14 resultados para Lba4404
Resumo:
The Agrobacterium-mediated transformation system was extended to two indica cultivars: a widely cultivated breeding line IR-64 and an elite basmati cultivar Karnal Local. Root tips and shoot tips of seedlings, and scutellar-calli derived from mature seeds showed high-efficiency Agrobacterium tumefaciens infection and stable transformation. In addition to the superbinary vector pTOK233 in Agrobacterium strain LBA4404, almost equally high levels of transformation were achieved with a relatively much smaller (13.1 kb) binary vector (pCAMBIA1301) in a supervirulent host strain AGL1. In both cases, as well as in both cultivars, while 60–90% of the infected explants produced calli resistant to the selectable agent hygromycin, 59–75% of such calli tested positive for GUS. A high level (400 μM) of acetosyringone in the preinduction medium for Agrobacterium and a higher level (500 μM) in the cocultivation medium was necessary for an enhancement in transformation frequency of the binary vector to levels comparable to a superbinary. Hygromycin-resistant calli could be produced from all the explants used. Transformants could be regenerated for both cultivars using the superbinary and binary vector, but only for calli of scutellar origin. In addition to the molecular confirmation of hpt and gus gene transfer and transcription, absence of gene sequences outside the transferred DNA (T-DNA) region confirmed absence of any long T-DNA transfer.
Resumo:
Sorghum (Sorghum bicolor (L.) Moench) is the world’s fifth major cereal crop and holds importance as a construction material, food and fodder source. More recently, the potential of this plant as a biofuel source has been noted. Despite its agronomic importance, the use of sorghum production is being constrained by both biotic and abiotic factors. These challenges could be addressed by the use of genetic engineering strategies to complement conventional breeding techniques. However, sorghum is one of the most recalcitrant crops for genetic modification with the lack of an efficient tissue culture system being amongst the chief reasons. Therefore, the aim of this study was to develop an efficient tissue culture system for establishing regenerable embryogenic cell lines, micropropagation and acclimatisation for Sorghum bicolor and use this to optimise parameters for genetic transformation via Agrobacterium-mediated transformation and microprojectile bombardment. Using five different sorghum cultivars, SA281, 296B, SC49, Wray and Rio, numerous parameters were investigated in an attempt to establish an efficient and reproducible tissue culture and transformation system. Using immature embryos (IEs) as explants, regenerable embryogenic cell lines (ECLs) could only be established from cultivars SA281 and 296B. Large amounts of phenolics were produced from IEs of cultivars, SC49, Wary and Rio, and these compounds severely hindered callus formation and development. Cultivar SA281 also produced phenolics during regeneration. Attempts to suppress the production of these compounds in cultivars SA281 and SC49 using activated charcoal, PVP, ascorbic acid, citric acid and liquid filter paper bridge methods were either ineffective or had a detrimental effect on embryogenic callus formation, development and regeneration. Immature embryos sourced during summer were found to be far more responsive in vitro than those sourced during winter. In an attempt to overcome this problem, IEs were sourced from sorghum grown under summer conditions in either a temperature controlled glasshouse or a growth chamber. However, the performance of these explants was still inferior to that of natural summer-sourced explants. Leaf whorls, mature embryos, shoot tips and leaf primordia were found to be unsuitable as explants for establishing ECLs in sorghum cultivars SA281 and 296B. Using the florets of immature inflorescences (IFs) as explants, however, ECLs were established and regenerated for these cultivars, as well as for cultivar Tx430, using callus induction media, SCIM, and regeneration media, VWRM. The best in vitro responses, from the largest possible sized IFs, were obtained using plants at the FL-2 stage (where the last fully opened leaf was two leaves away from the flag leaf). Immature inflorescences could be stored at 25oC for up to three days without affecting their in vitro responses. Compared to IEs, the IFs were more robust in tissue culture and showed responses which were season and growth condition independent. A micropropagation protocol for sorghum was developed in this study. The optimum plant growth regulator (PGR) combination for the micropropagation of in vitro regenerated plantlets was found to be 1.0 mg/L BAP in combination with 0.5 mg/L NAA. With this protocol, cultivars 296B and SA281 produced an average of 57 and 13 off-shoots per plantlet, respectively. The plantlets were successfully acclimatised and developed into phenotypically normal plants that set seeds. A simplified acclimatisation protocol for in vitro regenerated plantlets was also developed. This protocol involved deflasking in vitro plantlets with at least 2 fully-opened healthy leaves and at least 3 roots longer than 1.5 cm, washing the media from the roots with running tap water, planting in 100 mm pots and placing in plastic trays covered with a clear plastic bag in a plant growth chamber. After seven days, the corners of the plastic cover were opened and the bags were completely removed after 10 days. All plantlets were successfully acclimatised regardless of whether 1:1 perlite:potting mix, potting mix, UC mix or vermiculite were used as potting substrates. Parameters were optimised for Agrobacterium-mediated transformation (AMT) of cultivars SA281, 296B and Tx430. The optimal conditions were the use of Agrobacterium strain LBA4404 at an inoculum density of 0.5 OD600nm, heat shock at 43oC for 3 min, use of the surfactant Pluronic F-68 (0.02% w/v) in the inoculation media with a pH of 5.2 and a 3 day co-cultivation period in dark at 22oC. Using these parameters, high frequencies of transient GFP expression was observed in IEs precultured on callus initiation media for 1-7 days as well as in four weeks old IE- and IF-derived callus. Cultivar SA281 appeared very sensitive to Agrobacterium since all tissue turned necrotic within two weeks post-exposure. For cultivar 296B, GFP expression was observed up to 20 days post co-cultivation but no stably transformed plants were regenerated. Using cultivar Tx430, GFP was expressed for up to 50 days post co-cultivation. Although no stably transformed plants of this cultivar were regenerated, this was most likely due to the use of unsuitable regeneration media. Parameters were optimised for transformation by particle bombardment (PB) of cultivars SA281, 296B and Tx430. The optimal conditions were use of 3-7 days old IEs and 4 weeks old IF callus, 4 hour pre- and post-bombardment osmoticum treatment, use of 0.6 µm gold microparticles, helium pressure of 1500 kPa and target distance of 15 cm. Using these parameters for PB, transient GFP expression was observed for up to 14, 30 and 50 days for cultivars SA281, 296B and Tx430, respectively. Further, the use of PB resulted in less tissue necrosis compared to AMT for the respective cultivars. Despite the presence of transient GFP expression, no stably transformed plants were regenerated. The establishment of regenerable ECLs and the optimization of AMT and PB parameters in this study provides a platform for future efforts to develop an efficient transformation protocol for sorghum. The development of GM sorghum will be an important step towards improving its agronomic properties as well as its exploitation for biofuel production.
Resumo:
The effects of preincubation of cut tobacco leaf explants on Agrobacterium transformation efficiency and induction of Agrobacterium virE-lacZ fusion were evaluated. Transformation efficiency was evaluated by histochemical and fluorometric analysis of beta-glucuronidase in leaf rings transformed with Agrobacterium tumefaciens strain LBA4404(pKIWI105). The transformation efficiency increased by 2-fold, 5-fold, and 4.3-fold upon preincubation for 24, 48, and 72 h, respectively. Preincubation for 24, 48, and 72 h increased the ability of tobacco leaf segments to induce Agrobacterium virE by 2.3-fold, 3.5-fold and 4.5-fold, respectively. The requirement of preincubation for increased transformation efficiency was obviated by the addition of 100 mu M acetosyringone to the freshly cut leaf rings cocultivated with Agrobacterium. The production of vii gene inducers by the leaf rings during the preincubation period is an important factor that contributes to increased transformation efficiency of Agrobacterium upon preincubation. (C) 1999 Elsevier Science Ireland Ltd. All rights reserved.
Resumo:
植物血红蛋白在共生固氮根瘤中主要是对固氮酶进行嫌氧保护,确保固氮酶活性,在植物根中协助氧的运输或作为感觉氧压的信号分子.豆科植物凝集素功能之一是对相应专一的根瘤菌有识别作用,并有利于根瘤菌的聚集和侵染。本论文将非豆科结瘤植物Parasponia andersonii血红蛋白基因及豌豆凝集索基因转入水稻,目的是此二基因表达后,豌豆凝集素可聚集、识别豌豆根瘤菌,并有助于它们的侵染,血红蛋白则可对根瘤菌固氮酶进行嫌氧保护,保障其发挥固氮作用,从而为实现水稻结瘤和固氮打下初步基础。 本论文将带有Parasponia血红蛋白基因的pL305质粒,带有潮霉素磷酸转移酶基因及Parasponia血红蛋白基因的农杆菌双元载体质粒pLX412-Hb用花粉管通道法转化水稻l用pLX412-Hb和带有Bar基因、豌豆凝集素基因、Parasponia血红蛋白基因的质粒pLHB用基因枪法转化水稻幼胚及愈伤组织,带有pLX412-Hb的Agrobactmum tumefaciens LBA4404转化烟草,得到如下结果: 1.用pL305质粒花粉管通道法转化水稻,运作1512朵花,得到707粒种子.将230粒种子萌发,发芽220粒;白化苗4株,成苗206株;计发芽率96%,白化苗率1.7%,成苗率90%。取120株提取DNA以Parasponia血红蛋白基因为探针进行点杂交,有6株为阳性结果,阳性率5%.再取4株DNA点杂交阳性植株DNA,以Parasponia血红蛋白基因为探针进行Southem杂交,有3株有阳性结果,阳性率为75%,照此推算转化植株约占总植株的4%.目前,这些转基因植株已开花结实。 2.用pLX412-Hb质粒花粉管通道法转化水稻,运作743朵花,得到340粒种子。将120粒种子萌发,发芽117粒,白化苗3株,成苗111株;计发芽率97. 5%,白化苗率2. 5%,成苗率92. 5%.取30株提取DNA以Parasponia血红蛋白基因为探针进行点杂交,有4株为阳性结果,阳性率13%。再取4株DNA点杂交呈阳性的植株DNA,以Parasponia血红蛋白基因为探针进行Southern杂交,有2株有阳性结果,阳性率为50%,照此推算转化植株约占总植株的7%。目前部分转基因植株巳开花结实. 3.用pLX412 - Hb质粒基因枪法转化水稻幼胚及愈伤组织,抗性筛选得到15株再生植株,以Parasponia血红蛋白基因为探针进行点杂交,有14株为阳性结果,阳性率93%.取7株DNA点杂交呈阳性的植株DNA,以Parasponia血红蛋白基因为探针进行Southern杂交,都为阳性结果,阳性率为100%,照此推算转化植株约占总植株的93%.目前,部分转基因植株已开花结实. 4.用pLX412 -Hb质粒通过Agrobacterrum tumeFaciens LBA4404转化烟草,抗性筛选得到的再生植株以Parasponia血红蛋白基因为探针进行Southern杂交,结果为阳性. 5.用pLHB基因枪法转化的愈伤组织,抗性筛选得到已分化出绿芽点的愈伤组织,以Parasponia血红蛋白基因为探针或以豌豆凝集素基因为探针进行Southern杂交,杂交结果均为阳性. 6.最近国外巳发现大麦有血红蛋白基因.本论文以大麦血红蛋白cDNA为探针对未转基因的水稻进行Southern杂交,结果有阳性带。说明水稻有与大麦血红蛋白基因高度同源序列。以Parasponia血红蛋白基因为探针时杂交结果为阴性,说明水稻血红蛋白基因与Parasponiaa血红蛋白基因核苷酸序列相差较大. 7.提取Southern杂交证明有Parasponia血红蛋白基因整合的水稻根及叶总RNA,以Parasponia血红蛋白基因cDNA为探针进行RNA点杂交,结果根总RNA为阳性,叶总RNA为阴性。初步证明Parasponia血红蛋白基因在水稻根中表达。 8.提取未转基因的水稻根及叶RNA,以大麦血红蛋白基因cDNA为探针进行RNA点杂交,结果:根总RNA为阳性结果,叶总RNA为阴性结果.初步证明水稻血红蛋白基因在水稻根中表达。 总之,本论文证明已将Parasponia血红蛋白基因整合进水稻植株染色体,将豌豆凝集素基因、Parasponia血红蛋白基因整合进水稻愈伤组织染色体,初步证明水稻有血红蛋白基因,内外源血红蛋白基因都有组织特异性表达,从而为本研究的战略设想奠定初步基础。
Resumo:
将pBIN35S-mGFP4质粒转入受体菌DH5α中,扩繁后提取纯化质粒DNA,待棉花盛花期时,用花粉管通道转化方法将其注射到授粉24小时左右的子房中。在被检测的950个发育10~20天左右的幼胚中,发现七个幼胚在蓝光(460~490nm)激发下发出绿色荧光,而对照发出程度不同的红色荧光。将收获的“转化种子”浸泡萌发得到生长5~6天的黄化无菌苗,在200粒种子来源的无菌苗中,检出两棵转化植株。在紫外光照射灯下转化植株发出绿色荧光,其叶片和下胚轴横切面在蓝光激发下也与对照明显不同。PCR及Southern blotting结果均证实转化植株的真实性,从而为花粉管通道转化方法的可行性提供了直接可靠的细胞及分子生物学证据。 将GFPmut1质粒的gfp通过一端平接一端粘接后重组到pBI121的BamH1和Sal1限制性酶切位点从而代替GUS基因,然后将新的重组质粒用三亲交配法转入到LBA4404菌株中得到双元载体,用于棉花下胚轴切段的转化。结果表明,gfp象gus一样可作为报告基因用于农杆菌介导的棉花转化。在对筛选培养基上生长的“抗性愈伤”进一步进行报告基因检测时,只需手持紫外灯就可以检出GFP阳性愈伤,大大减少了工作量和试验费用。 另外,在进行农杆菌转化前的棉花卡那霉素敏感性实验中发现,卡那霉素对棉花下胚轴的愈伤组织形成和增殖均有明显的抑制作用,随其浓度的增加,愈伤组织形成的频率降低,增殖的倍数减小;当浓度增加到100mg/L时,愈伤组织严重褐化,其正常生长受到完全抑制;下胚轴形态学上端切段较下端更易受卡那霉素的影响。
Resumo:
本论文主要包括以下两部分内容: 一、真菌诱导子对青蒿发根生长和青蒿素生物合成的影响 用3种真菌诱导子[大丽花轮枝孢(Verticillium dahliae Kleb.)、葡枝根霉(Rhizopus stolonifer (Ehrenb. ex Fr.) Vuill)和束状刺盘孢(Colleto trichumdematium (Pers.) Grove)]分别处理青蒿(Ar temisia annuaL.)的发根,这3种真菌诱导子均能促进发根中青蒿素的合成,其中以大丽花轮枝孢的诱导效果最好;对细胞生长均没有明显影响。经大丽花轮枝孢处理的发根中青蒿素含量达1. 12 mg/gDW,比对照(0. 77 mg/g DW)提高45%。诱导子的作用效果与诱导子浓度、诱导子作用时间及发根的生长状态有关。对大丽花轮枝孢来说,诱导子作用的最适浓度为每毫升培养基含糖0.4 mg;发根在指数生长末期对诱导作用最敏感:在加入诱导子4d后收获发根,发根中的青蒿素含量最高。 二、早花基因FPF1、co对青蒿开花时间的影响及开花与青蒿素生物合成的相关性 1.将来源于拟南芥的早花基因Flowering Promoting Factorl (FPFl)插入到植物表达载体pBI121中,构建CaMV 35S启动子控制下含FPFl基因的植物表达载体pBI121FPF/,用含有pBI121FPF/质粒的根癌农杆菌(Agrobacterium tumefaciens)LBA4404感染青蒿(Artemisia annua L.)叶片并诱导丛生芽,经卡那霉素筛选,获得转基因抗性植株。PCR、 PCR-Southem blot及Southern blot检测表明,外源基因FPFI已整合到青蒿基因组中:RT-PCR及RT-PCR Southern blot分析表明,外源基因在转录水平上已有表达。在短日照条件下,FPF1转基因植株的开花时间较对照提前20天左右,但提早开花的转基因植株与未开花的对照其青蒿素含量无明显差异,即提早开花并不能使开花植株的青蒿素含量有所提高,开花与青蒿素合成之间可能没有直接的关系。 2.将拟南芥的早花基因CONSTANS (CO)置于CaMV 35S启动子之下,通过根癌农杆菌(Agrobacterium tumefaciens)LBA4404介导转入青蒿(Artemisia annuaL.),使之在青蒿中表达,并得到了抗性植株。PCR、PCR-Southem blot及Southemblot检测表明,外源基因co已整合到青蒿基因组中;RT-PCR及RT-PCR Southemblot分析表明,外源基因在转录水平上已有表达。在短日照条件下,co转基因植株的开花时间较对照提前2周左右,但提早开花的转基因植株的青蒿素含量与未丌花的对照无明显差异,即植株开花前青蒿素含量的提高并不是由于开花本身引起的,再次证明,开花与青蒿素合成之间可能没有直接的关系。
Resumo:
过氧化氢(Hydrogen peroxide,H2O2)是植物和病原微生物互作中快速合成的一种早期活性氧类(reactive oxygen species, ROS ),它在植物受到病原微生物侵染后引发的一系列防御反应中起着非常重要的作用,因此通过外源基因导入提高植物体内过氧化氢的含量,可以增强植物的广谱抗病性。葡萄糖氧化酶(glucose oxidase, GO)可以催化β-D-葡萄糖氧化生成过氧化氢和葡萄糖酸,此酶已在数种细菌和真菌中检测到,但在植物和动物中仍未发现。为了尝试将此酶应用于水稻广谱抗病基因工程,本研究将葡萄糖氧化酶基因插入具有潮霉素抗性选择标记的双元载体pCAMBIA1301,新构建为水稻高效表达载体pCAG1301。将此质粒导入根癌农杆菌(Agrobacterium tumefaciens )菌株LBA4404后,转化粳稻(Oryza sativa )品种日本晴(Nipponbare)成熟胚来源的愈伤组织和幼胚,并由筛选出的潮霉素抗性愈伤组织分化再生植株。对所得到的潮霉素抗性植株的Southern杂交分析表明GO基因已整合到受体基因组,为单拷贝或双拷贝插入。利用过氧化氢与淀粉-碘化钾反应显蓝色的特性检测到了转基因植株产生的过氧化氢,证实GO基因表达产生的葡萄糖氧化酶已经在水稻中发挥功能,这是将GO基因转入单子叶植物的首例报道。 基于过氧化氢诱导的植物防御反应没有种属专一性的优点,可以预期所得转基因水稻植株很可能对水稻的多种病原菌具有良好的抗性。已完成的抗病性鉴定表明,所得转基因水稻植株对稻瘟病具有良好的抗性。
Resumo:
Lhcb2基因是LHCII基因家族中的一个重要成员。目前,对于其特性、结构和功能还不清楚。本文对豌豆Lhcb2基因的克隆、表达、功能及其在大肠杆菌中的表达产物与色素在体外的重组进行了比较系统的探讨,主要的结果如下: 1.采用RT-PCR技术,从豌豆幼叶中克隆了一个约800 bp的Lhcb2 cDNA。以特异探针进行Southern杂交的结果初步证明,Lhcb2基因以单拷贝形式存在于豌豆基因组中,这在文献中尚未见报道。 2.不同光照时间和温度对豌豆幼苗进行处理的RT-PCR,Northem blotting分析表明,Lhcb2基因转录水平上的表达受光照的控制,且明显地表现出对光照时间的依赖性。用400 μmolm-2.s-1的白光照射0~1.5小时Lhcb2基因未见表达,而在光照2小时以上则大量表达,推测该基因的表达可能要求某种(或某些)需光中间物的合成和积累。温度对Lhcb2基因的表达亦有显著的影响,相同的光照处理,4 ℃下Lhcb2基因的表达量比25℃下的表达量低一倍左右。 3.将豌豆Lhcb2基因反向插入植物表达载体pBIl21中,构建CaMV 35S启动子控制下反义Lhcb2基因的植物表达载体pBIantiLhcb2,通过农杆菌LBA4404介导,在Kan浓度为100 mg/L的筛选培养基上,获得120个抗Kan阳性植株。PCR检测表明至少有80个抗性植株为PCR阳性反应。Southern blotting分析表明,外源反义Lhcb2基因已整合到烟草基因组中。转基因植株在表型上主要表现为三大类型:叶色类似于未转基因的绿色植株、叶色发黄的植株、叶色发白甚至枯死的植株。这几类转基因植株光谱特性的分析表明,Lhcb2基因不仅影响光能的捕获,而且还可能参与激发能分配的调节作用。 4.将豌豆的Lhcb2基因亚克隆至原核表达载体pET-3d上,通过定点突变使其在大肠杆菌BL2l(DE3)中得到高效表达,其表达量约占大肠杆菌总蛋白的40%,并经纯化后获得了电泳纯的Lhcb2蛋白。应用改进的液氮/室温冻融重组方法将纯化的蛋白与色素进行体外重组,建立了高效的重组系统。实验结果表明重组后所获得的LHCB2单体与用生化方法从菠菜类囊体膜中分离纯化的天然LHC II单体相比较,其在部分变性胶的电泳行为,低温荧光发射光谱和激发光谱,以及室温吸收光谱和CD光谱的特征等方面都非常相似,说明大量表达的Lhcb2蛋白与色素已成功地重组,并具有与天然的LHCII单体相类似的组成和结构,这在国际上尚属首次。在此基础上又构建了N端和C端氨基酸残基缺失的突变体,并对这些缺失的氨基酸残基在LHCB2中的可能作用进行了初步的研究。结果表明,N端的前12个氨基酸残基、C端的前10个氨基酸残基和第11位的色氨基酸残基对LHCB2单体的形成不是必需的。 此外,从菠菜中纯化了LHCII,并对其多肽和色素组成及其光谱特性进行了比较系统的研究。同时对用不同浓度OGP和Mg2+处理所获得的不同聚集程度的LHCII的光谱特性进行了研究,并对Mg2+在其中的可能作用进行了初步的探讨。
Resumo:
谷胱甘肽还原酶(GR,EC1.6.4.2)是一重要的抗氧化酶,许多生理学和遗传工程研究都证明GR酶在抗氧化中的重要作用。但改变GR酶怎样影响植物的抗氧化系统却不清楚。GR是抗坏血酸-谷胱甘肽循环途径中的重要组成部分,其功能必然与其密切相关。本文用RNAi技术获得具有较低GR酶活性的转基因烟草,系统测定了非胁迫条件和胁迫条件下抗坏血酸-谷胱甘肽循环的变化,得出以下主要结果: 1.选择一烟草叶绿体GR酶编码基因(X76293, gi: 431954)进行RNAi载体构建,构建好的双元载体转化根癌农杆菌LBA4404,然后侵染转化烟草叶圆片。获得的转基因烟草具有30-70%的GR酶活性。分子检测结果表明GR在RNA和蛋白水平上与GR酶活性的变化一致。文中我们第一次用2-D电泳对烟草中GR同工酶进行分析,并确定发生抑制的GR同工酶在细胞中的定位。2-D电泳后的Western杂交检测到烟草的10种GR同工酶,pI值分布在4.5-6.3,其中3种GR同工酶定位在叶绿体内,其蛋白量占据所有GR酶含量的大部分。RNAi发生在叶绿体内和叶绿体外,表明发生抑制的GR同工酶的基因序列具有很高的同源性。igr转基因烟草在表型上与野生型对照烟草无明显差异。 2.所有igr转基因植株和对照植株中的活性氧(O2-和H2O2)、MDA含量和光合作用都无明显差异,表明正常生长条件下GR酶活性的降低不会引起氧化胁迫。测定正常生长条件下igr转基因烟草中谷胱甘肽库的变化。结果表明与对照烟草相比,GR酶活性降低70%会引起转基因植株中GSH/GSSG比率明显降低,而GSH和GSSG的含量稍有增加;测定抗坏血酸-谷胱甘肽循环的变化,结果显示igr转基因烟草中DHAR和MDHAR的酶活性升高,表明非胁迫条件下较低的GR酶活性可能会诱导抗坏血酸-谷胱甘肽循环不能正常的运转。这一作用可能与改变的谷胱甘肽库有关。GR酶活性降低30%的转基因烟草中未检测到这些变化,表明70%的GR酶活对于非胁迫条件下igr转基因烟草可能是足够的。 3. MV处理结果显示,igr转基因烟草的离体叶圆片和活体植株在MV处理后都发生比对照烟草严重的光漂白作用。igr转基因烟草的活性氧和MDA含量明显高于对照烟草,igr转基因烟草的光合作用明显低于对照烟草。以上这些指标表明igr转基因烟草对MV处理更为敏感。MV处理条件下igr转基因烟草谷胱甘肽的含量明显高于对照烟草,但是GSH/GSSG的比率明显低于对照烟草,GR酶活性仍明显低于对照烟草,表明在MV胁迫条件下igr转基因烟草中较低的GR酶活性不能有效的将GSSG还原生成GSH。igr转基因烟草中较高的谷胱甘肽净含量说明其谷胱甘肽的合成能力提高,但这仍不能补偿胁迫条件下较低GR酶引起的GSH/GSSG比率降低。MV处理条件下igr转基因烟草和对照烟草相比ASC的含量大大降低,导致DHA/ASC明显升高。测定MDHAR和DHAR的结果表明,MV处理后igr转基因烟草的MDHAR酶活性明显降低,这表明较低的GR酶活性引起ASC再生循环受到抑制。MV处理后较低的GR酶还引起igr转基因烟草中APX的活性大大降低。以上这些结果表明MV处理条件下降低GR酶活性会削弱抗坏血酸-谷胱甘肽循环,从而引起活性氧的大量积累,造成严重的氧化伤害。 4.低温处理的结果和MV处理的结果稍有不同。在GR酶活性较高的i2转基因烟草中所有检测指标与对照烟草无明显差异。而GR酶活性较低的i21、i28和i42植株与对照烟草相比表现出明显差异。低温下生长的对照烟草叶绿素含量明显高于i21、i28和i42植株。i21、i28和i42中活性氧(O2-和H2O2)和MDA的含量都明显高于对照烟草,表明低温处理下i21、i28和i42受到更严重的胁迫伤害。与MV处理后的变化相似,低温处理后i21、i28和i42中较低的 GR酶活性导致GSH/GSSG大大降低,ASC再生循环受抑制,APX活性明显降低,从而使抗坏血酸-谷胱甘肽循环不能高效的清除活性氧,导致ROS和MDA的大量积累,造成严重的低温伤害。
Resumo:
Phaseolus vulgaris L. e considerada recalcitrante a transformacao por Agrobacterium tumefaciens. Contudo, alteracoes no meio de co-cultivo, utilizacao de linhagens hipervirulentas de Agrobacterium e de vetores binarios contendo genes vir demostraram que o feijoeiro e susceptivel a essa bacteria. O objetivo do presente trabalho foi estudar o efeito da sonificacao nos tecidos vegetais de feijoeiro, bem como a penetracao da Agrobacterium nas camadas subepidermicas do tecido vegetal, usando a metodologia SAAT ("Sonification-Assisted Agrobacterium-mediated Transformation"). A variedade de feijoeiro utilizada foi a Olathe Pinto, a linhagem de A. tumefaciens foi LBA4404:pTOK.Os embrioes de feijao foram pre-tratados po 14 dias em meio de multibrotacao e, entao submetidos a sonificacao (de 0 ou 60 segundos) na presenca de Agrobacterium. Apos a inoculacao foram co-cultivados por 24 horas em meio liquido seguido de 48 horas em meio solido, ambos, contendo 20 m. L -1 de acetoceringona. Os explantes inoculados foram fixadas em solucao de Karnovsk para avaliacoes em microscopia optica e eletronica de varredura. As analises da microspia demostraram a presenca de rupturas na epiderme, quebras da parede celular e invasao da Agrobacterium nos tecidos subepidermicos. Os reultados demostraram que o metodo SAAT e uma tecnica viavel para a inoculcao de Agrobacterium em explantes de P. vulgaris.
Resumo:
O objetivo do presente trabalho foi otimizar o sistema de transformação genética de embriões somáticos de soja [Glycine max (L.) Merr.] utilizando a biolística e o sistema Agrobacterium de maneira integrada. Os antibióticos, adicionados ao meio de cultura para supressão da bactéria após a transferência do transgene, foram o alvo do estudo. Inicialmente, comparou-se o efeito de diferentes tratamentos com antibióticos sobre o tecido embriogênico de soja e sua eficiência na supressão da linhagem LBA4404 de Agrobacterium tumefaciens durante o processo de transformação. A carbenicilina (500 mg/l) apresentou efeitos diferentes sobre o tecido vegetal das duas cultivares testadas. Os tecidos embriogênicos da cv. IAS5 não apresentaram diferenças significativas em relação ao controle, enquanto que a proliferação dos embriões somáticos da cv. Bragg foi três vezes maior com a adição deste antibiótico ao meio de cultura. Contudo, a presença da carbenicilina nas duas concentrações testadas (500 e 1000 mg/l) não foi eficiente para supressão de Agrobacterium. Por outro lado, nos tratamentos com cefotaxima sozinha (350 e 500 mg/l), ou cefotaxima (250 mg/l) + vancomicina (250 mg/l) esta bactéria foi completamente suprimida da superfície dos embriões somáticos após 49 dias de tratamento. No entanto, enquanto a presença de cefotaxima, em qualquer concentração, foi prejudicial à sobrevivência do tecido embriogênico, a combinação de cefotaxima + vancomicina não afetou significativamente os embriões somáticos de soja até os 63 dias de tratamento. Portanto, os resultados indicam que o tratamento com cefotaxima + vancomicina por um período de 49 - 63 dias é o mais adequado para a transformação genética de soja, por suprimir Agrobacterium e apresentar mínimos efeitos sobre o tecido embriogênico. Por fim, conjuntos de embriões somáticos de soja foram transformados e tratados com a combinação recomendada de antibióticos para avaliação da eficiência do método na obtenção de transformantes estáveis. Foram obtidos 48 e 232 clones higromicina-resistentes para Bragg e IAS5, respectivamente. Para cv. Bragg, 26 plantas foram obtidas de um único clone, enquanto 580 plantas foram regeneradas de 105 clones da cv. IAS5. As plantas transgênicas eram férteis e morfologicamente normais. A presença do transgene no genoma destas plantas foi confirmada por análises moleculares. Portanto, a adequação dos antibióticos permitiu o desenvolvimento de um método de transformação altamente eficiente para soja. Os resultados do presente trabalho constituem o primeiro registro (1) do efeito de antibióticos sobre tecidos de soja ou de leguminosas e (2) de obtenção de transformantes estáveis de soja utilizando a biolística e o sistema Agrobacterium de maneira integrada.
Resumo:
Flowering is a fundamental process in the life cycle for plant. This process is marked by vegetative to reproductive apical meristem conversion, due to interactions between several factors, both internal and external to plant. Therefore, eight subtractive libraries were constructed using apical meristem induced or not induced for two contrasting species: Solanum lycopersicum cv. Micro-Tom and Solanum pimpinellifolium. Several cDNAs were identified and among these, were selected two cDNAs: one homologous cDNA to cyclophilin (LeCYP1) and the other to Auxin repressed protein (ARP). It has observed that LeCYP1 and ARP genes are important in the developmental process to plants. In silico analysis, were used several databases with the exclusion criterion E-value <1.0x10-15. As a result, conservation was observed for proteins analyzed by means of multiple alignments and the presence of functional domains. Then, overexpression cassettes were constructed for the ARP cDNA in sense and antisense orientations. For this step, it was used the CaMV35S promoter. The cDNA orientation (sense or antisense) in relation to the promoter was determined by restriction enzymes and sequencing. Then, this cassette was transferred to binary vector pZP211 and these cassettes were transferred into Agrobacterium tumefaciens LBA4404. S. lycopersicum cv. Micro-Tom (MT) and MT-Rg1 plants were transformed. In addition, seedlings were subjected to hormone treatments using a synthetic auxin (- naphthalene acetic acid) and cyclosporin A (cyclophilin inhibitor) treatments and it was found that the hormone treatment there were changes in development of lateral roots pattern, probably related to decreases in auxin signaling caused by reduction of LeCYP1 in MT-dgt plants while cyclosporin A treatments, there was a slight delay in flowering in cv. MT plants. Furthermore, assay with real-time PCR (RT-qPCR) were done for expression level analysis from LeCYP1 and ARP in order to functionally characterize these sequences in tomato plants.
Etr1-1 gene expression alters regeneration patterns in transgenic lettuce stimulating root formation
Resumo:
We have evaluated the transformation efficiency of two lettuce ( Lactuca sativa L.) cultivars, LE126 and Seagreen, using Agrobacterium tumefaciens- mediated gene transfer. Six- day- old cotyledons were co- cultivated with Agrobacterium cultures carrying binary vectors with two different genetic constructs. The first construct contained the beta- glucuronidase gene ( GUS) under the control of the cauliflower mosaic virus 35S promoter ( CaMV 35S), while the second construct contained the ethylene mutant receptor etr1- 1, which confers ethylene insensitivity, under the control of a leaf senescence- specific promoter ( sag12). Tissues co- cultivated with the GUS construct showed strong regeneration potential with over 90% of explants developing callus masses and 85% of the calli developing shoots. Histochemical GUS assays showed that 85.7% of the plants recovered were transgenic. Very different results were observed when cotyledon explants were co- cultivated with Agrobacteria carrying the etr1- 1 gene. There was a dramatic effect on the regeneration properties of the cultured explants with root formation taking place directly from the cotyledon tissue in 34% of the explants and no callus or shoots observed initially. Eventually callus formed in 10% of cotyledons and some organogenic shoots were obtained ( 2.86%). These results indicate that the ethylene insensitivity conferred by the etr1- 1 gene alters the normal pattern of regeneration in lettuce cotyledons, inhibiting the formation of shoots and stimulating root formation during regeneration.
Resumo:
Flowering is a fundamental process in the life cycle for plant. This process is marked by vegetative to reproductive apical meristem conversion, due to interactions between several factors, both internal and external to plant. Therefore, eight subtractive libraries were constructed using apical meristem induced or not induced for two contrasting species: Solanum lycopersicum cv. Micro-Tom and Solanum pimpinellifolium. Several cDNAs were identified and among these, were selected two cDNAs: one homologous cDNA to cyclophilin (LeCYP1) and the other to Auxin repressed protein (ARP). It has observed that LeCYP1 and ARP genes are important in the developmental process to plants. In silico analysis, were used several databases with the exclusion criterion E-value <1.0x10-15. As a result, conservation was observed for proteins analyzed by means of multiple alignments and the presence of functional domains. Then, overexpression cassettes were constructed for the ARP cDNA in sense and antisense orientations. For this step, it was used the CaMV35S promoter. The cDNA orientation (sense or antisense) in relation to the promoter was determined by restriction enzymes and sequencing. Then, this cassette was transferred to binary vector pZP211 and these cassettes were transferred into Agrobacterium tumefaciens LBA4404. S. lycopersicum cv. Micro-Tom (MT) and MT-Rg1 plants were transformed. In addition, seedlings were subjected to hormone treatments using a synthetic auxin (- naphthalene acetic acid) and cyclosporin A (cyclophilin inhibitor) treatments and it was found that the hormone treatment there were changes in development of lateral roots pattern, probably related to decreases in auxin signaling caused by reduction of LeCYP1 in MT-dgt plants while cyclosporin A treatments, there was a slight delay in flowering in cv. MT plants. Furthermore, assay with real-time PCR (RT-qPCR) were done for expression level analysis from LeCYP1 and ARP in order to functionally characterize these sequences in tomato plants.
