小麦矮腥黑粉菌及其近缘种的RPB2基因片段序列分析

以小麦矮腥黑粉菌（Tilletia controversa Kühn）及其近缘种小麦网腥黑粉菌［T. caries （DC.）Tul.］、小麦光腥黑粉菌(T. laevis Kühn)和其他6种黑粉菌的DNA为模板，用RNA聚合酶II的第2亚基RPB2基因的通用引物RPB2-740F/RPB2-1365R进行PCR扩增。结果表明，3种小麦腥黑粉菌均能扩增出617 bp大小的DNA片段，供试的其他6种黑粉菌没有任何扩增产物。利用DNAMAN软件进行序列分析结果表明，3种小麦腥黑粉菌的RPB2蛋白基因序列的相似性为99.08%，存在17个碱基的差异。利用RPB2基因的通用引物作为小麦腥黑粉菌的内置对照引物，与小麦矮腥黑粉菌的特异引物CQUTCK2/CQUTCK3相结合可提高小麦矮腥黑粉菌检测的准确性。

Sequence analysis of RPB2 gene of Tilletia controversa and its related species

The genomic DNA of Tilletia controversa Kiihn(TCK)and its related species,T.caries(DC.)Tul.amplified with the universal primers of RPB2 gene,RPB2-740F/RPB2-1365R.A 617 bp fragment was amplified from three Tilletia species on wheat but not from Ustilago spp.,T.horrida and Sporisorium spp.The similarity of the three Tilletia species Was 99.08%,with 17 different bases,based on the analysis by DNAMAN.The RPB2 gene primers,as internal control primers,combined with TCK specific primers CQUTCK2/CQUTCK3 could improve the accuracy of TCK molecular detection by PCR amplification.