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Prospects of endosperm DNA in maize seed characterization

机译:胚乳DNA在玉米种子鉴定中的应用前景。

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DNA based characterisation of maize germplasm has become the easiest and fastest approach to identify genetic diversity as compared to phenotyping. The conventional DNA source for genotyping is the leaf which required at least 2 weeks waiting period from seed planting to leaves sampling. This work exploits the use of endosperm DNA (EDNA) for the genotyping of maize germplasm. Maize endosperm was excised from maize seeds using pliers, ground and used for Genomic DNA extraction (gDNA). Leaves DNA (LDNA) was also extracted concurrently. The extracted LDNA and EDNA were quantified and subjected to SSR-PCR. The mean concentrations of DNA extracted were 1575 ng/ul for the leaves and 526 ng/ul for endosperm. Though the difference in quantity of EDNA and LDNA were highly significant, the quality (A260/A280) for both EDNA and LDNA fall within 1.6-1.8 range of pure DNA index. SSR-PCR products using phi032 were similar for both EDNA and LDNA, indicating the usability of EDNA in genotyping. This seed based method of gDNA extraction takes less than 24 hours from sampling to quantification and genotyping. It also allows germination of sampled seeds, selection before planting, avoids the delay of planting and waiting in leaf sampling and saves field space.
机译:与表型分析相比,基于DNA的玉米种质表征已成为鉴定遗传多样性的最简单,最快的方法。用于基因分型的常规DNA来源是叶子,从种子种植到叶子采样至少需要2周的等待时间。这项工作利用了胚乳DNA(EDNA)进行玉米种质基因分型。使用钳子从玉米种子中切下玉米胚乳,研磨后用于基因组DNA提取(gDNA)。还同时提取了叶片DNA(LDNA)。对提取的LDNA和EDNA进行定量,并进行SSR-PCR。叶片提取的DNA平均浓度为1575 ng / ul,胚乳为526 ng / ul。尽管EDNA和LDNA的数量差异非常显着,但EDNA和LDNA的质量(A260 / A280)都在纯DNA指数的1.6-1.8范围内。使用phi032的SSR-PCR产物的EDNA和LDNA相似,表明EDNA在基因分型中的可用性。从采样到定量和基因分型,这种基于种子的gDNA提取方法只需不到24小时。它还可以使取样的种子发芽,在播种前进行选择,避免播种延迟和叶片采样等待,并节省了田间空间。

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