酵母pro2基因转化紫云英的研究

用外植体－农杆菌共培养法将酵母脯氨酸合成酶基因２（ｐｒｏ２）导入豆科牧草紫云英,获得转基因植株。Ｓｏｕｔｈｅｒｎ ｂｌｏｔ分析检测到转化植株基因组中存在外源ＤＮＡ的同源顺序,证明酵母ｐｒｏ２基因已整合到紫云英细胞基因组中。转化植株具有强的ＮＰＴⅡ酶活性,而对照植株呈阴性反应。在含０．５％ＮａＣｌ的培养基上,紫云英植株内游离脯氨酸含量增高,一些转化植株叶片内游离脯氨酸含量显著高于对照,而且耐盐性有所     

转HS1~(pro1)基因番茄植株的获得

目的:为了减少根结线虫对番茄的危害,研究并获得转抗线虫基因HS1pro1番茄植株。方法:在鉴定表达载体之后,采用CaCl2法制作农杆菌EHA105感受态细胞,然后用冻融法将HS1pro1基因转入农杆菌中。通过农杆菌介导法将HS1pro1基因导入无菌番茄外植体中,获得抗根结线虫转化再生植株。用卡那霉素筛选到再生植株后,提取抗性芽的基因组,利用设计好的引物进行PCR鉴定。结果与结论:目的基因已整合到番茄基因组中,获得了转HS1pro1基因番茄植株。     

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。     

抗羟脯氨酸水稻变异系的筛选及其特性的研究

利用Hyp反复筛选经EMS处理的水稻愈伤组织,得到4个抗性细胞系。它们的游离脯氨酸含量高于对照2—25倍。Hyp(2 mmol/L)和NaCl(1%)胁迫对M_1、M_2变异系γ-谷氨酰磷酸合成活力及游离脯氨酸积累的影响呈一定的正相关性。变异系在0.8%,15NaCl 培养基中分化出植株。与对照相比,各变异系在愈伤组织、植株水平上均表现较强的耐盐性,且与游离脯氨酸的积累量呈正相关。     

牧草植物鹰嘴紫云英的遗传转化

鹰嘴紫云英(Astragalus cicer)是一种优良的豆科牧草。 15kD玉米醇溶蛋白是一种富硫的蛋白质,含硫氨基酸占总氨基酸量的15.63%。本文通过农杆菌(Agrobacterium)的介导将rbcS启动子调控的15kD玉米醇溶蛋白基因的嵌合质粒导入鹰嘴紫云英,得到转化的植株。这些植株具有NPTⅡ酶活性,抗卡那霉素。Southern blot分子杂交表明,15kD玉米醇溶五白基因已转化并整合入鹰嘴紫云英的核基因组中。     

太谷核不育小麦花药内游离脯氨酸和总氨基酸含量的变化及其与育性的关系

本文对显性单基因控制的太谷核不育小麦不同发育阶段的可育株和不育株的花药及雌蕊内游离肺氨酸和游离总氨基酸的含量进行了分析。结果表明:(1)在小孢子母细胞减数分裂期,不同育性花药之间游离脯氨酸的含量无明显差异,且含量较低。(2)在小孢子单核初期,可育花药内游离脯氨酸的含量显著高于不育花药,是不育花药的7倍,比减数分裂期增加20倍,高达其干重的1.65％,占其游离总氨基酸的50％。(3)在雌蕊中,游离脯氨酸的含量远远低于花药,不同育性植株之间差异不很明显。(4)关于游离总氨基酸的含量,在花药中减数分裂期,不同育性植株之间无明显差异;在小孢子单核初期,可育株高于不育株。在雌蕊中,相应于小孢子单核初期时,可育株稍高于不育株,受精后迅速趋于一致,但整个变化幅度不大。     

干旱响应转录因子DREB1A基因导入水稻光温敏核不育系的研究

以成熟胚诱导的愈伤组织作为农杆菌转化的受体材料,将诱导型启动子rd29A驱动的拟南芥DREB1A基因导入粳型光温敏核不育系水稻4008S,共获得67株再生苗.再生苗经0.75 mg/L除草剂草铵膦涂布筛选,有62株再生苗表现出对草铵膦抗性.PCR检测抗性苗中DREB1A基因,结果全为阳性.挑选部分进行Southem检测.结果表明目的基因已经整合到水稻基因组中.在干旱胁迫下,转基因水稻当代(T1代)植株的电导率显著低于非转基因对照植株(P＜0.05),脯氨酸含量显著高于对照植株(P＜0.05),证明DREBIA基因能提高水稻对干旱胁迫的耐受性.     

环己亚胺对盐诱导游离脯氨酸累积的影响

环己亚胺(CHX)单独作用会增加高梁苗中游离脯氨酸的含量,原因可能有:一是CHX抑制了根的正常吸收功能,导致植株失水,游离脯氨酸增加;二是CHX抑制了蛋白质合成,使总的游离氨基酸累积,从而也表现出游离脯氨酸含量的增加,后者可能更为主要。为此,用CHX研究与脯氨酸合成有关的基因活性化或表达时,一定要考虑CHX单独的作用。NaCl诱导的游离脯氨酸的累积可被CHX处理所抑制。在NaCl处理2～4h内加CHX后,抑制效果几乎可达到100％,以后随CHX处理的时间越长,其抑制作用越小。     

外源脱水应答转录因子DREB基因在转基因小麦中的诱导型表达与抗干旱生理效果研究

以冬小麦品种8901、5-98、99-92和104等品种的幼穗和幼胚为材料,用基因枪转化含逆境诱导转录因子DREB和bar基因的质粒pBAC128F（7024bp）。经筛选与植株再生,共获得70多个转基因小麦植株及其后代株系。转基因株系经PCR分析和RNA点杂交检测,结果表明外源转录因子DREB基因已稳定整合到转基因植株及其后代株系中,并且在部分后代株系中获得了表达。叶片脯氨酸含量测定表明,有16个转基因株系的脯氨酸含量与非转基因对照相比,增加相当显著,其中10个株系的脯氨酸含量在1100μg/g以上,比对照提高了2倍多。室内抗旱模拟实验表明,转基因株系停止浇水15d后,叶片仍然表现绿色,而对照叶片则失绿、枯干;复水10d后,转基因株系恢复活力,对照则死亡。研究表明,利用逆境诱导型启动子（rd29B）来增强外源DREB基因的表达,能显著改良小麦的抗旱性。     

旱后复水对东亚砂藓生理生化指标的影响

对经长期干旱的东亚砂藓（Racomitrium japonicum）材料按不同时间梯度复水处理,并测定游离脯氨酸含量、可溶性蛋白含量、超氧化物歧化酶（SOD）活性和过氧化物酶（POD）活性等4项生理指标。结果表明,经长期干旱的东亚砂藓4项生理指标在复水后2d内恢复到对照水平,而在复水过程中变化趋势有所不同：可溶性蛋白含量经长期干旱后在植物体内积累,SOD活性较高,在复水过程中与游离脯氨酸含量变化趋势一致,呈现升高后降低的波动状态恢复到对照水平;而游离脯氨酸含量和POD活性经长期干旱后和对照一致,在复水过程中POD活性迅速升高而后很快恢复到对照水平。这4种生理指标从一定程度上反应了耐旱东亚砂藓具有不同于其它植物的旱后复水的特殊生理机制。     

豇豆根瘤菌NGR234和紫云英根瘤菌109感染紫云英的比较研究

利用光学和电子显微镜对紫云英根瘤菌菌株109和广宿主的快生型根瘤菌菌株NGR234感染温带型豆科植物紫云英进行了研究,结果表明根瘤菌感染紫云英是通过在根毛中形成侵染线的途径。电子显微镜研究揭示了固氮根瘤中细胞内侵染线的存在。接种二天后,首先可观察到根毛的卷曲或分枝。接种四至五天后,在每株植物卷曲的根毛中可看到侵染线。接种八至十天后的植株出现肉眼可见的根瘤。菌株NGR234能够在紫云英上诱导根毛的卷曲,侵染线和根瘤的形成,但所形成的根瘤却未能固氮,根瘤中无明显的类菌体区,但有少数包有细菌的侵染线。NGR234抗抗菌素的衍生菌均未能使紫云英结瘤。将NGR234的共生质粒转移至三叶草、苜蓿、豌豆、快生型大豆根瘤菌和农杆菌,亦未能使这些细菌获得紫云英上结瘤的能力。     

Study on the conditions of Cell Transformation in Astragalus sinicus

The conditions of genetic transformation of cells in Astragalus sinicus were studied. The experimental results showed that Agrobacterium tumefaciens strain C58 (pKIW 105), when incubated in medium of low pH and low phosphate concentration in presence of acetosyringone could be induced and activated. When the activated bacteria were used to infect A. sinicus, the GUS gene transient expression in the hypocotyl protoplasts of A. sinicus was immediately and remarkably enhanced. This indicated that the vir gene of A. tumefaciens was activated under the above-mentioned incubation conditions which facilitated T-DNA transfer. In PEG-mediated DNA direct transfer, transient expression of GUS gene was promoted by higher pH and higher Ca2+ concentration of fusion medium. In the same experimental condition, expression of GUS gene under the control of MAS-CaMV 35S chimeric promoter was more effective than that under the control of CaMV 35S promoter, and intensity of GUS gene expression was positively correlated with the amount of foreign plasmid DNA in the range of 10--100 μg. Adventitious shoots were induced from cotyledon and hypocotyls explants treated with Agrobacterium turnefaciens strain PGV 2260 (pBI 121) and were subcultured on MS medium containing 50 mg/L kanamycin to select transformants, and then the transformed shoots were rooted. Stable expression of the foreign genes in the transformed plants was confirmed by assay of neomycin phosphotransferase Ⅱ (NPT Ⅱ ) and β-glucuronidase (GUS) activity.     

The common nodulation genes of Astragalus sinicus rhizobia are conserved despite chromosomal diversity

The nodulation genes of Mesorhizobium sp. (Astragalus sinicus) strain 7653R were cloned by functional complementation of Sinorhizobium meliloti nod mutants. The common nod genes, nodD, nodA, and nodBC, were identified by heterologous hybridization and sequence analysis. The nodA gene was found to be separated from nodBC by approximately 22 kb and was divergently transcribed. The 2. 0-kb nodDBC region was amplified by PCR from 24 rhizobial strains nodulating A. sinicus, which represented different chromosomal genotypes and geographic origins. No polymorphism was found in the size of PCR products, suggesting that the separation of nodA from nodBC is a common feature of A. sinicus rhizobia. Sequence analysis of the PCR-amplified nodA gene indicated that seven strains representing different 16S and 23S ribosomal DNA genotypes had identical nodA sequences. These data indicate that, whereas microsymbionts of A. sinicus exhibit chromosomal diversity, their nodulation genes are conserved, supporting the hypothesis of horizontal transfer of nod genes among diverse recipient bacteria.     

Cu2+污染土壤接种AM真菌对紫云英生长的影响

通过5个土壤Cu2 水平(0,20,50,100,150mgkg-1)的盆栽试验,研究了不同土壤Cu2 水平接种AM真菌对紫云英生长的影响。结果表明:(1)随着土壤Cu2 水平升高,紫云英生物量下降,与未接种相比,接种AM真菌明显提高了紫云英的生物量,接种G.intraradices对紫云英生物量的提高比接种G.mosseae更为明显,两者间呈显著性差异。(2)随着土壤Cu2 水平升高,紫云英根段浸染率下降,菌丝琥珀酸脱氢酶、碱性磷酸酶活性也下降。(3)在相同土壤Cu2 水平接种不同的AM真菌,紫云英根段浸染率有显著差异,接种G.intraradices的紫云英根段浸染率显著高于接种G.mosseae的处理,其菌丝琥珀酸脱氢酶活性及碱性磷酸酶活性也显著高于接种G.mosseae的处理。(4)接种G.intraradices能显著抑制Cu2 从紫云英地下部分向地上部分的运转,降低Cu2 的毒害,接种G.mosseae相对促进了Cu2 的运转。以上结果显示,Cu2 污染土壤中接种G.intraradices对紫云英生长具有促进作用。     

HAL1 mediate salt adaptation in Arabidopsis thaliana

INTRODUCTIONSalinity is a major environmental stress that isa substantial constraint to crop production both fordry land and irrigated agriculture. The detrimental impact of this stress is perpetuated and exacerbated by management practices used to facilitatehigh-output crop production. To overcome theselimitations and improve production efficiency in theface of a burgeoning world population, more salt tolerant crops must be developed. In contrast with traditional breeding, the direct ill…     

Expression of Potato Virus Y Coat Protein Gene in Transgenic Potato

Potato virus Y (PVY) N coat protein (CP) coding sequence was cloned into a plant expression vector pMON316 under the CaMV 35S promoter. Leaf discs of potato (Solanum tuberosum) were used to Agrobacterium-mediated gene transfer. A large number of regenerated putative transgenic plants were obtained based on kanamycin resistance. Using total DNA purified from transgenic plants as templates and two oligonucleotides synthesized from 5' and 3' of the PVY coat protein gene as primers, the authors carried out polymerase chain reaction (PCR) to check the presence of this gene and obtained a 0. 8 kb specific DNA fragment after 35 cycles of amplification. Southern blot indicated that the PCR product was indeed PVY CP gene which had been integrated into the potato genome. Enzyme-linked immunosorbent assay (ELISA) of our transgenic plants showed that CP gene was expressed in at least some transgenic potato plants.     

T-DNA-mediated transfer of Agrobacterium tumefaciens chromosomal DNA into plants

Besides the well-documented integration of DNA flanked by the transfer DNA borders, occasional insertion of fragments from the tumor-inducing plasmid into plant genomes has also been reported during Agrobacterium tumefaciens-mediated transformation. We demonstrate that large (up to approximately 18 kb) gene-bearing fragments of Agrobacterium chromosomal DNA (AchrDNA) can be integrated into Arabidopsis thaliana genomic DNA during transformation. One in every 250 transgenic plants may carry AchrDNA fragments. This has implications for horizontal gene transfer and indicates a need for greater scrutiny of transgenic plants for undesired bacterial DNA.     

Genetic improvement of heavy metal tolerance in plants by transfer of the yeast metallothionein gene (CUP1)

Cauliflower (Brassica oleracea var. botrytis) tolerates treatment with 25 µM CdCl2 for eight days, but is killed by that with a 50 µM concentration. However, even 15 µM CdCl2 is toxic in the presence of 1 mM L-buthionine sulfoximine (BSO), suggesting the presence of a Cd-inducible phytochelatin and its involvement in Cd-tolerance in cauliflower. To develop heavy metal-tolerant transgenic plants, we ligated the structural gene of yeast metallothionein gene (CUP1) downstream of CaMV35S promoter and introduced the fused gene into cauliflower. A Cd-tolerant transgenic cauliflower was selected, which grew well in the presence of 400 µM or less Cd, whereas the non-transformed cauliflower tolerated only up to 25 µM Cd. The transgenic cauliflower accumulated more Cd, especially in the upper leaves, than the non-transformed plant.In conclusion, by transfer of the yeast metallothionein gene into cauliflower increased Cd-tolerance and Cd-accumulating ability can be conferred to the plant.     

在杂交作物分子育种中利用普通核雄性不育的几个可能途径

由一对隐性基因控制的普通核雄性不育性遗传方式能够满足对植物最佳雄性不育系选育的要求,是水稻等作物杂种优势利用的极好遗传工具。如果能解决其不育系繁殖问题,将优于现有的其他杂种优势利用方式。克隆出普通核雄性不育性的可育基因,通过叶绿体转化,将核雄性不育性可育基因向普通核雄性不育株细胞质转移,创造普通核雄性不育株的保持系;通过种子成熟后表达的启动子;和以位点特异性重组技术为基础的基因开关以及化学诱导启动子的利用,都可能繁殖出100%不育株率的普通核雄性不育系,创造普通核雄性不育性利用的新途径,对植物杂种优势利用产业有十分重要的意义。