author_facet Mei, Henrik E.
Leipold, Michael D.
Maecker, Holden T.
Mei, Henrik E.
Leipold, Michael D.
Maecker, Holden T.
author Mei, Henrik E.
Leipold, Michael D.
Maecker, Holden T.
spellingShingle Mei, Henrik E.
Leipold, Michael D.
Maecker, Holden T.
Cytometry Part A
Platinum‐conjugated antibodies for application in mass cytometry
Cell Biology
Histology
Pathology and Forensic Medicine
author_sort mei, henrik e.
spelling Mei, Henrik E. Leipold, Michael D. Maecker, Holden T. 1552-4922 1552-4930 Wiley Cell Biology Histology Pathology and Forensic Medicine http://dx.doi.org/10.1002/cyto.a.22778 <jats:title>Abstract</jats:title><jats:p>Mass cytometry has overcome limitations of fluorescent single cell cytometry by allowing for the measurement of up to currently ∼40 different parameters on a single cell level. However, the cellular proteome comprises many more potential analytes, and current mass cytometry instrumentation allows for theoretically up to 121 different mass detection channels. The labeling of specific probes with appropriate metal ions is a significant hurdle for exploiting more of mass cytometry's analytical capacity. To this end, we here describe the labeling of antibody with natural abundance or isotopically purified platinum as formulated in cisplatin and circumventing the use of chelator‐loaded polymers. We confirm the utility of cisplatin–antibody‐conjugates for surface, intracellular, and phosphoepitope‐specific immunophenotyping, as well as for application in cell surface CD45‐based barcoding. Cisplatin‐labeling of antibody increases the analytical capacity of the CyTOF<jats:sup>®</jats:sup> platform by two channels based on available reagents, and has the potential to add a total of six channels for detection of specific probes, thus helping to better extend the analytical mass range of mass cytometers. © 2015 International Society for Advancement of Cytometry</jats:p> Platinum‐conjugated antibodies for application in mass cytometry Cytometry Part A
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series Cytometry Part A
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title Platinum‐conjugated antibodies for application in mass cytometry
title_unstemmed Platinum‐conjugated antibodies for application in mass cytometry
title_full Platinum‐conjugated antibodies for application in mass cytometry
title_fullStr Platinum‐conjugated antibodies for application in mass cytometry
title_full_unstemmed Platinum‐conjugated antibodies for application in mass cytometry
title_short Platinum‐conjugated antibodies for application in mass cytometry
title_sort platinum‐conjugated antibodies for application in mass cytometry
topic Cell Biology
Histology
Pathology and Forensic Medicine
url http://dx.doi.org/10.1002/cyto.a.22778
publishDate 2016
physical 292-300
description <jats:title>Abstract</jats:title><jats:p>Mass cytometry has overcome limitations of fluorescent single cell cytometry by allowing for the measurement of up to currently ∼40 different parameters on a single cell level. However, the cellular proteome comprises many more potential analytes, and current mass cytometry instrumentation allows for theoretically up to 121 different mass detection channels. The labeling of specific probes with appropriate metal ions is a significant hurdle for exploiting more of mass cytometry's analytical capacity. To this end, we here describe the labeling of antibody with natural abundance or isotopically purified platinum as formulated in cisplatin and circumventing the use of chelator‐loaded polymers. We confirm the utility of cisplatin–antibody‐conjugates for surface, intracellular, and phosphoepitope‐specific immunophenotyping, as well as for application in cell surface CD45‐based barcoding. Cisplatin‐labeling of antibody increases the analytical capacity of the CyTOF<jats:sup>®</jats:sup> platform by two channels based on available reagents, and has the potential to add a total of six channels for detection of specific probes, thus helping to better extend the analytical mass range of mass cytometers. © 2015 International Society for Advancement of Cytometry</jats:p>
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author Mei, Henrik E., Leipold, Michael D., Maecker, Holden T.
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author_sort mei, henrik e.
container_issue 3
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container_title Cytometry Part A
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description <jats:title>Abstract</jats:title><jats:p>Mass cytometry has overcome limitations of fluorescent single cell cytometry by allowing for the measurement of up to currently ∼40 different parameters on a single cell level. However, the cellular proteome comprises many more potential analytes, and current mass cytometry instrumentation allows for theoretically up to 121 different mass detection channels. The labeling of specific probes with appropriate metal ions is a significant hurdle for exploiting more of mass cytometry's analytical capacity. To this end, we here describe the labeling of antibody with natural abundance or isotopically purified platinum as formulated in cisplatin and circumventing the use of chelator‐loaded polymers. We confirm the utility of cisplatin–antibody‐conjugates for surface, intracellular, and phosphoepitope‐specific immunophenotyping, as well as for application in cell surface CD45‐based barcoding. Cisplatin‐labeling of antibody increases the analytical capacity of the CyTOF<jats:sup>®</jats:sup> platform by two channels based on available reagents, and has the potential to add a total of six channels for detection of specific probes, thus helping to better extend the analytical mass range of mass cytometers. © 2015 International Society for Advancement of Cytometry</jats:p>
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spelling Mei, Henrik E. Leipold, Michael D. Maecker, Holden T. 1552-4922 1552-4930 Wiley Cell Biology Histology Pathology and Forensic Medicine http://dx.doi.org/10.1002/cyto.a.22778 <jats:title>Abstract</jats:title><jats:p>Mass cytometry has overcome limitations of fluorescent single cell cytometry by allowing for the measurement of up to currently ∼40 different parameters on a single cell level. However, the cellular proteome comprises many more potential analytes, and current mass cytometry instrumentation allows for theoretically up to 121 different mass detection channels. The labeling of specific probes with appropriate metal ions is a significant hurdle for exploiting more of mass cytometry's analytical capacity. To this end, we here describe the labeling of antibody with natural abundance or isotopically purified platinum as formulated in cisplatin and circumventing the use of chelator‐loaded polymers. We confirm the utility of cisplatin–antibody‐conjugates for surface, intracellular, and phosphoepitope‐specific immunophenotyping, as well as for application in cell surface CD45‐based barcoding. Cisplatin‐labeling of antibody increases the analytical capacity of the CyTOF<jats:sup>®</jats:sup> platform by two channels based on available reagents, and has the potential to add a total of six channels for detection of specific probes, thus helping to better extend the analytical mass range of mass cytometers. © 2015 International Society for Advancement of Cytometry</jats:p> Platinum‐conjugated antibodies for application in mass cytometry Cytometry Part A
spellingShingle Mei, Henrik E., Leipold, Michael D., Maecker, Holden T., Cytometry Part A, Platinum‐conjugated antibodies for application in mass cytometry, Cell Biology, Histology, Pathology and Forensic Medicine
title Platinum‐conjugated antibodies for application in mass cytometry
title_full Platinum‐conjugated antibodies for application in mass cytometry
title_fullStr Platinum‐conjugated antibodies for application in mass cytometry
title_full_unstemmed Platinum‐conjugated antibodies for application in mass cytometry
title_short Platinum‐conjugated antibodies for application in mass cytometry
title_sort platinum‐conjugated antibodies for application in mass cytometry
title_unstemmed Platinum‐conjugated antibodies for application in mass cytometry
topic Cell Biology, Histology, Pathology and Forensic Medicine
url http://dx.doi.org/10.1002/cyto.a.22778