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Auxin analysis using laser microdissected plant tissues sections

机译:使用激光显微切割的植物组织切片进行生长素分析

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Quantitative measurement of actual auxin levels in plant tissue is complimentary to molecular methods measuring the expression of auxin related genes. Current analytical methods to quantify auxin have pushed the limit of detection to where auxin can be routinely quantified at the pictogram (pg) level, reducing the amount of tissue needed to perform these kinds of studies to amounts never imagined a few years ago. In parallel, the development of technologies like laser microdissection microscopy (LMD) has allowed specific cells to be harvested from discrete tissues without including adjacent cells. This method has gained popularity in recent years, especially for enabling a higher degree of spatial resolution in transcriptome profiling. As with other quantitative measurements, including hormone quantifications, sampling using traditional LMD is still challenging because sample preparation clearly compromises the preservation of analytes. Thus, we have developed and validated a sample preparation protocol combining cryosectioning, freeze-drying, and capturing with a laser microdissection microscope to provide high-quality and well-preserved plant materials suitable for ultrasensitive, spatially-resolved auxin quantification. We developed a new method to provide discrete plant tissues for indole-3-acetic acid (IAA) quantification while preserving the plant tissue in the best possible condition to prevent auxin degradation. The method combines the use of cryosectioning, freeze-drying and LMD. The protocol may also be used for other applications that require small molecule analysis with high tissue-specificity where degradation of biological compounds may be an issue. It was possible to collect the equivalent to 15?mg of very specific tissue in approximately 4?h using LMD. We have shown, by proof of concept, that freeze dried cryosections of plant tissue were suitable for LMD harvest and quantification of the phytohormone auxin using GC-MS/MS. We expect that the ability to resolve auxin levels with both spatial- and temporal resolution with high accuracy will enable experiments on complex processes, which will increase our knowledge of the many roles of auxins (and, in time, other phytohormones) in plant development.
机译:定量测量植物组织中实际植物生长素的水平与测量植物生长素相关基因表达的分子方法相辅相成。当前定量植物生长素的分析方法将检测极限推到了可以在象形图(pg)级别常规定量植物生长素的水平,从而将进行此类研究所需的组织数量减少到几年前无法想象的数量。同时,诸如激光显微切割显微镜(LMD)之类的技术发展已允许从不连续的组织中收获特定的细胞,而无需包括相邻的细胞。近年来,这种方法获得了普及,尤其是在转录组分析中实现更高程度的空间分辨率方面。与其他定量测量(包括激素定量)一样,使用传统LMD进行采样仍然具有挑战性,因为样品制备明显损害了分析物的保存。因此,我们开发并验证了将冷冻切片,冷冻干燥和激光显微解剖显微镜相结合的样品前处理方案,以提供适用于超灵敏,空间分辨的生长素定量的高质量且保存完好的植物材料。我们开发了一种新方法,可为离散的植物组织提供吲哚-3-乙酸(IAA)定量,同时将植物组织保存在最佳状态以防止生长素降解。该方法结合了冷冻切片,冷冻干燥和LMD的使用。该协议还可以用于需要对小分子进行高组织特异性分析的其他应用,其中生物化合物的降解可能是一个问题。使用LMD可以在大约4?h内收集相当于15?mg非常特殊的组织的信息。通过概念证明,我们已经证明植物组织的冷冻干燥冷冻切片适用于LMD收获和使用GC-MS / MS定量植物激素生长素。我们希望能够以高精度的时空分辨率解析生长素水平,从而能够进行复杂过程的实验,这将增加我们对生长素(以及其他植物激素)在植物发育中的许多作用的认识。

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