Viral abundance and productivity in the Southern Ocean - data collected from the BROKE-West voyage of the Aurora Australis, 2006

Samples were taken at 3 stations along leg 1. 9 depths were sampled at the 3 sites and depths were chosen based on the fluorescence maximum on the downcast of the CTD. Data acquisition Samples were collected at the 3 sites at 9 different depths. Depths included the bottom depth as well as 8 samples...

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Bibliographic Details
Other Authors: AADC (originator), AU/AADC > Australian Antarctic Data Centre, Australia (resourceProvider)
Format: Dataset
Language:unknown
Published: Australian Ocean Data Network
Subjects:
biota
oceans
BACTERIA/ARCHAEA
EARTH SCIENCE
BIOLOGICAL CLASSIFICATION
MICROALGAE
PLANTS
PLANKTON
BIOSPHERE
AQUATIC ECOSYSTEMS
viral abundance
Viral productivity
southern ocean
Date
Leg number
Latitude
Longitude
Subsample
Depth
Bottle Number
Viscosity
CTD &gt
Conductivity
Temperature
SHIPS
R/V AA &gt
R/V Aurora Australis
AMD/AU
CEOS
AMD
ACE/CRC
OCEAN &gt
CONTINENT &gt
ANTARCTICA
GEOGRAPHIC REGION &gt
POLAR
Southern Ocean
Antarc*
Antarctica
aurora australis
Online Access:https://researchdata.ands.org.au/viral-abundance-productivity-australis-2006/684846
https://data.aad.gov.au/metadata/records/BROKE-West_viralabundance
http://data.aad.gov.au/aadc/marine_science/bottle_data/index.cfm
https://secure3.aad.gov.au/proms/public/projects/report_project_public.cfm?project_no=2655
https://secure3.aad.gov.au/proms/public/projects/report_project_public.cfm?project_no=2679
http://data.aad.gov.au/aadc/metadata/citation.cfm?entry_id=BROKE-West_viralabundance
Description
Summary:Samples were taken at 3 stations along leg 1. 9 depths were sampled at the 3 sites and depths were chosen based on the fluorescence maximum on the downcast of the CTD. Data acquisition Samples were collected at the 3 sites at 9 different depths. Depths included the bottom depth as well as 8 samples in the top 200M. 50ml samples were collected from the niskin bottles attached to the CTD. 20ml was filtered through a 0.02 microlitre filter to remove the viruses and larger organisms from the sample. 1ml of this virus free water was then pipetted into individual cryovials. A further 1ml was then taken from the original seawater sample and was then passed through a 0.2 microlitre filter, which retained all the bacteria and algae. The 0.2 microlitre filter was then placed in the cryovial with the 1ml of virus free seawater. Samples were then fixed with glutaraldehyde (5 microlitre, 50% concentration) at hourly intervals for 4 hours. After fixation samples were placed in liquid nitrogen and later stored at -80 degrees C. All samples will be analysed using a flowcytometer. The fields in these datasets are: Date Leg number Latitude Longitude Subsample Depth (m) Bottle Number Viscosity (cP) This work was completed as part of ASAC projects 2655 and 2679 (ASAC_2655, ASAC_2679).

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