Department of Physiology, Radboud Institute for Molecular Life Sciences, Radboud University Medical Center, Nijmegen, the Netherlands.
Reference Center for Hereditary Kidney and Childhood Diseases (Maladies Rénales Héréditaires de l'Enfant et de l'Adulte, MARHEA), Paris, France.
J Am Soc Nephrol. 2023 Feb 1;34(2):333-345. doi: 10.1681/ASN.2022050627. Epub 2022 Nov 9.
Gitelman syndrome is a salt-losing tubulopathy characterized by hypokalemic alkalosis and hypomagnesemia. It is caused by homozygous recessive or compound heterozygous pathogenic variants in SLC12A3 , which encodes the Na + -Cl - cotransporter (NCC). In up to 10% of patients with Gitelman syndrome, current genetic techniques detect only one specific pathogenic variant. This study aimed to identify a second pathogenic variant in introns, splice sites, or promoters to increase the diagnostic yield.
Long-read sequencing of SLC12A3 was performed in 67 DNA samples from individuals with suspected Gitelman syndrome in whom a single likely pathogenic or pathogenic variant was previously detected. In addition, we sequenced DNA samples from 28 individuals with one variant of uncertain significance or no candidate variant. Midigene splice assays assessed the pathogenicity of novel intronic variants.
A second likely pathogenic/pathogenic variant was identified in 45 (67%) patients. Those with two likely pathogenic/pathogenic variants had a more severe electrolyte phenotype than other patients. Of the 45 patients, 16 had intronic variants outside of canonic splice sites (nine variants, mostly deep intronic, six novel), whereas 29 patients had an exonic variant or canonic splice site variant. Midigene splice assays of the previously known c.1670-191C>T variant and intronic candidate variants demonstrated aberrant splicing patterns.
Intronic pathogenic variants explain an important part of the missing heritability in Gitelman syndrome. Long-read sequencing should be considered in diagnostic workflows for Gitelman syndrome.
Gitelman 综合征是一种盐丢失性肾小管病,其特征为低钾性碱中毒和低镁血症。它是由 SLC12A3 中的纯合隐性或复合杂合致病性变异引起的,该基因编码 Na+-Cl-共转运蛋白(NCC)。在多达 10%的 Gitelman 综合征患者中,目前的遗传技术仅检测到一种特定的致病性变异。本研究旨在鉴定内含子、剪接位点或启动子中的第二个致病性变异,以提高诊断率。
对 67 例疑似 Gitelman 综合征患者的 DNA 样本进行 SLC12A3 的长读测序,这些患者之前检测到一种单一的可能致病性或致病性变异。此外,我们还对 28 例具有一种意义不明的变异或无候选变异的个体进行了 DNA 样本测序。Midigene 剪接分析评估了新的内含子变异的致病性。
在 45 例(67%)患者中鉴定出第二种可能致病性/致病性变异。那些具有两种可能致病性/致病性变异的患者的电解质表型比其他患者更严重。在这 45 例患者中,有 16 例具有非经典剪接位点之外的内含子变异(9 个变异,主要是深内含子,6 个新变异),而 29 例患者具有外显子变异或经典剪接位点变异。先前已知的 c.1670-191C>T 变异和内含子候选变异的 Midigene 剪接分析显示出异常的剪接模式。
内含子致病性变异解释了 Gitelman 综合征中重要的遗传缺失部分。长读测序应考虑用于 Gitelman 综合征的诊断工作流程。
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