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            <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/dataset/3780.rdf" xlink:actuate="onRequest">Experimental results from a study of Pseudo-nitzschia multiseries growth rates and cellular domoic acid under varying pCO2 and phosphate levels (PhytoTM_in_HighCO2 project)</gmx:Anchor>
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                <gmx:Anchor xlink:href="http://orcid.org/0000-0002-0502-893X" xlink:title="ORCID" xlink:actuate="onRequest">Feixue Fu</gmx:Anchor>
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                <gmx:Anchor xlink:href="https://ror.org/03taz7m60" xlink:title="ROR ID" xlink:actuate="onRequest">University of Southern California</gmx:Anchor>
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            <gco:CharacterString>Cite this dataset as: Fu, F., Hutchins, D. A., Sanudo-Wilhelmy, S. A. (2012) Experimental results from a study of Pseudo-nitzschia multiseries growth rates and cellular domoic acid under varying pCO2 and phosphate levels (PhytoTM_in_HighCO2 project). Biological and Chemical Oceanography Data Management Office (BCO-DMO). (Version 15 Nov 2012) Version Date 2012-11-15 [if applicable, indicate subset used]. http://lod.bco-dmo.org/id/dataset/3780 [access date]</gco:CharacterString>
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        <gco:CharacterString>Pseudo-nitzschia multiseries growth rates and cellular domoic acid under varying pCO2 and phosphate levels (for all replicates). Dataset Description: &amp;lt;p&amp;gt;Experimental data examining &amp;lt;i&amp;gt;Pseudo-nitzschia multiseries&amp;lt;/i&amp;gt; (CCMP  2708) domic acid production and growth rates under varying pCO2 and phosphate treatments. Values are reported for each replicate bottle (three replicates for each of the three pCO2 treatments).&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
Data and methods are described in:&amp;lt;br /&amp;gt;
&amp;lt;b&amp;gt;Sun&amp;lt;/b&amp;gt; J., Hutchins D. A., Feng Y., Seubert E. L., Caron D. A.,   &amp;amp;amp; Fu F.-X., 2011. Effects of changing pCO2 and phosphate   availability on domoic acid production and physiology of the marine   harmful bloom diatom Pseudo-nitzschia multiseries. Limnology and   Oceanography 56(3):829-840. DOI: &amp;lt;a href=&amp;quot;http://dx.doi.org/10.4319/lo.2011.56.3.0829&amp;quot; target=&amp;quot;_blank&amp;quot;&amp;gt;10.4319/lo.2011.56.3.0829&amp;lt;/a&amp;gt;&amp;lt;/p&amp;gt; Methods and Sampling: &amp;lt;p&amp;gt;The methods below are described in Sun et al. 2011.&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Cultures and growth conditions&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
Stock cultures of marine diatom &amp;lt;i&amp;gt;Pseudo-nitzschia multiseries&amp;lt;/i&amp;gt;   (Hasle) (CCMP 2708, originally isolated from Eastern Canada) were   maintained at 17 degrees C in 0.2 um-filtered, microwave-sterilized   natural seawater, enriched with levels of phosphate, nitrate, silicate,   vitamins, and trace nutrients as in Price et al. (1988). Light was   provided on a 12 h dark:12 h light cycle using cool white fluorescent   bulbs at 120 umol photons per square meter per second. Irradiance was   measured with a biospherical LICOR sensor (model LI-250).&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Experimental design and determination of growth rates&amp;lt;br /&amp;gt;
&amp;lt;/b&amp;gt;Semi-continuous culturing methods were used in order to measure the   effects of P availability and/or pCO2 levels during acclimated,   steady-state growth.  Cultures were diluted daily with medium that was   previously adjusted to the appropriate temperature and pCO2. Each bottle   was diluted back to the same cell density present in that bottle   directly after the previous day&amp;amp;rsquo;s dilution. Cultures were harvested   following approximately 4 to 6 weeks of semi-continuous incubation when   they were fully acclimated to the experimental conditions, after   statistically invariant growth rates were recorded for at least 4 to 6   consecutive dilutions.&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
Samples from each culture bottle were always taken at the same time in  the diel cycle, between 09:00 h and 10:00 h in the morning, to measure  cell density and thus determine changes in growth rate. Dilutions were  done in real time using biomass estimates made by in vivo fluorescence,  and were subsequently validated using preserved cell count samples.  Growth rates were calculated based on the equation:&amp;lt;br /&amp;gt;
&amp;amp;nbsp;&amp;amp;nbsp; u = (lnNb - lnNa) / (tb - ta),&amp;lt;br /&amp;gt;
where Na and Nb are the average cell density at times ta (directly after  a dilution) and tb (directly before the next day&amp;amp;rsquo;s dilution). For cell  counts, whole-culture samples were fixed with glutaraldehyde (2.5% v to v  final concentration) and counted in triplicate. About 1000 cells per  replicate were enumerated in a 1-mL Sedgewick-Rafter counting chamber,  using an Olympus BX51 epifluorescence microscope at 100-fold  magnification.&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
Triplicate bottles at two conditions of phosphate availability were   equilibrated at three different CO2 concentrations by gentle bubbling   with commercially prepared certified standard air and CO2 gas mixtures   (Praxair Gas).  CO2 concentrations examined included preindustrial   atmospheric levels (~22 Pa), near-present day concentrations (~41 Pa),   and values predicted to occur before the end of this century (~74 Pa,   IPCC 2007).  In-line high efficiency particulate air (HEPA) filters were   used to avoid contamination from particles in the gas tanks or lines.    Phosphate levels used were 20 umol per liter (P replete) and 0.5 umol   per liter (P limited).  A total of six different phosphate and CO2   conditions were used in this study: 20 umol per liter P and ~22 Pa CO2;   20 umol per liter P and ~41 Pa CO2; 20 umol per liter P and ~74 Pa CO2;   0.5 umol per liter P and ~22 Pa CO2; 0.5 umol per liter P and ~41 Pa   CO2; and 0.5 umol per liter P and ~74 Pa CO2.&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Carbonate buffer system measurements and pCO2 treatments&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
The pH in each bottle was monitored daily using a high sensitivity   microprocessor pH-meter (Orion EA 940), calibrated with pH 4, 7 and 10   buffer solutions. The relative precision of this instrument is ~0.01 and   accuracy is ~0.03 pH units. For the analysis of total dissolved   inorganic carbon (DIC), DIC samples were stored in 2 mL capped   borosilicate vials free of air bubbles and were preserved with 20 uL   saturated HgCl2 per liter, and stored at 4 degrees C until analyzed.    Total DIC was measured by acidifying 2-mL 10% of H3PO4 and quantifying   the CO2 trapped in an acid sparging column (model CM 5230) with a carbon   coulometer (model CM 140, UIC). Certified reference materials obtained   from Andrew Dickson (University of California, San Diego,   http://andrew.ucsd.edu/co2qc/index.html) were measured periodically   during the run and used for calibration. pH values remained invariant   before and after the dilution, suggesting that bubbling rates were   sufficient to maintain the target CO2 equilibration levels in the   medium, regardless of diel changes in photosynthesis and respiration.    Based in the daily measurements of pH and DIC, pCO2 stabilized during   the early part of the semi-continuous growth period and then remained   steady throughout the latter part of the incubation period.  Calculated   pCO2 values (using CO2SYS;   http://www.cdiac.ornl.gov/ftp/co2sys/CO2SYS_calc_XLS ) for the three CO2   treatments in both P treatments ranged from 22-23 Pa, 39-42 Pa, and   73-75 Pa (see table below where the numbers in parenthenses are the   standard deviations of triplicate samples), very close to the certified   standard gas mixture values.  For convenience, these values were   averaged and rounded to 22 Pa, 41 Pa, and 74 Pa when referring to the   three pCO2 treatments throughout the dataset and paper (Sun et al.   2011).&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Treatment conditions and calculated pCO2:&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;table cellspacing=&amp;quot;0&amp;quot; cellpadding=&amp;quot;2&amp;quot; border=&amp;quot;1&amp;quot;&amp;gt;
    &amp;lt;tbody&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;Treatment&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Measured pH (sd)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Measured DIC (sd); umol/L&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Calculated CO2 (sd); umol/L&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Calculated pCO2 (sd); Pa&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-limited, 22 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.38 (0.05)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;1917 (38)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.4 (0.6)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;23 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-limited, 41 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.15 (0.02)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2029 (8)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;13.9 (0.7)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;42 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-limited, 74 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.94 (0.01)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2145 (9)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;24.5 (0.6)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;75 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-replete, 22 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.40 (0.03)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;1970 (4)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.1 (0.5)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;22 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-replete, 41 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.19 (0.02)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2066 (11)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;12.8 (0.8)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;40 (3)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-replete, 74 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.96 (0.01)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2177 (6)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;23.9 (0.4)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;73 (1)&amp;lt;/td&amp;gt;
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    &amp;lt;/tbody&amp;gt;
&amp;lt;/table&amp;gt;
&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Analysis of domoic acid concentrations&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
Particulate and dissolved domoic acid was measured using amnesic  shellfish poison (ASP) enzyme-linked immunosorbent assay (ELISA) kits  available from Biosense Laboratories. Particulate domoic acid samples  were collected on uncombusted Whatman GF/F filters and frozen at &amp;amp;ndash;20  degrees C until analyzed.  The filtrate from each sample was also  collected, frozen and later analyzed for dissolved DA.  Sample  preparation and ELISA tests were carried out following the protocol of  Biosense Laboratories (2005 version).  The limit of detection for the  ELISA method for particulate DA is 6.8 ng per liter.  Total DA produced  per cell (including the sum of both particulate and dissolved DA) was  calculated by dividing the DA content of the whole-culture sample by the  cell density.&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;References:&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;b&amp;gt;Platt&amp;lt;/b&amp;gt;, T., C. L. Gallegos, and W. G. Harrison. 1980.  Photoinhibition of photosynthesis in natural assemblages of marine  phytoplankton. J. Mar. Res. 38: 687-701.&amp;lt;/p&amp;gt;</gco:CharacterString>
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(1) Laboratory experiments will measure the trace metal quotas of steady-state cultures of key phytoplankton functional groups like diatoms, coccolithophores, Phaeocystis, and diazotrophic and pico-cyanobacteria while varying pCO2 both alone, and together with other limiting factors such as iron, temperature, and light.&lt;br /&gt;
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	Name: condition
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	Description: &lt;p&gt;Phosphate treatment/condition. Limited =0.5 umol per liter P; Replete = 20 umol per liter P.&lt;/p&gt; 
http://lod.bco-dmo.org/id/dataset-parameter/30767.rdf
	Name: pCO2
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	Name: sp_growth_rate
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http://lod.bco-dmo.org/id/dataset-parameter/30769.rdf
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                <gco:CharacterString>&amp;lt;p&amp;gt;The methods below are described in Sun et al. 2011.&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Cultures and growth conditions&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
Stock cultures of marine diatom &amp;lt;i&amp;gt;Pseudo-nitzschia multiseries&amp;lt;/i&amp;gt;   (Hasle) (CCMP 2708, originally isolated from Eastern Canada) were   maintained at 17 degrees C in 0.2 um-filtered, microwave-sterilized   natural seawater, enriched with levels of phosphate, nitrate, silicate,   vitamins, and trace nutrients as in Price et al. (1988). Light was   provided on a 12 h dark:12 h light cycle using cool white fluorescent   bulbs at 120 umol photons per square meter per second. Irradiance was   measured with a biospherical LICOR sensor (model LI-250).&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Experimental design and determination of growth rates&amp;lt;br /&amp;gt;
&amp;lt;/b&amp;gt;Semi-continuous culturing methods were used in order to measure the   effects of P availability and/or pCO2 levels during acclimated,   steady-state growth.  Cultures were diluted daily with medium that was   previously adjusted to the appropriate temperature and pCO2. Each bottle   was diluted back to the same cell density present in that bottle   directly after the previous day&amp;amp;rsquo;s dilution. Cultures were harvested   following approximately 4 to 6 weeks of semi-continuous incubation when   they were fully acclimated to the experimental conditions, after   statistically invariant growth rates were recorded for at least 4 to 6   consecutive dilutions.&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
Samples from each culture bottle were always taken at the same time in  the diel cycle, between 09:00 h and 10:00 h in the morning, to measure  cell density and thus determine changes in growth rate. Dilutions were  done in real time using biomass estimates made by in vivo fluorescence,  and were subsequently validated using preserved cell count samples.  Growth rates were calculated based on the equation:&amp;lt;br /&amp;gt;
&amp;amp;nbsp;&amp;amp;nbsp; u = (lnNb - lnNa) / (tb - ta),&amp;lt;br /&amp;gt;
where Na and Nb are the average cell density at times ta (directly after  a dilution) and tb (directly before the next day&amp;amp;rsquo;s dilution). For cell  counts, whole-culture samples were fixed with glutaraldehyde (2.5% v to v  final concentration) and counted in triplicate. About 1000 cells per  replicate were enumerated in a 1-mL Sedgewick-Rafter counting chamber,  using an Olympus BX51 epifluorescence microscope at 100-fold  magnification.&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
Triplicate bottles at two conditions of phosphate availability were   equilibrated at three different CO2 concentrations by gentle bubbling   with commercially prepared certified standard air and CO2 gas mixtures   (Praxair Gas).  CO2 concentrations examined included preindustrial   atmospheric levels (~22 Pa), near-present day concentrations (~41 Pa),   and values predicted to occur before the end of this century (~74 Pa,   IPCC 2007).  In-line high efficiency particulate air (HEPA) filters were   used to avoid contamination from particles in the gas tanks or lines.    Phosphate levels used were 20 umol per liter (P replete) and 0.5 umol   per liter (P limited).  A total of six different phosphate and CO2   conditions were used in this study: 20 umol per liter P and ~22 Pa CO2;   20 umol per liter P and ~41 Pa CO2; 20 umol per liter P and ~74 Pa CO2;   0.5 umol per liter P and ~22 Pa CO2; 0.5 umol per liter P and ~41 Pa   CO2; and 0.5 umol per liter P and ~74 Pa CO2.&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Carbonate buffer system measurements and pCO2 treatments&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
The pH in each bottle was monitored daily using a high sensitivity   microprocessor pH-meter (Orion EA 940), calibrated with pH 4, 7 and 10   buffer solutions. The relative precision of this instrument is ~0.01 and   accuracy is ~0.03 pH units. For the analysis of total dissolved   inorganic carbon (DIC), DIC samples were stored in 2 mL capped   borosilicate vials free of air bubbles and were preserved with 20 uL   saturated HgCl2 per liter, and stored at 4 degrees C until analyzed.    Total DIC was measured by acidifying 2-mL 10% of H3PO4 and quantifying   the CO2 trapped in an acid sparging column (model CM 5230) with a carbon   coulometer (model CM 140, UIC). Certified reference materials obtained   from Andrew Dickson (University of California, San Diego,   http://andrew.ucsd.edu/co2qc/index.html) were measured periodically   during the run and used for calibration. pH values remained invariant   before and after the dilution, suggesting that bubbling rates were   sufficient to maintain the target CO2 equilibration levels in the   medium, regardless of diel changes in photosynthesis and respiration.    Based in the daily measurements of pH and DIC, pCO2 stabilized during   the early part of the semi-continuous growth period and then remained   steady throughout the latter part of the incubation period.  Calculated   pCO2 values (using CO2SYS;   http://www.cdiac.ornl.gov/ftp/co2sys/CO2SYS_calc_XLS ) for the three CO2   treatments in both P treatments ranged from 22-23 Pa, 39-42 Pa, and   73-75 Pa (see table below where the numbers in parenthenses are the   standard deviations of triplicate samples), very close to the certified   standard gas mixture values.  For convenience, these values were   averaged and rounded to 22 Pa, 41 Pa, and 74 Pa when referring to the   three pCO2 treatments throughout the dataset and paper (Sun et al.   2011).&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Treatment conditions and calculated pCO2:&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;table cellspacing=&amp;quot;0&amp;quot; cellpadding=&amp;quot;2&amp;quot; border=&amp;quot;1&amp;quot;&amp;gt;
    &amp;lt;tbody&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;Treatment&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Measured pH (sd)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Measured DIC (sd); umol/L&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Calculated CO2 (sd); umol/L&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;Calculated pCO2 (sd); Pa&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-limited, 22 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.38 (0.05)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;1917 (38)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.4 (0.6)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;23 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-limited, 41 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.15 (0.02)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2029 (8)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;13.9 (0.7)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;42 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-limited, 74 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.94 (0.01)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2145 (9)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;24.5 (0.6)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;75 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-replete, 22 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.40 (0.03)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;1970 (4)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.1 (0.5)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;22 (2)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-replete, 41 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;8.19 (0.02)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2066 (11)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;12.8 (0.8)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;40 (3)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
        &amp;lt;tr&amp;gt;
            &amp;lt;td&amp;gt;P-replete, 74 Pa&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;7.96 (0.01)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;2177 (6)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;23.9 (0.4)&amp;lt;/td&amp;gt;
            &amp;lt;td&amp;gt;73 (1)&amp;lt;/td&amp;gt;
        &amp;lt;/tr&amp;gt;
    &amp;lt;/tbody&amp;gt;
&amp;lt;/table&amp;gt;
&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;Analysis of domoic acid concentrations&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
Particulate and dissolved domoic acid was measured using amnesic  shellfish poison (ASP) enzyme-linked immunosorbent assay (ELISA) kits  available from Biosense Laboratories. Particulate domoic acid samples  were collected on uncombusted Whatman GF/F filters and frozen at &amp;amp;ndash;20  degrees C until analyzed.  The filtrate from each sample was also  collected, frozen and later analyzed for dissolved DA.  Sample  preparation and ELISA tests were carried out following the protocol of  Biosense Laboratories (2005 version).  The limit of detection for the  ELISA method for particulate DA is 6.8 ng per liter.  Total DA produced  per cell (including the sum of both particulate and dissolved DA) was  calculated by dividing the DA content of the whole-culture sample by the  cell density.&amp;lt;/p&amp;gt;
&amp;lt;p&amp;gt;&amp;lt;b&amp;gt;References:&amp;lt;/b&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;b&amp;gt;Platt&amp;lt;/b&amp;gt;, T., C. L. Gallegos, and W. G. Harrison. 1980.  Photoinhibition of photosynthesis in natural assemblages of marine  phytoplankton. J. Mar. Res. 38: 687-701.&amp;lt;/p&amp;gt;</gco:CharacterString>
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                          <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/person/51585.rdf" xlink:actuate="onRequest">Feixue Fu</gmx:Anchor>
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                          <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/affiliation/306.rdf" xlink:title="Affiliation" xlink:actuate="onRequest">University of Southern California</gmx:Anchor>
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