Characterization, Antioxidant and Cytotoxic Evaluation of Demethoxycurcumin and Bisdemethoxycurcumin from Curcuma longa Cultivated in Costa Rica

A. M. Araya-Sibaja, Felipe Vargas-Huertas, Silvia Quesada, Gabriela Azofeifa, J. Vega-baudrit, Mirtha Navarro-Hoyos
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Abstract

The biological activities of curcuminoids, the main polyphenol constituents of Curcuma longa (turmeric), have been the subject of many studies in recent years. However, these studies have focused on the major active compound, curcumin (CUR), while other important constituents, demethoxycurcumin (DMC) and bisdemethoxycurcumin (BDM) have been less studied and reported in the literature regarding their bioactivity as well as their isolation and solid-state characterization. Hence, in this study, DMC and BDM were isolated using pressurized liquid extraction (PLE) followed by column chromatography and crystallization. HRMS and 1H and 13C NMR were used to characterize them. Solid-state characterization was performed through powder X-ray diffraction (PXRD), Fourier transform infrared spectroscopy (FT-IR), differential scanning calorimetry (DSC), and scanning electron microscopy (SEM) techniques. Further, powder dissolution profiles were performed in two media, antioxidant and cytotoxic activities were determined through 2,2-diphenyl-1-picrylhidrazyl (DPPH) and an MTT assay on gastric adenocarcinoma (AGS), colorectal adenocarcinoma (SW-620), and hepatocellular carcinoma (HepG2) cell lines. DMC and BDM were extracted from Curcuma longa cultivated in Costa Rica, using pressurized liquid extraction (PLE), then isolated and purified, combining column chromatography and crystallization techniques. The highly pure solids obtained were shown to be crystalline with an amorphous component. Although the PXRD pattern of BDM suggested a high amorphous component, the crystal exhibited a well-defined and faceted shape. Meanwhile, DMC crystallized in a botryoidal habit, and this constitutes the first report for this compound. On the other hand, BDM was slightly more soluble than DMC, which in turn showed an antioxidant IC50 value 28% higher than BDM (12.46 and 17.94 µg/mL, respectively). In respect to the cytotoxic effects, DMC showed a better IC50 value than BDM for both the SW-620 and AGS cell lines, while BDM exhibited a better IC50 value than DMC against the HepG2 cell line (64.7 μM). In terms of selectivity, BDM and DMC had the highest SI value for SW-620 cells compared to non-tumoral cells, while both compounds also displayed the best cytotoxic effect against these colon adenocarcinoma SW-620 cells, indicating BDM and DMC as potential chemotherapeutic drugs.
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哥斯达黎加种植的莪术中的去甲氧基姜黄素和双去甲氧基姜黄素的特性、抗氧化性和细胞毒性评估
姜黄素是姜黄的主要多酚成分,其生物活性是近年来许多研究的主题。不过,这些研究主要集中在主要活性化合物姜黄素(CUR)上,而对其他重要成分,如去甲氧基姜黄素(DMC)和双去甲氧基姜黄素(BDM)的生物活性、分离和固态表征研究较少,文献报道也较少。因此,本研究采用加压液体萃取法(PLE)分离 DMC 和 BDM,然后进行柱层析和结晶。利用 HRMS 以及 1H 和 13C NMR 对它们进行了表征。通过粉末 X 射线衍射 (PXRD)、傅立叶变换红外光谱 (FT-IR)、差示扫描量热 (DSC) 和扫描电子显微镜 (SEM) 技术进行了固态表征。此外,还在两种介质中进行了粉末溶解度分析,并通过 2,2-二苯基-1-苦基肼(DPPH)和 MTT 法测定了胃腺癌(AGS)、结直肠腺癌(SW-620)和肝癌(HepG2)细胞系的抗氧化性和细胞毒性活性。利用加压液体萃取(PLE)技术从哥斯达黎加种植的莪术中提取出 DMC 和 BDM,然后结合柱层析和结晶技术进行分离和纯化。结果表明,所获得的高纯度固体为晶体,其中含有无定形成分。虽然 BDM 的 PXRD 图谱显示其无定形成分较多,但晶体却呈现出清晰的刻面形状。与此同时,DMC 的结晶呈类杏仁状,这是该化合物的首次报道。另一方面,BDM 的溶解度略高于 DMC,而 DMC 的抗氧化 IC50 值比 BDM 高 28%(分别为 12.46 和 17.94 µg/mL)。在细胞毒性效应方面,DMC 对 SW-620 和 AGS 细胞系的 IC50 值均优于 BDM,而 BDM 对 HepG2 细胞系的 IC50 值(64.7 μM)优于 DMC。在选择性方面,与非肿瘤细胞相比,BDM 和 DMC 对 SW-620 细胞的 SI 值最高,同时这两种化合物对结肠腺癌 SW-620 细胞的细胞毒性效果也最好,这表明 BDM 和 DMC 是潜在的化疗药物。
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