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使用来自存档DNA的人工限制性片段长度多态性PCR对DR3和DR4进行HLA分型。

HLA typing for DR3 and DR4 using artificial restriction fragment length polymorphism PCR from archival DNA.

作者信息

Horton V A, Bunce M, Davies D R, Turner R C, Lo Y M

机构信息

Diabetes Research Laboratories, Radcliffe Infirmary, Oxford.

出版信息

J Clin Pathol. 1995 Jan;48(1):33-6. doi: 10.1136/jcp.48.1.33.

Abstract

AIM

To develop polymerase chain reaction based artificial restriction fragment length polymorphism (artificial RFLP PCR) assays for DR3 and DR4 alleles of the multiallelic DRB1 locus and to apply them to paraffin wax embedded archival material.

METHODS

Sixty five samples from DRB1 typed cell lines were analysed using the artificial RFLP PCR method to determine the specificity and sensitivity of the system.

RESULTS

The artificial RFLP PCR method for typing the DRB1 locus showed 100% accuracy in the 65 samples previously typed using allele specific PCR and serology. The samples included 18 combinations of alleles that included DR3, 18 that included DR4, four that were DR3/DR4 heterozygotes, and 10 samples that were neither DR3 nor DR4. Typing of 10 paraffin wax embedded samples using artificial RFLP PCR was in complete agreement with previous typing at the DRB1 locus.

CONCLUSION

The application of artificial RFLP PCR for the analysis of multiallelic loci, such as those of the HLA system, in archival DNA samples has been achieved. Artificial RFLP PCR is a robust, easily implemented, non-isotopic system and may be useful for large retrospective studies.

摘要

目的

开发基于聚合酶链反应的多等位基因DRB1位点DR3和DR4等位基因的人工限制性片段长度多态性(人工RFLP PCR)检测方法,并将其应用于石蜡包埋的存档材料。

方法

使用人工RFLP PCR方法分析65个DRB1分型细胞系样本,以确定该系统的特异性和敏感性。

结果

用于DRB1位点分型的人工RFLP PCR方法在先前使用等位基因特异性PCR和血清学分型的65个样本中显示出100%的准确性。这些样本包括18种包含DR3的等位基因组合、18种包含DR4的等位基因组合、4种DR3/DR4杂合子以及10个既非DR3也非DR4的样本。使用人工RFLP PCR对10个石蜡包埋样本进行分型,与先前DRB1位点的分型完全一致。

结论

已实现将人工RFLP PCR应用于存档DNA样本中多等位基因位点(如HLA系统的位点)的分析。人工RFLP PCR是一种稳健、易于实施的非同位素系统,可能对大型回顾性研究有用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f57f/502258/3c4a17cfa0b8/jclinpath00226-0039-a.jpg

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