Images of histological sections of oocytes for the bivalves Astarte crenata and Bathyarca glacialis from the Western Barents Sea under ambient and near-future climate change conditions.

Images of histological sections of oocytes to quantify the interactive effects of ocean warming and ocean acidification based on near-future climate change projections on oocyte size frequency distributions of benthic invertebrates (the bivalves Astarte crenata and Bathyarca glacialis) from the West...

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Bibliographic Details
Main Authors: Reed, Adam, Godbold, Jasmin, Solan, Martin, Grange, Laura
Format: Dataset
Language:English
Published: NERC EDS UK Polar Data Centre 2021
Subjects:
"EARTH SCIENCE","BIOSPHERE","ECOLOGICAL DYNAMICS","SPECIES/POPULATION INTERACTIONS","SPECIES LIFE HISTORY"
"EARTH SCIENCE","BIOLOGICAL CLASSIFICATION","ANIMALS/INVERTEBRATES"
dynamic energy budget
functional response
life history
metabolic plasticity
oogenesis
Arctic
Arctic Ocean
Barents Sea
Toledo
Olympus
Climate change
Ocean acidification
Sea ice
Online Access:https://dx.doi.org/10.5285/04766a75-502c-4431-b771-107326a8585c
https://data.bas.ac.uk/full-record.php?id=GB/NERC/BAS/PDC/01564
Description
Summary:Images of histological sections of oocytes to quantify the interactive effects of ocean warming and ocean acidification based on near-future climate change projections on oocyte size frequency distributions of benthic invertebrates (the bivalves Astarte crenata and Bathyarca glacialis) from the Western Barents Sea. Supported by The Changing Arctic Ocean Seafloor (ChAOS) - how changing sea ice conditions impact biological communities, biogeochemical processes and ecosystems project (NE/N015894/1 and NE/P006426/1, 2017-2021), Natural Environment Research Council (NERC) in the UK. : Specimens were collected from each of 1 station in 2017 (B13) and 2 stations in 2018 (B16 and B17) during two consecutive cruises (RRS James Clark Ross: JR16006, 30th June to 8th August 2017; JR17007: 10th July to 5th August, 2018) following a transect along the 30°E meridian. At each station similar-sized specimens of the infaunal bivalves Astarte crenata and Bathyarca glacialis were obtained by Agassiz trawl. Surficial sediment < 10 cm deep was collected using SMBA box cores, sieved to remove macrofauna (500 µm mesh), and homogenised by stirring. Both infaunal bivalves and sediment were maintained under aerated seawater and returned to the Biodiversity and Ecosystem Futures Facility, University of Southampton at ambient temperature (1.5 + 1°C). Ten centimetres of homogenised sediment were transferred to transparent acrylic aquaria (internal dimensions, LWH: 20 x 20 x 34 cm) and overlain with ~8 L (20cm depth) surface seawater (salinity, ~34). Aquaria were maintained in the dark at ambient conditions (1-2 °C and ~400 ppm [CO2]), and randomly distributed between two insulated fibreglass seawater baths (LWH: 1.2 x 1.2 x 0.8m, Tanks Direct, UK). Three B. glacialis were introduced to each of twelve aquaria (n = 36; ambient 18, future 18) and six A.crenata were introduced to each of ten aquaria (n = 60; 30 ambient, 30 future). After a 30-day acclimation period to aquarium conditions, temperature and [CO2] were manually adjusted (1 °C and ~100 ppm CO2 week -1) to achieve near-future treatment conditions (3-5 °C and ~550 ppm [CO2]). We periodically measured pH, temperature and salinity and total alkalinity. The bivalves were fed ad libitum three time per week (100 ml cultured live Isochrysis sp., Tetraselmis sp., and Phaeodactylum sp.), and overlying water exchanged weekly. Experiments were run for 120 days (B. glacialis, 21//11/2017-20/03/2018) or 135 days (A. crenata, 08/10/2018-19/02/2019) after which animals were removed and fixed in 4 neutral buffered formaldehyde. Oocyte images: Images of stained slides of histological sections from individual females were captured using a Nikon D5000 digital SLR camera mounted on an Olympus (BH-2) stereomicroscope and analysed using ImageJ v 1.48. Slides were photographed at X10 magnification. Replicate photographs were taken to ensure 100 unique oocytes were measured for each female. Composite images were generated for easy analysis wherever possible. Full descriptions and additional information provided in Reed et al. 2021 Frontiers in Marine Science in main manuscript and supplementary information. : Resolution: Biometric measurements (i.e., shell length, shell height and tumidity (width) to two decimal places. Wet weight to four decimal places. Oocyte Equivalent Circular Diameter to two decimal places. Instrumentation: Mettler-Toledo InLab Expert Pro temperature-pH combination electrode Mettler-Toledo InLab 737 IP67 temperature-conductivity combination electrode Digital vernier calliper Balance (+/-0.000g) Rotary microtome Nikon D5000 digital SLR camera Olympus BHS (BH-2) stereomicroscope : Standard protocols were followed and data entry double checked by independent person.

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