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Microsatellite Enrichment by Magnetic Beads in Chrysanthemum

机译:Chrysanthemum磁珠的微卫星富集

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Chrysanthemum (Chrysanthemum morifolium), originating from China, is an important ornamental, edible, tea and medicine plant, but now there is still a lack of knowledge about its genetic and molecular backgrounds.The objectives of this study were to set up an efficient protocol to isolate microsatellite and screen SSR (Simple sequence repeat) primers for chrysanthemum DNA fingerprint development.Genomic DNAs of chrysanthemum were cleaved with Mse I, fragments of 250-1500 bp DNA were recovered, then added with adapters, and amplified by PCR later.The 300-1500 bp DNA fractions containing microsatellite sequences were captured by hybridizing the digested genomic DNA fragments with the oligo nucleotide probes (CT)15 or (TGA)8 attached to streptavidin-coated magnetic beads (Dynal) respectively.The enriched DNA fragments were ligated into pGEM-T Easy vector and then transformed into Escherichia coli Top10 competent cells to form two enriched microsatellite sequence libraries.144 and 118 microsatellite clones were obtained from the two libraries respectively with PCR identification of microsatellite arrays (PIMA), further 91 and 92 microsateilite sequences were obtained respectively by sequencing analysis.Eighty-eight microsatellite sequences can be used to design primers.According to the 88 microsatellite sequences 142 primer pairs were designed.23 SSR primer pairs with high polymorphism were obtained by primary screening.
机译:来自中国的菊花(菊花)是一种重要的装饰,食用,茶和药品植物,但现在仍然缺乏关于其遗传和分子背景的知识。本研究的目的是建立一个有效的协议用于隔离微卫星和筛网SSR(简单序列重复)菊花DNA指纹开发的引物。用MSE I切割菊花的甘蓝颗粒组,回收250-1500bp DNA的片段,然后用适应剂加入并通过PCR扩增。通过将消化的基因组DNA片段与附着于链霉蛋白涂覆的磁珠(染子)的寡核苷酸探针(CT)15或(TGA)8杂交,捕获含有微卫星序列的300-1500bp DNA级分。富集的DNA片段连接进入PGEM-T易于载体,然后转化为大肠杆菌TOP10主管细胞以形成两种富集的微卫星序列文库.144和118 MICR从两种文库中获得替代素克隆,分别通过PCR鉴定进行微卫星阵列(PIMA),另外通过测序分析获得91和92微盐素序列。可以使用Igighty-8微卫星序列来设计引物。根据88微卫星序列设计了142个引物对,通过初级筛选获得具有高多态性的SSR引物对。

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