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Sediment was collected with an MC-800 multicorer aborad the R/V Oceanus (expedition 1703A) approximately 0-300 km off the coast of San Francisco, CA, USA. Cores were stored at 4C until extrusion and sectioning within 24h of collection. Cores were sectioned into 2.5-5cm vertical horizons, and approximately 2g of sediment were sampled from each horizon with a cut-off syringe, flash frozen in liquid nitrogen, and stored at -80C until extraction of nucleic acids. DNA was extracted with an RNeasy PowerSoil DNA elution kit (Qiagen, cat. no 12867-25) in combination with an RNeasy PowerSoil Total RNA kit (Qiagen, cat. no 12866-25). The manufacturer's protocol was modified to include a bead-beating step of 5.5 m/s for 2x45s with a FastPrep-24 instrument. DNA and RNA were eluted in 100 microliters of DNAse and RNAse-free water or 1xTE and stored at -80C. Total RNA was treated with DNAse (Thermo Fisher Scientific,cat. no AM1907). Three DNA samples were additionally processed for long-read sequencing by size-selection with the BluePippin instrument targeting the size range of 10-50kb and a library was prepared for sequencing with the 10x Genomics Chromium system according to manufacturer's protocol and described in Bishara et al. (2018, https://doi.org/10.1038/nbt.4266). Chromium libraries were sequenced with 2 x 151bp sequencing on an HiSeq 4000 instrument (Illumina). All other samples were processed by the Joint Genome Institute (Department of Energy). DNA was sheared to approximately 300bp using a Covaris LE220 ultrasonicator and size selected with SPRI beads and libraries prepared and barcoded using Kapa Biosystems library preparation kit. Total RNA was treated with Ribo-Zero rRNA removal kit (Illumina) and cDNA libraries generated using the Illumina Truseq Stranded mRNA Library Prep kit. The rRNA depleted RNA was fragmented and reversed transcribed using random hexamers and SSII (Invitrogen) followed by second strand synthesis. The fragmented cDNA was treated with end-pair, A-tailing, adapter ligation, and 10 cycles of PCR. DNA and cDNA were sequenced with 2 x 151bp sequencing on a Nova Seq S4 (Illumina) instrument.
BCO-DMO Processing: - replaced "na" with "nd" (no data)
General term for a laboratory instrument used for deciphering the order of bases in a strand of DNA. Sanger sequencers detect fluorescence from different dyes that are used to identify the A, C, G, and T extension reactions. Contemporary or Pyrosequencer methods are based on detecting the activity of DNA polymerase (a DNA synthesizing enzyme) with another chemoluminescent enzyme. Essentially, the method allows sequencing of a single strand of DNA by synthesizing the complementary strand along it, one base pair at a time, and detecting which base was actually added at each step.
provided real-time collection of depth, temperature, salinity
Conductivity, Temperature, Depth (CTD) sensor package from SeaBird Electronics, no specific unit identified. This instrument designation is used when specific make and model are not known. See also other SeaBird instruments listed under CTD. More information from Sea-Bird Electronics.
The Multi Corer is a benthic coring device used to collect multiple, simultaneous, undisturbed sediment/water samples from the seafloor. Multiple coring tubes with varying sampling capacity depending on tube dimensions are mounted in a frame designed to sample the deep ocean seafloor. For more information, see Barnett et al. (1984) in Oceanologica Acta, 7, pp. 399-408.
An automated DNA size selection instrument, with pulsed-field electrophoresis for resolving and collecting high molecular weight DNA. The instrument is used to automatically extract DNA fragments of a user selected size for downstream technologies such as miRNA isolation, DNA sequencing, RNA-seq, genotyping, DNA sequencing, ChIP-seq, and Long-read sequencing. The instrument uses electrophoresis along with laser detection or other imaging technology to determine when to start collecting DNA based on size ranges entered by the user. Once the DNA is no longer in the desired size range, collection ceases. The instrument has electrophoresis voltage options: 25V, 100V or 150V constant, or 100V pulsed field. The optical detection wavelength is 470 nm excitation, and 525 nm emission. The instrument can run up to 5 samples/gel cassettes at a time, with no possibility of cross contamination.
BioProject accession
BioSample accession
SRA run accession
Hyperlink to SRA run
SRA study accession
SRA title
Sequence library type
Source of nucleic acids
Library selection
Library layout
Sequencing platform
Sequencer model
Sampling design
Depth from sea level surface
Depth from seafloor
Sampling latitude
Sampling longitude
Date sample collected; format: YYYY-MM-DD
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