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Single molecule mRNA fluorescent in situ hybridization combined with immunofluorescence in S. cerevisiae: Dataset and quantification

机译:酿酒酵母中的单分子mRNA荧光原位杂交与免疫荧光相结合:数据集和定量

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摘要

Single-molecule fluorescent in situ hybridization (smFISH) has emerged as a powerful technique that allows one to localize and quantify the absolute number of mRNAs in single cells. In combination with immunofluorescence (IF), smFISH can be used to correlate the expression of an mRNA and a protein of interest in single cells. Here, we provide and quantify an smFISH-IF dataset in We measured the expression of the cell cycle-controlled mRNA and the cell cycle marker alpha-tubulin. The smFISH-IF protocol describing the dataset generation is published in the accompanying article “Simultaneous detection of mRNA and protein in by single-molecule FISH and Immunofluorescence” . Here, we analyze the smFISH data using the freely available software FISH-quant . The provided datasets are intended to assist scientists interested in setting up smFISH-IF protocol in their laboratory. Furthermore, scientists interested in the generation of imaging analysis tools for single-cell approaches may find the provided dataset useful. To this end, we provide the differential interference contrast (DIC) channel, as well as multicolor, raw Z-stacks for smFISH, IF and DAPI.
机译:单分子荧光原位杂交(smFISH)已经成为一种强大的技术,它允许人们定位和量化单个细胞中mRNA的绝对数量。结合免疫荧光(IF),smFISH可用于关联单细胞中mRNA和目的蛋白的表达。在这里,我们提供并量化了smFISH-IF数据集中的数据。我们测量了细胞周期控制的mRNA和细胞周期标志物α-微管蛋白的表达。描述数据集生成的smFISH-IF方案发表在随附的文章“通过单分子FISH和免疫荧光同时检测mRNA和蛋白质”中。在这里,我们使用免费的软件FISH-quant分析smFISH数据。提供的数据集旨在帮助有兴趣在自己的实验室中建立smFISH-IF方案的科学家。此外,对生成用于单细胞方法的成像分析工具感兴趣的科学家可能会发现提供的数据集很有用。为此,我们提供了差分干涉对比(DIC)通道,以及用于smFISH,IF和DAPI的多色原始Z堆栈。

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