http://lod.bco-dmo.org/id/dataset/826583
eng; USA
utf8
dataset
Highest level of data collection, from a common set of sensors or instrumentation, usually within the same research project
Biological and Chemical Oceanography Data Management Office (BCO-DMO)
Unavailable
508-289-2009
WHOI MS#36
Woods Hole
MA
02543
USA
info@bco-dmo.org
http://www.bco-dmo.org
Monday - Friday 8:00am - 5:00pm
For questions regarding this resource, please contact BCO-DMO via the email address provided.
pointOfContact
2020-10-14
ISO 19115-2 Geographic Information - Metadata - Part 2: Extensions for Imagery and Gridded Data
ISO 19115-2:2009(E)
Sample and treatment information from NMR assays of metabolite experiments on Thalassiosira pseudonanna 1335 inoculated with three bacterial strains
2020-10-14
publication
2020-10-14
revision
Marine Biological Laboratory/Woods Hole Oceanographic Institution Library (MBLWHOI DLA)
2020-11-04
publication
https://doi.org/10.26008/1912/bco-dmo.826583.1
Arthur Edison
University of Georgia
principalInvestigator
Biological and Chemical Oceanography Data Management Office (BCO-DMO)
Unavailable
508-289-2009
WHOI MS#36
Woods Hole
MA
02543
USA
info@bco-dmo.org
http://www.bco-dmo.org
Monday - Friday 8:00am - 5:00pm
For questions regarding this resource, please contact BCO-DMO via the email address provided.
publisher
Cite this dataset as: Edison, A. (2020) Sample and treatment information from NMR assays of metabolite experiments on Thalassiosira pseudonanna 1335 inoculated with three bacterial strains. Biological and Chemical Oceanography Data Management Office (BCO-DMO). (Version 1) Version Date 2020-10-14 [if applicable, indicate subset used]. doi:10.26008/1912/bco-dmo.826583.1 [access date]
MetaboLights accessions: NMR samples Dataset Description: <p>The study examined the ability of bacteria to draw down exometabolites from the culture medium as detected by novel approaches using magnetic resonance (NMR) analysis. See related dataset on parallel experiments using mass spectrometry (MS).This dataset includes information about samples and treatments analyzed with NMR. Bacteria Ruegeria pomeroyi DSS-3, Stenotrophomonas sp. SKA14, and Polaribacter dokdonensis MED152 were collected 48 hours after individual inoculation into a diatom Thalassiosira psuedonana culture and resulting metabolites were analysed.</p>
<p>Raw data files are located at Metabolights, MetaboLights accession number MTBLS1544;<br />
<a href="https://www.ebi.ac.uk/metabolights/MTBLS1544/files" target="_blank">https://www.ebi.ac.uk/metabolights/MTBLS1544/files</a><br />
<a href="https://www.ebi.ac.uk/metabolights/MTBLS1544/samples" target="_blank">https://www.ebi.ac.uk/metabolights/MTBLS1544/samples</a></p> Methods and Sampling: <p>An axenic Thalassiosira pseudonana 1335 culture (National Center for Marine Algae) was grown in 500 ml of L1 +Si medium[1] in a 600 ml vented tissue culture flask at 18 °C under 16 h light at 160 µmol photons/m^2/s and 8 h dark. After the diatom cultures had been growing for 7 d, bacteria pre-grown in 1/2 YTSS medium at 30 °C (Ruegeria pomeroyi DSS-3 (treatment A) and Stenotrophomonas sp. SKA14 (treatment D)) or 1/10 YTSS medium at 25 °C (Polaribacter dokdonensis (treatment E)) were washed 5 times in sterile L1 medium and inoculated into the diatom cultures and glucose controls at ~10^6 (Stenotrophomonas sp. and P. dokdonensis) or ~10^7 (R. pomeroyi) cells/ml. 3 or 4 replicates were collected for each co-culture. Axenic T. pseudonana and unamended L1+Si medium were maintained and sampled alongside the co-cultures as controls (treatment X and C). Samples were collected after 48 h.</p>
<p>Microbial cells were removed from co-cultures by filtration through 0.2 µm pore-size filters. Uninoculated medium served as the blank. Metabolites in the 48 h samples were lyophilized, homogenized dry, reconstituted in dimethyl-sulfoxide-d6 (DMSO-d6), and re-homogenized. The supernatant was analyzed using two-dimensional HSQC-NMR using acquisition parameters modified from a Bruker hsqcetgpsisp2.2 pulse program (TopSpin V4.0.6).&nbsp;</p>
Funding provided by NSF Division of Integrative Organismal Systems (NSF IOS) Award Number: IOS-1656311 Award URL: http://www.nsf.gov/awardsearch/showAward.do?AwardNumber=1656311
Funding provided by Gordon and Betty Moore Foundation: Marine Microbiology Initiative (MMI) Award Number: GBMF5503 Award URL: https://www.moore.org/grant-detail?grantId=GBMF5503
completed
Arthur Edison
University of Georgia
Department of Biochemistry
Athens
GA
30602
USA
aedison@uga.edu
pointOfContact
asNeeded
Dataset Version: 1
Unknown
Source_Name
Organism
Organism_part
Treatment
Time_elapsed_hrs
Replicate
MetaboLights_accession_number
Bruker 800 MHz NEO with 1.7 mm cryoprobe
theme
None, User defined
sample identification
taxon
treatment
time_elapsed
replicate
accession number
featureType
BCO-DMO Standard Parameters
Nuclear Magnetic Resonance Spectrometers
instrument
BCO-DMO Standard Instruments
otherRestrictions
otherRestrictions
Access Constraints: none. Use Constraints: Please follow guidelines at: http://www.bco-dmo.org/terms-use Distribution liability: Under no circumstances shall BCO-DMO be liable for any direct, incidental, special, consequential, indirect, or punitive damages that result from the use of, or the inability to use, the materials in this data submission. If you are dissatisfied with any materials in this data submission your sole and exclusive remedy is to discontinue use.
Marine Microbiology Initiative
https://www.moore.org/initiative-strategy-detail?initiativeId=marine-microbiology-initiative
Marine Microbiology Initiative
A Gordon and Betty Moore Foundation Program.
Forging a new paradigm in marine microbial ecology:
Microbes in the ocean produce half of the oxygen on the planet and remove vast amounts of carbon dioxide, a greenhouse gas, from the atmosphere. Yet, we have known surprisingly little about these microscopic organisms. As we discover answers to some long-standing puzzles about the roles that marine microorganisms play in supporting the ocean’s food webs and driving global elemental cycles, we realized that we still need to learn much more about what these organisms do and how they do it—including how they evolved and contribute to our ocean's health and productivity.
The Marine Microbiology Initiative seeks to gain a comprehensive understanding of marine microbial communities, including their diversity, functions and behaviors; their ecological roles; and their origins and evolution. Our focus has been to enable researchers to uncover the principles that govern the interactions among microbes and that govern microbially mediated nutrient flow in the sea. To address these opportunities, we support leaders in the field through investigator awards, multidisciplinary team research projects, and efforts to create resources of broad use to the research community. We also support development of new instrumentation, tools, technologies and genetic approaches.
Through the efforts of many scientists from around the world, the initiative has been catalyzing new science through advances in methods and technology, and to reduce interdisciplinary barriers slowing progress. With our support, researchers are quantifying nutrient pools in the ocean, deciphering the genetic and biochemical bases of microbial metabolism, and understanding how microbes interact with one another. The initiative has five grant portfolios:
Individual investigator awards for current and emerging leaders in the field.
Multidisciplinary projects that support collaboration across disciplines.
New instrumentation, tools and technology that enable scientists to ask new questions in ways previously not possible.
Community resource efforts that fund the creation and sharing of data and the development of tools, methods and infrastructure of widespread utility.
Projects that advance genetic tools to enable development of experimental model systems in marine microbial ecology.
We also bring together scientists to discuss timely subjects and to facilitate scientific exchange.
Our path to marine microbial ecology was a confluence of new technology that could accelerate science and an opportunity to support a field that was not well funded relative to potential impact. Around the time we began this work in 2004, the life sciences were entering a new era of DNA sequencing and genomics, expanding possibilities for scientific research – including the nascent field of marine microbial ecology. Through conversations with pioneers inside and outside the field, an opportunity was identified: to apply these new sequencing tools to advance knowledge of marine microbial communities and reveal how they support and influence ocean systems.
After many years of success, we will wind down this effort and close the initiative in 2021. We will have invested more than $250 million over 17 years to deepen understanding of the diversity, ecological activities and evolution of marine microbial communities. Thanks to the work of hundreds of scientists and others involved with the initiative, the goals have been achieved and the field has been profoundly enriched; it is now positioned to address new scientific questions using innovative technologies and methods.
MMI
largerWorkCitation
program
Metabolic Currencies of the Ocean Carbon Cycle
https://www.bco-dmo.org/project/765521
Metabolic Currencies of the Ocean Carbon Cycle
<p><em>NSF Award Abstract:</em><br />
The roles of microbes in cycling carbon and nutrients in the ocean - the largest biological system on Earth - were initially described about 40 years ago. Now, it is known that half of Earth's primary production is carried out by marine phytoplankton, and half of that is recycled within weeks by marine bacteria. This proposal is a collaboration between microbiologists and chemists to identify the specific compounds that pass between phytoplankton and bacteria in surface ocean waters. Identifying the key chemicals of the ocean's microbial food web will provide insights into how the marine carbon cycle is regulated, generate data to improve ocean carbon models, and train new scientists at the interface of microbiology and chemistry. Hands-on learning opportunities in microbial ecology will be provided for high school students, both in the classroom and in marine ecosystems of the Georgia coast.</p>
<p>Phytoplankton metabolites that sustain the flow of carbon between microbial autotrophs and heterotrophs in the surface ocean carbon cycle will be identified in this project. A matrix of model systems consisting of bacteria-phytoplankton co-cultures will be used as biological assays for key metabolites based on expression patterns of bacterial transporter genes. The chemical identity of candidate metabolites and evaluation of their potential ecological role will be carried out by exometabolomic analysis of co-cultures with bacterial transporter mutants. Both advanced mass spectrometry and NMR will be used for metabolomics analysis, taking advantage of the sensitivity and compound identification strengths of each. The distribution of candidate metabolites in the ocean microbiome and other microbial systems will be characterized by mining environmental sequence datasets for orthologous transporter genes. This project represents a novel approach to identifying metabolites important in microbiome function, compounds often difficult to address with standard chemical approaches because of their low concentrations and high biological demand.</p>
Metabolic Currencies
largerWorkCitation
project
Assessing the Movement of Carbon Currencies Between Marine Microbes
https://www.bco-dmo.org/project/828305
Assessing the Movement of Carbon Currencies Between Marine Microbes
<p>In support of using advanced analytical instrumentation and protein characterization tools to measure the flux of nutrients exchanged between marine microbes.</p>
Carbon Currencies Microbes
largerWorkCitation
project
eng; USA
biota
oceans
2018-01-01
2018-12-31
Laboratory cultures
0
BCO-DMO catalogue of parameters from Sample and treatment information from NMR assays of metabolite experiments on Thalassiosira pseudonanna 1335 inoculated with three bacterial strains
Biological and Chemical Oceanography Data Management Office (BCO-DMO)
Unavailable
508-289-2009
WHOI MS#36
Woods Hole
MA
02543
USA
info@bco-dmo.org
http://www.bco-dmo.org
Monday - Friday 8:00am - 5:00pm
For questions regarding this resource, please contact BCO-DMO via the email address provided.
pointOfContact
http://lod.bco-dmo.org/id/dataset-parameter/826605.rdf
Name: Source_Name
Units: unitless
Description: sample name
http://lod.bco-dmo.org/id/dataset-parameter/826606.rdf
Name: Organism
Units: unitless
Description: identification of organism sampled
http://lod.bco-dmo.org/id/dataset-parameter/826607.rdf
Name: Organism_part
Units: unitless
Description: description of the part of the organism sampled
http://lod.bco-dmo.org/id/dataset-parameter/826608.rdf
Name: Treatment
Units: unitless
Description: treatment type
http://lod.bco-dmo.org/id/dataset-parameter/826609.rdf
Name: Time_elapsed_hrs
Units: hours
Description: time of sample collection
http://lod.bco-dmo.org/id/dataset-parameter/826610.rdf
Name: Replicate
Units: unitless
Description: replicate number
http://lod.bco-dmo.org/id/dataset-parameter/826611.rdf
Name: MetaboLights_accession_number
Units: unitless
Description: accession number for data access at Metabolights
GB/NERC/BODC > British Oceanographic Data Centre, Natural Environment Research Council, United Kingdom
Biological and Chemical Oceanography Data Management Office (BCO-DMO)
Unavailable
508-289-2009
WHOI MS#36
Woods Hole
MA
02543
USA
info@bco-dmo.org
http://www.bco-dmo.org
Monday - Friday 8:00am - 5:00pm
For questions regarding this resource, please contact BCO-DMO via the email address provided.
pointOfContact
1978
https://darchive.mblwhoilibrary.org/bitstream/1912/26366/1/dataset-826583_diatom-matrix-nmr__v1.tsv
download
https://doi.org/10.26008/1912/bco-dmo.826583.1
download
onLine
dataset
<p>An axenic Thalassiosira pseudonana 1335 culture (National Center for Marine Algae) was grown in 500 ml of L1 +Si medium[1] in a 600 ml vented tissue culture flask at 18 °C under 16 h light at 160 µmol photons/m^2/s and 8 h dark. After the diatom cultures had been growing for 7 d, bacteria pre-grown in 1/2 YTSS medium at 30 °C (Ruegeria pomeroyi DSS-3 (treatment A) and Stenotrophomonas sp. SKA14 (treatment D)) or 1/10 YTSS medium at 25 °C (Polaribacter dokdonensis (treatment E)) were washed 5 times in sterile L1 medium and inoculated into the diatom cultures and glucose controls at ~10^6 (Stenotrophomonas sp. and P. dokdonensis) or ~10^7 (R. pomeroyi) cells/ml. 3 or 4 replicates were collected for each co-culture. Axenic T. pseudonana and unamended L1+Si medium were maintained and sampled alongside the co-cultures as controls (treatment X and C). Samples were collected after 48 h.</p>
<p>Microbial cells were removed from co-cultures by filtration through 0.2 µm pore-size filters. Uninoculated medium served as the blank. Metabolites in the 48 h samples were lyophilized, homogenized dry, reconstituted in dimethyl-sulfoxide-d6 (DMSO-d6), and re-homogenized. The supernatant was analyzed using two-dimensional HSQC-NMR using acquisition parameters modified from a Bruker hsqcetgpsisp2.2 pulse program (TopSpin V4.0.6).&nbsp;</p>
Specified by the Principal Investigator(s)
<p><strong>BCO-DMO Processing Notes:</strong><br />
- data submitted in Excel file "MTBLS1544 for BCODMO.xlsx" sheet "Sheet1" extracted to csv<br />
- added conventional header with dataset name, PI name, version date<br />
-&nbsp;modified parameter names to conform with BCO-DMO naming conventions</p>
Specified by the Principal Investigator(s)
asNeeded
7.x-1.1
Biological and Chemical Oceanography Data Management Office (BCO-DMO)
Unavailable
508-289-2009
WHOI MS#36
Woods Hole
MA
02543
USA
info@bco-dmo.org
http://www.bco-dmo.org
Monday - Friday 8:00am - 5:00pm
For questions regarding this resource, please contact BCO-DMO via the email address provided.
pointOfContact
Bruker 800 MHz NEO with 1.7 mm cryoprobe
Bruker 800 MHz NEO with 1.7 mm cryoprobe
PI Supplied Instrument Name: Bruker 800 MHz NEO with 1.7 mm cryoprobe Instrument Name: Nuclear Magnetic Resonance Spectrometers Instrument Short Name:NMR Instrument Description: Instruments that identify and quantify magnetically active chemical entities by subjecting a sample to orthogonal magnetic and electrical fields. Community Standard Description: http://vocab.nerc.ac.uk/collection/L05/current/LAB18/