苏云金芽胞杆菌YBT1520杀虫晶体蛋白基因的属性

通过Southern杂交发现高毒力苏云金芽胞杆菌(\%Bacillus thuringiensis)\% YBT1520菌株含有两个杀虫晶体蛋白基因片段,其5’末端所在HindⅢ片段分别为68kb和46kb,它们对应的基因分别命名为cry218和cry46。经PCR鉴定,该菌含有cry1Aa\,cry1Ab和cry1Ac基因,以及cry2基因,其中cry218属于cry1Ac。分析了cry218基因4190bp的核苷酸序列,在杀虫晶体蛋白基因分类系统中被命名为cry1Ac10。结合Southern杂交和PCR结果可判断3个cry1A基因的拷贝数不同,其中cry1Ac拷贝数最高,YBT1520菌株与其它库斯塔克亚种的杀虫晶体蛋白基因所在限制性内切酶位置明显不同。     

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。     

31株苏云金芽孢杆菌杀虫晶体蛋白基因型鉴定及表达产物研究

利用已建立的苏云金芽孢杆菌cry基因的PCRRFLP鉴定体系,鉴定了31株Bt菌株的cry基因类型,并进行了SDSPAGE分析和杀虫生物活性测定。研究表明：25株含cry1基因,表达蛋白130～150kD;其中16株含有对鞘翅目和鳞翅目害虫皆有活性的cry1I基因,其表达蛋白为81kD;15株同时含有cry1和cry2基因(13株表达蛋白约为60kD);10株含有未知待定基因;6株不含所鉴定的cry基因(其中2株有表达产物)。室内生物测定表明：cry1、cry2基因表达的菌株对鳞翅目害虫具有高杀虫活性,7株对舞毒蛾和膜翅目——杨叶蜂幼虫具有较高杀虫活性;含有cry1Aa\,cry1Ac\,cry2或cry1Ab\,cry1Ac\,cry2基因组合的菌株对棉铃虫幼虫均显示杀虫活性,其中6、12、30号菌株毒力最强。不含上述cry基因的菌株均无杀虫活性。以上结果证明,通过cry基因类型鉴定和表达产物的SDSPAGE分析可以预测菌株的杀虫活性。     

苏云金芽孢杆菌科默尔亚种15A3株的cry基因分析及杀虫特性

筛选的苏云金芽孢杆菌野生菌株15A3经鉴定属血清H21型科默尔亚种。用PCR及RFLP方法对其cry1类基因分析证明其含有cry1Aa,\%cry1\%Ac,\%cry1\%Ca,\%cry1\%D,\%cry1\%I及cry2六种cry基因,其cry1A基因N末端145kb片段与已发表的序列有差异。表达晶体蛋白质的分子量分别为130,79,70,65,51和45kD。对家蝇致畸实验证明其不含β外毒素。发酵液对棉铃虫,甜菜夜蛾,小菜蛾及美国白蛾均具较高的毒力。证明野生的苏云金芽孢杆菌资源中也有具国外工程菌所特有的高效杀虫晶体蛋白基因组合的优良菌株。     

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。     

假单胞菌M18rsmA-突变株的构建及其对Plt和PCA合成的区别性调控作用

假单胞菌(Pseudomonas sp.)M18是促进植物生长的根际细菌,能产生吩嗪1羧酸（PCA）和藤黄绿菌素（Plt）两种不同的抗生素抑制植物病原菌,保护植物免受病害。运用PCR方法,从M18基因组中,扩增出rsmA基因部分片段,并以该片段为探针,从M18的基因组柯斯文库中筛出阳性克隆,切取带有rsmA基因及两侧序列的15kb片段,中间插入编码Kmr的DNA片段,获得rsmA-体外突变体。运用同源重组剔除技术,构建了M18菌株的rsmA突变株M18R-。突变株M18R-生物合成Plt的能力比野生型M18提高4倍,但是,PCA产量仅为野生型的20%。研究结果表明,全局性调控基因rsmA可能通过不同的机制区别性地影响Plt和PCA的生物合成。     

苏云金芽孢杆菌以色列亚种P19基因的初步研究

以含有P19和cyt1A基因的以色列亚种72MD质粒的9 7kb HindⅢ片段为模板进行PCR扩增,分别获得Ｐ19基因和cyt1A基因片段。与表达 载体pUHE24连接转化大肠杆菌XL１,获得3个克隆株。LZ19含有P19基因;pLZcyt1A含 有cyt1A基因;LZ19A含有P19和cyt1A两个基因。利用cyt1A蛋白质可使大肠杆菌细胞致 死的特性,在IPTG诱导下,测定了各克隆基因表达对大肠杆菌有致死作用;pLZ19A对大肠杆菌的起始致死作用明显快于pLZcyt1A,这种现象可能是P19基因促进cyt1A基因高表达的结果。     

大肠杆菌\%otsA\%基因的克隆和表达

用PCR方法扩增了15kb的otsA基因片段,将该片段连接到多拷贝克隆载体后转化otsBA缺失和otsA缺陷的大肠杆菌菌株,使转化株重新获得otsA基因功能。生长曲线表明转化株在高渗培养基中生长良好,薄层层析法(TLC)检测海藻糖实验说明转化株细胞经诱导后合成海藻糖,otsA基因的克隆和表达为赋予转基因植物抗高渗、耐干旱能力提供了实验依据和材料。     

苏云金芽孢杆菌4.0718菌株的杀虫晶体蛋白基因分析

根据苏云金杆菌(Bacillus thuringiensis)cry1、cry2和cry3型基因的保守区分别设计了3对通用引物Un1(d)/Un1?、Un2(d)/Un2?和Un3(d)/Un3?,以Bt4.0718菌株质粒DNA为模板进行PCR扩增,通过扩增产物片段的分子量大小来确定该菌株所含有的杀虫晶体蛋白基因类型。随后根据上述3类cry基因的高变区设计特异引物再次进行PCR鉴定。结果表明:Bt4.0718菌株含有cry1Aa、cry1Ab、cry1Ac、cry1Cb、cry2Ac和新基因cry4.5等6种基因类型。这一结果为利用该菌株构建高效广谱杀虫工程菌提供了客观依据。     

应用膜反向斑点杂交技术快速检测结核分支杆菌耐乙胺丁醇基因型的研究

应用膜反向斑点杂交技术快速检测结核分支杆菌对乙胺丁醇（EMB）耐药性。设计与合成用于检测结核分支杆菌耐EMB基因embB的寡核苷酸探针,点于硝酸纤维素膜上,与结核分支杆菌临床分离株生物素标记的聚合酶链反应（PCR）产物进行反向斑点杂交,并与PCR单链构象多态性（PCRSSCP）和PCR直接测序（PCRDS）结果比较。对81株结核分支杆菌临床分离株进行分析,31株EMB敏感株中,26株embB基因的SSCP图谱、膜反向斑点杂交结果与标准株(H37Rv)完全相同;其余5株SSCP图谱出现泳动变位,其中3株E1b杂交阳性,PCRDS分析为embB基因306位密码子ATG→GTG突变;2株E1d杂交阳性,PCRDS分析为embB基因306位密码子ATG→ATA突变。50株耐EMB菌株中,24株PCRSSCP 图谱与标准菌株相同,E1杂交阳性;26株PCRSSCP图谱出现泳动变位,其中18株E1b杂交阳性,2株E1c杂交阳性,5株E1d杂交阳性,1株E1e杂交阳性,未发现E1f杂交阳性,与PCRSSCP、PCRDS分析结果一致。突变检出率为52%。 膜反向斑点杂交技术可能成为检测部分结核分支杆菌乙胺丁醇耐药基因型简便、快速的方法。     

对鳞翅目害虫高毒力的Bt cry1Aa基因的分离克隆及表达

Bt菌Ly30株是我国自行分离的对多种害虫具有高毒力的苏云金芽孢杆菌,经CAPS(cleaved amplified polymorphic sequences)系统鉴定,它含有cry1Aa基因。以全长基因PCR产物的粘端定向克隆的方法, 设计一对特异引物,分别引入NcoⅠ和BamHⅠ/NcoⅠ酶切位点。以Ly30质粒DNA为模板扩增cry1Aa全长基因,与表达载体Pkk233-2相应酶切产物连接,转化大肠杆菌,获得含有cry1Aa基因重组质粒pKKLy1Aa。完成了该基因的亚克隆和序列测定,结果表明,该基因的编码区为3 531 bp,编码蛋白分子量为133.2kD,含1.176个氨基酸,等电点Pi为4.99。该基因序列已在GenBank中登记注册,登录号为AF384211,并被国际Bt杀虫晶体蛋白基因命名委员会正式命名为cry1Aa12。对重组菌KKLy1Aa进行诱导表达研究。在0.6 mmol/L IPTG、37℃、8 h培养条件下,该基因获得高效表达,SDS-PAGE电泳检测到明显的133.2 kD蛋白带。室内生测结果表明,Cry1Aa蛋白对不同的小菜蛾品系均有较高的杀虫活性,其LC₅₀值分别为0.203 μg/mL和0.554 μg/mL。     

5种中国苏云金芽孢杆菌的伴孢 晶体蛋白基因分析

利用聚合酶联反应(PCR)和聚丙烯酰胺凝胶电泳(SDS-PAGE)技术分析了5种中国苏云金杆菌制剂菌株的伴孢晶体蛋白及其基因组成。结果发现,5种菌株均含有cry1Aa和/或c和/或d和/或b基因,只有Bt+Virus菌株含有cry1Ab基因,cry1A基因编码的伴孢晶体蛋白分子量约为130 kD;仅有JS-Bt C菌株含有cry1B基因,其编码的伴孢晶体蛋白分子量约为138 kD;除HB Bt C菌株外,其余4个菌株均含有cry2Aa和/或b基因,这类基因编码分子量为70 kD的伴孢晶体蛋白;所有5个菌株都含有cry1I基因,其编码的伴孢晶体蛋白分子量应为81.2 kD,但实验中未曾检测到cry1I基因的表达;所有的菌株都不含有cry1C和cry1D基因。     

Expression of a cry2Aa gene in an acrystalliferous Bacillus thuringiensis strain and toxicity of Cry2Aa against Helicoverpa armigera

In the recent past research has been mainly focused on the expression of cry1 genes of Bacillus thuringiensis (Bt) to engineer lepidopteran insect resistance in plants. Search for structurally different toxins is necessary for the management of resistance development in insects. The intact cry2Aa operon (3.95 kb) of a new isolate of Bt, 47-8, was subcloned into a Bt shuttle vector, pHT3101 (6.7 kb). Recombinant pHT3101 containing the cry2Aa operon of Bt strain 47-8 was named as pTN2Aa and used to transform acrystalliferous Bt strain 4Q7 by electroporation. Phase contrast microscopic observation revealed the presence of crystalline inclusions in the transformants of Bt strain 4Q7 harbouring pTN2Aa. SDS–PAGE of a spore–crystal mixture prepared from transformants of acrystalliferous Bt strain 4Q7 harbouring pTN2Aa showed a single band of about 65 kDa alone confirming the expression of the cloned cry2Aa. Bioassay with Helicoverpa armigera showed 71.4% mortality caused by the proteins encoded by the newly cloned cry2Aa gene (at the concentration of 2.3 g/l) on the seventh day and all the survivors that escaped from Cry2Aa toxicity showed severe (81–99%) inhibition in larval growth.     

Distribution and diversity of cry genes in native strains of Bacillus thuringiensis obtained from different ecosystems from Colombia

Colombia is a tropical country located at the north of South America. It is considered to be one of the most important countries in terms of its biodiversity worldwide. One hundred and eight soil samples obtained from agricultural crops and wild ecosystems were evaluated in terms of the presence of Bacillus thuringiensis (Bt) native strains. One hundred and eight different Bt strains were isolated and characterized by the presence of crystal proteins by SDS-PAGE and a multiplex PCR with general and specific primers for cry1 and cry3, cry7, and cry8 gene detection. Most of the Bt strains (73%) reacted with the cry1 general primers; 27.8% of the Bt strains reacted with cry3, cry7, and cry8 general primers and 17.8% of strains did not react with any of these two sets of primers. Thirty different PCR profiles were found in the strains with cry1 genes when they were analyzed with specific primers (cry1A to cry1F). A high frequency of joint occurrence was observed for cry1Aa/cry1Ab, cry1Aa/cry1Ac, cry1Ab/cry1Ac, and cry1C/cry1D genes with a Pearson coefficient of 0.88, 0.74, 0.76, and 0.87, respectively. Other distinctive characteristics were found in the Colombian collection as the presence of 22.2% of native strains which presented, at the same time, lepidopteran and coleopteran active genes. Interesting relations were found as well between the cry gene distribution and the geographical areas sampled. Finally, some strains with moderate to high biopesticide activity against Spodoptera frugiperda (Lepidoptera) and Premnotrypes vorax (Coleoptera) insects were identified, this being important to explore future microbial strategies for the control of these crop pests in the region.     

Characterization of <Emphasis Type="Italic">Bacillus thuringiensis</Emphasis> Strain DOR4 Toxic to Castor Semilooper <Emphasis Type="Italic">Achaea janata</Emphasis>: Proteolytic Processing and Binding of Toxins to Receptors

We have isolated a strain of Bacillus thuringiensis (Bt) from Indian soil samples that was shown to be toxic to Achaea janata larvae. The isolate, named B. thuringiensis DOR4, serotypically identified with the standard subspecies kurstaki (H3a3b3c) and produced bipyramidal inclusions along with an amorphous type. Although the plasmid pattern of DOR4 was different from that of the reference strain, a crystal protein profile showed the presence of two major bands (130 and 65 kDa) similar to those of Bt subsp. kurstaki HD-1. To verify the cry gene content of DOR4, triplex PCR analysis was performed; it showed amplification of the cry1C gene in addition to cry1Aa, cry1Ac, cry2A, and cry2B genes, but not the cry1Ab gene. RT-PCR analysis showed the expression of cry1Aa and cry1Ac genes. In vitro proteolysis of DOR4 protoxin with midgut extract generated products of different sizes. Zymogram analysis of DOR4 protoxin as substrate pointed to a number of distinct proteases that were responsible for activation of protoxins. Furthermore, toxin overlay analysis revealed the presence of multiple toxin-binding proteins in midgut epithelium. Based on all these characterizations, we suggest that the Bt DOR4 strain can be exploited for an A. janata control program.     

Evaluating the Insecticidal Genes and Their Expressed Products in Bacillus thuringiensis Strains by Combining PCR with Mass Spectrometry

By a combination of PCR and mass spectrometry, a total of five cry genes (cry1Aa, cry1Ac, cry2Aa, cry2Ab, and cry1Ia) were detected in genomic DNA from the wild-type Bacillus thuringiensis strain 4.0718, and three protoxins (Cry1Aa, Cry1Ac, and Cry2Aa) were identified in the strain's parasporal crystals. These results indicated that this complementary method may be useful in evaluating B. thuringiensis strains at both the gene and protein levels.     

Strategy for amplification and sequencing of insecticidal <Emphasis Type="Italic">cry1A</Emphasis> genes from <Emphasis Type="Italic">Bacillus thuringiensis</Emphasis>

A feasible and fully described strategy, with a detailed list of primers, for amplifying, cloning and sequencing known and potentially novel cry1A genes harboured by a Bacillus thuringiensis strain was successfully established. Based on the analysis of conserved regions of the cry1A genes, the 1AF and 1UR oligonucleotide primers were designed to amplify the whole open reading frame of these genes. The PCR products obtained revealed the successful amplification of cry1A genes from 13 B. thuringiensis strains. These bacteria were previously known to harbour at least one cry1A gene. An Argentinean B. thuringiensis isolate INTA Mo1-12 was randomly chosen for cloning and sequencing of cry1A genes by using a primer set developed in this study. Both nucleotide and amino acid sequences similarity analysis revealed that cry1Aa and cry1Ac from B. thuringiensis INTA Mo1-12 are new natural variants, showing several differences with the other known cry1A subclasses. These genes were named by the B. thuringiensis Pesticidal Crystal Protein Nomenclature Committee as cry1Aa15 and cry1Ac21 respectively.     

二化螟钙黏蛋白CAD1的原核表达及与Cry1Ac、Cry2Aa蛋白的结合

【目的】二化螟是水稻的重要害虫之一,钙黏蛋白(cadherin,CAD)是一类重要的Bt杀虫蛋白受体,在获得二化螟钙黏蛋白基因(Cs CAD1)的基础上,明确Cs CAD1蛋白与Cry1Ac和Cry2Aa蛋白的结合能力。【方法】利用PCR技术克隆Cs CAD1基因片段,将构建的p ET-28a-(+)-Cs CAD1重组质粒转入原核表达菌株BL21(DE3)中,IPTG诱导表达。目的蛋白经Ni柱亲和纯化后SDS-PAGE电泳检测,利用western blot和ligand blot技术分析其与Cry1Ac和Cry2Aa蛋白的结合能力。【结果】重组载体可在表达菌株BL21中表达一个约44 ku的蛋白,原核表达载体构建成功。SDS-PAGE显示该蛋白条带单一,且纯度较好。Ni柱亲和层析纯化该目的蛋白后进行Ligand blot分析,结果显示Cs CAD1重组蛋白可以与Cry1Ac和Cry2Aa蛋白结合。【结论】Cs CAD1蛋白可以与Cry1Ac和Cry2Aa蛋白结合,是潜在的Cry蛋白受体,所得结果有助于阐明Cry1Ac和Cry2Aa蛋白对二化螟的作用机制。