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            <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/dataset/762912.rdf" xlink:actuate="onRequest">Genetic accession numbers and sampling information for metaviromes collected during the R/V Thomas G. Thompson cruise TN-280 along Line P in the northeast Pacific Ocean in May of 2012</gmx:Anchor>
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            <gco:CharacterString>Cite this dataset as: Rocap, G., Carlson, M. (2019) Genetic accession numbers and sampling information for metaviromes collected during the R/V Thomas G. Thompson cruise TN-280 along Line P in the northeast Pacific Ocean in May of 2012. Biological and Chemical Oceanography Data Management Office (BCO-DMO). (Version 1) Version Date 2019-03-25 [if applicable, indicate subset used]. http://lod.bco-dmo.org/id/dataset/762912 [access date]</gco:CharacterString>
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        <gco:CharacterString>Dataset Description: This dataset contains genetic accession numbers and sampling information for metaviromes collected during the R/V Thomas G. Thompson cruise TN-280 along Line P in the northeast Pacific Ocean in May of 2012.  The accessions identified in this dataset are housed at the National Center for Biotechnology Information (NCBI) under BioProject PRJNA437470.   

The status of this page will be &amp;quot;Data not available yet&amp;quot; until the genetic accessions are publicly available at NCBI. Methods and Sampling: Samples were obtained from Stations P1 (48.58 N, 125.50 W), P4 (48.65 N, 126.67 W), P6 (48.74 N, 127.67 W) and P8 (48.82 N, 128.66 W) on cruise TN280 between May 17-20 2012.
Water from all samples was obtained from Niskin bottles on the CTD Rosette. Plankton were collected on a 2.0 μm pore-size filter (142 mm diameter polycarbonate) and a 0.2 μm pore-size filter (142 mm diameter Supor) following prefiltration through a 53 μm pore-size filter. 20L of the &amp;lt;0.2 μm filtrate was amended with iron chloride (1g L-1) and incubated for at least 1 hour at room temperature to flocculate viruses (John et al. 2011). Viral flocculates were filtered onto 0.6 μm polycarbonate filters and stored at 4C. The GenBank BioSample accession numbers are SAMN08663113- SAMN08663116.
Viruses were resuspended from filters by incubating them with 0.2M ascorbate-0.25M EDTA-Mg2-0.25M Tris-HCL for at least 24 hours with periodic shaking (John et al. 2011). Viral suspensions were incubated for 2 hours at room temperature with DNase 1 (100 U ml-1, Ambion) to remove contaminating extracellular DNA. Viral DNA was extracted using a MoBio PowerSoil Total RNA isolation kit with the DNA elution column accessory, according to the manufacturers instructions. To convert single stranded DNA (ssDNA) viruses to double stranded DNA (dsDNA), complementary strands were synthesized using a modified random priming-mediated sequence-independent single-primer amplification (RP-SISPA) method designed to generate quantitative whole genome shotgun libraries (Djikeng et al. 2008, Culley et al. 2010). Triplicate 20 μl reactions for each sample and a no template control containing 10 μl template (or water), 0.2mM dNTPs, 0.5 mM DTT, 1 μM FR26RV-N primer (5-GCCGGAGCTCTGCAGATATCNNNNNN -3), 1mM MgCl2, and 1X Klenow buffer were heated to 94 C for 3 minutes and snap cooled on ice. 2.5 U of Klenow Fragment, 3-5 exo- (New England Biolands) was added to each reaction then incubated at 37 C for 60 minutes followed by 75 C for 10 minutes. Reactions were pooled, cleaned with ethanol precipitation, and resuspended in T low-E (10mM Tris-HCl, 0.1 mM EDTA pH 8.0). 

To construct Illumina shotgun metagenome libraries, viral DNA was sheared to 800-1000 bp using a Covaris nebulizer and cleaned with AmPure XP beads. Viral metagenomes (viromes) were constructed using the Rubicon ThruPLEX-FD Kit, which uses qPCR to linearly amplify low concentration DNA templates. Libraries were sequenced on an Illumina HiSeq 2500 with 150 paired end reads at the Michigan State University Sequencing Center. FASTQ files of the raw sequence reads are deposited in the Sequence Read Archive under study SRP134205  and the individual file accession numbers SRR6819460-SRR6819463.

Virome reads were trimmed of adapter sequences and low quality regions and filtered to remove low quality reads with the Trimmomatic pipeline (Bolger et al., 2014). Sequences were de novo assembled into contigs by first using diginorm (Brown et al., 2012) followed by the velvet assembler (Zerbino and Birney, 2008) with k-mer length set at 25, 29, 33, 51 for P1, P4, P6, and P8 respectively. Assemblies have been deposited in the Whole Genome Shotgun archive under the accession numbers 
GeoMICS_DNAvirome_P1   PYID00000000
GeoMICS_DNAvirome_P4    PYIE00000000
GeoMICS_DNAvirome_P6    PYIF00000000
GeoMICS_DNAvirome_P8    PYIG00000000</gco:CharacterString>
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        <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/award/665011.rdf" xlink:title="OCE-1356779" xlink:actuate="onRequest">Funding provided by NSF Division of Ocean Sciences (NSF OCE) Award Number: OCE-1356779 Award URL: https://www.nsf.gov/awardsearch/show-award?AWD_ID=1356779</gmx:Anchor>
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&lt;p&gt;Overview: Viruses play critical roles in aquatic ecosystems. Phages infecting marine bacteria are abundant members of the plankton that contribute to cell mortality, structure population diversity and drive genome evolution though horizontal gene transfer. Viruses infecting eukaryotic phytoplankton have been demonstrated to induce both life cycle switching and programmed cell death in coccolithophorids and be significant agents of mortality in blooms of pelagophytes, haptophytes and raphidophytes. However, much less is known about viruses infecting one of the largest, most diverse and most productive groups of algae, the diatoms. Only thirteen diatom infecting viruses have been reported, and little is known about their mechanisms of infection, effects on host metabolism or diversity and dynamics in the field. This is a remarkable knowledge gap considering the ecological importance of the diatoms. Infection with a clonal virus on Pseudo-nitzschia multiseries can result in complete host lysis within 12-16 hours. The P. multiseries virus (PmDNAV) is a single stranded DNA virus with an icosahedral capsid of 50 nm. The PmDNAV infects the widest host range of any marine eukaryote-infecting virus, lysing other strains of P. multiseries, other species of Pseudo-nitzschia, and other genera of diatoms including many centric diatoms. With the recent completion of the genome of the host, P. multiseries, we now have a model system to investigate the response of the host to viral infection and the potential impacts of viruses on diatom mortality in the field. The objectives of this project are to:&lt;br /&gt;
1. isolate and characterize additional diatom viruses utilizing established methods, using a variety of host strains and field viral concentrate combinations&lt;br /&gt;
2. use RNA-Seq to determine the transcriptional profiles of three diatoms (P. multiseries, P. pungens and T. pseudonana) during the course of viral infection&lt;br /&gt;
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Viral and host genes whose expression is diagnostic of viral infection, will be identified by observing genomic responses to infection in culture. These genes, along with viruses assembled in the metaviromes, will be combined with eukaryotic metatranscriptomes already available from the same waters to assess virus activity in the field.&lt;/p&gt;
&lt;p&gt;Intellectual Merit: This project seeks to strengthen the model system initiated by the discovery of the Pseudo-nitzschia multiseries DNA virus. The host-virus transcriptomics will lay the groundwork for assessing the impact of viruses on diatom communities in the environment. In turn, the paired metaviromes and metatranscriptomes will reveal new questions about both diatom virus diversity and function that can then be further explored by controlled, culture-based experiments. This research will be the first extensive exploration of diatom virus ecology and function and will ultimately help further connect viruses and diatoms to global biogeochemical cycles, unravel complex organismal interactions, and inform ocean-related public health.&lt;/p&gt;</gco:CharacterString>
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Water from all samples was obtained from Niskin bottles on the CTD Rosette. Plankton were collected on a 2.0 μm pore-size filter (142 mm diameter polycarbonate) and a 0.2 μm pore-size filter (142 mm diameter Supor) following prefiltration through a 53 μm pore-size filter. 20L of the &amp;lt;0.2 μm filtrate was amended with iron chloride (1g L-1) and incubated for at least 1 hour at room temperature to flocculate viruses (John et al. 2011). Viral flocculates were filtered onto 0.6 μm polycarbonate filters and stored at 4C. The GenBank BioSample accession numbers are SAMN08663113- SAMN08663116.
Viruses were resuspended from filters by incubating them with 0.2M ascorbate-0.25M EDTA-Mg2-0.25M Tris-HCL for at least 24 hours with periodic shaking (John et al. 2011). Viral suspensions were incubated for 2 hours at room temperature with DNase 1 (100 U ml-1, Ambion) to remove contaminating extracellular DNA. Viral DNA was extracted using a MoBio PowerSoil Total RNA isolation kit with the DNA elution column accessory, according to the manufacturers instructions. To convert single stranded DNA (ssDNA) viruses to double stranded DNA (dsDNA), complementary strands were synthesized using a modified random priming-mediated sequence-independent single-primer amplification (RP-SISPA) method designed to generate quantitative whole genome shotgun libraries (Djikeng et al. 2008, Culley et al. 2010). Triplicate 20 μl reactions for each sample and a no template control containing 10 μl template (or water), 0.2mM dNTPs, 0.5 mM DTT, 1 μM FR26RV-N primer (5-GCCGGAGCTCTGCAGATATCNNNNNN -3), 1mM MgCl2, and 1X Klenow buffer were heated to 94 C for 3 minutes and snap cooled on ice. 2.5 U of Klenow Fragment, 3-5 exo- (New England Biolands) was added to each reaction then incubated at 37 C for 60 minutes followed by 75 C for 10 minutes. Reactions were pooled, cleaned with ethanol precipitation, and resuspended in T low-E (10mM Tris-HCl, 0.1 mM EDTA pH 8.0). 

To construct Illumina shotgun metagenome libraries, viral DNA was sheared to 800-1000 bp using a Covaris nebulizer and cleaned with AmPure XP beads. Viral metagenomes (viromes) were constructed using the Rubicon ThruPLEX-FD Kit, which uses qPCR to linearly amplify low concentration DNA templates. Libraries were sequenced on an Illumina HiSeq 2500 with 150 paired end reads at the Michigan State University Sequencing Center. FASTQ files of the raw sequence reads are deposited in the Sequence Read Archive under study SRP134205  and the individual file accession numbers SRR6819460-SRR6819463.

Virome reads were trimmed of adapter sequences and low quality regions and filtered to remove low quality reads with the Trimmomatic pipeline (Bolger et al., 2014). Sequences were de novo assembled into contigs by first using diginorm (Brown et al., 2012) followed by the velvet assembler (Zerbino and Birney, 2008) with k-mer length set at 25, 29, 33, 51 for P1, P4, P6, and P8 respectively. Assemblies have been deposited in the Whole Genome Shotgun archive under the accession numbers 
GeoMICS_DNAvirome_P1   PYID00000000
GeoMICS_DNAvirome_P4    PYIE00000000
GeoMICS_DNAvirome_P6    PYIF00000000
GeoMICS_DNAvirome_P8    PYIG00000000</gco:CharacterString>
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&amp;lt;div&amp;gt;* added a conventional header with dataset name, PI name, version date&amp;lt;/div&amp;gt;

&amp;lt;div&amp;gt;* modified parameter names to conform with BCO-DMO naming conventions&amp;lt;/div&amp;gt;

&amp;lt;div&amp;gt;* Converted date to ISO 8601 format&amp;lt;/div&amp;gt;

&amp;lt;div&amp;gt;* parsed column with lat and lon into separate latitude and longitue columns in decimal degrees.&amp;lt;/div&amp;gt;

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