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Extraction of DNA suitable for PCR applications from mature leaves of Mangifera indica L.

机译:从印度芒果的成熟叶片中提取适合PCR应用的DNA。

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摘要

Good quality deoxyribonucleic acid (DNA) is the pre-requisite for its downstream applications. The presence of high concentrations of polysaccharides, polyphenols, proteins, and other secondary metabolites in mango leaves poses problem in getting good quality DNA fit for polymerase chain reaction (PCR) applications. The problem is exacerbated when DNA is extracted from mature mango leaves. A reliable and modified protocol based on the cetyltrimethylammonium bromide (CTAB) method for DNA extraction from mature mango leaves is described here. High concentrations of inert salt were used to remove polysaccharides; Polyvinylpyrrolidone (PVP) and β-mercaptoethanol were employed to manage phenolic compounds. Extended chloroform-isoamyl alcohol treatment followed by RNase treatment yielded 950‒1050 µg of good quality DNA, free of protein and RNA. The problems of DNA degradation, contamination, and low yield due to irreversible binding of phenolic compounds and coprecipitation of polysaccharides with DNA were avoided by this method. The DNA isolated by the modified method showed good PCR amplification using simple sequence repeat (SSR) primers. This modified protocol can also be used to extract DNA from other woody plants having similar problems.
机译:高质量的脱氧核糖核酸(DNA)是其下游应用的先决条件。芒果叶中高浓度的多糖,多酚,蛋白质和其他次生代谢产物的存在为获得适合聚合酶链反应(PCR)应用的高质量DNA带来了问题。当从成熟的芒果叶中提取DNA时,这个问题更加严重。本文描述了一种基于十六烷基三甲基溴化铵(CTAB)方法的可靠且经过改进的方案,用于从成熟芒果叶中提取DNA。使用高浓度的惰性盐去除多糖;聚乙烯吡咯烷酮(PVP)和β-巯基乙醇用于管理酚类化合物。扩展的氯仿-异戊醇处理,再用RNase处理,可得到950×1050 µg高质量的DNA,不含蛋白质和RNA。该方法避免了由于酚类化合物不可逆结合以及多糖与DNA共沉淀而导致的DNA降解,污染和低收率的问题。通过改良方法分离的DNA使用简单序列重复(SSR)引物显示出良好的PCR扩增。此修改后的协议也可以用于从具有类似问题的其他木本植物中提取DNA。

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