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首页> 外文期刊>Journal of Neurochemistry: Offical Journal of the International Society for Neurochemistry >Alternative splicing in single cells dissected from complex tissues: separate expression of prepro-tachykinin A mRNA splice variants in sensory neurones.
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Alternative splicing in single cells dissected from complex tissues: separate expression of prepro-tachykinin A mRNA splice variants in sensory neurones.

机译:从复杂组织解剖的单细胞中的选择性剪接:速激肽原A mRNA剪接变体在感觉神经元中的独立表达。

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摘要

Tachykinins play an important role in peripheral inflammatory diseases and disorders of the CNS. Most members of the tachykinin family are generated by alternative post-transcriptional splicing of the prepro-tachykinin (PPT) A gene. Here, we examined the simultaneous expression of PPT-A splice variants in individual neurones of the nodose ganglion. In extracts of ganglia, the expression of the four PPT-A mRNA splice variants and their four encoded peptides was shown by RT-PCR and combined HPLC and radioimmunoassay respectively. In order to examine prepro-tachykinin A expression in individual cells, single neurones were isolated from the ganglia using laser-assisted microdissection and processed for RT-PCR. Some 31.9% of the neurones investigated expressed a specific PPT-A transcript. Each individual neurone was found to express only a single splice variant. This is the first study to analyse the differential expression of PPT-A splice variants at the single-cell level. In view of the large number of alternatively spliced genes in the human genome and the resulting profound physiological effects, including several diseases, the technique described here is useful for isolating cells without possible confounding effects of dissociated neuronal cultures. For PPT-A, the results indicate that alternative post-transcriptional splicing determines the tachykinergic phenotype and may therefore have important functional implications.
机译:速激肽在外周炎症性疾病和中枢神经系统疾病中起重要作用。速激肽家族的大多数成员是由速激肽原(PPT)A前基因的选择性转录后剪接产生的。在这里,我们检查了结节神经节的单个神经元中PPT-A剪接变体的同时表达。在神经节的提取物中,通过RT-PCR,结合HPLC和放射免疫分析分别显示了四个PPT-A mRNA剪接变体及其四个编码的肽的表达。为了检查速激肽原A在单个细胞中的表达,使用激光辅助显微解剖从神经节中分离出单个神经元,并进行RT-PCR处理。约31.9%的神经元表达了特定的PPT-A转录本。发现每个神经元仅表达单个剪接变体。这是第一项在单细胞水平分析PPT-A剪接变体差异表达的研究。鉴于人类基因组中大量剪接的基因以及由此产生的深刻的生理效应,包括多种疾病,此处描述的技术可用于分离细胞,而不会混淆分离的神经元培养物的作用。对于PPT-A,结果表明替代的转录后剪接决定了速激肽的表型,因此可能具有重要的功能含义。

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