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A simplified method for combined immunohistochemistry and in-situ hybridization in fresh-frozen, cryocut mouse brain sections.

机译:一种在新鲜冷冻的冷冻小鼠大脑切片中结合免疫组织化学和原位杂交的简化方法。

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摘要

A method is described to perform combined immunohistochemistry and in situ hybridization in mouse brain sections. The protocol is specific to sections mounted on glass slides. In contrast to earlier methods that require either paraffin embedding or perfusion of the brain with paraformaldehyde, this protocol can be carried out on fresh-frozen, cryostat cut post-fixed sections. This simple and concise protocol increases the applicability of the technique as the RNAse-free immunodetection of antigen is useful by itself for immunologically identifying specific cells of interest and then examining gene expression in those cells using techniques such as real-time PCR and microarray analysis. The use of fresh-frozen, cryocut sections enables reliable detection of easily perturbable post-translational modifications such as phosphorylation and improves the quality of results obtained in subsequent in situ hybridization by reducing the background signal and interference from lower cell layers. Inducible transgenic mice that express either a dominant negative mutant form of the cAMP response element binding protein (mCREB) or CREB, in discrete brain regions, were used in this study. The combined immunohistochemistry and in situ hybridization protocol was used to examine colocalization of enkephalin or dynorphin mRNA, both downstream targets of CREB-mediated gene expression, in cells expressing transgenic mCREB or CREB.
机译:描述了一种在小鼠脑切片中进行免疫组织化学和原位杂交相结合的方法。该协议特定于安装在载玻片上的部分。与需要石蜡包埋或用多聚甲醛灌注大脑的早期方法相比,该方案可以在新鲜冷冻,低温恒温器切割后的固定切片上进行。这个简单而简明的方案增加了该技术的适用性,因为抗原的无RNAse免疫检测本身可用于免疫学鉴定感兴趣的特定细胞,然后使用实时PCR和微阵列分析等技术检查这些细胞中的基因表达。使用新鲜冷冻的切片可以可靠地检测易扰动的翻译后修饰,例如磷酸化,并通过减少背景信号和来自较低细胞层的干扰来提高后续原位杂交获得的结果的质量。在这项研究中使用了可诱导的转基因小鼠,该小鼠在离散的大脑区域表达cAMP反应元件结合蛋白(mCREB)或CREB的显性负突变形式。组合的免疫组织化学和原位杂交方案用于检查在表达转基因mCREB或CREB的细胞中脑啡肽或强啡肽mRNA的共定位,这两个都是CREB介导的基因表达的下游靶标。

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