Dataset: bacteria
Deployment: EN198

Bacterial abundance, thymidine incorporation, bottle casts

Principal Investigator:

Hugh W. Ducklow (Marine Biological Laboratory Ecosystems Center, MBL - Ecosystems)

BCO-DMO Data Manager:

Cynthia L. Chandler (Woods Hole Oceanographic Institution, WHOI BCO-DMO)

Project:

U.S. JGOFS North Atlantic Bloom Experiment (NABE)

Version:

November 28, 2001

Deployment Synonyms:

END-198

Version Date:

2001-11-28

Data URL:

https://osprey.bco-dmo.org/dataset-deployment/450717/data

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Description

Bacterial abundance, thymidine incorporation, bottle casts

Methods & Sampling

Dataset acquisition description

PI: Hugh Ducklow of: Virginia Institute of Marine Science dataset: Bacteria abundance, thymidine incorporation dates: June 30, 1989 to July 04, 1989 location: N: 59.535 S: 59.4733 W: -21.0183 E: -20.8217 project/cruise: North Atlantic Bloom Experiment/Endeavor 198 ship: R/V Endeavor DMO Note: Bacteria data from the NABE Atlantis II cruise
are reported with the biology dataset for that cruise.

Methodology

BACTERIAL ABUNDANCE & BACTERIAL THYMIDINE & LEUCINE INCORPORATION (Ducklow, HPEL)

Abundance samples preserved in 1.25% glutaraldehyde and stored at 5ï¿½ C until microscopy was performed at Horn Point Environmental Laboratory. All samples were enumerated according to the Acridine Orange Direct Count technique of Hobbie et al., (1977) with modifications by Helen Quinby. Samples were enumerated on a Nikon Optiphot epifluorescence microscope at 1850x with a 100 watt Mercury lamp.

Thymidine incorporation samples collected from Niskin rosette casts were immediately processed as described in Ducklow and Hill (1985), with the following modifications: Samples were incubated with 5 nM 3H-thymidine (New England Nuclear, sp. act. 81 Ci/mmol) in polycarbonate bottles, disposable polyproplyene centrifuge tubes or Whirl-Pak bags. Incubations were terminated with addition of 0.37% formaldehyde, then filtered onto 0.2 ï¿½m Nuclepore filters. Extractions were carried out by rinsing each filter on its funnel support 3 times with 5% ice cold TCA, over a weak vacuum (<10 in. Hg), then 3 times with 80% ice cold ethanol. All extracted filters were stored dry in scintillation vials for counting at Horn Point Environmental Laboratory.

Leucine incorporation samples were treated according to the method described in Kirchman et al., (1985), with the following modifications: Samples were incubated with 0.5 nM 3H- leucine (NEN; Sp. Act. 73 Ci/mmol) and 10 nM nonradioactive leucine, then treated as described for thymidine.

US JGOFS NABE Bacterial Data

 
    Bacterial data were collected on the US JGOFS NABE cruises aboard RV 
ATLANTIS II legs 2 and 3 and Endeavor cruise 198 by Hugh Ducklow, David 
Kirchman, Helen Quinby and Hans Dam. On cruise 2, only bacterial abundance 
was measured. On cruise 3, bacterial abundance, and bacterial thymidine and 
leucine incorporation were measured.  On Endeavor cruise 198 only bacteria 
abundance and thymidine incorporation were measured by the following methods:

Abundance:

Samples preserved in 1.25% glutaraldehyde and stored at 5C until microscopy was
performed at Horn Point. All samples were enumerated according to the Acridine
Orange Direct Count technique of Hobbie et al., (1977) with modifications by
Helen Quinby. Samples were enumerated on a Nikon Optiphot epifluorescence
microscope at 1850X with a 100 watt Mercury lamp.

Thymidine Incorporation:

Samples collected from Niskin rosette casts were immediately processed as
described in Ducklow and Hill (1985), with the following modifications:

Samples were incubated with 5 nM 3H-thymidine (New England Nuclear, sp. act. 81
Ci/mmol) in polycarbonate bottles, disposable polyproplyene centrifuge tubes or
Whirl-Pak bags. Incubations were terminated with addition of 0.37%
formaldehyde, then filtered onto 0.2 um Nuclepore filters. Extractions were
carried out by rinsing each filter on its funnel support 3 times with 5% ice
cold TCA, over a weak vacuum (< 10 in. Hg), then 3 times with 80% ice cold
ethanol. All extracted filters were stored dry in scintillation vials for
counting at Horn Point.

Additional samples were treated to purify the labelled DNA following the method
of Wicks et al., (1987). 95% of the label in the cold TCA extracts was in pure
DNA. (Data available from HWD).

Leucine Incorporation:

Samples were treated according to the method described in Kirchman et al.,
(1985), with the following modifications:

Samples were incubated with 0.5 nM 3H-leucine (NEN; Sp. Act. 73 Ci/mmol) and 10
nM nonradioactive leucine, then treated as described for thymidine.

Biomass/production/systhesis rate conversions:
 
The bacteria abundance data can be converted into bacterial biomass (ugC or ugN l-1)
as described for example in Lee and Fuhrman (1988). We will be measuring cell
biovolumes for this conversion and have not supplied nominal biomass data at
this time.

The THYINCORP data can be converted into bacterial production rates (ugC or ugN
l-1 hr-1) as discussed in Ducklow and Hill (1985). We performed separate
experiments to determine the conversion factors, and will report the data
separately. The THYINCORP data provide a relative index of differences in
bacterial production in space and time. Data on the biovolume and rate
conversion factors are required for translation into absolute units.

The LEUINCORP data can be converted into bacterial protein synthesis rates (ugC
or ugN l-1 hr-1) as discussed in Chin-Leo and Kirchman, (1988). We performed
separate experiments to determine the conversion factors, and will report the
data separately. The LEUINCORP data provide a relative index of differences in
protein synthesis in space and time. Data on the biovolume and rate conversion
factors are required for translation into absolute units.


References

Chin-Leo, G. And D.L. Kirchman. 1988. Estimating bacterial production in
     natural waters from the simultaneous incorporation of thymidine and
     leucine. Appl. Environ. Microbiol. 54:1934-39.

Ducklow, H.W., and S.M. Hill. 1985b. Tritiated thymidine incorporation and the
     growth of heterotrophic bacteria in warm core rings. Limnol. Oceanogr.
     30:260-272.

Hobbie, J.E., R.J. Daley, and S. Jasper. 1977. Use of Nuclepore filters for
     counting bacteria by fluorescence microscopy. Appl. Environ. Microbiol.
     33: 1225-1228.

Kirchman, D., E. K'nees and R. Hodson. 1985. Leucine incorporation and its
     potential as a measure of protein synthesis by bacteria in natural waters.
     Appl. Environ. Microbiol. 49: 599-607.

Lee, S. and J.A. Fuhrman. 1987. Relationships between biovolume and biomass of
     naturally-derived marine bacterioplankton. Appl. Environ. Microbiol.
     52:1298-1303.

Wicks, R.J. and R.D.Robarts, 1987, The extraction and purification of DNA
     labelled with methyl-3H-thymidine in aquatic bacterial production studies,
     J. Plankton Res. 9:1159-66.

 
DMO note:
 The Data Management Office has changed the units of the parameters
 "bact_het_mic" from cells/liter*10^9 to cells/milliliter

Deployment-specific acquisition description

Methodology

BACTERIAL ABUNDANCE & BACTERIAL THYMIDINE & LEUCINE INCORPORATION (Ducklow, HPEL)

US JGOFS NABE Bacterial Data

 
    Bacterial data were collected on the US JGOFS NABE cruises aboard RV 
ATLANTIS II legs 2 and 3 and Endeavor cruise 198 by Hugh Ducklow, David 
Kirchman, Helen Quinby and Hans Dam. On cruise 2, only bacterial abundance 
was measured. On cruise 3, bacterial abundance, and bacterial thymidine and 
leucine incorporation were measured.  On Endeavor cruise 198 only bacteria 
abundance and thymidine incorporation were measured by the following methods:

Abundance:

Samples preserved in 1.25% glutaraldehyde and stored at 5C until microscopy was
performed at Horn Point. All samples were enumerated according to the Acridine
Orange Direct Count technique of Hobbie et al., (1977) with modifications by
Helen Quinby. Samples were enumerated on a Nikon Optiphot epifluorescence
microscope at 1850X with a 100 watt Mercury lamp.

Thymidine Incorporation:

Samples collected from Niskin rosette casts were immediately processed as
described in Ducklow and Hill (1985), with the following modifications:

Samples were incubated with 5 nM 3H-thymidine (New England Nuclear, sp. act. 81
Ci/mmol) in polycarbonate bottles, disposable polyproplyene centrifuge tubes or
Whirl-Pak bags. Incubations were terminated with addition of 0.37%
formaldehyde, then filtered onto 0.2 um Nuclepore filters. Extractions were
carried out by rinsing each filter on its funnel support 3 times with 5% ice
cold TCA, over a weak vacuum (< 10 in. Hg), then 3 times with 80% ice cold
ethanol. All extracted filters were stored dry in scintillation vials for
counting at Horn Point.

Additional samples were treated to purify the labelled DNA following the method
of Wicks et al., (1987). 95% of the label in the cold TCA extracts was in pure
DNA. (Data available from HWD).

Leucine Incorporation:

Samples were treated according to the method described in Kirchman et al.,
(1985), with the following modifications:

Samples were incubated with 0.5 nM 3H-leucine (NEN; Sp. Act. 73 Ci/mmol) and 10
nM nonradioactive leucine, then treated as described for thymidine.

Biomass/production/systhesis rate conversions:
 
The bacteria abundance data can be converted into bacterial biomass (ugC or ugN l-1)
as described for example in Lee and Fuhrman (1988). We will be measuring cell
biovolumes for this conversion and have not supplied nominal biomass data at
this time.

The THYINCORP data can be converted into bacterial production rates (ugC or ugN
l-1 hr-1) as discussed in Ducklow and Hill (1985). We performed separate
experiments to determine the conversion factors, and will report the data
separately. The THYINCORP data provide a relative index of differences in
bacterial production in space and time. Data on the biovolume and rate
conversion factors are required for translation into absolute units.

The LEUINCORP data can be converted into bacterial protein synthesis rates (ugC
or ugN l-1 hr-1) as discussed in Chin-Leo and Kirchman, (1988). We performed
separate experiments to determine the conversion factors, and will report the
data separately. The LEUINCORP data provide a relative index of differences in
protein synthesis in space and time. Data on the biovolume and rate conversion
factors are required for translation into absolute units.


References

Chin-Leo, G. And D.L. Kirchman. 1988. Estimating bacterial production in
     natural waters from the simultaneous incorporation of thymidine and
     leucine. Appl. Environ. Microbiol. 54:1934-39.

Ducklow, H.W., and S.M. Hill. 1985b. Tritiated thymidine incorporation and the
     growth of heterotrophic bacteria in warm core rings. Limnol. Oceanogr.
     30:260-272.

Hobbie, J.E., R.J. Daley, and S. Jasper. 1977. Use of Nuclepore filters for
     counting bacteria by fluorescence microscopy. Appl. Environ. Microbiol.
     33: 1225-1228.

Kirchman, D., E. K'nees and R. Hodson. 1985. Leucine incorporation and its
     potential as a measure of protein synthesis by bacteria in natural waters.
     Appl. Environ. Microbiol. 49: 599-607.

Lee, S. and J.A. Fuhrman. 1987. Relationships between biovolume and biomass of
     naturally-derived marine bacterioplankton. Appl. Environ. Microbiol.
     52:1298-1303.

Wicks, R.J. and R.D.Robarts, 1987, The extraction and purification of DNA
     labelled with methyl-3H-thymidine in aquatic bacterial production studies,
     J. Plankton Res. 9:1159-66.

 
DMO note:
 The Data Management Office has changed the units of the parameters
 "bact_het_mic" from cells/liter*10^9 to cells/milliliter

Data Processing Description

Dataset Processing Description

More information about this dataset deployment

Funding

Award Number	Funding Source
unknown NABE NSF	National Science Foundation

Instruments

Niskin bottle

Supplied Name: Niskin Bottle

Supplied Description:

Niskin rosette bottles used to collect thymidine incorporation samples.

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.

Parameters

Supplied Name	Supplied description	Supplied Units	Standard Name
event	event number per event log	dimensionless	event
sta	station number per event log	dimensionless	sta
cast	cast number, consecutive within station	dimensionless	cast
date	date reported as YYYYMMDD	YYYYMMDD	date
time	time reported as HHmm, GMT	hours/minutes	time
lat	latitude, minus = south	decimal degrees	lat
lon	longitude, minus = west,	decimal degrees	lon
depth_n	nominal depth of sample	meters	depth_n
thy_incorp	thymidine incorporation	picomoles/liter/hour	thy_incorp
bact_het_orig	heterotrophic bacteria abundance, original units; microscopy	cells/liter *10^9	bact_het_orig
bact_het_mic	heterotrophic bacteria abundance, microscopy	cells/milliliter	bact_het_mic

Database

Contribute Data

Dataset: bacteria
Deployment: EN198

Dataset acquisition description

Methodology

BACTERIAL ABUNDANCE & BACTERIAL THYMIDINE & LEUCINE INCORPORATION (Ducklow, HPEL)

US JGOFS NABE Bacterial Data

Deployment-specific acquisition description

Methodology

BACTERIAL ABUNDANCE & BACTERIAL THYMIDINE & LEUCINE INCORPORATION (Ducklow, HPEL)

US JGOFS NABE Bacterial Data

Dataset Processing Description

Database

Contribute Data

Dataset: bacteriaDeployment: EN198

Dataset acquisition description

Methodology

BACTERIAL ABUNDANCE & BACTERIAL THYMIDINE & LEUCINE INCORPORATION (Ducklow, HPEL)

US JGOFS NABE Bacterial Data

Deployment-specific acquisition description

Methodology

BACTERIAL ABUNDANCE & BACTERIAL THYMIDINE & LEUCINE INCORPORATION (Ducklow, HPEL)

US JGOFS NABE Bacterial Data

Dataset Processing Description

Dataset: bacteria
Deployment: EN198