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            <title xml:lang="en">Proteotyping SARS-CoV-2 Virus from Nasopharyngeal Swabs: A Proof-of-Concept Focused on a 3 Min Mass Spectrometry Window</title>
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                <forename type="first">Duarte</forename>
                <surname>Gouveia</surname>
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              <email type="domain">evotec.com</email>
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                <forename type="first">Guylaine</forename>
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              <date type="whenSubmitted">2021-09-14 09:37:44</date>
              <date type="whenModified">2026-02-26 12:16:07</date>
              <date type="whenReleased">2021-09-14 09:37:44</date>
              <date type="whenProduced">2020-11-06</date>
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            <idno type="halRefHtml">&lt;i&gt;Journal of Proteome Research&lt;/i&gt;, 2020, 19 (11), pp.4407-4416. &lt;a target="_blank" href="https://dx.doi.org/10.1021/acs.jproteome.0c00535"&gt;&amp;#x27E8;10.1021/acs.jproteome.0c00535&amp;#x27E9;&lt;/a&gt;</idno>
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            <idno type="stamp" n="INSERM">INSERM - Institut national de la santé et de la recherche médicale</idno>
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            <idno type="stamp" n="CEA-UPSAY" corresp="CEA">CEA - Université Paris-Saclay</idno>
            <idno type="stamp" n="UNIV-PARIS-SACLAY">Université Paris-Saclay</idno>
            <idno type="stamp" n="BS">Biologie-Santé</idno>
            <idno type="stamp" n="UNIV-MONTPELLIER">Université de Montpellier</idno>
            <idno type="stamp" n="JOLIOT" corresp="CEA">Institut des Sciences du Vivant Frédéric JOLIOT</idno>
            <idno type="stamp" n="CEA-DRF" corresp="CEA">Direction de Recherche Fondamentale</idno>
            <idno type="stamp" n="DMTS" corresp="JOLIOT">Département Médicaments et Technologies pour la Santé</idno>
            <idno type="stamp" n="INRAE">Institut National de Recherche en Agriculture, Alimentation et Environnement</idno>
            <idno type="stamp" n="UNIVERSITE-PARIS-SACLAY" corresp="UNIV-PARIS-SACLAY">Université Paris-Saclay</idno>
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            <idno type="stamp" n="UM-2015-2021" corresp="UNIV-MONTPELLIER">Université de Montpellier (2015-2021)</idno>
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                <title xml:lang="en">Proteotyping SARS-CoV-2 Virus from Nasopharyngeal Swabs: A Proof-of-Concept Focused on a 3 Min Mass Spectrometry Window</title>
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                    <forename type="first">Albert</forename>
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                    <forename type="first">J.</forename>
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                <idno type="issn">1535-3893</idno>
                <idno type="eissn">1535-3907</idno>
                <title level="j">Journal of Proteome Research</title>
                <imprint>
                  <publisher>American Chemical Society</publisher>
                  <biblScope unit="volume">19</biblScope>
                  <biblScope unit="issue">11</biblScope>
                  <biblScope unit="pp">4407-4416</biblScope>
                  <date type="datePub">2020-11-06</date>
                </imprint>
              </monogr>
              <idno type="doi">10.1021/acs.jproteome.0c00535</idno>
              <idno type="pubmed">32697082</idno>
              <idno type="pubmedcentral">PMC7640971</idno>
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            <textClass>
              <keywords scheme="author">
                <term xml:lang="en">COVID-19</term>
                <term xml:lang="en">SARS-CoV-2</term>
                <term xml:lang="en">Nasopharyngeal swab</term>
                <term xml:lang="en">Mass spectrometry</term>
                <term xml:lang="en">Peptides</term>
                <term xml:lang="en">Proteomics</term>
                <term xml:lang="en">Viral protein detection</term>
              </keywords>
              <classCode scheme="mesh">Betacoronavirus / chemistry</classCode>
              <classCode scheme="mesh">Chromatography, Liquid</classCode>
              <classCode scheme="mesh">Phosphoproteins</classCode>
              <classCode scheme="mesh">Pneumonia, Viral* / diagnosis</classCode>
              <classCode scheme="mesh">Pneumonia, Viral* / virology</classCode>
              <classCode scheme="mesh">Tandem Mass Spectrometry / methods</classCode>
              <classCode scheme="mesh">Clinical Laboratory Techniques / methods</classCode>
              <classCode scheme="mesh">Coronavirus Infections* / diagnosis</classCode>
              <classCode scheme="mesh">Coronavirus Infections* / virology</classCode>
              <classCode scheme="mesh">Coronavirus Nucleocapsid Proteins</classCode>
              <classCode scheme="mesh">Nasopharynx / virology</classCode>
              <classCode scheme="mesh">Pandemics</classCode>
              <classCode scheme="halDomain" n="sdv.bbm">Life Sciences [q-bio]/Biochemistry, Molecular Biology</classCode>
              <classCode scheme="halDomain" n="sdv.mhep.mi">Life Sciences [q-bio]/Human health and pathology/Infectious diseases</classCode>
              <classCode scheme="halDomain" n="sdv.mhep.me">Life Sciences [q-bio]/Human health and pathology/Emerging diseases</classCode>
              <classCode scheme="halDomain" n="sdv.spee">Life Sciences [q-bio]/Santé publique et épidémiologie</classCode>
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            <abstract xml:lang="en">
              <p>Rapid but yet sensitive, specific, and high-throughput detection of the severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) in clinical samples is key to diagnose infected people and to better control the spread of the virus. Alternative methodologies to PCR and immunodiagnostics that would not require specific reagents are worthy to investigate not only for fighting the COVID-19 pandemic but also to detect other emergent pathogenic threats. Here, we propose the use of tandem mass spectrometry to detect SARS-CoV-2 marker peptides in nasopharyngeal swabs. We documented that the signal from the microbiota present in such samples is low and can be overlooked when interpreting shotgun proteomic data acquired on a restricted window of the peptidome landscape. In this proof-of-concept study, simili nasopharyngeal swabs spiked with different quantities of purified SARS-CoV-2 viral material were used to develop a nanoLC-MS/MS acquisition method, which was then successfully applied on COVID-19 clinical samples. We argue that peptides ADETQALPQR and GFYAQGSR from the nucleocapsid protein are of utmost interest as their signal is intense and their elution can be obtained within a 3 min window in the tested conditions. These results pave the way for the development of time-efficient viral diagnostic tests based on mass spectrometry.</p>
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          <orgName>Médicaments et Technologies pour la Santé</orgName>
          <orgName type="acronym">MTS</orgName>
          <date type="start">2020-01-01</date>
          <desc>
            <address>
              <addrLine>CEA- SPI- Bât. 136 Saclay 91191 GIF-SUR-YVETTE</addrLine>
              <country key="FR"/>
            </address>
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