Nonspecific Binding Correction for Single-Cell Mass Cytometric Analysis of Autophagy and Myoblast Differentiation

Satellite cells provide regenerative capacity to the skeletal muscle after injury. In this process, termed myogenesis, satellite cells get activated, proliferate, and differentiate. Myogenesis is recapitulated in the tissue culture of myoblasts that differentiate by fusion and then by the formation...

Ausführliche Beschreibung

Gespeichert in:

Bibliographische Detailangaben
Veröffentlicht in:	Analytical chemistry (Washington) 2021-01, Vol.93 (3), p.1401-1408
Hauptverfasser:	Brown, Heather M. G, Kuhns, Michelle M, Maxwell, Zoe, Arriaga, Edgar A
Format:	Artikel
Sprache:	eng
Schlagworte:	Analytical chemistry Animals Antibodies Autophagy Binding Cell culture Cell Differentiation Cells (biology) Cells, Cultured Chemistry Cytometry Differentiation Flow Cytometry Fluctuations Flux Isotypes Mass Spectrometry Mice Microscopy, Fluorescence Mitochondria Muscles Musculoskeletal system Myoblasts Myoblasts - pathology Myogenesis Myotubes Phagocytosis Rats Satellite cells Single-Cell Analysis Skeletal muscle Tissue culture
Online-Zugang:	Volltext
Tags:	Tag hinzufügen Keine Tags, Fügen Sie den ersten Tag hinzu!

container_end_page	1408
container_issue	3
container_start_page	1401
container_title	Analytical chemistry (Washington)
container_volume	93
creator	Brown, Heather M. G Kuhns, Michelle M Maxwell, Zoe Arriaga, Edgar A
description	Satellite cells provide regenerative capacity to the skeletal muscle after injury. In this process, termed myogenesis, satellite cells get activated, proliferate, and differentiate. Myogenesis is recapitulated in the tissue culture of myoblasts that differentiate by fusion and then by the formation of myotubes. Autophagy plays an important role in myogenesis, but the asynchronous and unique trajectory of differentiation of each myoblast along the myogenic lineage complicates teasing apart at what stages of differentiation autophagy plays a critical role. In this report, we describe a mass cytometric, multidimensional, individual cell analysis of differentiating myoblasts that characterizes autophagy flux (i.e., autophagy rate) at separate myogenesis stages. Because mass cytometry uses a set of lanthanide-tagged antibodies, each being specific for a desired molecular target, quantification of each molecular target could be exaggerated by nonspecific binding of its respective antibody to other nontarget cellular regions. In this report, we used lanthanide-tagged isotypes, which allowed for correction for nonspecific binding at the single-cell level. Using this approach, myoblasts were phenotypically identified by their position in the myogenic lineage, simultaneously with the quantification of autophagic flux in each identified subset. We found that generally autophagy flux is upregulated specifically during myoblast fusion and declines in myotubes. We also observed that mitophagy (i.e., selective autophagic degradation of mitochondria) is also active after myotube formation. The ability to track different types of autophagy is another feature of this methodology, which could be key to expand the current understanding of autophagy regulation in regenerating the skeletal muscle.
doi_str_mv	10.1021/acs.analchem.0c03211
format	Article
fullrecord	<record><control><sourceid>proquest_cross</sourceid><recordid>TN_cdi_proquest_miscellaneous_2472107287</recordid><sourceformat>XML</sourceformat><sourcesystem>PC</sourcesystem><sourcerecordid>2472107287</sourcerecordid><originalsourceid>FETCH-LOGICAL-a422t-c45a801bb7bff960ef934216a7e3a016198ca39b27d3a218274cd731764af32a3</originalsourceid><addsrcrecordid>eNp9kU1P3DAURS3Uqkyh_wBVlrrpJtPnj4md5TS0UAnaBe06enFsMEriwU4W-ff1aAYWLFhZss699tUh5ILBmgFn39CkNY7Ymwc7rMGA4IydkBXbcChKrfk7sgIAUXAFcEo-pvQIwBiw8gM5FUJIXSm9Ik-_w5h21njnDf3ux86P97QOMVoz-TBSFyK9y3e9LWrb9_QWU6L1MoXBTjFHtvkHS_KJBke38xR2D3i_UBw7eruEtsc00UvvnI12nDzuK8_Je4d9sp-O5xn59_PH3_q6uPlz9ave3hQoOZ8KIzeogbWtap2rSrCuEpKzEpUVmFewShsUVctVJ5AzzZU0nRJMlRKd4CjOyNdD7y6Gp9mmqRl8MnkDjjbMqeFScQaKa5XRL6_QxzDHvGxPaVFKJvgmU_JAmRhSitY1u-gHjEvDoNkrabKS5llJc1SSY5-P5XM72O4l9OwgA3AA9vGXh9_s_A-xeJsL</addsrcrecordid><sourcetype>Aggregation Database</sourcetype><iscdi>true</iscdi><recordtype>article</recordtype><pqid>2483641325</pqid></control><display><type>article</type><title>Nonspecific Binding Correction for Single-Cell Mass Cytometric Analysis of Autophagy and Myoblast Differentiation</title><source>MEDLINE</source><source>ACS Publications</source><creator>Brown, Heather M. G ; Kuhns, Michelle M ; Maxwell, Zoe ; Arriaga, Edgar A</creator><creatorcontrib>Brown, Heather M. G ; Kuhns, Michelle M ; Maxwell, Zoe ; Arriaga, Edgar A</creatorcontrib><description>Satellite cells provide regenerative capacity to the skeletal muscle after injury. In this process, termed myogenesis, satellite cells get activated, proliferate, and differentiate. Myogenesis is recapitulated in the tissue culture of myoblasts that differentiate by fusion and then by the formation of myotubes. Autophagy plays an important role in myogenesis, but the asynchronous and unique trajectory of differentiation of each myoblast along the myogenic lineage complicates teasing apart at what stages of differentiation autophagy plays a critical role. In this report, we describe a mass cytometric, multidimensional, individual cell analysis of differentiating myoblasts that characterizes autophagy flux (i.e., autophagy rate) at separate myogenesis stages. Because mass cytometry uses a set of lanthanide-tagged antibodies, each being specific for a desired molecular target, quantification of each molecular target could be exaggerated by nonspecific binding of its respective antibody to other nontarget cellular regions. In this report, we used lanthanide-tagged isotypes, which allowed for correction for nonspecific binding at the single-cell level. Using this approach, myoblasts were phenotypically identified by their position in the myogenic lineage, simultaneously with the quantification of autophagic flux in each identified subset. We found that generally autophagy flux is upregulated specifically during myoblast fusion and declines in myotubes. We also observed that mitophagy (i.e., selective autophagic degradation of mitochondria) is also active after myotube formation. The ability to track different types of autophagy is another feature of this methodology, which could be key to expand the current understanding of autophagy regulation in regenerating the skeletal muscle.</description><identifier>ISSN: 0003-2700</identifier><identifier>EISSN: 1520-6882</identifier><identifier>DOI: 10.1021/acs.analchem.0c03211</identifier><identifier>PMID: 33348978</identifier><language>eng</language><publisher>United States: American Chemical Society</publisher><subject>Analytical chemistry ; Animals ; Antibodies ; Autophagy ; Binding ; Cell culture ; Cell Differentiation ; Cells (biology) ; Cells, Cultured ; Chemistry ; Cytometry ; Differentiation ; Flow Cytometry ; Fluctuations ; Flux ; Isotypes ; Mass Spectrometry ; Mice ; Microscopy, Fluorescence ; Mitochondria ; Muscles ; Musculoskeletal system ; Myoblasts ; Myoblasts - pathology ; Myogenesis ; Myotubes ; Phagocytosis ; Rats ; Satellite cells ; Single-Cell Analysis ; Skeletal muscle ; Tissue culture</subject><ispartof>Analytical chemistry (Washington), 2021-01, Vol.93 (3), p.1401-1408</ispartof><rights>2020 American Chemical Society</rights><rights>Copyright American Chemical Society Jan 26, 2021</rights><lds50>peer_reviewed</lds50><oa>free_for_read</oa><woscitedreferencessubscribed>false</woscitedreferencessubscribed><citedby>FETCH-LOGICAL-a422t-c45a801bb7bff960ef934216a7e3a016198ca39b27d3a218274cd731764af32a3</citedby><cites>FETCH-LOGICAL-a422t-c45a801bb7bff960ef934216a7e3a016198ca39b27d3a218274cd731764af32a3</cites><orcidid>0000-0001-8863-6174</orcidid></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Tsyndetics_thumb_exl</thumbnail><linktopdf>$$Uhttps://pubs.acs.org/doi/pdf/10.1021/acs.analchem.0c03211$$EPDF$$P50$$Gacs$$H</linktopdf><linktohtml>$$Uhttps://pubs.acs.org/doi/10.1021/acs.analchem.0c03211$$EHTML$$P50$$Gacs$$H</linktohtml><link.rule.ids>314,780,784,2765,27076,27924,27925,56738,56788</link.rule.ids><backlink>$$Uhttps://www.ncbi.nlm.nih.gov/pubmed/33348978$$D View this record in MEDLINE/PubMed$$Hfree_for_read</backlink></links><search><creatorcontrib>Brown, Heather M. G</creatorcontrib><creatorcontrib>Kuhns, Michelle M</creatorcontrib><creatorcontrib>Maxwell, Zoe</creatorcontrib><creatorcontrib>Arriaga, Edgar A</creatorcontrib><title>Nonspecific Binding Correction for Single-Cell Mass Cytometric Analysis of Autophagy and Myoblast Differentiation</title><title>Analytical chemistry (Washington)</title><addtitle>Anal. Chem</addtitle><description>Satellite cells provide regenerative capacity to the skeletal muscle after injury. In this process, termed myogenesis, satellite cells get activated, proliferate, and differentiate. Myogenesis is recapitulated in the tissue culture of myoblasts that differentiate by fusion and then by the formation of myotubes. Autophagy plays an important role in myogenesis, but the asynchronous and unique trajectory of differentiation of each myoblast along the myogenic lineage complicates teasing apart at what stages of differentiation autophagy plays a critical role. In this report, we describe a mass cytometric, multidimensional, individual cell analysis of differentiating myoblasts that characterizes autophagy flux (i.e., autophagy rate) at separate myogenesis stages. Because mass cytometry uses a set of lanthanide-tagged antibodies, each being specific for a desired molecular target, quantification of each molecular target could be exaggerated by nonspecific binding of its respective antibody to other nontarget cellular regions. In this report, we used lanthanide-tagged isotypes, which allowed for correction for nonspecific binding at the single-cell level. Using this approach, myoblasts were phenotypically identified by their position in the myogenic lineage, simultaneously with the quantification of autophagic flux in each identified subset. We found that generally autophagy flux is upregulated specifically during myoblast fusion and declines in myotubes. We also observed that mitophagy (i.e., selective autophagic degradation of mitochondria) is also active after myotube formation. The ability to track different types of autophagy is another feature of this methodology, which could be key to expand the current understanding of autophagy regulation in regenerating the skeletal muscle.</description><subject>Analytical chemistry</subject><subject>Animals</subject><subject>Antibodies</subject><subject>Autophagy</subject><subject>Binding</subject><subject>Cell culture</subject><subject>Cell Differentiation</subject><subject>Cells (biology)</subject><subject>Cells, Cultured</subject><subject>Chemistry</subject><subject>Cytometry</subject><subject>Differentiation</subject><subject>Flow Cytometry</subject><subject>Fluctuations</subject><subject>Flux</subject><subject>Isotypes</subject><subject>Mass Spectrometry</subject><subject>Mice</subject><subject>Microscopy, Fluorescence</subject><subject>Mitochondria</subject><subject>Muscles</subject><subject>Musculoskeletal system</subject><subject>Myoblasts</subject><subject>Myoblasts - pathology</subject><subject>Myogenesis</subject><subject>Myotubes</subject><subject>Phagocytosis</subject><subject>Rats</subject><subject>Satellite cells</subject><subject>Single-Cell Analysis</subject><subject>Skeletal muscle</subject><subject>Tissue culture</subject><issn>0003-2700</issn><issn>1520-6882</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2021</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNp9kU1P3DAURS3Uqkyh_wBVlrrpJtPnj4md5TS0UAnaBe06enFsMEriwU4W-ff1aAYWLFhZss699tUh5ILBmgFn39CkNY7Ymwc7rMGA4IydkBXbcChKrfk7sgIAUXAFcEo-pvQIwBiw8gM5FUJIXSm9Ik-_w5h21njnDf3ux86P97QOMVoz-TBSFyK9y3e9LWrb9_QWU6L1MoXBTjFHtvkHS_KJBke38xR2D3i_UBw7eruEtsc00UvvnI12nDzuK8_Je4d9sp-O5xn59_PH3_q6uPlz9ave3hQoOZ8KIzeogbWtap2rSrCuEpKzEpUVmFewShsUVctVJ5AzzZU0nRJMlRKd4CjOyNdD7y6Gp9mmqRl8MnkDjjbMqeFScQaKa5XRL6_QxzDHvGxPaVFKJvgmU_JAmRhSitY1u-gHjEvDoNkrabKS5llJc1SSY5-P5XM72O4l9OwgA3AA9vGXh9_s_A-xeJsL</recordid><startdate>20210126</startdate><enddate>20210126</enddate><creator>Brown, Heather M. G</creator><creator>Kuhns, Michelle M</creator><creator>Maxwell, Zoe</creator><creator>Arriaga, Edgar A</creator><general>American Chemical Society</general><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>7QF</scope><scope>7QO</scope><scope>7QQ</scope><scope>7SC</scope><scope>7SE</scope><scope>7SP</scope><scope>7SR</scope><scope>7TA</scope><scope>7TB</scope><scope>7TM</scope><scope>7U5</scope><scope>7U7</scope><scope>7U9</scope><scope>8BQ</scope><scope>8FD</scope><scope>C1K</scope><scope>F28</scope><scope>FR3</scope><scope>H8D</scope><scope>H8G</scope><scope>H94</scope><scope>JG9</scope><scope>JQ2</scope><scope>KR7</scope><scope>L7M</scope><scope>L~C</scope><scope>L~D</scope><scope>P64</scope><scope>7X8</scope><orcidid>https://orcid.org/0000-0001-8863-6174</orcidid></search><sort><creationdate>20210126</creationdate><title>Nonspecific Binding Correction for Single-Cell Mass Cytometric Analysis of Autophagy and Myoblast Differentiation</title><author>Brown, Heather M. G ; Kuhns, Michelle M ; Maxwell, Zoe ; Arriaga, Edgar A</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-a422t-c45a801bb7bff960ef934216a7e3a016198ca39b27d3a218274cd731764af32a3</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2021</creationdate><topic>Analytical chemistry</topic><topic>Animals</topic><topic>Antibodies</topic><topic>Autophagy</topic><topic>Binding</topic><topic>Cell culture</topic><topic>Cell Differentiation</topic><topic>Cells (biology)</topic><topic>Cells, Cultured</topic><topic>Chemistry</topic><topic>Cytometry</topic><topic>Differentiation</topic><topic>Flow Cytometry</topic><topic>Fluctuations</topic><topic>Flux</topic><topic>Isotypes</topic><topic>Mass Spectrometry</topic><topic>Mice</topic><topic>Microscopy, Fluorescence</topic><topic>Mitochondria</topic><topic>Muscles</topic><topic>Musculoskeletal system</topic><topic>Myoblasts</topic><topic>Myoblasts - pathology</topic><topic>Myogenesis</topic><topic>Myotubes</topic><topic>Phagocytosis</topic><topic>Rats</topic><topic>Satellite cells</topic><topic>Single-Cell Analysis</topic><topic>Skeletal muscle</topic><topic>Tissue culture</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Brown, Heather M. G</creatorcontrib><creatorcontrib>Kuhns, Michelle M</creatorcontrib><creatorcontrib>Maxwell, Zoe</creatorcontrib><creatorcontrib>Arriaga, Edgar A</creatorcontrib><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>CrossRef</collection><collection>Aluminium Industry Abstracts</collection><collection>Biotechnology Research Abstracts</collection><collection>Ceramic Abstracts</collection><collection>Computer and Information Systems Abstracts</collection><collection>Corrosion Abstracts</collection><collection>Electronics & Communications Abstracts</collection><collection>Engineered Materials Abstracts</collection><collection>Materials Business File</collection><collection>Mechanical & Transportation Engineering Abstracts</collection><collection>Nucleic Acids Abstracts</collection><collection>Solid State and Superconductivity Abstracts</collection><collection>Toxicology Abstracts</collection><collection>Virology and AIDS Abstracts</collection><collection>METADEX</collection><collection>Technology Research Database</collection><collection>Environmental Sciences and Pollution Management</collection><collection>ANTE: Abstracts in New Technology & Engineering</collection><collection>Engineering Research Database</collection><collection>Aerospace Database</collection><collection>Copper Technical Reference Library</collection><collection>AIDS and Cancer Research Abstracts</collection><collection>Materials Research Database</collection><collection>ProQuest Computer Science Collection</collection><collection>Civil Engineering Abstracts</collection><collection>Advanced Technologies Database with Aerospace</collection><collection>Computer and Information Systems Abstracts Academic</collection><collection>Computer and Information Systems Abstracts Professional</collection><collection>Biotechnology and BioEngineering Abstracts</collection><collection>MEDLINE - Academic</collection><jtitle>Analytical chemistry (Washington)</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Brown, Heather M. G</au><au>Kuhns, Michelle M</au><au>Maxwell, Zoe</au><au>Arriaga, Edgar A</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Nonspecific Binding Correction for Single-Cell Mass Cytometric Analysis of Autophagy and Myoblast Differentiation</atitle><jtitle>Analytical chemistry (Washington)</jtitle><addtitle>Anal. Chem</addtitle><date>2021-01-26</date><risdate>2021</risdate><volume>93</volume><issue>3</issue><spage>1401</spage><epage>1408</epage><pages>1401-1408</pages><issn>0003-2700</issn><eissn>1520-6882</eissn><abstract>Satellite cells provide regenerative capacity to the skeletal muscle after injury. In this process, termed myogenesis, satellite cells get activated, proliferate, and differentiate. Myogenesis is recapitulated in the tissue culture of myoblasts that differentiate by fusion and then by the formation of myotubes. Autophagy plays an important role in myogenesis, but the asynchronous and unique trajectory of differentiation of each myoblast along the myogenic lineage complicates teasing apart at what stages of differentiation autophagy plays a critical role. In this report, we describe a mass cytometric, multidimensional, individual cell analysis of differentiating myoblasts that characterizes autophagy flux (i.e., autophagy rate) at separate myogenesis stages. Because mass cytometry uses a set of lanthanide-tagged antibodies, each being specific for a desired molecular target, quantification of each molecular target could be exaggerated by nonspecific binding of its respective antibody to other nontarget cellular regions. In this report, we used lanthanide-tagged isotypes, which allowed for correction for nonspecific binding at the single-cell level. Using this approach, myoblasts were phenotypically identified by their position in the myogenic lineage, simultaneously with the quantification of autophagic flux in each identified subset. We found that generally autophagy flux is upregulated specifically during myoblast fusion and declines in myotubes. We also observed that mitophagy (i.e., selective autophagic degradation of mitochondria) is also active after myotube formation. The ability to track different types of autophagy is another feature of this methodology, which could be key to expand the current understanding of autophagy regulation in regenerating the skeletal muscle.</abstract><cop>United States</cop><pub>American Chemical Society</pub><pmid>33348978</pmid><doi>10.1021/acs.analchem.0c03211</doi><tpages>8</tpages><orcidid>https://orcid.org/0000-0001-8863-6174</orcidid><oa>free_for_read</oa></addata></record>
fulltext	fulltext
identifier	ISSN: 0003-2700
ispartof	Analytical chemistry (Washington), 2021-01, Vol.93 (3), p.1401-1408
issn	0003-2700 1520-6882
language	eng
recordid	cdi_proquest_miscellaneous_2472107287
source	MEDLINE; ACS Publications
subjects	Analytical chemistry Animals Antibodies Autophagy Binding Cell culture Cell Differentiation Cells (biology) Cells, Cultured Chemistry Cytometry Differentiation Flow Cytometry Fluctuations Flux Isotypes Mass Spectrometry Mice Microscopy, Fluorescence Mitochondria Muscles Musculoskeletal system Myoblasts Myoblasts - pathology Myogenesis Myotubes Phagocytosis Rats Satellite cells Single-Cell Analysis Skeletal muscle Tissue culture
title	Nonspecific Binding Correction for Single-Cell Mass Cytometric Analysis of Autophagy and Myoblast Differentiation
url	https://sfx.bib-bvb.de/sfx_tum?ctx_ver=Z39.88-2004&ctx_enc=info:ofi/enc:UTF-8&ctx_tim=2025-01-07T09%3A42%3A25IST&url_ver=Z39.88-2004&url_ctx_fmt=infofi/fmt:kev:mtx:ctx&rfr_id=info:sid/primo.exlibrisgroup.com:primo3-Article-proquest_cross&rft_val_fmt=info:ofi/fmt:kev:mtx:journal&rft.genre=article&rft.atitle=Nonspecific%20Binding%20Correction%20for%20Single-Cell%20Mass%20Cytometric%20Analysis%20of%20Autophagy%20and%20Myoblast%20Differentiation&rft.jtitle=Analytical%20chemistry%20(Washington)&rft.au=Brown,%20Heather%20M.%20G&rft.date=2021-01-26&rft.volume=93&rft.issue=3&rft.spage=1401&rft.epage=1408&rft.pages=1401-1408&rft.issn=0003-2700&rft.eissn=1520-6882&rft_id=info:doi/10.1021/acs.analchem.0c03211&rft_dat=%3Cproquest_cross%3E2472107287%3C/proquest_cross%3E%3Curl%3E%3C/url%3E&disable_directlink=true&sfx.directlink=off&sfx.report_link=0&rft_id=info:oai/&rft_pqid=2483641325&rft_id=info:pmid/33348978&rfr_iscdi=true