Qualitative and quantitative analysis of FBN1 mRNA from 16 patients with Marfan Syndrome

Qualitative and quantitative analysis of FBN1 mRNA from 16 patients with Marfan Syndrome

Pathogenic mutations in FBN1, encoding the glycoprotein, fibrillin-1, cause Marfan syndrome (MFS) and related connective tissue disorders. In the present study, qualitative and quantitative effects of 16 mutations, identified in FBN1 in MFS patients with systematically described phenotypes, were inv...

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Veröffentlicht in:BMC medical genetics 2015-12, Vol.16 (1), p.113-113, Article 113
Hauptverfasser: Tjeldhorn, Lena, Amundsen, Silja Svanstrøm, Barøy, Tuva, Rand-Hendriksen, Svend, Geiran, Odd, Frengen, Eirik, Paus, Benedicte
Format: Artikel
Sprache:eng
Schlagworte:
Base Sequence
Cells, Cultured
Connective tissue
Diagnosis
DNA Mutational Analysis
Epidermal growth factor
Fibrillin-1
Fibrillins
Fibroblasts
Fibroblasts - metabolism
Gene mutations
Genetic aspects
Genetic Predisposition to Disease - genetics
Genotype
Humans
Marfan syndrome
Marfan Syndrome - genetics
Marfan Syndrome - metabolism
Marfan Syndrome - pathology
Microfilament Proteins - genetics
Mutation
Mutation, Missense
Pathogenesis
Physiological aspects
Proteins
Reverse Transcriptase Polymerase Chain Reaction
Risk factors
RNA Splice Sites - genetics
RNA Splicing - genetics
RNA, Messenger - genetics
RNA, Messenger - metabolism
Sequence Deletion
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Zusammenfassung:Pathogenic mutations in FBN1, encoding the glycoprotein, fibrillin-1, cause Marfan syndrome (MFS) and related connective tissue disorders. In the present study, qualitative and quantitative effects of 16 mutations, identified in FBN1 in MFS patients with systematically described phenotypes, were investigated in vitro. Qualitative analysis was performed with reverse transcription-PCR (RT-PCR) and gel electrophoresis, and quantitative analysis to determine the FBN1 mRNA levels in fibroblasts from the 16 patients with MFS was performed with real-time PCR. Qualitative analysis documented that the mutations c.4817-2delA and c.A4925G led to aberrant FBN1 mRNA splicing leading to in frame deletion of exon 39 and in exon 39, respectively. No difference in the mean FBN1 mRNA level was observed between the entire group of cases and controls, nor between the group of patients with missense mutations and controls. The mean expression levels associated with premature termination codon (PTC) and splice site mutations were significantly lower than the levels in patients with missense mutations. A high level of FBN1 mRNA in the patient with the missense mutation c.G2447T did not segregate with the mutation in three of his first degree relatives. No association was indicated between the FBN1 transcript level and specific phenotypic manifestations. Abnormal FBN1 transcripts were indicated in fibroblasts from patients with the splice site mutation c.4817-2delA and the missense mutation c.A4925G. While the mean FBN1 mRNA expression level in fibroblasts from patients with splice site and PTC mutations were lower than the mean level in patients with missense mutations and controls, inter-individual variability was high. The observation that high level of FBN1 mRNA in the patient with the missense mutation c.G2447T did not segregate with the mutation in the family suggests that variable expression of the normal FBN1 allele may contribute to explain the variability in FBN1 mRNA level.
ISSN:1471-2350
1471-2350
DOI:10.1186/s12881-015-0260-4