High-Throughput Quantification of GFP-LC3 + Dots by Automated Fluorescence Microscopy
Macroautophagy is a specific variant of autophagy that involves a dedicated double-membraned organelle commonly known as autophagosome. Various methods have been developed to quantify the size of the autophagosomal compartment, which is an indirect indicator of macroautophagic responses, based on th...
Gespeichert in:
| Veröffentlicht in: | Methods in enzymology 2017, Vol.587, p.71-86 |
|---|---|
| Hauptverfasser: | , , , , , , , , |
| Format: | Artikel |
| Sprache: | eng |
| Schlagworte: | |
| Online-Zugang: | Volltext |
| Tags: |
Tag hinzufügen
Keine Tags, Fügen Sie den ersten Tag hinzu!
|
| container_end_page | 86 |
|---|---|
| container_issue | |
| container_start_page | 71 |
| container_title | Methods in enzymology |
| container_volume | 587 |
| creator | Bravo-San Pedro, J M Pietrocola, F Sica, V Izzo, V Sauvat, A Kepp, O Maiuri, M C Kroemer, G Galluzzi, L |
| description | Macroautophagy is a specific variant of autophagy that involves a dedicated double-membraned organelle commonly known as autophagosome. Various methods have been developed to quantify the size of the autophagosomal compartment, which is an indirect indicator of macroautophagic responses, based on the peculiar ability of microtubule-associated protein 1 light chain 3 beta (MAP1LC3B; best known as LC3) to accumulate in forming autophagosomes upon maturation. One particularly convenient method to monitor the accumulation of mature LC3 within autophagosomes relies on a green fluorescent protein (GFP)-tagged variant of this protein and fluorescence microscopy. In physiological conditions, cells transfected temporarily or stably with a GFP-LC3-encoding construct exhibit a diffuse green fluorescence over the cytoplasm and nucleus. Conversely, in response to macroautophagy-promoting stimuli, the GFP-LC3 signal becomes punctate and often (but not always) predominantly cytoplasmic. The accumulation of GFP-LC3 in cytoplasmic dots, however, also ensues the blockage of any of the steps that ensure the degradation of mature autophagosomes, calling for the implementation of strategies that accurately discriminate between an increase in autophagic flux and an arrest in autophagic degradation. Various cell lines have been engineered to stably express GFP-LC3, which-combined with the appropriate controls of flux, high-throughput imaging stations, and automated image analysis-offer a relatively straightforward tool to screen large chemical or biological libraries for inducers or inhibitors of autophagy. Here, we describe a simple and robust method for the high-throughput quantification of GFP-LC3
dots by automated fluorescence microscopy. |
| doi_str_mv | 10.1016/bs.mie.2016.10.022 |
| format | Article |
| fullrecord | <record><control><sourceid>proquest_pubme</sourceid><recordid>TN_cdi_proquest_miscellaneous_1874445105</recordid><sourceformat>XML</sourceformat><sourcesystem>PC</sourcesystem><sourcerecordid>1874445105</sourcerecordid><originalsourceid>FETCH-LOGICAL-c326t-948fedc840ca2d8e1603f3a68085db64d78bff0023ce2205539a4f94c0fde72a3</originalsourceid><addsrcrecordid>eNo1kE9LwzAAxYMgbk6_gAfJUZDW_G3S45huEyYqbOeSpskWaZvaJId9ewvq6T0ej8ePB8AdRjlGuHiqQ945k5PJT0GOCLkAc8y5yEQp5Qxch_CFEBGyxFdgRiThtBRiDg5bdzxl-9Po0_E0pAg_k-qjs06r6HwPvYWb9Ue2W1H4CJ99DLA-w2WKvlPRNHDdJj-aoE2vDXxzevRB--F8Ay6taoO5_dMFOKxf9qtttnvfvK6Wu0xTUsSsZNKaRkuGtCKNNLhA1FJVSCR5UxesEbK2dsKm2hCC-MSsmC2ZRrYxgii6AA-_u8Pov5MJsercBNO2qjc-hQpLwRjjGPGpev9XTXVnmmoYXafGc_V_Bf0BYwZfHA</addsrcrecordid><sourcetype>Aggregation Database</sourcetype><iscdi>true</iscdi><recordtype>article</recordtype><pqid>1874445105</pqid></control><display><type>article</type><title>High-Throughput Quantification of GFP-LC3 + Dots by Automated Fluorescence Microscopy</title><source>MEDLINE</source><source>Elsevier ScienceDirect Journals</source><creator>Bravo-San Pedro, J M ; Pietrocola, F ; Sica, V ; Izzo, V ; Sauvat, A ; Kepp, O ; Maiuri, M C ; Kroemer, G ; Galluzzi, L</creator><creatorcontrib>Bravo-San Pedro, J M ; Pietrocola, F ; Sica, V ; Izzo, V ; Sauvat, A ; Kepp, O ; Maiuri, M C ; Kroemer, G ; Galluzzi, L</creatorcontrib><description>Macroautophagy is a specific variant of autophagy that involves a dedicated double-membraned organelle commonly known as autophagosome. Various methods have been developed to quantify the size of the autophagosomal compartment, which is an indirect indicator of macroautophagic responses, based on the peculiar ability of microtubule-associated protein 1 light chain 3 beta (MAP1LC3B; best known as LC3) to accumulate in forming autophagosomes upon maturation. One particularly convenient method to monitor the accumulation of mature LC3 within autophagosomes relies on a green fluorescent protein (GFP)-tagged variant of this protein and fluorescence microscopy. In physiological conditions, cells transfected temporarily or stably with a GFP-LC3-encoding construct exhibit a diffuse green fluorescence over the cytoplasm and nucleus. Conversely, in response to macroautophagy-promoting stimuli, the GFP-LC3 signal becomes punctate and often (but not always) predominantly cytoplasmic. The accumulation of GFP-LC3 in cytoplasmic dots, however, also ensues the blockage of any of the steps that ensure the degradation of mature autophagosomes, calling for the implementation of strategies that accurately discriminate between an increase in autophagic flux and an arrest in autophagic degradation. Various cell lines have been engineered to stably express GFP-LC3, which-combined with the appropriate controls of flux, high-throughput imaging stations, and automated image analysis-offer a relatively straightforward tool to screen large chemical or biological libraries for inducers or inhibitors of autophagy. Here, we describe a simple and robust method for the high-throughput quantification of GFP-LC3
dots by automated fluorescence microscopy.</description><identifier>EISSN: 1557-7988</identifier><identifier>DOI: 10.1016/bs.mie.2016.10.022</identifier><identifier>PMID: 28253977</identifier><language>eng</language><publisher>United States</publisher><subject>Automation ; Autophagosomes - metabolism ; Cell Line, Tumor ; Cytoplasm - metabolism ; Green Fluorescent Proteins - analysis ; Green Fluorescent Proteins - genetics ; High-Throughput Screening Assays - methods ; Humans ; Image Processing, Computer-Assisted ; Microscopy, Fluorescence - methods ; Microtubule-Associated Proteins - analysis ; Microtubule-Associated Proteins - genetics ; Microtubule-Associated Proteins - metabolism ; Neoplasms - metabolism ; Recombinant Proteins - analysis ; Recombinant Proteins - genetics ; Recombinant Proteins - metabolism</subject><ispartof>Methods in enzymology, 2017, Vol.587, p.71-86</ispartof><rights>2017 Elsevier Inc. All rights reserved.</rights><lds50>peer_reviewed</lds50><woscitedreferencessubscribed>false</woscitedreferencessubscribed><citedby>FETCH-LOGICAL-c326t-948fedc840ca2d8e1603f3a68085db64d78bff0023ce2205539a4f94c0fde72a3</citedby></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Tsyndetics_thumb_exl</thumbnail><link.rule.ids>314,776,780,4010,27900,27901,27902</link.rule.ids><backlink>$$Uhttps://www.ncbi.nlm.nih.gov/pubmed/28253977$$D View this record in MEDLINE/PubMed$$Hfree_for_read</backlink></links><search><creatorcontrib>Bravo-San Pedro, J M</creatorcontrib><creatorcontrib>Pietrocola, F</creatorcontrib><creatorcontrib>Sica, V</creatorcontrib><creatorcontrib>Izzo, V</creatorcontrib><creatorcontrib>Sauvat, A</creatorcontrib><creatorcontrib>Kepp, O</creatorcontrib><creatorcontrib>Maiuri, M C</creatorcontrib><creatorcontrib>Kroemer, G</creatorcontrib><creatorcontrib>Galluzzi, L</creatorcontrib><title>High-Throughput Quantification of GFP-LC3 + Dots by Automated Fluorescence Microscopy</title><title>Methods in enzymology</title><addtitle>Methods Enzymol</addtitle><description>Macroautophagy is a specific variant of autophagy that involves a dedicated double-membraned organelle commonly known as autophagosome. Various methods have been developed to quantify the size of the autophagosomal compartment, which is an indirect indicator of macroautophagic responses, based on the peculiar ability of microtubule-associated protein 1 light chain 3 beta (MAP1LC3B; best known as LC3) to accumulate in forming autophagosomes upon maturation. One particularly convenient method to monitor the accumulation of mature LC3 within autophagosomes relies on a green fluorescent protein (GFP)-tagged variant of this protein and fluorescence microscopy. In physiological conditions, cells transfected temporarily or stably with a GFP-LC3-encoding construct exhibit a diffuse green fluorescence over the cytoplasm and nucleus. Conversely, in response to macroautophagy-promoting stimuli, the GFP-LC3 signal becomes punctate and often (but not always) predominantly cytoplasmic. The accumulation of GFP-LC3 in cytoplasmic dots, however, also ensues the blockage of any of the steps that ensure the degradation of mature autophagosomes, calling for the implementation of strategies that accurately discriminate between an increase in autophagic flux and an arrest in autophagic degradation. Various cell lines have been engineered to stably express GFP-LC3, which-combined with the appropriate controls of flux, high-throughput imaging stations, and automated image analysis-offer a relatively straightforward tool to screen large chemical or biological libraries for inducers or inhibitors of autophagy. Here, we describe a simple and robust method for the high-throughput quantification of GFP-LC3
dots by automated fluorescence microscopy.</description><subject>Automation</subject><subject>Autophagosomes - metabolism</subject><subject>Cell Line, Tumor</subject><subject>Cytoplasm - metabolism</subject><subject>Green Fluorescent Proteins - analysis</subject><subject>Green Fluorescent Proteins - genetics</subject><subject>High-Throughput Screening Assays - methods</subject><subject>Humans</subject><subject>Image Processing, Computer-Assisted</subject><subject>Microscopy, Fluorescence - methods</subject><subject>Microtubule-Associated Proteins - analysis</subject><subject>Microtubule-Associated Proteins - genetics</subject><subject>Microtubule-Associated Proteins - metabolism</subject><subject>Neoplasms - metabolism</subject><subject>Recombinant Proteins - analysis</subject><subject>Recombinant Proteins - genetics</subject><subject>Recombinant Proteins - metabolism</subject><issn>1557-7988</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2017</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNo1kE9LwzAAxYMgbk6_gAfJUZDW_G3S45huEyYqbOeSpskWaZvaJId9ewvq6T0ej8ePB8AdRjlGuHiqQ945k5PJT0GOCLkAc8y5yEQp5Qxch_CFEBGyxFdgRiThtBRiDg5bdzxl-9Po0_E0pAg_k-qjs06r6HwPvYWb9Ue2W1H4CJ99DLA-w2WKvlPRNHDdJj-aoE2vDXxzevRB--F8Ay6taoO5_dMFOKxf9qtttnvfvK6Wu0xTUsSsZNKaRkuGtCKNNLhA1FJVSCR5UxesEbK2dsKm2hCC-MSsmC2ZRrYxgii6AA-_u8Pov5MJsercBNO2qjc-hQpLwRjjGPGpev9XTXVnmmoYXafGc_V_Bf0BYwZfHA</recordid><startdate>2017</startdate><enddate>2017</enddate><creator>Bravo-San Pedro, J M</creator><creator>Pietrocola, F</creator><creator>Sica, V</creator><creator>Izzo, V</creator><creator>Sauvat, A</creator><creator>Kepp, O</creator><creator>Maiuri, M C</creator><creator>Kroemer, G</creator><creator>Galluzzi, L</creator><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>7X8</scope></search><sort><creationdate>2017</creationdate><title>High-Throughput Quantification of GFP-LC3 + Dots by Automated Fluorescence Microscopy</title><author>Bravo-San Pedro, J M ; Pietrocola, F ; Sica, V ; Izzo, V ; Sauvat, A ; Kepp, O ; Maiuri, M C ; Kroemer, G ; Galluzzi, L</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c326t-948fedc840ca2d8e1603f3a68085db64d78bff0023ce2205539a4f94c0fde72a3</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2017</creationdate><topic>Automation</topic><topic>Autophagosomes - metabolism</topic><topic>Cell Line, Tumor</topic><topic>Cytoplasm - metabolism</topic><topic>Green Fluorescent Proteins - analysis</topic><topic>Green Fluorescent Proteins - genetics</topic><topic>High-Throughput Screening Assays - methods</topic><topic>Humans</topic><topic>Image Processing, Computer-Assisted</topic><topic>Microscopy, Fluorescence - methods</topic><topic>Microtubule-Associated Proteins - analysis</topic><topic>Microtubule-Associated Proteins - genetics</topic><topic>Microtubule-Associated Proteins - metabolism</topic><topic>Neoplasms - metabolism</topic><topic>Recombinant Proteins - analysis</topic><topic>Recombinant Proteins - genetics</topic><topic>Recombinant Proteins - metabolism</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Bravo-San Pedro, J M</creatorcontrib><creatorcontrib>Pietrocola, F</creatorcontrib><creatorcontrib>Sica, V</creatorcontrib><creatorcontrib>Izzo, V</creatorcontrib><creatorcontrib>Sauvat, A</creatorcontrib><creatorcontrib>Kepp, O</creatorcontrib><creatorcontrib>Maiuri, M C</creatorcontrib><creatorcontrib>Kroemer, G</creatorcontrib><creatorcontrib>Galluzzi, L</creatorcontrib><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>MEDLINE - Academic</collection><jtitle>Methods in enzymology</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Bravo-San Pedro, J M</au><au>Pietrocola, F</au><au>Sica, V</au><au>Izzo, V</au><au>Sauvat, A</au><au>Kepp, O</au><au>Maiuri, M C</au><au>Kroemer, G</au><au>Galluzzi, L</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>High-Throughput Quantification of GFP-LC3 + Dots by Automated Fluorescence Microscopy</atitle><jtitle>Methods in enzymology</jtitle><addtitle>Methods Enzymol</addtitle><date>2017</date><risdate>2017</risdate><volume>587</volume><spage>71</spage><epage>86</epage><pages>71-86</pages><eissn>1557-7988</eissn><abstract>Macroautophagy is a specific variant of autophagy that involves a dedicated double-membraned organelle commonly known as autophagosome. Various methods have been developed to quantify the size of the autophagosomal compartment, which is an indirect indicator of macroautophagic responses, based on the peculiar ability of microtubule-associated protein 1 light chain 3 beta (MAP1LC3B; best known as LC3) to accumulate in forming autophagosomes upon maturation. One particularly convenient method to monitor the accumulation of mature LC3 within autophagosomes relies on a green fluorescent protein (GFP)-tagged variant of this protein and fluorescence microscopy. In physiological conditions, cells transfected temporarily or stably with a GFP-LC3-encoding construct exhibit a diffuse green fluorescence over the cytoplasm and nucleus. Conversely, in response to macroautophagy-promoting stimuli, the GFP-LC3 signal becomes punctate and often (but not always) predominantly cytoplasmic. The accumulation of GFP-LC3 in cytoplasmic dots, however, also ensues the blockage of any of the steps that ensure the degradation of mature autophagosomes, calling for the implementation of strategies that accurately discriminate between an increase in autophagic flux and an arrest in autophagic degradation. Various cell lines have been engineered to stably express GFP-LC3, which-combined with the appropriate controls of flux, high-throughput imaging stations, and automated image analysis-offer a relatively straightforward tool to screen large chemical or biological libraries for inducers or inhibitors of autophagy. Here, we describe a simple and robust method for the high-throughput quantification of GFP-LC3
dots by automated fluorescence microscopy.</abstract><cop>United States</cop><pmid>28253977</pmid><doi>10.1016/bs.mie.2016.10.022</doi><tpages>16</tpages></addata></record> |
| fulltext | fulltext |
| identifier | EISSN: 1557-7988 |
| ispartof | Methods in enzymology, 2017, Vol.587, p.71-86 |
| issn | 1557-7988 |
| language | eng |
| recordid | cdi_proquest_miscellaneous_1874445105 |
| source | MEDLINE; Elsevier ScienceDirect Journals |
| subjects | Automation Autophagosomes - metabolism Cell Line, Tumor Cytoplasm - metabolism Green Fluorescent Proteins - analysis Green Fluorescent Proteins - genetics High-Throughput Screening Assays - methods Humans Image Processing, Computer-Assisted Microscopy, Fluorescence - methods Microtubule-Associated Proteins - analysis Microtubule-Associated Proteins - genetics Microtubule-Associated Proteins - metabolism Neoplasms - metabolism Recombinant Proteins - analysis Recombinant Proteins - genetics Recombinant Proteins - metabolism |
| title | High-Throughput Quantification of GFP-LC3 + Dots by Automated Fluorescence Microscopy |
| url | https://sfx.bib-bvb.de/sfx_tum?ctx_ver=Z39.88-2004&ctx_enc=info:ofi/enc:UTF-8&ctx_tim=2025-01-31T07%3A47%3A15IST&url_ver=Z39.88-2004&url_ctx_fmt=infofi/fmt:kev:mtx:ctx&rfr_id=info:sid/primo.exlibrisgroup.com:primo3-Article-proquest_pubme&rft_val_fmt=info:ofi/fmt:kev:mtx:journal&rft.genre=article&rft.atitle=High-Throughput%20Quantification%20of%20GFP-LC3%20+%20Dots%20by%20Automated%20Fluorescence%20Microscopy&rft.jtitle=Methods%20in%20enzymology&rft.au=Bravo-San%20Pedro,%20J%20M&rft.date=2017&rft.volume=587&rft.spage=71&rft.epage=86&rft.pages=71-86&rft.eissn=1557-7988&rft_id=info:doi/10.1016/bs.mie.2016.10.022&rft_dat=%3Cproquest_pubme%3E1874445105%3C/proquest_pubme%3E%3Curl%3E%3C/url%3E&disable_directlink=true&sfx.directlink=off&sfx.report_link=0&rft_id=info:oai/&rft_pqid=1874445105&rft_id=info:pmid/28253977&rfr_iscdi=true |