RNA sequencing reveals a complete picture of a homozygous missense variant in a patient with VPS13D movement disorder: a case report and review of the literature

Elizabeth K Baker; Jingfen Han; William A Langley; Michael A Reott Jr; Barbara E Hallinan; Robert J Hopkin; Wenying Zhang

doi:10.1007/s00438-023-02044-y

RNA sequencing reveals a complete picture of a homozygous missense variant in a patient with VPS13D movement disorder: a case report and review of the literature

Mol Genet Genomics. 2023 Sep;298(5):1185-1199. doi: 10.1007/s00438-023-02044-y. Epub 2023 Jun 20.

Authors

Elizabeth K Baker^{1

2}, Jingfen Han¹, William A Langley³, Michael A Reott Jr³, Barbara E Hallinan^{2

4}, Robert J Hopkin^{1

2}, Wenying Zhang^{5

6}

Affiliations

¹ Division of Human Genetics, Cincinnati Children's Hospital Medical Center, 3333 Burnet Avenue, ML7016, Cincinnati, OH, 45229, USA.
² Department of Pediatrics, University of Cincinnati College of Medicine, Cincinnati, OH, USA.
³ MNG Laboratories, a Labcorp Company, Atlanta, GA, USA.
⁴ Division of Neurology, Cincinnati Children's Hospital Medicine, Cincinnati, OH, USA.
⁵ Division of Human Genetics, Cincinnati Children's Hospital Medical Center, 3333 Burnet Avenue, ML7016, Cincinnati, OH, 45229, USA. wenying.zhang@cchmc.org.
⁶ Department of Pediatrics, University of Cincinnati College of Medicine, Cincinnati, OH, USA. wenying.zhang@cchmc.org.

PMID: 37340120
DOI: 10.1007/s00438-023-02044-y

Abstract

RNA sequencing (RNA-seq) is a complementary diagnostic tool to exome sequencing (ES), only recently clinically available to undiagnosed patients post-ES, that provides functional information on variants of unknown significance (VUS) by evaluating its effect on RNA transcription. ES became clinically available in the early 2010s and promised an agnostic platform for patients with a neurological disease, especially for those who believed to have a genetic etiology. However, the massive data generated by ES pose challenges in variant interpretation, especially for rare missense, synonymous, and deep intronic variants that may have a splicing effect. Without functional study and/or family segregation analysis, these rare variants would be likely interpreted as VUS which is difficult for clinicians to use in clinical care. Clinicians are able to assess the VUS for phenotypic overlap, but this additional information alone is usually not enough to re-classify a variant. Here, we report a case of a 14-month-old male who presented to clinic with a history of seizures, nystagmus, cerebral palsy, oral aversion, global developmental delay, and poor weight gain requiring gastric tube placement. ES revealed a previously unreported homozygous missense VUS, c.7406A > G p.(Asn2469Ser), in VPS13D. This variant has not been previously reported in genome aggregation database (gnomAD), ClinVar, or in any peer-reviewed published literature. By RNA-seq, we demonstrated that this variant mainly impacts splicing and results in a frameshift and early termination. It is expected to generate either a truncated protein, p.(Val2468fs*19), or no protein from this transcript due to nonsense-mediated mRNA decay leading to VPS13D deficiency. To our knowledge, this is the first case utilizing RNA-seq to further functionally characterize a homozygous novel missense VUS in VPS13D and confirm its impact on splicing. This confirmed pathogenicity gave the diagnosis of VPS13D movement disorder to this patient. Therefore, clinicians should consider utilizing RNA-seq to clarify VUS by evaluating its effect on RNA transcription.

Keywords: Missense; Movement disorder; RNA sequencing; VPS13D; Variant of unknown significance.

Publication types

Review
Case Reports

MeSH terms

Exome Sequencing
Humans
Infant
Male
Movement Disorders*
Mutation
Proteins
RNA*
Sequence Analysis, RNA

Substances

RNA
VPS13D protein, human
Proteins