UMLS:C0276640 - FACTA Search

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Query: UMLS:C0276640 (TEM)
20,729 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

The effect of IH764-3, a potent component isolated from Salvia miltiorrhiza, on the proliferation and function of cultured fibroblasts was studied. It was found that the fibroblast growth curve had a dose-dependent relationship with IH764-3 concentration. The incorporation of 3H-TdR and 3H-proline into fibroblasts was significantly inhibited by IH764-3, and calmodulin, fibronectin and thrombospondin contents in the test group were obviously lower than those in the control group. Flow cytometry showed that in the IH764-3-treated group, the percentage of cells in G0/G1 phase was higher than that in the control. Electron microscopic observation (TEM and SEM) showed that in the treated group, collagen secretion was decreased. All of these results indicate that IH764-3 exerts a direct inhibitory effect on fibroblast proliferation and affects their ability to synthesize collagen.
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PMID:The effect of IH764-3 on fibroblast proliferation and function. 128 82

It has been suggested that matrix molecules like fibronectin and laminin influence the differentiation and migration of embryonic cells. We investigated the role of these two glycoproteins in somitogenesis as well as in the differentiation and migration of the avian Wolffian (pronephric and mesonephric) duct. At first, we described essential steps in the development of these two organ anlagen by light microscopy, SEM and TEM. To localize fibronectin and laminin more exactly in the actual stages, we used the indirect immunoperoxidase reaction at the light microscopic level and the peroxidase-antiperoxidase technique at the ultrastructural level. Fibronectin was found at the surface of the unsegmented paraxial mesoderm, increasing in the cranial direction, and in the basal laminae of somites and Wolffian duct. The mesenchymal tip of the duct contains a moderate amount of fibronectin. In the two investigated organ anlagen, laminin was found mainly in the basal laminae. The role of fibronectin and laminin was investigated further by using synthetic peptides that mimic the main cell binding domain of either fibronectin or laminin, and that competitively inhibit their cell surface receptors. Thus, the pentapeptides GRGDS, YIGSR, and for control, SHLVE were micro-injected under the ectoderm of 2-day-old embryos. After treatment with GRDS, the Wolffian duct and the segmental plate are more compact. The rounded cells exhibit only short processes and narrow intercellular spaces. At the side of injection the duct shows a delay in migration. After treatment with YIGSR the Wolffian duct migrated laterally over the somatopleure. The basal laminae seem to be incomplete. SHLVE had no effect. Our results suggest that fibronectin is a prerequisite for the migration of the Wolffian duct, and that laminin probably plays a role in guiding the duct. The epithelialization during somitogenesis and differentiation of the duct is a more complex process involving also fibronectin and laminin.
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PMID:The role of fibronectin and laminin in development and migration of the avian Wolffian duct with reference to somitogenesis. 186 90

One of the factors proposed to control initiation of migration of neural crest (NC) cells is disruption of the basal lamina (BL) that is presumed to exist over the dorsal portion of the neural tube. Previously, we discovered that, in the mouse embryo, a continuous BL is not deposited over the dorsal portion of the neural tube until emigration of the NC cells is terminated. Here, we show that the pattern of BL deposition in chick embryos is similar, but not identical, to that in the mouse. In particular, (i) patches of BL are deposited on the premigratory NC cells in the chick but not in the mouse and (ii) BL is thicker and more interstitial matrix is deposited at the same stage of development in the chick. In addition, immunofluorescent and immunogold labelling of collagen IV, laminin and fibronectin show that (i) patches of young BL contain all three molecules; (ii) collagen IV and laminin are present in BL throughout neurulation but fibronectin either disappears or becomes masked in more mature BL and (iii) collagen IV and especially fibronectin are present in the interstitial matrix, but the relative abundance of fibronectin changes with time. The simultaneous use of immunolabelling for both light and TEM sections has allowed us to determine unambiguously that presence of a basement membrane (light microscopy) does not necessarily imply presence of basal lamina. We conclude that, as in mouse, the BL cannot be involved in the timing of the initiation of migration of NC cells. Our evidence in both the mouse and the chick, together with work in the axolotl, suggests that the basic pattern of BL deposition during neurulation may be a general phenomenon in embryonic development. Moreover, these results, in conjunction with the work of others, suggest that the critical step for initiation of migration of NC cells may be the loss of adhesions between cells.
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PMID:Basal lamina is not a barrier to neural crest cell emigration: documentation by TEM and by immunofluorescent and immunogold labelling. 333 60

Numerous investigations have demonstrated that basement membranes (BMs) are composed of type IV collagen, laminin, heparan sulfate proteoglycan, nidogen, and possibly fibronectin. The precise proportion and supramolecular organization of these molecules within BMs is unclear, but is believed to be tissue-specific. In an effort to provide morphological evidence for BM specificity, we studied isolated bovine retinal capillary BMs by high-resolution SEM. Cryofractured specimens demonstrated that surfaces of BM leaflets and pericytic matrix (PCM) within the retinal capillary BM complex are composed of 20- to 100-nm granules and beaded fibrils arranged in patterns which are specific for each cell type. Subendothelial BMs and the subjacent PCM are composed of 20- to 30-nm granules loosely arranged and marked by numerous pits, features that are consistent with their TEM morphology and known susceptibility to proteolytic attack. These BMs also frequently exhibit large openings or fenestrations. These compare favorably with their fragmented image by TEM and probably represent BM discontinuities necessary for direct contact of pericytes and endothelial cells. Muller cell BMs are also composed of granules though they are much larger (40-100 nm) and more densely packed then those of subendothelial BMs. Moreover, they frequently contain interstitial collagen fibrils which could account for the tube-like structural rigidity exhibited by acellular retinal vessel BMs in SEM views. Data in the current study provide morphological evidence for direct contact of pericytes and endothelial cells in vivo and support the view that tissue specificity of BMs may be more exquisite than previously believed, extending even to surface topography of BM leaflets within capillary BM complexes.
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PMID:Topographical specificity in isolated retinal capillary basement membranes: a high-resolution scanning electron microscope analysis. 336 94

Indirect immunofluorescent staining with anti-tubulin antibodies, SEM and TEM were applied to study microtubule (MT) assembly in clones isolated from Friend leukemia cells (FLC, 745 A strain) on the basis of their sensitivity to exogenous fibronectin (FN). Kinetics of cell spreading and elongation were studied using computerized image analysis and SEM. In contrast to 745 A cells, FN-sensitive clones (referred to as FF clones) showed elaborate MT networks when observed by immunofluorescent staining as well as by TEM. A good correlation was found between the degree of spreading and elongation of FF cells and the degree and cellular distribution of their MT. The highest concentration of MT networks oriented parallel to the main cellular axis was observed in very elongated FF cells. The majority of MT in interphase FF cells radiated from the centrosomes; some MT apparently originated from the nuclear membranes. TEM showed the existence of morphological differences between centrosomes of 745 A and FF cells. The characteristic ultrastructure of the centrosomes of FF cells was maintained in trypsinized cells, even if such FF cells lost MT's and acquired a spherical morphology. FF cells, treated with a wide spectrum of MT-disrupting agents, promptly acquired a rounded morphology with rapid dissolution of polymerized tubulin. Removal of MT-disrupting agents from the culture medium rapidly restored a flattened morphology with concurrent regeneration of MT's. During recovery from MT-disrupting agents, FF cells showed increased numbers of centrosomes per cell. We conclude that MT networks cooperate in the attachment, spreading and elongation of FF cells isolated from FLC. Moreover, we hypothesize the existence in FF cells of a variant form of centrosomes as compared with those of 745 A cells.
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PMID:Induction and maintenance of flattened morphology in highly adhesive Friend leukemia clones depends on the time- and space-specific assembly of microtubular networks. 390 71

The pericytes of capillaries are interesting cells which resemble the smooth muscle cells of larger vessels in some aspects of their morphology and behavior. In this report, their relationship to the underlying endothelium has been investigated in some detail. Using indirect, fluorescent immunocytochemical techniques on fresh and fixed tissues, it was found that fibronectin (an adhesive protein in many tissue culture systems) is concentrated in spots along vessels and is only faintly visible in the basement membranes of exhaustively perfused preparations. By electron microscopy, using a peroxidase immunocytochemical marker, these concentrations of fibronectin were seen to be localized to the pericyte-endothelial interstitia. Examination by TEM using a new fixation procedure demonstrated the organization of microfilaments and dense plaques along the pericyte membrane with fibrous and basement membrane-like material within this interstitial space. The arrangements of these elements suggest a mechanical linkage between the two cells. Such a linkage would allow contractions or relaxation of the pericyte to affect vessel diameter.
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PMID:Fibronectin in the microvasculature: localization in the pericyte-endothelial interstitium. 634 2

Antigenic markers characteristic of astrocytes and their differentiative states (i.e., glial fibrillary acidic protein (GFAP), vimentin, and M1 and C1 antigens) were investigated in the pineal gland of mouse and rat using double immunolabeling techniques. In both species the so-called interstitial cells as characterized by TEM were shown to be astrocytes, since they expressed vimentin, but neither fibronectin (a marker for fibroblasts and endothelial cells) nor the neuron-specific L1 antigen or tetanus toxin receptors. Subpopulations of vimentin-positive pineal astrocytes were also GFAP- and C1- antigen-positive. M1- antigen-positive cells were not detected. It is concluded that a considerable proportion of interstitial cells in the pineal gland of rat and mouse are immature astrocytes which, in contrast to other parts of the central nervous system, persist into adulthood.
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PMID:Glial cells in the pineal gland of mice and rats. A combined immunofluorescence and electron-microscopic study. 647 92

Fibronectin has been localized to basement membranes and cell surfaces with the light microscope by fluorescent staining of thick sections, and with the TEM by immunoperoxidase reaction. However, these methods are limited because it is difficult to appreciate the patterned distribution of fibronectin from sectioned material. We have developed a probe for fibronectin that facilitates its identification with the SEM. Our probe consists of two parts; the first component is a derivatized methacrylate microsphere 90 nm in diameter, linked to purified sheep anti-rabbit IgG. The second component is anti-fibronectin IgG raised in rabbits. Stage-3 to -12 chick embryos were fixed and the ectoderm covering the cranial mesoderm was removed. Embryos were treated with testicular hyaluronidase, exposed to rabbit anti-fibronectin IgG and finally to sheep anti-rabbit IgG conjugated microspheres. As expected, the basal lamina of surface and neural ectoderm as well as the remaining fibrous ECM were heavily decorated with microspheres, whereas control embryos treated with preimmune serum were beadless. Fibronectin was localized on the cell soma and processes of primary mesenchyme as early as stage 3. In addition, it was possible to decorate to various extents, populations of prosencephalic, mesencephalic, and rhombencephalic cranial neural crest cells. Our studies suggest that fibronectin is present in the cranium of chick embryos at earlier times than heretofore realized, and that fibronectin accumulates in a cranial to caudal gradient that reflects the sequential differentiation of the embryonic axis.
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PMID:SEM localization of cell-surface-associated fibronectin in the cranium of chick embryos utilizing immunolatex microspheres. 674 25

Mother-fetus exchanges at the placental level are found to be altered in women affected by hypertensive or diabetic pregnancies following the onset of microenvironmental, circulatory, trophic or tissue disorders. Our aim was therefore to assess the alterations occurring within the umbilical cord, particularly its venous endothelial component and underlying smooth muscle layer, using transmission (TEM) and scanning electron microscopy (SEM) and immunohistochemical analyses. Immunohistochemical data appear to support the ultrastructural evidence for an activated state of these vascular structures, in both conditions (hypertension and diabetes). Furthermore, mainly during diabetic pregnancies, extracellular matrix molecules such as tenascin and fibronectin also quantitatively increase at the vein wall level. The umbilical cord seems to be a structure capable of responding actively to abnormal microenvironmental conditions which seriously threaten the health of the fetus and also the mother herself.
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PMID:The human umbilical vein in normal, hypertensive and diabetic pregnancies: immunomorphological and ultrastructural evidence. 754 29

IH764-3, a potent component isolated from Salviae miltiorrhizae (a component of TML) was used to study the effect on proliferation and functions of cultured fibroblasts. The fibroblast growth curve demonstrated a dose-dependent relationship between growth and IH764-3 concentration. The incorporation of 3H-TdR and 3H-proline into fibroblasts was significantly inhibited by IH764-3. Calmodulin level, fibronectin and thrombospondin contents in the test group were obviously lower than those in the control group. Flow-cytometry showed that in the IH764-3 treated group, the percentage of cells in G0 + G1 phase was higher than that in the control. Electron microscopic observation (TEM and SEM) showed that in the treated group, the secretory function of collagen had decreased. All the results indicated that IH764-3 exerts a direct inhibitory effect on fibroblast proliferation and affects their ability to synthesize and secrete collagenous substances.
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PMID:[The effect of IH764-3 on proliferation and function of fibroblasts]. 822 6

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