油菜ICE1基因表达载体构建及转化烟草

从油菜中克隆得到了ICE1基因的开放阅读框序列.构建了以CaMV35S为启动子的植物表达载体,经农杆菌介导法转化烟草,获得转基因植株.通过PCR检测,目的基因成功转入烟草中.将转油菜ICE1基因的烟草和非转基因烟草置于2℃处理7 d,非转基因烟草出现萎蔫,转基因烟草没有明显变化,非转基因烟草丙二醛浓度明显高于转基因烟草.将转基因烟草与非转基因烟草分别置于0、-2、-4℃各1 h后,转基因烟草APX、SOD活性明显高于非转基因烟草.     

TaNHX2基因植物表达载体的构建及在烟草中的表达

将TaNHX2基因重组于质粒pBIN438的CaMV 35S启动子下游,构建含TaNHX2基因的植物双元表达载体pBIN438-TaNHX2.采用农杆菌介导转化烟草(Nicotiana tobacum L.),获得含TaNHX2的转基因烟草植株.经PCR、RT-PCR分析表明,TaNHX2基因已整合到烟草中,并且得到表达.耐盐分析表明,外源基因TaNHX2提高了转基因植株的耐盐性.     

基于Gene-Deletor系统的安全复合性状转基因烟草研究

本研究利用农杆菌介导法将带有水稻花粉特异启动子籼稻花粉过敏原基因(OSIPA)启动子驱动的Gene-Deletor外源基因清除系统,水稻Os GA3ox2(D18)启动子驱动水稻Os GA2ox1基因,玉米Ubiquitin启动子驱动BAR::GUS融合基因为筛选标记基因以及水稻Actin1启动子驱动驱动抗虫Cry1Ab基因复合性状植物表达载体p GM626-D18-Os GA2ox1遗传转化三星烟草。通过GUS组织化学染色及PCR分子鉴定,获得了43株转基因烟草植株。结果表明,水稻OsGA2ox1基因在烟草中表达能降低转基因烟草植株高度,但不影响植株生殖生长。转基因烟草对烟草斜纹夜蛾幼虫具有抗性,可抑制烟草斜纹夜蛾幼虫的取食与发育。以50 mg/L的除草剂Basta处理野生型和转基因烟草离体叶片,发现BAR基因提高了烟草抗除草剂的能力。对12株转基因烟草T0代花粉外源基因清除效率进行研究,发现部分烟草株系外源基因清除可达到100%,其他未完全清除外源基因株系的清除效率介于42.84%~99.97%之间。     

复苏植物牛耳草BhLEA2基因启动子的分离和基因表达模式研究

为研究干旱诱导的基因表达模式,利用Inverse-PCR和Tail-PCR的方法从复苏植物牛耳草（Boea hygrometrica（Bunge）R Br．）中扩增出胚胎发育晚期丰富蛋白编码基因BhLEA2的1215bp启动子序列,命名为PBhLEA2。构建了由PBhLEA2启动子引导GUS嵌合基因的植物表达载体pBhLEA2-GUS,并经农杆菌介导导入到烟草中,得到4株转基因烟草植株。GUS检测分析表明,该启动子可驱动GUS报告基因在转基因烟草的种子和刚萌发的小苗的子叶和胚轴中高效表达,在10-20d苗龄的植株中不表达,表现出一定的发育阶段和组织特异性。干旱、高盐胁迫及脱落酸（ABA）、乙烯和H2O2等信号分子可在不同程度上诱导GUS报告基因在20d苗龄的转基因植株的叶片中表达,但只有ABA可诱导其在根中表达,表明该启动子对BhLEA2基因表达的调控受环境信号影响。     

苦瓜McAG2启动子的克隆与表达研究

文中从苦瓜基因组中克隆得到长为1417 bp的McAG2基因5′上游片段并进行了DNA序列分析.通过PCR得到了其缺失片段,将其插入pBI121载体替换CaMV35S启动子,得到了McAG2基因5′侧翼缺失表达载体.并利用农杆菌介导转化烟草,建立了相应的转基因烟草植株,以研究其在不同器官组织中的表达特性. β-glucuronidase(GUS)染色结果显示该启动子在转基因烟草叶片和根组织中没有表达活性.     

杂交鹅掌楸LhARF2基因启动子的克隆及瞬时表达分析

生长素响应因子(Auxin response factor, ARF)参与调控植物生长发育的多个途径。本研究利用Tail-PCR技术从杂交鹅掌楸中克隆LhARF2基因5′端上游2 637 bp序列,即pLhARF2启动子,并利用生物信息学软件PlantCARE分析其包含的调控元件,发现其含有启动子必需元件TATA-box和CAAT-box,以及压力响应、激素响应、光信号转导和代谢循环过程元件。构建pLhARF2-pCAMBIA1300:GUS植物表达载体并瞬时浸染本氏烟草叶片,利用GUS组织化学染色法鉴定烟草叶片中瞬时表达活性,发现在烟草叶片中有蓝色斑块,但颜色较浅。实验结果推测杂交鹅掌楸pLhARF2启动子可以调控GUS基因活性,为下一步研究启动子遗传转化的组织表达活性奠定了基础。     

拟南芥HSP70基因启动子表达载体的构建及在烟草BY2细胞中的应用

探讨了拟南芥的HSP70基因在液体悬浮培养的烟草BY2细胞中的表达及应用.用PCR扩增的方法从拟南芥col生态型基因组中扩增获得HSP70基因启动子序列,将其连入p1300表达载体且以GFP为报告基因,将该表达载体采用农杆菌转基因转入液体悬浮培养的烟草BY2细胞中,观察转基因细胞中报告基因GFP的表达情况.结果显示:HSP70:GFP转基因液体悬浮培养的烟草BY2细胞中有GFP的表达.该表达载体可在液体悬浮培养的BY2细胞中正常表达,且可在较短时间内获得大量实验材料,对拟南芥的HSP70基因启动子的进一步研究提供理论依据和丰富的实验材料,且可明显缩短实验周期.     

拟南芥器官大小调控基因AtKIX8启动子的克隆和表达分析

为研究拟南芥器官大小调控基因AtKIX8的表达模式,以期进一步研究其功能机制,克隆了该基因启动子序列,获取了启动子-GUS转基因报告植株.利用GUS组织化学染色检测了该启动子作用位置,利用荧光定量PCR分析了启动子对外源激素及冷胁迫的响应.结果表明该启动子诱导GUS基因在幼苗茎尖分生区,成株茎、叶主脉中特异性表达,生长素和低温处理显著提高GUS基因的表达量.说明拟南芥AtKIX8基因启动子具备组织特异性表达模式,且能受到外源生长素和低温的诱导.     

烟草维管束发育相关基因Nvas启动子顺式作用元件鉴定

为研究烟草维管束发育相关基因Nvas启动子顺式作用元件,将克隆得到的Nvas启动子ATG+1~-463区域分为10个不同长度的片段与GFP报告基因融合构建了植物表达载体并完成了5'端缺失分析.利用根癌农杆菌介导转化W38型烟草叶盘,得到了含有不同长度Nvas启动子片段的转基因烟草植株.体视显微镜下观察到含Nvas启动子-216~-463区域的转基因烟草均有绿色荧光蛋白的表达,表达部位集中在维管束组织.结果表明Nvas启动子能使外源基因在维管束组织中特异表达.该启动子活性高于Ca MV35S,在ATG+1~-216区域存在核心启动子元件,在-337~-379区域存在能增强启动子活性的元件.     

转蔗糖: 蔗糖-1-果糖基转移酶基因提高烟草的耐旱性

蔗糖: 蔗糖-1-果糖基转移酶（sucrose: sucrose 1-fructosyltransferase, 1-SST）以蔗糖为底物催化生成蔗果三糖等低聚合度的果聚糖.将从莴苣中克隆的1-SST基因重组到pCAMBIA1300-als中，构建了在CaMV 35S启动子调控下的植物表达载体，利用农杆菌介导的叶盘转化法将1-SST基因导入烟草中，PCR和Southern杂交检测表明获得了转基因植株，RT-PCR结果表明该基因在烟草中正常表达. 对T₀代转基因烟草进行的耐旱性分析结果表明，干旱胁迫6d的转基因植株丙二醛含量和电解质渗漏率显著低于未转基因对照，叶片相对含水量下降速度也明显比对照慢. 对转基因植株叶片糖分分析表明，转基因烟草植株积累果聚糖，并在干旱胁迫后含量明显增加，而未转基因对照植株不积累果聚糖. 在14%PEG溶液中未转基因烟草种子的萌发率仅为转基因烟草种子的一半；在附加200mmol/L甘露醇的培养基中未转基因烟草种子根的生长明显受到抑制，而转基因烟草根的生长发育正常. 以上研究结果表明，转1-SST基因烟草植株耐旱性的提高可能与该基因的表达有关.     

小鼠液胞H~+-ATPase 15 K启动子(M15 K)的克隆及其在植物体内的表达特性研究

PCR克隆了小鼠液胞H+-ATPase 15K启动子,构建具有Kan抗性和GUS intron报告基因的植物表达载体LpPMG.通过M15K启动子指导的GUS intron基因在烟草叶片内的瞬时性表达,比较了其植物表达特性.结果表明:M15K启动子可启动GUS在植物体内的表达.其表达活性相当于2×35S启动子的87.0%±17.3%.     

Obtaining High Pest-resistant Tobacco Plants Carrying B.t. insecticidal Gene

To increase the expression level of CryIA(c) gene in transgenic plants, a plant expression vector pBinMoBc carrying the CryIA(c) gene under control of chimeric OM promoter and Ω factor was constructed. As a control, pBinoBc carrying the CryIA(c) gene with the CaMV 35S promoter was also constructed. The vectors were transferred into tobacco plants respectively via Agrobacterium-mediated transformation. ELISA assay showed that the expression level of the CryIA(c) gene in pBinMoBc transgenic tobacco plants was 2.44-times that in pBinoBc transgenic tobacco plants, and it could be up to 0.255% of total soluble proteins. Bioassay showed that pBinMoBc transgenic tobacco plants had more notable insecticidal effect than pBinoBc transgenic tobacco plants. The above results showed that the chimeric OM promoter was a stronger promoter than CaMV 35S promoter that was widely used in plant genetic engineering, and this is very useful in pest-resistant plant genetic engineering.     

Kas基因启动子区的克隆及功能初步分析

利用TAIL-PCR技术，克隆到了与辣椒素合成有关的胎座特异表达基因——3-酮酯酰．ACP合成酶基因（Kas）上游400bp的调控区域．将其全长片段与GUS基因连接构建植物表达载体并转化烟草．GUS组织化学染色表明，克隆到的440bp片段具有启动子活性．对该片段进行序列分析发现，在起始密码子ATG上游存在2个TATA-box，分别为-316～-311位的TATAAA和-224～-219位的TATAAA；在TATA-box上游还存在1个位于-378～-374处的CAAT-box，序列为CCAAT．该研究旨在为利用基因调控辣椒素的生物合成，提高辣椒果实中的辣椒素含量奠定基础．     

利用番茄U3snRNA基因上游启动区构建植物表达载体及对烟草的转化

利用番茄U3snRNA基因上游启动区和ACC合成酶反义RNA-核酶嵌合基因DNA片段,构建含U3snRNA基因上游启动区-ACC合成酶的反义RNA-核酶嵌合序列的表达载体,重组于植物双元表达载体pGA643中,得到pGU3R.用三亲融合法导入农杆菌LBA4404中,采用叶盘法转化烟草,诱导再生小植株,获得了卡那霉素的抗性植株.提取抗性植株总DNA,通过PCR、PCRSouthern杂交检测并分别用启动区序列和ACC合成酶的反义RNA-核酶嵌合序列作探针,通过Southern杂交检测,已筛选出整合有外源基因的转化植株.为进一步研究U3snRNA上游启动区增强反义RNA-核酶基因的表达奠定了基础.     

Regulatory effect of cotton leaf curl virus AC2 on virion sense promoter

The AC2 gene of cotton leaf curl virus (CLCuV) was obtained by polymerase chain reaction (PCR) . The total DNA of the CLCuV infected tomato leaves was used as template, and the amplified DNA fragment was inserted into a cloning vector. Transient expression vectors were constructed by inserting the AC2 gene into downstream region of CaMV 35S promoter. These constructs were delivered into tobacco and cotton leaf cells for transient expression by particle bombardment. The results indicated that the virion sense promoter was activated by AC2 and its activity increased remarkably. However, the activity of transactivated virion sense promoter was still lower than that of the complementary sense promoter. The expression pattern of transactivated virion sense promoter was similar to that of the complementary sense promoter, namely with high activity in both mesophyll and vascular tissues. The possibility of application of AC2 in plant genetic manipulation was also explored.     

活体烟草BY-2悬浮细胞微丝骨架的标记

微丝骨架是细胞骨架的重要成员,在细胞的多项生理活动中发挥着重要作用.本论文利用荧光标记鬼笔环肽技术和GFP融合蛋白技术,对活体烟草BY-2悬浮细胞中微丝骨架的标记方法进行了探索,结果表明,10nmol/L的Alexa488-Phalloidin为细胞微丝骨架标记的最佳浓度,利用PCR等技术构建pPZP-NtFABD2-GFP植物表达载体后,转化烟草BY-2悬浮细胞,激光共聚焦扫描显微镜观察发现,NtFABD2-GFP融合蛋白能够清晰地显示活体烟草悬浮细胞内的微丝骨架.这些结果为进一步深入研究微丝骨架在活体植物细胞中的功能奠定了基础.     

Function of resveratrol derived from transgenic plant expressing resveratrol synthase gene

Two genes from grapevine coding for resveratrol synthase, named RS1 and RS2, were cloned by RT-PCR. AnEscherichia coli expression vector was constructed by insertion of RS1 into pBV221. A specific protein with the same molecular weight (42 ku) as the resveratrol synthase was expressed and used to prepare the rabbit antiserum. A plant expression vector was constructed by inserting the RS1 gene into pBin438 downstream of the doubled CaMV 35S promoter and TMV-Ω fragment. PCR-positive transgenic tobacco plants were obtained after transformation withAgrobacterium tumefaciens LBA4404 harboring the plant expression vector. Southern blot analysis demonstrated that the foreign gene was integrated into the tobacco genome. The results of RT-PCR and Western blot indicated that the RS1 gene was transcribed and expressed. Formation of resveratrol in transgenic tobacco was further determined by thin-layer chromatography of silica gel and HPLC. Increased accumulation of human breast adenocarcinoma cells in G₀ and G₁ phases of cell cycle was observed in cells treated with resveratrol purified from transgenic tobacco as compared to the untreated cells.     

Activity of the truncated promoter of pollen-specific G9 gene of cotton and the transgenic recessive nuclei-sterile tobacco

A 557 bp fragment from the translation initiation site of the G9 gene expressed in maturing pollens of cotton was isolated from genomic DNA of upland cotton (Gossypium hirsutum L.) cv. “Zhongkang 17”, and two expression vectors for plant transformation were constructed via fusing this fragment with β-glucuronidase gene (Gus) and cytotoxin gene Barnase. The promoter activity of this fragment was demonstrated via transient expression of Gus gene in cotton and by the integrated expression of Barnase gene in tobacco. This promoter can initiate the expression of exogenous gene specifically and efficiently in plant pollen. The transgenic tobacco plant containing G9-Barnase fusion gene showed the characteristics of recessive nuclei-sterility.     

Identification of a bi-directional promoter from Tomato yellow leaf curl China virus

A bi-directional promoter of Tomato yellow leaf curl China virus (TYLCCNV) was obtained with the total DNA from TYLCCNV isolate Y10 infected tobacco leaves as a template. Plant expression vectors were constructed by fusing the amplified DNA fragment with the gus gene and nopaline terminator in different orientations. The vectors containing promoter fragments were transferred into leaf cells and plant stems of Nicotiana benthamiana by Agrobacterium-mediated method. Transient expression results showed that both the complementary and virion-sense promoters could drive the gus gene to express, and the GUS activity of the complementary-sense promoter was stronger than that of the virion-sense. Co-expression of the vector containing βC1 gene of TYLCCNV DNAβ with the vector containing a bi-directional promoter revealed that the βC1 protein has no impact on expression of either the virion- or the complementary-sense promoter.