棉花品系Y18在草甘膦胁迫下的epsps基因表达分析研究

5-烯醇丙酮酰-莽草酸-3-磷酸合成酶（5-enolpyruvyl-shikimate-3-phosphate synthase,EPSPS）是植物或微生物体内合成芳香族氨基酸所必需的一个关键酶,但其受广谱性除草剂草甘膦的强烈抑制。通过对草甘膦胁迫下的棉花品系Y18进行研究发现：棉花品系Y18具有两个不同的5-烯醇丙酮酰-莽草酸-3-磷酸合成酶基因epsps1和epsps2,并且两个基因的编码区与其他植物的epsps基因具有较高的同源性,在草甘膦胁迫作用下,棉花的epsps1基因中表达较为稳定,epsps2基因表达量却提高了1．85～2．3倍,初步认为epsps基因的表达量提高是生物在受到胁迫作用时的一种应激反应。     

耐草甘膦基因克隆和作物转化研究新进展

评述了耐草甘膦基因克隆和作物转化研究的新进展。生物耐草甘膦的机理主要在于1）过量表达EPSPS（磷酸烯醇式丙酮酰莽草酸合成酶）基因;2）EPSPS基因发生突变而对草甘膦的亲和力减弱。或3）解毒酶作用。现已从大肠杆菌、鼠伤寒沙门氏菌、矮牵牛、拟南芥、烟草、胡萝卜等中克隆了aroA等EPSPS基因并进行了分子生物学研究。作物转基因抗草甘膦育种主要通过三条途径;1）转入经过修饰的或突变的耐草甘膦EPSPS基因,2）转入过表达的EPSPS基因;3）导入草甘膦代谢酶基因。     

EPSP合酶的研究进展

5-烯醇式丙酮酰莽草酸-3-磷酸合酶(5-Enolpyruvylshikimate-3-phosphate synthase,EPSP合酶)是莽草酸途径中的第六位酶,参与合成芳香族氨基酸以及部分次生代谢的产物,同时EPSP合酶不仅是除草剂草甘膦、抗菌素、抗寄生虫药物的作用靶酶,而且也是促进生物体内莽草酸积累的重要调控位点。近年来,随着分子生物学技术的快速发展和对EPSP合酶的深入研究,EPSP合酶基因在耐草甘膦转基因作物、医药卫生等方面被广泛应用。对EPSP合酶的研究进展进行综述及展望。     

核盘菌5-烯醇丙酮酰莽草酸-3-磷酸合酶的酶学性质

核盘菌5-烯醇丙酮酰莽草酸-3-磷酸合酶（EPSP合酶）是AROM多功能酶的活性之一.该酶催化莽草酸磷酸（S3P）和磷酸烯醇式丙酮酸（PEP）产生5-烯醇丙酮酰莽草酸-3-磷酸和无机磷酸的可逆反应,受除草剂草甘膦（N-（膦羧甲基）甘氨酸）抑制.纯化了核盘菌AROM蛋白并对EPSP合酶进行了酶学特征研究.结果显示,该酶反应的最适pH值为7.2,最适温度为30℃.热失活反应活化能是69.62 kJ/mol.底物S3P和PEP浓度分别高于1 mmol/L和2 mmol/L时,对EPSP合酶反应产生抑制作用.用双底物反应恒态动力学Dalziel方程求得的Km(PEP)为140.98 μmol/L,K _m(S3P)为139.58 μmol/L.酶动力学模型遵循顺序反应机制.草甘膦是该酶反应底物PEP的竞争性抑制剂（Ki为0.32 μmol/L）和S3P的非竞争性抑制剂.正向反应受K⁺激活.当［K⁺］增加时,K _m(PEP)随之降低,Km(S3P)不规律变化,而K _i(PEP)随［K⁺］增加而提高.     

甘薯草甘膦抗性基因EPSPS克隆和序列分析

EPSPS基因编码5-烯醇式丙酮酰莽草酸-3-磷酸合成酶,该酶是芳香族氨基酸合成的关键酶,该基因在细菌、真菌、藻类和植物中被广泛克隆和研究。EPSPS酶是草甘膦除草剂的靶点酶,过量表达EPSPS基因可以提高作物的草甘膦抗性。该研究根据甘薯基因组数据库设计引物,以‘广薯87’为材料提取RNA,通过RT-PCR方法扩增甘薯IbEPSPS基因,测序后进行生物信息学分析和表达分析。结果表明:(1)成功克隆获得甘薯IbEPSPS基因,该基因全长CDS为1569 bp,编码522个氨基酸,其中在第98~113、173~183位氨基酸序列具有2个EPSPS的保守结构域。(2)系统进化树分析结果表明,甘薯IbEPSPS基因与三裂叶薯(Ipomoea triloba)、打碗花(Calystegia hederacea)、田旋花(Convolvulus arvensis)和牵牛(Ipomoea nil)聚在一类,其中与三裂叶薯的亲缘关系最近。(3)实时荧光定量PCR分析结果表明,甘薯IbEPSPS基因在茎、叶和茎尖表达量较高,同时受到草甘膦胁迫后IbEPSPS基因表达量提高。该研究结果为进一步探讨甘薯IbEPSPS基因的功能及甘薯对草甘膦的耐药性机制奠定了基础。     

油菜转抗草甘膦、抗虫基因获得双抗植株

以草甘膦为筛选剂,用农杆菌介导法将编码5-烯醇式丙酮酸莽草酸-3-磷酸合成酶（EPSPS）的aroA—M12基因和编码苏云金杆菌毒蛋白的Btslm基因导入到甘蓝型油菜优良品种湘油15号中。在用草甘膦对转化体进行筛选的基础上．对转基因再生植株进行了PCR检测、Southern blot和Western blot分析．结果证明外源基因确已导入到该油菜品种中,而且表达了相应的蛋白。对转基因植株进行抗草甘膦、抗虫性鉴定的结果表明．转基因植株具有抗草甘膦、抗虫的双重特性。研究结果还表明抗草甘膦的aroA—M12基因在植物基因转化中,既可以用作抗除草剂基因,又可以代替常用的抗生素标记,用作植物筛选标记基因。     

核盘菌arom基因的克隆及其在酿酒酵母中的表达

核盘菌(Sclerotinia sclerotiorum)arom基因已经被克隆、测序。该基因编码的AROM蛋白是芳香族氨基酸合成途径中催化第二步到第六步的五功能多肽。为了对扩增的核盘菌arom基因进行功能验证和探索大量获得AROM蛋白的成熟方法,克隆了arom基因的编码框序列,并将其与载体pYES2连接,构建了酵母表达载体pYES2-arom。用LiAc/SSDNA/PEG方法将该表达载体转入酿酒酵母H158(Saccharomyces cerevisiaeH158)中。酶活测定、RT-PCR和Northern杂交结果显示,核盘菌arom基因在酿酒酵母胞内获得了表达,转化子具有AROM蛋白结构域之一5-烯醇丙酮酰莽草酸-3-磷酸合酶的催化活性。不同培养时间取样样品的酶活检测结果表明,当转化子在30℃的条件下,在SC-U酵母尿嘧啶营养缺陷型选择培养基中以180r/min被振荡培养时,其外源AROM蛋白的5-烯醇丙酮酰莽草酸-3-磷酸合酶酶活在培养72h达到最高。     

核盘菌AROM蛋白的三级结构分析

核盘菌编码AROM蛋白的arom基因已经被克隆测序,本文根据该基因翻译的氨基酸序列用同源模建方法和从头模建方法分析了AROM蛋白各结构域的三级结构和功能位点,以及该蛋白二聚体可能的组装方式。结果表明,核盘菌AROM蛋白的脱氢奎尼酸合酶结构域进一步由N-端含有一个Rossmann折叠的α/β结构域和C-端的α螺旋结构域组成;5-烯醇丙酮酰莽草酸-3-磷酸合酶结构域则由两个相似结构域组成,每个结构域含有不同拷贝数的β折叠和α螺旋;莽草酸激酶结构域的N-端由三个β折叠组成;脱氢奎尼酸酶结构域为(α2β2)3多肽,在N-端有一对反平行的β链,在C-端有loop环;莽草酸脱氢酶结构域含有一个由α/β组成的催化结构域和一个含有Rossmann折叠的NADPH结合结构域。     

突变肠杆菌株NRS-1中5个草甘膦逆境应答基因的克隆与功能研究

【目的】微生物对草甘膦的抗性受复杂的遗传体系调控,涉及靶基因和大量相关调控基因。对肠杆菌属细菌NRS-1突变菌株在高浓度草甘膦逆境下的5个重要差异表达基因进行功能研究,以期深入了解非靶标基因在抗草甘膦微生物的作用特点,为发掘优异基因资源,服务抗草甘膦转基因生物育种提供参考。【方法】NRS-1的差异表达基因可能在蛋白质合成、代谢、细胞膜等水平发挥作用,保护细胞免受高浓度草甘膦逆境,因此分别选取易位酶延伸因子fus A、丁二酸脱氢酶sdh A、胸苷磷酸化酶deo A、鸟氨酸氨甲酰转移酶arg F、周质蛋白osm Y进行克隆,采用大肠杆菌原核表达、转化拟南芥实验研究其功能,并通过细菌双杂及KEGG pathway分析基因间互作特点。【结果】在明确5个基因结构特点基础上,通过大肠杆菌原核表达及转基因拟南芥鉴定,发现这5个基因及草甘膦的靶基因5-烯醇式丙酮莽草酸-3-磷酸合成酶基因aro A对提高2种生物的草甘膦耐性均有不同程度的作用,其中arg F、deo A的抗性较好,与aro A相当,表明在应对草甘膦逆境时,芳香族、含有胸腺嘧啶氨基酸及精氨酸的合成代谢通路可能起重要作用;利用基因互作与KEGG分析发现5个基因与靶基因aro A间形成复杂的调控网络,但无直接的蛋白互作。【结论】NRS-1的5个差异表达基因对草甘膦逆境具有抗性,arg F、deo A优于其他3个基因,其与靶基因aro A间表现复杂的基因互作关系。     

水稻EPSP合酶基因的克隆、结构分析和定位

5-烯醇丙酮莽草酸-3-磷酸(EPSP)合酶是芳香族氨基酸合成途径中的一个关键酶, 该基因在植物抗除草剂基因工程中具有重要的应用价值. 根据水稻EPSP合酶基因的EST序列设计探针, 在水稻TAC基因组文库中筛选到16个阳性克隆. 对阳性克隆E11进行亚克隆, 由此获得了由3661核苷酸组成的水稻EPSP合酶基因全序列. 序列分析和同源性比较揭示, 该基因由8个外显子和7个内含子组成. 以窄叶青8号/京系17组合构建的DH群体和分子图谱将水稻EPSP合酶基因定位于水稻第6条染色体的上端.     

Cloning of genomic DNA of rice 5-enolpyruvylshikimate 3-phosphate synthase gene and chromosomal localization of the gene

The shikimate pathway enzyme 5-enolpyruvylshikimate 3-phosphate synthase (EPSPs) is the target of nonselective herbicide glyphosate. A partial rice epsps cDNA was generated by RT-PCR with primers designed according to EST sequence in GenBank and used as probe for rice genomic library screening. In a screen of approximately 8.0×104 clones from the rice genomic library, sixteen positive clones were obtained, which strongly hybridized to the probe. One clone, E11, was selected for further analysis and the full-length 3661 bp rice epsps genomic sequence was obtained. Sequence analysis and homologous comparison revealed that epsps gene is composed of 8 exons and 7 introns. Analysis by restriction fragment length polymorphism with the probe of rice epsps cDNA fragment confirmed that rice epsps is located on chromosome 6 with an indica-japonica (ZYQ8-JX17) double-haploid (DH) population. This is the first report on the EPSP synthase from monocotyledons.     

The 5-enolpyruvylshikimate-3-phosphate synthase of glyphosate-tolerant soybean expressed in Escherichia coli shows no severe allergenicity

The recombinant gene was amplified from the chromosomal DNA of genetically-modified (GM) soybeans and identified as epsps encoding 5-enolpyruvylshikimate-3-phosphate synthase (EPSPS) which renders glyphosate resistance. The epsps structural gene was introduced in the pET28(a) plasmid for its expression in Escherichia coli BL21(DE3). It was confirmed that the maximal productivity of the EPSPS protein was achieved when cultivating the recombinant strain in a LB broth for 2 h after supplementing 1 mM isopropylbeta-D-thiogalactopyranoside (IPTG) in a 2 h-culture broth. Since the expressed EPSPS protein was found as an insoluble form in the inclusion body, it was extracted by 6 M urea after sonication, and then purified through immobilized nickel-affinity column chromatography to isolate EPSPS having a molecular mass of 57 kDa. When incubated in simulated gastric fluid containing pepsin at pH 1.5, the purified EPSPS protein was completely digested within 1 min. In addition, the passive cutaneous anaphylaxis reaction of the purified EPSPS protein was not observed in the Sprague Dawley rat system that was administered either orally or subcutaneously. Furthermore, treatment of the EPSPS protein to the culture of the sensitized peritoneal mast cells, or unsensitized but antisera-labeled mast cells, showed neither a remarkable change in the histamine release nor a cytokine production, including interleukin-4 (IL-4) and tumor necrosis factor-alpha (TNF-alpha). Thus, it can be concluded that the EPSPS protein in the GM soybean showed no significant allergenicity in the Sprague Dawley rats.     

Glyphosate effects on the gene expression of the apical bud in soybean (Glycine max)

Glyphosate is a broad spectrum, non-selective herbicide which has been widely used for weed control. Much work has focused on elucidating the high accumulation of glyphosate in shoot apical bud (shoot apex). However, to date little is known about the molecular mechanisms of the sensitivity of shoot apical bud to glyphosate. Global gene expression profiling of the soybean apical bud response to glyphosate treatment was performed in this study. The results revealed that the glyphosate inhibited tryptophan biosynthesis of the shikimic acid pathway in the soybean apical bud, which was the target site of glyphosate. Glyphosate inhibited the expression of most of the target herbicide site genes. The promoter sequence analysis of key target genes revealed that light responsive elements were important regulators in glyphosate induction. These results will facilitate further studies of cloning genes and molecular mechanisms of glyphosate on soybean shoot apical bud.     

水稻EPSP合酶cDNA克隆、序列分析及其拷贝数测定

根据本室分离的水稻EPSP合酶基因的基因组序列设计一对引物,利用RT-PCR方法首次从水稻(Oryza sativa L. subsp. indica)叶片的RNA中扩增获得了水稻编码EPSP合酶的全长为1 585 bp的cDNA片段,它含有一个完整的开放读码框,编码511个氨基酸,包括444个氨基酸组成的成熟肽序列以及N端的67个氨基酸组成的叶绿体转运肽序列.成熟肽氨基酸序列对比表明,除真菌来源的EPSP合酶变异较大外,其他来源的EPSP合酶同源性较高,均在51%以上.而叶绿体转运肽氨基酸序列同源性较低.Southern杂交表明水稻EPSP合酶基因在水稻基因组中以单拷贝形式存在.RT-PCR分析表明,水稻EPSP合酶基因在根、未成熟种子和叶片中均有转录表达,在叶片中表达量最高.     

水稻EPSP合酶cDNA克隆、序列分析及其拷贝数测定

根据本室分离的水稻EPSP合酶基因的基因组序列设计一对引物 ,利用RT_PCR方法首次从水稻 (Oryzasati vaL .subsp .indica)叶片的RNA中扩增获得了水稻编码EPSP合酶的全长为 15 85bp的cDNA片段 ,它含有一个完整的开放读码框 ,编码 5 11个氨基酸 ,包括 44 4个氨基酸组成的成熟肽序列以及N端的 6 7个氨基酸组成的叶绿体转运肽序列。成熟肽氨基酸序列对比表明 ,除真菌来源的EPSP合酶变异较大外 ,其他来源的EPSP合酶同源性较高 ,均在 5 1%以上。而叶绿体转运肽氨基酸序列同源性较低。Southern杂交表明水稻EPSP合酶基因在水稻基因组中以单拷贝形式存在。RT_PCR分析表明 ,水稻EPSP合酶基因在根、未成熟种子和叶片中均有转录表达 ,在叶片中表达量最高     

Acquiring transgenic tobacco plants with insect resistance and glyphosate tolerance by fusion gene transformation

The advantages of gene 'stacking' or 'pyramiding' are obvious in genetically modified (GM) crops, and several different multi-transgene-stacking methods are available. Using linker peptides for multiple gene transformation is considered to be a good method to meet a variety of needs. In our experiment, the Bt cry1Ah gene, which encodes the insect-resistance protein, and the mG ( 2 ) -epsps gene, which encodes the glyphosate-tolerance protein, were connected by a 2A or LP4/2A linker. Linker 2A is a peptide from the foot-and-mouth disease virus (FMDV) that has self-cleavage activity. LP4 is a peptide from Raphanus sativus seeds that has a recognition site and is cleaved by a protease. LP4/2A is a hybrid peptide that contains the first 9 amino acids of LP4 and 20 amino acids from 2A. We used the linker peptide to construct four coordinated expression vectors: pHAG, pHLAG, pGAH and pGLAH. Two single gene expression vectors, pSAh and pSmG(2), were used as controls. The six expression vectors and the pCAMBIA2301 vector were transferred into tobacco by Agrobacterium tumefaciens-mediated transformation, and 529 transformants were obtained. Molecular detection and bioassay detection data demonstrated that the transgenic tobaccos possessed good pest resistance and glyphosate tolerance. The two genes in the fusion vector were expressed simultaneously. The plants with the genes linked by the LP4/2A peptide showed better pest resistance and glyphosate tolerance than the plants with the genes linked by 2A. The expression level of the two genes linked by LP4/2A was not significantly different from the single gene vector. Key message The expression level of the two genes linked by LP4/2A was higher than those linked by 2A and was not significantly different from the single gene vector.     

Glyphosate selected amplification of the 5-enolpyruvylshikimate-3-phosphate synthase gene in cultured carrot cells

Summary CAR and C1, two carrot (Daucus carota L.) suspension cultures of different genotypes, were subjected to stepwise selection for tolerance to the herbicide glyphosate [(N-phosphonomethyl)glycine]. The specific activity of the target enzyme, 5-enolpyruvylshikimate-3-phosphate synthase (EPSPS), as well as the mRNA level and copy number of the structural gene increased with each glyphosate selection step. Therefore, the tolerance to glyphosate is due to stepwise amplification of the EPSPS genes. During the amplification process, DNA rearrangement did not occur within the EPSPS gene of the CAR cell line but did occur during the selection step from 28 to 35 mM glyphosate for the C1 cell line, as determined by Southern hybridization of selected cell DNA following EcoRI restriction endonuclease digestion. Two cell lines derived from a previously selected glyphosate-tolerant cell line (PR), which also had undergone EPSPS gene amplification but have been maintained in glyphosate-free medium for 2 and 5 years, have lost 36 and 100% of the increased EPSPS activity, respectively. Southern blot analysis of these lines confirms that the amplified DNA is relatively stable in the absence of selection. These studies demonstrate that stepwise selection for glyphosate resistance reproducibly produces stepwise amplification of the EPSPS genes. The relative stability of this amplification indicates that the amplified genes are not extrachromosomal.Abbreviations 2,4-D 2,4-dichlorophenoxyacetic acid - DTT dithiothreitol - EPSPS 5-enolpyruvylshikimate-3-phosphate synthase - I₅₀ 50% inhibitory concentration - Kb Kilobase (pairs) - PEP phosphoenolpyruvate - PMSF phenylmethylsulfonyl fluoride - PVPP polyvinylpolypyrrolidone - S-3-P shikimate-3-phosphate     

根癌农杆菌介导的转aroAM12基因棉花植株的草甘膦抗性

以中棉35无菌苗下胚轴为外植体,采用农杆菌介导法将含有通过基因优化技术获得的草甘膦抗性突变基因aroAM12导入棉花中.以aroAM12为选择标记,利用草甘膦直接筛选获得65棵再生植株.PCR和Southerablot分析表明,经过草甘膦筛选出的To代植株均整合有aroAM12基因.Western blot分析表明整合进的aroAM12基因得到了有效表达,且不同植株之间的表达不尽相同.大棚喷洒的实验结果表明To代转化植株具有很高的草甘膦抗性.对T1代棉花的草甘膦抗性遗传分析表明,aroAM12基因以孟德尔方式遗传.     

Gene flow from transgenic to nontransgenic soybean plants in the Cerrado region of Brazil

Evaluation of transgenic crops under field conditions is a fundamental step for the production of genetically engineered varieties. In order to determine if there is pollen dispersal from transgenic to nontransgenic soybean plants, a field release experiment was conducted in the Cerrado region of Brazil. Nontransgenic plants were cultivated in plots surrounding Roundup Ready transgenic plants carrying the cp4 epsps gene, which confers herbicide tolerance against glyphosate herbicide, and pollen dispersal was evaluated by checking for the dominant gene. The percentage of cross-pollination was calculated as a fraction of herbicide-tolerant and -nontolerant plants. The greatest amount of transgenic pollen dispersion was observed in the first row, located at one meter from the central (transgenic) plot, with a 0.52% average frequency. The frequency of pollen dispersion decreased to 0.12% in row 2, reaching 0% when the plants were up to 10 m distance from the central plot. Under these conditions pollen flow was higher for a short distance. This fact suggests that the management necessary to avoid cross-pollination from transgenic to nontransgenic plants in the seed production fields should be similar to the procedures currently utilized to produce commercial seeds.