从原肠胚胚胎中分离的果蝇原代细胞培养及其在RNAi筛选中的应用。

Culture of Drosophila primary cells dissociated from gastrula embryos and their use in RNAi screening.

作者信息

Bai Jianwu, Sepp Katharine J, Perrimon Norbert

机构信息

Department of Genetics, Harvard Medical School, Boston, Massachusetts, USA.

出版信息

Nat Protoc. 2009;4(10):1502-12. doi: 10.1038/nprot.2009.147. Epub 2009 Sep 24.

DOI:10.1038/nprot.2009.147

PMID:19798083

Abstract

We provide a detailed protocol for the mass culturing of primary cells dissociated from Drosophila embryos. The advantage of this protocol over others is that we have optimized it for a robust large-scale performance that is suitable for screening. More importantly, we further present conditions to treat these cells with double stranded (ds) RNAs for gene knockdown. Efficient RNAi in Drosophila primary cells is accomplished by simply bathing the cells in dsRNA-containing culture medium. This method provides the basis for functional genomic screens in differentiated cells, such as neurons and muscles, using RNAi or small molecules. The entire protocol takes approximately 14 d, whereas the preparation of primary cells from Drosophila embryos only requires 2-4 h.

摘要

我们提供了一份详细的方案，用于大规模培养从果蝇胚胎中解离出来的原代细胞。该方案相对于其他方案的优势在于，我们已针对适用于筛选的强大大规模操作对其进行了优化。更重要的是，我们进一步给出了用双链（ds）RNA处理这些细胞以进行基因敲低的条件。在果蝇原代细胞中，通过简单地将细胞置于含有dsRNA的培养基中培养即可实现高效的RNA干扰。该方法为使用RNA干扰或小分子在分化细胞（如神经元和肌肉细胞）中进行功能基因组筛选提供了基础。整个方案大约需要14天，而从果蝇胚胎制备原代细胞仅需2 - 4小时。

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从原肠胚胚胎中分离的果蝇原代细胞培养及其在RNAi筛选中的应用。

Culture of Drosophila primary cells dissociated from gastrula embryos and their use in RNAi screening.

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