Bleckmann Andrea, Dresselhaus Thomas
Cell Biology and Plant Biochemistry, Biochemie-Zentrum Regensburg, University of Regensburg, Universitätsstrasse 31, 93053 Regensburg, Germany.
Methods. 2016 Apr 1;98:66-73. doi: 10.1016/j.ymeth.2015.10.019. Epub 2015 Oct 30.
First evidence on gene function and regulation is provided by the cellular expression pattern in complex tissues. However, to understand the activity of a specific gene, it is essential to analyze the regulatory network, which controls the spatio-temporal translation pattern during the entire life span of the transcribed mRNA. To explore mechanisms which control mRNA abundance and localization in space and time, it is necessary to visualize mRNAs quantitatively with a subcellular resolution, without sectioning the tissues. We have adapted and optimized a protocol for colorimetric whole-mount RNA in situ hybridization (WISH) using egg cell-specific digoxigenin (DIG) labeled probes (Hejátko et al., 2006) [1] on ovules and early seeds of Arabidopsis. Furthermore, we established a fluorescent whole-mount RNA in situ hybridization (F-WISH) protocol, which allows mRNA visualization on a subcellular level. The polar localized mRNA of SBT4.13, encoding a subtilase, was identified using this protocol. Both methods are described and discussed in detail. Additionally a (F)-WISH flow-chart is provided along with a troubleshooting table.
复杂组织中的细胞表达模式提供了关于基因功能和调控的首个证据。然而,要了解特定基因的活性,分析调控网络至关重要,该网络控制着转录mRNA整个生命周期中的时空翻译模式。为了探究控制mRNA丰度以及在空间和时间上定位的机制,有必要在不切片组织的情况下,以亚细胞分辨率对mRNA进行定量可视化。我们采用并优化了一种比色全组织RNA原位杂交(WISH)方案,该方案使用卵细胞特异性地高辛配基(DIG)标记探针(Hejátko等人,2006年)[1],用于拟南芥胚珠和早期种子。此外,我们建立了一种荧光全组织RNA原位杂交(F-WISH)方案,该方案能够在亚细胞水平上实现mRNA的可视化。利用该方案鉴定出了编码枯草杆菌蛋白酶的SBT4.13的极性定位mRNA。对这两种方法都进行了详细描述和讨论。此外,还提供了一个(F)-WISH流程图以及一个故障排除表。
Zotero 插件