Laboratory of Clinical Investigation, National Institute on Aging, Baltimore, Maryland.
J Mol Diagn. 2013 Nov;15(6):745-53. doi: 10.1016/j.jmoldx.2013.06.001. Epub 2013 Sep 23.
Congenital adrenal hyperplasia, due to 21-hydroxylase deficiency (21-OHD) is an autosomal recessive disorder of adrenal steroidogenesis caused by mutations in the CYP21A2 gene. Direct comparison of established and novel methodologies of CYP21A2 genetic analysis in a large cohort representing a wide range of genotypes has not been previously reported. We genotyped a cohort of 129 unrelated patients with 21-OHD, along with 145 available parents, using Southern blot (SB) analysis, multiplex ligation-dependent probe amplification (MLPA), PCR-based restriction fragment length polymorphism (RFLP) analysis, multiplex minisequencing and conversion-specific PCR, duplication-specific amplification, and DNA sequencing. CYP21A2 genotyping identified four duplicated CYP21A2 genes (1.53%) and 79 chimeric CYP21A1P/CYP21A2 genes (30.15%). Parental SB data were essential for determining the CYP21 haplotype in three cases, whereas PCR-based RFLP analysis was necessary for MLPA results to be accurately interpreted in the majority of cases. The comparison of different methods in detecting deletion and duplication showed that MLPA with PCR-based RFLP was comparable with SB analysis, with parental data of 100% sensitivity and specificity. DNA sequencing was required for the identification of 16 (6.1%) rare point mutations and determination of clinically significant chimera junction sites. MLPA with PCR-based RFLP analysis is an excellent substitute for SB analysis in detecting CYP21A2 deletion and duplication and a combination of MLPA, PCR-based RFLP, duplication-specific amplification, and DNA sequencing is a convenient and comprehensive strategy for mutation analysis of the CYP21A2 gene in patients with 21-OHD.
先天性肾上腺皮质增生症,由于 21-羟化酶缺乏症(21-OHD)是一种常染色体隐性遗传性肾上腺类固醇生物合成障碍,由 CYP21A2 基因突变引起。以前没有报道过对代表广泛基因型的大样本队列中已建立和新方法的 CYP21A2 基因分析进行直接比较。我们使用 Southern 印迹(SB)分析、多重连接依赖性探针扩增(MLPA)、基于 PCR 的限制性片段长度多态性(RFLP)分析、多重 mini 测序和转换特异性 PCR、特异性扩增和 DNA 测序对 129 例 21-OHD 无关患者和 145 例可利用父母进行了 CYP21A2 基因分型。CYP21A2 基因分型确定了 4 个重复 CYP21A2 基因(1.53%)和 79 个嵌合 CYP21A1P/CYP21A2 基因(30.15%)。在三种情况下,父母的 SB 数据对于确定 CYP21 单倍型至关重要,而在大多数情况下,PCR 基于 RFLP 分析对于准确解释 MLPA 结果是必要的。不同方法检测缺失和重复的比较表明,MLPA 与基于 PCR 的 RFLP 与 SB 分析相当,具有 100%的敏感性和特异性的父母数据。DNA 测序对于鉴定 16 个(6.1%)罕见点突变和确定临床上重要的嵌合连接位点是必需的。MLPA 与基于 PCR 的 RFLP 分析是检测 CYP21A2 缺失和重复的 SB 分析的极好替代品,并且 MLPA、基于 PCR 的 RFLP、特异性扩增和 DNA 测序的组合是 21-OHD 患者 CYP21A2 基因突变分析的一种方便和综合的策略。