双价杀虫蛋白基因在荧光假单胞菌中的表达及增效

利用广宿主质粒载体pJMS6αlac将苏云金芽胞杆菌(Bacillus thuringiensis)杀虫晶体蛋白基因cry1Ac和cry2Aa基因分别及一起进行克隆，将重组质粒导入能在多种作物上定殖、对植物病菌有良好抑菌和防治作用的荧光假单胞菌(Pseudomonas fluorescens)P303菌株，分别得到工程菌株IPP101、IPP201和IPP202。PCRRFLP和Southern blot检测均证明目的基因已经导入了工程菌。SDSPAGE电泳显示工程菌中存在明显的Cry1Ac蛋白带；透射电镜观察发现含cry1Ac基因的两个菌株IPP101和IPP202中杀虫蛋白形成了典型的菱形晶体和蛋白包含体，而在野生P303菌株中均无这些结构。这些结果说明，工程菌中cry1Ac基因得到了很好表达。室内杀虫试验表明：工程菌对棉铃虫初孵幼虫的致死中浓度(LC50)，只含cry1Ac的IPP101为000812mL/g饲料，只含cry2Aa的IPP201为002604mL/g饲料，含双基因的IPP202为000186mL/g饲料；HD73为000170mL/g饲料。cry1Ac和cry2Aa双基因表达产物具有显著增效作用，共毒系数达3328。

EXPRESSION AND SYNERGISM OF TWO CRY INSECTICIDAL PROTEIN GENES IN PSEUDOMONAS FLUORESCENS

Several engineered Pseudomonas fluorescens(Pf) strains were constructed mainly based on a Pseudomonas plasmid pJMS6 alpha-lac and two insecticidal crystal protein genes of Bacillus thuringiensis, cry1Ac and cry2Aa, and the host Pf strain, P303, which was with highly antifungal activity to some plant disease fungi and colonizing ability on a wide range of plants. The DNA introduction was confirmed by PCR-RFLP and Southern blot. The 132 kD insecticidal protein was detected in IPP101 and IPP202 by SDS-PAGE and rhombic insecticidal protein crystals of them were observed through electron microscope, also indicating that cry1Ac gene was highly expressed. The results of insecticidal bioassay indicated that IPP101 was more toxic than IPP201, and IPP202 was the most toxic among the 3 strains. LC50 to the neonates of cotton boll worm(Helicoverpa armigera) were 0.02604, 0.00812 and 0.00186 mL/g feed, consecutively. In IPP202, two gene products showed significant synergism, with the co-toxicity coefficient of 332.8.