Dataset: qPCR data for archaeal amoA ecotypes
Deployment: KM1128

Abundance of ammonia monooxygenase subunit A (amoA) genes determined using TaqMan qPCR.

Principal Investigator:

Alyson E. Santoro (University of California-Santa Barbara, UCSB)

BCO-DMO Data Manager:

Shannon Rauch (Woods Hole Oceanographic Institution, WHOI BCO-DMO)

Project:

Connecting Trace Elements and Metalloenzymes Across Marine Biogeochemical Gradients (GPc03) (MetZyme)

Gene content, gene expression, and physiology in mesopelagic ammonia-oxidizing archaea (AmoA Archaea)

Current State:

Final no updates expected

Version:

24 May 2016

Deployment Synonyms:

GPc03, MetZyme

Version Date:

2016-05-24

Data URL:

https://www.bco-dmo.org/dataset-deployment/647626/data

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Description

Abundance of ammonia monooxygenase subunit A (amoA) genes determined using TaqMan quantitative polymerase chain reaction (qPCR). Archaeal amoA genes were quantified using quantitative PCR using the assay described in Mosier and Francis 2011. Complete methods are described in Santoro et al., submitted.

Related references:
Mosier, A. C., and C. A. Francis. 2011. Determining the distribution of marine and coastal ammonia-oxidizing archaea and bacteria using a quantitative approach. Methods Enzymol. 486: 205-221. doi:10.1016/B978-0-12-381294-0.00009-2

Santoro, A.E., Saito, M.A., Goepfert, T.J., Lamborg, C.H., Dupont, C.L., G.R. DiTullio. Thaumarchaeal ecotype distributions across the equatorial Pacific and their potential roles in nitrification and flux attenuation. Submitted to Limnology & Oceanography, April 2016.

Methods & Sampling

Dataset acquisition description

Water samples were collected at discrete depths using either a standard 24-bottle rosette sampler equipped with an SBE9plus conductivity-temperature-depth (CTD) sensor package (SeaBird Electronics, Bellevue, WA) or a 12-bottle trace metal clean rosette equipped with an SBE19 CTD. Samples for nucleic acid extraction and qPCR were collected from the rosette in 2-4 L polycarbonate bottles. Cells were harvested by pressure filtration onto 25 mm diameter, 0.2 um pore-size polyethersulfone membrane filters (Supor-200, Pall Corporation, Port Washington, NY) housed in polypropylene filter holders (Whatman SwinLok, GE Healthcare, Pittsburgh, PA) using a peristaltic pump and silicone tubing. For DNA extraction and analysis, 1-4 L sample volumes were filtered depending on the biomass present at each station and depth, and the filters were flash frozen in liquid nitrogen in 2 mL gasketed bead beating tubes (Fisher Scientific).

Data Processing Description

Dataset Processing Description

Nucleic acids (DNA) were extracted as described previously (Santoro et al. 2010), with slight modifications. Briefly, cells on the filters were lysed directly in the bead beating tubes with sucrose-ethylene diamine tetraacetic acid (EDTA) lysis buffer (0.75 M sucrose, 20 mM EDTA, 400 mM NaCl, 50 mM Tris) and 1% sodium dodecyl sulfate (SDS). Filter samples were subject to three freeze-thaw cycles of 5 min in liquid nitrogen and 5 min in a 65 degree C water bath. Tubes were then agitated in a bead beating machine (Biospec) for 1.5 min, and proteinase K (Invitrogen) was added to a final concentration of 0.5 mg mL-1. Filters were incubated at 55 degrees C for approximately 4 h and the resulting lysates were purified with the DNeasy kit (Qiagen) using a slightly modified protocol (Santoro et al. 2010). The purified nucleic acids were eluted in 200 uL of DNase, RNase-free water (Gibco) and quantified using a fluorometer (Qubit and Quanti-T BR reagent, Invitrogen Molecular Probes).

All qPCR assays were conducted using group-specific assays for the thaumarchaeal amoA gene for 'shallow' water column ecotype A (WCA) and 'deep' water column ecotype B (WCB) (Mosier and Francis 2011) with TaqMan Environmental Mastermix (Life Technologies) chemistry on a CFX96 qPCR machine (Bio-Rad, Inc., Hercules, CA). Detection limits for TaqMan assays were 1 copy mL-1 or better. All samples were run in triplicate against a standard curve spanning approximately 101 - 105 templates, run in duplicate. Plasmids containing cloned inserts of the target gene (TOPO pCR4 vector, Invitrogen or pGem vector, Promega) were used as standards. Standards were linearized with the restriction enzyme NotI (New England Biolabs), purified (DNeasy, Qiagen), quantified by fluorometry (Quanti-T HS reagent, Invitrogen), and stored at -80 degrees C. Fresh standard dilutions were made from frozen stocks for each day of analysis. qPCR was carried out using the following thermal profile: 95 degreesC for 10 min, followed by 40 cycles of 95 degrees C for 30 s and 55 degrees C for 30 s. A minimum of three negative control qPCR reactions to which no DNA template was added were run with every assay.

Gene copies per qPCR reaction were converted to volumetric concentrations (i.e. copies mL-1 seawater) using the volume of seawater filtered, the DNA elution volume, and the volume of purified DNA used per reaction, and are reported as the mean of triplicate analyses.

BCO-DMO Processing:
- re-formatted date and time; added ISO date/time field;
- copied station, date, time, lon, and lat from separate spreadsheet into dataset.

More information about this dataset deployment

Funding

Award Number	Funding Source
OCE-1031271	NSF Division of Ocean Sciences
OCE-1260006	NSF Division of Ocean Sciences

Instruments

CTD Sea-Bird SBE 911plus

Supplied Name:

Supplied Description:

Instrument Type

Generic Name: CTD Sea-Bird SBE 911plus

Acronym: CTD SBE 911plus

Community Identifier: http://vocab.nerc.ac.uk/collection/L22/current/TOOL0058/

Generic Description:

The Sea-Bird SBE 911 plus is a type of CTD instrument package for continuous measurement of conductivity, temperature and pressure. The SBE 911 plus includes the SBE 9plus Underwater Unit and the SBE 11plus Deck Unit (for real-time readout using conductive wire) for deployment from a vessel. The combination of the SBE 9 plus and SBE 11 plus is called a SBE 911 plus. The SBE 9 plus uses Sea-Bird's standard modular temperature and conductivity sensors (SBE 3 plus and SBE 4). The SBE 9 plus CTD can be configured with up to eight auxiliary sensors to measure other parameters including dissolved oxygen, pH, turbidity, fluorescence, light (PAR), light transmission, etc.). more information from Sea-Bird Electronics

CTD Sea-Bird SEACAT 19

Supplied Name:

Supplied Description:

Instrument Type

Generic Name: CTD Sea-Bird SEACAT 19

Acronym: CTD SBE 19

Community Identifier: http://vocab.nerc.ac.uk/collection/L22/current/TOOL0042/

Generic Description:

The Sea-Bird SBE 19 SEACAT Recorder measures conductivity, temperature, and pressure (depth). The SEACAT is self-powered and self-contained and can be deployed in profiling or moored mode. The SBE 19 SEACAT was replaced in 2001 by the 19plus. more information from Sea-Bird Electronics

Thermal Cycler

Supplied Name:

Supplied Description:

Instrument Type

Generic Name: Thermal Cycler

Generic Description:

A thermal cycler or "thermocycler" is a general term for a type of laboratory apparatus, commonly used for performing polymerase chain reaction (PCR), that is capable of repeatedly altering and maintaining specific temperatures for defined periods of time. The device has a thermal block with holes where tubes with the PCR reaction mixtures can be inserted. The cycler then raises and lowers the temperature of the block in discrete, pre-programmed steps. They can also be used to facilitate other temperature-sensitive reactions, including restriction enzyme digestion or rapid diagnostics.

(adapted from http://serc.carleton.edu/microbelife/research_methods/genomics/pcr.html)

Trace Metal Bottle

Supplied Name:

Supplied Description:

Instrument Type

Generic Name: Trace Metal Bottle

Acronym: TM Bottle

Community Identifier: http://vocab.nerc.ac.uk/collection/L05/current/30/

Generic Description:

Trace metal (TM) clean rosette bottle used for collecting trace metal clean seawater samples.

Parameters

Supplied Name	Supplied description	Supplied Units	Standard Name
cruise	Cruise identifier.	unitless	cruise_id
cast	Cast number. TMR = Trace Metal Rosette.	unitless	cast
station	Station number.	unitless	station
lon	Longitude east.	decimal degrees	lon
lat	Latitude north.	decimal degrees	lat
date	Month, day, and year; local time.	mm/dd/YYYY	date
time_local	Time in hours and minutes; local time.	HHMM	time_local
ISO_DateTime_Local	Date and time formatted to the ISO8601 standard.	YYYY-mm-ddTHH:MM:SS.xx	ISO_DateTime_Local
depth	Sample depth.	meters (m)	depth
niskin	Niskin bottle number.	unitless	bot_Nis
vol_filtered	Volume of water filtered.	liters (L)	vol_filt
WCB	WCB amoA abundance. WCB = water column ‘B’; assay for the deep ecotype of ammonia-oxidizing archaea.	copies per milliliter (copies/mL)	no_bcodmo_term
WCB_stdev	Standard deviation of WCB.	copies per milliliter (copies/mL)	std_dev
WCA	WCA amoA abundance. WCA = water column ‘A’; assay for the shallow ecotype of ammonia-oxidizing archaea.	copies per milliliter (copies/mL)	no_bcodmo_term
WCA_stdev	Standard deviation of WCA.	copies per milliliter (copies/mL)	std_dev
AOA	Total AOA amoA genes (calculated from WCA + WCB).	copies per milliliter (copies/mL)	no_bcodmo_term
pcnt_WCB	Percent WCB; calculated as WCB/totalAOA.	percent (%)	no_bcodmo_term

Database

Contribute Data

Dataset: qPCR data for archaeal amoA ecotypes
Deployment: KM1128

Dataset acquisition description

Dataset Processing Description

Database

Contribute Data

Dataset: qPCR data for archaeal amoA ecotypesDeployment: KM1128

Dataset acquisition description

Dataset Processing Description

Dataset: qPCR data for archaeal amoA ecotypes
Deployment: KM1128