农杆菌介导LJAMP2基因导入‘红阳’猕猴桃及分子鉴定

为了获得抗溃疡病的‘红阳’猕猴桃转基因植株,以红阳猕猴桃试管苗叶盘为转基因受体材料,通过根癌农杆菌介导将CaMV35S启动子调控下的LJAMP2基因导入红阳猕猴桃。450个叶盘与携带表达载体质粒pBI121的根癌农杆菌菌珠LBA4404共培养2 d后,转入含25 mg/L Kan的筛选培养基培养40 d,15 d转接1次,之后30 d继代1次。结果表明,在MS+3.0 mg/L BA+1.0 mg/L NAA筛选培养基中,Kanr芽率达85%以上,在1/2 MS+0.8 mg/L IBA培养基中,Kanr芽生根率达100%。共获得Kanr再生植株40株,经GUS组织染色和PCR分析证明,其中23株为转基因植株。阳性率为57.50%,转化率达5.11%。抗溃疡病基因LJAMP2已成功导入红阳猕猴桃,为红阳猕猴桃的抗病基因工程育种奠定了基础。     

基因枪法获得GAI转基因橡胶树植株的研究

将含有Camv35S启动子、卡那霉素抗性基因和GUS报告基因,目的基因为GAI基因的转化载体质粒pBI121,通过基因枪轰击巴西橡胶树(Hevea brasiliensis Muell-Arg.)花药愈伤组织,50 mg L~(-1)卡那霉素的继代培养基进行抗性筛选.获得了抗性再生植株,经过PCR、Southern检测结果表明:GAI基因已经成功转入橡胶树基因组中.     

基因枪法获得GAI转基因橡胶植株的研究

将含有Camv35S启动子、卡那霉素抗性基因和GUS报告基因,目的基因为GAI基因的转化载体质粒pBI121,通过基因枪轰击巴西橡胶树(Hevea brasiliensis Muell-Arg.)花药愈伤组织,50 mg L~(-1)卡那霉素的继代培养基进行抗性筛选.获得了抗性再生植株,经过PCR、Southern检测结果表明:GAI基因已经成功转入橡胶树基因组中.     

胡萝卜组织培养和高效遗传转化体系的建立

为了建立高效的胡萝卜遗传转化体系,本实验选用3个胡萝卜(Daucuscarotavar.sativa)栽培品种:‘金笋五寸’、‘Carol’和‘改良黑田七寸’,以它们的下胚轴和子叶为外植体,首先建立了高频愈伤诱导体系。在此基础上,以Carol的下胚轴和愈伤组织为受体材料,利用根癌农杆菌LBA4404介导转化质粒pBI121。经X-Gluc染色,证明GUS基因瞬间表达成功,经PCR方法鉴定,证明GUS基因已整合到胡萝卜的染色体中,从而建立了高效的胡萝卜遗传转化体系。     

罗汉果叶片离体再生快繁技术

以罗汉果(Ssiraiti grosvenori)叶片为外植体,探讨培养方式、激素组合对愈伤组织诱导和不定芽分化的影响。结果表明:罗汉果叶片在培养基MS+BA 1.0 mg/L+IBA 0.7 mg/L上培养4周愈伤组织的诱导率达90%以上;罗汉果愈伤组织在培养基MS+BA 1.0 mg/L+IBA0.2 mg/L+赛苯隆(TDZ)0.1 mg/L上不定芽的分化率可达70%,平均出芽指数3.7;罗汉果试管苗在培养基MS+BA 2.0 mg/L+IBA 0.2 mg/L上茎芽增殖比较稳定,在培养基MS+IBA0.1 mg/L上培养2周开始分化不定根,其生根率在90%以上。     

串叶松香草高效再生体系的建立与兔出血症病毒YL株外壳蛋白基因VP60对其遗传转化

通过对串叶松香草(Silphium perfoliatumL.)不同激素浓度配比的诱导分化实验,建立了串叶松香草离体培养高效再生体系,结果表明MS 6-BA(2.0mg/L) NAA0.1(mg/L)培养基可高效诱导愈伤组织和芽的分化,1/2MS IBA(0.1mg/L)培养基可快速诱导根的生成,形成再生植株。构建了植物表达载体pBI121-VP60,利用根癌农杆菌(Agrobacterium tumefaciens)介导叶盘法转化串叶松香草以研究高效的串叶松香草转化体系,结果显示以农杆菌LBA4404为介导菌株、以叶片为转化外植体、3d预培养时间和3～4d共培养时间、400mg/L羧苄青霉素和40mg/L卡那霉素筛选浓度转化效果较好,并已筛选到两株拟转基因植株,为利用串叶松香草生产兔出血症病毒动物可食用疫苗建立了初步的技术基础。     

影响根癌农杆菌介导水稻转化的因素分析

根癌农杆菌与来自水稻成熟种子盾片的愈伤组织共培养,将GUS基因导入水稻愈伤组织,并获得了转基因植株。通过比较影响根癌农杆菌转化频率的各种因素,表明激素配比为2,4-D1mg/L、TDZ0.5mg/L、NAA1mg/L时,可以大大促进籼稻愈伤组织的分化能力;酚类化合物的加入使农杆菌的转化频率提高8.9%-23.5%;共培养时农杆菌的稀释方式及适当调整潮霉素（hygB）的使用浓度影响到农杆菌的转化频率。     

苏云金杆菌内毒素蛋白基因转入葡萄胚性愈伤组织细胞及转基因植株再生的研究

以葡萄的胚性愈伤组织作为农杆菌介导,Ti质粒转化材料,利用共培养法将苏云金杆菌内毒素蛋白基因转入葡萄胚性愈伤组织细胞,通过胚状体发生途径再生转基因植株。实验发现:80μmol/L的乙酰丁香酮诱导处理农杆菌和葡萄愈伤组织后可将转化效率提高50倍。OD值为0.8的农杆菌菌液稀释8—10信后与在G培养基预培养10天的胚性愈伤组织共培养2—3夭,Ti质粒对葡萄愈伤组织细胞的转化效率可达50%左右。筛选得到的转基因植株在含Km 30 mg/L的选择培养基上继代存活6个月,生长正常;提取叶片染色体DNA做Southern blot,杂交结果为阳性。将转基因植株各部分切段置于含Km 50 mg/L的选择培养基上,能够脱分化产生抗性愈伤组织并能增殖。     

外源基因在烟草绿色组织中的高效表达研究

研究外源基因在受体绿色组织中的特异表达情况,分别构建由棉花PsbP启动子驱动的GUS基因及CP4 epsps 基因的植物表达载体pBI121-P、pBI121-PE.农杆菌介导法转化到烟草中,获得20株转pBI121栽体、40株转pBI121-P栽体和32株转pBI121-PE载体的烟草阳性植株.组织化学染色分析表明,GhPsbP启动子驱动的GUS基因只在转基因烟草的叶片和茎中表达,在根中不表达;Real-time PCR分析表明,PsbP启动子驱动CP4 epsps基因在叶和茎中的表达量分别是根中的15倍和10倍;草甘膦抗性试验证明,PsbP启动子驱动的CP4 epsps基因在烟草叶及茎的绿色组织中的表达量足以忍受1%浓度草甘膦的毒害.证明GhPsbp启动子可以有效地驱动外源基因在烟草的绿色组织中高效特异的表达.     

无核白葡萄愈伤组织瞬时转化体系的优化与应用

为了优化根癌农杆菌介导的葡萄愈伤组织瞬时转化体系,该研究以欧洲葡萄品种无核白(Vitis vinifera L.cv.Thompson Seedless)单芽茎段诱导的愈伤组织为材料,探讨重悬液pH、菌液浓度、真空渗透时间等主要因素对葡萄愈伤组织瞬时转化效率的影响。结果表明:(1)以激素组合分别为1.0mg/L BAP、1.0mg/L BAP+0.02mg/L NAA、2.0mg/L BAP+0.02mg/L NAA和4.0mg/L BAP+0.02mg/L NAA的系列培养基更适合无核白葡萄单芽茎段逐步诱导胚性愈伤组织。(2)葡萄愈伤组织瞬时转化体系中,重悬液pH 5.1,菌液浓度OD6001.0,真空渗透20min为转化效率最佳条件。(3)利用优化的瞬时转化体系瞬时转化无核白葡萄的不同组织,发现在不同器官中转化效率存在显著差异。其中以愈伤组织为受体的转化效率显著高于其他器官(65 231.99±3 339.29mU/g),而且愈伤组织的GUS组织化学染色最深,以叶片为受体的转化效率则最低。利用该体系转化质粒载体pCAMBIA0390∷GUS,瞬时表达产物经过GUS蛋白活性检测,结果表明该研究优化的葡萄愈伤组织瞬时转化体系有助于外源基因在葡萄愈伤组织内的表达,为后期通过转基因技术研究目标基因功能奠定了技术基础。     

Effects of antibiotics on the elimination of <Emphasis Type="Italic">Agrobacterium tumefaciens</Emphasis> from loblolly pine (<Emphasis Type="Italic">Pinus taeda</Emphasis>) zygotic embryo explants and on transgenic plant regeneration

Three antibiotics were evaluated for their effects on the elimination of Agrobacterium tumefaciens during the genetic transformation of loblolly pine ( Pinus taeda L.) using mature zygotic embryos as targets. Agrobacterium tumefaciens strains, EHA105, GV3101, and LBA 4404, all harbouring the plasmid pCAMBIA1301, which carries the selectable marker gene, hygromycin phosphotransferase ( hpt) controlled by the cauliflower mosaic virus 35S promoter and terminator, and the uidA reporter gene (GUS) driven by the cauliflower mosaic virus 35S promoter and the terminator of nopaline synthase gene, were used in this study. Exposure to 350 mg l^-1 carbenicillin, claforan, and timentin respectively for up to 6 weeks did not eliminate the Agrobacterium, while antibiotics at 500 mg l^-1 eradicated them from the co-cultivated zygotic embryos. All three antibiotics increased callus growth and shoot regeneration at 350 and 500 mg l^-1 each, but reduced callus growth and shoot regeneration at 650 mg l^-1 when compared with controls. Putative transgenic calli were selected for continued proliferation and differentiation on 4.5 mg l^-1 hygromycin-containing medium. Transformed calli and transgenic plants produced on a selection medium containing 4.5 mg l^-1 hygromycin were confirmed by GUS histochemical assays, by polymerase chain reaction (PCR), and by Southern blot analysis. These results are useful for future studies on optimizing genetic transformation procedures in loblolly pine.     

带内含子卡那霉素抗性基因双元载体构建及烟草转化

农杆菌介导法是植物基因转化的常用方法,然而由于筛选培养基中常用的抗生素头孢霉素和羧苄青霉素具有类植物激素活性,影响外植体的再生和转化频率。将一个植物的内含子插入卡那霉素抗性基因编码区的N端,合成了一个带内含子的卡那霉素抗性基因。构建带该基因的植物双元表达栽体pYP1202并转化烟草,受侵外植体在含卡那霉素50～200mg/L的选择培养基中抗性芽分化频率不受卡那霉素浓度影响,然而具有GUS活性的转化子占分化芽的比例却随着卡那霉素浓度的增加而升高。当培养基中加入500mg/L羧苄青霉素后受侵外植体产生的抗性芽频率比单一的卡那霉素筛选提高近1倍,高达91.4％,然而具GUS活性的转化子占抗性芽的比例仅有26.7％,在200m/L的卡那霉素筛选下,比例升至93.3％。用带内含子卡那霉素抗性基因构建的植物表达载体转化植物可以减少假抗性芽的产生。     

火炬松成熟合子胚培养直接器官发生和植株再生

基因型Ｈｂ,Ｍａ和Ｍｃ的火炬松成熟合子胚在附加１．０ｍｇ／ＬＮＡＡ,４．０ｍｇ／ＬＢＡ,５００ｍｇ／ＬＬＨ和５００ｍｇ／Ｌ谷氨酰胺的ＴＥ培养基上培养１２周后,在子叶和胚轴部位形成不定芽原基。然后将合子胚转移到附加０．５ｍｇ／／ＬＮＡＡ,０．０５ｍｇ／ＬＩＢＡ,２ｍｇ／ＬＢＡ,５００ｍｇ／ＬＬＨ和５００ｍｇ／Ｌ谷氨酰胺的ＴＥ不定芽分化培养基上,６周后分化产生大量不定芽,３种基因型中,Ｈｂ的直接不定芽     

用RAPD法研究火炬松愈伤组织发生的遗传特性(英文)

体外培养对于植物的快速繁殖是非常有效的。和其它一些松果类硬木植物一样,火炬松的体外培养成功率却一直很低。本工作研究了不同的基本培养基和低温条件对于火炬松Ｊ－５６, Ｓ－１００３, ａｎｄ Ｅ－４４０等三个品系的成熟合子胚形成愈伤组织、分化出芽、成苗的影响。在不同的基本培养基条件下芽分化的程度差异很大。合子胚经过９－１２周培养,开始分化,形成具有器官发生的愈伤组织（Ｆｉｇ．２ａ）。分化后３周,开始诱导出芽（Ｆｉｇ．２ｂ）,芽的生长快慢不同（Ｆｉｇ．２ｃ,ｄ）。同一个愈伤组织上会生出几个芽来（Ｆｉｇ．２ｅ）。在添加有ＩＢＡ和ＢＡ的ＴＥ培养基上芽生长最快（Ｆｉｇ．１）。低温条件持续 １５天,能增加芽的数量和分化的程度（Ｔａｂｌｅ１）。上述培养基中增加ＧＡ３时表明,ＧＡ３对于根的诱导有决定性的作用。将９８株再生苗转移到特殊的混合土壤上;成活了７５株苗（Ｆｉｇ．２ｆ）。以这三种火炬松的再生苗尖为材料制备ＤＮＡ。用２０个引物进行ＲＡＰＤ分析,结果表明：这三种火炬松苗的扩增产物是相同的（Ｆｉｇ．２ｇ,ｈ＆ｉ）。这说明：用愈伤组织克隆植株的过程中没有引起植物遗传变异。     

Agrobacterium－mediated transformation and assessment of factors influencing transgene expression in loblolly pine（Pinus taeda L.）

This investigation reports a protocol for transfer and expression of foreign chimeric genes in loblolly pine (Pinus taeda L.). Transformation was achieved by co-cultivation of mature zygotic embryos with Agrobacterium tumefaciens strain LBA4404 which harbored a binary vector (pBI121) including genes for beta-glucuronidase (GUS) and neomycin phosphotransferase (NPTII). Factors influencing transgene expression including seed sources of loblolly pine, concentration of bacteria, and the wounding procedures of target explants were investigated. The expression of foreign gene was confirmed by the ability of mature zygotic embryos to produce calli in the presence of kanamycin, by histochemical assays of GUS activity, by PCR analysis, and by Southern blot. The successful expression of the GUS gene in different families of loblolly pine suggests that this transformation system is probably useful for the production of the genetically modified conifers.     

抗生素对农杆菌的抑制和对油菜外植体分化的影响

通过哌拉青霉素、氨苄青霉素、青霉素钠、羧苄青霉素、头孢拉定、头孢唑啉钠、磷霉素钠、乳糖酸红霉素、白霉素9种抗生素对根癌农杆菌EHA105和LBA4404的抑制效果,以及对油菜子叶柄分化影响的研究,结果表明：羧苄青霉素在500mg／L时对农杆菌EHA105的抑菌效果最好,而其它8种抗生素对EHA105无明显的抑菌作用;对于LBA4404浓度为200mg／L的羧苄青霉素、氨苄青霉素和头孢唑啉钠都有良好的抑菌效果。不同抗生素对油菜子叶柄的分化试验结果表明,羧苄青霉素和头孢唑啉钠对离体油菜子叶柄再生分化及生长没有影响,磷霉素钠、乳糖酸红霉素、自霉素几乎完全抑制了油菜子叶柄分化。同时对卡那霉素(作为筛选剂)的浓度进行了筛选,确定了油菜33B的筛选浓度为15mg／L,油菜918B的筛选浓度为10mg／L。     

Regeneration of transgenic loblolly pine (Pinus taeda L.) from zygotic embryos transformed with Agrobacterium tumefaciens

Embryos of 24 open-pollinated families of loblolly pine (Pinus teade L.) were used as explants to conduct in vitro regeneration. Then, Agrobacterium tumefaciens strain GV3101 harboring the plasmid pPCV6NFHygGUSINT was used to transform mature zygotic embryos of seven families of loblolly pine. The frequency of transformation varied among families infected with A. tumefaciens. The highest frequency (100%) of transient beta-glucuronidase (GUS)-expressing embryos was obtained from family 11-1029 with over 300 blue spots per embryo. Expression of the GUS reporter gene was observed in cotyledons, hypocotyls, and radicles of co-cultivated mature zygotic embryos, as well as in callus and shoots derived from co-cultivated mature zygotic embryos. Ninety transgenic plants were regenerated from hygromycin-resistant callus derived from families W03. 8-1082 and 11-1029. and 19 transgenic plantlets were established in soil. The presence of the GUS gene in the plant genome was confirmed by polymerase chain reaction. Southern blot, and plant DNA/T-DNA junction analysis. These results suggest that an efficient A. tumefaciens-mediated transformation protocol for stable integration of foreign genes into loblolly pine has been developed and that this transformation system could be useful for future studies on transferring economically important genes to loblolly pine.     

<Emphasis Type="Italic">Agrobacterium tumefaciens</Emphasis>-Mediated genetic transformation in tea (<Emphasis Type="Italic">Camellia sinensis</Emphasis> [L.] O. Kuntze)

We have developed a system to produce transgenic plants in tea (Camelia sinensis [L.] O. Kuntze) viaAgrobacterium tumefaciens-mediated transformation of embryogenic calli. Cotyledon-derived embryogenic callus cultures were cocultivated with anA. tumefaciens strain (AGL 1) harboring a binary vector carrying the hygromycin phosphotransferase (hpt II), glucuronidase (uid A), and green fluorescent protein (GFP) genes in the tDNA region. Following cocultivation, embryogenic calli were cultured in medium containing 500 mg/L carbenicillin for 1 wk and cultured on an antibiotic selection medium containing 75 mg/L hygromycin for 8–10 wk. Hygromycin-resistant somatic embryos were selected. The highest production efficiency of hygromycin-resistant calli occurred with cocultivation for 6–7 d in the presence of 400 μM acetosyringone (AS). Hygromycin-resistant somatic embryos developed into complete plantlets in regeneration medium containing half-strength Murashige and Skoog (MS) salts with 1 mg/L benzyl amino purine (BAP) and 9 mg/L giberellic acid (GA₃). Transformants were subjected to GFP expression analysis, β-glucuronidase (GUS) histochemical assay, PCR analysis, and Southern hybridization to confirm gene integration.     

药用植物川东獐牙菜的组织培养

针对川东獐牙菜野生资源受到严重破坏的情况 ,系统地探讨了通过组织培养为手段进行人工繁殖的方法 ,旨在为川东獐牙菜的保护提供坚实的理论依据。研究结果表明 :在所有的实验方案中 ,幼茎和老叶是理想的外植体材料。对叶片来说 ,较适宜的诱导愈伤组织的激素组合是 Zt1.0 m g/L +NAA 0 .0 5m g/L +IBA0 .0 5mg/L、BA 0 .5m g/L+2 ,4 - D0 .5mg/L或 BA 0 .2 m g/L+2 ,4 - D0 .2 mg/L+IBA0 .1m g/L ,对茎段来说 ,较适宜的诱导愈伤组织的激素组合是 BA0 .0 5m g/L+kt0 .0 5mg/L+IBA0 .0 5m g/L;诱导不定芽的适宜激素组合是 BA2 .0 mg/L+N AA0 .0 5mg/L或 BA 2 .0 mg/L+IBA 0 .1m g/L ;而根的诱导则是 MS+BA 0 .0 5mg/L+kt1.0 mg/L+N AA0 .1m g/L或 MS+BA1.0 m g/L+kt0 .3mg/L +IA A0 .5mg/L培养基上进行。