美容杜鹃叶片再生及愈伤组织耐热生理研究

以美容杜鹃幼叶为外植体,通过三因素三水平的正交试验,探究不同培养基、激素对愈伤组织诱导、分化和植株再生的影响,并对愈伤组织进行38℃热胁迫,探讨热胁迫下其耐热生理指标随时间的变化规律。结果表明:(1)愈伤组织诱导和芽分化最佳培养基均为Read+0.1mg/L NAA+0.2mg/L TDZ;最佳壮苗培养基为改良MS+0.1mg/L KT+0.2mg/L NAA;最佳生根培养基为1/2改良MS+2.0mg/L GA3。(2)随着热胁迫时间的延长,愈伤组织中的可溶性糖和游离脯氨酸含量变化不明显,而MDA和可溶性蛋白质的含量呈上升趋势,超氧化物歧化酶(SOD)和过氧化物酶(POD)活性则表现为先升后降趋势;其中,MDA含量、可溶性蛋白质含量、SOD和POD活性随时间变化显著,可作为评价美容杜鹃耐热性的生理指标。     

芥菜型油菜抗虫转基因植株及其后代株系的研究*

带有1～2mm子叶柄的芥菜型油菜子叶经农杆菌感染后,培养在附加10～20mg/L卡那霉素的MS选择培养基上筛选转化愈伤组织及不定芽。卡那霉素抗性苗相继在含30～50mg/L卡那霉素的选择培养基上继代培养,再转移到含20mg/L卡那霉素的生根培养基上诱导生根。以苏云金杆菌杀虫晶体蛋白基因为探针,进行Southern blot分子杂交,得到阳性结果。PCR分析也证明外源基因整合到油菜基因组并稳定传递到后代。转基因植株的抗虫性和卡那霉素抗性在自交后代中得到保持,筛选得到纯合的转基因植株后代株系。     

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。     

皂质芦荟的组织培养

将皂质芦荟的茎段及幼苗作为外植体进行组织培养,试验结果表明：皂质芦荟的茎段经40d左右可诱导形成愈伤组织,再经20d萌生再生芽：幼苗培养需要30d左右基部直接分化再生芽。同时经试验筛选出愈伤组织形成、再生芽分化和生根的最适培养基为：MS＋6－BA 2.0mg/L NAA 0.1mg/L、MS 6-BA 3.0mg/L NAA 0.1mg/L和MS NAA 0.3mg/L。     

根癌农杆菌对健康和患丛枝病泡桐的遗传转化

选取健康及患丛枝病泡桐（Paulownia spp.)为材料,建立组织培养和植株再生系统,以茎段作为转化受体,诱导分化和生根的最佳激素组合分别是MS＋BA4mg/L NAA0.2mg/L和1／2MS＋KT0.5mg/L IBA0.25mg/L。芽分化频率可达22．8％。健康和患病泡桐的茎段经农杆菌共培养3d后,在附加50mg/Lm的选择分化培养基上培养20d左右再生出抗性芽,经培养、诱导生根,获得了转基因再生植株,建立了泡桐的遗传转化体系。PCR和Southern杂交检测证明外源基因已整合到泡桐的基因组,标记基因ITPⅡ在再生植株中也得到表达,同时对影响转化的一因素进行了探讨。     

AtNDPK2 基因转化敖汉苜蓿及其耐盐性分析

植物核苷二磷酸激酶(NDPKs),属于蛋白激酶家族,参与植物的多种生理生化过程,在植物响应非生物胁迫过程中发挥重要作用。NDPK2基因转化紫花苜蓿,对提高紫花苜蓿的耐逆性具有重要意义。试验以"敖汉"苜蓿下胚轴的再生系统为基础,通过农杆菌介导法将SWPA2驱动的AtNDPK2基因转入紫花苜蓿下胚轴,获得抗性植株。通过PCR初步检测证明该基因已经整合到"敖汉"苜蓿的基因组,阳性植株转化率为23.3%。不同浓度NaCl胁迫测定转基因植株的SOD、POD活性及质膜相对电导率、MDA含量,结果发现在0.4%~1.0%NaCl胁迫下转基因植株的SOD、POD酶活性显著高于对照,相对电导率、MDA含量显著的低于对照,进一步说明AtNDPK2基因的转入增强了"敖汉"苜蓿的耐盐性。     

干旱耐逆基因（HS1）转化甘薯获得转基因植株

以甘薯（1pomoeabatatas（L.）Lam．）品种栗子香的胚性悬浮细胞为受体材料,用根癌农杆菌介导法,获得了表达除草剂抗性基因bar基因的转HSl基因甘薯植株。共计380个遗传转化的胚性细胞团,在添加2mg／L2．4-D、100mg／L Carb和10mg／L Glu（glufosinate）的固体Ms培养基上选择培养9周后,得到了12个Glu抗性愈伤组织。将这些抗性愈伤组织转移到添加1mg／L ABA、100mg／L羧苄青霉素和10mg／L Glu的固体MS培养基上,其中的3个抗性愈伤组织再生出拟转基因植株。PCR鉴定它们为转基因植株。Southern blot分析表明,HS1基因已整合到基因组中。转基因植株具有稳定的除草剂抗性。结薯观察实验结果表明,转基因植株结薯正常。     

AtNHX1基因对荞麦的遗传转化及抗盐再生植株的获得

通过农杆菌介导法将拟南芥液泡膜Na /H 反向转运蛋白基因AtNHX1转入荞麦中,在2·0mg/L6-BA、0·1mg/LIAA、1mg/LKT、50mg/L卡那霉素和500mg/L头孢霉素的MS培养基上进行选择培养,从来源于864块外植体的36块抗性愈伤组织中共获得426棵再生植株(转化频率为4·17%)。经PCR、Southern印迹分析、RT-PCR和Northern检测,初步证实AtNHX1基因已整合至荞麦基因组中。用200mmol/L的盐水对转基因植株和对照植株进行胁迫处理6周,转基因植株能够生存,而对照植株死亡。用不同浓度的NaCl溶液处理转基因植株和对照植株,发现Na 及脯氨酸含量在转基因植株中的积累水平显著高于对照植株,而K 的含量在转基因植株中的积累水平低于对照植株。次生代谢产物黄酮类化合物芦丁在转基因植株根、茎和叶片中的含量也比对照植株明显要高。这些结果表明利用基因工程手段提高作物的耐盐性是可行的。     

过表达ZmSKIP基因提高烟草抗低温胁迫的能力

以野生型和过表达ZmSKIP基因烟草为试材, 研究了低温胁迫下过表达ZmSKIP对烟草抗氧化能力的影响。测定了不同低温处理时间下过表达ZmSKIP转基因烟草T3代植株和野生型植株抗氧化酶如超氧化物歧化酶（SOD）、过氧化氢酶（CAT）、过氧化物酶（POD）活性和丙二醛（MDA）含量以及相对电导率, 结果表明, 低温下, 相对于野生型植株, 转基因烟草具有较高的抗氧化酶活性和较低的相对电导率和MDA含量, 说明过表达ZmSKIP提高了转基因植株的耐低温胁迫能力。     

转金属硫蛋白基因(MT1)烟草耐NaCl胁迫能力

为明确柽柳(Tamarix sp.)金属硫蛋白(MT1)基因过量表达对提高植物耐NaCl能力的作用,对转MT1因烟草进行分子检测和生理特性分析,结果表明具有卡那霉素抗性的转基因植株经RT-PCR Southern杂交均表现为阳性,说明外源MT1基因已整合到烟草基因组,并且得到了表达。金属硫蛋白基因的过量表达提高了转基因烟草植株的耐NaCl能力,表现为在含有150mmol/L和300mmol/L NaCl的MS培养基上,转基因植株的株高和鲜重均明显优于非转基因株系;在生理性状上表现为转基因植株丙二醛(MDA)含量明显低于非转基因株系,而超氧化物歧化酶(SOD)、过氧化物酶(POD)活性比非转基因株系明显增加。     

农杆菌介导的转化芦荟的研究

芦荟（Aloe）是美容和医疗保健工业的重要植物资源,然而基因工程途径改良芦荟鲜有报道。本实验研究了次氯酸钠、升汞不同浓度和时间对芦荟外植体的灭菌效果,比较了芦荟不同部位（叶片、叶鞘和茎段）的再生能力,利用GUS基因瞬间表达技术（X-Gluc染色）探讨了不同农杆菌对不同芦荟外植体的侵染效果,确定了G418筛选剂在芦荟转化后的最适筛选浓度,摸索了适宜于农杆菌—芦荟共培养用培养基组成和共培养条件,通过转化、筛选和移栽共获得了67棵抗性再生植株,进一步对抗性再生植株进行了PCR、Southern blotting和ELISA检测。结果表明,芦荟外植体灭菌方法为20.0%次氯酸钠溶液浸泡25min,效果优于利用0.1%升汞灭菌处理,茎部切段的再生能力高于叶片切段和叶鞘切段,适宜的共培养条件为芦荟外植体浸泡在含有农杆菌的液体共培养基中半小时后,在无菌滤纸上、24℃、10h光照共培养3天;EHA105农杆菌菌系对芦荟茎部细胞的侵染能力明显强于C58C1,EHA105侵染后GUS基因瞬时表达率达到了80.0%左右,而C58C1侵染后GUS基因瞬时表达率只有30.0%左右。G418用于筛选抗性再生芽和抗性植株的适宜浓度为10.0～25.0mg/L。PCR和Southern blotting检测证实外源基因已成功整合到芦荟基因组中,转化效率为0.9%,单拷贝整合占80.0%,2～3拷贝整合占20.0%,ELISA检测证明外源基因已在转基因芦荟中稳定表达。综上所述,初步建立了农杆菌介导转化芦荟的技术体系,为利用基因工程途径改良芦荟奠定了基础。     

Improvement of cold tolerance of the half-high bush Northland blueberry by transformation with the <Emphasis Type="Italic">LEA</Emphasis> gene from <Emphasis Type="Italic">Tamarix androssowii</Emphasis>

Previous studies have shown that the late embryogenesis abundant (LEA) gene of Tamarix androssowii can enhance the drought tolerance of transgenic tobacco. In this study, the cloned LEA gene was transformed into half-high bush Northland blueberry in order to enhance its ability to tolerate cold stress. The cephalosporin antibiotics ceftriaxone, cefotaxime and cefazolin were used to optimize transformation of leaf explants, and kanamycin sulfate was used to select for transgenic shoots. PCR and Southern blot analysis confirmed 8 transformants with LEA gene copy numbers ranging from 1 to 7. The LEA chimeric gene was found to be normally transcribed in 6 transgenic lines by RT-PCR. The 8 transgenic lines were tested for cold tolerance by measuring the activities of peroxidase (POD) and superoxide dismutase (SOD), malondialdehyde (MDA) content and relative electrolyte leakage (REL). Overexpression of the LEA gene enhanced the activity of both POD and SOD under low temperature stress conditions. Lipid peroxidation in the transgenic lines was significantly lower than in non-transgenic plants after cold stress, as determined by MDA content and REL. Thus, our findings indicate that the LEA gene confers increased cold tolerance in the Northland blueberry and implicate the metabolic pathways through which it exerts this effect.     

农杆菌介导的半夏凝集素基因(Pinellia Ternate Agglutinin Gene,pta)对小麦的遗传转化及鉴定

以甘肃主要推广春小麦品种陇春22幼胚为转基因受体材料,建立了农杆菌介导的小麦遗传转化体系。以预培养4天的幼胚愈伤组织为受体,C58c1农杆菌菌株为供体,将含有半夏凝集素基因的重组质粒pBIpta转入了小麦,经G418 25 mg/L抗性筛选、PCR检测和荧光定量PCR检测共获得转基因植株3株,外源基因的插入拷贝数分别为2、1、3。同时对转基因小麦的T₁代植株进行了PCR检测和抗虫性分析,表明半夏凝集素基因在转基因植株的后代中得到了遗传并有一定的抗蚜虫作用。     

超量表达MrCN基因提高烟草植株对TMV的抗性

利用农杆菌介导的遗传转化法将含有普通烟草Ubi．U4启动子驱动MrCN基因表达的元件导入TMV敏感烟草品种K326中,对筛选鉴定出的T0代转基因植株接种TMV,测定其接种前后不同时期的理化指标,以接种TMV的野生型植株为对照。结果显示,转基因植株和野生型植株接种TMV前叶绿素（Chl）和MDA含量YLSOD、POD和CAT酶活力均无显著差异,但接种TMV后野生型植株Chl含量逐渐降低,转基因植株Chl含量先增后降,在接种TMV后5d时转基因植株叶片Chl含量显著高于野生型植株。接种前期（0-3d）转基因植株MDA含量略低于野生型植株,但差异不显著;但接种后期（3～5d）前者的MDA含量显著低于后者。接种TMV后转基因植株中SOD、POD及CAT酶活性变化幅度较野生型植株高,以CAT的变幅最为显著。另外,Real-timePCR分析结果表明,接种TMV后3d时转基因植株删蹦、PR-1α及NrCN表达量均显著高于野生型植株。以上结果表明,通过转基因技术提高烟草抗病基NNrCN的表达量,能提高防御酶活性及病程相关基因的表达量,从而延缓植株感染TMV的发病时间,增强敏感植株对TMV的抗性。     

导入TaNHX2基因提高了转基因普那菊苣的耐盐性

我国部分地区土地盐碱化的日益严重,对作物的生长和生态环境产生了显著影响,因此通过植物基因工程手段培育耐盐碱的转基因作物品种对改善作物的生存能力和生态环境,提高作物产量具有重要的意义。采用农杆菌介导法将来自小麦(Triticum aestivum Linn)的Na⁺ /H⁺逆向转运蛋白的基因(vacuolar Na⁺/H⁺ exchanger or antiporter,简称NHX、NHE或NHA),对普那菊苣(Cichorium intybus L.cv.Puna)植株进行了遗传转化。经抗生素筛选以及针对TaNHX2基因的PCR检测和Southern杂交分析,证明获得了28株转TaNHX2基因的普那菊苣植株。用不同浓度NaCl溶液对普那菊苣野生型和T₀代种子、愈伤组织和幼苗生长情况胁迫的研究,结果表明:转TaNHX2基因普那菊苣植株表现出一定的抗性,比野生型明显提高。在300 mmol/L NaCl胁迫下转基因植株种子的出芽率、外植体出愈率和分化率是野生型植株的2-4倍,而500 mmol/L NaCl浓度为野生型和转基因外植体能否生长的临界点。在此临界值下野生型外植体或不能形成愈伤组织、或幼苗不能正常生根、或已生根幼苗不能正常成长,而转基因外植体可以继续形成愈伤组织并正常生根生长。同时对500 mmol/L NaCl胁迫下野生型和转基因普那菊苣幼苗其体内丙二醛含量(MDA)、过氧化氢酶(POD)和超氧化物歧化酶(SOD)活性进行测定,结果表明 转基因植株比野生型植株的MDA含量降低了1-3倍,POD活性提高了1-3倍,SOD活性提高了2-3倍,分析发现普那菊苣的耐盐性与其体内的丙二醛含量(MDA)、过氧化氢酶(POD)和超氧化物歧化酶(SOD)活性密切相关。     

Optimization of TaDREB3 gene expression in transgenic barley using cold‐inducible promoters

Constitutive over‐expression of the TaDREB3 gene in barley improved frost tolerance of transgenic plants at the vegetative stage of plant development, but leads to stunted phenotypes and 3‐ to 6‐week delays in flowering compared to control plants. In this work, two cold‐inducible promoters with contrasting properties, the WRKY71 gene promoter from rice and the Cor39 gene promoter from durum wheat, were applied to optimize expression of TaDREB3. The aim of the work was to increase plant frost tolerance and to decrease or prevent negative developmental phenotypes observed during constitutive expression of TaDREB3. The OsWRKY71 and TdCor39 promoters had low‐to‐moderate basal activity and were activated by cold treatment in leaves, stems and developing spikes of transgenic barley and rice. Expression of the TaDREB3 gene, driven by either of the tested promoters, led to a significant improvement in frost tolerance. The presence of the functional TaDREB3 protein in transgenic plants was confirmed by the detection of strong up‐regulation of cold‐responsive target genes. The OsWRKY71 promoter–driven TaDREB3 provides stronger activation of the same target genes than the TdCor39 promoter. Analysis of the development of transgenic plants in the absence of stress revealed small or no differences in plant characteristics and grain yield compared with wild‐type plants. The WRKY71–TaDREB3 promoter–transgene combination appears to be a promising tool for the enhancement of cold and frost tolerance in crop plants but field evaluation will be needed to confirm that negative development phenotypes have been controlled.     

Two critical factors are required for efficient transformation of multiple soybean cultivars: <Emphasis Type="Italic">Agrobacterium</Emphasis> strain and orientation of immature cotyledonary explant

An efficient transformation system was developed for multiple soybean [Glycine max (L.) Merrill.] cultivars using Agrobacterium-mediated gene transfer. A significantly high number of hygromycin-resistant somatic embryos (SEs) was obtained when immature zygotic cotyledons were inoculated with Agrobacterium tumefaciens strain KYRT1 and when the abaxial side of explants was oriented upwards (i.e., the adaxial side of explants was in contact with the medium). Most hygromycin-resistant SEs on selective medium were induced along the periphery of the abaxial side of cotyledonary explants. Extended periods of selection (up to 10 weeks post-cocultivation) increased the frequency of somatic embryogenesis, and more than 50% of selected SEs tested positive for beta-glucuronidase (GUS). Following maturation and regeneration of selected SEs, ten independent transgenic soybean plants of cv Jack were obtained, and the overall transformation frequency ranged from 1.1 to 1.7%. Six and two transgenic plantlets were obtained from cvs Dwight and Williams, respectively. In addition, transgenic suspension lines were established from cvs Jack, Williams, Dwight, Rend and Ina. Molecular analysis of embryogenic lines and/or transgenic plants, established from different cultivars, confirmed stable integration, expression, and/or inheritance of transgenes in both T0 and T1 plants.     

高羊茅和黑麦草农杆菌介导转化体系的研究

利用C58C1农杆菌菌系（携带的表达载体上含GUS基因和nptII基因）感染4个草坪草品种追寻者、爱神特、腾跃和守门员成熟胚来源的愈伤组织,共培养后部分愈伤组织进行X-Gluc组织化学染色检测,其余愈伤组织在含G418 10-25 mg/L的MS改良培养上先后筛选抗性愈伤组织和分化抗性再生植株,对移栽成活的144棵抗性再生植株分别进行了ELISA检测、PCR检测和组织化学染色检测。愈伤组织阶段X-Gluc染色检测结果表明,4个草坪草品种GUS基因瞬间表达率8.6%～46.9%,爱神特愈伤组织对农杆菌侵染最为敏感,其次是腾跃和守门员,追寻者最不敏感;ELISA检测结果表明,45株呈现阳性,证明nptII基因已转入草坪草并已表达;PCR检测结果与ELISA检测结果一致,表明nptII基因确实已经整合到了草坪草基因组中,且没有发生沉默现象;转基因植株X-Gluc染色检测结果表明,GUS基因在43株中得到了稳定表达,在2株中发生了沉默现象。4个草坪草品种抗性再生植株分化率0～43.5%,转化率0～21.5 %。结果还表明,GUS基因瞬间表达率与稳定转化率在草坪草上很不一致,不能作为衡量基因型转化效果的指标。     

Transformation of pollen embryo-derived explants by <Emphasis Type="Italic">Agrobacterium tumefaciens</Emphasis> in <Emphasis Type="Italic">Hyoscyamus niger</Emphasis>

Leaf, root, stem, petiole, hypocotyl, and zygotic embryo explants, as well as pollen embryoids, and redifferentiated tissues from pollen embryoid-derived plantlets of Hyoscyamus niger L. (black henbane) were inoculated with Agrobacterium tumefaciens, harboring binary vectors (pGS Gluc1) and then cultured on media containing kanamycin. Transient -glucuronidase activity and kanamycin resistant callus formation were influenced by explant origin. Transgenic calluses were obtained at a frequency of up to 30% from all the explants tested. However, transgenic shoots were obtained only from the hypocotyl of plantlets derived from pollen embryoids. Transformation was confirmed by the ability of leaf segments to produce kanamycin resistant calluses, -glucuronidase histochemical and flurometric assays, polymerase chain reaction and Southern blot analysis. The results show that pollen embryoid-derived explants may be an alternative source for both efficient transformation and regeneration of transgenic plants in recalcitrant species.     

文心兰原球茎形态发生与可溶性物质及抗氧化酶的关系

以文心兰切花品种'南茜'无菌苗为材料,取其茎尖通过组织培养诱导形成原球茎和幼苗,观察并分析了原球茎各形态发生阶段的特征及其可溶性糖和蛋白质含量、抗氧化酶(POD、CAT和SOD)活性以及相关同功酶(POD、EST和SOD)的变化.结果显示:(1)文心兰原球茎形态发生可分为外植体期、外植体膨大期、愈伤组织期、原球茎形成期、原球茎成熟期、叶鞘伸展期、顶端腋芽发育期及幼苗期8个阶段.(2)可溶性糖和蛋白质含量均在叶鞘伸展期出现最大峰值;POD活性在外植体膨大期、CAT和SOD活性在愈伤组织期分别出现最大峰值.SOD同工酶的2条酶带在愈伤组织期到幼苗期交替出现;EST同工酶在原球茎形成期有2条特异酶带.研究表明,可溶性糖和蛋白质的含量以及POD、CAT、SOD活性的特异变化与文心兰茎尖脱分化及原球茎再分化的实现密切相关,不同类型的同工酶在原球茎同一发生阶段表现出较大差异,EST同工酶的2条特异酶带可作为原球茎形成的标志.