Design and application of 60mer oligonucleotide microarray in SARS coronavirus detection 被引量：7

Design and application of 60mer oligonucleotide microarray in SARS coronavirus detection

导出

摘要 The 60mer oligonucleotide microarray was designed and applied to detecting of SARS (severe acute respiratory syndrome) coronavirus. Thirty 60mer specific oligos were designed to cover the whole genome of the first submitted coronavirus strain, according to the sequence of TOR2 (GENEBANK Accession: AY274119). These primers were synthesized and printed into a microarray with 12×12 spots. RNAs were extracted from the throat swab and gargling fluid of SARS patients and reverse-transcripted into the double strand cDNAs. The cDNAs were prepared as restricted cDNA fragments by the restriction display (RD) technique and labeled by PCR with the Cy5-universal primer. The labeled samples were then applied to the oligo microarray for hybridization. The diagnostic capability of the microarray was evaluated after the washing and scanning steps. The scanning result showed that samples of SARS patients were hybridized with multiple SARS probes on the microarray, and there is no signal on the negative and blank controls. These results indicate that the genome of SARS coronavirus can be detected in parallel by the 60mer oligonucleotide microarray, which can improve the positive ratio of the diagnosis. The oligo microarray can also be used for monitoring the behavior of the virus genes in different stages of the disease status. The 60mer oligonucleotide microarray was designed and applied to detecting of SARS (severe acute res-piratory syndrome) coronavirus. Thirty 60mer specific oligos were designed to cover the whole genome of the first submit-ted coronavirus strain, according to the sequence of TOR2 (GENEBANK Accession: AY274119). These primers were synthesized and printed into a microarray with 12×12 spots. RNAs were extracted from the throat swab and gargling fluid of SARS patients and reverse-transcripted into the double strand cDNAs. The cDNAs were prepared as re-stricted cDNA fragments by the restriction display (RD) technique and labeled by PCR with the Cy5-universal primer. The labeled samples were then applied to the oligo microar-ray for hybridization. The diagnostic capability of the mi-croarray was evaluated after the washing and scanning steps. The scanning result showed that samples of SARS patients were hybridized with multiple SARS probes on the microar-ray, and there is no signal on the negative and blank controls. These results indicate that the genome of SARS coronavirus can be detected in parallel by the 60mer oligonucleotide mi-croarray, which can improve the positive ratio of the diagno-sis. The oligo microarray can also be used for monitoring the behavior of the virus genes in different stages of the disease status.

作者 SHIRong MAWenli WUQinghua ZHANGBao SONGYanbin GUOQiuye XIAOWeiwei WANGYan ZHENGWenling

机构地区 InstituteofMolecularBiology DepartmentofMedicalResearch

出处《Chinese Science Bulletin》 SCIE EI CAS 2003年第2期1165-1169,共5页

关键词寡核苷酸微队列 SARS 冠状病毒检测 RD技术荧光标记分子杂交 SARS coronavirus, oligonucleotide microarray, RD tech-nique, fluorescent labeling, molecular hybridization.

分类号 R373.1 [医药卫生—病原生物学]

引文网络
相关文献

参考文献3

1QIN E'de,ZHU Qingyu,YU Man, FAN Baochang,CHANG Guohui,SI Bingyin,YANG Bao,PENG Wenming,JIANG Tao,LIU Bohua,DENG Yongqiang,LIU Hong,ZHANG Yu,WANG Cui,LI Yuquan,GAN Yonghua,LI Xiaoyu,L Fushuang,TAN Gang,CAO Wuchun,YANG Ruifu,WANG Jian,LI Wei,XU Zuyuan,LI Yan,WU Qingfa,LIN Wei,CHEN Weijun,TANG Lin,DENG Yajun,HAN Yujun,LI Changfeng,LEI Meng,LI Guoqing,LI Wenjie,L Hong,SHI Jianping,TONG Zongzhong,ZHANG Feng,LI Songgang,LIU Bin,LIU Siqi,DONG Wei,WANG Jun,Gane K-S Wong,YU Jun,YANG Huanming.A complete sequence and comparative analysis of a SARS-associated virus(Isolate BJ01)[J].Chinese Science Bulletin,2003,48(10):941-948. 被引量：122
2石嵘,马文丽,宋艳斌,李凌,刘翠华,郑文岭.两种限制性标记方法提高基因芯片杂交结果的信噪比[J].第一军医大学学报,2003,23(2):124-126. 被引量：11
3王艳,马文丽,宋艳斌,肖维威,张宝,黄海,王洪敏,马晓冬,郑文岭.反转录巢式PCR方法检测SARS冠状病毒[J].第一军医大学学报,2003,23(5):421-423. 被引量：19

二级参考文献19

1[1]Satio-Hisaminato A, Katagiri T, Kakiuchi S, et al. Genome-wide profiling of gene expression in 29 normal human tissues with a cDNA microarray[J]. DNA Res, 2002, 9(2): 35-45
2[2]Schmitt ME, Brown TA, Trumpower BL. A rapid and simple method for preparation of RNA from Saccharomyces cerevisiae [J]. Nucleic Acids Res, 1990, 18(10): 3091-2.
3[6]Spellman PT, Sherlock G, Zhang MQ, et al. Comprehensive identification of cell cycle-regnlated genes of the yeast Saccharomyces cerevisiae by microarray hybridization [J]. Mol Biol Cell, 1998, 9(12): 3273-97.
4Peiris J, Lai S, Poon L, et al. Coronavirus as a possible cause of severe acute respiratory syndrome [J]. Lancet, 2003, 361 (9366):1319-25.
5Ksiazek TG, Erdman D, Goldsmith CS, et al. A novel coronavirus associated with severe acute respiratory syndrome[ J ]. N Engl J Med,2003, 348(20): 1953-66.
6Marra MA, Jones SJ, Astell CR, et al. The genome sequence of the SARS-associatedcoronavirus. Science. May 1, 2003, Available:http://www.sciencemag.org/cgi/rapidpdf/1085953v l .pdf.
7Parry J. SARS show no sign of coming under control[J]. BMJ, 2003326(7394): 839-45.
8Parry J. SARS virus identified, but the disease is still spreading[J].BM J, 2003, 326(7395): 897-903.
9Drosten C, Gunther S, Preiser W, et al. Identification of a novel coronavirus in patients with severe acute respiratory syndrome. N Engl J Med, April 10, 2003. Available:http://content.nejm.org/cgi/reprint/NEJMoa030747v2.pdf.
10Lee,N,Hui,D,Wu,A. et al.A major outbreak of severe acute respiratory syndrome inHongKong[].The New England Journal of Medicine.

共引文献145

1陆韻,陈应华.SARS相关病毒与鼠肝炎病毒S蛋白的同源暗示一个潜在受体结合区的存在[J].科学通报,2003,48(11):1197-1199. 被引量：3
2刘志伟,龙北国,赵卫.SARS冠状病毒Mc区原核表达及包涵体复性的研究[J].微生物学免疫学进展,2007,35(3):12-15. 被引量：1
3广东省防治非典型肺炎科技攻关病原分离组,石嵘,马文丽,吴清华,张宝,宋艳斌,郭秋野,肖维威,王艳,郑文岭.SARS冠状病毒检测60mer寡核苷酸基因芯片的设计及应用[J].广东医学,2003,24(z1):14-17.
4高金拽,王小强,祁会彩,黄鹤,陈超,李铮.猪3种重要病毒寡核苷酸芯片诊断方法的建立[J].中国兽医学报,2008,28(9):1000-1003. 被引量：2
5姜焱,张常印,张敬友.SARS病毒的分子生物学研究进展[J].生物信息学,2004,2(1):32-34.
6曹聪.权威、合作和科学发现 SARS和中国科学共同体[J].科学文化评论,2006,3(6):5-19. 被引量：7
7王晓明,邢旺兴.SARS防治药物的研究概况[J].东南国防医药,2003,5(3):235-239.
8SHI Rong,MA Wenli,WU Qinghua,ZHANG Bao,SONG Yanbin,GUO Qiuye,XIAO Weiwei,WANG Yan,ZHENG Wenling.Design and application of 60mer oligonucleotide microarray in SARS coronavirus detection[J].Chinese Science Bulletin,2003,48(12):1165-1169. 被引量：4
9GAO Lei,QI Ji,WEI Haibin,SUN Yigang,HAO Bailin.Molecular phylogeny of coronaviruses including human SARS-CoV[J].Chinese Science Bulletin,2003,48(12):1170-1174. 被引量：7
10QI Zhen,HU Yu,LI Wei,CHEN Yanjun,ZHANG Zhihua,SUN Shiwei,LU Hongchao,ZHANG Jingfen,BU Dongbo,LING Lunjiang,CHEN Runsheng.Phylogeny of SARS-CoV as inferred from complete genome comparison[J].Chinese Science Bulletin,2003,48(12):1175-1178.

同被引文献94

1DONG Jin,HE Zhentian,HAN Chenggui,CHEN Xiulan,ZHANG Lingdi,LIU Weihua,HAN Yuepeng,WANG Jinrong,ZHAI Yafeng,YU Jialin,LIU Yi,XIAO Yueyan.Generation of transgenic wheat resistant to wheat yellow mosaic virus and identification of gene silence induced by virus infection[J].Chinese Science Bulletin,2002,47(17):1446-1450. 被引量：3
2王艳,马文丽,宋艳斌,肖维威,张宝,黄海,王洪敏,马晓冬,郑文岭.反转录巢式PCR方法检测SARS冠状病毒[J].第一军医大学学报,2003,23(5):421-423. 被引量：19
3JINWeiwu,HULiangxiang,DUZhenglin,GAOQiang,GAOHong,NINGYe,FENGJidong,ZHANGJiansan,YINWeidong,LINing.Genome sequence variationanalysis of two SARS coronavirus isolates afterpassage in Vero cell culture[J].Chinese Science Bulletin,2004,49(17):1824-1827. 被引量：1
4MIAO YuChen,GUO JingGong,LIU ErTao,LI Kun,DAI Jie,WANG PengCheng,CHEN Jia,SONG ChunPeng.Osmotically stress-regulated the expression of glutathione peroxidase 3 in Arabidopsis[J].Chinese Science Bulletin,2007,52(1):127-130. 被引量：1
5YANG Hui1,2 & Zhang YaPing1,3 1 Laboratory of Cellular and Molecular Evolution, Kunming Institute of Zoology, Chinese Academy of Sciences, Kunming 650223, China,2 Graduate University of the Chinese Academy of Sciences, Beijing 100049, China,3 Laboratory for Conservation and Utilization of Bio-resources, Yunnan University, Kunming 650091, China.Genomic organization and sequence analysis of the vomeronasal receptor V2R genes in mouse genome[J].Chinese Science Bulletin,2007,52(3):336-342. 被引量：1
6LONG ManYuan,ZHU ZuoYan.Male non-coding RNA genes identified by comparative genomic analysis of the Drosophila genomes[J].Chinese Science Bulletin,2007,52(6):721-724. 被引量：1
7HOU Lei LIU Hao LI JiaBao YANG Xia XIAO YueHua LUO Ming SONG ShuiQing YANG GuangWei PEI Yan.SCFP, a novel fiber-specific promoter in cotton[J].Chinese Science Bulletin,2008,53(17):2639-2645. 被引量：2
8MIGUEL A Esteban.Induced pluripotent stem cell (iPS) technology:promises and challenges[J].Chinese Science Bulletin,2009,54(1):2-8. 被引量：1
9WANG YiXuan,LIU Sheng,LAI LiangXue,GAO ShaoRong.Nuclear reprogramming by nuclear transplantation and defined transcription factors[J].Chinese Science Bulletin,2009,54(1):14-18. 被引量：1
10WANG Yaping, HU Wei, WU Gang,SUN Yonghua, CHEN Shangping, ZHANG Fuying,ZHU Zuoyan, FENG Jianxin & ZHANG Xirui1. State Key Laboratory of Freshwater Ecology and Biotechnology, Institute of Hydrobiology, Chinese Academy of Sciences, Wuhan 430072, China,2. Henan Institute of Aquaculture, Zhengzhou 450044, China.Genetic analysis of "all-fish" growth hormone gene transferred carp (Cyprinus carpio L.) and its F_1 generation[J].Chinese Science Bulletin,2001,46(14):1174-1178. 被引量：23

引证文献7

1吴清华,马文丽,石嵘,郭秋野,张宝,李凌,张海燕,郑文岭.Poly-L-Lysine玻片在寡核苷酸芯片制备中的改进[J].第一军医大学学报,2004,24(11):1236-1241. 被引量：1
2HAI YAN ZHANG,WEN LI MA,XIAO MING ZHANG,WEN LING ZHENG.Fabrication of oligonucleotide microarray for the detection of Japanese encephalitis virus[J].Journal of Microbiology and Immunology,2006,4(2):96-99.
3吴清华,马文丽,朱利娜,张宝.交联型丙烯酸酯聚合物分子层用于固定寡核苷酸分子初探[J].局解手术学杂志,2008,17(4):228-230.
4Xuming Jia,Rui An,Xiao-Ya Chen.From Chinese Science Bulletin to Science Bulletin: celebrate the coming 50th birthday[J].Science Bulletin,2015,60(24):2145-2150. 被引量：1
5Minzhe Shen,Ying Zhou,Jiawei Ye,Abdu Ahmed Abdullah AL-maskri,Yu Kang,Su Zeng,Sheng Cai.Recent advances and perspectives of nucleic acid detection for coronavirus[J].Journal of Pharmaceutical Analysis,2020,10(2):97-101. 被引量：30
6Koel Sinha,Sutapa Som Chaudhury,Pramita Sharma,Bhuban Ruidas.COVID-19 rhapsody:Rage towards advanced diagnostics and therapeutic strategy[J].Journal of Pharmaceutical Analysis,2021,11(5):529-540.
7Ayushi Bisht,Abhishek Mishra,Harender Bisht,R.M.Tripathi.Nanomaterial Based Biosensors for Detection of Viruses Including SARS-CoV-2:A Review[J].Journal of Analysis and Testing,2021,5(4):327-340. 被引量：3

二级引证文献35

1李子玥,杨同仁,杨歌,黄渊余.病原微生物的核酸检测分析研究进展[J].应用化学,2021,38(5):592-604. 被引量：2
2姜尧月,赵宝银,李斌,张久聪,李初谊,何昱静,于晓辉.多组学在新型冠状病毒肺炎诊断中的作用及研究进展[J].热带医学杂志,2023,23(3):420-424.
3Abdollah Yari,Samaneh Penhani.A New Highly Sensitive Optical Sensor Based on Congo-Red for the Determination of Thorium(Ⅳ) in Aqueous Solution[J].Journal of Analysis and Testing,2023,7(4):416-424.
4Zi-Jian Wang,Qiang Li,Li-Li Tan,Chun-Guo Liu,Li Shang.Metal–Organic Frameworks-Mediated Assembly of Gold Nanoclusters for Sensing Applications[J].Journal of Analysis and Testing,2022,6(2):163-177. 被引量：4
5刘莹,刁波,何泽民,薛燕南,黄前川,丁进亚.化学发光免疫分析技术和量子点免疫荧光组织化学检测新型冠状病毒特异性抗体及其应用评价[J].华南国防医学杂志,2021,35(9):630-634. 被引量：1
6崔杰,宋彭,燕宇帆,邵良俊,王浩源,刘方,冯峰,瞿体明,刘华军.用于46 T全超导磁体装置的26 T REBa_(2)Cu_(3)O_(7-δ)高温超导内插磁体电磁设计研究[J].低温物理学报,2021,43(5):249-258.
7徐秋林,马文丽,李凌,石嵘,毛向明,吴清华,郑文岭.GFP质控芯片的初步研究[J].生物技术,2005,15(4):16-20.
8张喆傲,高钟镐,黄伟.新型冠状病毒SARS-CoV-2检测分析技术研究进展[J].药物分析杂志,2020,40(10):1715-1726. 被引量：3
9毛佳泉(综述),鲁彦,寇炜(审校).新型冠状病毒实验室特异性检测技术研究进展[J].检验医学与临床,2020,17(23):3526-3529. 被引量：1
10王星,吴茜,李红蔚,华静娜,李莉,秦中华.天津地区新型冠状病毒肺炎患者特异性IgM和IgG动态变化研究[J].天津医药,2021,49(1):41-44. 被引量：4

1SHI Rong,MA Wenli,WU Qinghua,ZHANG Bao,SONG Yanbin,GUO Qiuye,XIAO Weiwei,WANG Yan,ZHENG Wenling.Design and application of 60mer oligonucleotide microarray in SARS coronavirus detection[J].Chinese Science Bulletin,2003,48(12):1165-1169. 被引量：4
2YiSHI Hai-FengLUO Chang-DeLU You-XinJIN.The Suppression of SARS Coronavirus Gene Expression by Antisense ODN and siRNA[J].Acta Biochimica et Biophysica Sinica,2004,36(2):155-155.
3石磊,张其鹏,芮伟,卢铭,景霞,尚彤,国强华.SARS冠状病毒推定结构蛋白序列分析[J].北京大学学报（医学版）,2003,35(B05):132-134. 被引量：5
4Min WANG.The Composite and Hybridization Approach in Developing New Biomaterials[J].功能材料信息,2016,13(4):36-36.
5周密,李凡.SARS冠状病毒S蛋白研究进展[J].中国实验诊断学,2003,7(6):549-551.
6WenbingChen ShousongLi BiyingShao TengZheng ShuxunJiang XiaorongHuan KaizhenCai ZhidengZhang.Preliminary Study on Detecting the SARS-CoV Specific Target cDNA Fragments by Multiplex PCR[J].Genomics, Proteomics & Bioinformatics,2004,2(1):55-58. 被引量：2
7JINWeiwu,HULiangxiang,DUZhenglin,GAOQiang,GAOHong,NINGYe,FENGJidong,ZHANGJiansan,YINWeidong,LINing.Genome sequence variationanalysis of two SARS coronavirus isolates afterpassage in Vero cell culture[J].Chinese Science Bulletin,2004,49(17):1824-1827. 被引量：1
8杨瑞锋,徐国宾,闫存玲,张国华,李海霞,夏铁安.SARS冠状病毒的生物学性状及实验室检测方法研究进展[J].北京大学学报（医学版）,2003,35(B05):121-123. 被引量：7
9Yao Dezhong,Yang Shaoguo(Dep. of Auto,UEST of China,Chengdu 610054,P. R. China).THE DESIGN AND APPLICATION OF RELAXANT MONITORING SYSTEM[J].Chinese Journal of Biomedical Engineering(English Edition),1995,4(4):219-219.
10孙朝晖,郑文岭,彭翼飞,张宝,马文丽.应用限制性显示技术制备HCVcDNA诊断基因芯片的初步研究[J].微生物学报,2005,45(2):226-230. 被引量：5

Chinese Science Bulletin

2003年第2期

浏览历史

内容加载中请稍等...