利用错配碱基引物的ASO-PCR检测小麦赤霉病菌对多菌灵中抗菌株Codon^(200) TTC→TAC基因型  

ASO-PCR amplified by the primers with mismatches to detect moderately carbendazim-resistant genotype (codon^(200) TTC→TAC) of Fusarium asiaticum

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作  者:陈长军[1] 蔡倩[1] 王建新[1] 周明国[1] 

机构地区:[1]南京农业大学植物病理学系,南京210095

出  处:《植物病理学报》2011年第3期278-284,共7页Acta Phytopathologica Sinica

基  金:国家"973"项目(2006CB101900);国家/江苏省自然科学基金项目(30671048;30671348)/BK2008337;国家博士点基金项目(20050307034)

摘  要:采用在引物3′端引入错配碱基,建立了特异性检测小麦赤霉病菌对多菌灵中抗菌株(Codon200TTC→TAC)基因型的ASO-PCR分子检测技术。结果表明含有错配碱基的引物对NT-7 R1/NT-7 Err5 F能够特异性检测小麦赤霉病菌对多菌灵的中抗菌株(Codon200TTC→TAC),扩增条件为94℃预热5 min;94℃变性60 S,56℃退火60 S,72℃延伸60 S,35个循环;最后72℃延伸15 min。并利用26种常见植物病原真菌验证了所设计引物的PCR扩增特异性。整个检测过程快速,操作简单,结果准确,在6小时内完成。An allele specific oligonucleotide-PCR(ASO-PCR) with mismatches at the 3′ terminal of the primer was set up to detect moderately carbendazim(MBC)-resistant genotype(Codon200 TTC→TAC) of Fusarium asiaticum.The results showed that a pair of probe,NT-7 R1/NT-7 Err5 F with mismatches was deve-loped to successfully detect moderately MBC-resistant isolates(Codon200 TTC→TAC).The ASO-PCR amplification by MBCRF/MBCRR3 was conducted with the following parameters: an initial pre-heat at 94℃ for 5 min,following by 35 cycles of denaturation at 94℃ for 60 s,annealing at 56℃ for 60 s,extension at 72℃ for 60 s and terminated with a final extension at 72℃ for 15 min.26 important plant fungi were used to test the amplification specificity of the primer pair.This method is simple,accurate and time-saving.The result was obtained within 6 h.

关 键 词:小麦赤霉病菌 多菌灵抗药性 ASO-PCR检测 Codon200 TTC→TAC基因型 错配碱基引物 

分 类 号:S435.72[农业科学—农业昆虫与害虫防治]

 

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