%A 王永胜,李浩戈,仇润祥,刘中大,扈廷茂 %T 特异切割番茄 1-氨基环丙烷羧酸合成酶mRNA的核酶基因序列的合成与克隆 %0 Journal Article %D 1998 %J 遗传 %R %P 28-32 %V 20 %N 1 %U {http://www.chinagene.cn/CN/abstract/article_4703.shtml} %8 1998-02-10 %X 根据番茄1-氨基环丙烷羧酸合成酶(ACC合成酶)基因cDNA序列, 按照锤头状核酶作用模式, 设计合成长度分别为40mer和48mer的一对引物,经体外退火、延伸、连接,插入质粒pGEM-3Zf(+)的KpnI和BamHI位点之间,经菌落原位杂交、双酶切、聚丙烯酰胺凝胶电泳和序列分析证明,人工合成了特异切割ACC合成酶mRNA第667-669位点GUC序列的核酶基因序列。
Abstract:In order to interrupting the ACC synthase activity in tomato,a hammerhead ribozyme targeting to cleave GUC triplet at the position 667~699 of ACC synthase mRNA was established and integrated into KpnI and BanHI site of vector pGEM-3Zf(+).Four positive clones were gotten by in situ hybridization.The recombinatant plasmids were digested with restriction endonuclease KpnI and BanHI.By polyacrylamide gels electrophoresis and sequence analysis,the size and the sequence of one of the digested product was the same as those of what we expected.These results showed that the ribozyme gene sequence has been obtained.