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Carbon dots doped by nitrogen and sulfur for dual-mode colorimetric and fluorometric determination of Fe3+ and histidine and intracellular imaging of Fe3+ in living cells.
Amiri, Mojtaba; Haji Shabani, Ali Mohammad; Dadfarnia, Shayessteh; Shokoufi, Nader; Hajipour-Verdom, Behnam; Sadjadi, Sodeh.
Afiliación
  • Amiri M; Department of Chemistry, Yazd University, Safaieh, P.O. Box 89195-741, Yazd, Iran.
  • Haji Shabani AM; Department of Chemistry, Yazd University, Safaieh, P.O. Box 89195-741, Yazd, Iran. hshabani@yazd.ac.ir.
  • Dadfarnia S; Department of Chemistry, Yazd University, Safaieh, P.O. Box 89195-741, Yazd, Iran. sdadfarnia@yazd.ac.ir.
  • Shokoufi N; Analytical Instrumentation and Spectroscopy Laboratory, Faculty of Clean Technologies, Chemistry and Chemical Engineering Research Center of Iran, P.O. Box 14665-1513, Tehran, Iran.
  • Hajipour-Verdom B; Department of Biophysics, Faculty of Biological Sciences, Tarbiat Modares University, P.O. Box 14115-154, Tehran, Iran.
  • Sadjadi S; Radiation Application Research School, Nuclear Science and Technology Research Institute, P.O. Box 11365-3486, Tehran, Iran.
Mikrochim Acta ; 187(10): 562, 2020 Sep 12.
Article en En | MEDLINE | ID: mdl-32920698
ABSTRACT
The first dual-modality highly intensive fluorescent and colorimetric nanoprobe for Fe3+ ions and histidine is reported. The carbon dots doped by nitrogen and sulfur (N,S-CDs) prepared by the one-pot hydrothermal method have an excitation/emission wavelength of 320/420 nm with 56% quantum yield. N,S-CDs exhibit strong visible fluorescence with high stability at pH ~ 7.0. The fluorescence intensity of the N,S-CDs is quenched in the presence of Fe3+ ions which are recovered upon the addition of histidine. The addition of Fe3+ ions also induces a color change from yellow to red. Using colorimetric determination, Fe3+ and histidine exhibited linearity in the range 75-675 and 100-375 µmol L-1, respectively, while with fluorometric determinations the dynamic range was 0.1-275 and 0.1-3 µmol L-1 for Fe3+ and histidine, respectively. The limits of detection were 19 nmol L-1 and 0.03 µmol L-1 using fluorometry and 20 µmol L-1 and 24.2 µmol L-1 using colorimetry, for Fe3+ and histidine respectively. The relative standard deviations (n = 5) for Fe3+ (10 µmol L-1) and histidine (1 µmol L-1) using fluorometry were 4.6 and 7.3% and using colorimetry at 100 µmol L-1 of Fe3+ and 150 µmol L-1 of histidine were 3.2 and 5.6%, respectively. The developed fluorometric method was applied for the determination of Fe3+ and histidine in various foods and biological fluid samples as well as intracellular imaging of iron. The accuracy of the method for iron determination was confirmed by the analysis of certified reference materials (wheat flour, tomato leaves, and whole milk powder) and quality control materials (whole milk powder, serum, and urine), whereas for histidine, the accuracy was determined by recovery experiment and independent analysis. Good recovery values in ranges of 92-96% and 94-98% were achieved for Fe3+ and histidine, respectively. Graphical abstract.
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Texto completo: 1 Colección: 01-internacional Banco de datos: MEDLINE Asunto principal: Azufre / Colorimetría / Puntos Cuánticos / Fluorometría / Histidina / Hierro / Nitrógeno Límite: Humans Idioma: En Revista: Mikrochim Acta Año: 2020 Tipo del documento: Article País de afiliación: Irán
Texto completo
Imprimir
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Texto completo: 1 Colección: 01-internacional Banco de datos: MEDLINE Asunto principal: Azufre / Colorimetría / Puntos Cuánticos / Fluorometría / Histidina / Hierro / Nitrógeno Límite: Humans Idioma: En Revista: Mikrochim Acta Año: 2020 Tipo del documento: Article País de afiliación: Irán