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A gene-specific primer extension and liquid bead array system for killer-cell immunoglobulin-like receptor genotyping.

机译:基因特异性引物延伸和液珠阵列系统用于杀伤细胞免疫球蛋白样受体基因分型。

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摘要

A simple and accurate method for killer-cell immunoglobulin-like receptor (KIR) genotyping is developed using KIR gene-specific primer extension (GSPE) followed by bead array hybridization (GSPE method). After amplification of exons 4, 5, and 9, KIR GSPE and bead array hybridization were performed to verify the presence or absence of 16 KIR subfamilies. GSPE method was validated with natural killer/KIR reference panel I consisting of 48 cell types provided by 13th International Histocompatibility Working Group (IHWG) and genomic DNA from 17 peripheral blood cells, 8 cell lines, and 8 buccal cells. The results of reference panel from GSPE method were 100% concordant with the IHWG reference typing information. All genomic DNAs except reference panel were typed for KIR genes with sequence-specific primer methods and showed 100% identical typing results using this novel system. In addition, GSPE method can obtain results in 8 h from DNA with 10 ng genomic DNA in a 96-well-based assay format.
机译:使用KIR基因特异性引物延伸(GSPE),然后进行磁珠阵列杂交(GSPE方法),开发了一种简单而准确的杀伤细胞免疫球蛋白样受体(KIR)基因分型方法。外显子4、5和9扩增后,进行KIR GSPE和珠阵列杂交以验证是否存在16个KIR亚家族。 GSPE方法已由第13国际组织相容性工作组(IHWG)提供的48种细胞类型以及来自17个外周血细胞,8个细胞系和8个颊细胞的基因组DNA组成的自然杀手/ KIR参考组I进行了验证。 GSPE方法的参考小组的结果与IHWG参考打字信息100%一致。除参考面板外,所有基因组DNA均使用序列特异性引物方法对KIR基因进行分型,并使用该新型系统显示出100%相同的分型结果。此外,GSPE方法可在基于96孔测定的形式中,从具有10 ng基因组DNA的DNA在8小时内获得结果。

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