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The R/V METEOR cruise M60/3 took place from January 13 through February 14, 2004. Target area was the Logatchev hydrothermal field situated on the Mid-Atlantic Ridge (MAR) with main spots around 14°45'N and 44°59'W and 14°55'N and 44°55'W. The active Logatchev hydrothermal field lies on a small plateau on the eastern flank of the inner rift valley in 2900 m to 3060 m water depth. It is characterized by sites of active, high-T fluid emanation and sulfide precipitation as well as by inactive sites. CTD data for 17 stations located in the vicinity of the Logatchev hydrothermal field were recorded using a SEABIRD CTD Type 911, mostly for the entire water column. CTD sensors had been calibrated by SEABIRD directly before the cruise; additional calibrations of the data obtained, e.g. by salinometer measurements of selected samples were not accomplished. For most stations, no indication of hydrothermal plumes could be identified within the CTD-profiles. An exception is station M60/3-37-CTD-R for which the S/T plot evidences the intrusion of a component relatively depleted in salinity for the depth area from 2600m to 2700m water depth.

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Fluorescence in situ hybridization (FISH) with rRNA-targeted oligonucleotide probes was used to investigate the phylogenetic composition of bacterioplankton communities in several freshwater and marine samples. An average of about 50% of the cells were detected by probes for the domains Bacteria and Archaea. Cells were concentrated from water samples (1 to 100 ml) on white polycarbonate filters (diameter, 47 mm; pore size, 0.2 mm; type GTTP 4700 [Millipore, Eschborn, Germany]) by applying a vacuum of <25 kPa. They were subsequently fixed by covering the filter with 3 ml of a freshly prepared, phosphate-buffered saline (pH 7.2)-4% paraformaldehyde (Sigma, Deisenhofen, Germany) solution for 30 min at room temperature. Airdried filters are ready for hybridization and can be stored at 220°C or room temperature for several months without showing apparent changes. Probes BET42a, GAM42a, and PLA886 were used with competitor oligonucleotides as described previously amongst others in Manz et al., (1992; doi:10.1016/S0723-2020(11)80121-9). The filters were transferred to a vial containing 50 ml of prewarmed (48°C) washing solution (70 mM NaCl, 20 mM Tris-HCl [pH 7.4], 5 mM EDTA, 0.01% sodium dodecyl sulfate) and incubated freely floating without shaking at 48°C for 15 min. The filter sections were dried on Whatman 3M paper (Whatman Ltd., Maidstone, United Kingdom) and covered with 50 ml of DAPI solution (1 mg/ml in distilled water filtered through at 0.2-mm filter) for 5 min at room temperature in the dark. For each sample and probe, more than 500 cells were enumerated; for the DAPI examination, more than 1,500 cells were counted per sample. All probe-specific cell counts are presented as the percentage of cells visualized by DAPI. The mean abundances and standard deviations were calculated from the counts of 10 to 20 randomly chosen fields on each filter section. All counts were corrected by subtracting the counts obtained with the negative control NON338. Mean and standard deviation were calculated from the counts of 10 to 20 randomly chosen fields on each filter section.