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OAS accession Detail for 0299424, meta_version: 2. Current meta_version is: 2
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Title: Morphometrics of black sea bass reared at contrasting pCO2 conditions in laboratory experiments conduced with embryos from adults collected in Long Island Sound in 2022 (NCEI Accession 0299424)
Abstract: This dataset contains biological, chemical, physical, and survey - biological data collected from 2022-05-20 to 2022-06-04. These data include Partial pressure of CO2, fish_len, pH, salinity, species, and water temperature. The instruments used to collect these data include Automated Larval Fish Rearing System, Camera, and Microscope - Optical. These data were collected by Hannes Baumann of University of Connecticut as part of the "Collaborative research: The genomic underpinnings of local adaptation despite gene flow along a coastal environmental cline (GenomAdapt)" and "Collaborative research: Understanding the effects of acidification and hypoxia within and across generations in a coastal marine fish (HYPOA)" projects. The Biological and Chemical Oceanography Data Management Office (BCO-DMO) submitted these data to NCEI on 2024-09-16.

The following is the text of the dataset description provided by BCO-DMO:

See "Related Datasets" section for other data from these same laboratory experiments published in results paper Zavell et al. (2024).

Methods and Sampling:
Spawning ripe black sea bass (BSB) were collected on May 20 th , 2022 via hook and line angling in Long Island Sound off Stonington Borough, CT (41.3359°N, 71.9059°W) and brought to the University of Connecticut seawater laboratory on the Avery Point campus (Groton, CT) for future strip-spawning.

Experimental Design:

Our experiment assessed the CO 2 sensitivity of embryos and early life stages of BSB at a single static temperature (22°C) and three p CO 2 conditions (~400, ~2200, ~4200 µatm). On May 23rd , 2022, we strip-spawned wild, running-ripe BSB (N female/male = 4/3) to produce viable embryos. Upon water-hardening a 5 ml sample of eggs was randomly allocated to a replicate 19-l rearing container held within one of nine recirculating systems within the Baumann labs automated larval rearing system (ALFiRiS).

For this experiment, three ALFiRiS systems were assigned each pCO2 treatment and received eight individual replicates. Replicate containers consisted of 750 ml plastic cups with 100 µm mesh bottoms, which were floated in larger 19-l containers. 19-l containers were fitted with four 150 µm mesh screens to allow for water transfer and each 750 ml rearing container received a gravity-fed flow of treatment water to maintain embryos in the water column (4-l hour -1). For the ambient and elevated treatments each replicate ALFiRiS tank received eight 750 ml rearing containers, while two of the extreme treatments received eight rearing containers the other received 16. Actual pCO2 values were measured by taking 300 ml filtered water samples from each tank every nine days for endpoint titrations. Tank temperature, pH, and total alkalinity values were used to calculate pCO2 using CO2SYS (V2.3, Lewis and Wallace 2021; available at https://www.ncei.noaa.gov/access/ocean-carbon-acidification-data-system/oceans/CO2SYS/co2rprt.html). Throughout the experiment pH was recorded once an hour and temperature were recorded every five minutes. Additionally, ammonia (ppm) was measured once a week while salinity was measured every nine days (psu).

At 22°C hatching occurred approximately 48 hours post fertilization (hpf). Immediately, following hatch four of the eight (or eight of sixteen for one tank) replicates were euthanized with an overdose of MS-222 and immediately fixed in cold (2-4°C) paraformaldehyde (PFA) in phosphate buffered saline (PBS). The remaining replicates were reared until 10 dph, upon which they were euthanized and fixed as previously described. For the first two dph larvae were fed greenwater (RGComplete, Reed Mariculture, Campbell CA, USA) ad libitum 3× a day. Starting on 1 dph larvae were fed live L-type rotifers (Reed Mariculture, Campbell CA, USA) ad libitum 3× a day.

Response Traits
* See "Related Datasets" section for access to hatching, survival and growth data.

We estimated percent hatch at the number of hatched larvae at 0 days post hatch (dph) divided by the sum of hatched larvae and unhatched embryos × 100. Since replicate containers which were reared to 10 dph were not sampled at 0 dph to determine percent hatch, the number of embryos was estimated as the average number of embryos from the nine extra sample allocations which was then multiplied by the ALFiRiS system average hatching success to estimate total larvae at 0 dph. Subsequently, percent survival was the number of surviving larvae at 10 dph divided by the estimated number of larvae at 0 dph × 100.

At both 0 and 10 dph we individually photographed each larvae using calibrated images (Nikon SMZ1000, Image-Pro-Premier V.9.3.3) to measure individual for total length (TL; mm) and body depth (BD; mm). 10 dph larvae were also measured for notochord length (NL; mm), eye diameter (ED; mm), and mandible length (ML; mm).

Length growth rates (GR, mm d -1) were calculated by dividing the difference between replicate TL means at 0 and 10 dph by 10.

Organism Identifier (LSID, Life Sciences Identifier)
Centropristis striata , urn:lsid:marinespecies.org:taxname:159348
Date received: 20240916
Start date: 20220520
End date: 20220604
Seanames:
West boundary: -72.01861
East boundary: -71.9059
North boundary: 41.3359
South boundary: 41.32361
Observation types: biological, chemical, physical, survey - biological
Instrument types: camera, microscope
Datatypes: INDIVIDUAL FISH EXAMINATION - LENGTH, partial pressure of carbon dioxide - water, pH, SALINITY, SPECIES IDENTIFICATION, WATER TEMPERATURE
Submitter:
Submitting institution: Biological and Chemical Oceanography Data Management Office
Collecting institutions: University of Connecticut
Contributing projects:
Platforms:
Number of observations:
Supplementary information:
Availability date:
Metadata version: 2
Keydate: 2024-11-29 15:42:35+00
Editdate: 2025-01-27 20:23:01+00