Introduced reindeer and their effects on the vegetation and the epigeic invertebrate fauna of South Georgia (subantarctic)

Summary The introduced reindeer of South Georgia have had a serious impact on the vegetation throughout the range of three populations on the island. Exclosure experiments in areas where the reindeer were introduced have resulted in a dramatic change in the composition of the protected vegetation. Poa flabellata (the major winter food) and Acaena magellanica (a major summer food) have recovered to their former status inside the exclosures, while Deschampsia antarctia and the introduced grass Poa annua tolerate grazing and trampling and have spread over the grazed areas. Festuca contracta and Rostkovia magellanica are not eaten by the reindeer. Trampling has resulted in a high proportion of bare soil and peat in sites freely accessible to reindeer. However, the changes in the vegetation have not had such a significant effect on the associated invertebrate fauna. Thus in grazed and protected areas the faunistic composition is qualitatively similar, although there are quantitative differences, and some of the trends can probably be attributed to the presence of the reindeer. Compared with reindeer-free areas, the abundance of the perimylopid beetle Hydromedion sparsutum (a major primary decomposer) is reduced. The frequency of their egg parasite Notomymar aptenosoma (Hymenoptera, Mymaridae) increases. Consequently the ratio of perimylopoids to mymarids found in pitfall traps shifts from 1:0.01 (ungrazed areas) to 1:0.54 (grazed areas). Also the frequency of sciarids was found to be higher in reindeer areas. The larvae of these probably introduced gnats do not play a role in the natural terrestrial ecosystem of South Georgia, but in reindeer areas they appear to establish larger populations because they are able to live deeper in the soil and in hardened substrates. There is also a shift in the ratio between Collembola (major prey) to spiders from 1:1.3 (ungrazed areas) to 1:0.82 (grazed areas), for animals collected in pitfall traps. This may be a result of the trampling effect of the reindeer.     

A time-lapse video image intensification analysis of cytoplasmic organelle movements during endosome translocation

Vital fluorescence staining has been used in conjunction with time- lapse video image intensification microscopy to analyze the distribution and movement of endosomes, lysosomes, and mitochondria in cultured rat ovarian granulosa cells. Exposure of 5-d granulosa cell cultures to pyrene-concanavalin A (P-Con A) or 3,3'- dioctadecylindocarbocyanine-labeled low-density lipoprotein (dil-LDL) at 4 degrees C results in the formation of randomly distributed endosomes 10 min after warming to 37 degrees C that exhibit saltatory motion for 20 min. If granulosa cells are labeled at 4 degrees C with both P-Con A and dil-LDL and warmed to 37 degrees C, both ligands are found within the same endosomes which migrate centripetally to the cell center where label accumulates within phase-dense structures by 60 min. The initial endosome saltations occur over short distances (mean distance = 4.6 micron) with a mean velocity of 0.03 micron/s. Endosome saltations then cease and are followed by a gradual centriptal migration of endosomes to the cell center where they accumulate and fuse with phase-dense structures. The second phase of movement involves a continuous, unidirectional migration of endosomes over distances ranging from 5 to 40 micron at a mean velocity of 0.05 micron/s. Lysosomes were simultaneously visualized as acridine orange-staining, phase-dense structures in control cells and cells exposed to fluorescent ligands. In untreated cells, lysosomes are dispersed throughout the cytoplasm and undergo bidirectional saltations covering a mean distance of 8.7 micron with a mean velocity of 0.3 micron/s. Lysosomes redistribute centripetally to the perinuclear region of the cell by saltatory movement within 20 min of exposure to ligand. Mitochondria were visualized with the fluorescent dye rhodamine 123 in granulosa cells labeled with P-Con A and were found to redistribute to the cell center coincident with endosomes. The microtubule-disrupting agent nocodazole was found to inhibit lysosome saltations and all phases of endosome movement. Taxol, a microtubule-stabilizing agent, partially impaired lysosome movement and led to a redistribution of lysosomes into linear aggregates surrounding the nucleus. Taxol was also found to inhibit endosome movement. The data indicate that (a) endosome movement proceeds initially by saltation and later by a nonsaltatory centripetal migration in association with mitochondria, that (b) lysosomes and endosomes undergo a temporally distinct but spatially similar change in cytoplasmic distribution, and that (c) microtubules are required for the directed translocation of endosomes and lysosomes towards the cell center.     

Electron microscopic localization of neuron-specific enolase in rat and mouse brain

The cellular distribution and intracellular localization of neuron-specific enolase (NSE) has been studied by electron microscopic immunocytochemistry in the brain of the rat and of the mouse. Although the intensity of staining was less in the mouse, the same structures were positive in both species. In the cerebrum, the neuronal perikarya and dendrites were intensely stained, but staining was almost entirely absent in the presynaptic terminals. The deep neurons of the brain stem were also positive. In the cerebellum, perikarya, axons, and parallel fibers of the granule cell neurons were stained as were the synaptic vesicles and presynaptic membranes of the synapses between the parallel fibers and the Purkinje cell dendrites. Golgi cell dendrites, basket cells and their axons, and mossy fibers were also positive. In contrast, the Purkinje cells including their dendrites, and the climbing fibers that formed synapses with the Purkinje cell dendrites were not stained. The majority of the myelinated axons in both the cerebrum and the cerebellum did not stain, but the fibrillary astrocytic processes between myelinated axons in the white matter did. Oligodendroglia, protoplasmic astrocytes, Bergmann glia, astrocytes investing capillaries, and vascular endothelial cells were negative for reaction product. In the positively staining cells and their processes, the positivity was dispersed throughout the cytoplasm and corresponded most closely to the distribution of ribosomes, the granular endoplasmic reticulum, and microtubules. Nuclei, mitochondria, the cisternae of the Golgi complex, myelin lamellae, and most membranes were not stained.     

云南叶螨属一新种(蜱螨目:叶螨科)

在鉴定云南叶螨标本时,发现叶螨属一新种,现记述如下。模式标本保存于上海农学院。本文量度单位均为微米。 食禾叶螨Tetranychus graminivorus新种(图1—14) 雌螨 体长(包括喙)454,宽298。椭圆形。浅黄绿色。须肢端感器圆柱形,长6.8,     

Mechanism of complement-induced stimulation of prostacyclin production by isolated rabbit peritoneum

The interaction between the complement system and prostaglandin synthesis has not thoroughly been explored, although both mediators are known to be involved in inflammatory reactions and endotoxic shock. When rabbit peritoneum, a rich source of prostacyclin forming activity was incubated in serum in which the complement system was activated (CVF, LPS, zymosan), the tissue produced significantly more PGI2, when compared with appropriate controls, indicating that by activation of the complement, factors were generated that stimulated PGI2 biosynthesis. Further results indicated that tryptic cleavage products of complement factor C3 and C5 also led to the appearance of PGI2 releasing principles with a molecular weight of about 7000-11000. The stimulation of PGI2 biosynthesis was explained by enhanced release of AA, and not due to increased activity of cyclo-oxygenase or PGI2 synthetase. Our results suggest that complement-derived products may promote the supply of prostaglandins at the site of inflammation.