Microbiome profiling of bacterioplankton communities on sponge excurrent water, coral exudate water, and surface reef water.
Project
| Contributors | Affiliation | Role |
|---|---|---|
| Apprill, Amy | Woods Hole Oceanographic Institution (WHOI) | Co-Principal Investigator |
| Easson, Cole G. | Middle Tennessee State University | Co-Principal Investigator |
| Fiore, Cara L. | Appalachian State University | Co-Principal Investigator, Contact |
| Reigel, Alicia M. | Appalachian State University | Scientist |
| Fortier, Katrina | Appalachian State University | Student |
| Moore, Danielle | Appalachian State University | Technician |
| Soenen, Karen | Woods Hole Oceanographic Institution (WHOI BCO-DMO) | BCO-DMO Data Manager |
Abstract
Seawater sampled from the incubation ‘soup’ or bottles was used for multiple nutrient analyses and DNA extraction.
The rest of the seawater was filtered through an Omnipore 0.2 um filter using a peristaltic pump and acid and milliQ water rinsed Pharmed BP tubing and Teflon filter holders. The filter was stored at -80C until DNA extraction.
The NCBI dataset is the microbiome profiling data of the incubation experiment. These are the reads of 16S rRNA genes for each sample in the incubation experiment. Bottle incubations were set up as described in the methods for dataset 963872. The seawater from the bottles were filtered at T0 and at T48 and the filters were used for DNA extraction, amplification of the v4 region of the 16S rRNA gene, and Illumina sequencing. Additional details available through the NCBI accession link.
DNA from the Omnipore filters was extracted using a commercial kit and the 16S rRNA gene was amplified using the modified earth microbiome primer set for the V4 region (515F and 806R, Apprill et al. 2015). PCRs were sent to Middle Tennessee State University for library construction and sequencing on an Illumina MiSeq, producing FASTQ files as output.
*Added sampling date to dataset
| File |
|---|
964182_v1_ncbi.csv (Comma Separated Values (.csv), 54.15 KB) MD5:2a3b2a60824d28a21e5b850328e7f272 Primary data file for dataset ID 964182, version 1 |
Relationship Description: Incubation experiment.
| Parameter | Description | Units |
| Bioproject_Accession | NCBI Bioproject accession ID | unitless |
| Biosample_accession | NCBI Biosample accession ID | unitless |
| Sample_Name | Submitter sample name | unitless |
| SRA_run_ID | NCBI SRA run accession ID | unitless |
| SRA_run_link | Link to SRA data on NCBI | unitless |
| SPUID | SPUID (Submitter Provided Unique Identifier), a unique identifier assigned by the submitter to a sample in the NCBI BioSample database | unitless |
| Organism | Biological entity | unitless |
| Tax_ID | Unique numerical identifier assigned by unique numerical identifier assigned by the NCBI Taxonomy database to each organism or taxonase to each organism or taxon | unitless |
| library_ID | Unique identifier for the sequencing library (can be the sample name repeated). | unitless |
| SRA_study_ID | NCBI study accession ID | unitless |
| SRA_title | Title of SRA run | unitless |
| library_strategy | Sequencing library strategy | unitless |
| library_source | Source of sequencing library | unitless |
| library_selection | Selection used for sequencing library | unitless |
| library_layout | single or paired end sequencing reads | unitless |
| platform | Sequencing platform manufacturer | unitless |
| instrument_model | Sequencer model | unitless |
| design_description | Description explaining how this library was prepared and sequenced | unitless |
| filetype | File type | unitless |
| filename | Forward reads file name | unitless |
| filetype2 | File type | unitless |
| filename2 | Reverse reads file name | unitless |
| depth | Sampling depth | meters (m) |
| latitude | Sampling latitude, south is negative | decimal degrees |
| longitude | Sampling longitude, west is negative | decimal degrees |
| sample_date | Sample date |
| Dataset-specific Instrument Name | Illumina MiSeq |
| Generic Instrument Name | Automated DNA Sequencer |
| Generic Instrument Description | A DNA sequencer is an instrument that determines the order of deoxynucleotides in deoxyribonucleic acid sequences. |
Collaborative Research: The Influence of Sponge Holobiont Metabolism on Coral Reef Dissolved Organic Matter and Reef Microorganisms (Sponge Holobiont DOM)
NSF Award Abstract:
The seawater around coral reefs is typically low in nutrients, yet coral reefs are teeming with life and are often compared to oases in a desert. Life exists in these 'marine deserts' in large part, due to symbiotic associations between single-celled microbes and invertebrates such as corals and sponges. The concentration and type of dissolved organic matter (DOM), a complex pool of organic nutrients such as amino acids, vitamins, and other diverse compounds, also affects the health of coral reefs. The composition of DOM on coral reefs is linked to both the composition of free-living microbes in the seawater and to the nutrition of filter-feeding organisms, such as corals and sponges. However, the factors that influence the composition of DOM on coral reefs and the consequences of how it changes are not well understood. Recent work suggests that sponges could have a significant impact on the composition of reef dissolved organic nutrients, depending on sponge species due to differences in filtration capacity and in their symbiotic microbial communities. This project characterizes how diverse sponge species process DOM on coral reefs and determines the impacts of this processing on the free-living microbial community. Seawater is collected from sponges (pre- and post- sponge filtration) on coral reefs in the relatively pristine region of Curacao, and incubation experiments measure the impact of sponge filtration on the growth of the free-living microbial community. The organic nutrients of seawater samples are analyzed using cutting-edge techniques to distinguish the types of nutrients that are processed by sponges. The incubation experiments, using free-living microbes collected from the coral reef, quantify the impact of sponge filtration on the growth and composition of this community. This project provides fundamental understanding of how sponges contribute to the base of the coral reef food web. As the human-driven impacts continue to alter the composition of organisms on reefs, this understanding is necessary to predict changes to reef microbial food webs and is thus essential for scientists, reef managers, and policy decision makers. This project trains undergraduate students and a postdoctoral scholar and contributes to undergraduate and K-12 education through development of sponge-centric lessons that focus on local U.S. east coast aquatic environments as well as coral reef ecosystems.
Sponges vary in their capacity to filter seawater and in their associated microbial communities, leading to diverse metabolic strategies that often coexist in one habitat. While it is well-established that sponges are important in processing dissolved organic matter (DOM), an important reservoir of reduced carbon compounds, and transferring this energy to benthic food webs, there has been limited work to understand the consequences of sponge processing on the composition of coral reef DOM and on pelagic food webs. Specifically, while studies have shown that exudates of corals and algae select for specific groups of picoplankton (autotrophic and heterotrophic, respectively), similar data for sponges are required to understand the multiple factors that shape the composition of DOM and of the picoplankton community on coral reefs. Thus, this project is aimed at addressing a major knowledge gap of the role of sponge-derived DOM (sponge exometabolome) in coral reef biogeochemistry. An in situ sampling design targeting prominent Caribbean sponges and picoplankton incubation experiments is coupled to address both the composition of sponge exometabolomes and delineate shifts in the picoplankton community derived from sponge exometabolomes. Molecular-level changes to seawater DOM by sponge processing and the impact of these changes on the overall coral reef DOM profile is assessed with two DOM analysis techniques: a commonly used fluorometry technique (fDOM analysis) and with high-resolution mass spectrometry (LC-MS/MS). Additionally, microbiome and functional gene profiling, growth metrics, and nutrient analyses are employed to assess changes in the picoplankton community in response to sponge exometabolomes. Advanced data analysis techniques then synthesize data generated by each approach to provide novel insight on a poorly uncharacterized biogeochemical pathway on coral reefs. The work outlined here represents entirely novel information on the impact of sponge metabolism on the composition of DOM, sheds light on biologically important molecules involved in benthic-pelagic coupling, and importantly, generates data using standardized methods, thus facilitating comparison to previous and future DOM datasets.
This award reflects NSF's statutory mission and has been deemed worthy of support through evaluation using the Foundation's intellectual merit and broader impacts review criteria.
| Funding Source | Award |
|---|---|
| NSF Division of Ocean Sciences (NSF OCE) | |
| NSF Division of Ocean Sciences (NSF OCE) |
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