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CryK13V基因对绿色木霉原生质体的转化

Transformation of CryK13V gene into protoplasts of Trichoderma viride.

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【作者】 刘士旺郭泽建蒋冬花王政逸

【Author】 LIU Shi-wang~(1,3),GUO Ze-jian~(1,3),JIANG Dong-hua~3,WANG Zheng-yi~3(1.College of Biology and Chemistry Engineering,Zhejiang University of Science and Technology,Hangzhou 310023,China;2.College of Agronomy & Biotechnology,China Agricultural University,Beijing 100094,China;(3.Biotechnology) Institute,Zhejiang University,Hangzhou 310029,China)

【机构】 浙江科技学院生物与化学工程学院中国农业大学农学与生物技术学院浙江大学生物技术研究所浙江大学生物技术研究所 浙江杭州310023浙江杭州310029北京100094

【摘要】 将Cry基因的13位赖氨酸(K)突变成缬氨酸(V)的突变基因CryK13 V,构建于pCSN43载体,完成绿色木霉转化载体pCSNTCCm的构建.在研究绿色木霉(Trichoderma viride)原生质体形成和再生基础上,初步研究了绿色木霉转化条件.结果表明,绿色木霉原生质体形成的合适条件为:pH 6.98磷酸盐缓冲液加入4 mg?mL-1glucanex,培养24 h的菌丝,40 r?min-1振荡条件下30℃酶解4 h,原生质体产量达到4.7×107个?mg-1.原生质体在0.3 mol?L-1肌醇和0.3 mol?L-1KCl的CM培养基上再生率为14.5%.用限制酶XhoⅠ介导将带有潮霉素抗性标记的CryK13 V基因转化到绿色木霉中,转化率为每微克DNA得到1~2个转化子,转化子稳定性和PCR鉴定结果表明,外源基因已转入受体菌绿色木霉中.

【Abstract】 The lysine in site 13 of cryptogein protein was mutated to valine(K13V) through PCR site-directed mutagenesis.The mutant fragment(CryK13V) was confirmed by enzyme digestion and DNA sequencing.The CryK13V gene was expressed in Trichoderma viride,with constructed vector pCSNTCCm.Transformation was carried out by restriction enzyme(XhoⅠ) mediated integration and transformants were obtained on the CM media contained 200 μg.mL-1 hygromycin B,and the transformation rate was 1-2 transformants per microgramme vector DNA.The optimum of isolation,regeneration of the protoplasts from T.viride was that: pH=6.98 phosphate buffer,4 mg·mL-1 glucanex,hypha cultured 24 hours,digested at 30 ℃ for 4 hours,and the yields of the protoplasts was 4.7×107 per·mg-1.On the CM medium containing 0.3 mol·L1 KCl and 0.3 mol·L-1 Inositol,the regeneration rate was 14.5%.

【基金】 国家自然科学基金资助项目(39980033);浙江省自然科学基金资助项目(Y305208)
  • 【文献出处】 浙江大学学报(农业与生命科学版) ,Journal of Zhejiang University(Agriculture and Life Sciences) , 编辑部邮箱 ,2006年03期
  • 【分类号】S476
  • 【被引频次】6
  • 【下载频次】232
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