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非同位素原位杂交法检测塑料包埋组织中的鸡Sox基因mRNA

Non-isotopic in situ hybridization to detect chick Sox gene mRNA in plastic-embedded tissue.

作者信息

Church R J, Hand N M, Rex M, Scotting P J

机构信息

Division of Pathology, Clinical Laboratory Sciences, University Hospital, Queen's Medical Centre, Nottingham, UK.

出版信息

Histochem J. 1997 Aug;29(8):625-9. doi: 10.1023/a:1026440412830.

Abstract

In situ hybridization techniques have rapidly become widely used by the molecular biologist for the localization of specific nucleic acid sequences in individual cells or tissues. We describe the demonstration of Sox gene mRNA in chick tissue that has been embedded in the plastic methyl methacrylate to permit the preparation of sections for high-resolution light microscopy. Polymerization of the plastic was induced by using either N,N-dimethylaniline or N,N-3,5-tetramethylaniline. The in situ hybridization technique used was non-isotopic and used a digoxigenin-labelled probe detected with an antibody bound to alkaline phosphatase, which was then localized using X-phosphate-Nitro BT as a substrate-chromogen mix. Various pretreatments of the tissue sections were investigated, including the use of proteinase K, and heat-mediated techniques using a microwave oven and a pressure cooker. The best results were produced using pressure cooking on tissue in which the plastic had been chemically polymerized with N,N-3,5-tetramethylaniline. For the demonstration of Sox 11, this combination had a critical influence on the staining results, but for Sox 21 all protocols used produced good staining.

摘要

原位杂交技术已迅速被分子生物学家广泛用于在单个细胞或组织中定位特定核酸序列。我们描述了在嵌入塑料甲基丙烯酸甲酯中的鸡组织中Sox基因mRNA的显示,以便制备用于高分辨率光学显微镜检查的切片。使用N,N-二甲基苯胺或N,N-3,5-四甲基苯胺诱导塑料聚合。所使用的原位杂交技术是非同位素的,使用地高辛标记的探针,该探针用与碱性磷酸酶结合的抗体检测,然后使用X-磷酸盐-硝基蓝四唑作为底物-显色剂混合物进行定位。研究了组织切片的各种预处理,包括使用蛋白酶K以及使用微波炉和高压锅的热介导技术。在使用N,N-3,5-四甲基苯胺进行化学聚合的塑料组织上进行压力烹饪可产生最佳结果。对于Sox 11的显示,这种组合对染色结果有至关重要的影响,但对于Sox 21,所有使用的方案都产生了良好的染色效果。

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