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首页> 外文期刊>Journal of Virological Methods >A reliable and inexpensive method of nucleic acid extraction for the PCR-based detection of diverse plant pathogens
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A reliable and inexpensive method of nucleic acid extraction for the PCR-based detection of diverse plant pathogens

机译:一种可靠且廉价的核酸提取方法,用于基于PCR的多种植物病原体检测

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摘要

A reliable extraction method is described for the preparation of total nucleic acids from at least ten plant genera for subsequent detection of plant pathogens by PCR-based techniques. The method combined a modified CTAB (cetyltrimethylammonium bromide) extraction protocol with a semi-automatic homogenizer (FastPrep((R)) instrument) for rapid sample processing and low potential of cross contamination. The method was applied to sample preparation for PCR-based detection of 28 different RNA and DNA viruses, six viroids, two phytoplasmas and two bacterial pathogens from a range of infected host plants including sweet potato, small fruits and fruit trees. The procedure is cost-effective and the qualities of the nucleic acid preparations are comparable to those prepared by commonly used commercial kits. The efficiency of the procedure permits processing of numerous samples and the use of a single nucleic acid preparation for testing both RNA and DNA genomes by PCR, making this an appealing method for testing multiple pathogens in certification and quarantine programs.
机译:描述了一种可靠的提取方法,用于从至少十个植物属中制备总核酸,以便随后通过基于PCR的技术检测植物病原体。该方法将改进的CTAB(十六烷基三甲基溴化铵)萃取方案与半自动均质器(FastPrep(R)仪器)结合使用,可快速进行样品处理并降低交叉污染的可能性。该方法已应用于样品制备,以基于PCR的方式检测了一系列感染宿主植物(包括甘薯,小果和果树)中的28种不同的RNA和DNA病毒,6种类病毒,2种质原体和2种细菌病原体。该方法是成本有效的,并且核酸制剂的质量可与常用商业试剂盒制备的核酸相媲美。该过程的效率允许处理大量样品,并使用一种核酸制剂通过PCR测试RNA和DNA基因组,这使其成为一种在认证和检疫程序中测试多种病原体的有吸引力的方法。

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