番荔枝叶提取物体外抗炎和抗氧化活性的研究

Idorenyin Nwaehujor, S. Akande, O. Atolani, G. Olatunji
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摘要

文章历史:收稿日期:2019年5月3日接收日期:2020年5月28日炎症在许多人类疾病中具有重要意义,引起了全世界的科学兴趣。大多数炎症是由活性氧或自由基引起的。研究了番荔枝叶提取物的体外抗氧化和抗炎活性。番荔枝叶在室温下干燥,用磨机混合。用不同极性的溶剂萃取。所用溶剂为己烷、乙酸乙酯和乙醇。依次提取粗提物后,通过脂氧合酶抑制、蛋白酶抑制、白蛋白变性抑制、红细胞稳定等实验检测其体外抗炎活性,并通过DPPH、ABTS和过氧化氢实验检测其抗氧化活性。结果表明,在500 μg/mL浓度下,乙醇提取物对白蛋白变性的抑制活性显著提高(p < 0.01)。各提取物对蛋白酶的抑制活性均随提取物浓度的增加而降低。吲哚美辛(标准)、乙醇提取物和乙酸乙酯提取物均表现出剂量依赖性的脂氧合酶活性增加。乙醇提取物在500 μg/mL时具有较高的红细胞稳定活性,其活性与标准品双氯芬酸相当。过氧化氢清除活性在20 ~ 100 μg/mL范围内与标准品(维生素C)相当。乙醇提取物对DPPH自由基的清除能力极显著高于其他提取物(p < 0.01)。ABTS自由基清除活性也有类似的趋势。一般来说,乙醇提取物在大多数试验中表现出较高的抗炎和抗氧化活性,这可能归因于提取物中存在的极性化合物。
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Studies on In-vitro Anti-inflammatory and Antioxidant Potentials of Annona muricata Leaf Extracts
Article history: Received: May 3, 2019 Accepted: May 28, 2020 Inflammation has stimulated significant worldwide scientific interest because of its implication in many human diseases. Most inflammations are caused by reactive oxygen species or free radicals. Annona muricata leaf extracts were investigated for their in-vitro antioxidant and anti-inflammatory potentials. Annona muricata leaves were dried at room temperature, blended using a mill. and extracted with solvents of varying degree of polarities. The solvents used were hexane, ethyl acetate, and ethanol. After sequential extraction, the crude extracts were examined for their in-vitro anti-inflammatory activities on lipoxygenase inhibition, proteinase inhibition, albumin denaturation inhibition, and red blood cell membrane stabilization assays, while the antioxidant activities were examined using DPPH, ABTS and hydrogen peroxide assays. The results showed that the ethanol extract had significantly higher albumin denaturation inhibition activity at 500 μg/mL (p < 0.01). The activity of all the extracts on proteinase inhibition decreased with the increase in concentration of the extracts. Indomethacin (standard), ethanol extract, and ethyl acetate extract exhibited a dose dependent increase in lipoxygenase activity. The ethanol extract showed high red blood cell membrane stabilization activity at 500 μg/mL and the activity was comparable with that of the standard (diclofenac). Hydrogen peroxide scavenging activity of the extracts and standard (Vitamin C) were comparable at 20 – 100 μg/mL. The ethanol extract showed significantly higher (p < 0.01) DPPH radical scavenging activity compared with other extracts. A similar trend was also observed for ABTS radical scavenging activity. Generally, the ethanol extract exhibited higher antiinflammatory and antioxidant activities in most of the assays, this could be attributed to the polar compounds present in the extract.
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