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Development and initial characterization of a HAPPY panel for mapping the X. Tropicalis genome

机译:HAPPY面板的开发和初步表征,用于定位热带假单胞菌基因组

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HAPPY mapping was designed to pursue the analysis of approximately random HAPloid DNA breakage samples using the PolYmerase chain reaction for mapping genomes. In the present study, we improved the method and integrated two other molecular techniques into the process: whole genome amplification and the Sequenom SNP (single nucleotide polymor-phism) genotyping assay in order to facilitate whole genome mapping of X. tropicalis. The former technique amplified enough DNA materials to genotype a large number of markers, while the latter allowed for relatively high throughput marker genotyping with multiplex assays on the HAPPY lines. A total of 58 X. tropicalis genes were genotyped on an initial panel of 383 HAPPY lines, which contributed to formation of a working panel of 146 lines. Further genotyping of 29 markers on the working panel led to construction of a HAPPY map for the X. tropicalis genome. We believe that our improved HAPPY method described in the present study has paved the way for the community to map different genomes with a simple, but powerful approach.
机译:HAPPY作图旨在利用PolYmerase链反应对基因组作图,以分析大约随机的HAPloid DNA断裂样品。在本研究中,我们改进了该方法,并将其他两种分子技术整合到了过程中:全基因组扩增和Sequenom SNP(单核苷酸多态性)基因分型测定法,以促进热带热带假单胞菌的全基因组作图。前一种技术扩增了足够的DNA材料以对大量标记进行基因分型,而后一种技术则允许通过HAPPY品系上的多重检测进行相对高通量的标记基因分型。在383个HAPPY品系的初始面板上对58个热带热带假单胞菌基因进行了基因分型,这有助于形成146个品系的工作面板。在工作面板上对29个标记进行进一步的基因分型,导致构建了热带假单胞菌基因组的HAPPY图。我们相信,本研究中描述的改进的HAPPY方法为社区使用简单但功能强大的方法绘制不同基因组图谱铺平了道路。

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