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A high-performance liquid chromatographic (HPLC) method is described that allows improved resolution of several chemotaxonomically significant phytoplankton pigments. The protocol, which employs two pumps and a modified Mantoura and Llewellyn (1983) solvent system, can be easily adapted for many HPLC systems currently in use. The most unique aspect of the method is the use of a polymeric C18 reversed phase HPLC column (VYDAC 201TP). In comparison to the monomeric C18 columns typically used in the characterization of phytoplankton pigments, polymeric C18 columns offer superior selectivity for structurally similar compounds. The protocol was evaluated for the ability to resolve most of the phytoplankton pigments of diagnostic importance using algal cultures from nine classes. Pigment pairs that were resolved by the method include a) lutein and zeaxanthin, b) neoxanthin and 19′-hexanoyloxyfucoxanthin, and c) α-carotene and β-carotene, and partial resolution of chlorophyll c1 and chlorophyll c2.  相似文献   
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Groups of 10 menhaden were placed in a round behavioral monitoring pool and exposed to repeated 200 kv/m electromagnetic pulses (EMP). Their swimming activity was recorded on video tape for a 30-min period before, during and after pulsing. The recordings were analyzed for fish swimming speed and rate of change of direction. No significant differences (P > 0.05) were détécted in either paramétér as a result of EMP exposure.  相似文献   
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Concentrations of the accessory phytoplankton pigment 19′-butanoyloxyfucoxanthin (but-fuco), derived from archived high performance liquid chromatography (HPLC) data from the Atlantic coastal bays of Maryland and Virginia (1993–1995 and 1999–2002), were used to determine the presence of Aureococcus anophagefferens at 18 stations. Paired data of direct cell counts of A. anophagefferens and but-fuco concentration data from 2000 to 2002 were linearly regressed (R2 = 0.78). This regression was used to estimate historical cell densities from 1994 to 1995 and to improve the spatial resolution from 1999 to 2002. Although the HPLC method used did not permit quantification of but-fuco before 1994, the records indicate that qualitatively A. anophagefferens was present in 1993. Quantitative measurements grouped into bloom index categories showed that annually, peak densities occurred in May to July. Severe Category 3 blooms (>200,000 cells ml−1) were found in 1995, 2001, and 2002. Spatially, concentrations of but-fuco were higher in the northern extent of the study region than in the lower Chincoteague Bay, and along the western shore of Chincoteague Bay than on the eastern side. On an interannual basis, it appeared that A. anophagefferens became more geographically widespread and blooms more intense throughout the study period.  相似文献   
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