Gene/Protein Disease Symptom Drug Enzyme Compound
Pivot Concepts:   Target Concepts:
Query: UNIPROT:Q9UIJ5 (Rec)
 58,342 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

Neuroepithelial endocrine (NEE) cells were for the first time identified in the lung of the entirely aquatic urodele, Ambystoma mexicanum, by using light and electron microscopy, histochemistry, and immunocytochemistry. In the basal part of the ciliated epithelium and, less often, in the respiratory portion of the lung, NEE cells were found to occur both solitarily and in small clusters. No typical neuroepithelial bodies could be found. Using the method of Fernandez Pascual, some NEE cells were found to be argyrophilic. Microspectrofluorimetric analysis of formaldehyde-induced fluorescence and immunocytochemistry revealed the presence of 5-hydroxytryptamine. With antibodies to neuron-specific enolase only a few NEE cells exhibited a faint immunostaining. Electron-microscopically, the NEE cells are provided with distinctive cytoplasmic membrane-bound dense granules of variable size, which gave a positive argentaffin reaction. The images of emiocytotic granule release are indicative of a secretory function. In the tracheal epithelium. NEE cells seem to occur only solitarily. They bear the same ultrastructural characteristics as the intrapulmonary NEE cells but here, the dense granules are larger and associated with numerous bundles of microfilaments. Intraepithelial nerve endings were observed near the airway lumen. Between nerve terminals and NEE cells, synaptic complexes with aggregations of clear-centered vesicles close to the presynaptic membrane thickenings were observed. In addition, some nerve endings from "reciprocal synapses" with NEE cells. A receptosecretory function for NEE cells in the lung of A. mexicanum is supposed.
Anat Rec 1989 Oct
PMID:Neuroepithelial endocrine cells in the lung of Ambystoma mexicanum. 281 28

Collagen fibrils were present within membrane-bound vacuoles in the cytoplasm of mouse decidual cells on the 7th day of pregnancy. The space between the vacuole membranes and the fibrils was narrow and frequently filled with a granular electron-dense material. The loss of banding of the collagen fibrils, their association with lysosomelike bodies, and the demonstration of acid phosphatase activity in the vacuoles indicate that the fibrils were internalized by the decidual cells and were being digested. It is suggested that phagocytosis of collagen is a mechanism of remodeling of the mouse decidua.
Anat Rec 1989 Oct
PMID:Phagocytosis of collagen by mouse decidual cells. 281 34

As a result of screening procedures employed for animals entering the AI service, two bulls were identified as being persistently infected with bovine virus diarrhoea virus by isolation of the virus from blood. Semen was collected on two occasions from these bulls; its quality as measured by density and motility was poor. Gross abnormalities of the sperm head, termed 'collapsed' heads, were seen in 28 to 45 per cent of sperm from one bull and in 1 per cent of sperm from the other. The collapsed heads were small and the whole head or its anterior part had the appearance of a dried pea. Electron microscopy showed the defect to consist of convoluted nuclear material with membrane-bound vacuoles and invaginations containing membranous debris and lamellar structures. In the 'high incidence' bull there was a corresponding increase in enlarged sperm heads. The 'low incidence' bull had sperm with heads of similar mean size to sperm from control bulls but with an increased variance. The semen was diluted in a lactose diluent, frozen and stored in liquid nitrogen. The distribution of viral antigen was determined and virus was isolated from several fractions of the semen, both before and after processing and cryopreservation. In one animal raw semen failed to yield virus but virus was recovered after processing, suggesting that raw semen may not be suitable for the efficient detection of the virus.
Vet Rec 1988 Jul 30
PMID:Some observations on the semen of bulls persistently infected with bovine virus diarrhoea virus. 284 30

The enamel organ of growing rat incisors was perfusion-fixed with a mixture of formaldehyde and glutaraldehyde and processed for ultracytochemical demonstration of ouabain-resistant, K+-stimulated p-nitrophenylphosphatase representing the second dephosphorylative step of H-K-ATPase by use of the one-step lead method. Throughout the stages of amelogenesis, the enzymatic activity was found in the plasma membranes, mitochondrial membranes, and lysosomal structures of the cells of stratum intermedium, papillary layer, and ameloblast layer. Gap junctions and desmosomes between these cells were, however, free of reaction product or showed slight precipitates of reaction. The stellate reticulum and the outer enamel epithelium at the stage of enamel secretion were usually negative for reaction. Although secretory, transition, and ruffle-ended maturation ameloblasts showed enzymatic activity at their basolateral cell surfaces, their distal cell surfaces facing the enamel were always free of reaction product. On the other hand, the smooth-ended maturation ameloblasts seldom showed a positive reaction, except in lysosomes and along their basal cell surfaces. An energy-dispersive X-ray microanalysis of reaction products of H-K-ATPase in unosmicated tissue sections demonstrated that they were composed of lead and phosphorus, which had been released during the dephosphorylation of substrate. In cytochemical controls, the enzymatic activity was completely dependent on substrate and potassium ion, resistant to ouabain and levamisole, and inhibited by nolinium bromide, a specific inhibitor of H-K-ATPase. In addition, inorganic trimetaphosphatase as enzymatic marker of lysosome was localized in dark and pale lysosomes, phagosomes, multivesicular bodies, and ferritin-containing vesicles of the ameloblasts and the cells of stratum intermedium and papillary layer. These membrane-bound structures were also positive for H-K-ATPase reaction. These results suggest that: 1) H-K-ATPase functions to maintain an acidic internal pH of lysosomes in the enamel organ cells; and 2) H-K-ATPase localization in the plasma membranes of enamel organ cells is concerned with efflux of protons derived from cytoplasmic water.
Anat Rec 1988 Aug
PMID:H+-K+-ATPase activity in the rat incisor enamel organ during enamel formation. 284 91

Cells of the U937 cell line were grown in delipidated calf serum for 24 and 48 hr. These cells are known cholesterol auxotrophs. When grown for 48 hr without an exogenous source of cholesterol, these cells are known to become depleted of their intracellular cholesterol stores by greater than 95%. The result is an aggregation of the cells upon mild agitation of the culture. Examination of the cell aggregate from these cultures revealed cells in various stages of altered morphology. There was a loss of microvilli from the cells. Subsequently, the Golgi complex became dilated, and secondary lysosomes and myelin figures accumulated in the cytoplasm. The cells became swollen, and the rough endoplasmic reticulum became dilated. A small percentage of the cells showed complete disintegration, with release of membrane-bound fragments and other intercellular debris. These events suggest that the depletion of cholesterol results in the inability of the cell to produce usable membrane. As a consequence, the synthetic apparatus of the cell becomes disrupted.
Anat Rec 1987 Oct
PMID:The effects of cholesterol depletion on cellular morphology. 331 56

The binding of NK cells to a target cell appears to be a necessary step for NK cell-mediated cytolysis. In this report, we demonstrated effector-target binding by immunoelectron microscopy by using monoclonal antibodies against NK cells (Leu-7, Leu-11a) and T-cell subsets (Leu-2a/T8, Leu-3a/T4). The surfaces of NK and K562 cells were characterized by antitransferrin receptor antibody and various lectins. In addition, the controversial phagocytic activity of NK cells was studied by incubation of peripheral blood mononuclear cells with opsonized Staphylococcus aureus and labeling with anti-Leu-7 or anti-Leu-11a antibody. Results showed that only Leu-11a+ cells displayed a broad cell-to-cell contact with the target by a shallow intercellular interdigitation of cytoplasmic projections, while Leu-7+, Leu-2a+, or Leu3a+ cells showed only a partial contact with target without interdigitation. The Leu-11a+ cells were frequently observed in small clusters and in close association with monocytes. Cluster formation and association with monocytes were not observed in other NK and T-cell immunophenotypes. In Leu-11a+ cells conjugated with target cells, membrane-bound granules, small vesicles, parallel tubular arrays, Golgi apparatus, endoplasmic reticulum, and small vacuoles were evident and concentrated toward the target. The surface of NK cells was intensely stained for glycoprotein by chromic acid-phosphotungstic acid, whereas target cells were not stained. Transferrin receptors were stained only on the surface of target cells. Only the lectins RCA and UEA labeled the surfaces of both NK and target cells. Phagocytic vacuoles containing cell debris or fragments and ingested bacteria were found in the cytoplasm of Leu-11a+ cells but not in Leu-7+ cells. NK cells were also found within the cytoplasm of K562 target cells. All these findings suggest that Leu-11a+ cells are the true functional NK cells involved in NK cell-mediated cytolysis, phagocytosis, and emperipolesis. Therefore, the NK cell is probably "a phagocyte in lymphocyte's clothing." The presence of peroxidase in the small vesicles of NK cells and endocytotic vesicles of target cells at the effector-target contact area indicates that cytolytic enzymes or factors derived from NK cells may be transported into the target by endocytosis.
Anat Rec 1987 Mar
PMID:Immunoultrastructural studies of human NK cells: II. Effector-target cell binding and phagocytosis. 357 43

Granulomatous lymphadenopathy, associated with the presence of needle-like refractile particles, was recognised in two dogs. The material was detected in macrophages, either free within the cytoplasm or in membrane-bound lysosomes. By mineral analysis under direct vision in an electron microscope microanalyser (EMMA 4) the particles were found to contain aluminosilicate.
Vet Rec 1986 Apr 19
PMID:Lymphadenopathy in dogs associated with aluminosilicate. 371 7

The ultrastructure of globule leukocytes is described in the nasal and tracheal respiratory epithelium of three boys suffering from chronic airway infections. The globule leukocytes lie free in the intercellular spaces and appear to be migratory cells. They are characterized by intracytoplasmic membrane-bound globules, variable in number, size, shape, and internal structure. The globules may apparently release their content between the neighboring epithelial cells. Human globule leukocytes are also characterized by the presence of intracytoplasmic rod-shaped bodies, the significance of which is not known. They usually display an extended juxta-nuclear Golgi apparatus, presumably involved in the formation of the globules. Comparison of the fine structure of the globules in the globule leukocytes with that of the granules found in the subepithelial mast cells does not support a mast cell origin for human globule leukocytes. On morphological grounds, natural killer cells are postulated as a possible source for globule leukocytes. The function of globule leukocytes is briefly discussed. We presume that the globule leukocytes belong to the group of migrating and secreting cells involved in the defense of the organism against foreign material.
Anat Rec 1985 Jun
PMID:Globule leukocytes in the respiratory epithelium of human upper airways: an ultrastructural study. 384 37

Cardiac myocytes have been shown to occur in the tunica media and adventitia at the region near the hepatic end of the portal vein of the mouse and rat, and have been studied by electron microscopy in the mouse portal vein. They measured 3-10 microns in breadth at their nuclear level, possessed centrally located nuclei, and were connected with each other by the intercalated disk. In these myocytes in the mouse portal vein, sarcoplasmic reticulum was represented by a rather simple and loose network of the anastomosing tubules. The membrane-bound granules, which closely resemble the atrial specific granules, were found in many of the mouse portal vein myocytes. Transverse tubules, 40-200 nm in diameter, were sometimes detectable at the Z line level. The nexus occupied about 3-5% of the whole junctional area between cardiac myocytes in the tunica media, whereas in the tunica adventitia the corresponding value was about 17%. Blood capillaries with fenestrated endothelium supplied the cardiac myocytes in the adventitia of mouse portal vein. The closest relationship between the adrenergic axon and portal vein cardiac myocytes was observed to be ca. 0.3 micron apart. The significance of these findings is discussed in relation to pulsations of the portal vein.
Anat Rec 1985 May
PMID:Occurrence of cardiac muscle in the hepatic portal vein wall of the mouse and rat. 407 40

The secretory acinar cells of parotid glands from rats of varying ages have been examined by electron microscopy to determine what age-related changes occur in these cells. The most prominent change noted in these cells is the progressive increase in the amount of lipofuscin granules with age. Lipofuscin granules are membrane-bound structures consisting of lipids, other subcomponents, and a matrix. In addition, these cells contain lipid droplets that are not associated with any other components and tend to accumulate at the base of the cells in older rats. Also, many acinar cells in the glands of old rats contain altered secretory granules which appear to be in the process of degeneration. The accumulation of lipid and degenerating secretory granules appears to be related to the reduced level of cellular secretory activity in the glands of older rats. It is possible that these two types of inclusions contribute to the formation of lipofuscin granules. Lipofuscin and degenerating secretory granules are associated with acid phosphatase, which is demonstrated cytochemically, indicating that these granules are lysosomal structures.
Anat Rec 1984 Jul
PMID:Changes in the secretory acinar cells of the rat parotid gland during aging. 646 43


<< Previous 1 2 3 4 5 Next >>