Enantiomeric separation of flavanone on Chiralpak® IA column and determination of the chiral mechanism

Author:

Ali Imran1ORCID,Mimouni Fatima Zohra2,Belboukhari Nasser2,Sekkoum Khaled2,Locatelli Marcello3,Demir Ersin4,Yusuf Kareem5

Affiliation:

1. Department of Chemistry Jamia Millia Islamia (Central University) New Delhi India

2. Bioactive Molecules & Chiral Separation Laboratory, Faculty of Exact Sciences University Tahri Mohamed of Béchar Béchar Algeria

3. Department of Pharmacy University “G. d'Annunzio” of Chieti‐Pescara Chieti Italy

4. Faculty of Pharmacy, Department of Analytical Chemistry Afyonkarahisar Health Sciences University Afyonkarahisar Turkey

5. Department of Chemistry, College of Science King Saud University Riyadh Saudi Arabia

Abstract

AbstractThirteen flavanone racemates were successfully separated using a Chiralpak® IA column and isopropanol‐hexane (50:50, v/v). The mobile phase flow rate and detection wavelength were 0.5 mL/min and 254 nm. The retention times values ranged from 5.50 and 56.45 min. The values of the retention, separation, and resolution factors ranged from 0.63 to 21.67, 1.12 to 2.45, and 0.13 to 11.94. The docking binding energies ranged from −6.2 to −8.2 kcal/mol, showing enthalpy‐determined host‐guest complex formation. The molecular docking results and the experimental data were agreed well. The results showed that S‐enantiomers had stronger bindings with chiral selectors compared to R‐enantiomers. Consequently, the R‐enantiomers eluted first followed by S‐enantiomers. The reported method is highly useful to determine the enantiomeric composition of the reported flavanone in any sample.

Funder

King Saud University

Publisher

Wiley

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