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Suitable transfection methods for single particle tracing in plant suspension cells

机译:用于在植物悬浮细胞中追踪单颗粒的合适转染方法

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Background A multitude of different imaging systems are already available to image genetically altered RNA species; however, only a few of these techniques are actually suitable to visualize endogenous RNA. One possibility is to use fluorescently-labelled and hybridization-sensitive probes. In order to yield more information about the exact localization and movement of a single RNA molecule, it is necessary to image such probes with highly sensitive microscope setups. More challenges arise if such experiments are conducted in plant cells due to their high autofluorescence and demanding transfection procedures. Results Here, we report in planta imaging of single RNA molecules using fluorescently labeled molecular beacons. We tested three different transfection protocols in order to identify optimal conditions for transfection of fluorescent DNA probes and their subsequent detection at the single molecule level. Conclusions We found that an optimized heat shock protocol provided a vastly improved transfection method for small DNA molecules which were used for subsequent single RNA molecule detection in living plant suspension cells.
机译:背景技术已经有许多不同的成像系统可以对遗传改变的RNA种类进行成像。但是,这些技术中只有少数实际上适合可视化内源RNA。一种可能性是使用荧光标记的杂交敏感探针。为了获得有关单个RNA分子确切定位和运动的更多信息,有必要使用高度灵敏的显微镜设置对此类探针成像。如果在植物细胞中进行此类实验,则由于其较高的自发荧光和高要求的转染程序,将带来更多挑战。结果在这里,我们报道了使用荧光标记的分子信标在单个RNA分子的植物成像中。我们测试了三种不同的转染方案,以鉴定荧光DNA探针转染的最佳条件及其在单分子水平的后续检测。结论我们发现优化的热休克方案为小DNA分子提供了大大改进的转染方法,该DNA分子可用于随后在活植物悬浮细胞中检测单个RNA分子。

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