Binding site identification of anticancer drug gefitinib to HSA and DNA in the presence of five different probes.

AO: Acridine Orange ATP: Adenosine TriPhosphate BSA: Bovine Serum Albumin DMSO: Dimethyl Sulfoxide EB: Ethidium Bromide FDA: Food and Drug Administration FRET: Fluorescence Resonance Energy Transfer GEF: Gefitinib HO: Hoechst HSA: Human Serum Albumin IBU: Ibuprofen MB: Methylene Blue WAR: Warfarin calf thymus DNA ctDNA: calf thymus DNA fluorescence spectroscopy gefitinib human serum albumin molecular modeling zeta potential Δ: Enthalpy changes Δ: Entropy changes Δ: Gibbs free energy

Journal

Journal of biomolecular structure & dynamics
ISSN: 1538-0254
Titre abrégé: J Biomol Struct Dyn
Pays: England
ID NLM: 8404176

Informations de publication

Date de publication:
03 2019
Historique:
pubmed: 16 2 2018
medline: 27 2 2020
entrez: 16 2 2018
Statut: ppublish

Résumé

This study was carried out to evaluate the binding interaction of gefitinib (GEF) with human serum albumin (HSA) and calf thymus DNA (ct-DNA) using fluorescence, UV-Visible, zeta potential measurements and molecular docking methods in order to understand its pharmacokinetic mechanism. By increasing the temperature, a steady decrease in Stern-Volmer quenching constants was observed for HSA binding properties; this indicates a static type of fluorescence quenching. Negative values were calculated for Gibbs free energy (ΔG), enthalpy (ΔH), and entropy (ΔS) changes, indicating that the reaction is spontaneous and enthalpy-driven. Probe competitive experimental results showed that GEF contains the same binding site as warfarin and are consistent with modeling results. The zeta potential of the HSA increased with increasing GEF, which represents the presence of electrostatic interactions in the system. DNA binding properties were investigated in the presence of three probes. The experimental results showed that by increasing GEF to DNA-AO (acridine-orange) and DNA-MB (methylene-blue) system, the fluorescence intensity and absorbance spectra had no considerable change. Furthermore, with the addition of GEF to DNA, the zeta potential decreased gradually, indicating that the hydrophobic interaction between the GEF and the bases of DNA is the major factor. Thus, GEF can bind to DNA via a groove binding mode. It was also found that GEF entered into the minor groove in the A-T rich region of DNA fragment and bind via van der-Waals forces and three H-bond with double strands of DNA. This is in good agreement with experimental results.

Identifiants

pubmed: 29447084
doi: 10.1080/07391102.2018.1441073
doi:

Substances chimiques

Antineoplastic Agents 0
Fluorescent Dyes 0
DNA 9007-49-2
calf thymus DNA 91080-16-9
Gefitinib S65743JHBS
Serum Albumin, Human ZIF514RVZR

Types de publication

Journal Article

Langues

eng

Sous-ensembles de citation

IM

Pagination

823-836

Auteurs

Hamid Tanzadehpanah (H)

a Research Center for Molecular Medicine , Hamadan University of Medical Sciences , Hamadan , Iran.

Hanie Mahaki (H)

b Department of Immunology, School of Medicine , Hamadan University of Medical Sciences , Hamadan , Iran.

Neda Hosseinpour Moghadam (NH)

c Faculty of Chemistry , Bu-Ali Sina University , Hamedan , Iran.

Sadegh Salehzadeh (S)

c Faculty of Chemistry , Bu-Ali Sina University , Hamedan , Iran.

Omid Rajabi (O)

d Medical Chemistry Department, School of Pharmacy , Mashhad University of Medical Sciences , Mashhad , Iran.

Rezvan Najafi (R)

a Research Center for Molecular Medicine , Hamadan University of Medical Sciences , Hamadan , Iran.

Razieh Amini (R)

a Research Center for Molecular Medicine , Hamadan University of Medical Sciences , Hamadan , Iran.

Massoud Saidijam (M)

a Research Center for Molecular Medicine , Hamadan University of Medical Sciences , Hamadan , Iran.

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