- 作者:L. Carraresi ; R. Parini ; C. Filoni ; A. Caciotti ; G. Sersale ; S. Tomatsu ; C. Orl ; o ; E. Zammarchi ; R. Guerrini ; M.A. Donati ; A. Morrone
- 关键词:Morquio A ; GALNS expression profiling ; Real-time RT-PCR
- 刊名:Clinica Chimica Acta
- 出版年:2008
- 出版时间:November 2008
- 年:2008
- 卷:397
- 期:1-2
- 页码:72-76
- 全文大小:343 K
BackgroundQuantification studies of mutated mRNAs have not been carried out on Morquio A patients. Such studies are very important for the determination of stability of premature termination codons (PTC) bearing transcripts in order to assess the appropriateness of introducing the newly developed therapeutic strategies such as “stop codon read-through therapy”.Methods
This paper focuses on the study of the GALNS gene and mRNAs in two severe forms of Morquio A patients' fibroblasts with development of a new and rapid real-time RT-PCR for detection and quantification of absolute mRNA copy number.
Results
We identified two new mutations c.385A > T (p.K129X) and c.899 − 1G > C) in Pt1 and a known splicing defect c.120 + 1G > A in Pt2. Using RT-PCR and real-time RT-PCR in Pt2 we detected low levels of mRNAs, suggesting its instability; in Pt1, we detected three aberrant mRNAs introducing premature stop codons, suggesting that both the c.385A > T and c.899 − 1G > C mutations produce mRNAs capable of escaping the nonsense-mediated decay (NMD) pathway.
Conclusions
The development of a real-time RT-PCR assay allows to absolutely quantify the GALNS mRNAs carrying mutations that lead to PTCs bearing transcripts, which escape the NMD process and are potentially suitable for the new therapeutic approach.