Mtx1和Cry4Ba毒蛋白基因工程研究进展

球形芽孢杆菌(Bacillus sphaericuss,Bs)Mtx1和苏云金芽孢杆菌以色列亚种(Bacillus thuringiensis israelens,Bti)Cry4Ba是主要的杀蚊毒蛋白。通过对Mtx1毒蛋白杀蚊的作用机理,Cry4Ba毒蛋白的结构与作用机理的介绍,综述Mtx1毒蛋白和Cry4Ba毒蛋白基因工程研究进展,并对Mtx1毒蛋白和Cry4Ba毒蛋白的未来研究进行了思考。

杀蚊苏云金芽胞杆菌毒素Cry4Ba柔韧性分析

采用整合正则模式分析(NMA)的Flexserv程序、WEBnm@程序和TTM@程序分析了杀蚊苏云金芽孢杆菌毒素Cry4Ba的柔韧性。对模拟结果进行了主成分、B-因子、低频振动下的归一化原子平方位移和氨基酸残基运动相关性计算,并对Cry4Ba结构域Ⅰ的α4和α5螺旋在细胞膜中的运动进行了模拟。结果表明,Cry4结构域Ⅰ和结构域Ⅱ表现较大柔韧性,其中N端结构域Ⅰ的螺旋α3、α4和α5柔性表现较大。α4和α5螺旋在细胞膜中的旋转运动、平动、滑动和倾斜运动具有相似的幅度和方向,α4和α5的运动具有较好的协同性。结构域Ⅱ的顶端3个突环都表现较大的柔韧性。各个结构域内部的氨基酸残基运动具有一定的相关性,而各结构域之间运动的相关性较小。研究结果支持Cry4Ba结构域Ⅰ在细胞膜上形成孔道的伞状模型机制并显示结构域Ⅱ顶端突环重要性。

Efficient transcription of the larvicidal <i>cry</i>4<i>Ba</i>gene from <i>Bacillus thuringiensis</i>in transgenic chloroplasts of the green algal <i>Chlamydomonas reinhardtii</i>

Unicellular micro-alga Chlamydomonas reinhardtii has been recognized as a promising host for expressing recombinant proteins albeit its limited utility due to low levels of heterologous protein expression. Here, transcription of the 3.4-kb mosquito-larvicidal cry4Ba gene from Bacillus thuringiensis in transgenic C. reinhardtii chloroplasts under control of the promoter and 5’-untranslated region of photosynthetic psbA gene was accomplished. Inverted repeats in chloroplast genomes of the host strain with deleted endogenous psbA genes were selected as recombination targets. Two transformant lines were obtained by dual-phenotypic screening via exhibition of resistance to spectinomycin and restoration of photosynthetic activity. Stable and site-specific integration of intact cry4Ba and psbA genes into chloroplast genomes found in both transgenic lines implied homoplasmy of organelle populations. Achievement in cotranscription of cry4Ba and psbA transgenes revealed by RT-PCR and Northern blot analyses demonstrates the sufficiency of this system’s transcription machinery, offering the further innovation for insecticidal protein production.