Princess Srisavangavadhana College of Medicine, Chulabhorn Royal Academy, Bangkok, Thailand.
Department of Molecular Tropical Medicine and Genetics, Faculty of Tropical Medicine, Mahidol University, Bangkok, Thailand.
PLoS One. 2023 Nov 15;18(11):e0294200. doi: 10.1371/journal.pone.0294200. eCollection 2023.
Glucose-6-phosphate dehydrogenase (G6PD) deficiency is an X-linked enzymopathy caused by mutations in the G6PD gene. A medical concern associated with G6PD deficiency is acute hemolytic anemia induced by certain foods, drugs, and infections. Although phenotypic tests can correctly identify hemizygous males, as well as homozygous and compound heterozygous females, heterozygous females with a wide range of G6PD activity may be misclassified as normal. This study aimed to develop multiplex high-resolution melting (HRM) analyses to enable the accurate detection of G6PD mutations, especially among females with heterozygous deficiency. Multiplex HRM assays were developed to detect six G6PD variants, i.e., G6PD Gaohe (c.95A>G), G6PD Chinese-4 (c.392G>T), G6PD Mahidol (c.487G>A), G6PD Viangchan (c.871G>A), G6PD Chinese-5 (c.1024C>T), and G6PD Union (c.1360C>T) in two reactions. The assays were validated and then applied to genotype G6PD mutations in 248 Thai females. The sensitivity of the HRM assays developed was 100% [95% confidence interval (CI): 94.40%-100%] with a specificity of 100% (95% CI: 88.78%-100%) for detecting these six mutations. The prevalence of G6PD deficiency was estimated as 3.63% (9/248) for G6PD deficiency and 31.05% (77/248) for intermediate deficiency by phenotypic assay. The developed HRM assays identified three participants with normal enzyme activity as heterozygous for G6PD Viangchan. Interestingly, a deletion in intron 5 nucleotide position 637/638 (c.486-34delT) was also detected by the developed HRM assays. G6PD genotyping revealed a total of 12 G6PD genotypes, with a high prevalence of intronic variants. Our results suggested that HRM analysis-based genotyping is a simple and reliable approach for detecting G6PD mutations, and could be used to prevent the misdiagnosis of heterozygous females by phenotypic assay. This study also sheds light on the possibility of overlooking intronic variants, which could affect G6PD expression and contribute to enzyme deficiency.
葡萄糖-6-磷酸脱氢酶(G6PD)缺乏症是一种由 G6PD 基因突变引起的 X 连锁酶病。与 G6PD 缺乏症相关的医学问题是某些食物、药物和感染引起的急性溶血性贫血。虽然表型测试可以正确识别半合子男性以及纯合子和复合杂合子女性,但 G6PD 活性广泛的杂合子女性可能被误诊为正常。本研究旨在开发多重高分辨率熔解(HRM)分析方法,以准确检测 G6PD 突变,特别是在杂合子缺乏的女性中。开发了多重 HRM 分析方法来检测六种 G6PD 变体,即 G6PD Gaohe(c.95A>G)、G6PD Chinese-4(c.392G>T)、G6PD Mahidol(c.487G>A)、G6PD Viangchan(c.871G>A)、G6PD Chinese-5(c.1024C>T)和 G6PD Union(c.1360C>T)在两个反应中。该分析方法经过验证后,用于检测 248 名泰国女性的 G6PD 基因突变。HRM 分析方法的灵敏度为 100%(95%置信区间:94.40%-100%),特异性为 100%(95%置信区间:88.78%-100%),用于检测这六种突变。表型检测估计 G6PD 缺乏症的患病率为 3.63%(9/248),中间缺乏症的患病率为 31.05%(77/248)。开发的 HRM 分析方法确定了三个具有正常酶活性的参与者为 G6PD Viangchan 的杂合子。有趣的是,还通过开发的 HRM 分析方法检测到内含子 5 核苷酸位置 637/638(c.486-34delT)的缺失。G6PD 基因分型共发现 12 种 G6PD 基因型,内含子变异的发生率很高。我们的结果表明,基于 HRM 分析的基因分型是一种简单可靠的检测 G6PD 突变的方法,可以防止表型检测误诊杂合子女性。本研究还表明,可能会忽略影响 G6PD 表达并导致酶缺乏的内含子变异。
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