Expression of aquaporin-4 water channels in the digestive tract of the guinea pig

Expression of the aquaporin-4 (AQP4) water channel was systematically studied in the digestive tract of the guinea pig using Western blot and immunofluorescence techniques. The results showed that AQP4 was expressed widely in different segments of the guinea pig digestive tract. AQP4-immunoreactivity was confined to parietal cells in the stomach, and absorptive and glandular epithelial cells of small and large intestine. AQP4 protein was also expressed by enteric glial cells of submucosal and myenteric ganglia and primary nerve trunks. AQP4 was expressed by both type I and type II enteric gliocytes, but not by type III or type IV enteric gliocytes, indicating that enteric gliocytes have a heterogeneous distribution in the gut wall. In addition, different patterns of AQP4 expression in the enteric nervous system of human, guinea pig, rat and mouse colon mucosa were identified: in rat and mouse AQP4 was localised to a small subpopulation of neurons; in the guinea pig AQP4 was localised to enteric glial cells; and in the human colon mucosa, AQP4 was also detected mainly in the glial cells. It has been speculated that AQP4 may be involved in water transport in the gastrointestinal tract. Its role in enteric neurons and glia is unknown, but, by analogy with the brain, AQP4 may be involved in the formation and resolution of edema.     

Development of protective functions of the pig digestive tract in ontogenesis

It has been found that the state of protective functions of the digestive tract change during postnatal period. The biosynthesis and secretion of glycoproteins of mucus layer which is the main protective structure of digestive tract depend on the hormonal background and the nutrition conditions. The biosynthesis stages and secretion glycoproteins result in sexual maturity and in conditions of definitive nutrition. Opposite to that, the antiradical activity of adherent mucous layer decreases with age. The allocation of the studied components of adherent mucous layer in the stomach and in the intestine is determined.     

The effect of phospholipases on the active uptake of norepinephrine by synaptosomes isolated from the cerebral cortex of guinea pig

—Phospholipase A (EC 3.1.1.4) and phospholipase C (EC 3.1.4.3) were used for studying the role of phospholipid of synaptosomal membrane on norepinephrine uptake activity. Synaptosomes were isolated from cerebral cortex of guinea pigs and treated with phospholipase A or phospholipase C before the uptake experiments. Treatment of synaptosomes with phospholipase A has resulted in severe inhibition of norepinephrine-uptake. Under similar conditions, the activity of synaptosomal (Na + K)-ATPase (EC 3.6.1.4) was also inhibited by phospholipase A treatment whereas the activity of synaptosomal acetylcholinesterase (EC 3.1.1.8) was not affected. On the other hand, the norepinephrine-uptake was not influenced by phospholipase C treatment. The inhibition of norepinephrine-uptake after phospholipase A treatment may be due to the liberation of lyso-components of phospholipids since a low concentration of lysolecithin as well as other detergents (deoxycholate and sodium dodecyl sulphate) also inhibit the uptake activity. However, electron microscopic examination indicated that the synaptosomal particles still maintain their morphological features after phospholipase A treatment. It is possible that the active uptake of norepinephrine depends upon the fine arrangement of phospholipids present at the active sites of the synaptosomal membrane.     

On the mechanism of binding of human lymphocyte products to guinea pig macrophages

When lymphocytes from a majority of patients with cancer are incubated with encephalitogenic factor, a lymphocyte product is released that reduces the anodic electrophoretic mobilities of guinea pig macrophages and fixed, tanned sheep erythrocytes. Although these reactions are not specific for cancer, it is distinctly possible that in patients with cancer, products from stimulated lymphocytes are capable of altering the surfaces of the patients' own macrophages, thereby modifying the course of their disease. In this paper, we attempt to elucidate some mechanisms for the binding of lymphocyte products to macrophages, such as occurs in the macrophage electrophoretic mobility (MEM) test, since this may be of general interest. Binding of lymphocyte product to macrophages has been monitored by measurements of their electrophoretic mobilities and by electron microscopic determination of the density of binding of electron-dense, cationic colloidal iron hydroxide particles to their surfaces. The results show that the lymphocyte products reduce the net surface negativity of the macrophages by (coulombic) binding of this net positively charged material to sialic acids at the macrophage surface. Product-binding can be prevented by prior treatment of the macrophages with neuraminidase. It appears that only a minority of sialic acids are involved in the binding process, which occurs without demonstrable blocking of adjacent sialic acids or redistribution of such sites over the macrophage surface. Parallel experiments with fixed tanned erythrocytes also suggest that binding of lymphocyte products is not solely determined by surface sialic acids, although it cannot occur without them.     

Kinetic mechanism of guinea pig neutrophil 5-lipoxygenase

The kinetic mechanism of guinea pig neutrophil 5-lipoxygenase was investigated using a continuous spectrophotometric assay that monitors product diene formation at 236 nm due to substrate oxygenation. Progress curves for reactions with both arachidonic acid and eicosapentaenoic acid are characterized by 1-3-min lag phases in the attainment of steady-state velocities and product inhibition, as indicated by the total cessation of the reaction prior to complete depletion of substrate. The dependence of the steady-state velocity on arachidonic acid concentration appears to follow Michaelis-Menten kinetics, with Vmax = 4.2 +/- 0.4 nmol of 5-hydroxy-6,8,11,14-eicosatetraenoic acid/min/mg of protein and Ks = 25 +/- 4 microM. The addition of Ca2+ results in an overall activation: lag phases are shortened to 10-20 s, Vmax increases to 24 +/- 2 nmol/min/mg of protein, and Ks decreases to 7.7 +/- 1.7 microM; and a change in a mechanism to one involving substrate inhibition (Kss = 13 +/- 1 microM). The observed activation by Ca2+ has a half-maximal response at around 30 microM. In the presence of Ca2+, ATP causes an increase in Vmax to 30 +/- 4 nmol/min/mg of protein without changing Ks or Kss and a reduction of the lag to less than 5 s. The half-maximal response for ATP is 31 +/- 7 microM. Oxygenation of eicosapentaenoic acid in the presence of Ca2+ and ATP occurs with similar kinetics, except for significantly less substrate inhibition: Vmax = 31 +/- 6 nmol/min/mg of protein, Ks = 7 +/- 1 microM, and Kss = 33 +/- 2 microM. This is the first report suggesting a kinetic mechanism for 5-lipoxygenase, which accounts for substrate inhibition, regulation by Ca2+, and ATP and substrate specificity.     

臭椿沟眶象幼虫消化道解剖方法

臭椿沟眶象幼虫消化道柔软脆弱,尤其是1龄与2龄幼虫的消化道纤细易断,解剖难度较大。本文介绍了臭椿沟眶象幼虫消化道的具体解剖方法,根据不同龄期幼虫脂肪含量与消化道韧性差异,对1-2龄和3-7龄幼虫,分别使用纵切法和剥离法解剖。结果表明:臭椿沟眶象幼虫消化道分为前肠、中肠和后肠。前肠为窄而细的管状,没有明显的嗉囊和前胃。中肠分为2部分,前部膨大,后部为光滑的管状。后肠由回肠和直肠组成。马氏管6根。这两个方法提高了此幼虫消化道解剖的效率与成功率,希望能为具有体壁柔软、消化道脆弱易损等特点昆虫幼虫的消化道解剖提供借鉴与参考。     

5-Hydroxytryptamine in the enterochromaffin cells of the guinea pig alimentary tract

Summary The histoohemical properties of the EC in the guinea pig alimentary canal were studied using the paraformaldehyde-induced fluorescence and five ordinary staining reactions. The fluorescence reaction was observed to be the most sensitive and specific one in the demonstration of the EC. Using the fluorescence and argyrophil techniques concomitantly, it was stated that all the fluorescent EC had also argyrophil properties. These observations lend further support to the author's earlier statement (Penttilä), 1966) that there is only one principal type of EC in the gastrointestinal tract. The argentaffin and other staining reactions were not able to colour all the EC, except in the duodenum.In the quantitative part of this study the EC number (No./mm) and the 5-HT (g/g) concentration were determined from the adjacent tissue pieces. Both quantities were absolutely at its highest in the duodenum and decreased in the caudal direction of the intestine. In the stomach the values were of the same magnitude as in the middle part of the intestinal tract. In the oesophagus there were no EC and the 5-HT content was negligible in comparison to the other gastrointestinal sites. The correlation between the EC number and the 5-HT content was highly significant from the stomach to the rectum. The 5-HT content per one EC was the largest in the duodenum. Comparing the histochemical and quantitative results the 5-HT location in the enterochromaffin system was discussed.     

Culturable microorganisms from the earthworm digestive tract

The cultured aerobic copiotrophic bacteria and fungi from food-free digestive tracts of Aporrectodea caliginosa, Lumbricus terrestris, and Eisenia fetida earthworms, soil (compost), and fresh earthworm excrements were investigated. The microorganisms were isolated on nutrient media and identified by sequencing the fragments of bacterial 16S rRNA and fungal 28S rRNA (D1/D2 domain) gene sequences with subsequent phylogenetic analysis. Bacteria isolated from the digestive tracts of earthworms belonged to the families Aeromonadaceae, Comamonadaceae, Enterobacteriaceae, Flavobacteriaceae, Moraxellaceae, Pseudomonadaceae, and Sphingobacteriaceae (Bacteroidetes), as well as Actinobacteria. For five strains, namely Ochrobactrum sp. 341-2 (α-Proteobacteria), Massilia sp. 557-1 (β-Proteobacteria), Sphingobacterium sp. 611-2 (Bacteroidetes), Leifsonia sp. 555-1, and a bacterium from the family Microbacteriaceae, isolate 521-1 (Actinobacteria), the similarity to known 16S rRNA sequences was 93–97%; they therefore, probably belong to new species and genera. Bacterial groups isolated from the digestive tracts of earthworms were significantly different from those isolated from soil and excrements. Some bacterial taxa occurred in different sections of A. caliginosa intestine and in intestines of different earthworm species; however, the overall composition of bacterial communities in these objects is different. Existence of bacterial groupings symbiotically associated with intestines is proposed. Among the fungi, Bjerkandera adusta and Syspastospora parasitica were isolated from the cleaned digestive tracts as light-colored, sterile mycelium, as well as Geotrichum candidum, Acremonium murorum (A. murorum var. felina), Alternaria alternata, Aspergillus candidus, A. versicolor, Cladosporium cladosporioides, Rhizomucor racemosus, Mucor hiemalis, Fusarium (F. oxysporum, Fusarium sp.), and Penicillium spp. These fungi survive for a long time in the earthworm’s digestive environment. Investigation of the functional characteristics and role in the host organism is required to confirm the symbiotic status of the microorganisms associated with the earthworm digestive tract.     

On the mechanism of binding of human lymphocyte products to guinea pig macrophages.

When lymphocytes from a majority of patients with cancer are incubated with encephalitogenic factor, a lymphocyte product is released that reduces the anodic electrophoretic mobilities of guinea pig macrophages and fixed, tanned sheep erythrocytes. Although these reactions are not specific for cancer, it is distinctly possible that in patients with cancer, products from stimulated lymphocytes are capable of altering the surfaces of the patients' own macrophages, thereby modifying the course of their disease. In this paper, we attempt to elucidate some mechanisms for the binding of lymphocyte products to macrophages, such as occurs in the macrophage electrophoretic mobility (MEM) test, since this may be of general interest. Binding of lymphocyte product to macrophages has been monitored by measurements of their electrophoretic mobilities and by electron microscopic determination of the density of binding of electron-dense, cationic colloidal iron hydroxide particles to their surfaces. The results show that the lymphocyte products reduce the net surface negativity of the macrophages by (coulombic) binding of this net positively charged material to sialic acids at the macrophage surface. Product-binding can be prevented by prior treatment of the macrophages with neuraminidase. It appears that only a minority of sialic acids are involved in the binding process, which occurs without demonstrable blocking of adjacent sialic acids or redistribution of such sites over the macrophage surface. Parallel experiments with fixed tanned erythrocytes also suggest that binding of lymphocyte product is not solely determined by surface sialic acids, although it cannot occur without them.