| Literature DB >> 33627970 |
Yuanyuan Jiang1,2, Jiangrong Peng2, Yunpeng Cao3, Zhiqiang Han3, Ling Zhang2, Wenbing Su2, Shunquan Lin2, Yuan Yuan1,2, Bin Wang1, Xianghui Yang2, Zhike Zhang2.
Abstract
As tools of plant molecular biology, fluorescence microscopy and Nicotiana benthamiana have been used frequently to study the structure and function of plant cells. However, it is difficult to obtain ideal micrographs; for example, the images are typically unclear, the inner cell structure cannot be observed under a high-power lens by fluorescence microscopy, etc. Here, we describe a method for observing the cell structure of N. benthamiana. This method significantly improves imaging by fluorescence microscopy and allows clear images to be obtained under a high-power lens. This method is easy to perform with good stability, and the stomatal structure, nucleus, nucleolus, chloroplast and other organelles in N. benthamiana cells as well as protein localizations and the locations of protein-protein interactions have been observed clearly. Furthermore, compared with traditional methods, fluorescent dye more efficiently dyes cells with this method. The applicability of this method was verified by performing confocal scanning laser microscopy (CSLM), and CSLM imaging was greatly improved. Thus, our results provided a method to visualize the subcellular structures of live cells in the leaves of N. benthamiana by greatly improving imaging under a fluorescence microscope and provided new insights and references for the study of cell structures and functions in other plants. SUPPLEMENTARY INFORMATION: The online version contains supplementary material available at 10.1007/s12298-021-00931-5. © Prof. H.S. Srivastava Foundation for Science and Society 2021.Entities:
Keywords: Bimolecular fluorescence complementation (BiFC); Fluorescence microscopy; Method; Staining; Tobacco
Year: 2021 PMID: 33627970 PMCID: PMC7873200 DOI: 10.1007/s12298-021-00931-5
Source DB: PubMed Journal: Physiol Mol Biol Plants ISSN: 0974-0430