CTNS mRNA molecular analysis revealed a novel mutation in a child with infantile nephropathic cystinosis: a case report

Svetlana Papizh; Victoria Serzhanova; Alexandra Filatova; Mikhail Skoblov; Vyacheslav Tabakov; Lambert van den Heuvel; Elena Levtchenko; Larisa Prikhodina

doi:10.1186/s12882-019-1589-2

CTNS mRNA molecular analysis revealed a novel mutation in a child with infantile nephropathic cystinosis: a case report

BMC Nephrol. 2019 Oct 31;20(1):400. doi: 10.1186/s12882-019-1589-2.

Authors

Svetlana Papizh¹, Victoria Serzhanova², Alexandra Filatova², Mikhail Skoblov², Vyacheslav Tabakov², Lambert van den Heuvel³, Elena Levtchenko³, Larisa Prikhodina⁴

Affiliations

¹ Department of hereditary and acquired kidney diseases, Research and Clinical Institute for Pediatrics at the Pirogov Russian National Research Medical University, 125412, Taldomskaya st., 2, Moscow, Russia. papijsveta@mail.ru.
² Research Centre for Medical Genetics, 115522, Russia, Moscow.
³ Department of Pediatrics/Pediatric Nephrology, University Hospital Gasthuisberg, Leuven, Belgium.
⁴ Department of hereditary and acquired kidney diseases, Research and Clinical Institute for Pediatrics at the Pirogov Russian National Research Medical University, 125412, Taldomskaya st., 2, Moscow, Russia.

Abstract

Background: Cystinosis is an autosomal recessive lysosomal storage disorder characterized by accumulation of cystine in lysosomes throughout the body. Cystinosis is caused by mutations in the CTNS gene that encodes the lysosomal cystine carrier protein cystinosin. CTNS mutations result in either complete absence or reduced cystine transporting function of the protein. The diagnosis of nephropathic cystinosis is generally based on measuring leukocyte cystine level, demonstration of corneal cystine crystals by the slit lamp examination and confirmed by genetic analysis of the CTNS gene.

Case presentation: A boy born to consanguineous Caucasian parents had the characteristic clinical features of the infantile nephropathic cystinosis including renal Fanconi syndrome (polydipsia/polyuria, metabolic acidosis, hypokalemia, hypophosphatemia, low molecular weight proteinuria, glycosuria, cystine crystals in the cornea) and elevated WBC cystine levels. Initially we performed RFLP analysis of the common in the Northern European population 57-kb deletion of proband's DNA, then a direct Sanger sequencing which revealed no mutations in the coding part of the CTNS gene. To confirm the diagnosis we performed RT-PCR analysis of total RNA obtained from patient-derived fibroblasts in combination with cDNA sequencing. This revealed the skipping of exon 4 and exon 5 in the CTNS in our patient. Therefore, we detected a novel 9-kb homozygous deletion in the CTNS gene at genomic DNA level, spanning region from intron 3 to intron 5. In order to identify the inheritance pattern of the deletion we analyzed DNA of proband's mother and father. Both parents were found to be heterozygous carriers of the CTNS mutation.

Conclusions: Analysis of CTNS gene transcript allowed to identify a large homozygous deletion in the patient with infantile nephropathic cystinosis. Mutational detection at RNA level may be an efficient tool to establish the genetic defect in some cystinosis patients.

Keywords: CTNS; Fanconi syndrome; Nephropathic cystinosis; mRNA analysis.

Publication types

Case Reports

MeSH terms

Amino Acid Transport Systems, Neutral / genetics*
Child, Preschool
Consanguinity
Cysteamine / therapeutic use
Cystine Depleting Agents / therapeutic use
Cystinosis / drug therapy
Cystinosis / genetics*
Cystinosis / metabolism
DNA Mutational Analysis
Exons / genetics
Fibroblasts / chemistry
Humans
Infant
Introns / genetics
Male
Mutation*
RNA, Messenger / genetics
Real-Time Polymerase Chain Reaction

Substances

Amino Acid Transport Systems, Neutral
CTNS protein, human
Cystine Depleting Agents
RNA, Messenger
Cysteamine

Supplementary concepts

Cystinosis, Infantile Nephropathic