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            <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/dataset/859671.rdf" xlink:actuate="onRequest">Diatom metabolites under P-limited and P-replete growth from laboratory cultures in July of 2013</gmx:Anchor>
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            <gco:CharacterString>Cite this dataset as: Kujawinski, E. (2021) Diatom metabolites under P-limited and P-replete growth from laboratory cultures in July of 2013. Biological and Chemical Oceanography Data Management Office (BCO-DMO). (Version 1) Version Date 2021-08-27 [if applicable, indicate subset used]. http://lod.bco-dmo.org/id/dataset/859671 [access date]</gco:CharacterString>
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        <gco:CharacterString>Dataset Description: &amp;lt;p&amp;gt;Raw Spectral Data Files are available in the MetaboLights database under study ID &amp;quot;MTBLS154&amp;quot; (&amp;lt;span style=&amp;quot;font-size:13px&amp;quot;&amp;gt;https://www.ebi.ac.uk/metabolights/MTBLS154&amp;lt;/span&amp;gt;/).&amp;amp;nbsp; Sample, assay,&amp;amp;nbsp;and metabolite information in ISAtab format are also available from that MetaboLights study.&amp;lt;/p&amp;gt; Methods and Sampling: &amp;lt;div&amp;gt;Metadata from &amp;quot;&amp;lt;span style=&amp;quot;font-size:13px&amp;quot;&amp;gt;MTBLS154: Phosphorus availability regulates intracellular nucleotides in marine eukaryotic phytoplankton&amp;lt;/span&amp;gt;&amp;quot; at https://www.ebi.ac.uk/metabolights/MTBLS154/samples&amp;lt;br /&amp;gt;
&amp;amp;nbsp;&amp;lt;/div&amp;gt;

&amp;lt;div&amp;gt;&amp;lt;strong&amp;gt;Sample Collection:&amp;lt;/strong&amp;gt;&amp;lt;br /&amp;gt;
&amp;amp;nbsp;
&amp;lt;div&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;Thalassiosira pseudonana (CCMP number 1335) was cultured axenically in a modified version of L1 media made with Turks Island Salts in order to reduce the background concentration of dissolved organic carbon in the media. The phosphate-replete treatment contained 36 µM PO4 and the phosphate-limited treatment had 0.4 µM PO4. Prior to the experiment, the culture had been maintained through two culture transfers of phosphate-replete or phosphate-limited media. The experiment began with the addition of 30 ml of T. pseudonana in exponential phase to two-thirds of the flasks which contained 300 ml of media. The remaining one-third of the flasks were designated as cell-free controls. Two flasks with cells and one cell-free control for each media (phosphate-replete or phosphate-limited) were sampled at four time points: 0, 2, 8, and 10 days.&amp;lt;/span&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;&amp;amp;nbsp;&amp;lt;/span&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;strong&amp;gt;Extraction:&amp;amp;nbsp;&amp;lt;/strong&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;The intracellular metabolites were extracted using a method modified from a protocol previously described in Rabinowitz and Kimball (2007). Briefly, the filter was extracted three times with ice-cold extraction solvent (acetonitrile:methanol:water with 0.1 M formic acid, 40:40:20). The combined extracts were neutralized with ammonium hydroxide and dried in a vacufuge.&amp;lt;/span&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;The samples for the targeted mass spectrometry analysis were re-dissolved in 95:5 (v/v) water:acetonitrile and combined with deuterated biotin (final concentration 0.05 µg/ml)as an internal standard.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For untargeted analysis, the extracts had to undergo an additional de-salting step prior to analysis. Therefore, the dried extracts were re-dissolved in 0.01 M hydrochloric acid and extracted using a 50 mg/1 cc PPL cartridge following the protocol of Dittmar et al. (2008). The resulting methanol extracts were re-dissolved in 95:5 water:acetonitrile and deuterated biotin.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;strong&amp;gt;Chromatography:&amp;lt;/strong&amp;gt;&amp;lt;/p&amp;gt;
&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For targeted metabolomics analysis, the samples were analyzed with a Synergi 4 µm Fusion – RP 80 Å, 150 × 2.00 mm column (Phenomenex, Torrance, CA) coupled to a Thermo Scientific TSQ Vantage Triple Stage Quadrupole Mass Spectrometer. The chromatography gradient was: an initial hold of 95% A (0.1% formic acid in water) : 5% B (0.1% formic acid in acetonitrile) for 2 minutes, ramp to 65% B from 2 to 20 minutes, ramp to 100% B from 20 to 25 min, and hold until 32.5 minutes. The column was re-equilibrated for 7 min between samples with solvent A. Each metabolite was quantified using multiple reaction monitoring (MRM) mode with optimal parameters determined from infusion of authentic standards. Eight-point external calibration curves (0.5, 1, 5, 10, 50, 100, 250, and 500 ng/ml) were generated for each compound by plotting peak area against concentration.&amp;lt;/span&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For untargeted metabolomics analysis, LC separation was performed using a Synergi Fusion reversed phase column (Phenomenex, Torrance, CA) with the same gradient as for targeted analysis.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;strong&amp;gt;Mass spectroscopy:&amp;lt;/strong&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For targeted analysis, samples were analyzed with a Thermo Scientific TSQ Vantage Triple Stage Quadrupole Mass Spectrometer. This instrument allows polarity switching between positive and negative ion mode within a single LC run. Analysis of authentic standards was used to determine the optimal ionization mode for each metabolite.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For untargeted analysis, samples were analyzed in both negative and positive ion mode with liquid chromatography (LC) coupled by electrospray ionization to a 7-Tesla Fourier-transform ion cyclotron resonance mass spectrometer (FT-ICR MS). In parallel to the FT acquisition, four data dependent MS/MS scans were collected at nominal mass resolution in the ion trap (LTQ). Samples were analyzed in random order with a pooled sampled run every six samples in order to assess instrument variability.&amp;lt;/span&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;strong&amp;gt;Metabolite identification:&amp;lt;/strong&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;The targeted metabolomics compound identifications were based on measurements of authentic standards on the same mass spectrometer. Note that the LC/mass spectrometry system cannot distinguish between leucine and isoleucine, therefore the data are presented as 'leucine/isoleucine'.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;
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        <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/award/847419.rdf" xlink:title="GBMF3304" xlink:actuate="onRequest">Funding provided by Gordon and Betty Moore Foundation: Marine Microbiology Initiative (MMI) Award Number: GBMF3304 Award URL: https://www.moore.org/grant-detail?grantId=GBMF3304</gmx:Anchor>
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Individual investigator awards for current and emerging leaders in the field.
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Community resource efforts that fund the creation and sharing of data and the development of tools, methods and infrastructure of widespread utility.
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&amp;lt;div&amp;gt;&amp;lt;strong&amp;gt;Sample Collection:&amp;lt;/strong&amp;gt;&amp;lt;br /&amp;gt;
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&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;The intracellular metabolites were extracted using a method modified from a protocol previously described in Rabinowitz and Kimball (2007). Briefly, the filter was extracted three times with ice-cold extraction solvent (acetonitrile:methanol:water with 0.1 M formic acid, 40:40:20). The combined extracts were neutralized with ammonium hydroxide and dried in a vacufuge.&amp;lt;/span&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;The samples for the targeted mass spectrometry analysis were re-dissolved in 95:5 (v/v) water:acetonitrile and combined with deuterated biotin (final concentration 0.05 µg/ml)as an internal standard.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For untargeted analysis, the extracts had to undergo an additional de-salting step prior to analysis. Therefore, the dried extracts were re-dissolved in 0.01 M hydrochloric acid and extracted using a 50 mg/1 cc PPL cartridge following the protocol of Dittmar et al. (2008). The resulting methanol extracts were re-dissolved in 95:5 water:acetonitrile and deuterated biotin.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;strong&amp;gt;Chromatography:&amp;lt;/strong&amp;gt;&amp;lt;/p&amp;gt;
&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For targeted metabolomics analysis, the samples were analyzed with a Synergi 4 µm Fusion – RP 80 Å, 150 × 2.00 mm column (Phenomenex, Torrance, CA) coupled to a Thermo Scientific TSQ Vantage Triple Stage Quadrupole Mass Spectrometer. The chromatography gradient was: an initial hold of 95% A (0.1% formic acid in water) : 5% B (0.1% formic acid in acetonitrile) for 2 minutes, ramp to 65% B from 2 to 20 minutes, ramp to 100% B from 20 to 25 min, and hold until 32.5 minutes. The column was re-equilibrated for 7 min between samples with solvent A. Each metabolite was quantified using multiple reaction monitoring (MRM) mode with optimal parameters determined from infusion of authentic standards. Eight-point external calibration curves (0.5, 1, 5, 10, 50, 100, 250, and 500 ng/ml) were generated for each compound by plotting peak area against concentration.&amp;lt;/span&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For untargeted metabolomics analysis, LC separation was performed using a Synergi Fusion reversed phase column (Phenomenex, Torrance, CA) with the same gradient as for targeted analysis.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;strong&amp;gt;Mass spectroscopy:&amp;lt;/strong&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For targeted analysis, samples were analyzed with a Thermo Scientific TSQ Vantage Triple Stage Quadrupole Mass Spectrometer. This instrument allows polarity switching between positive and negative ion mode within a single LC run. Analysis of authentic standards was used to determine the optimal ionization mode for each metabolite.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;For untargeted analysis, samples were analyzed in both negative and positive ion mode with liquid chromatography (LC) coupled by electrospray ionization to a 7-Tesla Fourier-transform ion cyclotron resonance mass spectrometer (FT-ICR MS). In parallel to the FT acquisition, four data dependent MS/MS scans were collected at nominal mass resolution in the ion trap (LTQ). Samples were analyzed in random order with a pooled sampled run every six samples in order to assess instrument variability.&amp;lt;/span&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;strong&amp;gt;Metabolite identification:&amp;lt;/strong&amp;gt;&amp;lt;br /&amp;gt;
&amp;lt;br /&amp;gt;
&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;The targeted metabolomics compound identifications were based on measurements of authentic standards on the same mass spectrometer. Note that the LC/mass spectrometry system cannot distinguish between leucine and isoleucine, therefore the data are presented as 'leucine/isoleucine'.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;
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&amp;lt;p&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;Untargeted metabolomics data Data were collected as XCalibur RAW files which were converted to mzXML files using the msConvert tool within ProteoWizard (Chambers&amp;amp;nbsp; et al., 2012). Features were extracted from the LC-MS data using XCMS (Smith&amp;amp;nbsp; et al., 2006), where a feature is defined as a unique combination of a mass-to-charge (m/z) ratio and a retention time. Peak finding was performed with the centWave algorithm (Tautenhahn &amp;amp;nbsp;et al.,&amp;amp;nbsp;2008), and only peaks that fit a Gaussian shape were retained. Features were aligned across samples based on retention time and m/z value using the group.nearest function in XCMS; fillPeaks was used to reconsider features missed in the initial peak finding steps. CAMERA was used 1) to find compounds differing by adduct ion and stable isotope composition (Kuhl&amp;amp;nbsp;&amp;lt;/span&amp;gt;&amp;lt;span style=&amp;quot;color:rgb(74, 74, 74); font-family:blinkmacsystemfont,-apple-system,segoe ui,roboto,oxygen,ubuntu,cantarell,fira sans,droid sans,helvetica neue,helvetica,arial,sans-serif; font-size:16px&amp;quot;&amp;gt;et al.,&amp;amp;nbsp;2012) and 2) to extract the intensities and m/z values for the associated MS/MS spectra.&amp;lt;/span&amp;gt;&amp;lt;/p&amp;gt;</gco:CharacterString>
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