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Chlorogenic Acid: HPLC Quantification and In Vitro Assessment of Proliferative and Migration Effects on Human Dermal Fibroblast Cells

dc.contributor.authorAkpınar, Abdulbaki
dc.contributor.authorDemirkaya Miloğlu, Fatma
dc.contributor.authorGündoğdu, Gülşah
dc.contributor.authorGüven, Leyla
dc.contributor.authorBayrak, Burak
dc.contributor.authorKadıoğlu, Yücel
dc.date.accessioned2026-01-04T20:36:45Z
dc.date.issued2024-06-30
dc.description.abstractChlorogenic acid (CA) exhibits diverse biological activities, including antioxidant and antiinflammatory effects. This research aims to develop, optimize, and validate an HPLC method to quantify CA in methanol and investigate its in vitro proliferative and cell migration effects on human-dermal-fibroblast (HDF) cell lines in a dose-dependent manner. The HPLC experimental conditions were optimized using the central composite design (CCD) method for determining CA. Chromatographic separation occurred at a wavelength of 330 nm. Under the optimized conditions, the method exhibited linearity across a concentration range of 0.1-100 µg/mL, demonstrating sensitivity (LOQ:0.1µg/mL), precision (RSD%≤3.32), and accuracy (RE%≤4.05). To evaluate the in vitro proliferative and cell migration effects on HDFs, we employed the XTT cell proliferation assay and TAS-TOS commercial kits. The XTT assay revealed that CA displayed a proliferative effect within the concentration range of 75-250 µM (P <0.01), and at a concentration of 125 µM, TAS levels increased significantly (P<0.05). The scratch assay demonstrated that HDF cell migration increased at 12 h, with substantial closure of the wound area at 24 h when treated with CA concentrations between 75-125 µM. The results demonstrate that pure chlorogenic acid extracted from plants exhibits dose-dependent effects on cell proliferation, antioxidant, and cell migration
dc.description.urihttps://doi.org/10.17776/csj.1440382
dc.description.urihttps://hdl.handle.net/11499/57664
dc.description.urihttps://avesis.atauni.edu.tr/publication/details/60f2ff3a-b4de-436d-9b8b-08aef3bbb415/oai
dc.description.urihttps://dergipark.org.tr/tr/pub/csj/issue/85631/1440382
dc.description.urihttps://doi.org/https://doi.org/10.17776/csj.1440382
dc.identifier.doi10.17776/csj.1440382
dc.identifier.endpage308
dc.identifier.issn2587-2680
dc.identifier.openairedoi_dedup___::d97a66a1d7193880ffa9ed5dba450a04
dc.identifier.orcid0000-0001-7318-6529
dc.identifier.orcid0000-0001-5729-7181
dc.identifier.orcid0000-0002-9924-5176
dc.identifier.orcid0000-0002-3189-6415
dc.identifier.orcid0000-0001-6550-6916
dc.identifier.orcid0000-0001-6590-7306
dc.identifier.startpage299
dc.identifier.urihttps://hdl.handle.net/20.500.12597/41919
dc.identifier.volume45
dc.publisherCumhuriyet University
dc.relation.ispartofCumhuriyet Science Journal
dc.rightsOPEN
dc.subjectChlorogenic acid
dc.subjectHPLC
dc.subjectExperimental design
dc.subjectCentral composite design
dc.subjectQuality Assurance, Chemometrics, Traceability and Metrological Chemistry
dc.subjectKalite Kontrolü, Kemometri, İzlenebilirlik ve Metrolojik Kimya
dc.titleChlorogenic Acid: HPLC Quantification and In Vitro Assessment of Proliferative and Migration Effects on Human Dermal Fibroblast Cells
dc.typeArticle
dspace.entity.typePublication
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This research aims to develop, optimize, and validate an HPLC method to quantify CA in methanol and investigate its in vitro proliferative and cell migration effects on human-dermal-fibroblast (HDF) cell lines in a dose-dependent manner. The HPLC experimental conditions were optimized using the central composite design (CCD) method for determining CA. Chromatographic separation occurred at a wavelength of 330 nm. Under the optimized conditions, the method exhibited linearity across a concentration range of 0.1-100 µg/mL, demonstrating sensitivity (LOQ:0.1µg/mL), precision (RSD%≤3.32), and accuracy (RE%≤4.05). To evaluate the in vitro proliferative and cell migration effects on HDFs, we employed the XTT cell proliferation assay and TAS-TOS commercial kits. The XTT assay revealed that CA displayed a proliferative effect within the concentration range of 75-250 µM (P &amp;lt;0.01), and at a concentration of 125 µM, TAS levels increased significantly (P&amp;lt;0.05). The scratch assay demonstrated that HDF cell migration increased at 12 h, with substantial closure of the wound area at 24 h when treated with CA concentrations between 75-125 µM. 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