| Literature DB >> 29459630 |
Shogo Minamikawa1, Kandai Nozu2, Yoshimi Nozu1, Tomohiko Yamamura1, Mariko Taniguchi-Ikeda1, Keita Nakanishi1, Junya Fujimura1, Tomoko Horinouchi1, Yuko Shima3, Koichi Nakanishi4, Masuji Hattori5, Kyoko Kanda6, Ryojiro Tanaka6, Naoya Morisada1, China Nagano1, Nana Sakakibara1, Hiroaki Nagase1, Ichiro Morioka1, Hiroshi Kaito1, Kazumoto Iijima1.
Abstract
The pattern of X-chromosome inactivation (XCI) can affect the clinical severity of X-linked disorders in females. XCI pattern analysis has been conducted mainly by HUMARA assay, a polymerase chain reaction-based assay using a methylation-sensitive restriction enzyme. However, this assay examines the XCI ratio of the androgen receptor gene at the genomic DNA level and does not reflect the ratio of either targeted gene directly or at the mRNA level. Here, we report four females with Dent disease, and we clarified the correlation between XCI and female cases of Dent disease using not only HUMARA assay but also a novel analytical method by RNA sequencing. We constructed genetic analysis for 4 female cases showing high level of urinary low-molecular-weight proteinuria and their parents. Their XCI pattern was analyzed by both HUMARA assay and an ultra-deep targeted RNA sequencing of the CLCN5 gene using genomic DNA and mRNA extracted from both leukocytes and urine sediment. All four cases possessed pathogenic variants of the CLCN5 gene. XCI analysis revealed skewed XCI in only two cases, while the other two showed random XCI. All assay results of HUMARA and targeted RNA sequencing in both leukocytes and urinary sediment were clearly identical in all four cases. We developed a novel XCI analytical assay of ultra-deep targeted RNA sequencing and revealed that skewed XCI explains the mechanism of onset of female Dent disease in only half of such cases.Entities:
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Year: 2018 PMID: 29459630 DOI: 10.1038/s10038-018-0415-1
Source DB: PubMed Journal: J Hum Genet ISSN: 1434-5161 Impact factor: 3.172