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首页> 外文期刊>Acta Histochemica: Zeitschrift fur Histologische Topochemie >Improved cryosections and specific immunohistochemical methods for detecting hypoxia in mouse and rat cochleae.
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Improved cryosections and specific immunohistochemical methods for detecting hypoxia in mouse and rat cochleae.

机译:改进的冰冻切片和特异性免疫组织化学方法,可检测小鼠和大鼠耳蜗缺氧。

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The present study was undertaken to develop an improved cryoembedding method for analysis of mice and rat cochleae, which permits high-quality cryosections and preserves overall structure and cellular resolution as shown by hematoxylin/eosin staining. The preservation of morphology and antigenicity is mandatory to achieve optimal results. A total of 20 male cd/1 mice and 14 male Sprague-Dawley rats were used in experiments for optimization of preservation, fixative, decalcification, embedding and cryosectioning of cochleae from adult and aged rodents. In addition, a novel immunohistochemical procedure (using Hydroxyprobe-1 kit) was developed for detecting regions of hypoxia in mice and rat cochlea. This method employs a primary fluorescent-conjugated monoclonal antibody directed against pimonidazole protein adducts that are created in hypoxic tissues. Subsequent studies of hypoxia inducible factor-1alpha (HIF-1alpha) by immunofluorescence in the cochlea of these animals were performed in order to confirm that immunochemical detection of pimonidazole protein is representative of a hypoxic environment. We conclude that the present method results in high-quality cryosections of cochlear tissues presenting good anatomical and histological preservation. Furthermore, our optimized procedures provide novel tools for the investigation of neuro-sensory-epithelium in physio-pathological situations associated with hypoxia and/or ischemia, such as inner ear development, plasticity, regeneration and senescence.
机译:进行本研究是为了开发一种改进的冷冻嵌入方法,用于分析小鼠和大鼠的耳蜗,该方法可进行高质量的冷冻切片,并保留苏木精/曙红染色所显示的整体结构和细胞分辨率。必须保持形态和抗原性才能获得最佳结果。实验共使用20只雄性cd / 1小鼠和14只雄性Sprague-Dawley大鼠进行实验,以优化成年和老年啮齿动物耳蜗的保存,固定,脱钙,包埋和冷冻切片。此外,开发了一种新的免疫组织化学方法(使用Hydroxyprobe-1试剂盒)来检测小鼠和大鼠耳蜗中的缺氧区域。该方法采用针对在缺氧组织中产生的吡莫尼唑蛋白加合物的荧光偶联初级单克隆抗体。随后通过免疫荧光在这些动物的耳蜗中进行了缺氧诱导因子-1α(HIF-1alpha)的研究,以确认吡莫尼唑蛋白的免疫化学检测代表了低氧环境。我们得出的结论是,本方法导致高质量的耳蜗组织冰冻切片,呈现出良好的解剖学和组织学保存。此外,我们的优化程序为研究与缺氧和/或缺血(例如内耳发育,可塑性,再生和衰老)相关的生理病理情况下的神经感觉上皮提供了新颖的工具。

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