Resistance to Potato Virus X Infection in Transgenic Tobacco Plants with Coat Protein Gene of Virus

A major commercial cultivar of tobacco was transformed via Agrobacterium mediated procedure. Tobacco leaves started to form shoots on shoot inducing medium containing kanamycin after infected by Agrobacterium containing the plasmid with PVX CP gene. Regenerated plants were obtained in two weeks on hormone-free MS medium containing kanamycin. The transgenic tobacco plants were identified with nopaline detection,enzyme-linked immunosorbent assay and western blot analysis, symptom appearance was significantly delayed and virus accumulation was either absent or reduced in PVX CP gene transformed plants. Progenies of transgenic tobacco plants also gained resistance to PVX infection to a certain degree. These experiments demonstrate that CP protection is effective against PVX.     

马铃薯S病毒外壳蛋白基因的克隆与原核表达

依据马铃薯S病毒 (PotatovirusS ,PVS)外壳蛋白 (CP)基因序列 (885bp)设计合成了两对引物 ,通过RT PCR扩增得到长 0 .8kb的目的片段 ,将目的片段转入大肠杆菌 ,酶切鉴定证明得到了含有目的片段的重组子 ,测定序列结果与其他PVS分离物CP基因的序列比较 ,发现其核苷酸同源性达 95 %左右 ;构建了含PVSCP基因的融合蛋白原核表达载体 ,并在大肠杆菌中得到表达 ,SDS PAGE测定融合蛋白的分子量为 5 8kD。     

马铃薯Y病毒外壳蛋白基因在转基因马铃薯中的表达

ＰＶＹ是马铃薯Ｙ病毒组的典型成员,主要感染马铃薯、番茄、辣椒和烟草等。近年来,利用植物基因工程手段获得了不少抗病毒转基因工程植物,为培育抗病毒作物新品种提供了新途径［１］。病毒外壳蛋白基因导入并使之在植物中表达可获得抗相应病毒的转基因植物,已在烟草、番茄、马铃薯、苜蓿、黄瓜和番木瓜等植物中获得成功［１～３］。本室已成功地对在我国流行的ＰＶＹＮ株系外壳蛋白基因进行了克隆及序列测定［４］,在此基础上,我们构建了植物表达中间载体,通过土壤农杆菌介导的叶盘法转化马铃薯,获得了大量转基因植株。分子检测证明…     

转WMV-2外壳蛋白基因西瓜植株的病毒抗性

西瓜是夏季的重要水果,病毒病是影响其品质和产量的重要原因之一。植物基因工程的发展为抗病育种提供了新途径。利用外壳蛋白(coat protein)基因转化高等植物,赋予转基因植物以相应抗病性的成功例子已很多。本文报道WMV-2CP基因在自交子一代的分离符合孟德尔3：1的分离比。经过连续4代的选择鉴定,已从T7、T11和T323个独立转化子的后代中筛选获得8个转基因纯合株系,性状表现整齐一致。Western blot结果表明,R4T7-1、T4T11-3以及R4T32-73个不同来源的株系均能表达产生外壳蛋白。转基因纯合株系WMV-2感染后的病毒抗性实验表明,与未转基因对照相比,转基因株系可以推迟发病时间,减轻发病程度。实验筛选获得的转基因株系R4T32-7表现出对WMV-2的高度抗性,为利用植物转基因技术选育抗病新品种奠定了基础。     

应用核酶体外切割马铃薯卷叶病毒外壳蛋白基因的研究

针对马铃薯卷叶病毒外壳蛋白基因第356～358位点“GUC”．设计、合成了一种“锤头状”核酶。将核酶基因克隆在体外转录载体PSPT19的SP6启动子下游;同时将PLRVCPcDNA亚克隆在体外转录载体pSPT18的SP6启动子下游。利用SP6RNA聚合酶分别体外转录,获得核酶分子和靶RNA序列。在41℃保温进行核酶切割反应,检测到预期大小且被切开的两个RNA短片段。     

翻译和非翻译马铃薯Y病毒外壳蛋白基因介导的抗病性比较

利用RT－PCR方法克隆获得马铃薯Y病毒烟草叶脉坏死株系（PVY^N）的可翻译和不可翻译外壳蛋白（CP）基因,并分别插入pROKⅡ质粒中获得重组双元表达载体。通过根癌农杆菌（Agrobacterium tumefaciens）介导的基因转化方法,将可翻译和不可翻译的PVY^N-CP基因分别导入烟草栽培品种NC89叶片组织中,得到抗卡那霉素的再生植株,对所得到的抗卡那霉素的再生苗进行PCR检测表明,被导入可翻译和不可翻译CP基因的植株分别占卡那霉素抗性植株的95％和98％。攻毒实验表明,两种类型的转基因烟草对PVY^N的抗病性具有相似性,其表现型为：免疫、抗病和感病。免疫型转基因植株的抗病性不受接种物类型及其剂量的影响。Southern印迹杂交结果显示,目的基因已经整合到烟草基因组中。Northern印迹杂交证明,两种类型的CP基因都已在RNA水平上得到了表达,但细胞内RNA的积累量与转基因植株的抗病强度成负相关。Western印迹杂交表明,在表达不可翻译PVY^N－CP基因的转基因植株内 以CP蛋白,而在导入可翻译的PVY^N-CP基因的植株内检测到了CP蛋白,且CP蛋白含量与抗病性不存在正相关。本研究结果证明,表达可翻译与不可翻译PVY^N-CP基因的转基因烟草对PVY^N的抗病性均为RNA介导的抗病性。     

Transgenic Potato with PVY Coat Protein Gene and Its Small-Scale Field Test

Potato virus Y (PVY) infection may cause a severe yield depression up to 80%. To develop the potato (Solanum tuberosum L. ) cultivars that resist PVY infection is very crucial in potato production. The authors have been cloned the coat protein gene of PVY from its Chinese isolate. A chimaeric gene containing the cauliflower mosaic virus 35S promoter and PVY coat protein coding region was introduced into the potato cultivars “Favorita”, “Tiger head” and “K4” via Agrobacterium tumefaciens. Results from PCR and Southern blot analysis confirmed that the foreign gene has integrated into the potato chromosomes. These transgenic potato plants were mechanically inoculated with PVY virus (20 mg/L). The presence of the virus in the potato plants was determined by ELISA and method of back inoculation into tobacco. The authors observed a drastic reduction in the accumulation of virus in some transgenic potato lines. Furthermore, some transgenic potato lines produced more tubers per plant than the untransformed potato did, and the average weight of these transgenic plant tubers was also increased. In the field test, the morphology and development of these transgenic potato plants were normal, 3 transgenic lines of “Favorita” exhibited a higher yield than the untrasformed virus-free potato with an increase ranged from 20% to 30%. From these transgenic lines, it will be very hopeful to develop a potato cultivar which not only has a significant resistance to PVY infection, but also a good harvest in potato production.     

马铃薯卷叶病毒外壳蛋白基因的合成,分子克隆和全序列分析

以分离自马铃薯主栽品种“紫花白”的马铃薯卷叶病毒(PLRV)分离物的RNA为模板,用人工合成的引物,用反转录和随后PCR扩增的方法合成了PLRV外壳蛋白(CP)基因的cDNA,并克隆于pUC19中。进一步用限制酶切和核苷酸序列分析表明,合成的cDNA由627个核苷酸组成(包括起始和终止密码),序列中有Hinc Ⅱ和BamH Ⅰ两个酶切位点,与国外报道一致。和国外的4个PLRV分离物CP基因序列对比结果,具有高度同源性,其同源率达99.0—99.7％。     

改造的马铃薯Y病毒复制酶基因介导高度抗病性

提取马铃薯Y病毒中国分离株(PVY—c)的mRNA作为模板,随机六聚脱氧核苷酸和寡聚dT为引物合成了单链cDNA。通过聚合酶链式反应(PcR)获得了PVY—C的核内含体b(Nib)全长cDNA克隆。在对其进行全序列分析的基础上,构建了PVY—CNIb基因全长．5’端缺失381个碱基和Nib反义RNA三种不同形式高等植物表达载体。在土壤农杆菌LBA4404的介导下,转化烟草生产品种NC89,获得了所有三种表达载体的转基因植株。通过分子生物学检测和抗性分析发现不同形式的Nib基因序列的转基因植株对马铃薯Y病毒表现不同程度的抗性。其中,以5’端缺失的Nlb的基因转化植株表现最好,从总共20个这类转化株系中筛选到4个株系至少在100μg／m1 PVY—C接种浓度下,表现完全的抗病效果。从总共39个全长Nib基因转化株系中,仅有一个株系,在100μg／ml PVY—c的攻毒接种下具有完全的抗病性。所有33个Nib基因反义RNA的转化植株中,无一株系表现完全的抗病效果,但是有部分株系能不同程度地延缓或减轻发病程度,并有部分植株在发病后50d左右有恢复健康的趋势。虽然能够在上述3种形式的Nib基因序列的转基因植物中检测到相应的RNA的转录产物,但是均未能检测到其相应的蛋白表达产物。     

表达马铃薯Y病毒外壳蛋白的转基因烟草的抗病性研究

将马铃薯Ｙ病毒中国分离物（ＰＶＴ－Ｃ）的外壳蛋白（ＣＰ）基因,在土壤农杆菌ＬＢＡ４４０４的介导下,转化烟草生产品种ＮＣ８９,获得了６个烟草株系。通过抗性分析发现,６个株系中有一个株系在２００μｇ／ｍｌＰＶＹ－Ｃ的攻毒下,仍未发病,分子检测发现,转基因植物中抗性产生的程度并不是同ＰＶＹ－Ｃ外壳蛋白的表达水平成正相关。     

马铃薯X病毒外壳蛋白的表达水平与变偶密码子使用频率的相关性

把经密码子修饰的马铃薯X病毒（Potato Virus X, PVX）外壳蛋白（Coat Protein, CP）基因和未修饰的野生型外壳蛋白基因与CaMV 35S启动子融合后,构建成相应的植物表达载体,利用农杆菌介导转化烟草。分别对修饰CP和野生CP的转基因烟草进行Western blot和ELISA分析,结果表明经密码子修饰的PVX外壳蛋白的表达量是野生型蛋白表达量的1/3～1/5。Northern blot结果表明修饰和未修饰的外壳蛋白在转录水平上是一致的。以上结果暗示外源基因中稀有密码子的数量可能是限制外源基因表达的一个因素。改变基因中稀有密码子的数量有可能成为控制基因表达的一种有效途径。     

甜菜坏死黄脉病毒外壳蛋白基因在大肠杆菌中的高效表达

将甜菜坏死黄脉病毒内蒙古分离物的外壳蛋白基因亚克隆到ｐＪＷ２上构建成在大肠杆菌中表达的载体。ＳＤＳ－ＰＡＧＥ及Ｗｅｓｔｅｒｎ ｂｌｏｔｔｉｎｇ检测的结果表明,该表达载体在大肠杆菌ＤＨ５α中经温度诱导后特异地表达２１ｋＤ的甜菜坏死黄脉病毒外壳蛋白。经光密度扫描估测,其表达量占大肠杆菌总蛋白的１９．５％。     

番木瓜环斑病毒YsCP基因的序列分析和植物表达载体的构建

用双脱氧链终止法分析了克隆的番木瓜环斑病毒（PRV）Ys株系外壳蛋白（CP）基因的序列,结果表明YsCP基因全长858nt。对PRV国内外16个株系或分离物CP基因的比较发现,YsCP基因与国内株系或分离物CP基因的同源性较高（94．44％～97．68％）,而与国外株系或分离物CP基因的同源性较低（88．88％～92．70％）。CP基因之间的差异主要靠近基因5’端,特别是在YSCP基因第63nt后连续缺失6nt,SmGTHAI和SRI的CP基因也在此处缺失3nt。将YsCP基因插入中间质粒pRokⅡ的CaMV35S启动于和nos终止序列之间形成CP基因的植物表达载体pRPCY,通过三亲交配使pRPCY进入农杆菌LBA4404,与其中的pAL4404构成双元载体系统。     

黄瓜花叶病毒CP基因原核表达及抗血清的制备

把黄瓜花叶病毒 (CMV)西番莲分离物的外壳蛋白 (CP)基因 ,通过BamHI SacI位点定向插入pET 2 2b( )载体 ,转化大肠杆菌BL2 1 (DE3)中 ,经IPTG诱导下 37℃培养 6h ,SDS PAGE电泳示表达蛋白分子质量为 31 8kDa ,表达量占菌体总蛋白的 2 8 9%,表明该蛋白得到了高效表达。用冰冷的氯化钾溶液显色 ,用表达的特异蛋白质条带制备抗原 ,免疫家兔制备出病毒特异抗血清。采用ID ELISA测定抗血清效价为 1 0 -6;抗血清和CMV几个分离物均有特异反应 ,和TMV、菌体蛋白不发生非特异性反应 ;检测病毒灵敏度达 30ng ml,能够从稀释 31 2 5倍的感病植物汁液中检测出病毒     

悬浮细胞再生表达外壳蛋白的转基因Indica水稻对水稻条纹病毒的抗病性(英文)

合成、克隆了水稻条纹病毒中国株的外壳蛋白基因并进行了序列分析,由Indica水稻成熟胚的愈伤组织形成胚性运浮细胞。用含有CP基因的pROK2表达载体的DNA包被1.09μm直径钨粉颗粒轰击培养细胞。被轰击的培养物在含有G418（40mg／mL,）的培养基中进行选择培养,由对G418抵抗的愈伤组织中获得10株再生株。用32P－dCTP标记的CP基因作为探针,以Southernblot测定其转化特性。由抗病的和对照的植株抽提基因组DNA用EcoRI和BamHI进行酶切,其中两个植株显示出0.6kh和0.7kb两条条交带．其大小与CP基因相对应。Westernblot和ELISA测定进步证明CP（32kDa）在转基因水稻中表达。16株转基因植株和100株对照植株用带毒的叶蝉接种,接种病毒后24d只有37.5％的CP转基因植株产生病毒症状,而对照植株为96％。进一步证明转基因水稻植株具有对RSV的抗病性。转基因植株T1代CP的表达分离比例为3.6:1。     

Expression of Rice Stripe Virus Coat Protein Gene in Transgenic Rice Plants

Rice stripe virus (RSV) is a pathogen of rice stripe disease causing great damage to rice. The disease is transmitted by Laodelphax striatellus and three other planthoppers. RSV infects as much as 37 cereals including rice, wheat, maize and results in a significant reduction in yield in epidemic year. In order to develop efficient means of controlling the disease, authors have studied the amino acid composition of RSV coat protein (CP), synthesized and cloned the cDNA to CP, sequenced the full-length CP gene. Having inserted the RSV CP gene into plant expression vector pROK Ⅱ, authors transformed rice suspension culture via microprojectile bombardment and obtained transgenic plants expressing the CP gene. The suspension culture was initiated by inoculating yellowish, compact and embryogenic calli derived from seeds into suspension medium containing proline and maltose. After being cultured at 26℃ in the dark for about half a year, finely-dispersed and embryogenic suspension culture was estabolished. Before bombardment the suspension culture was evently applied onto three-layered filter-paper discs in a petri dish. CaCl2 and spermidine was employed to coat tungsten particle with plasmid DNA. 2.5 μl of coated particle was loaded onto bullet and each dish was bombarded three times. Immediately after being bombarded, the suspensions were cultured in modified N6 medium. 2 days later the suspensions were transferred to the same medium but containing G418, which were subcultured weekly. Being subject to G418 selection for two months, white and fast-growing clones were emerged from the brownish cultures. Green plants regenerated when the resistant calli were transferred to differentiation medium. The regenerated plants were firm enough to grow well in the greenhouse. 10 plants regenerated from G418 resistant calli were tested for their transformed nature by Southern blot using 32P-labelled CP gene as a probe. Among the plants tested, 2 plants showed clearly hy bridizing bands with a molecular weight corresponding to RSV CP gene. Western blot further demonstrated that RSV CP gene was expressed in transgenic rice plants. At present tests on the antiviral effects of transgenic plants by feeding plantphoppers infccted with RSV are being underway.     

烟草环斑病毒外壳蛋白基因的原核表达及抗血清的制备

烟草环斑病毒(Tobaccoringspotvirus,TRSV)是我国二类进境检疫危险性有害生物,对农业生产危害较大。本研究依据TRSV外壳蛋白基因cp序列设计合成了2条引物,通过RT-PCR扩增得到长约1500bp的目的片段。将目的片段与质粒pET-22b( )连接,构建了含TRSVcp基因的融合蛋白原核表达载体pETRSV-CP。序列分析表明,TRSV-SD1的cp基因全长1548bp,编码515个氨基酸与GenBank中其它TRSV分离物cp基因相比,核苷酸及推导的氨基酸序列同源性为90.7%~94.6%。将pETRSV-CP转入大肠杆菌,诱导表达。SDS-PAGE结果显示,表达的TRSVCP融合蛋白的相对分子质量约为58kDa。以此融合蛋白制备的抗血清的效价为1/1024,抗血清与TRSV具有良好的特异性反应。     

马铃薯单双三价抗病毒基因表达载体的构建

马铃薯Y病毒(PVY)、X病毒(PVX)和卷叶病毒(PLRV)引起的病害是造成我国马铃薯退化的主要原因,严重危害我国的马铃薯生产。PVY和PVX或PVY和PLRV混合侵染带来的损失远远大于各病毒单独侵染。国外科学家通过在马铃薯植株体内表达病毒外壳蛋白(CP)基因来减缓病毒病害的发生已取得相当的成功。 我们从河北省坝上地区农科所试验田中采集PLRV感病材料Burbank及87-1,参照文献提取病毒RNA并以其为模板,反转录合成cDNA。根据PLRV澳大利亚分离物已发表的序列,设计并