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1. Alkaline phosphatase (orthophosphoric-monoester phosphohydrolase (alkaline optimum), EC 3.1.3.1) in guinea pig thymus was extracted optimally in 10 mM Tris - HCl buffer at pH 8.0 containing 5 g/l Triton X-100. 2. alpha-Glycerophosphate, beta-glycerophosphate and phenolphthalein monophosphate were hydrolyzed by thymus extract with a pH optimum at 9.8-10.0, whereas p-nitrophenylphosphate and alpha-naphthylphosphate were hydrolyzed with pH optima at 10.7-10.8 and beta-naphthylphosphate at pH 11.2. P-Nitrophenylphosphate and phenolphthalein monophosphate proved to be the most suitable substrates. 3. Alkaline phosphatase was effectively inhibited by EDTA, Zn2+, histidine and urea therefore resembling the inhibition characteristics of alkaline phosphatase in the placenta and kidney, but not that in the liver and intestine, which differed markedly. 4. DEAE-cellulose chromatography and polyacrylamide disc electrophoresis revealed three enzyme peaks which did not differ in their substrate specificities and modifier characteristics. 5. Polyacrylamide disc electrophoresis of thymus, serum, placenta, kidney, liver, bone and intestine revealed no alkaline phosphatase bands definitely unique to thymus.  相似文献   

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Sites of alkaline phosphatase (APase) activity in a facultative thermophilic strain of Bacillus licheniformis MC14 have been localized by electron microscope histochemistry, using a lead capture method. The effects of 3% glutaraldehyde and 3.0 mM lead on APase activity were investigated, and these compounds were found to significantly inhibit enzyme activity, 68 and 18%, respectively. A number of parameters were varied in studies to localize APase activity, including: growth temperature (55 and 37 degrees C); substrate concentration in the histochemical mixture (0.06, 0.15, 0.30, 1.00 mM); fixatives; protoplast preparations and whole cells; phosphate-repressed and -derepressed cells; and age of vegetative cells (mid-log and late log). These variations affected the number but not the location of lead phosphate deposits, which appeared at discrete sites along the inner side of the cytoplasmic membrane. Control cells incubated in histochemical mixtures lacking substrate, lead, or both exhibited no lead phosphate depositis. The histochemical localization at membrane sites correlated well with biochemical localization data, which indicated that greater than 80% of the APase activity was associated with the membrane fraction in logarithmically growing cells.  相似文献   

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Putrefactive anaerobe 3679 (Clostridium sporogenes), a gram-positive bacterium, was examined by light and electron microscopy during normal growth and in a medium containing sorbate (50 mM, pH 6.5), hydrochloric acid (pH of medium adjusted from 7 to 5 with HCl), or nitrite (1 mM, pH 7). During the early exponential growth phase, untreated cells were filamentous and nonseptate, but became septate later and divided when the culture entered the stationary phase. Untreated short and filamentous cells had a double-layered cell wall. Sorbate-treated cells were usually filamentous and nonseptate, but with distorted shapes characterized by numerous bends and bulges. Septation, when present, resulted in minicells. The inner cell wall appeared to be thickened and the outer wall was absent in many areas. Acid-treated cells were similar to sorbate-treated cells but contained septa. Considerable cellular debris was present in the suspension. Nitrite-treated cells were also filamentous, bent, and bulged but the cell wall appeared normal. Considerable cellular debris was also present in suspensions of nitrite-treated cells. Changes in morphology are discussed in relation to possible mechanisms of cell growth regulation and the inhibitory action of sorbate, acid, and nitrite.  相似文献   

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C S Adams 《Acta anatomica》1983,116(2):146-151
The activities of alkaline phosphatase and reduced nicotinamide adenine dinucleotide (NADH) diaphorase in the principal cells of the guinea pig epididymis were studied histochemically. Alkaline phosphatase activity was absent from the principal cells but was present in the basement membrane of the epididymal epithelium. NADH diaphorase activity was distributed throughout the cytoplasm of the principal cells in each epididymal segment. There was a gradual increase in NADH diaphorase activity from segments 1 through 7. Possible functions of alkaline phosphatase and NADH diaphorase in the epididymis are discussed.  相似文献   

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C S Adams 《Acta anatomica》1983,115(3):282-287
The activity of acid phosphatase in the principal cells of the guinea pig epididymis was studied histochemically. The enzyme activity was localized in the Golgi and apical regions in segments 1-4. In segments 5-7, the enzyme activity was distributed throughout the entire supranuclear cytoplasm. There was a gradual increase of acid phosphatase activity from segments 1-7. A possible function of acid phosphatase in the epididymis is discussed.  相似文献   

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Summary Early post mortem changes in the Organ of Corti are described. 15 minutes after death, when kept at room temperature, 20° C (63° F), an oedematous swelling is observed within the cytoplasm of hair cells and nerve endings, the latter being more severe affected. After 30 minutes post mortem the mitochondria of the hair cells have also become significantly swollen. Three hours post mortem the general character of the hair cells is still recognizable, but most of the nerve endings have been completely destroyed. Acknowledgement. We wish to express our appreciation of the skilful technical assistance of Mrs. B. Flock, Miss A.-M. Lundberg, Miss Sonja Löfvenius, Mr. G. Bornholm and Mr. Rune Ragnefjell.This work was supported by grants from the Swedish Medical Research Council, the National Institute of Health grant (no NB 03956-02), the Therese and Johan Anderssons minne, the Gustav and Tyra Svenssons fund and the King Gustav V Research Fund.  相似文献   

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Summary The ultrastructural localisation of acid phosphalase activity was investigated on the guinea pig conjunctival epithelium incubated in vivo with a suspension of latex spheres. Deposits of acid phosphatase reaction product were concentrated on the elements of GERL, the phagocytic vacuoles, and the cell membrane. Acid phosphatase activity in GERL was intense in basal and suprabasal cells and decreased towards the superficial cells. Phagosomes containing latex spheres and reaction product of acid phosphatase were observed mainly in the centrospheral region of the superficial and intermediate epithelial cells. Acid phosphatase activity in phagocytising cells was not increased as compared to that in non-phagocytising cells. The observations indicate that existing acid phosphatase in unstimulated conjunctival epithelial cells is released into heterophagosomes brought within the lysosomal compartment. The number of secondary phagosomes seems to be increased by intercellular transport of latex spheres to the acid phosphatase rich cells in the deep layers of the epithelium.  相似文献   

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Summary The distribution of glycogen, non-specific alkaline phosphatase, and specific phosphatases acting on adenosine monophosphate, adenosine triphosphate, inosine triphosphate, thiamine pyrophosphate, uridine diphosphate, fructose-6-phosphate, fructose-1:6-diphosphate, and glucose-6-phosphate is described in the placentae and accessory structures of the horse, sheep, cat, dog, ferret, rat, rabbit, guinea pig, and man, and in the yolk-sac of the chick, the oviviparous fish Limia maculata, and man.Correlation between the distribution of these substances and placental function is sought, and the results are discussed with respect to the trophoblast, decidua, giant cells, yolk-sac, non-placental chorion and maternal epithelium and uterine secretion, and allantois. The significance of the presence of the enzymes in the carnivore interstitial matrix, the ferret thickened endoderm and the rodent spongy zone is also considered.  相似文献   

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S Latkovic 《Histochemistry》1985,83(3):245-249
The ultrastructural localisation of acid phosphatase activity was investigated on the guinea pig conjunctival epithelium incubated in vivo with a suspension of latex spheres. Deposits of acid phosphatase reaction product were concentrated on the elements of GERL, the phagocytic vacuoles, and the cell membrane. Acid phosphatase activity in GERL was intense in basal and suprabasal cells and decreased towards the superficial cells. Phagosomes containing latex spheres and reaction product of acid phosphatase were observed mainly in the centrospheral region of the superficial and intermediate epithelial cells. Acid phosphatase activity in phagocytising cells was not increased as compared to that in non-phagocytising cells. The observations indicate that existing acid phosphatase in unstimulated conjunctival epithelial cells is released into heterophagosomes brought within the lysosomal compartment. The number of secondary phagosomes seems to be increased by intercellular transport of latex spheres to the acid phosphatase rich cells in the deep layers of the epithelium.  相似文献   

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