Long-term monitoring of the phytoplankton at the SOMLIT-Astan Station in the Western English Channel from 2000 to present

Описание

Записи данных

Данные этого sampling event ресурса были опубликованы в виде Darwin Core Archive (DwC-A), который является стандартным форматом для обмена данными о биоразнообразии в виде набора из одной или нескольких таблиц. Основная таблица данных содержит 884 записей.

Также в наличии 2 таблиц с данными расширений. Записи расширений содержат дополнительную информацию об основной записи. Число записей в каждой таблице данных расширения показано ниже.

Данный экземпляр IPT архивирует данные и таким образом служит хранилищем данных. Данные и метаданные ресурсов доступны для скачивания в разделе Загрузки. В таблице версий перечислены другие версии ресурса, которые были доступны публично, что позволяет отслеживать изменения, внесенные в ресурс с течением времени.

Версии

В таблице ниже указаны только опубликованные версии ресурса, которые доступны для свободного скачивания.

Как оформить ссылку

Исследователи должны дать ссылку на эту работу следующим образом:

Rigaut-Jalabert F, Simon N, Hoebeke M (2019): Long-term monitoring of the phytoplankton at the SOMLIT-Astan Station in the Western English Channel from 2000 to present. v1. Dataset/Samplingevent. https://doi.org/10.21411/7g10-dr41

Права

Исследователи должны соблюдать следующие права:

Эта работа находится под лицензией Creative Commons Attribution Non Commercial (CC-BY-NC 4.0).

Регистрация в GBIF

Этот ресурс не был зарегистрирован в GBIF

Ключевые слова

Phytoplankton; Biodiversity; Samplingevent

Контакты

Fabienne Rigaut-Jalabert

• Metadata Provider ●
• Originator ●
• Point Of Contact

Engineer

Station Biologique de Roscoff - CNRS / Sorbonne Université

FR

fabienne.jalabert@sb-roscoff.fr

http://orcid.org/0000-0002-5311-658X

Nathalie Simon

• Originator

Associate professor

Station Biologique de Roscoff - CNRS / Sorbonne Université

FR

nathalie.simon@sb-roscoff.fr

http://orcid.org/0000-0001-6434-7861

Mark Hoebeke

• Originator

Engineer

Stataion Biologique de Roscoff - Sorbonne Université CNRS

FR

mark.hoebeke@sb-roscoff.fr

http://orcid.org/0000-0001-6311-9752

Географический охват

SOMLIT-Astan - http://marineregions.org/mrgid/5372

Таксономический охват

Phytoplankton identifications and quantifications are made under inverted light microscope (at maximum magnification x400). Flowcytometry allowed to determine and quantifiy functionnal groups of pico-, nano-phytoplankton, heterotrophic and autotrophic bacteria.

Временной охват

Методы сбора

Different types of phytoplankton samples are collected at each sampling date. For qualitative analysis, under microscope (species semi-quantitative occurrences), net samples are collected using a 20µm nylon mesh cone towed during 3 minutes in subsurface. For quantitative analysis, under microscope and with a flow cytometeter (species and fonctionnal groups abundances), seawater samples are collected at 1m depth using a 5 liters Niskin bottle. For flow cytometry an additionnal sample is collected at -60m depth.

Описание этапа методики:

1. Microphytoplankton - Species abundances Seawater samples are collected at 1m depth using a 5 liters Niskin bottle. From 2000 to 2015, one hundred to 250 mL subsamples are were fixed with acid Logol's solution iodine according to Sournia (1978) back to the lab and stored in dark conditions at room temperature until analysis. From 2016, 250mL subsamples are fixed immediately after sampling with acid Lugol's solution iodine and stored at 4°C until analysis. For analysis, a sub-sample of lugol preserved water was gently poured into a 50 mL composite settling chamber (HYDRO-BIOS, Kiel), according to the standard Utermöhl settlement method described in Sournia (1978). Quantitative analyses based on the examination of lugol preserved samples were performed between 15 days and up to 1 year after sampling. Cell counts for either the whole chamber, or half a chamber, were obtained after sedimentation, under an inverted light microscope at 400x magnification. Samples from 2000 to May 2003, June 2003 to August 2008, and September 2008 onwards were examined with an Olympus CK2, an Olympus IX71, and a Leica DMI 3000, respectively. This latter microscope was equipped with a SPOT Insight digital camera 2 Mpx (Diagnostics Instruments, Sterling Heights, MI). Abundance is expressed for each taxa in number of cells per liter Reference citation to method - Guilloux L., Rigaut-Jalabert F., Jouenne F., Ristori S., Viprey M., Not F., Vaulot, D & Simon, N. 2013. An annotated checklist of Marine Phytoplankton taxa at the SOMLIT : Astan time series off Roscoff (Western Channel, France) : data collected from 2000 to 2010. Cah.Biol.Mar. 54. -Edler L. & Elbrächter M. 2010. The Utermöhl method for quantitative phytoplankton analysis. In: Karlson B, C Cusack & E Bresnan (eds). Microscopic and molecular methods for quantitative phytoplankton analysis, pp. 13-20. UNESCO Publishing, Paris. - NF EN 15204 (2006-12-01). Qualité de l’eau – Norme guide pour le dénombrement du phytoplancton par microscopie inversée (méthode Utermöhl). AFNOR. 39p. - Sournia A. 1978. Phytoplankton manual. Monographs on Oceanographic Methodology, 6: 337.
2. Microphytoplankton - Species semi-quantitative occurrences For qualitative analyses, net samples were collected using a simple 20 μm nylon mesh cone (24 cm opening diameter, 80 cm long) towed during 3 minutes in subsurface. A fraction of the net sample was preserved with formalin acidified with acetic acid (formalin (40%HCHO): glacial acetic acid; 1:1, v/v). For net samples, taxa lists were established after examination of a few drops of live or fixed samples Under light microscopes. Three different microscopes were used: an Olympus BH2 (samples from 2000 to July 2001), an Olympus BX51 (samples from August 2001 onwards) equipped with a SPOT RT-slider digital camera (Diagnostics Instruments, Sterling Heights, MI) and an inverted microscope Leica DMI 3000. All taxa are listed and occurrence is expressed according to : 1- present / 2- numerous / 3- dominant Reference to citation method - Guilloux L., Rigaut-Jalabert F., Jouenne F., Ristori S., Viprey M., Not F., Vaulot, D & Simon, N. 2013. An annotated checklist of Marine Phytoplankton taxa at the SOMLIT : Astan time series off Roscoff (Western Channel, France) : data collected from 2000 to 2010. Cah.Biol.Mar. 54. - Sournia A. 1978. Phytoplankton manual. Monographs on Oceanographic Methodology, 6: 337.
3. Pico-, nano-phytoplankton, hetero- and autotrophic bacteria - Fonctionnal Groups abundances Seawater samples are collected at -1m and -60m at SOMLIT-Astan Station using a 5 liters Niskin bottle. From 2000 to june 2015, samples are fixed back to the lab. 1485µl subsamples are fixed in cryotubes containing 15µl of Glutaraldehyde 25% (0.25% final concentration). After 15 minutes of fixation at room temperature, tubes are flash frozen in liquid nitrogen and stored at -80°C until FCM analysis. From july 2015, samples are fixed onboard. Cryotubes containing 15µl of a mix of Glutaraldehyde 25% (0.25% final concentration) and Poloxamer 10% (0.01% final concentration) are prepared in the lab and transported in a labtop cooler. The cooler keeps the Glutaraldehyde drops frozen in cryotubes, avoiding manipulator’s exposition when opening. Immediately after subsampling directly from the Niskin bottle (silicone tube, flask), cryotubes are filled with 1485µl seawater. Fixation time at ambient temperature and dark is respected (minimum 15 minutes, and then tubes are stored in the labtop cooler for gentle frozen (-20°C). Back to the lab, samples are stored in a -80°C freezer until analysis. Abundances are expressed in number of cells per milliliter for each functionnal group. Fluorescence intensity are associated to the counts : red autofluorescence for chlorophyll, orange for phycoerythrine and green for heterotroph cells tagged with Sybr Green. Reference to citation method - Troussellier M, Courties C, Zettelmaier S. 1995. Flow cytometric analysis of coastal lagoon bacterioplankton and picophytoplankton: Fixation and storage effects. Est Coast Shelf Sci 40:621-633. - Marie D., Brussaard C., Partensky F. and Vaulot D. Flow cytometric analysis of phytoplankton, bacteria and viruses. 1999. In: Current Protocols in Cytometry. John Wiley & Sons, Inc. 11.11.1-11.11.15. - Marie, D., Rigaut-Jalabert, F. and Vaulot, D. (2014), An improved protocol for flow cytometry analysis of phytoplankton cultures and natural samples. Cytometry, 85: 962–968. doi: 10.1002/cyto.a.22517.

Библиографические ссылки

1. Guilloux L., Rigaut-Jalabert F., Jouenne F., Ristori S., Viprey M., Not F., Vaulot, D & Simon, N. 2013. An annotated checklist of Marine Phytoplankton taxa at the SOMLIT : Astan time series off Roscoff (Western Channel, France) : data collected from 2000 to 2010. Cah.Biol.Mar. 54.

Дополнительные метаданные