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Isolation of Lineage Specific Nuclei Based on Distinct Endoreduplication Levels and Tissue-Specific Markers to Study Chromatin Accessibility Landscapes

机译:基于不同的末端综合水平和组织特异性标记的基于谱系特异性核的分离以研究染色蛋白可接近性景观

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摘要

The capacity for achieving immense specificity and resolution in science increases day to day. Fluorescence-activated nuclear sorting (FANS) offers this great precision, enabling one to count and separate distinct types of nuclei from specific cells of heterogeneous mixtures. We developed a workflow to collect nuclei from Arabidopsis thaliana by FANS according to cell lineage and endopolyploidy level with high efficiency. We sorted GFP-labeled nuclei with different ploidy levels from the epidermal tissue layer of three-day, dark-grown hypocotyls followed by a shift to light for one day and compared them to plants left in the dark. We then accessed early chromatin accessibility patterns associated with skotomorphogenesis and photomorphogenesis by the assay for transposase-accessible chromatin using sequencing (ATAC-seq) within primarily stomatal 2C and fully endoreduplicated 16C nuclei. Our quantitative analysis shows that dark- and light-treated samples in 2C nuclei do not exhibit any different chromatin accessibility landscapes, whereas changes in 16C can be linked to transcriptional changes involved in light response.
机译:在科学中实现巨大特异性和决议的能力会增加日期。荧光激活的核分选(风扇)提供了这种极大的精度,使得能够从异质混合物的特定细胞中计算和分离不同类型的核。我们开发了一个工作流程,根据细胞谱系和内支链倍性水平,球迷从拟南芥拟南芥中收集核。我们将GFP标记的核与三天的表皮组织层分类为不同的倍性水平,然后将乳头基的表皮组织层随后换光,并将它们与植物留在黑暗中。然后,通过主要气孔2C和完全结合的16C核在主要气孔2C和完全结合的16C核中,通过测定用于转座酶可接近的染色质的测定,进入与慢磷酸卟啉和光致血管发生相关的早期染色质染色质。我们的定量分析表明,2C核中的深色和光处理样品不会表现出任何不同的染色质可接近性景观,而16C的变化可以与光反应中所涉及的转录变化相关联。

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