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Anti-YTHDF2 RIP-Seq to identify YTHDF2 target mRNAs in hippocampus. Anti-YTHDF2 RIP-Seq to identify YTHDF2 target mRNAs in hippocampus

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NIAID Data Ecosystem2026-03-12 收录
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https://www.ncbi.nlm.nih.gov/bioproject/PRJNA720917
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To identify the target mRNAs of the m6A reader protein YTHDF2 in mouse hippocampus, we carired out anti YTHDF2 RNA Immunoprecipitation (RIP) followed by RNA-sequencencing. Using EZ-Magna RIP™ RNA-Binding Protein Immunoprecipitation Kit (Millipore), RNA from P40 wild type mouse hippocampus was pulled down by rabbit polyclonal anti-YTHDF2 (proteintech) and then sequenced on Illumina Novaseq 6000. The filtered reads were aligned to the mouse reference genome (GRCm38) using BWA mem (v 0.7.12).Then the MACS2 (version 2.1.0) peak calling software was used to identify regions of IP enrichment over background, followed by the motif detected by Homer (Heinz et al., 2010). Peak related genes are then confirmed by PeakAnnotator. Different peak analysis was based on the fold enrichment of peaks of different experiments. A peak was determined as different peak when the odds ratio between two groups was more than 2. Using the same method, genes associated with different peaks were identified. Finally, Biological replicates of anti-YTHDF2 RIP-Seq identified 408 mRNAs transcripts. This study provides gene lists which shows mRNA binding with YTHDF2 in mouse hippocampus. Overall design: 2 replicates, each containing input and IP samples

为鉴定小鼠海马体中m6A识别蛋白YTHDF2的靶信使RNA(mRNA),我们开展了抗YTHDF2 RNA免疫沉淀(RNA Immunoprecipitation, RIP)联合RNA测序的实验。使用EZ-Magna RIP™ RNA结合蛋白免疫沉淀试剂盒(Millipore),我们从出生后40天(P40)的野生型小鼠海马体中提取RNA,通过兔源多克隆抗YTHDF2抗体(Proteintech)进行富集拉取,随后在Illumina NovaSeq 6000测序平台完成上机测序。将过滤后的测序读段比对至小鼠参考基因组(GRCm38),比对工具采用BWA mem(版本0.7.12)。随后使用MACS2(版本2.1.0)峰调用软件鉴定相较于背景样本富集的免疫沉淀区域,并通过Homer工具(Heinz等,2010)检测结合基序。通过PeakAnnotator对峰关联基因进行验证。差异峰分析以不同实验的峰富集倍数为依据,当两组间比值比大于2时,即判定该峰为差异峰。采用相同方法鉴定得到与差异峰相关的基因。最终,本研究通过抗YTHDF2 RIP-seq的生物学重复实验共鉴定得到408条mRNA转录本。本研究提供了在小鼠海马体中与YTHDF2结合的mRNA的基因列表。整体实验设计:设置2次生物学重复,每个重复均包含输入(Input)样本与免疫沉淀(IP)样本。
创建时间:
2021-04-09
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