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Minisequencing on oligonucleotide microarrays: comparison of immobilisation chemistries

机译:寡核苷酸的微量测序 芯片:固定化化学的比较

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摘要

In the microarray format of the minisequencing method multiple oligonucleotide primers immobilised on a glass surface are extended with fluorescent ddNTPs using a DNA polymerase. The method is a promising tool for large-scale single nucleotide polymorphism (SNP) detection. We have compared eight chemical methods for covalent immobilisation of the oligonucleotide primers on glass surfaces. We included both commercially available, activated slides and slides that were modified by ourselves. In the comparison the differently derivatised glass slides were evaluated with respect to background fluorescence, efficiency of attaching oligonucleotides and performance of the primer arrays in minisequencing reactions. We found that there are significant differences in background fluorescence levels among the different coatings, and that the attachment efficiency, which was measured indirectly using extension by terminal transferase, varied largely depending on which immobilisation strategy was used. We also found that the attachment chemistry affects the genotyping accuracy, when minisequencing on microarrays is used as the genotyping method. The best genotyping results were observed using mercaptosilane-coated slides attaching disulfide-modified oligonucleotides.
机译:在微测序方法的微阵列格式中,使用DNA聚合酶用荧光ddNTP扩展固定在玻璃表面的多个寡核苷酸引物。该方法是用于大规模单核苷酸多态性(SNP)检测的有前途的工具。我们比较了八种化学方法将寡核苷酸引物共价固定在玻璃表面上。我们既包括市售的激活幻灯片,也包括我们自己修改的幻灯片。在比较中,就背景荧光,连接寡核苷酸的效率以及微测序反应中引物阵列的性能,对不同衍生化的载玻片进行了评估。我们发现不同涂层之间的背景荧光水平存在显着差异,并且使用末端转移酶的延伸间接测量的附着效率在很大程度上取决于所使用的固定化策略。我们还发现,当使用微阵列上的微测序作为基因分型方法时,附着化学会影响基因分型的准确性。 使用巯基硅烷涂布的载玻片观察到最佳的基因分型结果 连接二硫键修饰的寡核苷酸。

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