Epigenomic, cistromic, and transcriptomic profiling of primary kidney tubular cells

Zhiheng Liu, Lirong Zhang, Yupeng Chen
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Abstract

Spatiotemporal regulation of gene expression is essential for maintaining cellular homeostasis throughout kidney development and disease progression. Transcription factors (TFs) and epigenetic modifications play pivotal roles in controlling gene expression. Profiling chromatin modifications across the genome, along with the distribution and target regulation by TFs in specific kidney cell types, is crucial for understanding the dynamic changes in gene expression. Here, we presented a comprehensive workflow for epigenomic, cistromic, and transcriptomic analyses of primary kidney tubular cells. Specifically, our methodologies included the isolation of primary kidney tubular epithelial cells, RNA extraction, assay for transposase-accessible chromatin using sequencing, ultra-low-input micrococcal nuclease-based native chromatin immunoprecipitation, cleavage under targets and release using nuclease, and subsequent bioinformatic analysis. This protocol provides a methodological framework for investigating the roles of TFs and epigenetic modifications in kidney development and diseases.
原代肾小管细胞表观基因组、表观组和转录组特征分析
基因表达的时空调控对于在肾脏发育和疾病进展过程中维持细胞平衡至关重要。转录因子(TFs)和表观遗传修饰在控制基因表达方面发挥着关键作用。剖析整个基因组的染色质修饰以及转录因子在特定肾细胞类型中的分布和靶标调控,对于了解基因表达的动态变化至关重要。在这里,我们介绍了一种对原代肾小管细胞进行表观基因组学、表观组学和转录组学分析的综合工作流程。具体来说,我们的方法包括分离原代肾小管上皮细胞、提取 RNA、使用测序法测定转座酶可进入的染色质、超低投入微球核酸酶为基础的原生染色质免疫沉淀、在靶标下裂解和使用核酸酶释放,以及随后的生物信息学分析。该方案为研究 TFs 和表观遗传修饰在肾脏发育和疾病中的作用提供了一个方法框架。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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