Your search keyword '"Cetin Y"' showing total 164 results

151. Suitability of different staining methods for the identification of isolated and cultured cells from guinea pig (Cavia aperea porcellus) stomach.

Author

Giebel J, Arends H, Fanghänel J, Cetin Y, Thiedemann KU, and Schwenk M

Subjects

Animals, Cell Separation methods, Cells, Cultured, Coloring Agents, Guinea Pigs, Immunohistochemistry, Parietal Cells, Gastric cytology, Gastric Mucosa cytology

Abstract

Cell suspensions from the guinea pig gastric mucosa were obtained using a pronase/collagenase isolation method, and cultured on Petri dishes in minimum essential medium at 37 degrees C. For proper identification of different gastric cell types in cytospots, cell suspensions or culture, selective staining methods were employed, modified and evaluated. Mucous cells and mucous neck cells were detected by use of lectins. Mucous cells were stained on cytospots and in primary cultures with lectins from peanut, Helix pomatia, Ulex europaeus, wheat germ, and from soybean. Vital chief cells in suspensions but not in culture, were selectively stained by Nile blue sulphate, brilliant cresyl blue or the fluorescence dye dihexyloxacarbocyanine iodide. Pepsinogen granules of isolated and cultured chief cells were detected with a polyclonal antibody against porcine pepsinogen. Isolated parietal cells were identified in cytospots by using acidophilic dyes (aurantia, eosin). In suspensions and in cultures vital parietal cells were identified by enzymatic detection of succinic dehydrogenase or carboanhydrase activity and by the vital stain Janus green. In cultures exclusively, parietal cells were additionally identified by the vital stain rhodamine. Cytochemically, they were identified with phalloidin by binding to actin filaments. Endocrine cells in the suspension were visualised immunocytochemically with antibodies directed against different amines or peptides. Fibroblasts and endothelial cells were identified after isolation and in primary culture with a vimentin antibody. Mast cells in suspension were either visualised by a histamine antibody or by metachromatic staining behaviour to toluidine blue, respectively. Endothelial cells in suspension or culture were distinguished from fibroblasts by endocytosis of acetylated low-density-lipoprotein. In conclusion, the developed methods are highly suitable to identify guinea pig gastric cells after isolation and follow up their fate in primary culture.

Published

1995

152. GCAP-II: isolation and characterization of the circulating form of human uroguanylin.

Author

Hess R, Kuhn M, Schulz-Knappe P, Raida M, Fuchs M, Klodt J, Adermann K, Kaever V, Cetin Y, and Forssmann WG

Subjects

Amino Acid Sequence, Calcium-Binding Proteins blood, Calcium-Binding Proteins chemistry, Calcium-Binding Proteins physiology, Cyclic GMP metabolism, Guanylate Cyclase-Activating Proteins, Humans, Molecular Sequence Data, Natriuretic Peptides, Peptides chemistry, Sequence Homology, Amino Acid, Tumor Cells, Cultured, Calcium-Binding Proteins isolation & purification

Abstract

The systematic isolation of circulating regulatory peptides which generate cGMP as second messenger resulted in the identification of a novel member of the guanylin family. In the present study we describe the purification and amino acid sequence of a new guanylate cyclase C activating peptide (GCAP-II). GCAP-II contains 24 amino acids in the following sequence: FKTLRTIANDDCELCVNVACTGCL. Its molecular mass is 2597.7 Da. The 16 C-terminal amino acids are identical to uroguanylin from human urine. native and synthetic GCAP-II activate GC-C, the specific guanylate cyclase receptor, of cultured human colon carcinoma (T84) cells. GCAP-II stimulates chloride secretion in isolated human intestinal mucosa mediated by intracellular cGMP increase. GCAP-II specific antibodies were used to localize the peptide by immunohistochemistry in entero-endocrine cells of the colonic mucosa.

Published

1995

153. Differential distribution of synaptotagmin I and rab3 in the anterior pituitary of four mammalian species.

Author

Redecker P, Cetin Y, and Grube D

Subjects

Animals, Antibodies, Monoclonal, Cricetinae, Follicle Stimulating Hormone analysis, Gerbillinae, Guinea Pigs, Immunoblotting, Immunohistochemistry, Luteinizing Hormone analysis, Male, Mesocricetus, Rats, Rats, Inbred Lew, Species Specificity, Synaptotagmin I, Synaptotagmins, Tissue Distribution, rab3 GTP-Binding Proteins, Calcium-Binding Proteins, GTP-Binding Proteins analysis, Membrane Glycoproteins analysis, Nerve Tissue Proteins analysis, Pituitary Gland, Anterior chemistry

Abstract

In the anterior pituitary of rat, gerbil, hamster and guinea pig, the presence and cellular distribution of the synaptic vesicle-associated proteins synaptotagmin I and rab3 were analyzed by immunoblotting and by immunocytochemical staining of serial semithin sections. Our results show that rab3 proteins are ubiquitously expressed in all endocrine cell types of both the anterior and intermediate lobe. In many cells, rab3 immunoreactivity was concentrated beneath the plasmalemma. This intracellular distribution coincided with the distribution of secretory granules, suggesting a possible association of rab3 proteins with the latter organelles. The staining patterns observed using two monoclonal rab3 antibodies with different isoform specificities are compatible with the recent suggestion that rab3B is the dominant rab3 isoform in anterior pituitary cells. However, we could demonstrate that also rab3A is present in endocrine adenohypophyseal cells, albeit at low levels. In contrast to rab3, synaptotagmin I immunoreactivity was only detected in a limited number of adenohypophyseal endocrine cells. Whereas the monoclonal synaptotagmin I antibody consistently failed to immunostain lactotrophs and endocrine cells of the intermediate lobe, other endocrine cell types displayed variable immunoreactivities towards this antibody. Although a low level of synaptotagmin I expression in the immunonegative cells cannot be excluded, the above observation may reflect a differential distribution of synaptotagmin isoforms in endocrine organs, as it has been described for the nervous system. Our study has established that endocrine cells of the anterior pituitary are endowed with proteins of the rab3 and synaptotagmin families which are generally thought to play important roles in the regulation of the trafficking and/or exocytosis of secretory organelles and, hence, probably fulfil similar functions in adenohypophyseal cells.

Published

1995

154. Biogenic amines in the guinea pig endocrine pancreas.

Author

Cetin Y

Subjects

Animals, Aromatic Amino Acid Decarboxylase Inhibitors, Benserazide administration & dosage, Benserazide pharmacology, Glucagon analysis, Guinea Pigs, Immunoenzyme Techniques, Injections, Intraperitoneal, Insulin analysis, Male, Somatostatin analysis, Catecholamines analysis, Islets of Langerhans chemistry

Abstract

Pancreata of guinea-pigs were investigated for the presence and cellular distribution of biogenic amines. Out of the established endocrine cell types only insulin (B-) cells contained immunoreactivity for serotonin and noradrenaline. However, the B-cells' content of both amines was quite variable. Serotonin was also confined to enterochromaffin (EC-) cells. No immunoreactivity for dopamine or histamine was present in any islet cell. Treatment of guinea-pigs with Ro-4-4602 led to a marked decrease of serotonin and noradrenaline in pancreatic endocrine cells. The present findings suggest that serotonin and noradrenaline are involved in the function of the endocrine pancreas, particularly of islet B-cells.

Published

1992

155. Immunoreactivities for chromogranin A and B, and secretogranin II in the guinea pig entero-endocrine system: cellular distributions and intercellular heterogeneities.

Author

Cetin Y and Grube D

Subjects

Animals, Chromogranin A, Digestive System cytology, Endocrine Glands cytology, Endocrine Glands metabolism, Enterochromaffin Cells metabolism, Gastrointestinal Hormones metabolism, Guinea Pigs, Immunohistochemistry, Chromogranins metabolism, Digestive System metabolism, Proteins metabolism

Abstract

The family of the chromogranin/secretogranin proteins consists of three major subtypes: chromogranin A (CgA), chromogranin B (CgB) and secretogranin II (SgII). These proteins are present in various endocrine cells and organs. Using immunohistochemistry on serial semithin sections, we have investigated ten endocrine cell types of the guinea pig gastro-intestinal tract for their content of chromogranin/secretogranin proteins. The gastrin cell was the only cell type containing immunoreactivities for all three chromogranin subtypes. The majority of entero-endocrine cells showed immunoreactivities for CgA and SgII. Somatostatin cells lacked immunoreactivities for any of the chromogranins. Moreover, the densities of the corresponding immunoreactivities varied among the different endocrine cell types or even among endocrine cells of a given population. Aminergic endocrine cells (e.g., enterochromaffin and enterochromaffin-like cells) regularly exhibited strong immunoreactivities for CgA but failed to react for SgII. In peptidergic endocrine cells, the immunoreactivities for both CgA and SgII ranged from dense to faint. This was also true for CgB in gastrin cells. Hence, only CgA and SgII can be considered as regular constituents of entero-endocrine cells. The intercellular differences in immunoreactivities for all three chromogranin subtypes indicate that every endocrine cell has its own composition of chromogranin/secretogranin proteins. This may be due to differences in the regulation of biosynthesis or processing of the chromogranins in individual endocrine cells; this in turn might be related to the functional states of endocrine cells.

Published

1991

156. Immunohistochemistry of opioid peptides in the guinea pig endocrine pancreas.

Author

Cetin Y

Subjects

Animals, Guinea Pigs, Immunohistochemistry, Islets of Langerhans cytology, Dynorphins metabolism, Endorphins metabolism, Enkephalins metabolism, Islets of Langerhans metabolism

Abstract

Previous immunochemical investigations have demonstrated various opioid peptides in the pancreas. However, controversies exist related to the cellular localization of these peptides in the endocrine pancreas. Therefore, the guinea pig endocrine pancreas was immunohistochemically investigated for the presence of opioid peptides derived from pro-dynorphin, pro-enkephalin or pro-opiomelano-cortin. Immunoreactivities were demonstrated on serial semithin sections by the peroxidase anti-peroxidase technique. In routinely immunostained sections, immunoreactivities for dynorphin A and alpha-neo-endorphin were localized in pancreatic enterochromaffin cells, but not in islet cells. Immunoreactivity for Met-enkephalin was confined exclusively to B-cells and was localized only in some secretory granules. However, pre-treatment of semi-thin sections with trypsin and carboxypeptidase B led to a marked increase of Met-enkephalin immunoreactivity in B-cells. In addition, immunoreactivities for Met-enkephalin-Arg-Gly-Leu and bovine adrenal medulla dodecapeptide could be demonstrated in B- and A-cells, and beta-endorphin immunoreactivity was localized in A-cells. In no case, however, were immunoreactivities detected for bovine adrenal medulla docosapeptide, peptide F, corticotropin, melanotropin or dynorphin 1-32. The immunohistochemical findings indicate that opioids of different peptide families are present in the guinea pig endocrine pancreas. Since several opioid peptides of the corresponding pro-hormones could be demonstrated in the reference organs but not in the pancreas, it is concluded that the biosynthetic pathways of the respective precursors are different from those in the adrenal medulla or in the pituitary.

Published

1990

157. [Chromogranins in endocrine cells of the digestive system].

Author

Grube D, Bargsten G, Cetin Y, Jörns A, and Yoshie S

Subjects

APUD Cells cytology, Animals, Chromogranins metabolism, Humans, Immunohistochemistry, Species Specificity, Chromogranins analysis, Islets of Langerhans cytology

Published

1990

158. A novel endocrine cell type in the guinea-pig gastric mucosa: cellular source of pro-enkephalin-derived peptides. A histochemical, immunohistochemical, and electron microscopical characterization.

Author

Cetin Y

Subjects

APUD Cells ultrastructure, Animals, Chromogranin A, Chromogranins metabolism, Gastric Mucosa cytology, Guinea Pigs, Immunohistochemistry, Microscopy, Electron, APUD Cells metabolism, Enkephalin, Methionine analogs & derivatives, Enkephalin, Methionine metabolism, Gastric Mucosa metabolism, Protein Precursors metabolism

Abstract

A novel endocrine cell type has been identified in the guinea-pig gastric mucosa which preferentially occurs in the oxyntic area. Cells of this type exhibit immunoreactivities for bovine adrenal medulla dodecapeptide (BAM-12P) and in many cases for Met-enkephalin and are thus presumed to contain a pro-enkephalin-like precursor protein. Systematic immunohistochemical investigations show that these cells do not contain immunoreactivities for various enteric hormones, neuropeptides and biogenic amines (serotonin, histamine). However, they do contain immunoreactivity for chromogranin A, an acidic glycoprotein which is common to the majority of entero-endocrine cells. Using silver impregnation techniques BAM-12P immunoreactive cells prove to be argyrophil, but fail to react argentaffin. On the electron microscopical level, these cells contain a well-developed endoplasmic reticulum and Golgi apparatus and numerous polymorphous secretion granules which measure about 290 nm in diameter. The secretion granules are ovoid or pear-shaped but largely plump compared to those of enterochromaffin cells. Light and electron microscopical findings indicate that BAM-12P immunoreactive cells constitute an endocrine cell population of the gastric epithelium in addition to the "established" endocrine cells hitherto known in this location.

Published

1990

159. Multiple cellular forms of corticotrophs in surgically removed pituitary adenomas and periadenomatous tissue in Cushing's disease.

Author

Martin R, Cetin Y, Fehm HL, Fahlbusch R, and Voigt KH

Subjects

Adenoma ultrastructure, Adolescent, Adrenocorticotropic Hormone analysis, Adrenocorticotropic Hormone metabolism, Adult, Endorphins analysis, Female, Histocytochemistry, Humans, Immunologic Techniques, Male, Melanocyte-Stimulating Hormones analysis, Middle Aged, Nelson Syndrome pathology, Peptide Fragments analysis, Pituitary Gland, Anterior metabolism, Pituitary Hormones analysis, Pituitary Neoplasms ultrastructure, Adenoma pathology, Cushing Syndrome pathology, Pituitary Gland, Anterior pathology, Pituitary Neoplasms pathology, Pro-Opiomelanocortin

Abstract

Transsphenoidally removed samples of pituitary adenomas from 14 patients with Cushing's disease and 5 patients with Nelson's syndrome always contained groups of uniform small ACTH-cells. Antibodies against the pro-opiocortin precursor fragments beta-endorphin, ACTH, and 16k-peptide recognized material in typical adenoma cells. A subpopulation of these cells, varying in number from sample to sample, specifically exhibited alpha-melanotropin immunoreactivity. Most periadenomatous samples showed signs of severe degeneration. Typical Crooke cells only occurred in samples from patients with Cushing's syndrome, but, with this exception, no clear differences between pituitaries of patients with Cushing's and Nelson's syndromes could be discerned. Two other forms of ACTH-immunoreactive cells were observed: rare, single, highly immunoreactive cells, with characteristics of both normal and Crooke cells, and numerous syncytial groups of cells in an advanced state of disintegration, presumably the remnants of hyperplastic follicles. The four different corticotrophs are characterized according to their fine structure and immunoreactivity in this study.

Published

1982

160. Chromogranin A (CGA) in the gastro-entero-pancreatic (GEP) endocrine system. I. CGA in the mammalian endocrine pancreas.

Author

Grube D, Aunis D, Bader F, Cetin Y, Jörns A, and Yoshie S

Subjects

Animals, Cats, Cattle, Chromogranin A, Chromogranins immunology, Dogs, Enterochromaffin Cells metabolism, Glucagon metabolism, Guinea Pigs, Histocytochemistry, Humans, Immune Sera, Immunoenzyme Techniques, Insulin metabolism, Pancreatic Polypeptide metabolism, Rabbits, Rats, Somatostatin metabolism, Species Specificity, Specimen Handling, Swine, Swine, Miniature, Tupaia, Chromogranins analysis, Islets of Langerhans analysis, Nerve Tissue Proteins analysis

Abstract

Chromogranin A (CGA), a protein at first detected in the adrenal medulla, has recently been found also in other organs, e.g. the endocrine pancreas. However, immunohistochemical findings concerning the cellular source of pancreatic CGA were controversial. Therefore, the endocrine pancreas of 10 mammalian species (man, tupaia, mole, cat, dog, pig, guinea pig, rabbit, rat) was investigated immunohistochemically for CGA-like immunoreactivities on serial semithin plastic sections using a high-titer polyclonal antiserum against bovine CGA. The results show that basically all pancreatic endocrine cell types are CGA-immunoreactive; however, every species has its own pattern of CGA-immunoreactive cell types. Other findings of the present studies indicate that the physiological function of CGA in pancreatic endocrine cells is related to the storage mechanisms of peptide hormones. Finally, a methodological approach is given to obtain not only qualitative but also semi-quantitative data during immunohistochemical investigations.

Published

1986

161. Chromogranin A (CgA) in the gastro-entero-pancreatic (GEP) endocrine system. II. CgA in mammalian entero-endocrine cells.

Author

Cetin Y, Müller-Köppel L, Aunis D, Bader MF, and Grube D

Subjects

Animals, Cats, Cattle, Chromogranin A, Enterochromaffin Cells cytology, Gastric Mucosa cytology, Gastrointestinal Hormones analysis, Guinea Pigs, Humans, Immunohistochemistry, Intestinal Mucosa cytology, Swine, Chromaffin System analysis, Chromogranins analysis, Enterochromaffin Cells analysis, Gastric Mucosa analysis, Intestinal Mucosa analysis, Nerve Tissue Proteins analysis

Abstract

Chromogranin A (CgA) and related acidic proteins are widely distributed in the organism. They are also present in entero-endocrine cells and in other members of the paraneuron family. Therefore, CgA has been claimed as an universal marker of this cellular community. To yield precise data about the distribution of CgA in entero-endocrine cells, all segments of the gastro-intestinal tract of five mammalian species (man, cattle, pig, cat, guinea-pig) were investigated immunohistochemically for CgA. In serial semithin plastic sections, all CgA-immunoreactive endocrine cells were identified for resident amines or peptides. CgA could be found in ten hormonally identified endocrine cell types and in two or three other endocrine cell types. Entero-endocrine cells containing amines (histamine, serotonin) regularly exhibited CgA-immunoreactivities. In contrast, peptide-containing endocrine cells were largely heterogeneous: Their CgA-immunoreactivities varies among the species, among the gastro-intestinal segments, and even among the members of the same cell population. Hence, seen histochemically, CgA is no universal marker for entero-endocrine cells. Seen biochemically, the observed heterogeneities of CgA-immunoreactivities theoretically can be attributed to various factors (species-specificities of CgA, subclasses of chromogranins, processing of CgA or its pro-protein). Most probably, these heterogeneities are caused by species- or cell-specific differences in the extent of processing of CgA. In addition, some findings point to certain interrelations between the processing or storage of CgA and resident peptides in the secretion granules of enteroendocrine cells.

Published

1989

162. Immunohistochemistry of beta-neoendorphin and dynorphin in the endocrine pancreas of rat and man.

Author

Cetin Y

Subjects

Adrenocorticotropic Hormone analysis, Animals, Frozen Sections, Humans, Immune Sera, Immunoenzyme Techniques, Islets of Langerhans cytology, Peptide Fragments analysis, Rats, Species Specificity, Staining and Labeling, Dynorphins analysis, Enkephalins analysis, Islets of Langerhans analysis, Protein Precursors analysis

Abstract

Serial sections from araldite-embedded rat and man pancreata were investigated immunohistochemically for the presence of prodynorphin-related peptides and alpha-endorphin. Immunoreactivities were visualized by the avidin/biotin-peroxidase complex (ABC) technique. In the human pancreas, none of the endocrine cells could be immunostained for prodynorphin-, proopiomelanocortin-related peptides and enkephalins. In the rat pancreas, however, all glucagon cells exhibited immunoreactivities for both beta-neoendorphin and dynorphin A. In addition, these cells contain alpha-endorphin-like immunoreactivity but no immunoreactivities for corticotropin, melanotropin, 16 K-fragment, alpha-N-acetyl-alpha-endorphin and enkephalins. All specificity controls confirmed that the rat endocrine pancreas might be an other source of dynorphin and endorphin with a biosynthetic pathway different from that in the pituitary or in other locations. However, concerning synthesis or degradation of peptide precursor substances interspecies differences may exist.

Published

1985

163. Enterochromaffin (EC-) cells of the mammalian gastro-entero-pancreatic (GEP) endocrine system: cellular source of pro-dynorphin-derived peptides.

Author

Cetin Y

Subjects

Adrenal Medulla cytology, Animals, Cattle, Dogs, Dynorphins analysis, Dynorphins immunology, Endorphins analysis, Endorphins immunology, Enkephalins analysis, Guinea Pigs, Humans, Immunohistochemistry, Pituitary Gland cytology, Pro-Opiomelanocortin analysis, Pro-Opiomelanocortin immunology, Protein Precursors analysis, Chromaffin System ultrastructure, Digestive System cytology, Enkephalins immunology, Enterochromaffin Cells ultrastructure, Pancreas cytology, Protein Precursors immunology

Abstract

It has long been disputed whether mammalian enterochromaffin (EC-) cells contain a peptide in addition to serotonin. Previous immunohistochemical studies have provided evidence for the presence of enkephalins in EC-cells. These findings, however, are equivocal. Therefore, the problem of opioid peptides in EC-cells has been re-examined in the gastro-intestinal mucosa of dog, guinea-pig and man. A battery of antisera against derivatives of pro-opiomelanocortin, pro-enkephalin and pro-dynorphin have been applied to semithin serial sections of the tissues, in combination with fluorescence histochemistry and serotonin immunocytochemistry. Our findings indicate that EC-cells of the investigated species contain pro-dynorphin-related peptides, i.e. dynorphin A and alpha-neo-endorphin, but no derivatives from pro-opiomelanocortin or pro-enkephalin. Since remarkable interspecies variations occur with respect to the number and staining characteristics of opioid immunoreactive EC-cells, it is concluded that pro-dynorphin shows specific routes of post-translational processing depending upon the species and the gastro-intestinal segment investigated. Future studies should focus on the mutual relationships between serotonin and dynorphins and on the physiological significance of these peptides in the gastrointestinal tract.

Published

1988

164. Chromogranins in mammalian GEP endocrine cells: their distribution and interrelations with co-stored amines and peptides.

Author

Grube D, Bargsten G, Cetin Y, and Yoshie S

Subjects

Amines metabolism, Animals, Digestive System cytology, Endocrine Glands cytology, Immunohistochemistry, Pancreas cytology, Peptides metabolism, Chromogranins metabolism, Digestive System metabolism, Endocrine Glands metabolism, Nerve Tissue Proteins metabolism, Pancreas metabolism

Abstract

Chromogranins (Cg) are large acidic proteins, co-stored with amines or peptides in the secretory granules of a wide variety of paraneurons. By immunohistochemistry performed on serial semithin sections, the distribution of Cg in the gastroenteropancreatic (GEP) system was analyzed in the endocrine pancreas of 10 mammalian species and in enteroendocrine cells of 6 species. Of the Cg families, CgA is primarily localized in GEP endocrine cells. CgA was regularly present in amine containing cells (EC and EC-like cells). In 11 other endocrine cell types, CgA-immunoreactivities showed inter-species and intra-species variations in their distribution or in the intensity of staining. However, no endocrine cell type lacked CgA-immunoreactivities in all species investigated. Findings from extended studies indicate that CgA is involved in the intracellular storage of resident amines, and in the storage of newly formed amines after exogenous application of the corresponding precursors. Finally, densitometric findings on possible reciprocal relationships between CgA- and peptide-immunoreactivities suggest that CgA also participates in the intragranular storage of peptide hormones in certain GEP endocrine cells.

Published

1989