UMLS:C0276640 - FACTA Search

Gene/Protein Disease Symptom Drug Enzyme Compound
Pivot Concepts: Target Concepts:

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

The water-rich phase (tissue channels) of the intersititial tissue in rat ileum, knee joint capsules, kidneys, and implanted Guyton's capsules was examined electron microscopically by the SEM of plastic injection models, and by TEM and HVEM of ferrocyanide and ferritin as tracers. It was shown that the channels do in fact exist, and are not just vacuoles. Quantitative estimations of their numbers and diameters were made. These agreed well with estimates made by other methods.
...
PMID:The quantitative morphology of interstitial tissue channels in some tissues of the rat and rabbit. 72 12

This paper describes a simple technique for consistent production of clean, unwrinkled, flat thin (500-1000 A) sections for TEM and thick (1/2-1 micron) sections for HVEM mounted on Formvar-covered slot grids for use in conventional and high voltage electron microscopy. The technique centers around use of a Formvar-covered aluminum supporting rack onto which slot grids that contain sections suspended in water are placed.
...
PMID:A simple procedure for mounting wrinkle-free sections on formvar-coated slot grids. 80 Jun 84

This paper describes four investigations of the olfactory mucosa of the brown trout: 1) the ultrastructure of the olfactory mucosa as revealed by scanning (SEM), conventional transmission (TEM), and high voltage (HVEM) electron microscopy; 2) light and electron-microscopic investigations of retrograde transport of the tracer macromolecule horseradish peroxidase (HRP) when applied to the cut olfactory nerve; 3) SEM and TEM investigations of the effects of olfactory nerve transection on cell populations within the olfactory epithelium; and 4) ultrastructural investigations of reversible degeneration of olfactory receptors caused by elevated copper concentrations. The trout olfactory epithelium contains five cell types: ciliated epithelial cells, ciliated olfactory receptor cells, microvillar olfactory receptor cells, supporting cells, and basal cells. The ciliated and microvillar olfactory receptor cells and a small number of basal cells are backfilled by HRP when the tracer is applied to the cut olfactory nerve. When the olfactory nerve is cut, both ciliated and microvillar olfactory receptor cells degenerate within 2 days and are morphologically intact again within 8 days. When wild trout are taken from their native stream and placed in tanks with elevated copper concentrations, ciliated and microvillar cells degenerate. Replacement of these trout into their stream of origin is followed by morphologic restoration of both types of olfactory receptor cells. Ciliated and microvillar receptor cells are primary sensory bipolar neurons whose dendrites make contact with the environment; their axons travel directly to the brain. Consequently, substances can be transported directly from the environment into the brain via these "naked neurons." Since fish cannot escape from the water in which they swim, and since that water may occasionally contain brain-toxic substances, the ability to close off--and later reopen--this anatomic gateway to the brain would confer a tremendous selective advantage upon animals that evolved the "brain-sparing" capacity to do so. Consequently, the unique regenerative powers of vertebrate olfactory receptor neurons may have their evolutionary origin in fishes.
...
PMID:Ultrastructural neurobiology of the olfactory mucosa of the brown trout, Salmo trutta. 139 70

Cultured cells derived from a mouse adrenocortical tumor transplant are unspecialized in appearance, but produce basal levels of steroids and demonstrate a near-immediate steroidogenic response to ACTH. There is biochemical evidence that ACTH induces increases in the uptake of serum lipoproteins by these cells and that this material is hydrolyzed in lysosomes to free cholesterol, a precursor for steroid end products. To investigate morphologically the role of lysosomes in the steroidogenic activity of these cells, cultures were incubated for 4 h with and without ACTH, then processed for the ultrastructural localization of acid phosphatase (ACPase), a marker enzyme for lysosomes, and for GERL, the lysosome-forming subcompartment of the Golgi, and examined by TEM and HVEM. Steroid output was determined by a fluorometric technique. Unstimulated cells secreted basal levels of steroids. By TEM, large endosomes, some containing semi-compact material and ACPase reaction product, were occasionally seen at the cell periphery and in the Golgi region. The Golgi and GERL were poorly developed. Residual bodies, a few of them ACPase+, appeared in the Golgi region and in microtubule-associated clusters near the cell membrane. ACTH-stimulated cells secreted steroids at 8-10 fold basal values. In TEM records, they displayed numerous ACPase+ endosomes between the cell periphery and the Golgi. The Golgi and GERL regions appeared to be hypertrophied and many large, inclusion-containing, strongly ACPase+ residual bodies appeared here and in elongated microtubule-containing cell processes. HVEM micrographs showed more definitively that ACTH produced distinct increases in the size of GERL and in the number of ACPase+ organelles. Our results suggest that in unstimulated cells, endosomes, presumably containing media-derived material, gain lysosomal enzymes in or near GERL, are transformed to residual bodies as their contents are hydrolyzed, and are subsequently translocated by microtubules to the cell periphery for exocytosis. ACTH appears to intensify all of these effects. The "giant" lysosomes seen in stimulated cells may result from a fusion of smaller lysosomes. Their amorphous contents may reflect an inefficient hydrolysis of LDL to free cholesterol.
...
PMID:The effects of ACTH on acid phosphatase activity in endosomes, GERL and lysosomes of cultured adrenal tumor cells. 287 77

The development of protein bodies in proteinoplasts of tobacco (Nicotiana tabacum L. var. Wis. 38) roots was investigated with TEM, HVEM, and enzyme cytochemistry. These plastids contain a three-dimensional network of fenestrated tubules which originate from invaginations of the inner membrane of the plastid envelope. Elaboration of the network occurs in parallel with cell differentiation: slender tubules common to plastids in meristematic cells undergo dilation as protein accumulates during cell differentiation; proteinoplasts of vacuolate and root cap cells usually contain a large protein body. The contents of the peripheral tubules, originating from the inner membrane, are less electron dense than the tubules making up the central network. Localized dilations within the tubular network result in the formation of dense spheroidal structures, protein bodies, apparently as a result of continued protein accumulation via tubules connecting to the central network. Protein might be imported from segments of rough ER attached to or apposed to the outer membrane of the proteinoplast envelope. The presence of catalase (E.C. 1.11.1.6), peroxidase (E.C. 1.11.1.7), and cytochrome oxidase (E.C. 1.9.3.1) was demonstrated by cytochemistry with diaminobenzidine (DAB) as substrate. Oxidized DAB was found in protein bodies after incubation in each of the specific reaction media. While aminotriazole and sodium azide inhibited oxidation of DAB by catalase and peroxidase, respectively, only potassium cyanide completely inhibited oxidation of DAB in protein bodies. We conclude that protein bodies of proteinoplasts in tobacco roots are not sites for storage of protein, rather protein bodies contain heme protein(s) with strong oxidase activity that may convey a specific function to proteinoplasts.
...
PMID:Development and enzyme activity of protein bodies in proteinoplasts of tobacco root cells. 404 99

A 1 MeV EM-7 TEM has been modified to investigate the possibility that low-dose studies of biomacromolecular crystals might be more effectively carried out in an HVEM. The modifications include a TV viewing system, a deflection-type minimum exposure system, a side-entry, -150 degrees C transfer cold-stage and improvement of the working resolution to 0.2 nm. The advantages of HVEM for this type of study include a possible reduction in radiation damage rate, greater depth of focus on tilted specimens, broader instrumental contrast transfer function and a reduction in dynamical effects on thicker samples. Disadvantages and possible solutions to them are also discussed. Preliminary results on radiation damage in catalase at 400, 600 and 800 kV and images of catalase and squaric acid are included.
...
PMID:An HVEM for high resolution low-dose studies of biomacromolecules. 649 26

Human platelets have been observed by scanning electron microscopy after spreading on glass substrates followed by brief incubation in 1 mM ZnCl2 and subsequent shearing with a jet of buffer. The surfaces of many cells in such preparations are noted to consist of a reticular meshwork similar in appearance to the membrane skeleton of erythrocytes. In some preparations the reticular network is partially or almost entirely disrupted revealing an internal trabecular cytoskeleton and in the central region of the spread cell, granules associated with the cytoskeletal matrix. These results confirm previous observations obtained in TEM and HVEM studies of platelets and in addition provide information concerning the relative disposition of the filament systems in such spread cells. Preliminary results from sodium dodecyl sulfate-polyacrylamide gel electrophoretic analysis of platelets and isolated platelet membranes suggest a basis for the effect of ZnCl2 on various platelet cytoskeletal and membrane components.
...
PMID:The platelet reticular network. 654 84

The fine structure of the several layers and regional specializations in the Drosophila melanogaster eggshell has been studied by a combination of shell isolation procedures and ultrastructural techniques (conventional TEM, whole-mount TEM, SEM, HVEM, freeze-fracture electron microscopy utilizing rotary replication, shadow casting, optical diffraction and stereo imaging). The main shell consists of 5 layers: the vitelline membrane (300 nm thick), the wax layer, the innermost chorionic layer (40-50 nm), the endochorion (500-700 nm), and the exochorion (300-500 nm). The vitelline membrane consists of irregularly organized particles. The wax layer appears to contain multilayered hydrophobic plates which split tangenitally upon freeze fracturing. The innermost chorionic layer is composed of a crystalling lattice. The endochorion is made of a thin (40 nm) fenestrated floor composed of 40-nm fibres and an outer solid (200 nm) roof covered with a network of 40-nm strands. Intermittently spaced pillar connect these 2 parts. Similarities in the substructure of the floor, pillars and roof suggest that they may be composed of similar or identical structural elements. The specialized regions of the shell are the 2 respiratory appendages, the operculum area and the posterior pole. The appendages exhibit 2 sharply distinct surfaces, a dorsal side with isolated 1.5-micrometer plaques and a ventral side with strands of 40-50 nm connected in a network with openings of 70-80 nm. The operculum area, which includes the micropoyle and the collar, is distinguished by 3 unique types of cell imprints. The posterior pole contains 2 distinctive populations of cell imprints: the central area has very thin intercellular ridges and a thin, perforated, endochorionic roof, while the peripheral area contains mixed, thick and thin, intercellular ridges and serves as a transition zone to the main shell pattern. The pillars in the central area of the posterior pole have a distinct arrangement, forming one peripheral circle within each cell imprint. An analysis utilizing structural and developmental criteria indicates that as many as ten different populations of follicular epithelial cells may be involved in the construction of the various regions of the Drosophila eggshell.
...
PMID:The eggshell of Drosophila melanogaster. I. Fine structure of the layers and regions of the wild-type eggshell. 677 86