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Discrepancies in HLA typing by PCR-SSOP and SBT techniques: a case study.

机译:PCR-SSOP和SBT技术在HLA分型中的差异:一个案例研究。

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摘要

Six hundred twenty-one samples from Portugal, the Cabo Verde archipelago, and Guinea-Bissau were typed for HLA-A, HLA-B, and HLA-DRB1 using the polymerase chain reaction-sequence-specific oligonucleotide probe (PCR-SSOP) method and the sequence-based typing (SBT) method to characterize and compare discrepancies between the two methods. Fifty-three alleles (4.27% of 1242 chromosomes typed) identified by the PCR-SSOP method were not concordant with the results obtained using the SBT method. Thirty-four (2.74% of total chromosomes typed) PCR-SSOP mistyping results were discrepancies inside the same allele group and 19 others (1.53% of total chromosomes typed) were relative to nonconcordant results between different groups. PCR-SSOP allele mistyping is the result of interpretation difficulties resulting from less intense, absent, or dubious hybridization patterns. Noncommercial PCR-SSOP procedures are highly exigent on the technicians' experience and the availability of properly calibrated high-precision equipment.
机译:使用聚合酶链反应序列特异性寡核苷酸探针(PCR-SSOP)方法对葡萄牙,佛得角群岛和几内亚比绍的612个样品进行了HLA-A,HLA-B和HLA-DRB1的分型以及基于序列的键入(SBT)方法来表征和比较这两种方法之间的差异。通过PCR-SSOP方法鉴定的53个等位基因(占1242条染色体的4.27%)与使用SBT方法获得的结果不一致。 34个(占总染色体类型的2.74%)PCR-SSOP错译结果是同一等位基因组内部的差异,另外19个(占总染色体类型的1.53%)与不同组之间的非一致结果有关。 PCR-SSOP等位基因模糊是杂交强度降低,缺乏或不确定导致的解释困难的结果。非商业PCR-SSOP程序非常需要技术人员的经验以及正确校准的高精度设备的可用性。

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