摘要
对细菌E.amylovora,E.herbicola和Pseudomonassyringae的DNA提纯,并通过聚合酶链反应,发现引物B_5等可用以有效地鉴别E.amylovora.对E.amylovora细胞培养液直接稀释,加清洁剂处理后进行聚合酶链反应(PCR).据引物B_5测定,得到清晰而强烈的相同的DNA分子电泳光带,可有效反应测定500个细菌细胞;用引物B_5和B_6进一步测定细菌E.amylovora。E.herbicola和P.syringae,从E.herbicoda反应获得一个电泳光谱,从P.syringae获得3个泳谱;用引物B_5和B_7与细菌E.amylovora和P.syringae反应,从E.E.amylovora得到两条相同光带,从P.syringae反应获得了相似的带谱分布。
DNA isolation and amplification of E. amylovora,E. herbicola and Pseadomonas syringae wasdone to find specific primers for identify E. amylovora by PCR,The E.amylovora-cells,which weredirectly added to the PCR reaction mixture with detergent from incubated solution,were detected byprimer B_5,the same bands were got,and the results showed 500 cells were sufficient.E. mylora,E. herbicola and P. syringae were tested by primer B_5 and B_6,one pattern from E. herbicola and three pat-terns from P. syrigae were got.E. amylorora and P. syringae were tested by primer B_5 and B_7,two samebands from E. amylovora were got, and similar pattert1s of bands distribution were got from P. syringae.
出处
《西北师范大学学报(自然科学版)》
CAS
1994年第2期64-70,共7页
Journal of Northwest Normal University(Natural Science)
关键词
梨树
火疫病
聚合酶链反应
DNA
fire blight(Erwinia amylovora). polymerase chain reaction (PCR ),DNA
