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Allelic Imbalance in TOR1A mRNA Expression in Manifesting and Non-Manifesting Carriers of the GAG-Deletion

机译:GAG缺失表现载体和非表现载体中TOR1A mRNA表达的等位基因失衡

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Early onset dystonia (EOD) is associated with a 3bp-(ΔGAG) in-frame deletion in the TOR1A gene, which encodes for torsinA. Carriers of the mutant (ΔGAG) allele can either develop or escape a dystonic phenotype (~30% penetrance). The expression ratio of the two alleles could be important for the manifestation or prevention of the disease since wild-type (WT) torsinA is thought to have protective function. Absence of an antibody discriminating WT from ΔE torsinA has precluded the determination ΔE and WT torsinA levels in manifesting and nonmanifesting carriers. We performed quantitative analysis of TOR1A allele expression in manifesting (MC) and nonmanifesting (NMC) carriers using quantitative allele-specific PCR (qASPCR) to determine the levels of mutant versus WT torsinA mRNA. The technique described showed high degree of specificity in detecting the two alleles. The present study represents the first comprehensive analysis of biallelic expression of the TOR1A gene in lymphoblast and brain samples from patients and NMC relatives. We demonstrate that mRNA is transcribed from both the WT and ΔGAG allele in peripheral and neural tissues with a trend for increased expression of the ΔGAG allele compared to the WT in carriers regardless of their phenotype and thus cannot account for the reduced penetrance.
机译:早期发作的肌张力障碍(EOD)与TOR1A基因的3bp-(ΔGAG)读框内缺失相关,该基因编码TorsinA。突变体(ΔGAG)等位基因的携带者可以发展或摆脱张力障碍表型(〜30%渗透率)。这两个等位基因的表达比例可能对疾病的表现或预防很重要,因为人们认为野生型(WT)都灵A具有保护功能。缺少将WT与ΔE躯干蛋白A区分开的抗体,排除了在表现载体和非表现载体中确定ΔE和WT躯干A的水平。我们使用定量等位基因特异性PCR(qASPCR)对表达载体(MC)和非显性载体(NMC)进行了TOR1A等位基因表达的定量分析,以确定突变体与野生型torsinA mRNA的水平。所述技术在检测两个等位基因方面显示出高度的特异性。本研究代表了来自患者和NMC亲属的淋巴母细胞和脑样本中TOR1A基因双等位基因表达的首次全面分析。我们证明mRNA是从WT和ΔGAG等位基因在周围和神经组织中转录而来的,与携带者中的WT相比,无论其表型如何,ΔGAG等位基因的表达都有增加的趋势,因此不能解释降低的渗透率。

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