以潮霉素抗性为选择标记的毛壳霉原生质体转化

利用 PEG方法 ,将含有潮霉素抗性标记的质粒 p CB10 0 3转化毛壳霉原生质体 ,并在高于毛壳霉敏感的潮霉素浓度下筛选转化子。转化率达 1～ 2个转化子 / μg质粒 DNA。以潮霉素抗性的毛壳霉转化子的基因组 DNA为模板进行 PCR扩增及其产物的 Southern杂交。结果表明 ,潮霉素抗性基因已整合入毛壳霉染色体。稳定性试验表明 。

基因枪法转化小麦及转基因植株的获得

应用基因枪法转化了小麦幼胚、成熟胚及胚性愈伤组织,成功地将携带有豇豆胰蛋白酶抑制剂(CpTI)基因以及选择标记潮霉素磷酸转移酶(Hpt)基因的质粒pBCAHpt导入小麦胚性愈伤组织。通过在选择培养基上严格筛选后获得潮霉素抗性(hygr)愈伤组织,并进一步分化培养获得完整的小麦再生植株。PCR检测结果显示抗性愈伤组织和再生植株细胞内存在有目的基因序列。

Thansgenic peanut plants obtained by particle bombardment via somatic embryogenesis regeneration system

After pre-culture and treatment of osmosis, cotyledons of immature peanut (Arachis hypogaea L.) zygotic embryos were transformed via particle bombardment with a plasmid containing a chimeric hph gene conferring resistance to hygromycin and a chimeric intron-gus gene. Selection for hygromycin resistant calluses and somatic embryos was initiated at 10th d post-bombardment on medium containing 10-25 mg/L hygromycin. Under continuous selection, hygromycin resistant plantlets were regenerated from somatic embryos and were recovered from nearly 1.6% of the bombarded cotyledons. The presence and integration of foreign DNA in regenerated hygromycin resistant plants was confirmed by PCR (polymerase chain reaction) for the intron-gus gene and by Southern hybridization of the hph gene. GUS enzyme activity was detected in leaflets from transgenic plants but not from control, non-transformed plants. The production of transgenic plants are mainly based on a newly improved somatic embryogenesis regeneration system developed by us.