Your search keyword '"Microbial Collagenase pharmacology"' showing total 719 results

151. [Dental homotransplants].

Author

Spirescu I and Spirescu G

Subjects

Animals, Anti-Bacterial Agents pharmacology, Fluorides pharmacology, Graft Rejection drug effects, Graft Rejection radiation effects, Haplorhini, Histocompatibility Testing, Hyaluronoglucosaminidase pharmacology, Immunosuppressive Agents pharmacology, Microbial Collagenase pharmacology, Postoperative Complications, Pronase pharmacology, Rabbits, Root Resorption, Transplantation, Autologous, Transplantation, Homologous, Tooth transplantation, Transplantation Immunology

Published

1974

152. Biosynthesis and release of glycoproteins by human skin fibroblasts in culture.

Author

Sear CH, Grant ME, and Jackson DS

Subjects

Ascorbic Acid pharmacology, Cells, Cultured, Cysteine metabolism, Fibroblasts metabolism, Fucose metabolism, Humans, Macromolecular Substances, Microbial Collagenase pharmacology, Molecular Weight, Glycoproteins biosynthesis, Skin metabolism

Abstract

1. Confluent human skin fibroblasts maintained in a chemically defined medium incorporate l-[1-(3)H]fucose in a linear manner with time into non-diffusible macromolecules for up to 48h. Chromatographic analysis demonstrated that virtually all the macromolecule-associated (3)H was present as [(3)H]fucose. 2. Equilibrium CsCl-density-gradient centrifugation established that [(3)H]fucose-labelled macromolecules released into the medium were predominantly glycoproteins. Confirmation of this finding was provided by molecular-size analyses of the [(3)H]fucose-labelled material before and after trypsin digestion. 3. The [(3)H]fucose-labelled glycoproteins released into fibroblast culture medium were analysed by gel-filtration chromatography and sodium dodecyl sulphate/polyacrylamide-gel electrophoresis. These techniques demonstrated that the major fucosylated glycoprotein had an apparent mol.wt. of 230000-250000; several minor labelled species were also detected. 4. Dual-labelling experiments with [(3)H]fucose and (14)C-labelled amino acids indicated that the major fucosylated glycoprotein was synthesized de novo by cultured fibroblasts. The non-collagenous nature of this glycoprotein was established by three independent methods. 5. Gel-filtration analysis before and after reduction with dithiothreitol showed that the major glycoprotein occurs as a disulphide-bonded dimer when analysed under denaturing conditions. Further experiments demonstrated that this glycoprotein was the predominant labelled species released into the medium when fibroblasts were incubated with [(35)S]cysteine. 6. The relationship between the major fucosylated glycoprotein and a glycoprotein, or group of glycoproteins, variously known as fibronectin, LETS protein, cell-surface protein etc., is discussed.

Published

1977

153. Development of osteoarthritic lesions in mice by "metabolic" and "mechanical" alterations in the knee joints.

Author

van der Kraan PM, Vitters EL, van de Putte LB, and van den Berg WB

Subjects

Animals, Biomechanical Phenomena, Glycosaminoglycans antagonists & inhibitors, Glycosaminoglycans biosynthesis, Injections, Intra-Articular, Iodoacetates pharmacology, Iodoacetic Acid, Knee Joint pathology, Knee Joint physiopathology, Mice, Mice, Inbred C57BL, Microbial Collagenase pharmacology, Osteoarthritis chemically induced, Osteoarthritis physiopathology, Papain pharmacology, Time Factors, Knee Joint metabolism, Osteoarthritis pathology

Abstract

Male, 10-week-old C57B1 10 mice received a single intraarticular injection in the knee joints with papain, iodoacetate, or collagenase. This led to osteoarthritic lesions, such as matrix depletion, chondrocyte proliferation, and osteophyte formation, in the injected knee joints within several weeks. After injection of iodoacetate and papain, the main osteoarthritic alterations were localized in the femoropatellar joint, whereas injection of collagenase led to marked osteoarthritic lesions in the femorotibial joint. The mechanism of induction of these alterations appears to differ for iodoacetate and papain on one site and collagenase on the other site. Data are presented that collagenase injection, by way of damaging ligaments and tendons, destabilizes the knee joint eventually leading to osteoarthritic alterations. In contrast, injection of papain or iodoacetate directly interferes with cartilage metabolism resulting in osteoarthritic changes.

Published

1989

154. Colony growth in soft agar of human melanoma, sarcoma, and lung carcinoma cells disaggregated by mechanical and enzymatic methods.

Author

Pavelic ZP, Slocum HK, Rustum YM, Creaven PJ, Karakousis C, and Takita H

Subjects

Agar, Cell Aggregation, Cytological Techniques, Humans, Microbial Collagenase pharmacology, Soft Tissue Neoplasms pathology, Time Factors, Carcinoma pathology, Clone Cells, Lung Neoplasms pathology, Melanoma pathology, Sarcoma pathology

Abstract

The effect of mechanical and enzymatic disaggregation on human malignant melanoma, soft-tissue sarcoma and lung carcinoma colony growth in soft agar was studied. The enzymatic disaggregation was advantageous in most cases of melanoma and sarcoma, giving a larger number of colonies and increasing the probability of achieving growth in soft agar. Enzymatically treated pulmonary carcinoma cell populations had lower clonogeneic potential, especially in the case of anaplastic carcinomas. Morphological studies showed that the cells growing in soft-agar colonies had the same characteristics as those of the original tumor. A linear relationship was obtained between the number of enzymatically and mechanically treated tumor cells plated and the number of colonies. Delayed plating decreased the number of colonies.

Published

1980

155. Collagen prolyl hydroxylase activation in dermal cell primary cultures.

Author

Counts DF and Cutroneo KR

Subjects

Animals, Cells, Cultured, Enzyme Activation, Microbial Collagenase pharmacology, Rats, Skin cytology, Trypsin pharmacology, Endopeptidases pharmacology, Procollagen-Proline Dioxygenase metabolism, Skin enzymology

Published

1980

156. Human colonic intraepithelial and lamina proprial lymphocytes: cytotoxicity in vitro and the potential effects of the isolation method on their functional properties.

Author

Chiba M, Bartnik W, ReMine SG, Thayer WR, and Shorter RG

Subjects

Adolescent, Adult, Aged, Antibody-Dependent Cell Cytotoxicity, Cell Separation, Cytotoxicity Tests, Immunologic, Edetic Acid pharmacology, Female, Humans, Male, Microbial Collagenase pharmacology, Middle Aged, Colon immunology, Intestinal Diseases immunology, Intestinal Mucosa immunology, Lymphocytes immunology

Abstract

Colonic mucosal lymphoid cells, selectively enriched for intraepithelial (IEL) or lamina proprial lymphocytes (LPL), were isolated by sequential EDTA-collagenase treatment of resected human colons. Cytotoxic activities of colonic and peripheral blood lymphoid cells (PBL) were tested in three different assays, using chicken erythrocytes (CRBC) and Chang cells as targets. Antibody-dependent cell-mediated cytotoxicity (ADCC) and PHA-induced cytotoxicity (MICC) for both targets were shown by all the isolates of PBL, as was spontaneous cell-mediated cytotoxicity (SCMC) for Chang cells. However, no SCMC or ADCC for Chang cells was found with LPL, and IEL showed minimal or no activity in either assay. PBL, LPL and IEL demonstrated MICC for Chang cells but, contrasting with PBL and LPL, IEL showed no MCC for CRBC. No significant differences were found between the cytotoxic capabilities of colonic lymphoid cells from patients with inflammatory bowel disease and those from patients with other colonic diseases. Importantly, control studies with PBL showed that SCMC for Chang cells and ADCC for CRBC and Chang cells were reduced by collagenase treatment used in the isolation, of LPL. Also, SCMC for Chang cells was reduced by the treatment of PBL with EDTA. In contrast, neither EDTA nor collagenase reduced MICC for CRBC or Chang cells. Both forms of treatment induced variable degrees of cell losses in the PBL. By analogy, it can be implied that the isolation of intestinal mononuclear cells using EDTA and collagenase may influence some of their cytotoxic activities in vitro. This raises an important caveat in the interpretation of such studies.

Published

1981

157. Cellular reactivity to altered glomerular basement membrane in glomerulonephritis.

Author

Fillit HM, Read SE, Sherman RL, Zabriskie JB, and Van de Rijn I

Subjects

Antigens, Basement Membrane drug effects, Basement Membrane immunology, Cell Membrane immunology, Glycoside Hydrolases pharmacology, Humans, Kidney Glomerulus drug effects, Lymphocyte Activation, Microbial Collagenase pharmacology, Streptococcus immunology, Glomerulonephritis immunology, Kidney Glomerulus immunology

Abstract

Glomerular basement membrane may be altered during glomerulonephritis, exposing antigens that are recognized as foreign. Immunochemical studies suggest that removal of peripheral glycopeptides from the basement membrane with glycosidase mimics this pathogenetic event. To examine these hypotheses, we studied 24 patients with biopsy-proved glomerulonephritis by means of the lymphocyte-blast-transformation assay. Three preparations of normal glomerular basement membrane were used: two mimicked the native state for the peripheral glycopeptides, and one was altered by glycosidases. Results showed minimal differences in responses to native glomerular basement-membrane preparations among patients with glomerulonephritis and control groups. However, patients with glomerulonephritis had a significant blastogenic response to the glycosidase-treated glomerular basement membrane as compared to patients with nonglomerular renal disease and normal controls (P less than 0.0005). These studies suggest that cellular reactivity to altered glomerular basement-membrane antigens can be detected in certain forms of progressive glomerulonephritis.

Published

1978

158. Release of hydroxyproline from rat hearts perfused with collagenase.

Author

Nakatsu K and Warr JH

Subjects

Animals, Calcium pharmacology, Carbon Radioisotopes, Collagen metabolism, Hyaluronoglucosaminidase pharmacology, Hydrolysis, Rats, Trypsin pharmacology, Heart drug effects, Hydroxyproline metabolism, Microbial Collagenase pharmacology, Myocardium metabolism

Published

1975

159. [Erythrocyte changes in dogs after subcutaneous injection of collagenase].

Author

Linke A and Paul I

Subjects

Animals, Dogs, Female, Injections, Subcutaneous, Male, Microbial Collagenase administration & dosage, Microbial Collagenase blood, Erythrocytes drug effects, Microbial Collagenase pharmacology

Published

1974

160. The aggregation of human platelets by ascitic fluid: a possible mechanism for disseminated intravascular coagulation complicating LeVeen shunts.

Author

Salem HH, Koutts J, Handley C, van Der Weyden MB, Dudley FJ, and Firkin BG

Subjects

Adenosine pharmacology, Adult, Aged, Aspirin pharmacology, Disseminated Intravascular Coagulation etiology, Edetic Acid pharmacology, Female, Humans, Hydroxyproline analysis, Male, Microbial Collagenase pharmacology, Middle Aged, Ascitic Fluid analysis, Disseminated Intravascular Coagulation blood, Peritoneovenous Shunt adverse effects, Platelet Aggregation drug effects, Vascular Surgical Procedures adverse effects

Abstract

To identifiy causative factors responsible for the disseminated intravascular coagulation complicating peritoneovenous (LeVeen) shunts, the ascitic fluid from 12 patients with alcoholic liver disease or peritoneal malignancy was examined for its effects on human platelets. In all patients, concentrated ascitic fluid caused irreversible platelet aggregation. Properties of the aggregating factor suggested that it is collagen, and subsequently, the presence of collagen in ascitic fluid was confirmed. This finding, together with the known effects of collagen on platelets and contact clotting factors, would be sufficient to explain the development of disseminated intravascular coagulation following this procedure. Aspirin by inhibiting collagen-induced aggregation may have a therapeutic role in the management of this problem.

Published

1981

161. Collagen synthesis by lathyrogen-treated 3T6 fibroblasts.

Author

Aleo JJ, Novack R, and Levy E

Subjects

Animals, Cattle, Chromatography, Paper, Collagen analysis, Hydroxyproline analysis, In Vitro Techniques, Macromolecular Substances, Microbial Collagenase pharmacology, Proline analysis, Scintillation Counting, Spectrophotometry, Tritium, Aminopropionitrile pharmacology, Collagen biosynthesis, Fibroblasts metabolism

Published

1974

162. Markers to distinguish normal and neoplastic mammary epithelial cells in vitro: comparison of saturation density, morphology and concanavalin A reactivity.

Author

Voyles BA and McGrath CM

Subjects

Animals, Autoradiography, Cell Aggregation drug effects, Cell Line, Cells, Cultured, Female, Hemadsorption drug effects, Hyaluronoglucosaminidase pharmacology, Mice, Mice, Inbred Strains, Microbial Collagenase pharmacology, Trypsin pharmacology, Cell Transformation, Neoplastic, Concanavalin A pharmacology, Epithelial Cells, Epithelium, Mammary Neoplasms, Experimental pathology

Abstract

Normal and premalignant mouse mammary epithelial cells can be prepared in high yields by collagenase dissociation of minced glands followed by a brief, differential centrifugation to remove contaminating fibroblasts and fat cells. The major difficulties in preparing pure cultures in quantity are 1) incomplete dissociation of gland material, and 2) cell death during enzymatic digestion. These problems are eliminated by careful selection of collagenases for dissociation. Normal and premalignant mammary epithelial cells are morphologically indistinguishable from malignant mouse mammary epithelial cells in primary monolayer cultures. In addition, the growth rates and saturation densities achieved by normal mammary epithelial cells are indistinguishable from those of malignant mammary epithelial cells in primary culture. In both cases, a monolayer of cells is preserved with no evidence of focal overgrowth. Malignant adenocarcinoma mammary cells can however be distinguished from normal mammary epithelial cells by virtue of differences in their surface interactions with concanavalin A. A hemadsorption assay using Con-A-coated erythrocytes was the most sensitive indicator for these differences. In hemadsorption assays malignant mammary epithelial cells were half-maximally reactive with 2.5 mug/ml concanavalin A, while normal cells were completely unreactive even at concanavalin A concentrations five-times higher. Premalignant mammary epithelial cells were as reactive as malignant mammary epithelial cells in the hemadsorption assays. Hemadsorption of malignant cells was observed in primary and secondary cultures of epithelium as well as in cell lines. Malignant cells forming mammary adenocarcinomas were as highly reactive as malignant cells forming scirrhous carcinomas. Malignant cells not releasing mammary tumor virus (MuMTV) were as reactive as cells releasing that virus. Adsorption of concanavalin-A-coated erythrocytes to normal mammary epithelial cells could be induced by brief treatment of cell monolayers with hyaluronidase. Exposure of active sites was not affected with either trypsin or collagenase. Our results show that while the growth of malignant cells does not serve to distinguish them from normal cells in monolayer culture, surface changes do exist which can be identified by differences in concanavalin A reactivity. Since the earliest transformants identifiable in vivo (premalignant) have undergone conversion of the surface marker, concanavalin-A-mediated hemadsorption provides a sensitive measure for mammary epithelial cell transformants in vitro.

Published

1976

163. Collagenolytic systems in rheumatoid arthritis.

Author

Harris ED Jr, Faulkner CS 2nd, and Brown FE

Subjects

Adult, Aged, Animals, Arthritis, Rheumatoid blood, Arthritis, Rheumatoid diagnostic imaging, Blood, Cartilage, Articular pathology, Chemical Phenomena, Chemistry, Cytoplasm ultrastructure, Endoplasmic Reticulum ultrastructure, Female, Finger Joint diagnostic imaging, Finger Joint pathology, Finger Joint surgery, Hand diagnostic imaging, Humans, Joint Prosthesis, Leukocyte Count, Male, Microbial Collagenase metabolism, Microbial Collagenase pharmacology, Radiography, Rheumatoid Nodule pathology, Synovial Fluid enzymology, Synovial Membrane enzymology, Temperature, Trypsin pharmacology, Arthritis, Rheumatoid pathology, Collagen metabolism

Abstract

As the proliferative lesion of rheumatoid arthritis becomes polarized and invasion of articular cartilage and subchondral bone begins, it is likely that many mesenchymal cells, including periosteal and perichondral cells, and perhaps even the chondrocytes and osteoblasts themselves can be activated to produce destructive enzymes. Early in the course of RA cartilage proteoglycans are depleted, leaving the remaining collagen more susceptible to mechanical breakdown as well as to enzymatic breakdown. Specific collagenases are released by synovial cells and, in addition, by polymorphonuclear leukocytes. The latter enzyme may account for free collagenase found in synovial fluid, a finding possibly related to saturation of inhibitory proteins by proteases with greater affinity for them, leaving collagenase active. At this time in the course of rheumatoid arthritis, a joint would be under double jeopardy from enzymes released by the invading pannus as well as by collagenase free and active in the synovial fluid. Rapid destruction could occur. Although cartilage collagen has an intrinsic resistance to collagenase conferred by its primary structure and by higher order structure (e.g. intermolecular cross-links), it seems wise to cool down hot joints because increased temperature may increase the rate of collagen degradation and, therefore, cartilage destruction. In addition, superimposed sepsis or acute flares of rheumatoid disease result in enough influx of polymorphonuclear leukocytes into the joints to result in free collagenolytic activity being present. This provides a rationale for frequent aspiration of any joint fluid, septic or otherwise, containing high polymorphonuclear leukocyte counts.

Published

1975

164. [Studies on platelet aggregation induced by human cultured carcinoma cell lines].

Author

Niitsu Y, Mogi Y, Bannai K, Ishii B, Ishigaki S, Kumai R, Koshida Y, Kogawa K, Kohgo Y, and Urushizaki I

Subjects

Arginine analogs & derivatives, Cell Line, Cells, Cultured, Female, Humans, Lung Neoplasms blood, Membrane Proteins pharmacology, Microbial Collagenase pharmacology, Neoplasms pathology, Neoplastic Cells, Circulating, Neuraminidase pharmacology, Pipecolic Acids pharmacology, Stomach Neoplasms blood, Sulfonamides, Trypsin pharmacology, Neoplasms blood, Platelet Aggregation drug effects

Abstract

Attempts were made to clarify the mechanism of platelet aggregation and to characterize the platelet aggregating material employing established human cancer cell lines. Eleven out of the nineteen human cancer cell lines investigated showed platelet aggregating activity. The existence of divalent cation was required for the platelet aggregation induced by HMV-1 tumor cells. The platelet aggregations induced by tumor cells (HMV-1, PC-10, 3LL) were not suppressed by specific thrombin inhibitor (MD-805). The platelet aggregating activities of tumor cells (HMV-1, M 7609) were diminished by treatment with trypsin but not with collagenase or neuraminidase. Aggregating activity was preserved with a preparation of membrane from these tumor cells, although it was abolished by heating(100 degrees C 15 min) or sonication. By SDS PAGE (autoradiography), membrane proteins with MW of 20,000 daltons which specifically bound to platelets were commonly found in cells with platelet aggregating activity (HMV-1, M 7609), but were absent in platelet non-aggregating cells (HGC-25). It is therefore concluded that platelet aggregation induced by human tumor cells does not require the coexistence of thrombin, but is evoked by direct interaction of platelets with aggregating proteins (MW 20,000 daltons) on the cell membrane.

Published

1984

165. Mammalian collagenase predisposes bone surfaces to osteoclastic resorption.

Author

Chambers TJ, Darby JA, and Fuller K

Subjects

Animals, Bone and Bones drug effects, Osteoclasts cytology, Osteoclasts drug effects, Parietal Bone, Rabbits, Rats, Rats, Inbred Strains, Bone Resorption drug effects, Microbial Collagenase pharmacology, Osteoclasts physiology

Abstract

The cell-free endocranial surface of young adult rat parietal bones was used as a substrate for bone cell-derived mammalian collagenase. Incubation of parietal bones in a concentration of enzyme comparable to that secreted by osteoblastic cells in vitro caused destruction of surface osteoid, and resulted in exposure of mineral onto the bone surface. Bones so pre-treated were considerably more susceptible to osteoclastic resorption than bones pre-incubated in the absence of collagenase. These results are consistent with the view that the osteoid layer which covers bone surfaces acts as a barrier to osteoclastic contact with underlying, resorption-stimulating bone mineral; and that cells of the osteoblastic lineage induce osteoclastic resorption through collagenase secretion which, by digestion of the surface osteoid, exposes bone mineral to osteoclastic contact.

Published

1985

166. Aggregation of acetylcholine receptors in nerve-muscle cocultures is decreased by inhibitors of collagen production.

Author

Kalcheim C, Duksin D, and Vogel Z

Subjects

Animals, Autoradiography, Bungarotoxins metabolism, Culture Techniques, Muscles innervation, Rats, Spinal Cord drug effects, Collagen metabolism, Hydroxyproline pharmacology, Microbial Collagenase pharmacology, Neuromuscular Junction drug effects, Receptors, Cholinergic drug effects

Abstract

Coculturing of rat embryonic muscle cells with spinal cord explants resulted in the formation of large numbers of acetylcholine receptor aggregates on the myotube surface, compared to those found on muscle cells grown in the absence of nervous tissue. Remarkably fewer receptor aggregates were formed when, upon addition of nerve explants, these cocultures were treated with either cis-hydroxyproline (a specific inhibitor of collagen production) or collagenase. The possibility is raised that collagen participates in the aggregation of acetylcholine receptors and in synapse formation.

Published

1982

167. Bone cell cultures as an experimental model.

Author

Wong GL

Subjects

Cell Separation, Cells, Cultured, Digestion, Microbial Collagenase pharmacology, Models, Biological, Osteoblasts, Osteoclasts, Phenotype, Bone and Bones cytology

Abstract

The isolation and separation of bone cells with populations enriched for osteoclastic or osteoblastic phenotypes are described. Such systems offer the opportunity to compare and contrast the controls exerted by hormones, ions, and other agents on the functions of the individual bone cell types and may in the future provide explanation for the changes seen in bone tissue in various diseased states.

Published

1980

168. Enzyme release from skeletal muscle.

Author

Suarez-Kurtz G

Subjects

Animals, Anura, Cell Membrane metabolism, Cysteine pharmacology, In Vitro Techniques, Microbial Collagenase pharmacology, Osmotic Fragility, Polyelectrolytes, Polymers metabolism, Saline Solution, Hypertonic, Sarcoplasmic Reticulum enzymology, Creatine Kinase metabolism, L-Lactate Dehydrogenase metabolism, Muscles enzymology, Polyamines

Abstract

Several factors that modify the release of sarcoplasmic enzymes from skeletal muscle, with emphasis on data from isolated frog muscles, are reviewed. The evidence indicates that creatine kinase (CK) and lactate dehydrogenase (LDH) are released continuously from frog muscle fibers that have normal resting potentials and are presumably bound by an intact plasma membrane. The rates of release are determined not only by the transsarcolemmal efflux rates but also by the kinetics of the enzyme diffusion in the extracellular space. The release of CK and LDH is increased by sarcolemmal injury but is also stimulated by procedures that do not cause irreversible damage to membrane integrity as judged from morphological and electrophysiological parameters. Among these procedures are step changes in the tonicity of the bathing medium and brief exposure to nanomolar concentrations of polylysine or polyornithine, which increase the release rates from frog muscles by one order of magnitude. The possible mechanisms responsible for the efflux of sarcoplasmic enzymes and the relevance of these data to the increased enzyme loss from the muscles of patients with neuromuscular diseases are discussed.

Published

1983

169. A method for rapid preparation of single-cell suspensions from rat hepatocyte primary cultures on collagen substratum and the mechanism of cell dissociation.

Author

Miyazaki M, Suzuki Y, and Sato J

Subjects

Animals, Cell Aggregation drug effects, Collagen, Culture Media, Edetic Acid pharmacology, Microbial Collagenase pharmacology, Rats, Trypsin pharmacology, Cell Separation methods, Liver cytology

Abstract

A method has been developed for the rapid preparation of single-cell suspensions from rat hepatocyte primary cultures on collagen substratum. Hepatocytes were adequately dissociated into single cells when the cultures were first treated with a combination of trypsin and ethylenediaminetetraacetic acid (EDTA) and then with collagenase. However, when the order was reversed, hepatocytes were inadequately dispersed. The possible mechanism of cell dissociation is discussed on the basis of the experimental data obtained.

Published

1988

170. Factors affecting the time course of decay of end-plate currents: a possible cooperative action of acetylcholine on receptors at the frog neuromuscular junction.

Author

Magleby KL and Terrar DA

Subjects

Acetylcholine pharmacology, Animals, Binding Sites, Bungarotoxins pharmacology, Carbachol pharmacology, Curare pharmacology, Edrophonium pharmacology, Electrodes, Iontophoresis, Microbial Collagenase pharmacology, Motor Endplate physiology, Neostigmine pharmacology, Peptides pharmacology, Rana pipiens, Snake Venoms pharmacology, Solutions, Time Factors, Acetylcholine physiology, Neuromuscular Junction physiology, Receptors, Drug, Synaptic Transmission drug effects

Abstract

1. End-plate currents have been studied in gylcerol-treated frog sartorius nerve-muscle preparations with the voltage-clamp technique. 2. Adding the anticholinesterase prostigmine (3 muM) to the solution bathing the muscle caused a 2-7 (mean 3-3) times increase in the time constant of decay of end-plate currents. The anticholinesterase edrophonium (15 muM) also prolonged the time course of end-plate currents. 3. Pre-treatment of the preparation with collagenase, which leads to the removal of acetylcholinesterase in the synaptic cleft, prolongs the time course of end-plate currents. 4. Curare (1-2 muM), cobratoxin (0-13 muM), or alpha-bungarotoxin (0-13-0-26 muM) decreased the time constant of decay of end-plate currents in the presence of prostigmine. 5. These observations are consistant with the suggestion that repeated binding of acetylcholine (ACh) molecules to receptors as the ACh escapes from the synaptic cleft can contribute to the prolongation of end-plate currents which occurrs when acetylcholinesterase activity is eliminated. 6. Increasing the amount of transmitter released from the presynaptic nerve terminal leads to a prolongation of end-plate currents in the presence of prostigmine. 7. In the presence of prostigmine, the second of two end-plate currents (interval 2-10 msec) decays more slowly than the first. 8. ACh (1-40 muM) or carbachol (40 muM) applied in the solution bathing the muscle prolongs end-plate currents in the presence of prostigmine. 9. It is suggested on the basis of the observations described in paragraphs 6 to 8 that the time constant of decay of end-plate currents in the presence of prostigmine increases with increasing concentrations of ACh in the synaptic cleft. In the absence of prostigmine, increasing the concentration of ACh in the synaptic cleft did not change the time constant for decay of end-plate currents. 10. We interpret these results to suggest that ACh can have a cooperative action on receptors such that the association of ACh with one receptor (defined as binding a single ACh molecule) favours the binding or retention of ACh at other receptors. This implies that receptors can interact.

Published

1975

171. Bacterial collagenase. Proposed adjunct to vitrectomy with membranectomy.

Author

Moorhead LC, Redburn DA, Kirkpatrick DS, and Kretzer F

Subjects

Animals, Cicatrix therapy, Eye Diseases surgery, Membranes drug effects, Microbial Collagenase pharmacology, Microscopy, Electron, Rabbits, Retina drug effects, Retina ultrastructure, Vitreous Body drug effects, Microbial Collagenase therapeutic use, Retinal Diseases therapy, Vitreous Body surgery

Abstract

Clostridiopeptidase A digested preretinal cicatricial tissue without causing morphological alteration of normal retina during a 30-minute incubation in the rabbit. Light and transmission electron microscopy were used to determine effects on the inner limiting membrane and retinal ganglion and Müller's cells and to evaluate enzyme digestion of preretinal scarring. Removal of the injected collangenase by vitrectomy resulted in normal electroretinograms and retinal morphology 48 hours postoperatively. If the enzyme was left in the eye for 24 hours, lens opacities, partial erosion of the inner limiting membrane, and extensive hemorrhage resulted. The specificity of action of the collagenase is due to the high degree of purity of the enzyme used and a substantial biochemical difference between scar collagen and basement membrane collagen. The injection of purified collagenase capable of digesting vitreal scar tissue while leaving the retina undamaged could represent a new approach to vitrectomy, specifically to facilitate certain cases of membranectomy.

Published

1980

172. Extraction of immune and inflammatory cells from human lung parenchyma: evaluation of an enzymatic digestion procedure.

Author

Holt PG, Robinson BW, Reid M, Kees UR, Warton A, Dawson VH, Rose A, Schon-Hegrad M, and Papadimitriou JM

Subjects

Aged, Animals, Antigens, Surface analysis, Cell Count, Deoxyribonucleases pharmacology, Guinea Pigs, Humans, Killer Cells, Natural immunology, Lung immunology, Lung ultrastructure, Lymphocyte Activation, Mice, Microbial Collagenase pharmacology, Microscopy, Electron, Middle Aged, Rats, T-Lymphocytes immunology, Cytological Techniques, Lung cytology

Abstract

The inflammatory and immune cell populations of the human lung parenchyma have not been characterized in detail. This report describes a novel and efficient procedure for their extraction. Histologically normal human lung tissue samples from pneumonectomy specimens were sliced to 0.5 mm, and digested in collagenase/DNAse. Viable mononuclear cell yields ranged from 15-48 X 10(6)/g, and were markedly in excess of reported methods employing mechanical tissue disruption, which normally yield populations containing almost exclusively macrophages. The lung digest population was examined by flow cytometry using monoclonal antibodies against cell surface receptors, and found to comprise up to 40% T lymphocytes, 10% B lymphocytes and 30% macrophages, contaminated by less than 1% peripheral blood cells. Based upon these figures, the recoverable lung parenchymal lymphoid cell pool appears considerably larger than previously recognized, being of the same order as the peripheral blood pool. Initial functional studies suggest that such cellular activities as antigen-specific T cell proliferation, antigen-presentation, interleukin 1 production and natural killer cell activity survive the extraction process, and controlled enzymatic digestion experiments with peripheral blood cells indicate that the degree of enzyme-mediated damage to these functions and to cell-surface structures, was minimal. The extraction method thus appears suitable for studying the types and functions of human parenchymal lung cells in health and disease.

Published

1986

173. Evidence for reversible morphologic phenotypes (sprouts) of cultured endothelial cells.

Author

Makarski JS Jr

Subjects

1-Methyl-3-isobutylxanthine pharmacology, 8-Bromo Cyclic Adenosine Monophosphate, Animals, Aorta, Thoracic, Cattle, Cell Count, Cell Separation, Cholera Toxin pharmacology, Cyclic AMP analogs & derivatives, Cyclic AMP pharmacology, Microbial Collagenase pharmacology, Pancreatin pharmacology, Trypsin pharmacology, Cells, Cultured cytology, Endothelium cytology

Published

1982

174. [The influence of exposed cementum in various experimental conditions on the periodontal tissue repair (author's transl)].

Author

Ohsugi M

Subjects

Animals, Blood Physiological Phenomena, Calcium Chloride pharmacology, Edetic Acid pharmacology, Lipopolysaccharides pharmacology, Male, Microbial Collagenase pharmacology, Rats, Saliva physiology, Dental Cementum drug effects, Epithelial Attachment drug effects, Periodontal Diseases drug therapy, Periodontium drug effects, Wound Healing drug effects

Published

1979

175. Lectin binding to the developing forms of Onchocerca gutturosa microfilariae.

Author

Nwachukwu MA, Mackenzie CD, Litchfield TM, and Howard G

Subjects

Animals, Cattle, Chitinases pharmacology, Diethylcarbamazine pharmacology, Female, Ivermectin pharmacology, Microbial Collagenase pharmacology, Microfilariae drug effects, Microfilariae metabolism, Onchocerca drug effects, Peptide Hydrolases pharmacology, Skin parasitology, Trypsin pharmacology, Uterus parasitology, Lectins metabolism, Onchocerca metabolism

Abstract

Uterine and skin derived forms of microfilariae (mf) and earlier developing stages of the cattle filarial nematode Onchocerca gutturosa were examined for the lectin binding properties of their external surfaces (ie. egg shell and microfilarial cuticle). Both the uterine and skin derived forms of mf failed to bind any of the lectins tested. Incubation in known microfilaricides did not promote any binding of lectins to these parasites. Peanut agglutinin (PNA) was the only lectin found to bind specifically to earlier developing stages (i.e. the shells of freshly obtained eggs). Diethylcarbamazine (DEC) did not alter the binding pattern from that observed in untreated eggs. Ivermectin eliminated PNA binding but increased Ricinus communis lectin (RCA-1) positivity. Trypsin, collagenase and protease enzymes all affected the binding; chitinase however did not have any effect. These results support the concept that the eggshells of filariae can interact with the host defence responses.

Published

1987

176. Influence of proteolytic enzymes and calcium-binding agents on nuclear and cell surface topography.

Author

Thyberg J and Moskalewski S

Subjects

Animals, Cartilage ultrastructure, Cell Membrane drug effects, Cell Nucleus drug effects, Embryo, Mammalian, Fibroblasts ultrastructure, HeLa Cells ultrastructure, Humans, Mice, Microscopy, Electron, Skin ultrastructure, Calcimycin pharmacology, Cell Membrane ultrastructure, Cell Nucleus ultrastructure, Cysteine Endopeptidases, Egtazic Acid pharmacology, Endopeptidases pharmacology, Ethylene Glycols pharmacology, Microbial Collagenase pharmacology, Trypsin pharmacology

Abstract

Transmission electron microscopy was used to study the effects of proteolytic enzymes (collagenase, trypsin, clostripain), the calcium chelator ethyleneglycol-bis-(beta-aminoethyl ether) N,N,N',N'-tetraacetic acid (EGTA), and the calcium ionophore A 23187 on substrate adhesion and fine structure of chondrocytes and fibroblasts. Monolayer-cultured cells responded to treatment with the proteolytic enzymes followed by EGTA or A 23187 by rounding and detaching from the substrate. This was accompanied by the formation of a microvillous surface, deep nuclear folds, and numerous cytoplasmic vacuoles. Labeling experiments with colloidal thorium dioxide indicated that the vacuoles were formed by endocytosis and fusion of endocytic vesicles with preexisting lysosomes. To a variable extent, similar changes were produced by trypsin or EGTA alone. The cells regained their normal fine structure after withdrawal of the reagents and when seeded onto a substrate. In suspension culture, recovery was incomplete; the cells retained a rounded shape and an increased number of cytoplasmic vacuoles. The results suggest that changes in plasma membrane composition and its permeability to calcium represent the primary signal for cell rounding and detachment. The cellular mechanisms responsible for the associated folding of the nuclear envelope and the cell surface remain unidentified. Nevertheless, this is believed to represent a means of handling of excess membrane during sudden transition from a flattened to a rounded shape. Membrane stored in folds and vacuoles is reutilized when the cells reattach and spread out on a substrate.

Published

1984

177. Effect of the immunological antigenicity of the allogeneic tendons on tendon grafting.

Author

Minami A, Ishii S, Ogino T, Oikawa T, and Kobayashi H

Subjects

Achilles Tendon drug effects, Achilles Tendon immunology, Animals, Complement Fixation Tests, Cytotoxicity Tests, Immunologic, Formaldehyde immunology, Freezing, Glutaral immunology, Lymph Nodes immunology, Microbial Collagenase pharmacology, Mitomycin, Mitomycins immunology, Radiation, Rats, Rats, Inbred Strains, Sarcoma, Experimental immunology, Spleen immunology, Transplantation, Homologous, Trypsin pharmacology, Achilles Tendon transplantation, Graft Rejection, Histocompatibility Antigens immunology

Published

1982

178. Water content of equine articular cartilage: effects of enzymatic degradation and "artificial fibrillation".

Author

Simon WH and Wohl DL

Subjects

Animals, Hexosamines metabolism, Horses, Hyaluronoglucosaminidase pharmacology, Hydroxyproline metabolism, Microbial Collagenase pharmacology, Proteoglycans metabolism, Stress, Mechanical, Body Water metabolism, Cartilage, Articular metabolism

Abstract

A method is described for accurate and reproducible determination of wet and dry weights of small articular cartilage samples. The water content of the articular cartilage samples before and after treatment with selective degradative enzymes and "artificial fibrillation" was determined. It was found that the water content of articular cartilage can be altered by changing the physical and chemical composition of articular cartilage. The combination of protein polysaccharide degradation and "fibrillation" causes an increase in articular cartilage water content, while collagenase and the combination of collagenase and "fibrillation" causes a decrease. The relationship between these findings and function of normal and osteoarthritic cartilage is discussed.

Published

1982

179. Isolation of viable canine intestinal lymphocytes.

Author

Willard MD, Bull RW, and Coffman PJ

Subjects

Animals, Cell Separation methods, Edetic Acid pharmacology, In Vitro Techniques, Male, Microbial Collagenase pharmacology, Mitogens pharmacology, Dogs immunology, Intestinal Mucosa cytology, Jejunum cytology, Lymphocytes drug effects

Abstract

A modification of a previously reported enzymatic technique was used to isolate 60% to 90% pure populations of viable lymphocytes from canine small intestinal mucosa. Mitogenesis assays were then simultaneously performed on these and isolated peripheral blood lymphocytes from the same dogs. A technique to isolate intraepithelial lymphocytes was not successful. Intestinal mucosal lymphocytes were simultaneously purified by 2 different techniques (suspensions B and C), which produced cell populations that responded similarly to phytohemagglutinin (PHA), concanavalin A, and pokeweed mitogens. The peripheral blood lymphocytes demonstrated greater response to PHA and concanavalin A mitogens than did the intestinal mucosal lymphocytes (P less than 0.05). Furthermore, peripheral blood lymphocytes had a significantly higher response to PHA than to pokeweed mitogen (P less than 0.05). The impure preparation of intraepithelial lymphocytes (suspension A) did not show any evidence of reactivity to mitogens. Further studies are needed to determine whether the EDTA or collagenase had any effect upon the intestinal mucosal lymphocyte responsiveness. The present study demonstrated that viable mucosal lymphocytes can be isolated from the canine intestine and that they can maintain their responsiveness to mitogens.

Published

1982

180. Membrane properties of aggregate of collagenase-dissociated rat heart cells.

Author

de Bruijne J and Jongsma HJ

Subjects

Acetylcholine pharmacology, Action Potentials drug effects, Animals, Cell Aggregation, Cell Membrane physiology, Electric Stimulation, Epinephrine pharmacology, Manganese pharmacology, Rats, Tetrodotoxin pharmacology, Microbial Collagenase pharmacology, Myocardium cytology

Abstract

Aggregates of collagenase-dissociated neonatal rat heart cells have been tested for several membrane properties and shown to be comparable with cells from the intact heart. Action potentials, recorded from driven aggregates, are fully suppressed by tetrodotoxin (TTX). Under Mn2+, the plateau phase of the action potential disappears and no more mechanical activity can be detected. In aggregates, therefore, apparently both the fast sodium inward current and a slow inward current, which is at least partly carried by Ca2+ ions, contribute to the action potential. Pacemaker activity in spontaneously active aggregates is enhanced by adrenaline and slowed down by acetylcholine. Adrenaline also increases the plateau phase amplitude of the action potential and thereby the rate of repolarization. Acetylcholine shortens the action potential duration and increases the resting membrane potential. The electrical coupling between the cells in the aggregates is so tight that the aggregate seems to behave passively, like a single cell. It is concluded that aggregates of collagenase-dissociated neonatal rat heart cells may be used to study active electrical properties using the voltage clamp technique.

Published

1980

181. Enzymatic liberation of myogenic cells from adult rat muscle.

Author

Bischoff R

Subjects

Animals, Cell Differentiation, Cells, Cultured, Culture Media, Female, Fibroblasts, Histocytochemistry, Macrophages, Male, Microbial Collagenase pharmacology, Microscopy, Electron, Muscles drug effects, Muscles physiology, Myofibrils, Papain pharmacology, Pronase pharmacology, Rats, Regeneration, Trypsin pharmacology, Muscles cytology, Peptide Hydrolases pharmacology

Published

1974

182. A high yield method for isolating rat islets of Langerhans using differential sensitivity to freezing.

Author

Bank HL

Subjects

Animals, Dimethyl Sulfoxide pharmacology, Freezing, Microbial Collagenase pharmacology, Rats, Cell Separation methods, Islets of Langerhans cytology

Abstract

Conventional methods of isolating islets of Langerhans rely upon the differential sensitivity of the pancreatic acinar tissue vs islets to enzymatic dissociation by crude collagenase, however, the yield of intact islets obtainable with this technique is quite low. Higher yields of islets can be obtained with pharmacological or surgical methods which either destroy acinar cells or cause them to release their zymogen granules. However, because of the requirement to pretreat the donor, these methods cannot be scaled-up for potential clinical use. To overcome the limitations of the conventional isolation procedures, we exploited the differential sensitivity of acinar cells and islet cells to freezing damage. Using this approach we are able to isolate greater than 2500 islets from the pancreas of a single rat. Basically, we rapidly mince pancreatic tissue, subject the tissue to a short collagenase digestion, briefly freeze the tissue at -30 degrees C in the presence of glycerol, and immediately thaw it. Subsequent enzyme treatment digests the residual acinar tissue, collagen, DNA, and proteins. Preliminary results indicate that the islets are morphologically indistinguishable from islets isolated using conventional digestion techniques.

Published

1983

183. Different capacities for amino acid transport in periportal and perivenous hepatocytes isolated by digitonin/collagenase perfusion.

Author

Burger HJ, Gebhardt R, Mayer C, and Mecke D

Subjects

Animals, Biological Transport drug effects, Cells, Cultured, Dexamethasone pharmacology, Digitonin pharmacology, Glucagon pharmacology, Glutamate-Ammonia Ligase metabolism, Immunoenzyme Techniques, In Vitro Techniques, Insulin pharmacology, Liver cytology, Microbial Collagenase pharmacology, Perfusion, Pyruvate Kinase metabolism, Rats, Rats, Inbred Strains, Sodium physiology, Amino Acids metabolism, Liver metabolism

Abstract

Periportal and perivenous hepatocytes were isolated from rat liver by digitonin/collagenase perfusion for investigating the acinar heterogeneity of amino acid transport activities related to glutamine and ammonia metabolism. Immunocytochemical staining of the respective subpopulations for glutamine synthetase demonstrated that periportal subpopulations were essentially free of glutamine synthetase-positive cells, whereas perivenous subpopulations showed a 2- to 3-fold enrichment of glutamine synthetase-positive hepatocytes. The high perivenous/periportal ratio of 59 found for glutamine synthetase activity as well as the perivenous/periportal ratios of other marker enzymes further indicated the good separation of periportal and perivenous cells. alpha-Aminoisobutyric acid, histidine and glutamate were used to determine the distribution pattern of amino acid transport systems A, N and G-, as well as of the sodium-independent uptake of these compounds 1 hr after isolation and after maximal hormonal stimulation during primary culture. The strong heterogeneity of the sodium-independent transport of histidine, characterized by higher perivenous transport rates [perivenous/periportal ratio: 1.5 (1 hr) to 3.5 (48 hr)], suggests a significant role of facilitated diffusion, presumably in glutamine export. Conversely, the strong heterogeneity of the sodium-dependent glutamate transport (System G-) characterized by higher uptake rates in nonstimulated [perivenous/periportal ratio: 6.6 (1 hr)] and in hormonally treated perivenous hepatocytes (perivenous/periportal ratio: 2.2) reflects its possible significance with respect to the substrate availability for glutamine synthesis. The observed heterogeneities provide a basis for understanding how substrate fluxes related to glutamine metabolism might be established and regulated.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1989

184. [Resistance of heart valve bioprosthesis to the proteolytic effect of collagenase and elastase].

Author

Krasovskaia SM, Platonova LV, and Dzemeshkevich SL

Subjects

Collagen metabolism, Elastin metabolism, Humans, Hydrolysis, In Vitro Techniques, Prosthesis Failure, Bioprosthesis, Heart Valve Prosthesis, Microbial Collagenase pharmacology, Pancreatic Elastase pharmacology

Abstract

Proteolytic destruction of pig aortal valves was studied at various steps of their preparation to implantation (native tissue, the tissue treated with terrylytine as well as with terrylytine and glutaric aldehyde) using pig pancreatic elastase and bacterial collagenase. The rate of the tissue destruction was estimated by means of monitoring an increase in content of protein and amino nitrogen in the hydrolysates. The tissue treated with terrylytine and glutaricaldehyde was 10-40-fold more resistant to proteolysis as compared with native heart valve tissue. Inadequate stabilizing effect of glutaric aldehyde on elastin, as compared with that on collagen, was found, when proteolysis of native and modified with glutaric aldehyde elastin from bovine cervical ligament and of calf skin collagen was studied using elastase and collagenase, respectively.

Published

1989

185. The susceptibility of the mesangial matrix of isolated cell-free glomeruli to limited proteolysis.

Author

Krakower CA

Subjects

Animals, In Vitro Techniques, Microbial Collagenase pharmacology, Microscopy, Electron, Papain pharmacology, Pepsin A pharmacology, Pronase pharmacology, Rats, Trypsin pharmacology, Endopeptidases pharmacology, Glomerular Mesangium drug effects

Abstract

Selective lysis of mesangial matrix can be achieved by limited proteolysis of isolated cell-free glomeruli. Such treated glomeruli present unfolded and confluent capillary loops forming irregularly shaped, saccular lobular structures, comparable to those described for chemical mesangiolysis. It was observed that the parietal capsules of the glomeruli were also susceptible to limited proteolysis by comparison with the resistance of the basement membranes of the peripheral capillary loops.

Published

1983

186. Electron microscopical study of non-specific cholinesterase activity in simple lamellar corpuscles of glabrous skin from cat rhinarium: a histochemical evidence for the presence of collagenase-sensitive molecular forms and their secretion.

Author

Dubový P

Subjects

Animals, Cats anatomy & histology, Endoplasmic Reticulum enzymology, Female, Golgi Apparatus enzymology, Histocytochemistry, Male, Mechanoreceptors ultrastructure, Microbial Collagenase pharmacology, Microscopy, Electron, Nose, Skin enzymology, Cats metabolism, Cholinesterases analysis, Mechanoreceptors enzymology

Abstract

The distribution of nCHE activity was studied histochemically in simple lamellar corpuscles (SLCs) of glabrous skin from cat rhinarium. The Schwann cells forming myelin sheaths in preterminal part of SCLs exhibited no positive reaction for nCHE activity. Prevalent reaction product was localized extracellularly in the inne core enveloping terminal portion of unmyelinated sensory axon. A dot-like shaped reaction product was deposited in the basal lamina of the inner core cells and their cytoplasmic lamellae or was scattered in enlarged interlamellar spaces. Only small amount of fine end product was found to be associated with the plasma membrane of inner core lamellae. Fine reaction product for nCHE activity was consistently localized in perinuclear and rER cisternae and saccules of the Golgi apparatus of inner core cells. Some vesicles around rER and the Golgi apparatus, ones beneath the plasma membrane, and tubular-like cisternal profiles oriented towards the surface contained nCHE end product, as well. The intracellular and extracellular localization of nCHE reaction product suggests that this enzyme behaves in cat SLCs as a secreted rather than as an integral membrane protein. A large amount of dot-like reaction product in the interlamellar spaces disappeared if the skin sections were treated with collagenase before incubation in the medium for histochemical detection of nCHE activity. The decrease of nCHE end product in SLCs of the skin sections after collagenase digestion was corroborated by means of light microdensitometer and electrometrical measurement. The histochemical detection and electrometrical measurement revealed that the majority of the reaction product in the interlamellar spaces of inner core corresponds with the nCHE molecules sensitive to collagenase treatment and they are probably counted among asymmetrical molecular forms.

Published

1989

187. Purification and characterization of Leydig cells from rat testes.

Author

Janszen FH, Cooke BA, van Driel MJ, and van der Molen HJ

Subjects

Albumins pharmacology, Animals, Cell Separation methods, Centrifugation, Centrifugation, Density Gradient, Dextrans, Dose-Response Relationship, Drug, Esterases analysis, Ficoll pharmacology, Hydroxysteroid Dehydrogenases analysis, Luteinizing Hormone pharmacology, Male, Microbial Collagenase pharmacology, Osmolar Concentration, Rats, Spermatogenesis radiation effects, Testis drug effects, Testosterone biosynthesis, Leydig Cells analysis, Leydig Cells drug effects, Leydig Cells metabolism, Testis cytology

Abstract

An LH-responsive Leydig cell preparation (containing 6+/-2% Leydig cells) was obtained by collagenase treatment of rat testis. Centrifugation of this cell preparation through a 13% Ficoll solution for 10 min at 1500 g resulted in a four times purification of the Leydig cells, with a concomitant increases in steroidogenic activity. Addition of 0-2% albumin to the 13% Ficoll solution, adjusted to 280 mosmol/l, resulted in a further twofold purification of the Leydig cells paralleled by a twofold increase in steroidogenic activity. Centrifugation of these Ficoll-albumin-purified Leydig cells through a 6% dextran solution for 2 min at 100 g resulted in a further 1-7 times purification of the Leydig cells. A combination of the two centrifugation steps resulted in a 12-5 times purification of Leydig cells compared with the original crude cell suspension, while an increase in steroidogenic activity of 22-5 times was obtained. This final cell preparation contained 59 +/- 17% Leydig cells (mean +/- S.D., n = 6). The recovery of Leydig cells was 29%. Collagenase treatment of testes deficient in spermatogenesis resulted in a cell preparation with the same steroidogenic activity as Ficoll-purified cells from normal testes. Centrifugation of these cells through a 13% Ficoll solution gave only a limited increase in the steroidogenic activity. Isopycnic centrifugation of the crude cell preparation on a discontinous Ficoll metrizoate gradient resulted in two discrete peaks of Leydig cells, one peak at a density of 1-039-1-055 g/ml and one at a density of 1-068-1-088 g/ml. Both types of cells produced testosterone. In the presence of LH, cyclic AMP production in both types of Leydig cells increased, but testosterone production was only increased by LH in the "denser" Leydig cells and not in the "light" Leydig cells. No difference in sensitivity to LH could be observed between the Leydig cell preparations of different purity. Using a 60 min pre-incubation period the highest testosterone response was obtained with 100-1000 ng LH/ml. The same maximum testosterone response was obtained with 10-100 ng LH/ml when the pre-incubation period was omitted.

Published

1976

188. Neurophysiological and biophysical evidence on the mechanism of electric taste.

Author

Herness MS

Subjects

Animals, Electric Stimulation, Electrolytes pharmacology, Ethylmaleimide pharmacology, Iodoacetates pharmacology, Iodoacetic Acid, Iontophoresis, Lingual Nerve physiology, Male, Microbial Collagenase pharmacology, Rats, Rats, Inbred Strains, Reaction Time, Sodium Chloride pharmacology, Stimulation, Chemical, Taste Buds drug effects, Chorda Tympani Nerve physiology, Taste physiology, Taste Buds physiology, Tongue innervation

Abstract

The phenomenon of electric taste was investigated by recording from the chorda tympani nerve of the rat in response to both electrical and chemical stimulations of the tongue with electrolytes in order to gain some insight into its mechanism on both a neurophysiological and biophysical basis. The maximum neural response levels were identical for an individual salt (LiCl, NaCl, KCl, or CaCl2), whether it was presented as a chemical solution or as an anodal stimulus through a subthreshold solution. These observations support the idea that stimulation occurs by iontophoresis of ions to the receptors at these current densities (less than 100 microA/cm2). Electric responses through dilute HCl were smaller than the chemically applied stimulations, but the integrated anodal responses appeared similar to chemical acid responses, as evidenced by an OFF response to both forms of stimuli. Hydrogen may be more permeant to the lingual epithelium and would thus be shunted away from the taste receptors during anodal stimulation. When the anion of electric taste was varied via subthreshold salt solutions, the response magnitude increased as the mobility of the anion decreased. The transport numbers of the salts involved adequately explains these differences. The physical aspects of ion migration occurring within the adapting fluid on the tongue are also discussed. Direct neural stimulation by the current appears to occur only at higher current densities (greater than 300 microA/cm2). If the taste cells of the tongue were inactivated with either iodoacetic acid (IAA) or N-ethyl maleimide (NEM), or removed with collagenase, then responses from the chorda tympani could be obtained only at these higher current densities. Latency measurements before and after IAA or NEM treatment corroborated these findings. The results are discussed in terms of several proposed mechanisms of electric taste and it is concluded that an ion accumulation mechanism can adequately explain the data.

Published

1985

189. Enhancement of glomerular permeability to anionic ferritin induced by kidney perfusion with collagenase.

Author

Schaeverbeke J, Moreau Lalande H, Geloso-Meyer A, Perichon M, Borot-Laloi C, and Cheignon M

Subjects

Animals, Basement Membrane drug effects, Basement Membrane metabolism, Capillaries ultrastructure, Collagen metabolism, Female, Kidney Glomerulus metabolism, Kidney Glomerulus ultrastructure, Microscopy, Electron, Perfusion, Permeability, Rats, Ferritins metabolism, Kidney Glomerulus drug effects, Microbial Collagenase pharmacology

Abstract

The role of collagen in ultrafiltration properties of the glomerular basement membrane (GBM) was tested after a single administration of bacterial collagenase, using native ferritin as a tracer which does not pass through the GBM under physiological conditions. Experiments were performed both in situ and with isolated kidneys. Increased permeability to ferritin occurs 6 hr following enzyme perfusion and becomes patent after 30 hr, numerous tracer molecules appearing in urinary space, without any readily observable changes either in distribution of fixed negative charges (as revealed by colloidal iron and polyethyleneimine) or in structural organization of the glomerulus. Selective permeability of the GBM is progressively restored so that ferritin is almost confined to capillary lumen one month after enzyme injection. We conclude that collagen plays an important part in restricting plasma protein filtration.

Published

1985

190. Interactions between polymerized human albumin, hepatitis B surface antigen, and complement: II. Involvement of Clq in or near the hepatitis B surface antigen receptor for polyalbumin.

Author

Milich DR, Bhatnagar PK, Papas ED, and Vyas GN

Subjects

Blood, Complement Activating Enzymes immunology, Complement C1q, Hot Temperature, Humans, Hydrogen-Ion Concentration, Microbial Collagenase pharmacology, Osmolar Concentration, Serum Albumin, Human, Temperature, Complement Activating Enzymes metabolism, Hepatitis B Surface Antigens, Receptors, Antigen metabolism, Serum Albumin metabolism

Abstract

A species-specific receptor for polymerized human albumin (PHALB) has been reported on hepatitis B surface antigen (HBsAg)-carrying particles. Our previous observations that human Clq also binds PHALB in a species-restricted manner led us to investigate the possibility that HBsAg-associated Clq is involved in the PHALB receptor on HBsAg particles. The temperature, ionic strength, and pH requirements necessary for binding of PHALB to both Clq and HBsAg were compared and found to be similar. Normal human serum and purified Clq inhibited the PHALB-HBsAg interaction; the inhibition was markedly reduced in heat-inactivated and Clq-depleted serum. Heat-denatured or reduced and alkylated Clq failed to inhibit the PHALB-HBsAg binding. Moreover, human Clq was found to be present in purified preparations of HBsAg and the quantity detected paralleled the degree of PHALB-HBsAg binding. While anti-Clq inhibited the PHALB-HBsAg interaction, anti-Clr, - Cls, -C3, and -Ig were not inhibitory. Collagenase treatment of purified HBsAg reduced both PHALB-binding activity and the degree of HBsAg-associated Clq. These observations provide evidence that HBsAg-associated Clq is involved in or near the HBsAg-binding site for PHALB.

Published

1981

191. Collagenase digestion alters the organization and turnover of junctional acetylcholine receptors.

Author

Bloch RJ, Steinbach JH, Merlie JP, and Heinemann S

Subjects

Animals, Diaphragm innervation, Motor Endplate ultrastructure, Osmolar Concentration, Rats, Receptors, Cholinergic drug effects, Histological Techniques, Microbial Collagenase pharmacology, Neuromuscular Junction metabolism, Receptors, Cholinergic metabolism

Abstract

Acetylcholine receptors at the vertebrate neuromuscular junction are highly organized and metabolically very stable. We report here that digestion of adult rat skeletal muscle with collagenase disorganizes junctional receptors and increases their turnover rate.

Published

1986

192. Synthesis of type III collagen by fibroblasts from the embryonic chick cornea.

Author

Conrad GW, Dessau W, and von der Mark K

Subjects

Animals, Cell Separation, Cells, Cultured, Chick Embryo, Collagen analysis, Cornea metabolism, Fibroblasts metabolism, Fluorescent Antibody Technique, Microbial Collagenase pharmacology, Collagen biosynthesis, Cornea cytology

Abstract

Synthesis of collagen types I, II, III, and IV in cells from the embryonic chick cornea was studied using specific antibodies and immunofluorescence. Synthesis of radioactively labeled collagen types I and III was followed by fluorographic detection of cyanogen bromide peptides on polyacrylamide slab gels and by carboxymethylcellulose chromatography followed by disc gel electrophoresis. Type III collagen had been detected previously by indirect immunofluorescence in the corneal epithelial cells at Hamburger-Hamilton stages 20--30 but not in the stroma at any age. Intact corneas from embryos older than stage 30 contain and synthesize type I collagen but no detectable type III collagen. However, whole stromata subjected to collagenase treatment and scraping (to remove epithelium and endothelium) and stromal fibroblasts from such corneas inoculated in vitro begin synthesis of type III collagen within a few hours while continuing to synthesize type I collagen. As demonstrated by double-antibody staining, most corneal fibroblasts contain collagen types I and III simultaneously. Collagen type III was identified biochemically in cell layers and media after chromatography on carboxymethylcellulose be detection of disulfide-linked alpha l (III)3 by SDS gel electrophoresis. The conditions under which the corneal fibroblasts gain the ability to synthesize type III collagen are the same as those under which they lose the ability to synthesize the specific proteoglycan of the cornea: the presence of corneal-type keratan sulfate.

Published

1980

193. Comparison of androgen biosynthesis in isolated leydig cells from rat and mouse testis: incubation and superfusion studies.

Author

Kühn-Velten N, Schumacher H, Wolff J, and Staib W

Subjects

Androstenedione metabolism, Animals, Bucladesine pharmacology, Chorionic Gonadotropin pharmacology, In Vitro Techniques, Leydig Cells drug effects, Male, Mice, Microbial Collagenase pharmacology, Progesterone metabolism, Rats, Testosterone biosynthesis, Androgens biosynthesis, Leydig Cells metabolism

Abstract

Production of testosterone by highly purified Leydig cells prepared from rat and mouse testes is compared. Testosterone formation is improved to a higher degree in rat (2.7-fold) than in mouse (1.7-fold) cells by collagenase treatment of the testis compared with mechanical isolation. Mouse Leydig cells respond to exogenous stimuli (choriogonadotropin, dibutyryl cyclic AMP) with 2.4-fold higher testosterone secretion than rat cells. A 1.7-fold increased conversion of androgen precursors to testosterone by mouse compared with rat Leydig cells is demonstrated in static incubations as well as in steady-state superfusion experiments and can be derived from enhanced androstenedione reduction and a less inhibitory effect of progesterone on this process in mouse Leydig cells.

Published

1984

194. Factors which influence the thickness of basement membrane in diabetes. Evidence of humoral control.

Author

Fisher RF

Subjects

Animals, Basement Membrane drug effects, Basement Membrane pathology, Biometry, Lens, Crystalline drug effects, Microbial Collagenase pharmacology, Organ Size, Rats, Tensile Strength, Diabetes Mellitus pathology, Lens, Crystalline pathology

Published

1979

195. The extent of the odontoblast process in normal and carious human dentin.

Author

Yamada T, Nakamura K, Iwaku M, and Fusayama T

Subjects

Adult, Collagen metabolism, Humans, Microbial Collagenase pharmacology, Microscopy, Electron, Scanning, Molar, Dental Caries pathology, Dentin ultrastructure, Odontoblasts ultrastructure

Abstract

When observed by SEM, after being treated with the HCl-collagenase method, the odontoblast processes extended throughout the whole thickness of dentin in intact teeth and the whole thickness of normal and the inner carious dentin in carious teeth. Small holes and depressions were found on the processes in the transparent layer.

Published

1983

196. [Action of purified collagenase on the organic stroma of carious human dentin].

Author

Triller M

Subjects

Dental Caries, Dentin drug effects, Dentistry, Microbial Collagenase pharmacology

Published

1974

197. In vitro protection of the articular surface by cross-linking agents.

Author

Stanescu R and Stanescu V

Subjects

Animals, Cartilage, Articular ultrastructure, Femur Head drug effects, Femur Head ultrastructure, Glutaral pharmacology, In Vitro Techniques, Mice, Mice, Inbred BALB C, Microbial Collagenase antagonists & inhibitors, Microbial Collagenase pharmacology, Osmium Tetroxide pharmacology, Succinimides pharmacology, Surface Properties, Cartilage, Articular drug effects, Cross-Linking Reagents pharmacology

Abstract

The effects of cross-linking agents on the resistance of the articular surface to digestion with clostridial collagenase were studied using a described in vitro system. Mouse femoral heads were treated with various concentrations of glutaraldehyde, with osmium tetraoxide and with dithiobis (succinimydil propionate), digested with the enzyme, labeled with cationized ferritin and examined by electron microscopy. Collagenase alone caused disruption of the articular surface with penetration of the large marker into the cartilage matrix. After treatment of the femoral heads with the cross-linking agents, no effects on the morphology and on the labeling of the articular surface and no penetration of the label into the cartilage matrix were observed. Increasing cross-linking at the articular surface might be a new route for therapeutic intervention. However, experiments would be needed to assess the effect of the procedure on the viability and nutrition of chondrocytes and on the functional properties of the tissue.

Published

1988

198. Cellular sensitivity to collagen in bleomycin-treated rats.

Author

Schrier DJ, Phan SH, and Ward PA

Subjects

Animals, Humans, Immunity, Cellular drug effects, Kinetics, Lymphocyte Activation drug effects, Microbial Collagenase pharmacology, Pulmonary Fibrosis immunology, Rats, Spleen cytology, Spleen immunology, Trypsin pharmacology, Bleomycin pharmacology, Collagen pharmacology

Abstract

Previous reports have suggested that immune mechanisms are involved in the induction of certain types of pulmonary fibrosis. In this study endotracheal bleomycin was used to induce pulmonary fibrosis in rats, and they were then examined for cellular sensitivity to homologous interstitial collagens isolated from lung. Results indicate that rats treated with bleomycin develop transient cellular sensitivity to homologous collagen. Immunity appears to be selective to type I collagen with minimal response to type III collagen. The kinetics of the development of autoimmunity paralleled the transient increase in collagen synthesis in response to bleomycin treatment. This response was abolished upon prior treatment of the challenging antigen with purified bacterial collagenase, but was resistant to trypsin digestion. This finding confirms the true collagenous nature of the stimulating antigen and eliminates the possibility of a noncollagenous contaminant as the effective agent in the antigen preparation. The data suggest that cellular sensitivity to homologous collagen in response to bleomycin treatment may play a role in the overall fibrotic response.

Published

1982

199. [Effect of collagenase on neuromuscular transmission in the frog].

Author

Iurkanets EA

Subjects

Animals, In Vitro Techniques, Membrane Potentials drug effects, Rana temporaria, Microbial Collagenase pharmacology, Neuromuscular Junction drug effects, Synaptic Transmission drug effects

Abstract

Modification of synaptic function was estimated through the action of 0.1% solution of collagenase on neuromuscular junction in frog. Electrophysiological experiments revealed a decrease of the e.p.p. quantum content on single nerve stimulation with collagenase. The latter or the product of its splitting modify the action zones of mediator secretion. The demyelination action of collagenase on nerve is discussed.

Published

1987

200. [Method of determining the colloidal status of the vitreous body].

Author

Agafonov VA, Anisimov SI, and Fedorov SN

Subjects

Animals, Cattle, Colloids, Desiccation methods, Gels, Humans, Hyaluronoglucosaminidase pharmacology, Male, Microbial Collagenase pharmacology, Rabbits, Time Factors, Vitreous Body drug effects, Water analysis, Vitreous Body analysis

Abstract

A new method for the quantitative estimation of the vitreous body colloidal state has been suggested. For realization of the method a fragment of the vitreous body and an equal volume of water are dried out, and the drying time is registered. The higher is the ratio between the drying time of the vitreous body fragment and water, the higher is the density of the vitreous body gel. The drying out of the vitreous body fragment and water on the analytical balance cups permits the registration of the drying out process in the time course. Thus some additional parameters are obtained that characterize the object studied more completely. The method can be used in experimental and clinical investigations of the vitreous body and other biological liquids.

Published

1984