Maceda Agustín, Andrés-Hernández Agustina Rosa, Terrazas Teresa
Universidad Nacional Autónoma de México, Instituto de Biología, Departamento de Botánica, Apdo. postal 70-367, 04510 Coyoacán, Cd. Mx., Mexico.
Benemérita Universidad Autónoma de Puebla, Blvd. Val-sequillo y Av. San Claudio, Edificio 112-A, Ciudad Universitaria, Col. Jardines de San Manuel, 72570 Puebla, Puebla, Mexico.
MethodsX. 2024 Oct 10;13:102999. doi: 10.1016/j.mex.2024.102999. eCollection 2024 Dec.
The protocol shows the effectiveness of using safranin-fast green stain for fluorescence microscopy. This staining technique has been used in conventional microscopy to perform anatomical characterizations of plants. However, this protocol describes the procedure for using samples stained with safranin-fast green in conjunction with fluorescence microscopy. The strength of the protocol lies in the fact that the samples are permanent and allows for effective differentiation of lignified and cellulosic walls unlike conventional fluorescence microscopy stains such as Congo red-acridine orange, calcofluor, and autofluorescence. The protocol for making fluorescence intensity measurements is also standardized, allowing the data to be used for statistical analysis and inference about the chemical composition of plant cell walls.
该方案展示了使用番红-固绿染色进行荧光显微镜观察的有效性。这种染色技术已在传统显微镜中用于对植物进行解剖学特征描述。然而,本方案描述了使用经番红-固绿染色的样本结合荧光显微镜的操作步骤。该方案的优势在于样本是永久性的,并且与刚果红-吖啶橙、荧光增白剂和自发荧光等传统荧光显微镜染色不同,它能有效区分木质化壁和纤维素壁。进行荧光强度测量的方案也是标准化的,这使得数据可用于统计分析以及对植物细胞壁化学成分的推断。
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