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Chromatographic authentication of botanical origin: Herbaceous pollen profiling with HPLC, HPTLC and GC–MS analysis

Nozimova AzizaInstitute of Biochemistry Samarkand State University Samarkand UzbekistanKhislat KhaydarovInstitute of Biochemistry Samarkand State University Samarkand UzbekistanMuhammad Zafar-ul-HyeDepartment of Plant Sciences Quaid‐i‐Azam University Islamabad PakistanWaleed A. A. AlsakkafDepartment of Botany and Microbiology, College of Science King Saud University Riyadh Saudi ArabiaJawaher AlkahtaniDepartment of Botany and Microbiology, College of Science King Saud University Riyadh Saudi ArabiaMushtaq AhmadCollege of Life Science Neijiang Normal University Neijiang ChinaTrobjon MakhkamovDepartment of Forestry and Landscape Design Tashkent State Agrarian University Tashkent Region UzbekistanZamira DjumayevaInstitute of Biochemistry Samarkand State University Samarkand UzbekistanGokhan ZenginDepartment of Biology University of Selcuk Konya TurkeyTursunboev Khamdam EshboyevichAgroecology and Introduction of Medicinal Plants department Karakalpak State University Nukus UzbekistanAferin BeilerliDepartment of Obstetrics and Gynecology Tyumen State Medical University Tyumen RussiaIlgiz GareevBashkir State Medical University Ufa Republic of Bashkortostan RussiaUlugbek OchilovInstitute of Biochemistry Samarkand State University Samarkand UzbekistanIslamov Boston SultanovichInstitute of Biochemistry Samarkand State University Samarkand UzbekistanUmurzakova Zebiniso IskandarovnaInstitute of Biochemistry Samarkand State University Samarkand UzbekistanI Putu Agus Hendra WibawaResearch Center for Applied Botany Nasional Research and Innovation Agency BRIN Bogor Jawa Barat Indonesia
Biomedical Chromatographyjournal2024en
ABI

Abstract

Abstract This study describes a robust chromatographic authentication methodology for herbaceous pollen, employing gas chromatography–mass spectrometry (GC–MS), high‐performance liquid chromatography (HPLC) and high‐performance thin liquid chromatography (HPTLC) protocols. The comprehensive profiling of organic compounds not only distinguishes between different botanical sources but also establishes a reliable framework for quality control and assessment of herbaceous pollen authenticity. Traces of quercetin were detectable using HPTLC in Chaenomeles japonica , and the composition of the mobile phase led to distinct phenolic acid tracks in the extracts of free phenolic compounds. In Lonicera nummulariifolia , prominent chlorogenic acid signal and traces of 3,4‐dihydroxybenzoic acid were identified, along with the presence of vanillic, trans ‐ferulic, p ‐coumaric and p ‐hydroxybenzoic and sinapic as phenolic acid standards. The HPLC chromatogram identified six peaks representing bioactive phenolic compounds such as gallic acid measuring 5.89 ± 0.56 mg g −1 , hydroxybenzoic acid 2.39 ± 0.78 mg g −1 and caffeic acid 2.83 ± 0.11 mg g −1 . The combined use of GC–MS, HPTLC and HPLC techniques provides a powerful and reliable means of authenticating the botanical origin of herbaceous pollen, offering valuable insights for quality control and ensuring the accuracy of botanical source identification.

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