Real-time probing of β-amyloid self-assembly and inhibition using fluorescence self-quenching between neighbouring dyesElectronic supplementary information (ESI) available: Details of aggregation protocols, steady-state and time-resolved measurements, transmission electron microscopy characterization and Fig. S1-S10 and Tables S1-S6. See DOI: 10.1039/c3mb70272c

Real-time probing of β-amyloid self-assembly and inhibition using fluorescence self-quenching between neighbouring dyesElectronic supplementary information (ESI) available: Details of aggregation protocols, steady-state and time-resolved measurements, transmission electron microscopy characterization and Fig. S1-S10 and Tables S1-S6. See DOI: 10.1039/c3mb70272c

The fluorescence response of the Thioflavin-T (ThT) dye and derivatives has become the standard tool for detecting β-amyloid aggregates (Aβ) in solution. However, it is accepted that ThT-based methods suffer from important drawbacks. Some of these are due to the cationic structure of ThT, which limi...

Ausführliche Beschreibung

Gespeichert in:
Bibliographische Detailangaben
Hauptverfasser: Quinn, Steven D, Dalgarno, Paul A, Cameron, Ryan T, Hedley, Gordon J, Hacker, Christian, Lucocq, John M, Baillie, George S, Samuel, Ifor D. W, Penedo, J. Carlos
Format: Artikel
Sprache:
Online-Zugang:Volltext
Tags: Tag hinzufügen
Keine Tags, Fügen Sie den ersten Tag hinzu!
container_end_page 44
container_issue 1
container_start_page 34
container_title
container_volume 1
creator Quinn, Steven D
Dalgarno, Paul A
Cameron, Ryan T
Hedley, Gordon J
Hacker, Christian
Lucocq, John M
Baillie, George S
Samuel, Ifor D. W
Penedo, J. Carlos
description The fluorescence response of the Thioflavin-T (ThT) dye and derivatives has become the standard tool for detecting β-amyloid aggregates (Aβ) in solution. However, it is accepted that ThT-based methods suffer from important drawbacks. Some of these are due to the cationic structure of ThT, which limits its application at slightly acidic conditions; whereas some limitations are related to the general use of an extrinsic-dye sensing strategy and its intrinsic requirement for the formation of a sensor-binding site during the aggregation process. Here, we introduce fluorescence-self-quenching (FSQ) between N-terminally tagged peptides as a strategy to overcome some of these limitations. Using a combination of steady-state, picosecond time-resolved fluorescence and transmission electron microscopy, we characterize the fluorescence response of HiLyte fluor 555-labelled Aβ peptides and demonstrate that Aβ self-assembly organizes the covalently attached probes in close proximity to trigger the self-quenching sensing process over a broad range of conditions. Importantly, we prove that N-terminal tagging of β-amyloid peptides does not alter the self-assembly kinetics or the resulting aggregated structures. We also tested the ability of FSQ-based methods to monitor the inhibition of Aβ 1-42 aggregation using the small heat-shock protein Hsp20 as a model system. Overall, FSQ-based strategies for amyloid-sensing fill the gap between current morphology-specific protocols using extrinsic dyes, and highly-specialized single-molecule techniques that are difficult to implement in high-throughput analytical determinations. When performed in Förster resonance energy transfer (FRET) format, the method becomes a ratiometric platform to gain insights into amyloid structure and for standardizing in vitro studies of amyloid aggregation. A fluorescence self-quenching (FSQ) approach between β-amyloid peptides labelled at the N-terminal position demonstrates excellent performance to monitor in real-time the self-assembly mechanism across a wide range of experimental conditions.
doi_str_mv 10.1039/c3mb70272c
format Article
fullrecord <record><control><sourceid>rsc</sourceid><recordid>TN_cdi_rsc_primary_c3mb70272c</recordid><sourceformat>XML</sourceformat><sourcesystem>PC</sourcesystem><sourcerecordid>c3mb70272c</sourcerecordid><originalsourceid>FETCH-rsc_primary_c3mb70272c3</originalsourceid><addsrcrecordid>eNqFkbtOw0AQRQ0CifBo6JGmBAkHOwkJpCWJSIVEUtBF4_XYWbQPs7MOMp_Fh_BN2E4EBQXV3p25e-eMNgjO46gbR_37G9HXySjqjXpiP-jEo0Ev7EW38cGPHr4cBcfMr1HUvxvEUWdPPROq0EtNUDibSJODzeDrM0RdKStTYFJZiMykE1UBmhSkWctEemkNlNw8yFRpHbEgI2jrfytrvW56Cfl3IgOGZL5ObOmaYloRTxUJ76yRArgsCkWajEdX1fGZdRrb_MvpYn4FuEGpMFE0hgn5WnPDiHnuKN_6anRvhVV8DewJ0ypkj55a3Ga3sMazakMpaEIuXTusNnuHhrVkbkJoRwRaCmdZ2KICsUaHwpOTH9tJTeJM5l1YxOEijtr7smHjtjKsG0QweZqP4e-fnAaHGSqms915ElzMpsuHx9CxWBVO6nr_1a-9_1__G3NDp2w</addsrcrecordid><sourcetype>Publisher</sourcetype><iscdi>true</iscdi><recordtype>article</recordtype></control><display><type>article</type><title>Real-time probing of β-amyloid self-assembly and inhibition using fluorescence self-quenching between neighbouring dyesElectronic supplementary information (ESI) available: Details of aggregation protocols, steady-state and time-resolved measurements, transmission electron microscopy characterization and Fig. S1-S10 and Tables S1-S6. See DOI: 10.1039/c3mb70272c</title><source>Royal Society Of Chemistry Journals</source><source>Alma/SFX Local Collection</source><creator>Quinn, Steven D ; Dalgarno, Paul A ; Cameron, Ryan T ; Hedley, Gordon J ; Hacker, Christian ; Lucocq, John M ; Baillie, George S ; Samuel, Ifor D. W ; Penedo, J. Carlos</creator><creatorcontrib>Quinn, Steven D ; Dalgarno, Paul A ; Cameron, Ryan T ; Hedley, Gordon J ; Hacker, Christian ; Lucocq, John M ; Baillie, George S ; Samuel, Ifor D. W ; Penedo, J. Carlos</creatorcontrib><description>The fluorescence response of the Thioflavin-T (ThT) dye and derivatives has become the standard tool for detecting β-amyloid aggregates (Aβ) in solution. However, it is accepted that ThT-based methods suffer from important drawbacks. Some of these are due to the cationic structure of ThT, which limits its application at slightly acidic conditions; whereas some limitations are related to the general use of an extrinsic-dye sensing strategy and its intrinsic requirement for the formation of a sensor-binding site during the aggregation process. Here, we introduce fluorescence-self-quenching (FSQ) between N-terminally tagged peptides as a strategy to overcome some of these limitations. Using a combination of steady-state, picosecond time-resolved fluorescence and transmission electron microscopy, we characterize the fluorescence response of HiLyte fluor 555-labelled Aβ peptides and demonstrate that Aβ self-assembly organizes the covalently attached probes in close proximity to trigger the self-quenching sensing process over a broad range of conditions. Importantly, we prove that N-terminal tagging of β-amyloid peptides does not alter the self-assembly kinetics or the resulting aggregated structures. We also tested the ability of FSQ-based methods to monitor the inhibition of Aβ 1-42 aggregation using the small heat-shock protein Hsp20 as a model system. Overall, FSQ-based strategies for amyloid-sensing fill the gap between current morphology-specific protocols using extrinsic dyes, and highly-specialized single-molecule techniques that are difficult to implement in high-throughput analytical determinations. When performed in Förster resonance energy transfer (FRET) format, the method becomes a ratiometric platform to gain insights into amyloid structure and for standardizing in vitro studies of amyloid aggregation. A fluorescence self-quenching (FSQ) approach between β-amyloid peptides labelled at the N-terminal position demonstrates excellent performance to monitor in real-time the self-assembly mechanism across a wide range of experimental conditions.</description><identifier>ISSN: 1742-206X</identifier><identifier>EISSN: 1742-2051</identifier><identifier>DOI: 10.1039/c3mb70272c</identifier><creationdate>2013-11</creationdate><lds50>peer_reviewed</lds50><woscitedreferencessubscribed>false</woscitedreferencessubscribed></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Tsyndetics_thumb_exl</thumbnail><link.rule.ids>315,781,785,27929,27930</link.rule.ids></links><search><creatorcontrib>Quinn, Steven D</creatorcontrib><creatorcontrib>Dalgarno, Paul A</creatorcontrib><creatorcontrib>Cameron, Ryan T</creatorcontrib><creatorcontrib>Hedley, Gordon J</creatorcontrib><creatorcontrib>Hacker, Christian</creatorcontrib><creatorcontrib>Lucocq, John M</creatorcontrib><creatorcontrib>Baillie, George S</creatorcontrib><creatorcontrib>Samuel, Ifor D. W</creatorcontrib><creatorcontrib>Penedo, J. Carlos</creatorcontrib><title>Real-time probing of β-amyloid self-assembly and inhibition using fluorescence self-quenching between neighbouring dyesElectronic supplementary information (ESI) available: Details of aggregation protocols, steady-state and time-resolved measurements, transmission electron microscopy characterization and Fig. S1-S10 and Tables S1-S6. See DOI: 10.1039/c3mb70272c</title><description>The fluorescence response of the Thioflavin-T (ThT) dye and derivatives has become the standard tool for detecting β-amyloid aggregates (Aβ) in solution. However, it is accepted that ThT-based methods suffer from important drawbacks. Some of these are due to the cationic structure of ThT, which limits its application at slightly acidic conditions; whereas some limitations are related to the general use of an extrinsic-dye sensing strategy and its intrinsic requirement for the formation of a sensor-binding site during the aggregation process. Here, we introduce fluorescence-self-quenching (FSQ) between N-terminally tagged peptides as a strategy to overcome some of these limitations. Using a combination of steady-state, picosecond time-resolved fluorescence and transmission electron microscopy, we characterize the fluorescence response of HiLyte fluor 555-labelled Aβ peptides and demonstrate that Aβ self-assembly organizes the covalently attached probes in close proximity to trigger the self-quenching sensing process over a broad range of conditions. Importantly, we prove that N-terminal tagging of β-amyloid peptides does not alter the self-assembly kinetics or the resulting aggregated structures. We also tested the ability of FSQ-based methods to monitor the inhibition of Aβ 1-42 aggregation using the small heat-shock protein Hsp20 as a model system. Overall, FSQ-based strategies for amyloid-sensing fill the gap between current morphology-specific protocols using extrinsic dyes, and highly-specialized single-molecule techniques that are difficult to implement in high-throughput analytical determinations. When performed in Förster resonance energy transfer (FRET) format, the method becomes a ratiometric platform to gain insights into amyloid structure and for standardizing in vitro studies of amyloid aggregation. A fluorescence self-quenching (FSQ) approach between β-amyloid peptides labelled at the N-terminal position demonstrates excellent performance to monitor in real-time the self-assembly mechanism across a wide range of experimental conditions.</description><issn>1742-206X</issn><issn>1742-2051</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2013</creationdate><recordtype>article</recordtype><sourceid/><recordid>eNqFkbtOw0AQRQ0CifBo6JGmBAkHOwkJpCWJSIVEUtBF4_XYWbQPs7MOMp_Fh_BN2E4EBQXV3p25e-eMNgjO46gbR_37G9HXySjqjXpiP-jEo0Ev7EW38cGPHr4cBcfMr1HUvxvEUWdPPROq0EtNUDibSJODzeDrM0RdKStTYFJZiMykE1UBmhSkWctEemkNlNw8yFRpHbEgI2jrfytrvW56Cfl3IgOGZL5ObOmaYloRTxUJ76yRArgsCkWajEdX1fGZdRrb_MvpYn4FuEGpMFE0hgn5WnPDiHnuKN_6anRvhVV8DewJ0ypkj55a3Ga3sMazakMpaEIuXTusNnuHhrVkbkJoRwRaCmdZ2KICsUaHwpOTH9tJTeJM5l1YxOEijtr7smHjtjKsG0QweZqP4e-fnAaHGSqms915ElzMpsuHx9CxWBVO6nr_1a-9_1__G3NDp2w</recordid><startdate>20131126</startdate><enddate>20131126</enddate><creator>Quinn, Steven D</creator><creator>Dalgarno, Paul A</creator><creator>Cameron, Ryan T</creator><creator>Hedley, Gordon J</creator><creator>Hacker, Christian</creator><creator>Lucocq, John M</creator><creator>Baillie, George S</creator><creator>Samuel, Ifor D. W</creator><creator>Penedo, J. Carlos</creator><scope/></search><sort><creationdate>20131126</creationdate><title>Real-time probing of β-amyloid self-assembly and inhibition using fluorescence self-quenching between neighbouring dyesElectronic supplementary information (ESI) available: Details of aggregation protocols, steady-state and time-resolved measurements, transmission electron microscopy characterization and Fig. S1-S10 and Tables S1-S6. See DOI: 10.1039/c3mb70272c</title><author>Quinn, Steven D ; Dalgarno, Paul A ; Cameron, Ryan T ; Hedley, Gordon J ; Hacker, Christian ; Lucocq, John M ; Baillie, George S ; Samuel, Ifor D. W ; Penedo, J. Carlos</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-rsc_primary_c3mb70272c3</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><creationdate>2013</creationdate><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Quinn, Steven D</creatorcontrib><creatorcontrib>Dalgarno, Paul A</creatorcontrib><creatorcontrib>Cameron, Ryan T</creatorcontrib><creatorcontrib>Hedley, Gordon J</creatorcontrib><creatorcontrib>Hacker, Christian</creatorcontrib><creatorcontrib>Lucocq, John M</creatorcontrib><creatorcontrib>Baillie, George S</creatorcontrib><creatorcontrib>Samuel, Ifor D. W</creatorcontrib><creatorcontrib>Penedo, J. Carlos</creatorcontrib></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Quinn, Steven D</au><au>Dalgarno, Paul A</au><au>Cameron, Ryan T</au><au>Hedley, Gordon J</au><au>Hacker, Christian</au><au>Lucocq, John M</au><au>Baillie, George S</au><au>Samuel, Ifor D. W</au><au>Penedo, J. Carlos</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Real-time probing of β-amyloid self-assembly and inhibition using fluorescence self-quenching between neighbouring dyesElectronic supplementary information (ESI) available: Details of aggregation protocols, steady-state and time-resolved measurements, transmission electron microscopy characterization and Fig. S1-S10 and Tables S1-S6. See DOI: 10.1039/c3mb70272c</atitle><date>2013-11-26</date><risdate>2013</risdate><volume>1</volume><issue>1</issue><spage>34</spage><epage>44</epage><pages>34-44</pages><issn>1742-206X</issn><eissn>1742-2051</eissn><abstract>The fluorescence response of the Thioflavin-T (ThT) dye and derivatives has become the standard tool for detecting β-amyloid aggregates (Aβ) in solution. However, it is accepted that ThT-based methods suffer from important drawbacks. Some of these are due to the cationic structure of ThT, which limits its application at slightly acidic conditions; whereas some limitations are related to the general use of an extrinsic-dye sensing strategy and its intrinsic requirement for the formation of a sensor-binding site during the aggregation process. Here, we introduce fluorescence-self-quenching (FSQ) between N-terminally tagged peptides as a strategy to overcome some of these limitations. Using a combination of steady-state, picosecond time-resolved fluorescence and transmission electron microscopy, we characterize the fluorescence response of HiLyte fluor 555-labelled Aβ peptides and demonstrate that Aβ self-assembly organizes the covalently attached probes in close proximity to trigger the self-quenching sensing process over a broad range of conditions. Importantly, we prove that N-terminal tagging of β-amyloid peptides does not alter the self-assembly kinetics or the resulting aggregated structures. We also tested the ability of FSQ-based methods to monitor the inhibition of Aβ 1-42 aggregation using the small heat-shock protein Hsp20 as a model system. Overall, FSQ-based strategies for amyloid-sensing fill the gap between current morphology-specific protocols using extrinsic dyes, and highly-specialized single-molecule techniques that are difficult to implement in high-throughput analytical determinations. When performed in Förster resonance energy transfer (FRET) format, the method becomes a ratiometric platform to gain insights into amyloid structure and for standardizing in vitro studies of amyloid aggregation. A fluorescence self-quenching (FSQ) approach between β-amyloid peptides labelled at the N-terminal position demonstrates excellent performance to monitor in real-time the self-assembly mechanism across a wide range of experimental conditions.</abstract><doi>10.1039/c3mb70272c</doi><tpages>11</tpages></addata></record>
fulltext fulltext
identifier ISSN: 1742-206X
ispartof
issn 1742-206X
1742-2051
language
recordid cdi_rsc_primary_c3mb70272c
source Royal Society Of Chemistry Journals; Alma/SFX Local Collection
title Real-time probing of β-amyloid self-assembly and inhibition using fluorescence self-quenching between neighbouring dyesElectronic supplementary information (ESI) available: Details of aggregation protocols, steady-state and time-resolved measurements, transmission electron microscopy characterization and Fig. S1-S10 and Tables S1-S6. See DOI: 10.1039/c3mb70272c
url https://sfx.bib-bvb.de/sfx_tum?ctx_ver=Z39.88-2004&ctx_enc=info:ofi/enc:UTF-8&ctx_tim=2024-12-12T22%3A05%3A21IST&url_ver=Z39.88-2004&url_ctx_fmt=infofi/fmt:kev:mtx:ctx&rfr_id=info:sid/primo.exlibrisgroup.com:primo3-Article-rsc&rft_val_fmt=info:ofi/fmt:kev:mtx:journal&rft.genre=article&rft.atitle=Real-time%20probing%20of%20%CE%B2-amyloid%20self-assembly%20and%20inhibition%20using%20fluorescence%20self-quenching%20between%20neighbouring%20dyesElectronic%20supplementary%20information%20(ESI)%20available:%20Details%20of%20aggregation%20protocols,%20steady-state%20and%20time-resolved%20measurements,%20transmission%20electron%20microscopy%20characterization%20and%20Fig.%20S1-S10%20and%20Tables%20S1-S6.%20See%20DOI:%2010.1039/c3mb70272c&rft.au=Quinn,%20Steven%20D&rft.date=2013-11-26&rft.volume=1&rft.issue=1&rft.spage=34&rft.epage=44&rft.pages=34-44&rft.issn=1742-206X&rft.eissn=1742-2051&rft_id=info:doi/10.1039/c3mb70272c&rft_dat=%3Crsc%3Ec3mb70272c%3C/rsc%3E%3Curl%3E%3C/url%3E&disable_directlink=true&sfx.directlink=off&sfx.report_link=0&rft_id=info:oai/&rft_id=info:pmid/&rfr_iscdi=true