Background: Glucosinolates, anionic sulfur rich secondary metabolites, have been extensively studied because of their occurrence in the agriculturally important brassicaceae and their impact on human and animal health. There is also increasing interest in the biofumigant properties of toxic glucosinolate hydrolysis products as a method to control agricultural pests. Evaluating biofumigation potential requires rapid and accurate quantification of glucosinolates, but current commonly used methods of extraction prior to analysis involve a number of time consuming and hazardous steps; this study aimed to develop an improved method for glucosinolate extraction. Results: Three methods previously used to extract glucosinolates from brassicaceae tissues, namely extraction in cold methanol, extraction in boiling methanol, and extraction in boiling water were compared across tissue type (root, stem leaf ) and four brassicaceae species (B. juncea, S. alba, R. sativus, and E. sativa). Cold methanol extraction was shown to perform as well or better than all other tested methods for extraction of glucosinolates with the exception of glucoraphasatin in R. sativus shoots. It was also demonstrated that lyophilisation methods, routinely used during extraction to allow tissue disruption, can reduce final glucosinolate concentrations and that extracting from frozen wet tissue samples in cold 80% methanol is more effective. Conclusions: We present a simplified method for extracting glucosinolates from plant tissues which does not require the use of a freeze drier or boiling methanol, and is therefore less hazardous, and more time and cost effective. The presented method has been shown to have comparable or improved glucosinolate extraction efficiency relative to the commonly used ISO method for major glucosinolates in the Brassicaceae species studied: sinigrin and gluconasturtiin in B. juncea; sinalbin, glucotropaeolin, and gluconasturtiin in S. alba; glucoraphenin and glucoraphasatin in R. sativus; and glucosatavin, glucoerucin and glucoraphanin in E. sativa.
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机译:背景:芥子油苷,一种富含阴离子硫的次生代谢产物,由于其在农业上具有重要意义的十字花科中的存在及其对人和动物健康的影响,因此已得到广泛研究。作为控制农业害虫的方法,对有毒的芥子油苷水解产物的生物熏蒸特性也越来越感兴趣。评估生物熏蒸潜力需要快速,准确地定量芥子油苷,但是在分析之前,当前常用的提取方法涉及许多耗时且危险的步骤。这项研究旨在开发一种改进的芥子油苷提取方法。结果:比较了以前在芸苔科组织中提取芥子油苷的三种方法,即在冷的甲醇中提取,在沸腾的甲醇中提取和在沸水中提取的三种方法,分别针对不同的组织类型(根,茎叶)和四种芸苔科物种(B. juncea,S (alba,R。sativus和E. sativa)。甲醇冷提取法的表现优于或优于所有其他测试的芥子油苷提取方法,但在葡萄球茎中的葡糖phasatin除外。还证明了在提取过程中通常使用的冻干方法可以破坏组织,可以降低最终的芥子油苷浓度,并且从冷冻的湿组织样品中以80%的冷甲醇进行提取更为有效。结论:我们提出了一种从植物组织中提取芥子油苷的简化方法,该方法不需要使用冷冻干燥器或沸腾的甲醇,因此危险性较小,且时间和成本效益更高。与所研究的十字花科植物中主要的芥子油苷的常用ISO方法相比,所提出的方法已显示出可比或提高的芥子油苷的提取效率。 S. alba中的sinalbin,糖原蛋白和葡萄糖基松香苷;莴苣中的糖皮质激素和糖皮质激素;和E. sativa中的葡糖胺,葡糖苷和葡聚糖。
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