Cytotoxicity evaluation of uncaria gambir extract towards fibroblast cell

Fayyadhah Binti Mohd Azmi (P87451)

Please use this identifier to cite or link to this item: https://ptsldigital.ukm.my/jspui/handle/123456789/485654

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DC Field	Value	Language
dc.contributor.advisor	Ahmad Shuhud Irfani Zakaria, Dr.
dc.contributor.author	Fayyadhah Binti Mohd Azmi (P87451)
dc.date.accessioned	2023-10-10T08:28:43Z	-
dc.date.available	2023-10-10T08:28:43Z	-
dc.date.issued	2019-05-31
dc.identifier.other	ukmvital:119497
dc.identifier.uri	https://ptsldigital.ukm.my/jspui/handle/123456789/485654	-
dc.description	Uncaria gambir extracts consist of catechin, which has been shown to have anti-inflammatory and antibacterial properties. Traditionally, Uncaria gambir has been used for treatment of toothache and spongy gum, highlighting its potential use in dentistry. However, the cytotoxicity of this extract has never been investigated. The study aimed to determine the cytotoxicity of Uncaria gambir extracts towards fibroblast cells in vitro. Uncaria gambir extracts was dissolved in 1% DMSO and was diluted into two-fold dilutions with culture media into eight different concentrations, ranging from 7.8 μg/ml to 1000 μg/ml. After an initial incubation of 24 hours in the 96-well plates, MC3T3 fibroblast cells were treated with various concentrations of the extracts and incubated for 24 hours in triplicates. 10% DMSO and culture media were used as positive and negative controls respectively. Cell viability was measured using Alamar Blue, DNA Fluorescence and Neutral Red Uptake (NRU) assays. Morphological changes of the cell were determined using Field Emission Scanning Electron Microscope (FESEM) and LIVE/DEAD cell analysis. Both DNA Fluorescence and Alamar Blue assays showed no cytotoxic effects of the extract towards the fibroblast cells at all concentrations with the mean percentage of cell viability of more than 70%. However, NRU assay showed that the extract was not cytotoxic at concentration lower than 500 μg/ml and was cytotoxic at 1000 μg/ml. The half maximal inhibitory concentration (IC50) of the extract measured using Alamar Blue, DNA Fluorescence and NRU assays were 1751 μg/ml, 3109 μg/ml and 1031 μg/ml, respectively. Significant morphological changes of the cells were observed at 1000 μg/ml with marked shrinkage in size and ruptured cell membrane using FESEM. LIVE/DEAD cell analysis showed a mixture of red and green fluorescence in a low density cell population as compared to negative control. Conclusively, the Uncaria gambir extracts was not cytotoxic towards MC3T3 fibroblast cells at a concentration below than 500 μg/ml when tested in-vitro.,Ijazah Sarjana Doktor Pergigian Klinikal (Pergigian Pediatrik)
dc.language.iso	eng
dc.publisher	UKM, Kuala Lumpur
dc.relation	Faculty of Pharmacy / Fakulti Farmasi
dc.rights	UKM
dc.subject	Fibroblast Growth Factors
dc.subject	Universiti Kebangsaan Malaysia -- Dissertations
dc.subject	Dissertations, Academic -- Malaysia
dc.title	Cytotoxicity evaluation of uncaria gambir extract towards fibroblast cell
dc.type	Theses
dc.format.pages	31
dc.identifier.callno	9 Tesis Cd QU107. F286c 2019
Appears in Collections:	Faculty of Pharmacy / Fakulti Farmasi

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