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A Large-Scale Whole-Mount in situ Hybridization System: Rapid One-Tube Preparation of DIG-Labeled RNA Probes and High Throughput Hybridization using 96-Well Silent Screen Plates

机译:大规模的全安装原位杂交系统:快速一管制备DIG标签的RNA探针和使用96孔静音筛选板的高通量杂交

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摘要

Recent progress in multiple and automated-sequencing technology allows large-scale random cDNA sequencing, the so-called EST project, in various fields. In addition to the EST collection, the cDNA project requires analysis of spatiotemporal patterns of gene expression of a large number of clones by whole-mount in situ hybridization (WISH). To facilitate the multiple WISH procedures, we developed a protocol for rapid and uniform synthesis of multiple probes and multi-well based WISH processing. A DIG-labeled RNA probe for WISH was synthesized from a PCR-amplified template which contained an RNA promoter. All reactions of PCR and subsequent RNA synthesis were performed in a single tube by sequential addition of the reagents without phenol extraction or ethanol precipitation steps. An RNA probe was purified and condensed by a centrifugal ultrafilter to achieve high and stable purification efficiency. WISH of 96 samples were performed simultaneously in a 96-well plate attached to silent screen filters that were connected with a vacuum exhausting system. These processes eliminated the labor-intensive steps of WISH and provided opportunities to search for novel genes.
机译:多重和自动测序技术的最新进展允许在各个领域进行大规模的随机cDNA测序,即所谓的EST项目。除EST收集外,cDNA项目还需要通过整装原位杂交(WISH)分析大量克隆的基因表达的时空模式。为了促进多种WISH程序,我们开发了一种协议,用于快速均匀地合成多个探针和基于多孔的WISH处理。由含有RNA启动子的PCR扩增模板合成了用于WISH的DIG标记的RNA探针。 PCR的所有反应和随后的RNA合成均通过依次添加试剂而在单个试管中进行,无需酚提取或乙醇沉淀步骤。 RNA探针通过离心超滤器进行纯化和浓缩,以实现高且稳定的纯化效率。在连接至与真空抽气系统相连的无声滤网的96孔板上同时进行96个样品的WISH检测。这些过程消除了WISH的劳动密集型步骤,并提供了寻找新基因的机会。

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