Simultaneous studies of gene expression and alternative polyadenylation in primary human immune cells

被引:2
|
作者
Wilton, Joana [1 ,2 ,3 ]
Tellier, Michael [4 ]
Nojima, Takayuki [4 ,5 ]
Costa, Angela M. [6 ,7 ]
Oliveira, Maria Jose [6 ,7 ,8 ]
Moreira, Alexandra [2 ,3 ,9 ]
机构
[1] Univ Porto, ICBAS Inst Ciencias Biomed Abel Salazar, Grad Program Areas Basic & Appl Biol GABBA, PhD Program, Porto, Portugal
[2] Univ Porto, i3S Inst Invest & Inovacao Saude, Gene Regulat, Porto, Portugal
[3] IBMC Inst Biol Mol & Celular, Porto, Portugal
[4] Univ Oxford, Sir William Dunn Sch Pathol, Oxford, England
[5] Kyushu Univ, Med Inst Bioregulat, Fukuoka, Japan
[6] Univ Porto, I3S Inst Invest & Inovacao Saude, Tumor & Microenvironm Interact Grp, Porto, Portugal
[7] INEB Inst Nacl Engn Biomed, Porto, Portugal
[8] Univ Porto, Fac Med, Porto, Portugal
[9] Univ Porto, ICBAS Inst Ciencias Biomed Abel Salazar, Porto, Portugal
来源
基金
欧盟地平线“2020”;
关键词
3' UNTRANSLATED REGIONS; MESSENGER-RNAS; POLARIZATION; MACROPHAGES; INSIGHTS; UTRS; SEQ;
D O I
10.1016/bs.mie.2021.04.004
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Transcription termination in eukaryotic cells involves the recognition of polyadenylation signals (PAS) that signal the site of pre-mRNA cleavage and polyadenylation. Most eukaryotic genes contain multiple PAS that are used by alternative polyadenylation (APA), a co-transcriptional process that increases transcriptomic diversity and modulates the fate of the mRNA and protein produced. However, current tools to pinpoint the relationship between mRNAs in different subcellular fractions and the gene expression outcome are lacking, particularly in primary human immune cells, which, due to their nature, are challenging to study. Here, we describe an integrative approach using subcellular fractionation and RNA isolation, chromatin-bound and nucleoplasmic RNA-Sequencing, 30 RNA-Sequencing and bioinformatics, to identify accurate APA mRNA isoforms and to quantify gene expression in primary human macrophages. Our protocol includes macrophage differentiation and polarization, co-culture with cancer cells, and gene silencing by siRNA. This method allows the simultaneous identification of macrophage APA mRNA isoforms integrated with the characterization of nuclear APA events, the identification of the molecular mechanisms involved, as well as the gene expression alterations caused by the cancer-macrophage crosstalk. With this methodology we identified macrophage APA mRNA signatures driven by the cancer cells that alter the macrophage inflammatory and transcriptomic profiles, with consequences for macrophage physiology and tumor evasion.
引用
收藏
页码:349 / 399
页数:51
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