Dataset: BATS HPLC pigments

Name: HPLC and fluorometric derived phytoplankton pigment concentrations from seawater collected at the Bermuda Atlantic Time-series Study (BATS) site from October 1988 through December 2023
Published: 2024-09-13
Keywords: BATS, HPLC pigments, phytoplankton pigments, algal pigments, biota, oceans

Cite This Dataset

DOI:10.26008/1912/bco-dmo.893521.6

Spatial Extent: N:33.142 E:-62.718 S:27.823 W:-65.343

Bermuda Atlantic TimeSeries Study (BATS) station

Temporal Extent: 1988-10-21 - 2023-12-13

Project:

Bermuda Atlantic Time-series Study (BATS)

Program:

Ocean Carbon and Biogeochemistry (OCB)

U.S. Joint Global Ocean Flux Study (U.S. JGOFS)

Ocean Time-series Sites (Ocean Time-series)

Principal Investigator:

Nicholas Bates (Bermuda Institute of Ocean Sciences, BIOS)

Co-Principal Investigator:

Rodney J. Johnson (Bermuda Institute of Ocean Sciences, BIOS)

Scientist:

Paul J. Lethaby (Bermuda Institute of Ocean Sciences, BIOS)

Technician:

Claire Medley (Bermuda Institute of Ocean Sciences, BIOS)

Dominic Smith (Bermuda Institute of Ocean Sciences, BIOS)

BCO-DMO Data Manager:

Dana Stuart Gerlach (Woods Hole Oceanographic Institution, WHOI BCO-DMO)

Audrey Mickle (Woods Hole Oceanographic Institution, WHOI BCO-DMO)

Version:

Version Date:

2024-09-13

Restricted:

Validated:

Yes

Current State:

Final with updates expected

HPLC and fluorometric derived phytoplankton pigment concentrations from seawater collected at the Bermuda Atlantic Time-series Study (BATS) site from October 1988 through December 2023

Abstract:

Data presented here contain HPLC derived phytoplankton pigments and fluorometric chlorophyll-a from the BATS site for years 1988 to 2023. Water samples are typically collected from 12 depths in the upper 250 meters of the water column, and then filtered under low vacuum through a 25mm GF/F filter. The filter is then flash frozen in liquid nitrogen and stored at -80 degrees C. Shoreside, analysis is performed on an HPLC using a method modified by Dr. R. Bidigare from the Wright et al. (1991) procedure. This method identifies the pigments chlorophyll-c3, chlorophyll-c2, peridinin, 19’-butanoyloxyfucoxanthin, fucoxanthin, 19’-hexanoyloxyfucoxanthin, prasinoxanthin, diadinoxanthin, alloxanthin, diatoxanthin, lutein, zeaxanthin, chlorophyll-b, chlorophyll-a, divinyl chlorophyllide-a, alpha and beta carotene. Additionally, chlorophyll-a and phaeopigments are analyzed using a fluorometric assay.

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Archival Copy

Version Date	Archive	Persistent Identifier (PID)	Date PID Issued
2023-09-13	Marine Biological Laboratory/Woods Hole Oceanographic Institution Library (MBLWHOI DLA)	10.26008/1912/bco-dmo.893521.6	2024-11-07
2023-04-22	Marine Biological Laboratory/Woods Hole Oceanographic Institution Library (MBLWHOI DLA)	10.26008/1912/bco-dmo.893521.1	2023-04-23

Methods & Sampling

Phytoplankton use pigments to absorb energy from the sun to drive photosynthesis. Chlorophyll-a is used as the primary light harvesting molecule while other accessory pigments, such as chlorophyll-b, -c, and carotenoids assist by expanding the light absorption capability of the organism, therefore increasing efficiency and adaptability (Bidigare et al., 2002).

Many individual algal pigments or combinations and ratios are taxon-specific. Therefore, pigment composition from seawater samples can be used to separate major algal groups and result in chemotaxonomic characterization. These analyses can be used to determine phytoplankton community structure and physiological state of the autotrophic assemblage (Wallerstein et al., 1999; Bidigare et al., 2002)

The methodology described here is based on the Protocols for the Joint Global Ocean Flux Study (JGOFS) Core Measurements (BATS, 1997), and describes the use of high performance liquid chromatography (HPLC) for the rapid separation of phytoplankton pigments with detection limits for chlorophylls and carotenoids on the order of one nanogram (Bidigare, 1991). This HPLC method was adopted as BATS protocol in July 1994 (BATS 70 cruise). This method uses less solvent and gives improved peak separation and better resolution at lower concentrations.

Field sampling
Discrete samples are collected monthly using Niskin bottles at the Bermuda Atlantic Time-series Study site from depths ranging from the surface to 250 meters. Expeditious sampling and contamination prevention protocols were used to obtain the best possible samples, since the physico-chemical and biological parameters of the Niskin water become increasingly altered with time spent on deck, especially if in full sunlight. Sea water is filtered using glass fiber filters (GF/F) with standard pore size of 0.7 microns and the filtered samples then flash frozen and stored at -80ºC until analysis.

HPLC pigment measurements
Water samples were analyzed for the concentration of various phytoplankton pigments following the method of Wright et al. (1991) as modified by Dr. Robert Bidigare.

Pigments present in a seawater sample can be separated by high-performance liquid chromatography (HPLC) based on differences in polarity. Pigment polarities determine how the pigments interact with the solid phase (column) and the mobile phase (solvent) within the HPLC. Pigments that are less polar will be more attracted to the non-polar stationary phase and take longer to pass through than more polar pigments, thus a temporal separation is achieved. The length of time it takes for the pigment to elute is known as the retention time. Under comparable conditions, pigment retention times are consistent and can therefore be used for identification when compared to a reference. The retention times are determined using a diode array detector (DAD), which detects absorption across a range of wavelengths in the UV-Vis portion of the spectrum. The separated pigments are transported by the flowing mobile phase to the detector, where the solution passes through a flow cell and is dispersed by a diffraction grating. Photodiode arrays detect the light intensity for each wavelength, which is converted to an electrical signal, resulting in a visible peak on a chromatogram. Concentration is proportional to the area of the peak, and can be calculated using calibration factors determined from known standards (aka response factor), in addition to other parameters such as volume of water sampled and dilution factors.

The HPLC currently in use is an Agilent 1100 series. The results from two different wavelengths are reported in this method, 436nm and 450nm. All pigments except divinyl chlorophyll-a produce a signal at 436nm. However, divinyl and monovinyl chl-a cannot be separated at 436nm due to a similar detector response, so 450nm is also used to try and separate mono and divnyl chl-a since divnyl absorbs at this wavelength and monovinyl does not.

Fluorometric measurements
In addition to the HPLC measurements, pigment samples from BATS are also analyzed using fluorometric techniques. Fluorescence is the physical property of compounds to absorb light energy and instantaneously re-emit light at a different wavelength to the absorbed light. Fluorescent compounds, such as chlorophyll-a, have characteristic absorption and emission wavelengths. In fluorometry, a sample is excited at the appropriate absorption wavelength and the intensity of the emitted light is measured using a photodiode detector to give a raw fluorescence recorded value that is proportional to concentration. When compared to reference standards, the raw fluorescence measurements are used to calculate the concentration of the fluorescent material in the sample.

Prior to January 2020, fluorometry was performed on the Turner 10-AU fluorometer, whereas samples are currently analyzed using the Trilogy Fluorometer at BIOS. Data from the fluorometer is compared to the chlorophyll-a data from the HPLC which allows an extra quality control method to ensure data from both methods are similar. This data is being released as part of the BATS dataset since fluorometry is often used instead of HPLC in the oceanographic community for chlorophyll analysis.

Additional information
Additional details on methods, standardization, and calibration can be found in the BATS methods document (Protocols for the Bermuda Atlantic Time-series Study Core Measurements)

Data Processing Description

BATS HPLC Data Processing

Once a sample has been analysed, the peaks in the resulting chromatogram are manually integrated, as the automatic integration processing in the software (Agilent OpenLab Chemstation Version 2) is not suitable for the high number of analytes.

The manual integration tool within the software is used to draw a line along the baseline from the start to the end of the peak, from which the area of the peak can be determined. The peaks are identified and labelled using the saved retention times from calibration with known standards.

The signal from the HPLC is proportional to the concentration of the pigment in the sample and is used to calculate the final concentration (C) in ng/L of pigment using the following equation:

C = ( A * RF ) / V_inj * DF * V_ext/ V_f * 10⁶

where,

DF = ( V_vial+ V_ace+ V_H20) / V_vial

A = HPLC Peak Area

RF = HPLC Response factor (determined during calibration)

V_inj = Injection volume on HPLC (normally 200µl)

V_{ext =}Extraction volume of filter (normally 3.2ml)

V_{f =}volume of water filtered during sample collection (normally 4000ml)

V_vial = volume of sample decanted into HPLC vial (normally 1000µl)

V_{ace =}volume of acetone added to HPLC vial (usually zero)

V_H20= volume of water added to HPLC vial (usually 300µl)

10⁶ = volume conversion factor

Notes:

Extraction volume is 3.2ml due to the 3ml of acetone added and the 0.2ml of seawater retained on the filter

An in-house Matlab (Version 2015b) processing script is used to extract the data required for the concentration calculation from various sources, including sample ID files, HPLC chromatogram reports, and fluorescence results reports. It then calculates the concentration of each pigment for each sample in ng/L.

Finally, the reported data are converted to ng/kg simply by multiplying by 1000 and dividing by the density of the sample which is calculated using either the bottle salinity or CTD salinity at time of sample collection and an assumed laboratory temperature of 24°C.

BCO-DMO Processing

- imported "BATS_bottle_v006_unique_vessel_cruise_combos.txt", "bats_pigments_v006.txt", and "bats_pigments_qcmask_v006.txt" into BCO-DMO system
- joined ""BATS_bottle_v006_unique_vessel_cruise_combos.txt" and "bats_pigments_v006.txt" to add a new Vessel column based on the appropriate cruise number
- joined "bats_pigments_qcmask_v006.txt" and "bats_pigments_v006.txt" to add flag columns for the parameters
- converted longitude values to decimal degrees (degrees West are negative)
- converted date to yyyy-mm-dd format
- added filename, Cruise_type, Cruise_num, Cast, Cast_type, and Bottle_number columns (extracted from ID column)
- modified parameter names to conform with BCO-DMO naming conventions and to be more consistent with other BATS data submissions

Version History
- Version history supplemental file provided
- Addition cruises included since previous version: 10406-10411
- Flags were provided for this version and incorporated into the dataset
- File names are being adjusted to be more consistent with other BATS data submissions (see processing notes above and parameters listed)
- Author order adjusted
- Temporal and spatial extents updated

Data Files

File
893521_v6_bats_pigments.csv (Comma Separated Values (.csv), 1.30 MB) MD5:82bacbff0f8776f79cec071ec790398a Primary data file for dataset ID 893521, version 6

Supplemental Files

File
Update file for BATS pigments data for version 6 (V006). filename: bats_pigments_release_v006_update.txt (Plain Text, 485 bytes) MD5:54f01a08bfd9ac7882cc9fc1bb853e97 ASCII file listing update for BATS pigment data version 6 (V006) from previous submission version 5 (V005).

More Information about this dataset

Funding Sources

Funding Source	Award Number
NSF Division of Ocean Sciences	OCE-0752366
NSF Division of Ocean Sciences	OCE-1756105
NSF Division of Ocean Sciences	OCE-2241455

Deployments

Deployment	Synonyms	Start Date	Platform	Investigator
BATS_cruises	Bermuda Atlantic Time-series Study cruises	1988-10-20	Multiple Vessels	Nicholas Bates (Principal Investigator) Michael W. Lomas (Co-Principal Investigator) Rodney J. Johnson (Scientist) Theresa McKee (BCO-DMO Data Manager)	data info

Instruments

High-Performance Liquid Chromatograph

Supplied Name: Agilent 1100 series with diode array detector

Supplied Description:

The HPLC currently in use is an Agilent 1100 series

Instrument Type

Generic Name: High-Performance Liquid Chromatograph

Acronym: HPLC

Community Identifier: http://vocab.nerc.ac.uk/collection/L05/current/LAB11/

Generic Description:

A High-performance liquid chromatograph (HPLC) is a type of liquid chromatography used to separate compounds that are dissolved in solution. HPLC instruments consist of a reservoir of the mobile phase, a pump, an injector, a separation column, and a detector. Compounds are separated by high pressure pumping of the sample mixture onto a column packed with microspheres coated with the stationary phase. The different components in the mixture pass through the column at different rates due to differences in their partitioning behavior between the mobile liquid phase and the stationary phase.

Niskin bottle

Supplied Description:

Instrument Type

Generic Name: Niskin bottle

Community Identifier: http://vocab.nerc.ac.uk/collection/L22/current/TOOL0412/

Generic Description:

A Niskin bottle (a next generation water sampler based on the Nansen bottle) is a cylindrical, non-metallic water collection device with stoppers at both ends. The bottles can be attached individually on a hydrowire or deployed in 12, 24, or 36 bottle Rosette systems mounted on a frame and combined with a CTD. Niskin bottles are used to collect discrete water samples for a range of measurements including pigments, nutrients, plankton, etc.

Turner Designs Fluorometer 10-AU

Supplied Name: Turner 10-AU fluorometer

Supplied Description:

Prior to January 2020, fluorometry was performed on the Turner 10-AU fluorometer.

Instrument Type

Generic Name: Turner Designs Fluorometer 10-AU

Acronym: Turner Fluorometer 10-AU

Community Identifier: http://vocab.nerc.ac.uk/collection/L22/current/TOOL0393/

Generic Description:

The Turner Designs 10-AU Field Fluorometer is used to measure Chlorophyll fluorescence. The 10AU Fluorometer can be set up for continuous-flow monitoring or discrete sample analyses. A variety of compounds can be measured using application-specific optical filters available from the manufacturer. (read more from Turner Designs, turnerdesigns.com, Sunnyvale, CA, USA)

Turner Designs Trilogy fluorometer

Supplied Name: Trilogy fluorometer

Supplied Description:

Samples are currently analyzed using the Trilogy Fluorometer.

Instrument Type

Generic Name: Turner Designs Trilogy fluorometer

Acronym: Turner Trilogy

Generic Description:

The Trilogy Laboratory Fluorometer is a compact laboratory instrument for making fluorescence, absorbance, and turbidity measurements using the appropriate snap-in application module. Fluorescence modules are available for discrete sample measurements of various fluorescent materials including chlorophyll (in vivo and extracted), rhodamine, fluorescein, cyanobacteria pigments, ammonium, CDOM, optical brighteners, and other fluorescent compounds.

Parameters

Date and time formats are described in python strftime() syntax.

Supplied Name	Supplied description	Supplied Units	Standard Name
ID	Sample identification; a unique number which identifies cruise, cast, and bottle number	unitless	sample
ISO_DateTime_UTC	Collection time in UTC format Format: %Y-%m-%dT%H:%MZ	unitless	ISO_DateTime_UTC
Vessel	Name of vessel used for cruise	unitless	ship
Latitude	Latitude of sample collection	decimal degrees	lat
Longitude	Longitude of sample collection (West is negative)	decimal degrees	lon
Cruise_type	Cruise type (BATS Core, Bloom A, or Bloom B)	unitless	cruise_type
Cruise_num	BATS Cruise number	unitless	cruise_id
Cast	Cast Number (1-80 = CTD, 81-99 = Hydrocast)	unitless	cast
Cast_type	Cast type (CTD or Hydrocast)	unitless	cast_type
Bottle_number	Niskin bottle number	unitless	bot_Nis
QF_Niskin_GoFlo	Niskin/GoFlo quality flag (-3 = suspect, 1=unverified, 2= verified/acceptable)	uniteless	q_flag
Depth	Collection depth	meters (m)	depth
QF_depth	Quality control flag for depth; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p1	pigment 1 = Chlorophyll c3	nanograms per kilogram (ng/kg)	chl_c3
QF_p1	Quality control flag for p1; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p2	pigment 2 = Chlorophyllide_a	nanograms per kilogram (ng/kg)	chlide_a
QF_p2	Quality control flag for p2; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p3	pigment 3 = Chlorophyll c1 + c2	nanograms per kilogram (ng/kg)	chl_c1_c2
QF_p3	Quality control flag for p3; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p4	pigment 4 = Peridinin	nanograms per kilogram (ng/kg)	peridinin
QF_p4	Quality control flag for p4; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p5	pigment 5 = 19-prime-Butanoyloxyfucoxanthin	nanograms per kilogram (ng/kg)	fucox_but
QF_p5	Quality control flag for p5; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p6	pigment 6 = Fucoxanthin	nanograms per kilogram (ng/kg)	fucox
QF_p6	Quality control flag for p6; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p7	pigment 7 = 19-prime-Hexanoyloxyfucoxanthin	nanograms per kilogram (ng/kg)	fucox_hex
QF_p7	Quality control flag for p7; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p8	pigment 8 = Prasinoxanthin	nanograms per kilogram (ng/kg)	prasinox
QF_p8	Quality control flag for p8; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p9	pigment 9 = Diadinoxanthin	nanograms per kilogram (ng/kg)	diadinox
QF_p9	Quality control flag for p9; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p10	pigment 10 = Alloxanthin	nanograms per kilogram (ng/kg)	allox
QF_p10	Quality control flag for p10; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p11	pigment 11 = Diatoxanthin	nanograms per kilogram (ng/kg)	diatox
QF_p11	Quality control flag for p11; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p12	pigment 12 = Zeaxanthin + Lutein	nanograms per kilogram (ng/kg)	pigment_conc
QF_p12	Quality control flag for p12; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p13	pigment 13 = Chlorophyll b	nanograms per kilogram (ng/kg)	chl_b
QF_p13	Quality control flag for p13; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p14	pigment 14 = Chlorophyll a	nanograms per kilogram (ng/kg)	chl_a
QF_p14	Quality control flag for p14; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p15	pigment 15 = a + b Carotene	nanograms per kilogram (ng/kg)	carotene
QF_p15	Quality control flag for p15; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p16_Chl	pigment 16 = fluorometric Chlorophyll a	micrograms per kilogram (ug/kg)	chl_a_turner
QF_p16_Chl	Quality control flag for p16; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p17_Phae	pigment 17 = fluorometric Phaeopigments	micrograms per kilogram (ug/kg)	phaeo
QF_p17_Phae	Quality control flag for p17; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p18	pigment 18 = Lutein	nanograms per kilogram (ng/kg)	lutein
QF_p18	Quality control flag for p18; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p19	pigment 19 = Zeaxanthin	nanograms per kilogram (ng/kg)	zeax
QF_p19	Quality control flag for p19; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p20	pigment 20 = alpha-Carotene	nanograms per kilogram (ng/kg)	carotene_a
QF_p20	Quality control flag for p20; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
p21	pigment 21 = beta-Carotene	nanograms per kilogram (ng/kg)	carotene_b
QF_p21	Quality control flag for p21; Parameter quality flags defined as 1= unverified, 2= verified acceptable, 3= questionable, 4= bad, 9= no data	unitless	q_flag
yyyymmdd	Year Month Day of collection	unitless	date
decy	Decimal year	unitless	year_decimal
time	Time of collection	unitless	time

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Dataset: BATS HPLC pigments