ISOLASI SENYAWA AKTIF INHIBITOR ENZIM TIROSINASE DARI FRAKSI N-HEKSANA KULIT BATANG KAYU MANIS (CINNAMOMUM BURMANNII (NEES & T. NEES) BLUME)
Hyperpigmentation is described as one of skin disorder showed by the increase in melanin production. The tyrosinase enzyme acts as a catalyst during melanogenesis. Previous studies have shown that there were polyphenolic compounds in essential oils and triterpenoids in the n-hexane fraction of...
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| Format: | Final Project |
| Language: | Indonesia |
| Online Access: | https://digilib.itb.ac.id/gdl/view/78167 |
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| Institution: | Institut Teknologi Bandung |
| Language: | Indonesia |
| Summary: | Hyperpigmentation is described as one of skin disorder showed by the increase in melanin
production. The tyrosinase enzyme acts as a catalyst during melanogenesis. Previous studies have
shown that there were polyphenolic compounds in essential oils and triterpenoids in the n-hexane
fraction of cinnamon bark (Cinnamomum burmannii (Nees & T. Nees) Blume) which inhibited the
tyrosinase. This study aims to determine the potency of extracts and fractions of cinnamon bark
(C. burmannii) as inhibitors of the tyrosinase enzyme, to isolate the active compounds as inhibitors
of the tyrosinase enzyme in the n-hexane fraction of cinnamon bark, and followed by the isolate
characterization and identification. Crud drug was extracted by maceration with 96% ethanol.
Fractionation was carried out using the liquid-liquid extraction method using n-hexane, ethyl
acetate, and ethanol-water as solvents. Extracts and fractions were monitored by TLC using
universal and specific spray reagent. The inhibitory effect was determined qualitatively using the
bioautographic TLC method and quantitatively by calculating the IC50 value. The chromatogram of
bioautographic showed tyrosinase inhibition in the extract, n-hexane fraction, ethyl acetate
fraction, ethanol-water fraction, and kojic acid as a comparison. The ethanol extract, n-hexane
fraction, ethyl acetate fraction, ethanol-water fraction, and kojic acid had IC50 values of 6,496.83
± 267.44; 637.88 ± 37.11; 3,612.28 ± 73.53; >12,000 (37.23% inhibition at a concentration of 12,000
µg/mL); 8.40 ± 1.24 µg/mL respectively. Subfractionation and purification was carried out using
consecutive classical column chromatography method. The purity was checked using a single
development TLC method with three mobile phases and two-dimensional TLC. The results of the
purity test obtained isolate X which was tested for its activity qualitatively. Isolate X was
characterized by specific single spot appearance, IR spectrophotometry, and TLC densitometry. The
n-hexane fraction showed the strongest tyrosinase enzyme inhibitory activity, followed by the
ethyl acetate fraction and the ethanol extract. Meanwhile, the ethanol-water fraction only showed
inhibition below 50% at a 12,000 µg/mL. The Isolate X from n-hexane fraction of cinnamon bark
showed inhibition activity against tyrosinase qualitatively and identified as a flavonoid compound
of the isoflavone subgroup.
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