972 resultados para Mediterranean Ecosystem


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Sediment was collected by either push cores operated by the ROV Quest or by a television guided Multicorer. Nematodes abundance were calculated of the top 5 cm of the sediment to gain individual abundance per 10 cm**2.

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Sediment was collected by either push cores operated by the ROV Quest or by a television guided Multicorer. Nematodes abundance were calculated of the top 5 cm of the sediment to gain individual abundance per 10 cm**2.

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Here, for the first time, we have carried out synoptic measurements of viral production and decay rates in continental-shelf and deep-sea sediments of the Mediterranean Sea to explore the viral balance. The net viral production and decay rates were significantly correlated, and were also related to prokaryotic heterotrophic production. The addition of enzymes increased the decay rates in the surface sediments, but not in the subsurface sediments. Both the viral production and the decay rates decreased significantly in the deeper sediment layers, while the virus-to-prokaryote abundance ratio increased, suggesting a high preservation of viruses in the subsurface sediments. Viral decay did not balance viral production at any of the sites investigated, accounting on average for c. 32% of the gross viral production in the marine sediments. We estimate that the carbon (C) released by viral decay contributed 6-23% to the total C released by the viral shunt. Because only ca. 2% of the viruses produced can infect other prokaryotes, the majority is not subjected to direct lysis and potentially remains as a food source for benthic consumers. The results reported here suggest that viral decay can play an important role in biogeochemical cycles and benthic trophodynamics.

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The dataset is based on samples taken from 12 stations in Northern Aegean Sea, Southern Aegean Sea, Ionian Sea and Libyan Sea during August-September 2008. 12 Niskin bottles (8lt) made by PVC with rubber coated o rings and stainless steel ss springs. Seawater samples (150 mL) were collected from selected depths of the water column (2, 20, 50, 75, 100 m) for the identification and enumeration of phytoplankton cells (>= 5 µm). The samples were fixed with Lugol solution and concentrated to 25 mL by sedimentation. Phytoplankton species abundance was determined with an inverted light microscope (OLYMPUS IX70) according to the Utermohl method (Utermohl, 1958).