in the nanomolar range for high-affinity binding sites were calculated in a solid-phase assay with immobilized TGF-beta2. Peptide Asp45-Lys359 also contained a lower affinity binding site. Domains with lower affinity were also found in peptides Asp45-Leu155 and Arg63-Gly190. Peptide Leu155-Val260 also formed complexes with TGF-beta in the liquid phase as determined by equilibrium gel filtration. Furthermore, F(ab') fragments of polyclonal antibodies against peptide Leu155-Val260 interfered with TGF-beta binding to peptide Asp45-Lys359 in a dose-dependent manner. Peptide Leu155-Val260, however, is only a weak competitor of the binding of wild-type decorin to reconstituted type I collagen fibrils. Therefore, independent binding sites of decorin for TGF-beta and type I collagen should exist. In support of this hypothesis saturable binding of TGF-beta1 and TGF-beta2 to collagen-bound native decorin could be demonstrated. The bound cytokine could be released in a biologically active form by collagenase treatment. Thus, decorin may play a biological role in storing this cytokine temporarily in the extracellular matrix and in thereby modulating an interaction of TGF-beta with its signaling receptors., (Copyright 1998 Academic Press.)
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- 1998
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17. Receptor-mediated endocytosis of decorin: involvement of leucine-rich repeat structures.
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Hausser H, Schönherr E, Müller M, Liszio C, Bin Z, Fisher LW, and Kresse H
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- Binding, Competitive, Cell Line, Cells, Cultured, Decorin, Extracellular Matrix Proteins, Fibroblasts cytology, Fibroblasts metabolism, Humans, Kidney, Kinetics, Peptide Fragments pharmacology, Proteoglycans chemistry, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Recombinant Proteins pharmacology, Sequence Deletion, Skin cytology, Transfection, Endocytosis drug effects, Leucine, Proteoglycans metabolism, Proteoglycans pharmacology, Receptors, Growth Factor metabolism, Skin metabolism
- Abstract
Decorin, a small dermatan sulfate proteoglycan, is characterized by a core protein with central leucine-rich repeat structures and a single glycosaminoglycan chain. It is catabolized by receptor-mediated uptake and subsequent intralysosomal degradation. In the present study, the localization of the receptor binding site(s) along the core protein was investigated. Various recombinant decorin fragments were consistently able to inhibit the endocytosis of wild-type decorin. The most potent inhibitory peptides were those which encompassed the central Leu125-Val230 region, i.e., the fifth to eighth leucine-rich repeat, or at least a part of it. The peptide Leu125-Val230 bound directly to the 51-kDa endocytosis receptor, and Fab fragments of antibodies against this peptide inhibited the endocytosis of decorin in a dose-dependent manner. Decorin constructs expressed in human 293 cells and comprising the full-length coding region or lacking sequences N- and/or C-terminally of the Leu125-Val230 region were all endocytosed with similar clearance rates. These data suggest that the N- and C-terminal domains of the core protein are not required for endocytosis. The receptor binding site is rather represented by contiguous leucine-rich repeat structures of the central part of the core protein. This conclusion is supported by competition experiments with biglycan, a structurally related small proteoglycan.
- Published
- 1998
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18. Isolation and cellular localization of the decorin endocytosis receptor.
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Hausser H, Wedekind P, Sperber T, Peters R, Hasilik A, and Kresse H
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- Animals, Cell Fractionation, Cell Membrane chemistry, Cells, Cultured, Chromatography, Affinity, Decorin, Electrophoresis, Polyacrylamide Gel, Extracellular Matrix Proteins, Fluorescent Antibody Technique, Humans, Rats, Receptors, Growth Factor analysis, Receptors, Growth Factor immunology, Receptors, Growth Factor isolation & purification, Endocytosis, Proteoglycans metabolism, Receptors, Growth Factor metabolism
- Abstract
The small dermatan sulfate proteoglycans decorin and biglycan are efficiently internalized by a variety of cells of mesenchymal origin. This process is modulated, at least under tissue culture conditions, by cell surface-associated heparan sulfate proteoglycans. Receptor proteins of 51 and 26 kDa, respectively, bind to leucine-rich repeat structures of the core proteins of the small proteoglycans but also to highly sulfated domains of heparan sulfate. The 51 kDa protein was purified from rat brain tissue by subcellular fractionation, heparin affinity chromatography and subsequent SDS-PAGE, and was used for raising a polyclonal antiserum. Affinity-purified antibodies also recognize the 26 kDa protein and a few other low molecular weight proteins, suggesting that these proteins represent proteolytic degradation products of the 51 kDa receptor. By confocal laser microscopy, it could be demonstrated that the affinity-purified antibody reacted at 0 degree C with a protein that became internalized and was transported to a perinuclear compartment during 15 min of incubation at 37 degrees C. These findings provide direct evidence that the receptor protein(s) are internalized together with the ligand and reach an endosomal compartment where further sorting can occur.
- Published
- 1996
19. Altered immunohistochemical expression of small proteoglycans in the tumor tissue and stroma of basal cell carcinoma.
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Hunzelmann N, Schönherr E, Bonnekoh B, Hartmann C, Kresse H, and Krieg T
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- Animals, Biglycan, Decorin, Extracellular Matrix Proteins, Humans, Immunohistochemistry, Proteoglycans genetics, RNA, Messenger analysis, Rabbits, Carcinoma, Basal Cell chemistry, Proteoglycans analysis, Skin chemistry
- Abstract
Small proteoglycans have been shown to act as receptors for matrix molecules or growth factors and to influence the attachment and the migration of cells. We therefore report here on the immunocytochemical expression of three small proteoglycans, i.e., decorin, biglycan, and the recently described PG-100, in normal human skin and in basal cell carcinoma. In normal human skin, staining for decorin revealed expression throughout the dermis with an increased signal in the papillary dermis, whereas no expression was observed in the epidermis. Biglycan and PG-100 were mainly detected in the epidermis, with biglycan being expressed only in suprabasal layers. In addition, biglycan could be detected in a narrow zone below the basement membrane. In tissue specimens obtained from 12 basal cell carcinomas, the expression of biglycan and PG-100 was absent or strongly down-regulated in the tumor tissue. Tumor cells thus displayed a staining pattern similar to that found on the basal cells of normal human skin. In the stroma surrounding the tumor, however, the expression of biglycan and to a lesser degree decorin was increased when compared with normal human dermis. The increased deposition appears to be due to an increased synthesis of these molecules, as total RNA extracted from basal cell carcinoma tissue revealed an induction of biglycan and decorin mRNA. This study indicates that the expression of proteoglycans in basal cell carcinoma tumor cells and in tumor stroma is altered from that in normal skin.
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- 1995
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20. Endocytosis of decorin by bovine aortic endothelial cells. off.
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Götte M, Kresse H, and Hausser H
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- Animals, Aorta cytology, Cattle, Cell Polarity, Cells, Cultured, Decorin, Endothelium, Vascular cytology, Extracellular Matrix Proteins, Fluorescent Antibody Technique, Heparan Sulfate Proteoglycans, Heparitin Sulfate analysis, Heparitin Sulfate isolation & purification, Proteoglycans analysis, Proteoglycans isolation & purification, Receptors, Growth Factor isolation & purification, Endocytosis, Endothelium, Vascular metabolism, Proteoglycans metabolism
- Abstract
The small dermatan sulfate proteoglycan decorin is efficiently internalized by a variety of cells of mesenchymal origin. Decorin-binding receptor proteins of 51 and 26 kDa are involved in this process. Uptake is modulated by highly sulfated heparan sulfate which interacts with the receptor proteins, too. Compared with cultured skin fibroblasts, bovine aortic endothelial cells have a lower capacity for decorin endocytosis whereas their apparent concentration of receptor proteins is even higher. The low internalization rate is attributed to the greater occupancy of receptor proteins by heparan sulfate of the plasma membrane and/or the extracellular matrix. Growth of endothelial cells on Falcon 3090 tissue culture inserts made possible to study decorin uptake from the apical and basolateral membrane, respectively. Decorin uptake was at the limit of detection when the proteoglycan was added to the basolateral compartment. Uptake via the apical membrane was at least as efficient as in monolayer cultures on plastic. The basolateral membrane, however, was enriched in receptor proteins, but also in heparan sulfate proteoglycans. It is, therefore, suggested that endothelial cells are especially involved in the clearance of decorin which is present in blood plasma.
- Published
- 1995
21. Colocalization of a large heterodimeric proteoglycan with basement membrane proteins in cultured cells.
- Author
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Faber V, Quentin-Hoffmann E, Breuer B, Schittny J, Völker W, and Kresse H
- Subjects
- Cells, Cultured chemistry, Collagen chemistry, Endothelium, Vascular chemistry, Fibronectins chemistry, Heparitin Sulfate chemistry, Humans, Immunohistochemistry, Laminin chemistry, Proteoglycans chemistry, Basement Membrane chemistry, Cornea chemistry, Fibroblasts chemistry, Heparan Sulfate Proteoglycans, Proteoglycans analysis
- Abstract
A novel large heterodimeric dermatan sulfate proteoglycan with core proteins of 460 and 300 kDa, respectively, had been described as a secretory product of human fetal skin fibroblasts (Breuer et al., J. Biol. Chem. 266, 13224-13232 (1991)). Pulse-chase experiments showed a preferential association of the proteoglycan with the cell membrane. Immunogold labeling indicated its localization in fibrils on the cell surface as well as in fibrillar extensions from the cell body. Immunofluorescence studies yielded a fibrillar and punctate staining pattern which was also seen in cultured human and porcine endothelial cells. Dot-like structures were observed in transformed human keratinocytes. Various immunocytochemical double-labeling experiments indicated a remarkable colocalization of the proteoglycan with fibronectin, laminin, perlecan, and type IV collagen whereas only occasionally a colocalization with chondroitin-6-sulfate was found. No evidence for an enrichment of the proteoglycan in vinculin-containing structures was obtained. These results suggest that the proteoglycan is a widely distributed macromolecule which can associate with basement membrane components. Preliminary findings in rat cornea supported this conclusion.
- Published
- 1992
22. Interactions between thrombospondin and the small proteoglycan decorin: interference with cell attachment.
- Author
-
Winnemöller M, Schön P, Vischer P, and Kresse H
- Subjects
- Binding Sites, Cell Adhesion drug effects, Chondroitin Lyases, Decorin, Dose-Response Relationship, Drug, Extracellular Matrix Proteins, Heparin metabolism, Humans, Proteoglycans pharmacology, Thrombospondins, Blood Platelets chemistry, Platelet Membrane Glycoproteins metabolism, Proteoglycans metabolism
- Abstract
Decorin, a ubiquitous small interstitial dermatan sulfate proteoglycan, interacts with several extracellular matrix components, e.g., with type I collagen and fibronectin. Using a solid phase assay it is shown that the intact proteoglycan as well as its glycosaminoglycan-free core protein exhibits with KD values of about 5 nM and 2 nM, respectively, high affinity binding also to thrombospondin. However, the polysaccharide chain was required for an interaction with Sepharose-bound thrombospondin and served itself as ligand. In light of the results of binding studies with an N-terminal heparin-binding fragment of thrombospondin it is concluded that several structural features of thrombospondin and of decorin contribute to the mutual interaction of the two macromolecules. Thrombospondin substrata allowed attachment but prevented spreading of human skin fibroblasts. The addition of decorin or of its glycosaminoglycan-free core protein led to a considerable delay of cell attachment on a thrombospondin substrate. The strength of cell attachment appeared to be reduced. These data support the antiadhesive role of decorin regardless of whether subsequent cell spreading is supported or not.
- Published
- 1992
23. Influence of decorin on fibroblast adhesion to fibronectin.
- Author
-
Winnemöller M, Schmidt G, and Kresse H
- Subjects
- Cells, Cultured, Decorin, Extracellular Matrix Proteins, Humans, Kinetics, Receptors, Fibronectin, Receptors, Immunologic metabolism, Cell Adhesion, Fibroblasts metabolism, Fibronectins metabolism, Proteoglycans metabolism
- Abstract
Decorin is a ubiquitous small dermatan sulfate proteoglycan carrying a single glycosaminoglycan chain. It is known for its ability to bind, via its core protein, to interstitial collagens. Decorin was purified from the secretions of cultured human skin fibroblasts under non-denaturing conditions. The intact proteoglycan and its glycosaminoglycan-free core protein were tested for their interference with fibroblast adhesion to a fibronectin substrate. Concentrations of 40 nmoles or more of hexuronic acid/ml of decorin or equivalent amounts of core protein inhibited cell adhesion. Inhibition was caused by an interaction of core protein with fibronectin and not by masking of the fibronectin receptor. When cell-binding fragments of fibronectin were used as substrates, a similar inhibition of cell adhesion by decorin core protein was found, and in vitro assays demonstrated an interaction of core protein with the cell-binding domain of fibronectin. Decorin core protein also inhibited the low degree of cell adhesion to heparin-binding fragments on the N-terminus and near the C-terminus of the fibronectin molecules.
- Published
- 1991
24. Tay-Sachs disease: one-step assay of beta-N-acetylhexosaminidase in serum with a sulphated chromogenic substrate.
- Author
-
Fuchs W, Navon R, Kaback MM, and Kresse H
- Subjects
- Acetylglucosamine analogs & derivatives, Acetylglucosamine metabolism, Adolescent, Adult, Aged, Child, Chromogenic Compounds metabolism, Heterozygote, Hot Temperature, Humans, Hydrogen-Ion Concentration, Middle Aged, beta-N-Acetylhexosaminidases, Hexosaminidases blood, Isoenzymes blood, Tay-Sachs Disease blood
- Abstract
A sulphated chromogenic compound, p-nitrophenyl-6-sulpho-2-acetamido-2-deoxy-beta-D-glucopyranoside, which can be hydrolysed enzymatically to p-nitrophenol and the sulphated amino sugar, was used as a substrate for the determination of activity of beta-N-acetylhexosaminidase isoenzymes in human serum. The sera of six Tay-Sachs patients lacking isoenzyme A and heat-inactivated control serum exhibited 6% of the mean normal enzyme activity of 1.32 U/l (1-s range = 1.07-1.57 U/l). In 10 obligate carriers of the Tay-Sachs gene the enzyme activity was 52% (1-s range = 45-60%) of the mean normal value. Therefore, by using the sulphated chromogenic substrate Tay-Sachs disease can be diagnosed enzymatically in a simple one-step procedure, but the 2-s activity ranges of heterozygotes and normals overlap. The assay is not absolutely specific for isoenzyme A of beta-N-acetylhexosaminidase, because the substrate can be hydrolysed to a certain extent by beta-N-acetylhexosaminidase I.
- Published
- 1983
- Full Text
- View/download PDF
25. A sensitive procedure for the diagnosis of N-acetyl-galactosamine-6-sulfate sulfatase deficiency in classical Morquio's disease.
- Author
-
Glössl J and Kresse H
- Subjects
- Amniotic Fluid cytology, Amniotic Fluid enzymology, Cell Line, Child, Preschool, Chondroitin Sulfates, Chondroitinsulfatases metabolism, Chromatography, Ion Exchange, Fibroblasts enzymology, Genotype, Humans, Leukocytes enzymology, Male, Mucopolysaccharidosis IV enzymology, Chondroitinases and Chondroitin Lyases deficiency, Chondroitinsulfatases deficiency, Clinical Enzyme Tests methods, Mucopolysaccharidosis IV diagnosis
- Abstract
The trisaccharide 6-sulfo-N-acetylgalactosamine-glucuronic acid-6-sulfo-N-acetyl-[1-3H]galactosaminitol was used as a substrate for the determination of N-acetylgalactosamine-6-sulfate sulfatase activity. The amount of liberated sulfate was measured indirectly by separating monosulfated reaction products from the substrate on Dowex 1 X 2 microcolumns in a simple two step procedure. Fibroblast homogenates from patients with various genotypes, except classical Morquio's disease, released 410 +/- 90 pmol sulfate/h/mg cell protein. The enzyme exhibited a pH optimum of pH 4.8 and a KM of about 1 X 10(-4) mol/1. It was strongly inhibited by phosphate, sulfate and chloride ions. In three cell lines from patients with classical Morquio's disease a residual activity between 1 and 2% of the mean normal activity was found. All cell lines tested released sulfate from 6-sulfo-N-acetylglucosamine-glucuronic acid-[1-3H]-anhydromannitol. Cell extracts from cultured amniotic fluid cells exhibited a N-acetylgalactosamine-6-sulfate sulfatase activity between 120 and 320 pmol/h/mg protein. An enzyme activity of 370 +/- 100 pmol sulfate/h/mg protein was found in peripheral leucocytes from healthy donors. The determination of N-acetyl-galactosamine-6-sulfate sulfatase activity in one family with an affected patient indicated that the enzyme deficiency is also expressed in leucocytes.
- Published
- 1978
- Full Text
- View/download PDF
26. Thiosulfate-mediated increase of arylsulfatase activities in multiple sulfatase deficiency disorder fibroblasts.
- Author
-
Kresse H and Holtfrerich D
- Subjects
- Biological Transport, Cell Line, Enzyme Activation, Fibroblasts enzymology, Humans, Kinetics, Skin enzymology, Sulfoglycosphingolipids metabolism, Arylsulfatases metabolism, Sulfatases deficiency, Sulfatases metabolism, Thiosulfates pharmacology
- Published
- 1980
- Full Text
- View/download PDF
27. Evidence for degradation of heparan sulfate by endoglycosidases: glucosamine and hexuronic acid are reducing terminals of intracellular heparan sulfate from human skin fibroblasts.
- Author
-
Klein U, Kresse H, and von Figura K
- Subjects
- Animals, Aorta, Cattle, Cells, Cultured, Fibroblasts enzymology, Glucosamine analysis, Humans, Mucopolysaccharidosis I metabolism, Mucopolysaccharidosis III metabolism, Oligosaccharides analysis, Uronic Acids analysis, Glycosaminoglycans metabolism, Glycoside Hydrolases metabolism, Heparitin Sulfate metabolism, Skin enzymology
- Published
- 1976
- Full Text
- View/download PDF
28. Cell-free translation of mRNA encoding an arterial smooth muscle cell proteoglycan core protein.
- Author
-
Sandell LJ, Sawhney RS, Yeo TK, Poole AR, Rosenberg LC, Kresse H, and Wight TN
- Subjects
- Aggrecans, Animals, Cartilage analysis, Cartilage cytology, Cattle, Glycoproteins analysis, Haplorhini, Lectins, C-Type, Muscle, Smooth, Vascular analysis, Extracellular Matrix Proteins, Glycoproteins genetics, Muscle, Smooth, Vascular cytology, Protein Biosynthesis, Proteoglycans, RNA, Messenger genetics
- Abstract
The size and immunological reactivity of the primary gene products of a small non-aggregating dermatan sulfate proteoglycan from bovine and monkey arterial smooth muscle cells were examined after cell-free translation of mRNA. Antisera against the dermatan sulfate proteoglycans from bovine articular cartilage, DSPG II [Rosenberg et al. J. Biol. Chem. 260, 6304 (1985)] and human skin fibroblasts [Glossl et al. J. Biol. Chem. 259, 14144 (1984)] were used to show that the unmodified smooth muscle precursor core protein was immunologically related to both the cartilage and fibroblast core proteins. The size of the precursor core proteins within each species was identical regardless of the tissue source. Comparison of the precursor core proteins synthesized by primate and bovine cells revealed that the bovine core proteins were approximately 1500 Da larger than the primate core proteins as determined by sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis. A similar size difference was observed when the mature core proteins of monkey smooth muscle cells and bovine articular chondrocytes were compared after removal of the glycosaminoglycan chains. These results indicate that arterial smooth muscle cells synthesize a dermatan sulfate proteoglycan whose core protein is similar to, if not the same as, the cartilage and fibroblast dermatan sulfate proteoglycan core proteins. These core proteins may be encoded by the same gene that has diverged in size during speciation.
- Published
- 1988
29. A circadian susceptibility/resistance rhythm for potassium cyanide in male BALB/cCr mice.
- Author
-
Bafitis H, Smolensky MH, Hsi BP, Mahoney S, Schectman T, Kresse H, Powel S, and Dutton L
- Subjects
- Animals, Drug Resistance, Male, Mice, Mice, Inbred BALB C, Time Factors, Circadian Rhythm, Cyanides toxicity, Potassium Cyanide toxicity
- Abstract
Circadian rhythms in mortality and/or survival time following a single intraperitoneal injection of a LD50 of potassium cyanide were studied. In two investigations, different but comparable subgroups of inbred male BALB/cCr mice were treated at 4-h intervals (under conditions standardized for chronobiologic study) during 24-h spans. Mice were observed for exact time-to-death during the first hour after treatment as well as overall mortality during the entire 24-h post-injection span following each KCN treatment timepoint. In both studies, mortality from KCN exhibited a 24-h rhythm. Highest mortality occurred in mice injected at 1600 (80% mortality) in Experiment 1 and 2000 (100% mortality) in Experiment II. Lowest mortality occurred at 0400 (40% mortality) in Experiment I and 0800 (30% mortality) in Experiment II. The need to consider the circadian organization of physiologic function when bioassaying toxicity is discussed.
- Published
- 1978
- Full Text
- View/download PDF
30. Sanfilippo's disease type A: sulfamidase activity in peripheral leukocytes of normal, heterozygous and homozygous individuals.
- Author
-
Schmidt R, Von Figura K, Paschke E, and Kresse H
- Subjects
- Adolescent, Child, Female, Granulocytes enzymology, Humans, Lymphocytes enzymology, Male, Methods, Mucopolysaccharidosis III genetics, Pedigree, Time Factors, Leukocytes enzymology, Mucopolysaccharidoses enzymology, Mucopolysaccharidosis III enzymology, Sulfatases blood
- Published
- 1977
- Full Text
- View/download PDF
31. Deposition and ultrastructural organization of collagen and proteoglycans in the extracellular matrix of gel-cultured fibroblasts.
- Author
-
Schlumberger W, Thie M, Rauterberg J, Kresse H, and Robenek H
- Subjects
- Alginates, Cells, Cultured, Collagen biosynthesis, Extracellular Matrix analysis, Extracellular Matrix metabolism, Fibroblasts, Gels, Humans, Immunohistochemistry, Microscopy, Electron, Proteoglycans biosynthesis, Proteoglycans ultrastructure, Collagen ultrastructure, Extracellular Matrix ultrastructure, Proteoglycans analysis
- Abstract
Human skin fibroblasts were cultivated within the three-dimensional space of polymerized alginate and collagen, respectively. The in vitro synthesis of collagens and proteoglycans was measured during the first 3 days of culture, and the deposition as well as the ultrastructural organization of newly synthesized extracellular matrix components were examined by electron microscopy. The amount of collagens and proteoglycans synthesized by fibroblasts, embedded in calcium alginate gels as well as in collagen lattices, was lowered as compared to monolayer cultures. Furthermore, it was found that collagen synthesis was reduced to a greater extent in alginate gels than in collagen lattices. On the contrary, total proteoglycan biosynthesis was similarly reduced either in alginate gels or in collagen lattices. At the end of a 3-day-culture period, filamentous material as well as cross-striated banded structures were found extracellularly in the alginate gel. According to their periodicity, their banding pattern, their association with polyanionic matrix components and their sensitivity towards glycosaminoglycan-degrading enzymes we could distinguish (1) sheets of amorphous non-banded material consisting of irregularly arranged filaments and containing dermatan sulfate-rich proteoglycans (type I structures), (2) sheets of long-spacing fibrils consisting of parallel orientated filaments and containing chondroitin sulfate-rich proteoglycans (= zebra bodies; type II structures), and (3) fibrillar structures with a complex banding pattern different from that of native collagen fibrils (type III structures). In fibroblasts cultured in collagen lattices, we only sporadically found depositions which are identified as type I structures. Using indirect immunoelectron microscopy and monospecific polyclonal antibodies, we localized type VI collagen in type I structures and type II structures. Type III structures can be identified as type I collagen derived as becomes obvious by comparison with segment long spacing crystallites of type I collagen.
- Published
- 1989
32. Dyggve-Melchior-Clausen syndrome: normal degradation of proteodermatan sulfate, proteokeratan sulfate and heparan sulfate.
- Author
-
Beck M, Lücke R, and Kresse H
- Subjects
- Cells, Cultured, Child, Chondroitin Lyases metabolism, Dermatan Sulfate metabolism, Electrophoresis, Polyacrylamide Gel, Endocytosis, Fibroblasts metabolism, Humans, Leucine metabolism, Lumican, Male, Molecular Weight, Skin metabolism, Carbohydrate Metabolism, Inborn Errors metabolism, Chondroitin analogs & derivatives, Chondroitin Sulfate Proteoglycans metabolism, Dermatan Sulfate analogs & derivatives, Glycosaminoglycans metabolism, Heparitin Sulfate metabolism, Keratan Sulfate metabolism, Proteoglycans metabolism
- Abstract
It had been suggested that Dyggve-Melchior-Clausen syndrome may be due to the deficiency of a specific sulfatase and/or a protease involved in proteoglycan degradation. The ability of Dyggve-Melchior-Clausen fibroblasts to endocytose and degrade 3H-leucine- and 35S-sulfate-labelled proteodermatan sulfate and 35S-sulfate-labelled proteokeratan sulfate, respectively, was therefore investigated. The turnover of cell-associated 35S-sulfate-labelled heparan sulfate was also followed. In all these experiments Dyggve-Melchior-Clausen fibroblasts behaved normally.
- Published
- 1984
- Full Text
- View/download PDF
33. Uptake of hyaluronate by cultured cells.
- Author
-
Truppe W, Basner R, von Figura K, and Kresse H
- Subjects
- Endocytosis, Fibroblasts metabolism, Humans, Hyaluronic Acid analogs & derivatives, Kinetics, Liver metabolism, Muscle, Smooth metabolism, Oligosaccharides metabolism, Receptors, Drug metabolism, Structure-Activity Relationship, Synovial Fluid cytology, Cells, Cultured metabolism, Hyaluronic Acid metabolism
- Published
- 1977
- Full Text
- View/download PDF
34. Morquio disease, type B: activation of GM1-beta-galactosidase by GM1-activator protein.
- Author
-
Paschke E and Kresse H
- Subjects
- Cells, Cultured, Enzyme Activation, Fibroblasts enzymology, Humans, Kinetics, Saposins, Sphingolipid Activator Proteins, Galactosidases metabolism, Galactosylceramidase, Glycoproteins, Mucopolysaccharidosis IV enzymology, Proteins physiology, Skin enzymology
- Published
- 1982
- Full Text
- View/download PDF
35. [Use of ultrasonic diagnosis. I. Principles of ultrasonic diagnosis].
- Author
-
Kresse H
- Subjects
- Absorption, Humans, Methods, Ultrasonography
- Published
- 1973
36. The sanfilippo B corrective factor: a N-acetyl-alpha-D-glucosamindiase.
- Author
-
von Figura K and Kresse H
- Subjects
- Ammonium Sulfate, Cell Line, Chemical Precipitation, Chromatography, Gel, Chromatography, Ion Exchange, Electrophoresis, Fibroblasts enzymology, Hexosaminidases isolation & purification, Humans, Skin cytology, Skin enzymology, Urine enzymology, Carbohydrate Metabolism, Inborn Errors enzymology, Glycosaminoglycans metabolism, Glycoside Hydrolases, Intellectual Disability enzymology
- Published
- 1972
- Full Text
- View/download PDF
37. Mucopolysaccharidosis 3 A (Sanfilippo A disease): deficiency of a heparin sulfamidase in skin fibroblasts and leucocytes.
- Author
-
Kresse H
- Subjects
- Animals, Aorta metabolism, Cattle, Fibroblasts enzymology, Heparin, Humans, Hydrogen-Ion Concentration, Hydrolases, In Vitro Techniques, Sulfatases metabolism, Sulfates metabolism, Sulfur Radioisotopes, Acetylesterase metabolism, Carbohydrate Metabolism, Inborn Errors enzymology, Intellectual Disability enzymology, Leukocytes enzymology, Mucopolysaccharidoses metabolism, Skin enzymology
- Published
- 1973
- Full Text
- View/download PDF
38. Biochemical heterogeneity of the Sanfilippo syndrome: preliminary characterization of two deficient factors.
- Author
-
Kresse H, Wiesmann U, Cantz M, Hall CW, and Neufeld EF
- Subjects
- Electrophoresis, Fibroblasts metabolism, Genotype, Humans, Hydrogen-Ion Concentration, Molecular Weight, Proteinuria, Skin cytology, Sulfur Isotopes, Carbohydrate Metabolism, Inborn Errors metabolism, Glycosaminoglycans metabolism, Intellectual Disability metabolism, Proteins isolation & purification
- Published
- 1971
- Full Text
- View/download PDF
39. [Use of ultrasonic diagnosis. II. Diagnostic methods and their technical realization].
- Author
-
Kresse H
- Subjects
- Humans, Methods, Time Factors, Ultrasonics instrumentation, Ultrasonography
- Published
- 1973
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