抗肿瘤多肽9R-P201诱导下的肝癌HepG2细胞转录组测序分析

doi:10.13560/j.cnki.biotech.bull.1985.2017-0053

生物技术通报 ›› 2017, Vol. 33 ›› Issue (7): 210-215.doi: 10.13560/j.cnki.biotech.bull.1985.2017-0053

抗肿瘤多肽9R-P201诱导下的肝癌HepG2细胞转录组测序分析

刘文荣¹,丁若凡¹,张一鸣¹,李宇鹏¹,李玲²,郭志云¹

1. 西南交通大学生命科学与工程学院，成都 610031；
2. 成都市第三人民医院病理科，成都 610031

收稿日期:2017-01-26 出版日期:2017-07-11 发布日期:2017-07-11
作者简介:刘文荣，男，硕士研究生，研究方向：非编码RNA结构与功能；E-mail：liuzimu1992@gmail.com
基金资助:
中央高校基本科研业务费专项资金（2682016YXZT04），国家大学生创新性实验计划项目（201610613066）

Transcriptome Sequencing Analysis of Hepatocellular Carcinoma HepG2 Cells Induced by Antitumor Peptide 9R-P201

LIU Wen-rong¹ ,DING Ruo-fan¹, ZHANG Yi-ming¹ ,LI Yu-peng¹, LI Ling² ,GUO Zhi-yun¹

1. School of Life Science and Engineering，Southwest Jiaotong University，Chengdu 610031；
2. Department of Pathology，the Third People’s Hospital of Chengdu，Chengdu 610031

Received:2017-01-26 Published:2017-07-11 Online:2017-07-11

摘要/Abstract

摘要： 旨在探索多肽9R-P201处理肝癌HepG2细胞后基因融合、单核苷酸多态性（Single nucleotide polymorphism，SNP）突变、可变剪接等事件，并分析差异表达基因所参与的生物学进程与信号通路，以期解析多肽9R-P201在转录组水平对肝癌细胞的调控。通过转录组测序检测9R-P201处理肝癌HepG2细胞前后基因差异表达情况，tophat-fusion软件检测基因融合，SAMTOOLS软件检测SNP位点，rMATS软件鉴定可变剪接，使用基因本体（Gene Ontology，GO）和京都基因与基因组百科全书（Kyoto encyclopedia of genes and genomes，KEGG）富集分析方法对差异表达基因进行功能富集分析。结果共检测到可变剪接事件276个、SNP位点5 557个、基因融合事件45个；同时共得到显著差异表达基因 403个，其中上调269个而下调134个，基因的功能富集分析结果显示差异表达基因显著富集细胞生长、迁移等肿瘤相关生物进程，并参与多条与癌症相关的信号通路。研究表明在9R-P201诱导HepG2细胞后，导致表达差异基因显著与肿瘤生物学进程和通路相关，并发生了大量可变剪接、SNP突变、基因融合等事件，这暗示着该多肽有望作为后续肝癌介入治疗潜在药物分子。

关键词: 9R-P201, 肝细胞癌, 转录组测序, 基因

Abstract: This wok aims to elucidate the regulation of 9R-P201 on hepatoma cells（HepG2）at transcriptome level by investigating the gene fusion，SNP（Single Nucleotide Polymorphism）mutation，alternative splicing and other events after 9R-P201 treating HepG2，and analyzing the biological processes and signaling pathways involved by differentially expressed genes. The expression differences of the genes before and after the 9R-P201 treating HepG2 cell line were detected by transcriptome sequencing. Meanwhile，gene fusion，SNPs，and alternative splicing were identified by tophat-fusion，SAMTOOLS software，and rMATS respectively. Functional enrichment analysis of differentially expressed genes were performed by GO（Gene Ontology）and KEGG（Kyoto Encyclopedia of Genes and Genomes）. As results，276 alternative splicing events，5 557 SNP sites，and 45 gene fusion events were detected in the transcriptome sequencing. In addition，403 differentially expressed genes including 269 up-regulated and 134 down-regulated were detected. Gene GO and KEGG enrichment analysis showed that differentially expressed genes were significantly involved in the biological processes of cell growth，locomotion，as well as a number of cancer-related signaling pathways. In conclusion，the study revealed that the differentially expressed genes resulted from 9R-P201 treating HepG2 were significantly correlated with the biological processes and signaling pathways related to cancer and hepatocellular carcinoma HepG2 cell line，and a large number of alternative splicing events，SNP mutations，gene fusion events after 9R-P201 inducement occurred，suggesting this peptide may be used as a potential drug for subsequent hepatocellular carcinoma interventional therapy.

Key words: 9R-P201, hepatocellular carcinoma, transcriptome sequencing, gene

刘文荣,丁若凡,张一鸣,李宇鹏,李玲,郭志云. 抗肿瘤多肽9R-P201诱导下的肝癌HepG2细胞转录组测序分析[J]. 生物技术通报, 2017, 33(7): 210-215.

LIU Wen-rong ,DING Ruo-fan, ZHANG Yi-ming ,LI Yu-peng, LI Ling ,GUO Zhi-yun. Transcriptome Sequencing Analysis of Hepatocellular Carcinoma HepG2 Cells Induced by Antitumor Peptide 9R-P201[J]. Biotechnology Bulletin, 2017, 33(7): 210-215.

参考文献

[1] Ferlay J, Soerjomataram I, Dikshit R, et al. Cancer incidence and mortality worldwide：sources, methods and major patterns in GLOBOCAN 2012[J] . Int J Cancer, 2015, 136（5）：E359-386.
[2] Brito AF, Abrantes AM, Tralh?o JG, et al. Targeting hepatocellular carcinoma：what did we discover so far?[J] . Oncology Reviews, 2016, 10（2）：302.
[3] Deng GL, Zeng S, Shen H. Chemotherapy and target therapy for hepatocellular carcinoma：New advances and challenges[J] . World Journal of Hepatology, 2015, 7（5）：787-798.
[4] Meng Y, Gao X, Chen W, et al. Methionine enkephalin（MENK）mounts antitumor effect via regulating dendritic cells（DCs）[J] . International Immunopharmacology, 2017, 44：61-71.
[5] Xia L, Wu Y, Ma JI, et al. The antibacterial peptide from Bombyx mori cecropinXJ induced growth arrest and apoptosis in human hepatocellular carcinoma cells[J] . Oncology Letters, 2016, 12 （1）：57-62.
［6］Cui J, Huang J, Guo T, et al. Expression and selection of human foxm1c binding peptides and yheir inhibitions on MCF7 cancer cells［J］. Int J Pept Res Ther, 2014, 20（4）：447-456.
［7］Bi Z, Liu W, Ding R, et al. A novel peptide, 9R-P201, strongly inhibits the viability, proliferation and migration of liver cancer HepG2 cells and induces apoptosis by down-regulation of FoxM1 expression［J］. Eur J Pharmacol, 2017, 796：175-189.
［8］Trapnell C, Roberts A, Goff L, et al. Differential gene and transcript expression analysis of RNA-seq experiments with TopHat and Cufflinks［J］. Nature Protocols, 2012, 7（3）：562-578.
［9］Kim D, Salzberg SL. TopHat-Fusion：an algorithm for discovery of novel fusion transcripts［J］. Genome Biol, 2011, 12（8）：R72.
［10］Li HD, Menon R, Omenn GS, et al. The emerging era of genomic data integration for analyzing splice isoform function［J］. Trends in Genetics：TIG, 2014, 30（8）：340-347.
［11］Thomas PD, Mi H, Lewis S. Ontology annotation：mapping genomic regions to biological function［J］. Current Opinion in Chemical Biology, 2007, 11（1）：4-11.
［12］Kanehisa M, Araki M, Goto S, et al. KEGG for linking genomes to life and the environment［J］. Nucleic Acids Res, 2008, 36：D480-484.
［13］ Koberle B, Koch B, Fischer BM, et al. Single nucleotide polymorp-hisms in DNA repair genes and putative cancer risk［J］. Archives of Toxicology, 2016, 90（10）：2369-2388.
［14］Shastry BS. SNPs：impact on gene function and phenotype［J］. Methods in Molecular Biology, 2009, 578：3-22.
［15］Chen J, Driguneswar P, Shravan K, et al. Selecting cell lines for SNP human identification assay development［J］. Atlas Journal of Biotechnology, 2011, 1（1）：21-26, 2011.
［16］Gommans WM, Tatalias NE, Sie CP, et al. Screening of human SNP database identifies recoding sites of A-to-I RNA editing［J］. RNA, 2008, 14（10）：2074-2085.
［17］Eisenberg E, Adamsky K, Cohen L, et al. Identification of RNA editing sites in the SNP database［J］. Nucleic Acids Research, 2005, 33（14）：4612-4617.
［18］Guo J, Xu N, Yao Y, et al. Efficient expression of recombinant human heavy chain ferritin（FTH1）with modified peptides［J］. Protein Expression and Purification, 2016, 131：101-108.

[1]	娄慧, 朱金成, 杨洋, 张薇. 抗、感品种棉花根系分泌物对尖孢镰刀菌生长及基因表达的影响[J]. 生物技术通报, 2023, 39(9): 156-167.
[2]	刘玉玲, 王梦瑶, 孙琦, 马利花, 朱新霞. 启动子RD29A对转雪莲SikCDPK1基因烟草抗逆性的影响[J]. 生物技术通报, 2023, 39(9): 168-175.
[3]	王腾辉, 葛雯冬, 罗雅方, 范震宇, 王玉书. 基于极端混合池（BSA）全基因组重测序的羽衣甘蓝白色叶基因定位[J]. 生物技术通报, 2023, 39(9): 176-182.
[4]	王贵芳, 姚元涛, 许海峰, 相昆, 梁家慧, 张淑辉, 王文茹, 张明娟, 张美勇, 陈新. 核桃JrSnRK1α1.1调控种子油脂合成与积累[J]. 生物技术通报, 2023, 39(9): 183-191.
[5]	杨志晓, 侯骞, 刘国权, 卢志刚, 曹毅, 芶剑渝, 王轶, 林英超. 不同抗性烟草品系Rubisco及其活化酶对赤星病胁迫的响应[J]. 生物技术通报, 2023, 39(9): 202-212.
[6]	薛宁, 王瑾, 李世新, 刘叶, 程海娇, 张玥, 毛雨丰, 王猛. 多基因同步调控结合高通量筛选构建高产L-苯丙氨酸的谷氨酸棒杆菌工程菌株[J]. 生物技术通报, 2023, 39(9): 268-280.
[7]	李雪琪, 张素杰, 于曼, 黄金光, 周焕斌. 基于CRISPR/CasX介导的水稻基因组编辑技术的建立[J]. 生物技术通报, 2023, 39(9): 40-48.
[8]	陈小玲, 廖东庆, 黄尚飞, 陈英, 芦志龙, 陈东. 利用CRISPR/Cas9系统改造酿酒酵母的研究进展[J]. 生物技术通报, 2023, 39(8): 148-158.
[9]	吕秋谕, 孙培媛, 冉彬, 王佳蕊, 陈庆富, 李洪有. 苦荞转录因子基因FtbHLH3的克隆、亚细胞定位及表达分析[J]. 生物技术通报, 2023, 39(8): 194-203.
[10]	王佳蕊, 孙培媛, 柯瑾, 冉彬, 李洪有. 苦荞糖基转移酶基因FtUGT143的克隆及表达分析[J]. 生物技术通报, 2023, 39(8): 204-212.
[11]	付钰, 贾瑞瑞, 何荷, 王良桂, 杨秀莲. 两种砧木楸树嫁接苗生长差异及转录组比较分析[J]. 生物技术通报, 2023, 39(8): 251-261.
[12]	方澜, 黎妍妍, 江健伟, 成胜, 孙正祥, 周燚. 盘龙参内生真菌胞内细菌7-2H的分离鉴定和促生特性研究[J]. 生物技术通报, 2023, 39(8): 272-282.
[13]	饶紫环, 谢志雄. 一株Olivibacter jilunii 纤维素降解菌株的分离鉴定与降解能力分析[J]. 生物技术通报, 2023, 39(8): 283-290.
[14]	郭少华, 毛会丽, 刘征权, 付美媛, 赵平原, 马文博, 李旭东, 关建义. 一株鱼源致病性嗜水气单胞菌XDMG的全基因组测序及比较基因组分析[J]. 生物技术通报, 2023, 39(8): 291-306.
[15]	石佳鑫, 刘凯, 朱金洁, 祁显涛, 谢传晓, 刘昌林. 基因编辑技术改良玉米株型增加杂交种产量[J]. 生物技术通报, 2023, 39(8): 62-69.

抗肿瘤多肽9R-P201诱导下的肝癌HepG2细胞转录组测序分析

Transcriptome Sequencing Analysis of Hepatocellular Carcinoma HepG2 Cells Induced by Antitumor Peptide 9R-P201

PDF (PC)

可视化

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价