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HPTLC – Bioautographic methods for selective detection of the antioxidant and α-amylase inhibitory activity in plant extracts

机译:HPTLC –用于选择性检测植物提取物中抗氧化剂和α-淀粉酶抑制活性的生物自显影方法

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class="kwd-title">Method name: Measuring α-amylase inhibition class="kwd-title">Keywords: α-Amylase inhibition, Bioautography, Bioassay, Phytochemical analysis, Stigmasterol class="head no_bottom_margin" id="abs0010title">AbstractA high-performance thin-layer chromatography (HPTLC) method was developed for quantification of α-amylase inhibitory activity and stigmasterol content in ant plant extracts. An improved HPTLC method for the determination of total free radical scavenging activity in samples using DPPH• is also reported. For quantification of α-amylase inhibitory activity, the developed HPTLC plate is dipped into an α-amylase solution, and the bioautogram is then incubated at 25 °C for 30 min under humid conditions. For visualization of enzyme inhibitory activity, the starch test with an iodine indicator solution is used. The blue zone observed comes from the starch-iodine complex formed from starch that was not hydrolyzed by the amylase due to enzyme inhibition by the compound(s) present in the sample. The area of the blue zones was used to compare and quantify relative α-amylase inhibitory activity in different extracts. Location of the blue zones (hRF) on the plate was used to detect compounds that are responsible for the α-amylase inhibitory activity. Relative α-amylase activity was not related to the antioxidant activity, but was highly correlated with the stigmasterol content in the sample extracts (R = 0.95). Therefore, plant sterols present in the extracts might be responsible for α-amylase inhibitory activities in the extracts. class="first-line-outdent" id="lis0005">
  • • The developed method for quantification of α-amylase inhibitory activity provides an efficient and effective tool that can be used to screen, detect and quantify α-amylase inhibitory activity in plant extracts.
  • • The proposed protocol is easy to run, involves minimal sample preparation, with multiple samples able to be analyzed in parallel on the same chromatographic plate, in a short time.
  • • There were significant differences in α-amylase inhibitory activity, stigmasterol content, and total free radical scavenging activity between methanol, ethanol, dichloromethane, and ethyl acetate ant plant extracts.
    • 机译:<!-fig ft0-> <!-fig @ position =“ anchor” mode =文章f4-> <!-fig mode =“ anchred” f5-> <!-fig / graphic | fig / alternatives / graphic mode =“ anchored” m1-> class =“ kwd-title”>方法名称:测量α-淀粉酶抑制作用 class =“ kwd-title”>关键字:α-淀粉酶抑制,生物自显影,生物测定,植物化学分析,Stigmasterol class =“ head no_bottom_margin” id =“ abs0010title”>摘要开发了一种高效薄层色谱法(HPTLC)用于定量蚂蚁植物提取物中的α-淀粉酶抑制活性和豆甾醇含量。还报告了一种改进的HPTLC方法,该方法使用DPPH•测定样品中的总自由基清除活性。为了定量检测α-淀粉酶的抑制活性,将已开发的HPTLC板浸入α-淀粉酶溶液中,然后将生物自传体在25°C下于潮湿条件下孵育30分钟。为了可视化酶抑制活性,使用了含碘指示剂溶液的淀粉测试。观察到的蓝色区域来自淀粉-淀粉-碘复合物,该复合物由淀粉形成,由于样品中存在的一种或多种化合物对酶的抑制作用,淀粉复合物未被淀粉酶水解。蓝色区域的面积用于比较和定量不同提取物中的相对α-淀粉酶抑制活性。板上蓝色区域(hRF)的位置用于检测负责α-淀粉酶抑制活性的化合物。相对的α-淀粉酶活性与抗氧化活性无关,但与样品提取物中豆甾醇的含量高度相关(R = 0.95)。因此,提取物中存在的植物固醇可能负责提取物中的α-淀粉酶抑制活性。 class =“ first-line-outdent” id =“ lis0005”> <!-list-behavior =简单的前缀词= mark-type = none max-label-size = 9->
  • •开发的定量α-淀粉酶抑制活性的方法提供了一种有效且有效的工具,可用于筛选,检测并量化植物提取物中的α-淀粉酶抑制活性。
  • •拟议的方案易于操作,只需最少的样品制备,即可在同一色谱上并行分析多个样品
  • •在甲醇,乙醇,二氯甲烷和乙酸乙酯之间,α-淀粉酶的抑制活性,豆固醇含量和总自由基清除活性存在显着差异蚂蚁植物提取物。

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