Houba-Hérin N, Becker D, Post A, Larondelle Y, Starlinger P
Institut für Genetik, Universität zu Köln, Federal Republic of Germany.
Mol Gen Genet. 1990 Oct;224(1):17-23. doi: 10.1007/BF00259446.
The excision of a Ds-like transposable element (Ac delta) is mediated in trans by the transposable element Ac or its derivatives in Petunia protoplasts cotransfected with two plasmid DNAs. Excision restores the activity of the beta-glucuronidase (GUS) gene that is otherwise shut off by the presence of Ac delta in its leader sequence. A transient expression assay (histochemical test) is used to detect the beta-glucuronidase activity at the protoplast to detect the beta-glucuronidase activity at the protoplast level. The number of blue-stained protoplasts is a measure of the excision frequency. With Ac delta alone a near-zero background of GUS activity is detected, which is weakly enhanced by the presence, in trans, of either the wild-type Ac or the coding region (ORFa) transcribed from the 2' promoter of Agrobacterium tumefaciens TR-DNA. A strong enhancement is observed when a truncated Ac coding region, also under the control of the 2' promoter, is supplied in trans. The truncated version has ATG10 at codon 103 in frame with ORFa and is preceded by 7 out-of-frame ATGs. The assay is quick and well suited for detection of excision frequencies above the value obtained with the wild-type Ac. The presence of empty donor sites following excision can be demonstrated by PCR amplification and direct sequencing of the appropriate DNA fragment.
在矮牵牛原生质体中,与两个质粒DNA共转染时,Ds类转座元件(Ac delta)的切除由转座元件Ac或其衍生物反式介导。切除恢复了β-葡萄糖醛酸酶(GUS)基因的活性,否则该基因会因其前导序列中存在Ac delta而被关闭。采用瞬时表达分析(组织化学检测)来检测原生质体水平的β-葡萄糖醛酸酶活性。蓝色染色原生质体的数量是切除频率的一个衡量指标。单独使用Ac delta时,检测到的GUS活性背景接近零,野生型Ac或根癌农杆菌TR-DNA 2'启动子转录的编码区(ORFa)的反式存在会使其略有增强。当同样在2'启动子控制下的截短Ac编码区反式提供时,会观察到强烈增强。截短版本在第103位密码子处有与ORFa读框一致的ATG10,其前面有7个移码的ATG。该分析快速且非常适合检测高于野生型Ac获得的值的切除频率。切除后空供体位点的存在可通过适当DNA片段的PCR扩增和直接测序来证明。
