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Improved RNA preservation for immunolabeling and laser microdissection.

机译:改进的RNA保存,用于免疫标记和激光显微切割。

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摘要

Microdissection techniques have the potential to allow for transcriptome analyses in specific populations of cells that are isolated from heterogeneous tissues such as the nervous system and certain cancers. Problematically, RNA is not stable under the labeling conditions usually needed to identify the cells of interest for microdissection. We have developed an immunolabeling method that utilizes a high salt buffer to stabilize RNA during prolonged antibody incubations. We first assessed RNA integrity by three methods and found that tissue incubated in high salt buffer for at least 20 h yielded RNA of similar quality to that for RNA extracted from fresh-frozen tissue, which is considered highest quality. Notably, the integrity was superior to that for RNA extracted from tissue processed using rapid immunolabeling procedures (5 min total duration). We next established that high salt buffer was compatible with immunolabeling, as demonstrated by immunofluorescent detection of dopamine neurons in the brain. Finally, we laser microdissected dopamine neurons that were immunolabeled using high salt buffer and demonstrated that RNA integrity was preserved. Our described method yields high quality RNA from immunolabeled microdissected cells, an essential requirement for meaningful genomics investigations of normal and pathological cells isolated from complex tissues.
机译:显微解剖技术具有潜力,可以对从异质组织(例如神经系统和某些癌症)中分离出的特定细胞群进行转录组分析。问题在于,RNA在通常需要识别显微切割目的细胞的标记条件下不稳定。我们已经开发了一种免疫标记方法,可以在长时间的抗体孵育过程中利用高盐缓冲液来稳定RNA。我们首先通过三种方法评估RNA的完整性,发现在高盐缓冲液中孵育至少20 h的组织产生的质量与从新鲜冷冻组织提取的RNA相似的质量(被认为是最高质量)。值得注意的是,其完整性优于使用快速免疫标记程序(总持续时间5分钟)从处理过的组织中提取的RNA。接下来,我们确定了高盐缓冲液与免疫标记兼容,如脑中多巴胺神经元的免疫荧光检测所证明的。最后,我们激光显微切割了使用高盐缓冲液进行免疫标记的多巴胺神经元,并证明保留了RNA完整性。我们描述的方法从免疫标记的显微解剖细胞中产生高质量的RNA,这是对从复杂组织中分离的正常细胞和病理细胞进行有意义的基因组学研究的基本要求。

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  • 来源
    《RNA》 |2009年第12期|共11页
  • 作者

    Brown AL; Smith DW;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 核酸;
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