摘要： 建立和优化了大麦DNA单限制性酶切选择性扩增多态性技术体系(SADF).分别用限制酶PstI、EcoRI和MseI酶切大麦基因组DNA,再与各自相应的人工接头连接,使用带三个选择碱基的引物进行选择性扩增.结果表明:采用分别优化建立的标准PCR扩增检测体系,六个识别碱基的PstI和EcoRI的SADF均能得到丰富稳定的带形,四个识别碱基的MseI不能得到明显谱带.SADF扩增产物片段大小范围为:PstI一般在200～2000bp,而EcoRI在200～1000bp;两者在不同大麦品种中均能检测到多态性,可用于不同大麦品种的检测,但PstI得到的带型明显优于EcoRI,在大麦中得到的片段具有范围宽、分布均匀、易于观察、多态性高等特点。
Abstract:A method named selective amplification DNA fragments (SADF) using single restrictive enzyme was established and optimized in barley.The barley genome DNA was first restricted into fragments of varied length with PstI,EcoRI and MseI respectively,then ligated with synthetic adapters.The ligated sets of fragments were used as templates for PCR amplification.Ideal amplification results could be obtained with different amplification procedure for PstI and EcoRI.Except MseI,both PstI and EcoRI could obtain abundant and reproducible bands,but SADF of PstI was more suitable for barley studies because of wider,more recognizable and polymorphic distribution of bands.