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Stable silencing of SNAP-25 in PC12 cells by RNA interference

机译:RNA干扰可稳定PC12细胞中SNAP-25的沉默

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摘要

BackgroundSNAP-25 is a synaptic protein known to be involved in exocytosis of synaptic vesicles in neurons and of large dense-core vesicles in neuroendocrine cells. Its role in exocytosis has been studied in SNAP-25 knockout mice, in lysed synaptosomes lacking functional SNAP-25 and in cells after treatment with botulinum toxins A or E that specifically cleave SNAP-25. These studies have shown that SNAP-25 appears to be required for most but not all evoked secretion. In order to further study the role of SNAP-25 in catecholamine secretion from PC12 cells we have used the recently developed technique of RNA interference to generate PC12 cell lines with virtually undetectable levels of SNAP-25. RNA interference is the sequence-specific silencing or knockdown of gene expression triggered by the introduction of double-stranded RNA into a cell. RNA interference can be elicited in mammalian cells in a number of ways, one of which is by the expression of small hairpin RNAs from a transfected plasmid. Selection of stably transfected cell lines expressing a small hairpin RNA allows one-time characterization of the degree and specificity of gene silencing and affords a continuing source of well-characterized knockdown cells for experimentation.
机译:背景技术SNAP-25是一种突触蛋白,已知与神经元中的突触小泡和神经内分泌细胞中的大密核小泡的胞吐作用有关。已在SNAP-25基因敲除小鼠中,在缺乏功能性SNAP-25的裂解突触小体中以及在用能特异性裂解SNAP-25的肉毒杆菌毒素A或E处理后的细胞中研究了其在胞吐作用中的作用。这些研究表明,SNAP-25似乎是大多数但不是全部诱发分泌所必需的。为了进一步研究SNAP-25在PC12细胞分泌儿茶酚胺中的作用,我们使用了最近开发的RNA干扰技术来生成SNAP-25水平几乎检测不到的PC12细胞系。 RNA干扰是通过将双链RNA引入细胞而触发的基因表达的序列特异性沉默或基因敲低。 RNA干扰可以通过多种方式在哺乳动物细胞中引起,其中一种方式是通过转染质粒中小发夹RNA的表达。选择表达小发夹RNA的稳定转染的细胞系,可以对基因沉默的程度和特异性进行一次性表征,并为实验提供了一个连续不断的特征丰富的基因敲除细胞。

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