甘蔗黄叶病毒的RT-PCR检测技术  被引量:19

Detection of sugarcane yellow leaf virus by RT-PCR

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作  者:高三基[1] 郭晋隆[1] 孟岩[1] 黄振瑞[1] 陈如凯[1] 刘文荣[1] MICHAEL S Irey 

机构地区:[1]福建农林大学农业部甘蔗生理生态与遗传改良重点开放实验室,福建福州350002 [2]美国农业部农业研究服务中心美国园艺研究实验室,弗罗里达34945

出  处:《福建农林大学学报(自然科学版)》2006年第5期466-470,共5页Journal of Fujian Agriculture and Forestry University:Natural Science Edition

基  金:农业部"948"计划资助项目(2003-Q06);福建省自然科学基金资助项目(Z0516013)

摘  要:以甘蔗黄叶病毒(ScYLV)特异性引物YLSF111和YLSR462为引物,对福建蔗区8个罹病品种的疑似病株进行RT-PCR检测,扩增出352 bp特异性片段.将PCR产物克隆后测序,序列分析表明,该片段是ScYLV外壳蛋白(CP)基因的一部分,核苷酸和氨基酸序列同源性达95%以上,与美国、印度、巴西等国家ScYLV分离物(GeneBank登录号分别为AF157029、AY236971、AF141385)CP基因同源性达100%,证实我国福建地区甘蔗黄叶综合症的病原体为ScYLV.本研究同时建立了ScYLV的RT-PCR检测技术.Using primers YLSF111 and YLSR462, a 352 bp fragment was amplified by RT-PCR in total RNA extracted from leaves of eight infected sugarcane varieties in Fujian, P. R. China. The PCR product was cloned and sequenced. Nucleotide and deduced amino acid sequences were greater than 95% homologus with ScYLV isolates from other countries and were 100% homologus with ScYLV isolates from America, India and Brazil ( GenBank accession numbers AF157029, AY236971 and AF141385 respectively). The results confirmed that the causal organism of YLS of sugarcane in China was ScYLV. The protocol for the use of RT-PCR to detect ScYLV was described in the paper.

关 键 词:甘蔗 甘蔗黄叶病毒 RT—PCR 分子鉴定 

分 类 号:S566.1[农业科学—作物学] Q945.8[农业科学—植物病理学]

 

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