A novel FRET pair for detection of parallel DNA triplexes by the LightCycler

BACKGROUND: Melting temperature of DNA structures can be determined on the LightCycler using quenching of FAM. This method is very suitable for pH independent melting point (Tm) determination performed at basic or neutral pH, as a high throughput alternative to UV absorbance measurements. At acidic...

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Autores principales: Schneider, Uffe V, Severinsen, Jette K, Géci, Imrich, Okkels, Limei M, Jøhnk, Nina, Mikkelsen, Nikolaj D, Klinge, Teena, Pedersen, Erik B, Westh, Henrik, Lisby, Gorm
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2010
Materias:
Methodology Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2823659/
https://www.ncbi.nlm.nih.gov/pubmed/20102641
http://dx.doi.org/10.1186/1472-6750-10-4
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author Schneider, Uffe V
Severinsen, Jette K
Géci, Imrich
Okkels, Limei M
Jøhnk, Nina
Mikkelsen, Nikolaj D
Klinge, Teena
Pedersen, Erik B
Westh, Henrik
Lisby, Gorm
author_facet Schneider, Uffe V
Severinsen, Jette K
Géci, Imrich
Okkels, Limei M
Jøhnk, Nina
Mikkelsen, Nikolaj D
Klinge, Teena
Pedersen, Erik B
Westh, Henrik
Lisby, Gorm
author_sort Schneider, Uffe V
collection PubMed
description BACKGROUND: Melting temperature of DNA structures can be determined on the LightCycler using quenching of FAM. This method is very suitable for pH independent melting point (Tm) determination performed at basic or neutral pH, as a high throughput alternative to UV absorbance measurements. At acidic pH quenching of FAM is not very suitable, since the fluorescence of FAM is strongly pH dependent and drops with acidic pH. Hoogsteen based parallel triplex helix formation requires protonation of cytosines in the triplex forming strand. Therefore, nucleic acid triplexes show strong pH dependence and are stable only at acidic pH. This led us to establish a new pH independent fluorophore based measuring system on the LightCycler for thermal stability studies of parallel triplexes. RESULTS: A novel LightCycler FRET pair labelled with ATTO495 and ATTO647N was established for parallel triplex detection with antiparallel duplex as a control for the general applicability of these fluorophores for Tm determination. The ATTO fluorophores were pH stable from pH 4.5 to 7.5. Melting of triplex and duplex structures were accompanied by a large decrease in fluorescence intensity leading to well defined Tm and high reproducibility. Validation of Tm showed low intra- and inter-assay coefficient of variation; 0.11% and 0.14% for parallel triplex and 0.19% and 0.12% for antiparallel duplex. Measurements of Tm and fluorescence intensity over time and multiple runs showed great time and light stability of the ATTO fluorophores. The variance on Tm determinations was significant lower on the LightCycler platform compared to UV absorbance measurements, which enable discrimination of DNA structures with very similar Tm. Labelling of DNA probes with ATTO fluorophore increased Tm of antiparallel duplexes significantly, but not Tm of parallel triplexes. CONCLUSIONS: We have established a novel pH independent FRET pair with high fluorescence signals on the LightCycler platform for both antiparallel duplex and parallel triplex formation. The method has been thoroughly validated, and is characterized by an excellent accuracy and reproducibility. This FRET pair is especially suitable for ΔTm and Tm determinations of pH dependent parallel triplex formation.
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spelling pubmed-28236592010-02-18 A novel FRET pair for detection of parallel DNA triplexes by the LightCycler Schneider, Uffe V Severinsen, Jette K Géci, Imrich Okkels, Limei M Jøhnk, Nina Mikkelsen, Nikolaj D Klinge, Teena Pedersen, Erik B Westh, Henrik Lisby, Gorm BMC Biotechnol Methodology Article BACKGROUND: Melting temperature of DNA structures can be determined on the LightCycler using quenching of FAM. This method is very suitable for pH independent melting point (Tm) determination performed at basic or neutral pH, as a high throughput alternative to UV absorbance measurements. At acidic pH quenching of FAM is not very suitable, since the fluorescence of FAM is strongly pH dependent and drops with acidic pH. Hoogsteen based parallel triplex helix formation requires protonation of cytosines in the triplex forming strand. Therefore, nucleic acid triplexes show strong pH dependence and are stable only at acidic pH. This led us to establish a new pH independent fluorophore based measuring system on the LightCycler for thermal stability studies of parallel triplexes. RESULTS: A novel LightCycler FRET pair labelled with ATTO495 and ATTO647N was established for parallel triplex detection with antiparallel duplex as a control for the general applicability of these fluorophores for Tm determination. The ATTO fluorophores were pH stable from pH 4.5 to 7.5. Melting of triplex and duplex structures were accompanied by a large decrease in fluorescence intensity leading to well defined Tm and high reproducibility. Validation of Tm showed low intra- and inter-assay coefficient of variation; 0.11% and 0.14% for parallel triplex and 0.19% and 0.12% for antiparallel duplex. Measurements of Tm and fluorescence intensity over time and multiple runs showed great time and light stability of the ATTO fluorophores. The variance on Tm determinations was significant lower on the LightCycler platform compared to UV absorbance measurements, which enable discrimination of DNA structures with very similar Tm. Labelling of DNA probes with ATTO fluorophore increased Tm of antiparallel duplexes significantly, but not Tm of parallel triplexes. CONCLUSIONS: We have established a novel pH independent FRET pair with high fluorescence signals on the LightCycler platform for both antiparallel duplex and parallel triplex formation. The method has been thoroughly validated, and is characterized by an excellent accuracy and reproducibility. This FRET pair is especially suitable for ΔTm and Tm determinations of pH dependent parallel triplex formation. BioMed Central 2010-01-27 /pmc/articles/PMC2823659/ /pubmed/20102641 http://dx.doi.org/10.1186/1472-6750-10-4 Text en Copyright ©2010 Schneider et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methodology Article
Schneider, Uffe V
Severinsen, Jette K
Géci, Imrich
Okkels, Limei M
Jøhnk, Nina
Mikkelsen, Nikolaj D
Klinge, Teena
Pedersen, Erik B
Westh, Henrik
Lisby, Gorm
A novel FRET pair for detection of parallel DNA triplexes by the LightCycler
title A novel FRET pair for detection of parallel DNA triplexes by the LightCycler
title_full A novel FRET pair for detection of parallel DNA triplexes by the LightCycler
title_fullStr A novel FRET pair for detection of parallel DNA triplexes by the LightCycler
title_full_unstemmed A novel FRET pair for detection of parallel DNA triplexes by the LightCycler
title_short A novel FRET pair for detection of parallel DNA triplexes by the LightCycler
title_sort novel fret pair for detection of parallel dna triplexes by the lightcycler
topic Methodology Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2823659/
https://www.ncbi.nlm.nih.gov/pubmed/20102641
http://dx.doi.org/10.1186/1472-6750-10-4
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