Fluorescence of dyes in solutions with high absorbance. Inner filter effect correction
Fluorescence is a proven tool in all fields of knowledge, including biology and medicine. A significant obstacle in its use is the nonlinearity of the dependence of the fluorescence intensity on fluorophore concentration that is caused by the so-called primary inner filter effect. The existing metho...
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| description | Fluorescence is a proven tool in all fields of knowledge, including biology and medicine. A significant obstacle in its use is the nonlinearity of the dependence of the fluorescence intensity on fluorophore concentration that is caused by the so-called primary inner filter effect. The existing methods for correcting the fluorescence intensity are hard to implement in practice; thus, it is generally considered best to use dilute solutions. We showed that correction must be performed always. Furthermore, high-concentration solutions (high absorbance) are inherent condition in studying of the photophysical properties of fluorescent dyes and the functionally significant interactions of biological macromolecules. We proposed an easy to use method to correct the experimentally recorded total fluorescence intensity and showed that informative component of fluorescence intensity numerically equals to the product of the absorbance and the fluorescence quantum yield of the object. It is shown that if dye molecules do not interact with each other and there is no reabsorption (as for NATA) and spectrofluorimeter provides the proportionality of the detected fluorescence intensity to the part of the absorbed light (that is possible for spectrofluorimeter with horizontal slits) then the dependence of experimentally detected total fluorescence intensity of the dye on its absorbance coincides with the calculated dependence and the correction factor for eliminating the primary inner filter effect can be calculated on the basis of solution absorbance. It was experimentally shown for NATA fluorescence in the wide range of absorbance (at least up to 60). For ATTO-425, which fluorescence and absorption spectra overlap, the elimination of the primary and secondary filter effects and additional spectral analysis allow to conclude that the most probable reason of the deviation of experimentally detected fluorescence intensity dependence on solution absorbance from the calculated dependence is the dye molecules self-quenching, which accompanies resonance radiationless excitation energy transfer. |
| doi_str_mv | 10.1371/journal.pone.0103878 |
| format | Article |
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Inner filter effect correction</title><source>MEDLINE</source><source>DOAJ Directory of Open Access Journals</source><source>Public Library of Science (PLoS) Journals Open Access</source><source>EZB-FREE-00999 freely available EZB journals</source><source>PubMed Central</source><source>Free Full-Text Journals in Chemistry</source><creator>Fonin, Alexander V ; Sulatskaya, Anna I ; Kuznetsova, Irina M ; Turoverov, Konstantin K</creator><contributor>Permyakov, Eugene A.</contributor><creatorcontrib>Fonin, Alexander V ; Sulatskaya, Anna I ; Kuznetsova, Irina M ; Turoverov, Konstantin K ; Permyakov, Eugene A.</creatorcontrib><description>Fluorescence is a proven tool in all fields of knowledge, including biology and medicine. A significant obstacle in its use is the nonlinearity of the dependence of the fluorescence intensity on fluorophore concentration that is caused by the so-called primary inner filter effect. The existing methods for correcting the fluorescence intensity are hard to implement in practice; thus, it is generally considered best to use dilute solutions. We showed that correction must be performed always. Furthermore, high-concentration solutions (high absorbance) are inherent condition in studying of the photophysical properties of fluorescent dyes and the functionally significant interactions of biological macromolecules. We proposed an easy to use method to correct the experimentally recorded total fluorescence intensity and showed that informative component of fluorescence intensity numerically equals to the product of the absorbance and the fluorescence quantum yield of the object. It is shown that if dye molecules do not interact with each other and there is no reabsorption (as for NATA) and spectrofluorimeter provides the proportionality of the detected fluorescence intensity to the part of the absorbed light (that is possible for spectrofluorimeter with horizontal slits) then the dependence of experimentally detected total fluorescence intensity of the dye on its absorbance coincides with the calculated dependence and the correction factor for eliminating the primary inner filter effect can be calculated on the basis of solution absorbance. It was experimentally shown for NATA fluorescence in the wide range of absorbance (at least up to 60). For ATTO-425, which fluorescence and absorption spectra overlap, the elimination of the primary and secondary filter effects and additional spectral analysis allow to conclude that the most probable reason of the deviation of experimentally detected fluorescence intensity dependence on solution absorbance from the calculated dependence is the dye molecules self-quenching, which accompanies resonance radiationless excitation energy transfer.</description><identifier>ISSN: 1932-6203</identifier><identifier>EISSN: 1932-6203</identifier><identifier>DOI: 10.1371/journal.pone.0103878</identifier><identifier>PMID: 25072376</identifier><language>eng</language><publisher>United States: Public Library of Science</publisher><subject>Absorbance ; Absorption spectra ; Biology and Life Sciences ; Biophysics ; Cellular biology ; Dental caries ; Dilution ; Dyes ; Energy transfer ; Filtration - instrumentation ; Fluorescence ; Fluorescent dyes ; Fluorescent Dyes - chemistry ; Fluorescent indicators ; Laboratories ; Luminous intensity ; Macromolecules ; Methods ; Nonlinear systems ; Physical Sciences ; Protein folding ; Quantum Theory ; Reabsorption ; Slits ; Solutions - chemistry ; Spectral analysis ; Spectrometry, Fluorescence - instrumentation ; Spectrometry, Fluorescence - methods ; Spectrum analysis ; Studies</subject><ispartof>PloS one, 2014-07, Vol.9 (7), p.e103878-e103878</ispartof><rights>COPYRIGHT 2014 Public Library of Science</rights><rights>2014 Fonin et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. 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Inner filter effect correction</title><title>PloS one</title><addtitle>PLoS One</addtitle><description>Fluorescence is a proven tool in all fields of knowledge, including biology and medicine. A significant obstacle in its use is the nonlinearity of the dependence of the fluorescence intensity on fluorophore concentration that is caused by the so-called primary inner filter effect. The existing methods for correcting the fluorescence intensity are hard to implement in practice; thus, it is generally considered best to use dilute solutions. We showed that correction must be performed always. Furthermore, high-concentration solutions (high absorbance) are inherent condition in studying of the photophysical properties of fluorescent dyes and the functionally significant interactions of biological macromolecules. We proposed an easy to use method to correct the experimentally recorded total fluorescence intensity and showed that informative component of fluorescence intensity numerically equals to the product of the absorbance and the fluorescence quantum yield of the object. It is shown that if dye molecules do not interact with each other and there is no reabsorption (as for NATA) and spectrofluorimeter provides the proportionality of the detected fluorescence intensity to the part of the absorbed light (that is possible for spectrofluorimeter with horizontal slits) then the dependence of experimentally detected total fluorescence intensity of the dye on its absorbance coincides with the calculated dependence and the correction factor for eliminating the primary inner filter effect can be calculated on the basis of solution absorbance. It was experimentally shown for NATA fluorescence in the wide range of absorbance (at least up to 60). 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Academic</collection><collection>PubMed Central (Full Participant titles)</collection><collection>DOAJ Directory of Open Access Journals</collection><jtitle>PloS one</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Fonin, Alexander V</au><au>Sulatskaya, Anna I</au><au>Kuznetsova, Irina M</au><au>Turoverov, Konstantin K</au><au>Permyakov, Eugene A.</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Fluorescence of dyes in solutions with high absorbance. Inner filter effect correction</atitle><jtitle>PloS one</jtitle><addtitle>PLoS One</addtitle><date>2014-07-29</date><risdate>2014</risdate><volume>9</volume><issue>7</issue><spage>e103878</spage><epage>e103878</epage><pages>e103878-e103878</pages><issn>1932-6203</issn><eissn>1932-6203</eissn><abstract>Fluorescence is a proven tool in all fields of knowledge, including biology and medicine. A significant obstacle in its use is the nonlinearity of the dependence of the fluorescence intensity on fluorophore concentration that is caused by the so-called primary inner filter effect. The existing methods for correcting the fluorescence intensity are hard to implement in practice; thus, it is generally considered best to use dilute solutions. We showed that correction must be performed always. Furthermore, high-concentration solutions (high absorbance) are inherent condition in studying of the photophysical properties of fluorescent dyes and the functionally significant interactions of biological macromolecules. We proposed an easy to use method to correct the experimentally recorded total fluorescence intensity and showed that informative component of fluorescence intensity numerically equals to the product of the absorbance and the fluorescence quantum yield of the object. It is shown that if dye molecules do not interact with each other and there is no reabsorption (as for NATA) and spectrofluorimeter provides the proportionality of the detected fluorescence intensity to the part of the absorbed light (that is possible for spectrofluorimeter with horizontal slits) then the dependence of experimentally detected total fluorescence intensity of the dye on its absorbance coincides with the calculated dependence and the correction factor for eliminating the primary inner filter effect can be calculated on the basis of solution absorbance. It was experimentally shown for NATA fluorescence in the wide range of absorbance (at least up to 60). For ATTO-425, which fluorescence and absorption spectra overlap, the elimination of the primary and secondary filter effects and additional spectral analysis allow to conclude that the most probable reason of the deviation of experimentally detected fluorescence intensity dependence on solution absorbance from the calculated dependence is the dye molecules self-quenching, which accompanies resonance radiationless excitation energy transfer.</abstract><cop>United States</cop><pub>Public Library of Science</pub><pmid>25072376</pmid><doi>10.1371/journal.pone.0103878</doi><oa>free_for_read</oa></addata></record> |
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| subjects | Absorbance Absorption spectra Biology and Life Sciences Biophysics Cellular biology Dental caries Dilution Dyes Energy transfer Filtration - instrumentation Fluorescence Fluorescent dyes Fluorescent Dyes - chemistry Fluorescent indicators Laboratories Luminous intensity Macromolecules Methods Nonlinear systems Physical Sciences Protein folding Quantum Theory Reabsorption Slits Solutions - chemistry Spectral analysis Spectrometry, Fluorescence - instrumentation Spectrometry, Fluorescence - methods Spectrum analysis Studies |
| title | Fluorescence of dyes in solutions with high absorbance. Inner filter effect correction |
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