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A reliable and uniform vascular perfusion fixation method for the testis has been developed by using an initial washout solution containing a vasodilator and an anticoagulant. This is followed by a brief fixation with a sodium phosphate buffered formaldehyde-glutaraldehyde solution of conventional strenght, and then a second more concentrated aldehyde fixative solution containing picric acid. The method takes into account some of the unique features of the vascular supply of the male genital tract for its favorable perfusion and fixation. The advantages of this method are: (1) consistently favorable preservation of the testis; (2) simple and inexpensive apparatus; and (3) stable and relatively innocuous stock solutions.
Anat Rec 1977 Jul
PMID:An improved perfusion fixation method for the testis. 33 10

Trials were carried out to investigate the effectiveness of various methods of formaldehyde fumigation as a means of disinfecting calf houses. Houses were cleaned by the farmer, sealed and then fumigated. A significant reduction in bacterial numbers was obtained when the gas was produced by heating paraformaldehyde, mixing formalin with potassium permanganate or boiling formalin in calf houses that could be effectively sealed. Aerosol generators did not give satisfactory results. Efficient pre-cleaning and sealing of the houses were of paramount importance; relative humidity and temperature were less important.
Vet Rec 1977 Jul 02
PMID:Terminal disinfection of calf houses by formaldehyde fumigation. 56 Jul 46

The appearance and development of the primary and secondary sympathetic trunks in staged chick embryos was studied using the Falck-Owman histochemical method for the demonstration of primary monoamines. The earliest appearance of catecholamine (stage 20) was in individual fluorescent cells located in the region of the dorsal root ganglia about two stages prior to the formation of primary trunk aggregates. These cells are believed to be sympathetic precursor cells and correspond to formaldehyde-induced fluorescent cells observed in recent explantation experiments. Aggregates of fluorescent cells had formed bilaterally dorsolateral to the aorta at stage 22. These aggregates became continuous to form primary trunks by stage 24. The secondary sympathetic trunks were first seen in stage 25 and appeared to form at least partially by dorsal migration of cells from the primary trunks. Fluorescent cell processes were first observed at this stage. Secondary trunk formation was essentially complete by stage 28, and the primary trunks had become small and discontinuous. Definite rami communicantes could be observed by the early part of stage 28 in silver preparations. The significance of the development of two successive trunks in avians is discussed.
Anat Rec 1976 Nov
PMID:A correlative histofluorescence and light microscopic study of the formation of the sympathetic trunks in chick embryos. 99 37

The epithelial cells lining the oxyntic mucosa in the stomach "corpus" were identified, localized, and counted in 2-month-old male C57BL-6 mice, using glutaraldehyde-formaldehyde fixation and osmium tetroxide postfixation for studies in the light microscope (LM) while adding tannic acid to the fixative and postfixing in ferrocyanide-osmium for studies in the electron microscope (EM). The cells form a single epithelium, which invaginates into blind tubular units. Each unit is divided into four successive regions: pit, isthmus, neck, and base. On the average, a unit contains 194.2 cells. The cells have been classified into three groups totaling 11 types, listed with their mean number per unit. The first group is composed of three well-characterized cell types, each restricted to a region: (1) 37.0 surface mucous cells, hereafter called pit cells, in the "pit" region, (2) 12.6 mucous neck cells, simply called neck cells, in the "neck" region, and (3) 67.4 zymogenic cells in the "base" region. The second group is also composed of three well-characterized cell types, distributed over the four regions: (1) 26.0 parietal cells, (2) 13.2 entero-endocrine cells, and (3) 0.6 caveolated cell. The third group consists of five cell types, which have been little or not characterized in the past. Four are located in the "isthmus" region and show EM features indicative of immaturity, that is, a nucleus with mainly diffuse chromatin and large reticulated nucleoli, and a scanty cytoplasm rich in free ribosomes: (1) 17.2 cells are the least differentiated in the epithelium; they are devoid of secretory granules and accordingly named granule-free cells, (2) 10.0 cells contain a few dense secretory granules smaller than, but otherwise similar to, those in pit cells; they are referred to as pre-pit cells, (3) 1.8 cells possess a few marbled secretory granules that often exhibit a pale core and are smaller than, but otherwise similar to, those in neck cells; they are called pre-neck cells, (4) 0.6 cells display long microvilli and/or small canaliculi similar to those in parietal cells; they are named pre-parietal cells, and (5) 5.6 cells restricted to the base region are characterized by secretory granules with features intermediate between those of neck and zymogenic cells; they are named pre-zymogenic cells. The observations suggest the following hypothesis on cell filiation.(ABSTRACT TRUNCATED AT 400 WORDS)
Anat Rec 1992 Feb
PMID:Identifying and counting epithelial cell types in the "corpus" of the mouse stomach. 154 2

Lectin binding was studied in the developing airways of Syrian golden hamsters on gestational days 11-16 (day 16 is the day of birth). The trachea and lungs were fixed in 4% formaldehyde-1% glutaraldehyde, 6% mercuric chloride-1% sodium acetate-0.1% glutaraldehyde, and 95% ethanol; embedded in paraffin; and stained with eight lectin-horseradish peroxidase conjugates: Triticum vulgare (WGA), Dolichos biflorus (DBA), Helix pomatia (HPA), Maclura pomifera (MPA), Griffonia simplicifolia I-B4 (GSA I-B4), Arachis hypogaea (PNA), Ulex europeus I (UEA I), and Limulus polyphemus (LPA). Each lectin yielded a characteristic staining pattern, which modulated throughout development. In general, changes in staining characteristics of the tracheal epithelium preceded similar changes in the lobar bronchus, bronchiole, and alveolus. In the case of UEA I, MPA, WGA, and HPA, staining increased with time uniformly over the luminal surface of all epithelial cells. However, in the case of PNA, GSA I-B4, and LPA, after the differentiation of ciliated and secretory cells, the apical surfaces of the ciliated cells stained more intensely than the apical surfaces of the secretory cells. Neuraminidase pretreatment enhanced PNA and GSA I-B4 staining in both cell types. In the case of PNA, these light microscopic observations were confirmed by ultrastructural study. Unlike the other lectins, the pattern of staining with DBA was unusual. Staining was moderate at first, then decreased (days 13 and 14), then increased at all airway levels. This study shows that different glycoconjugates modulate in airway epithelial cells throughout fetal development.
Anat Rec 1990 Oct
PMID:Changes in glycoconjugates revealed by lectin staining in the developing airways of Syrian golden hamsters. 170 Jun 50

beta-Galactosidase activities (beta-GA) of E. coli strains carrying the fusion gene of recA and lacZ, GE94 and its DNA repair-deficient derivatives such as KY946[uvrA], KY945[recA] and KY943[lexA] treated with UV, 4NQO, MNNG and MMC were examined. The beta-GA, reflecting the SOS-inducing activity, of GE94 and KY946 treated with these compounds increased significantly with a clear dose-response relationship, and reached a maximum level within 60 min, while no response was seen in KY945 and KY943. Using KY946 and KY945 as a positive and a negative indicator, respectively, the SOS-inducing activity of oxidative mutagens, i.e., hydrogen peroxide (H2O2), formaldehyde, tert-butyl hydroperoxide, cumene hydroperoxide and streptonigrin, was investigated. Clear dose-dependent increases in beta-GA were observed in KY946 treated with all oxidative mutagens tested, but not in KY945. Significant increases in beta-GA were observed with a lower concentration of H2O2 and a shorter incubation time of 4NQO in this assay than in the umu-test. The assay, called 'Rec-lac test' by us, may be useful to detect environmental genotoxic substances.
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PMID:'Rec-lac test' for detecting SOS-inducing activity of environmental genotoxic substance. 189 67

A procedure has been developed for the three-dimensional immunoelectron microscopic localization of cytoskeletal filaments by a deep-etching replica method in combination with immunogold labeling and/or myosin subfragment 1 (S1) decoration techniques. Neonatal hamster heart cells grown on glass coverslips were extracted with Triton X-100 or physically permeabilized by breaking open the cell membranes. S1 decoration was performed on some specimens immediately after the permeabilization. After prefixation in formaldehyde, samples were immunostained with poly- or monoclonal antibodies to desmin or vimentin, and indirectly tagged with colloidal gold probes by the biotin-streptavidin method. After postfixation with glutaraldehyde, tannic acid and osmium tetroxide, the cells were freeze-etched and rotary-replicated with platinum and carbon in a freeze-fracture apparatus. Replicas were viewed with a transmission electron microscope using a tilting specimen stage to obtain stereo images. The procedure made it possible to identify the specific filaments within the complex cytoskeletal networks in cultured hamster heart muscle and nonmuscle cells at high resolution and in three dimensions. The method has advantages in its three-dimensionality and feasibility to evaluate the data by comparing them with those obtained by alternative light microscopic methods. Details of the protocol and a description of the results of using three different antibodies are given.
Anat Rec 1991 Mar
PMID:Deep-etching immunogold replica electron microscopy of cytoskeletal elements in cultured hamster heart cells. 202 81

Diabetes induces osteopenia, which is characterized by a deficiency of osteoid and decreased activity of osteoblasts. We recently found that tetracyclines prevent the loss of osteoid and bone matrix and the degeneration of osteoblasts in diabetic rats by a mechanism independent of their antimicrobial efficacy. However, bone remodeling requires the activity of osteoclasts as well as osteoblasts. To determine the in vivo effects of tetracycline on osteoclasts in long bones, either a tetracycline (minocycline, TC) or its chemically modified non-antibiotic analogue (CMT), 4-de-dimethylaminotetracycline, was administrated daily to streptozotocin-induced diabetic rats by oral intubation. After 21 days, the rats were perfusion-fixed with a mixture of formaldehyde and glutaraldehyde, and the humeri were dissected and processed for ultracytochemical demonstration of acid trimetaphosphatase (ACPase) activity. In untreated non-diabetic (control) rats, the osteoclasts at the zone of provisional ossification exhibited abundant mitochondria and cisterns of rough endoplasmic reticulum (RER) throughout the cytoplasm, prominent stacks of Golgi membranes, and lysosomes in the perinuclear cytoplasm, and numerous various pale vacuoles in the cytoplasmic area adjacent to well-developed ruffled border. Intense ACPase activity was observed in the Golgi saccules, lysosomes, pale vacuoles, and the extracellular canals of ruffled border. The reaction products were also noted along the resorbing bone surfaces associated with the osteoclast ruffled border. The osteoclasts in the untreated diabetic rats showed a cytoplasmic organization similar to that of the non-diabetic control rats, but showed little or no ruffled border which was replaced by a broad clear zone in some of these cells. However, most of the osteoclasts on bone matrix in the diabetics were devoid of both a ruffled border and a clear zone. ACPase activity was detected in the osteoclast cytoplasm of diabetic rat, as in the controls, but to a much lesser extent along the broad clear zone facing the resorbing bone surfaces. The osteoclasts in TC-treated diabetic rats possessed both a clear zone and a small ruffled border. However, in some cases, they lacked both structures reminiscent of the untreated diabetic cells. The osteoclasts of CMT-treated diabetic rats exhibited structural and enzymatic features essentially identical to those of the non-diabetic control rats. These results suggest that the diabetes-induced osteopenia results, at least in part, from degeneration of osteoclasts (as well as atrophic osteoblasts) and that tetracyclines may be effective in preventing these abnormalities by a mechanism not dependent on the drugs' antimicrobial properties.
Anat Rec 1990 Aug
PMID:Tetracycline administration normalizes the structure and acid phosphatase activity of osteoclasts in streptozotocin-induced diabetic rats. 216 33

A simple method for the simultaneous staining of nerve cells and fibers, applicable to sections of pieces embedded in methacrylate, is described. Sections of 12 micron in thickness were attached to slides and stained for 10-18 hours in the following solution: 0.03% thionin, 0.5% formaldehyde, 0.5% acetic acid in distilled water. They were then rinsed in acetic water (0.5% acetic acid) for 30 seconds, washed in distilled water, dehydrated through 96% and absolute ethanol, cleared in eucalyptol, and mounted in Eukitt.
Anat Rec 1987 Mar
PMID:Differential technique to stain nerve cells and fibers in methacrylate sections. 243 34

A simple, rapid method for the differential staining of myelinated nerve fibers and nerve cell bodies, applicable to sections of central nervous system pieces embedded in paraffin, is described. Experimental material fixed by perfusion with mixed aldehydes or necropsy material fixed in formaldehyde can be used. Constant and homogeneous results are obtained with this technique, and the most important characteristic is the absence of differentiation in either of the steps: staining of myelinated fibers and staining of nerve cell bodies. Sections 15 microns thick were attached to slides, dewaxed, and hydrated. After hydration, sections are mordanted (30 min) in 2.5% iron alum (SO4)2FeNH4, and rinsed (1 min) in distilled water. Staining is for 180 min in the following solution: 5 ml freshly made 20% alcoholic hematoxylin diluted with 25 ml of distilled water and 25 ml of absolute ethanol to which 10 ml of 1% Li2CO3 is added. The sections are washed in distilled water (5 min) and stained during 5 min in the following solution: 0.2% pyronine, 20% formaldehyde in distilled water. The sections are dehydrated through 96% and absolute ethanol, cleared in eucalyptol, and mounted in Eukitt. Myelinated fibers appear dark blue, whereas nerve cell bodies are stained red and the cell nucleoli dark blue. This procedure provides an adequate contrast for observation and photography.
Anat Rec 1988 Dec
PMID:New technique for differential staining of myelinated fibers and nerve cells on paraffin sections. 246 6

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