Descripción
The present study was conducted in the continental shelf of Heraklion Bay in depths from 50 to 200 meters, covering an area exposed to wave action. The coastal zone is affected by small-scale freshwater inputs and urban waste discharges while the offshore system is characterised by marked oligotrophy. The study area is located outside the local bottom trawling fishing grounds.
Versiones
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¿Cómo referenciar?
Los usuarios deben citar este trabajo de la siguiente manera:
Panayota (Yolanda) Koulouri, Heraklion Bay Sampling, MOUNT Project, 01-06 June 2019.
Derechos
Los usuarios deben respetar los siguientes derechos de uso:
El publicador y propietario de los derechos de este trabajo es Hellenic Center for Marine Research. Esta obra está bajo una licencia Creative Commons de Atribución/Reconocimiento (CC-BY 4.0).
Registro GBIF
Este recurso no ha sido registrado en GBIF
Palabras clave
Metadata; benthic boundary layer macrofauna; hyperbenthos; macrobenthos; macrozooplankton; benthic crustaceans; continental shelf; Heraklion Bay; eastern Mediterranean; Metadata
Contactos
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Cobertura geográfica
Sampling was carried out in one transect of three stations (St.1, St. 2, St. 3) at depths of 50,100 and 200 m. St. 1 Lat. 35.362000, Lon. 25.1000667 / St. 2 Lat. 35. 382883, Lon. 25.099350 / St. 3 Lat. 35. 422783, Lon. 25.094817
Coordenadas límite | Latitud Mínima Longitud Mínima [35,264, 24,78], Latitud Máxima Longitud Máxima [35,528, 25,659] |
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Cobertura taxonómica
hyperbenthic, (endo-)benthic and planktonic macrofaunal taxa (species of crustaceans, polychaets, molluscs)
Filo | Mollusca |
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Subfilo | Crustacea |
Class | Polychaeta |
Cobertura temporal
Fecha Inicial / Fecha Final | 2019-06-01 / 2019-06-04 |
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Datos del proyecto
Development and application of innovative methodologies for the study of Benthic Boundary Layer. The benthic boundary layer (BBL) supports epibenthic, hyperbenthic and zooplanktonic, mostly macrofaunal, organisms with different degrees of mobility and bottom dependence. BBL species constitute a very important link in marine food webs as consumers of detritus particles and associate microbes, meiobenthos and plankton and as prey for demersal fish and epibenthic crustaceans, many of which are commercially important. Nevertheless, the significance of this particular macrofauna is underestimated, especially in studies of benthic-pelagic coupling related to energy fluxes and also in holistic approaches of the marine ecosystem, mainly due to the difficulties in accessibility of this habitat. A research team of IMBBC has developed new sampling gears for the study of BBL habitat focused mainly on the sampling of macrofauna as well as the simultaneous measurement of relevant physical and biogeochemical parametres. These methodologies will contribute towards a better understanding of the role of BBL biodiversity with respect to nutrient regeneration, carbon cycling and energy transfer to higher trophic levels.
Título | MOdern UNifying Trends in marine biology |
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Identificador | PA (Partnership Agreement for the Development Framework) 2014-2020: 5002470 |
Fuentes de Financiación | EPAnEK 2014-2020, Operational Programme, Competitiveness, Entrepreneurship, Innovation. |
Descripción del área de estudio | The present study was conducted in the continental shelf of Heraklion Bay in depths from 50 to 200 metres. |
Descripción del diseño | One field survey was conducted on the continental shelf of Heraklion Bay. Sampling was carried out in one transect of three stations (St.1, St. 2, St. 3) at depths of 50,100 and 200 m. At each station: -the physical properties of the water column (temperature, salinity, photosynthetically active radiation (PAR)) were measured by means of a Sea-Bird Electronics (SBE-19) CTD system - water samples were collected by using Niskin bottles (5L) within 0.5 m above the seabed and a relatively new bottom water sampling method (Dounas, 2006) for the determination of chlorophyll a (Chl a), phaeopigments (Phaeo), particulate organic carbon (POC) concentrations. Samples were filtered through Whatman GF/F glass fibre filters on board, frozen immediately and stored at 20oC and analysed upon return to the laboratory. - one surface sediment sample (0-1 cm) was taken by using Smith McIntyre grab (0.10m2, sampling surface) for grain size analysis performed according to Buchanan (1984) and for the determination of Chl-a, phaeopigments and POC concentrations and stored at 20oC for subsequent laboratory analysis. Chloroplastic pigments concentrations in both sediment and water column samples were determined according to the fluorometric method of Yentsch and Menzel (1963), Lorenzen and Jeffrey (1980), using a Turner 112 fluorometer. POC measurements were determined according to the method of Hedges and Stern (1984), using a Perkin Elmer CHN 2400 analyzer. -three tows were carried out by the hyperbenthic sledge modified in the framework of MOUNT project. Hyperbenthic samples were collected during daylight hours. -five sediment samples were taken using a Smith McIntyre grab (0.10 m2). -five plankton samples were taken by means of a WP2 plankton net (0.5 mm mesh size) from a depth ranging from ~3 m above the seabed throughout the water column to the water surface. Biological samples were preserved in 90% alcohol on board immediately after collection and sorted under a dissecting microscope upon return to the laboratory. |
Personas asociadas al proyecto:
Métodos de muestreo
1.the physical properties of the water column were measured by means of a Sea-Bird Electronics (SBE-25) CTD system 2.water samples were collected by using Niskin bottles (5L) and by using a new bottom water sampling method (Dounas, 2006) 3.surface sediment samples (0-1 cm) were taken by using Smith McIntyre grab (0.10m2, sampling surface) 4. hyperbenthic samples were carried out by the hyperbenthic sledge modified in the framework of MOUNT project 5.endobenthic samples were taken by using a Smith McIntyre grab (0.10 m2) 6.macroplanktonic samples were taken by means of a WP2 plankton net (0.5 mm mesh size)
Área de Estudio | One field survey (1-4 June 2019) was conducted on the continental shelf of Heraklion Bay. Sampling was carried out in one transect of three stations (St.1, St. 2, St. 3) at depths of 50,100 and 200 m. |
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Control de Calidad | Taxonomy mapped according to WoRMS and locations according to Marine Regions |
Descripción de la metodología paso a paso:
- Sampling was carried out in one transect of three stations at depths of 50,100 and 200 m. At each station: -the physical properties of the water column (temperature, salinity, photosynthetically active radiation (PAR)) were measured by means of a Sea-Bird Electronics (SBE-19) CTD system - water samples were collected by using Niskin bottles (5L) within 0.5 m above the seabed and a relatively new bottom water sampling method (Dounas, 2006) for the determination of chlorophyll a (Chl a), phaeopigments (Phaeo), particulate organic carbon (POC) concentrations. Samples were filtered through Whatman GF/F glass fibre filters on board, frozen immediately and stored at 20oC and analysed upon return to the laboratory. - one surface sediment sample (0-1 cm) was taken by using Smith McIntyre grab (0.10m2, sampling surface) for grain size analysis performed according to Buchanan (1984) and for the determination of Chl-a, phaeopigments and POC concentrations and stored at 20oC for subsequent laboratory analysis. Chloroplastic pigments concentrations in both sediment and water column samples were determined according to the fluorometric method of Yentsch and Menzel (1963), Lorenzen and Jeffrey (1980), using a Turner 112 fluorometer. POC measurements were determined according to the method of Hedges and Stern (1984), using a Perkin Elmer CHN 2400 analyzer. -three tows were carried out by the hyperbenthic sledge modified in the framework of MOUNT project. Hyperbenthic samples were collected during daylight hours. -five sediment samples were taken using a Smith McIntyre grab (0.10 m2). -five plankton samples were taken by means of a WP2 plankton net (0.5 mm mesh size) from a depth ranging from ~3 m above the seabed throughout the water column to the water surface. Biological samples were preserved in 90% alcohol on board immediately after collection and sorted under a dissecting microscope upon return to the laboratory.
Metadatos adicionales
Identificadores alternativos | http://192.135.166.161/resource?r=mount |
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