人乳头瘤病毒31和33亚型L1基因导入水稻及转基因植株的鉴定

目的:结合水稻胚乳生物反应器的优点,将人乳头瘤病毒(HPV)31、33亚型的L1蛋白编码基因导入水稻,构建HPV31 L1、HPV33 L1植物表达载体,最终实现其在水稻胚乳表达系统中的表达。方法:利用生物信息学方法分析并优化合成HPV31及HPV33 L1蛋白编码基因,将其重组于中间载体pMP3和植物表达载体pCAMBIA1300中,分别构建植物双元表达载体pCAMBIA1300-pMP3-HPV-31 L1和pCAMBIA1300-pMP3-HPV-33 L1,采用遗传转化法经根癌农杆菌介导转化水稻TP309种子的愈伤组织,经共培养、潮霉素筛选和分化再生,获得潮霉素抗性植株。结果和结论:构建了HPV31 L1、HPV33 L1的植物表达载体,经根癌农杆菌介导转化水稻TP309种子的愈伤组织,获得转基因植株。     

金针菇G蛋白偶联受体基因的CRISPR/Cas9基因组编辑载体构建及转化研究

通过氨基酸同源比对（Blast P）以及金针菇冷诱导前后菌丝阶段和原基阶段的转录组数据分析,获得了金针菇中的两个假定G蛋白偶联受体基因Fvgpcr1、Fvgpcr2。对获得的金针菇假定G蛋白偶联受体基因Fvgpcr1、Fvgpcr2构建了基因组编辑（CRISPR/Cas9）的pCAMBIA0390-hph-Fvcas9-Fvgpcr1- sgRNA1/sgRNA2、pCAMBIA0390-hph-Fvcas9-Fvgpcr2-sgRNA1/sgRNA2等4个表达载体。通过农杆菌介导（ATMT）将表达载体pCAMBIA0390-hph-Fvcas9-Fvgpcr-sgRNA转化金针菇菌丝体,采用潮霉素和头孢毒素低浓度初筛和高浓度复筛,经两段筛选获得金针菇拟转化子。经对拟转化子进行PCR鉴定、RT-qPCR检测和Western杂交验证,结果显示表达载体pCAMBIA0390-hph-Fvcas9-Fvgpcr-sgRNA成功整合进金针菇基因组中,FvCas9蛋白正常表达,但未得到Fvgpcr基因敲除突变体。本研究利用农杆菌介导转化法在金针菇中构建了CRISPR/Cas9敲除体系,对后续目标基因的敲除有着重要意义。     

农杆菌Ti质粒的改造及其衍生的质粒载体

Ti质粒是农杆菌介导基因转化的重要部件,它是农杆菌染色体外的遗传物质。野生型Ti 质粒虽然是植物基因工程的一种天然载体,但把它用作常规的克隆载体却存在4点缺陷,为了使Ti质粒适于基因工程的需要,必须对其进行改造。改造Ti质粒方法目前有:共整合载体和双元载体。     

根癌农杆菌介导里氏木霉转化体系的建立和条件优化

目的:采用根癌农杆菌介导的转化方法实现丝状真菌里氏木霉的遗传转化,并优化转化条件.方法:构建含潮霉素抗性基因(hph)的双元载体pCAM-hph后,转化根癌农杆菌LBA4404获得转化菌株.将根癌农杆菌的转化菌株和里氏木霉的分生孢子共培养后在含100μg/mL潮霉素的抗性平板上筛选里氏木霉转化子,并采用PCR扩增和序列测定对转化子中的插入片段进行了分析.结果:使用根癌农杆菌介导的转化方法转化里氏木霉,每106个分生孢子可获得25.8个转化子.最佳的转化条件为:农杆菌初始浓度为OD660约为0.8,孢子数为106个,共培养时间为48h,pH为5.0～5.5,培养温度为28℃.结论:建立了根癌农杆菌介导的里氏木霉转化方法,并获得了最佳的转化条件.     

农杆菌介导的水稻双载体共转化法中部分影响因素的研究

以T-DNA区分别只含有潮霉素选择标记基因(HPT)和GUS报告基因的双元载体pCAMBIA1300和pCAMBIA0301用于农杆菌介导的水稻共转化试验。根据经农杆菌浸染并共培养3d后水稻愈伤组织中的GUS瞬间表达情况及其稳定共转化率,测定了不同农杆菌菌株搭配及其不同浓度配比对共转化效率的影响。结果表明,在两种农杆菌菌液浓度比为1:1的情况下,农杆菌EHA105/pCAMBIA1300与EHA105/pCAMBIA0301组合共转化水稻的效率要高于其他菌株的组合;在以农杆菌EHA105/pCAMBIA1300与EHA105/pCAMBIA0301进行共转化时,两种菌液浓度比为1:2时共转化效率最高。     

根癌农杆菌介导转化川草二号老芒麦胚性愈伤组织

以川草二号老芒麦成熟种子为外植体,经过对培养基的筛选和培养条件优化,建立了愈伤组织再生系统。转化载体为pCAMBIA1304质粒,其T—DNA上携有潮霉素抗性基因（hptII）和类产碱假单胞菌杀虫蛋白基因（ppIP）,经根癌农杆菌EHA105介导转化结构致窑、颗粒状、黄白色的胚性愈伤组织。通过潮霉素筛选和对抗性植株进行分子检测,获得了转基因植株。同时优化了农杆菌遗传基因转化的参数,建立了农杆菌介导的川草二号老芒麦程序化转基因方案。     

申克孢子丝菌STE20基因RNA干扰菌株的构建方法

目的 构建真菌通用的RNA干扰载体,以广泛用在多种真菌基因干扰的研究中。方法 利用现有的植物双元表达载体进行改造,将pBlueScriptⅡ的多克隆位点(MCS)酶切下来构建干扰载体;为使载体适于农杆菌转化,加入T-DNA边界重复序列;为便于转化后的筛选,将潮霉素抗性基因构建到干扰载体上。改造以前的干扰载体仅适于青霉菌属的RNA干扰,为扩大干扰范围,扩增pSilent-1质粒中的真菌通用启动子Ptrpc,间隔序列和终止子Ttrpc,并引入潮霉素抗性基因,使其在间隔序列两侧加上目的基因的正反向干扰序列以构建载体。结果 利用本实验构建的载体PCB309-PSUST及优化的反应体系成功实现了对孢子丝菌STE20基因的有效干扰,操作简便、转化效率高、转化子稳定。结论 成功构建的这种载体适于根癌农杆菌介导,能够对多种丝状真菌基因进行RNA干扰研究用。     

根癌农杆菌介导的灰葡萄孢菌遗传转化研究

以pCAMBIA1300-N载体为骨架, 成功构建了以绿色荧光蛋白(gfp)为报告基因, 潮霉素(hph)为抗性筛选标记的载体pKPG, 并利用根癌农杆菌介导转化系统, 成功获得了能表达绿色荧光蛋白的重组灰葡萄孢菌。通过PCR检测转化子的绿色荧光蛋白基因和潮霉素抗性表达框, 观察菌丝和分生孢子的荧光表型, 以及gfp基因的Southern杂交验证, 结果表明：被测转化子基因组中均成功整合了目的基因片段。     

根癌农杆菌介导的巨大口蘑遗传转化体系的构建

以巨大口蘑菌丝为受体材料,利用含有双元质粒plasmid4的根癌农杆菌EHA105介导,首次成功建立了巨大口蘑的遗传转化体系。通过潮霉素抗性筛选、PCR鉴定和绿色荧光蛋白的检测,表明潮霉素抗性基因（Hyg）已经整合到巨大口蘑基因组中,增强型绿色荧光蛋白基因（eGFP）在巨大口蘑菌丝中获得表达,并能够稳定遗传。本研究建立了农杆菌介导的巨大口蘑遗传转化体系,为今后巨大口蘑的基因功能研究奠定了基础。     

蒙古冰草MwLEA3基因植物表达载体的构建

以植物双元表达载体pCAMBIA2300为基础,设计分别带有酶切位点XbaI和PstI的一对引物,从克隆载体pGM-T-MwLEA3中扩增到目的基因MwLEA3。用XbaI和PstI双酶切该目的基因及表达载体pCAMBIA2300,回收后利用T4DNA连接酶连接,获得植物表达载体pCAM-MwLEA3。通过冻融法将所获得的植物表达载体重组质粒导入根癌农杆菌LBA4404菌株中,为该基因的功能鉴定及通过农杆菌介导法将MwLEA3基因导入植物提高相关抗性奠定了基础。     

利用转基因烟草确定AtELHYPRP2蛋白对赤霉菌的抗性及其亚细胞定位特征

采用遗传转化技术获得了整合有拟南芥AtELHYPRP2(EARLI1-LIKE HYBRID PROLINE-RICH PROTEIN 2,AT4G12500)基因的转基因烟草株系,研究了该基因编码蛋白对真菌病原体赤霉菌的抗性及其亚细胞定位特征。以拟南芥Col-0生态型基因组DNA为模板,通过聚合酶链反应扩增AtELHYPRP2基因编码序列,经限制性酶切后连接至pCAMBIA1302载体,构建产生pCAMBIA1302-AtELHYPRP2-GFP融合表达载体。进一步采用农杆菌LBA4404转化烟草叶片外植体,筛选得到转基因烟草植株。RT-PCR、Western blotting印迹分析结果显示,AtELHYPRP2基因在转化体中可以有效表达。激光共聚焦显微观察发现AtELHYPRP2-GFP融合蛋白产生的绿色荧光与碘化丙啶染色后产生的红色荧光能够重合,说明AtELHYPRP2蛋白定位于细胞表面。真菌侵染实验结果显示,组成性表达AtELHYPRP2基因能够增强烟草对赤霉菌的抗性,被侵染部位有明显的H2O2积累。转基因烟草植株中PR1基因的本底表达水平比野生型高,PR1和PR5基因的系统表达水平比野生型高,说明AtELHYPRP2基因可能在SAR反应中具有一定的作用。     

Agrobacterium tumefaciens mediated transformation of marine microalgae Schizochytrium

Schizochytrium was a known docosahexaenoic acid producing marine microalgae. In this study, we have developed a novel transformation approach of Schizochytrium using the Agrobacterium tumefaciens (A. tumefaciens) binary vector system. After co-cultivation of Schizochytrium protoplasts with A. tumefaciens harboring pCAMBIA2301 containing the neomycin phosphotransferase II (NPT II) gene as the selectable marker which confers resistance to G418, the Schizochytrium transformants were successfully obtained on the G418-containing plates. The integration and expression of the transgenes were confirmed by PCR analysis and GUS activity assay. To further validate the transformation system, pCAMBIA2301-EGFP containing the egfp gene was introduced into Schizochytrium. The following results demonstrated that the exogenous egfp gene has been successfully incorporated into the genome of Schizochytrium. In addition, the introduced egfp gene expressed efficiently according to the Western blot and fluorescence assay results. More importantly, the majority of the transformants displayed similar biomass and fatty acid production comparing with the wild type strain. Our results demonstrated that exogenous genes could be expressed efficiently in transgenic Schizochytrium, suggesting that genetically engineered Schizochytrium could be explored by this system.     

根癌农杆菌介导大花蕙兰遗传转化的研究

以大花蕙兰原球茎(PLBs)为外植体,采用EHA105和LBA4404 2种根癌农杆菌菌株与pCAMBIA1301质粒构建工程菌介导,以建立大花蕙兰遗传转化体系,并比较不同受体处理方式、菌液浓度和侵染方式等对大花蕙兰转化的影响.结果表明:(1)以切成3 mm左右的PLBs小块作为受体材料,用OD600值为0.6的LBA4404根癌农杆菌菌株,并用MS+1.0 mg/L BA+200μmol/L AS(乙酰丁香酮)的液体培养基将菌液等体积稀释侵染,转化率可达62.5%.(2)大花蕙兰对潮霉素(Hyg)十分敏感,5 mg/L Hyg对转化后的PLBs有较好的筛选效果,筛选后最高成活率为13.0%.(3)PCR检测初步证明,通过根癌农杆菌介导的方法获得了2株转基因大花蕙兰植株.     

Additional virulence genes and sonication enhance <Emphasis Type="Italic">Agrobacterium tumefaciens</Emphasis>-mediated loblolly pine transformation

Additional virulence (vir) genes in Agrobacterium tumefaciens and sonication were investigated for their impact on transformation efficiency in loblolly pine (Pinus taeda L.). Mature zygotic embryos of loblolly pine were co-cultivated with disarmed A. tumefaciens strain EHA105 containing either plasmid vector pCAMBIA1301 or vector pCAMBIA1301 with an additional 15.8-kb fragment carrying extra copies of the Vir B, Vir C, and Vir G regions from the supervirulent plasmid pTOK47. pCAMBIA1301 contains hygromycin resistance and the beta-glucuronidase (GUS) reporter gene. Expression of GUS was observed after 3-6 days of co-cultivation, with peak expression at approximately 21 days. The highest numbers of GUS-expressing areas were visible up to 21 days after co-cultivation, declining rapidly thereafter. Both transient and stable transformation efficiencies increased when the explants were sonicated before co-cultivation and/or the additional virB, virC, and virG genes were included with the pCAMBIA1301 plasmid T-DNA. Use of the plasmid with additional vir genes and sonication dramatically enhanced the efficiency of Agrobacterium-mediated gene transfer not only in transient expression but also in the recovery of hygromycin-resistant lines. Stably transformed cultures and transgenic plants were produced from embryos transformed with A. tumefaciens EHA105 carrying pCAMBIA1301 or pCAMBIA1301+pTOK47 in the three families of loblolly pine. The presence of the introduced GUS and hygromycin phosphotransferase genes in the transgenic plants was confirmed by polymerase chain reaction and Southern hybridization analyses.     

Agrobacterium tumefaciens-mediated transformation of the plant pathogenic fungus Rosellinia necatrix

Rosellinia necatrix is a soil-borne root pathogen affecting a wide range of commercially important plant species. The mycelium of R. necatrix was transformed to hygromycin B resistance by an Agrobacterium tumefaciens-mediated transformation system using a binary plasmid vector containing the hygromycin B phosphotransferase (hph) gene controlled by the heterologous fungal Aspergillus nidulans P-gpd (glyceraldehyde 3-phosphate dehydrogenase) promoter and the trpC terminator. Co-cultivation of R. necatrix strain W1015 and A. tumefaciens strain AGL-1 at 25 degrees C using the binary vector pAN26-CB1300, which contained the hygromycin B resistance cassette based on pAN26 and pCAMBIA1300, resulted in high frequencies of transformation. The presence of the hph gene in the transformants was detected by PCR, and single-copy integration of the marker gene was demonstrated by Southern blot analysis. This report of an Agrobacterium-mediated transformation method should allow the development of T-DNA tagging as a system f or insertional mutagenesis in R necatrix and provide a simple and reliable method for genetic manipulation.     

根癌农杆菌介导的日本曲霉转化体系的建立

【目的】通过根癌农杆菌介导的方法构建日本曲霉转化子库,从而筛选出高产甘没氧化酶的日本曲霉突变菌株。【方法】本文通过三亲杂交的方法将双元载体pBI-hphII转移至根癌农杆菌EHA105中并作为侵染菌株,以日本曲霉As5999为受体菌株,建立了农杆菌介导的日本曲霉转化体系,构建了突变体库,并对影响转化效率的根癌农杆菌浓度,乙酰丁香酮(As)加入与否,共培养时间,共培养温度等因素进行了分析。【结果】对转化子的PCR检测和Southern杂交分析表明,T-DNA已整合进日本曲霉基因组中,随机挑选的9个转化子连续转接10代后均能稳定遗传。【结论】该转化体系的建立为筛选出高产甘油氧化酶的日本曲霉突变菌株奠定了基础。     

农杆菌介导GUS基因对多年生黑麦草转化的研究

通过检测愈伤组织中GUS基因的瞬间表达,研究农杆菌LBA4404/pCAMBIA1301介导多年生黑麦草的转化体系。通过对多年生黑麦草瞬间表达率的比较,确立了其遗传转化的最佳优化条件。研究发现,多年生黑麦草不同品种的转化率在25%~45%之间变化。多年生黑麦草遗传转化最佳优化条件是预培养10d的胚性愈伤组织、浓度为0.5~0.8OD的农杆菌菌液以及2d共培养时间。在共培养基中添加100μmol/L乙酰丁香酮能有效地提高植物瞬间表达率。两种侵染处理方法比较结果为滤纸滴加法比浸泡法更优。转化后对愈伤组织的干燥处理能抑制农杆菌过度繁殖,能改善愈伤状态,有利于提高转化率。     

番木瓜β-Gal基因RNAi双T-DNA植物表达载体的构建及其遗传转化的初步研究

克隆了番木瓜(Carica papaya L.)果肉的细胞壁水解关键酶β-半乳糖苷酶(β-GAL)基因保守区,将其反向重复插入载体pKANNIBAL,构建RNAi中间表达载体pKAN/RG,将其上的发夹结构取代经改造的载体pCAMBIA 1300上hpt II基因,构建中间表达载体p1300~-/MFRG,分离单T-DNA区段,与载体pCAMBIA 2301构建RNAi双T-DNA植物表达载体p2301/TTRG.酶切分析和PCR检测表明,p2301/TTRG已被成功导入农杆菌EHA 105.通过遗传转化,初步获得了GUS染色呈阳性且具Kan抗性的番木瓜胚性愈伤组织.