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Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters

A fluorometric method was proposed for the determination of Fe(3+) and ascorbic acid (AA) based on blue and red dual fluorescence emissions of glutathione (GSH) stabilized-gold nanoclusters (AuNCs). AuNCs were synthesized from GSH and tetrachloroauric acid. The fluorescence peaks of AuNCs were at 42...

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Autores principales: Zhang, Shuai, Zhang, Cong, Shao, Xiaodong, Guan, Rentian, Hu, Yingying, Zhang, Keying, Liu, Wenjing, Hong, Min, Yue, Qiaoli
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The Royal Society of Chemistry 2021
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9032689/
https://www.ncbi.nlm.nih.gov/pubmed/35479669
http://dx.doi.org/10.1039/d0ra10281d
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author Zhang, Shuai
Zhang, Cong
Shao, Xiaodong
Guan, Rentian
Hu, Yingying
Zhang, Keying
Liu, Wenjing
Hong, Min
Yue, Qiaoli
author_facet Zhang, Shuai
Zhang, Cong
Shao, Xiaodong
Guan, Rentian
Hu, Yingying
Zhang, Keying
Liu, Wenjing
Hong, Min
Yue, Qiaoli
author_sort Zhang, Shuai
collection PubMed
description A fluorometric method was proposed for the determination of Fe(3+) and ascorbic acid (AA) based on blue and red dual fluorescence emissions of glutathione (GSH) stabilized-gold nanoclusters (AuNCs). AuNCs were synthesized from GSH and tetrachloroauric acid. The fluorescence peaks of AuNCs were at 425 nm and 585 nm, respectively. In the presence of Fe(3+), the fluorescence peak at 425 nm can be enhanced and that at 585 nm can be quenched. There is a good linear relationship between the fluorescence intensity ratio for the 425 and 585 nm peaks (F(425)/F(585)) and the concentration of Fe(3+) in the range of 0.75–125 μM. However, when AA was added to the AuNCs–Fe(3+) system, the value of F(425)/F(585) decreased consistently with the concentration of AA in the range of 0.25–35 μM. The limit of detection for Fe(3+) and AA was 227 and 75.8 nM, respectively. The interaction between AuNCs and Fe(3+) can induce the ligand–metal charge transfer (LMCT) effect leading to the fluorescence increment at 425 nm, while AA can reduce Fe(3+) to Fe(2+). The production of Fe(2+) can not enhance or quench the fluorescence of AuNCs. By comparison with previous literature, the AuNCs prepared here show two fluorescence peaks without additional fluorescence labels. Furthermore, the method was successfully applied in the determination of Fe(3+) and AA in some real samples, such as water, human serum and tablets.
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spelling pubmed-90326892022-04-26 Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters Zhang, Shuai Zhang, Cong Shao, Xiaodong Guan, Rentian Hu, Yingying Zhang, Keying Liu, Wenjing Hong, Min Yue, Qiaoli RSC Adv Chemistry A fluorometric method was proposed for the determination of Fe(3+) and ascorbic acid (AA) based on blue and red dual fluorescence emissions of glutathione (GSH) stabilized-gold nanoclusters (AuNCs). AuNCs were synthesized from GSH and tetrachloroauric acid. The fluorescence peaks of AuNCs were at 425 nm and 585 nm, respectively. In the presence of Fe(3+), the fluorescence peak at 425 nm can be enhanced and that at 585 nm can be quenched. There is a good linear relationship between the fluorescence intensity ratio for the 425 and 585 nm peaks (F(425)/F(585)) and the concentration of Fe(3+) in the range of 0.75–125 μM. However, when AA was added to the AuNCs–Fe(3+) system, the value of F(425)/F(585) decreased consistently with the concentration of AA in the range of 0.25–35 μM. The limit of detection for Fe(3+) and AA was 227 and 75.8 nM, respectively. The interaction between AuNCs and Fe(3+) can induce the ligand–metal charge transfer (LMCT) effect leading to the fluorescence increment at 425 nm, while AA can reduce Fe(3+) to Fe(2+). The production of Fe(2+) can not enhance or quench the fluorescence of AuNCs. By comparison with previous literature, the AuNCs prepared here show two fluorescence peaks without additional fluorescence labels. Furthermore, the method was successfully applied in the determination of Fe(3+) and AA in some real samples, such as water, human serum and tablets. The Royal Society of Chemistry 2021-05-11 /pmc/articles/PMC9032689/ /pubmed/35479669 http://dx.doi.org/10.1039/d0ra10281d Text en This journal is © The Royal Society of Chemistry https://creativecommons.org/licenses/by-nc/3.0/
spellingShingle Chemistry
Zhang, Shuai
Zhang, Cong
Shao, Xiaodong
Guan, Rentian
Hu, Yingying
Zhang, Keying
Liu, Wenjing
Hong, Min
Yue, Qiaoli
Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters
title Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters
title_full Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters
title_fullStr Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters
title_full_unstemmed Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters
title_short Dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters
title_sort dual-emission ratio fluorescence for selective and sensitive detection of ferric ions and ascorbic acid based on one-pot synthesis of glutathione protected gold nanoclusters
topic Chemistry
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9032689/
https://www.ncbi.nlm.nih.gov/pubmed/35479669
http://dx.doi.org/10.1039/d0ra10281d
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