苏云金杆菌辅助蛋白P19对杀虫晶体蛋白Cry11Aa表达的影响

苏云金杆菌以色列亚种的p19基因、cry11Aa基因和p20基因位于同一操纵子上,据推测辅助蛋白P19可能与Cry11Aa蛋白的晶体化相关。本研究利用穿梭载体pHT3101构建了两个重组质粒pHcy1和pHcy3,两质粒均携带cry11Aa基因,但后者完全缺失了cry11Aa基因上游的p19基因。将重组质粒电激转化至苏云金杆菌无晶体突变株4Q7中进行蛋白表达,SDS-PAGE结果表明在4Q7(pHcy1)和4Q7(pHcy3)中均能检测到正常表达的Cry11Aa蛋白,但单位体积培养液的Cry11Aa蛋白在辅助蛋白P19存在时的表达量明显高于其单独表达的表达量;透射电镜观察显示两菌株中的Cry11Aa蛋白形成了大小相近、形状相似的双梯形晶体;另外,生物测定结果表明重组菌株4Q7(pHcy1)和4Q7(pHcy3)对三龄致倦库蚊的杀虫活性没有显著性差异。该现象说明辅助蛋白P19的缺失对Cry11Aa蛋白的晶体形成和杀蚊活性没有影响,但P19作为分子伴侣在一定程度上帮助提高了Cry11Aa蛋白的表达水平。     

苏云金芽孢杆菌Cry1Aa和Cry1Ca结构域交换对晶体形态和杀虫活性影响

通过体外重组的方法,实现了苏云金芽孢杆菌杀虫晶体蛋白Cry1Aa和Cry1Ca的功能性结构域Ⅰ、Ⅱ和Ⅲ的互换,得到了6株苏云金杆菌重组菌株BT-ACC,BT-AAC,BT-ACA,BT-CAA,BT-CCA和BT-CAC。SDS-PAGE和Westernblot分析表明,重组菌株BT-CAA和BT-CCA能表达产生135kDa左右的杂交晶体蛋白Cry1CAA和Cry1CCA,但其蛋白表达量较野生型Cry1Aa和Cry1Ca低。用牛胰蛋白酶对杂交晶体蛋白Cry1CAA、Cry1CCA及野生型Cry1Aa和Cry1Ca进行消化,证明所有晶体蛋白都能产生65kDa的活性毒素。电镜观察发现,野生菌株BT-Cry1Aa和BT-Cry1Ca形成典型的菱形晶体,而重组菌株BT-CCA和BT-CAA则形成球形或颗粒状杂交晶体。纯化晶体的生物测定显示,杂交晶体蛋白Cry1CAA和Cry1CCA对甜菜夜蛾的毒力比野生型晶体蛋白降低3~5倍,对棉铃虫的毒力比野生型晶体蛋白降低了190~260倍。研究结果表明,苏云金杆菌晶体蛋白不同结构域的相互作用会影响杂交晶体蛋白的表达、晶体形态和杀虫活性。     

苏云金芽孢杆菌Cry1Ac杀虫晶体蛋白及其分子设计

cry1Ac编码的杀虫晶体蛋白是苏云金芽孢杆菌(Bt)产生的多种杀虫晶体蛋白中对鳞翅目昆虫有很高毒性的蛋白.第一个Cry1Ac杀虫晶体蛋白最早在库斯塔克亚种HD73中以伴胞晶体形式分离获得,其编码区为3 534 bp,编码蛋白分子量为133 kD,含1 178个氨基酸,等电点为4.84.自此以来,Cry1Ac杀虫晶体蛋白结构、功能以及应用研究一直是Bt杀虫晶体蛋白研究的重要方向.本文介绍了苏云金芽孢杆菌中应用最广泛的Cry1Ac杀虫晶体蛋白家族的结构、功能及其基因分类,并进一步就基于苏云金芽孢杆菌Cry1Ac杀虫晶体蛋白的基因工程研究做了分析,提出了持续利用BtCry1Ac杀虫晶体蛋白的一些见解.     

苏云金芽孢杆菌以色列亚种cyt1 Aa基因在球形芽孢杆菌中表达

将编码cyt1Aa基因和 p2 0蛋白基因的DNA片段分别克隆连接于两个不同的穿梭载体 pBU 4和pMK 3上 ,构建了重组质粒 pBA 30和 pMA 6,通过电击法 ,将重组质粒分别转化 B .s野生株2 2 97,获得了转化菌株Bs 97 30和Bs 97 6。SDS PAGE和Westernblot分析证实了cyt1Aa基因在转化菌株Bs 97 30中获得了表达 ,而在转化菌株Bs 97 6中未检测到cyt1Aa基因表达的蛋白。转化菌株Bs 97 30中 ,cyt1Aa基因与B .s二元毒素基因同步于菌体生长的对数期起始表达 ,并持续至芽孢形成。生测结果表明 ,转化菌株Bs 97 30中cyt1Aa基因的表达并未明显增强其对敏感和抗性致倦库蚊幼虫的毒力。其原因可能是弱毒性的 cyt1Aa蛋白在转化菌株中的表达量不高。     

苏云金芽孢杆菌cry2Aa操纵元蛋白对杀虫蛋白晶体形成作用的研究

利用重叠PCR的方法,通过两次PCR扩增,分别获得cry2A10操纵元的orf1、orf1 orf2与cry2Ab5基因的融合片段。融合片段经BamHⅠ和EcoRⅠ双酶切与pHT315连接,分别构建了基因融合片段的原核表达载体pFU(orf1 2Ab)和pFU(orf1 orf2 2Ab),电转化Bt无晶体突变株4Q7后,扫描电镜下可观察到典型的方形晶体,通过SDS-PAGE可检测到60kD大小的蛋白表达带。结果表明,cry2Ab5可在cry2a0的启动子帮助下有效转录和表达,并在orf2产物帮助下形成蛋白晶体。     

苏云金芽孢杆菌cry2Aa操纵元蛋白对杀虫蛋白晶体形成作用的研究

利用重叠PCR的方法,通过两次PCR扩增,分别获得cry2Aa10操纵元的orf1、orf1+orf2与cry2Ab5基因的融合片段。融合片段经BamHⅠ和EcoRⅠ双酶切与pHT315连接,分别构建了基因融合片段的原核表达载体pFU(orf1+2Ab)和pFU(orf1+orf2+2Ab),电转化Bt无晶体突变株4Q7后,扫描电镜下可观察到典型的方形晶体,通过SDSPAGE可检测到60kD大小的蛋白表达带。结果表明,cry2Ab5可在cry2Aa10的启动子帮助下有效转录和表达,并在orf2产物帮助下形成蛋白晶体。     

苏云金芽孢杆菌辅助蛋白的研究进展

杀虫晶体蛋白是苏云金芽孢杆菌所产生的主要杀虫成分 ,在其超量表达与晶体形成过程中有时需要辅助蛋白的参与。在这些辅助蛋白中有的能够防止正在翻译过程中的杀虫晶体蛋白被菌体内的蛋白酶降解 ,起着分子伴侣的作用 ;有的在晶体形成过程中起着脚手架的作用。本文对辅助蛋白 P₂ 0、P1₉以及ORF₁、ORF_{2等在杀虫晶体蛋白表达及晶体形成过程中的作用作了综述。}     

苏云金杆菌辅助蛋白基因p19和orf1-orf2对杀虫晶体蛋白Cyt1 Aa表达的影响(英文)

为检测苏云金杆菌辅助蛋白P19和ORF1 ORF2对杀虫晶体蛋白Cyt1Aa表达的影响 ,构建了 5个重组表达质粒。 5个质粒都含有cyt1Aa基因 ,但pT1只含有cyt1Aa基因 ,pT2同时含有p19基因 ,pT3同时含有orf1 orf2串联基因 ,pT4同时含有p19基因和p2 0基因 ,pT5同时含有orf1 orf2串联基因和p2 0基因。将这 5个表达质粒和质粒pWF4 5电转化到苏云金杆菌晶体缺陷型 4Q7中 ,分别获得转化菌株Bt T1、Bt T2、Bt T3、Bt T4、Bt T5和Bt WF4 5。SDS PAGE结果显示 ,菌株Bt T1、Bt T2和Bt T3只产生少量的 2 7kDCyt1Aa蛋白 ,而且部分降解为大约 2 4kD的蛋白。而Bt T4和Bt T5能产生大量的Cyt1Aa蛋白 ,但Bt T4和Bt T5的Cyt1Aa蛋白产量都明显少于Bt WF4 5。电镜观察和生物测定结果表明Bt T4和Bt T5与Bt WF4 5的晶体大小和杀蚊毒力没有显著性差异。研究表明P19和ORF1 ORF2对Cyt1Aa蛋白的合成显示可能有抑制作用。     

苏云金芽孢杆菌沉默基因cry2Ab3在大肠杆菌中表达及杀虫活性研究

对苏云金芽孢杆菌C002菌株cry2Ab基因阳性克隆pHT3152Ab进行亚克隆和序列测定,在CenBank注册后经国际Bt杀虫蛋白基因委员会正式命名为cry2Ab3。序列分析表明该基因含有芽孢杆菌特异的RBS序列,但没有功能性启动子,为沉默基因。根据大肠杆菌T7表达载体pET21b克隆位点和cry2Ab3开放阅读框架(ORF)两端序列,设计合成一对特异引物L2ab5和L2ab3,高保真PCR扩增获得cry2Ab3完整ORF,经酶切、连接构建了重组表达质粒pET2Ab3。表达质粒导入大肠杆菌BL21(DE3),IPTG诱导后,SDSPAGE电泳证实了cry2Ab3的表达。生物测定显示诱导培养物对棉铃虫初孵幼虫和小菜蛾二龄幼虫具有杀虫活性,能明显抑制二化螟二龄幼虫生长,但对甜菜夜蛾和玉米螟没有明显活性。进一步提取Cry2Ab3蛋白,生测结果表明其对棉铃虫LC50为32.55μg/g。     

苏云金芽胞杆菌cry1A启动子上游区缺失体的研究

利用ＰＣＲ方法,设计相应的扩增引物,以ｐＨＴ／２７２ｕｐ－ｐＳＧＮＵ质粒ＤＮＡ为模板,扩增得到缺失相应序列的上游片段,然后将其连接到ｐＨＴ－ｐＳＧＭＵ穿梭载体的ＢｒＩ－ｌａｃＺ融合基因表达的影响。结果表明,缺失反向重复区,保留弯曲区（ＰＣＲＡ）,对ＢｔＩ－ｌａｃＺ融合基因在库斯塔克亚种菌株８０－２１中的表达与完整上游区的增强作用相一致,而在鲇泽亚种中,ＢｔＩ－ｌａｃＺ基因表达量明显比未缺失体低。这     

Isolation and characterization of a novel Bacillus thuringiensis strain expressing a novel crystal protein with cytocidal activity against human cancer cells

AIMS: To characterize a novel, unusual, Bacillus thuringiensis strain, to clone its Cry gene and determine the spectrum of action of the encoded Cry protein. METHODS AND RESULTS: The B. thuringiensis strain, referred to as M15, was isolated from dead two-spotted spider mites (Tetranychus urticae Koch; Arthropoda: Arachnida: Tetranychidae). It is an autoagglutination-positive strain and is therefore non-serotypeable. A sporulated culture produces a roughly spherical parasporal inclusion body, the crystal, tightly coupled to the spore. Although the crystal appears to be composed of at least two major polypeptides of 86 and 79 kDa as estimated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, Southern hybridization indicates that the corresponding crystal protein gene is likely present in only one copy. The crystal protein gene was cloned and, based on nucleotide sequence homology with an orthologous cry31Aa1 gene, assigned the name cry31Aa2. Although initially isolated from spider mites, B. thuringiensis M15 is non-toxic to spider mites and it does not produce the wide spectrum beta-exotoxin. Assays on mammalian cells, however, reveal that Cry31Aa2, when cleaved with trypsin, is cytocidal to some human cancer cells but not to normal human cells. No cytocidal activity was induced after protease treatment of Cry31Aa2 with either chymotrypsin or proteinase K. Trypsin, chymotrypsin and proteinase K cleavage sites were determined. CONCLUSIONS: The B. thuringiensis strain M15 exhibits specific cytocidal activities against some human cancer cells. Significance and Impact of the Study: This study raises questions as to the actual role of this bacterial strain and its crystal protein in the environment. It may be possible to further develop the Cry31Aa2 protein to target specific human cancer cells.     

苏云金杆菌以色列亚种杀蚊蛋白Cyt1Aa在离中不粘柄菌中的表达

在蚊幼虫生活水域里的离中不粘柄菌(Asticcacaulis excentricus,Ae)中已成功表达苏云金芽孢杆菌以色列亚种(Bacillus thuringiensis subsp.israelensis,Bti)杀蚊蛋白基因cry11Aa的基础上,将另一Bti杀蚊蛋白基因cyt1Aa转化入Ae中表达。构建并转化了分别单独含有cyt1Aa基因、及同时含有cry11Aa基因的表达质粒pSODCyt20和pSODCryCyt20,蛋白免疫杂交检测相应的Ae重组子分别表达产生了Cyt1Aa和Cry11Aa蛋白。为了探究Ae(pSODCryCyt20)重组子不能表达cyt1Aa的原因,提取了重组子总RNA、并与同是革兰氏染色阴性的大肠杆菌的总RNA比较,结果显示两者RNA系统显著不同,推测Ae中多个外源基因的表达,可能要求每个基因必需一个启动子。     

云南草地贪夜蛾田间种群对Bt毒素的抗性基因频率监测研究

转基因Bt作物的广泛应用和产业化推广不仅有效遏制了虫害的大规模暴发,显著减少了化学农药的施用量,更重要的是缓解了由此带来的农药残留及环境污染问题。为了监测我国云南地区草地贪夜蛾Spodoptera frugiperda田间种群对Bt毒素的抗性,本研究以云南寻甸地区草地贪夜蛾田间种群为研究对象,通过F2代结合诊断剂量法对草地贪夜蛾田间种群进行抗性监测,系统评估了该地区草地贪夜蛾对Bt毒素的抗性水平。检测结果显示,仅发现3个单雌系对Cry1Ab具有低频抗性（抗性等位基因频率为0.006）,而对Vip3Aa仍保持高度敏感。本研究表明云南地区草地贪夜蛾种群尚未形成明显抗性,这为该区域Bt转基因作物的可持续推广提供了重要科学依据,并建议继续开展长期监测和抗性治理策略研究。     

苏云金芽孢杆菌分子伴侣串联基因p19-p29的克隆和表达载体的构建

根据已知序列设计一对PCR引物(ORF5S,ORF3N),可从cry2Aa或cry2Ac操纵子中扩增出包含串联分子伴侣基因p19p29的DNA片段,预期大小分别为16kb和20kb。对150株苏云金芽孢杆菌菌株进行PCR检测,从26株中获得了大小为16kb的扩增片段,但未获得20kb的片段。这表明cry2Aa型操纵子p19p29基因存在较广泛,而cry2Ac型较罕见。将来自Y2菌株的16kb片段回收,通过一系列亚克隆,最终构建成一个含有p19p29串联基因的Bt表达载体,为进一步研究p19p29串联基因的功能奠定了基础。     

Expression and crystallization of a Cry3Aa–Cry1Ac chimerical proteinof Bacillus thuringiensis

The insecticidal Cry1 proteins of Bacillus thuringiensis form a typical bipyramidal parasporal crystal and their protoxins contain a highly conserved C-terminal region. A chimerical gene was constructed with the coding regions of the Cry3Aa protein's toxic domain, and of the Cry1Ac protoxin's C-terminal fragment. This chimerical construction expressed a truncated (70kDa) protein in the acrystalliferous strain 4Q7 of B. thuringiensis, assembled in spherical to amorphous parasporal crystals. This protein was recognized only by antibodies raised against the Cry3Aa protein. When the protease-deficient mutant BL21 of Escherichia coli was transformed with the same chimerical construction, a complete (140kDa) chimerical protein was expressed. However, the formation of a crystalline inclusion was unclear. This protein was recognized by antibodies raised against the proteins Cry1Ac and Cry3Aa. Both chimerical proteins showed toxicity against larvae of Leptinotarsa texana, being much more active when expressed truncated in B. thuringiensis. These results suggest that the formation of bipyramidal crystals requires more than just the presence of the C-terminal region of Cryl protoxins. They also suggest that proteolysis plays an important role during the post-translational processing of Cry proteins.     

Expression of chitinase A (chiA) gene from a local isolate of Serratia marcescens in Coleoptera-specific Bacillus thuringiensis

Aims:  The present study focused on cloning and expression of chiA gene from a highly chitinolytic local isolate of Serratia marcescens in an anti-Coleopteran Bacillus thuringiensis and comparison of the characteristics of the native and recombinant ChiAs.
Methods and Results:  chiA gene from Ser . marcescens was cloned, sequenced and compared with the previously cloned chiA genes. chiA gene was PCR cloned and expressed in anti-Coleopteran B. thuringiensis strain 3023 as verified by Western blot analysis. Specific ChiA activity of the recombinant B. thuringiensis (strain 3023-SCHI) reached its highest level at 21st hour of growth (16·93 U mg⁻¹), which was 5·2- and 1·3-fold higher than that of its parental strain and Ser . marcescens , respectively. Temperature and pH effects on native and recombinant ChiAs were next determined. The recombinant plasmid was quite stable over 240 generations.
Conclusions:  Serratia marcescens ChiA was heterologously expressed in an anti-Coleopteran B. thuringiensis at levels even higher than that produced by the source organism.
Significance and Impact of the Study:  Bacillus thuringiensis 3023-SCHI co-expressing anti-Coleopteran Cry3Aa protein and Ser . marcescens chitinase offers a viable alternative to the use of chitinolytic microbes/enzymes in combination with entamopathogenic bacteria for an increased potency because of synergistic interaction between them.