Functional analysis of two SLC9A6 frameshift variants in lymphoblastoid cells from patients with Christianson syndrome

Hailan He; Huiwen Zhang; Hui Chen; Fang He; Fei Yin; Tobias Stauber; Xiaomin Zou; Jing Peng

doi:10.1111/cns.14329

Functional analysis of two SLC9A6 frameshift variants in lymphoblastoid cells from patients with Christianson syndrome

CNS Neurosci Ther. 2023 Dec;29(12):4059-4069. doi: 10.1111/cns.14329. Epub 2023 Jun 28.

Authors

Hailan He^{1

2}, Huiwen Zhang³, Hui Chen⁴, Fang He^{1

2}, Fei Yin^{1

2}, Tobias Stauber⁵, Xiaomin Zou^{1

2}, Jing Peng^{1

2}

Affiliations

¹ Department of Pediatrics, Xiangya Hospital, Central South University, Changsha, China.
² Hunan Intellectual and Developmental Disabilities Research Center, Changsha, China.
³ Department of Pediatric Endocrinology and Genetic Metabolism, Xinhua Hospital, Shanghai Institute for Pediatric Research, Shanghai Jiao Tong University School of Medicine, Shanghai, China.
⁴ Department of Neurology, Jiangxi Provincial Children's Hospital, Nanchang, China.
⁵ Department of Human Medicine and Institute for Molecular Medicine, MSH Medical School Hamburg, Hamburg, Germany.

Abstract

Background: Christianson syndrome (CS) is caused by mutations in SLC9A6 and is characterized by global developmental delay, epilepsy, hyperkinesis, ataxia, microcephaly, and behavioral disorder. However, the molecular mechanism by which these SLC9A6 mutations cause CS in humans is not entirely understood, and there is no objective method to determine the pathogenicity of single SLC9A6 variants.

Methods: Trio-based whole exome sequencing (WES) was carried out on two individuals with suspicion of CS. qRT-PCR, western blot analysis, filipin staining, lysosomal enzymatic assays, and electron microscopy examination, using EBV-LCLs established from the two patients, were performed.

Results: Trio-based WES identified a hemizygous SLC9A6 c.1560dupT, p.T521Yfs*23 variant in proband 1 and a hemizygous SLC9A6 c.608delA, p.H203Lfs*10 variant in proband 2. Both children exhibited typical phenotypes associated with CS. Expression analysis in EBV-LCLs derived from the two patients showed a significant decrease in mRNA levels and no detectable normal NHE6 protein. EBV-LCLs showed a statistically significant increase in unesterified cholesterol in patient 1, but only non-significant increase in patient 2 when stained with filipin. Activities of lysosomal enzymes (β-hexosaminidase A, β-hexosaminidase A + B, β-galactosidase, galactocerebrosidase, arylsulfatase A) of EBV-LCLs did not significantly differ between the two patients and six controls. Importantly, by electron microscopy we detected an accumulation of lamellated membrane structures, deformed mitochondria, and lipid droplets in the patients' EBV-LCLs.

Conclusions: The SLC9A6 p.T521Yfs*23 and p.H203Lfs*10 variants in our patients result in loss of NHE6. Alterations of mitochondria and lipid metabolism may play a role in the pathogenesis of CS. Moreover, the combination of filipin staining with electron microscopy examination of patient lymphoblastoid cells can serve as a useful complementary diagnostic method for CS.

Keywords: SLC9A6; Christianson syndrome; NHE6; lipid; lymphoblastoid cells; mitochondria.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Ataxia / genetics
Child
Epilepsy* / genetics
Filipin
Humans
Microcephaly* / genetics
Microcephaly* / pathology
beta-N-Acetylhexosaminidases

Functional analysis of two SLC9A6 frameshift variants in lymphoblastoid cells from patients with Christianson syndrome

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