Characterization of two novel intronic OPA1 mutations resulting in aberrant pre-mRNA splicing

Background We report two novel splice region mutations in OPA1 in two unrelated families presenting with autosomal-dominant optic atrophy type 1 (ADOA1) (ADOA or Kjer type optic atrophy). Mutations in OPA1 encoding a mitochondrial inner membrane protein are a major cause of ADOA. Methods We analyzed...

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Vydáno v:BMC medical genetics Ročník 18; číslo 1; s. 22
Hlavní autoři: Bolognini, Ramona, Gerth-Kahlert, Christina, Abegg, Mathias, Bartholdi, Deborah, Mathis, Nicolas, Sturm, Veit, Gallati, Sabina, Schaller, André
Médium: Journal Article
Jazyk:angličtina
Vydáno: London BioMed Central 28.02.2017
Témata:
Atrophy
Base Sequence
Biomedical and Life Sciences
Biomedicine
Blindness
Clinical-Molecular Genetics and Cytogenetics
Cytogenetics
DNA - chemistry
DNA - isolation & purification
DNA - metabolism
DNA Mutational Analysis
Exons
Families & family life
Gene Function
Genetic testing
GTP Phosphohydrolases - genetics
Heterozygote
Human Genetics
Humans
INDEL Mutation
Introns
Mitochondrial DNA
Mutation
Optic Atrophy, Autosomal Dominant - genetics
Optics
Parents & parenting
Patients
Pedigree
Proteins
Research Article
Retina - diagnostic imaging
RNA Precursors - genetics
RNA Precursors - metabolism
RNA Splicing
Tomography
Tomography, Optical Coherence
Visual acuity
Visual impairment
Optic neuropathies
Splice site mutation
Autosomal dominant optic atrophy
OPA1
Kjer type optic atrophy
ISSN:1471-2350, 1471-2350
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Shrnutí:Background We report two novel splice region mutations in OPA1 in two unrelated families presenting with autosomal-dominant optic atrophy type 1 (ADOA1) (ADOA or Kjer type optic atrophy). Mutations in OPA1 encoding a mitochondrial inner membrane protein are a major cause of ADOA. Methods We analyzed two unrelated families including four affected individuals clinically suspicious of ADOA. Standard ocular examinations were performed in affected individuals of both families. All coding exons, as well as exon-intron boundaries of the OPA1 gene were sequenced. In addition, multiplex ligation-dependent probe amplification (MLPA) was performed to uncover copy number variations in OPA1 . mRNA processing was monitored using RT-PCR and subsequent cDNA analysis. Results We report two novel splice region mutations in OPA1 in two unrelated individuals and their affected relatives, which were previously not described in the literature. In one family the heterozygous insertion and deletion c.[611-37_611-38insACTGGAGAATGTAAAGGGCTTT;611-6_611-16delCATATTTATCT] was found in all investigated family members leading to the activation of an intronic cryptic splice site. In the second family sequencing of OPA1 disclosed a de novo heterozygous deletion c.2012+4_2012+7delAGTA resulting in exon 18 and 19 skipping, which was not detected in healthy family members. Conclusion We identified two novel intronic mutations in OPA1 affecting the correct OPA1 pre-mRNA splicing, which was confirmed by OPA1 cDNA analysis. This study shows the importance of transcript analysis to determine the consequences of unclear intronic mutations in OPA1 in proximity to the intron-exon boundaries.
Bibliografie:ObjectType-Article-1
SourceType-Scholarly Journals-1
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ISSN:1471-2350
1471-2350
DOI:10.1186/s12881-017-0383-x