过量表达辣椒CaNPR1提高烟草对青枯菌的抗性

对水稻和拟南芥等模式植物的研究表明,NPR1(nonexpressor of pathogenesis-related genes 1)是依赖于SA通路的防御反应调节基因,但在辣椒和烟草等茄科作物中该蛋白的功能还鲜有报道.研究从辣椒cDNA文库中分离获得一个NPR1的类似物全长cDNA(CaNPR1),并获得了其超表达的转基因烟草T1代株系.研究结果表明,这些株系与其野生型植株没有明显表型差异,但却表现出较野生型植株更高的抗青枯菌侵染活性.同时,研究还发现CaNPR1的超表达还显著提高了防御相关基因的表达,表明NPR1在不同植物间具有较强的功能保守性.     

拟南芥NPR1基因的克隆与表达载体的构建

NPR1基因为植物抗病基因表达和系统获得性抗性中的一个关键基因。该文以DNA PCR扩增的方法,从拟南芥基因组DNA中克隆出NPR1基因,通过序列分析,所克隆的 NPR1 基因与报道的基因序列完全一致。将其构建成植物表达载体,为今后植物抗病基因工程的开展奠定了基础。     

辣椒多聚半乳糖醛酸酶基因CaPG的克隆与序列分析

以耐贮辣椒品系P98为材料,采用RACE方法,首次获得辣椒果实多聚半乳糖醛酶(PG)基因的全长cDNA,命名为CaPG,登录号为FJ596175.序列分析结果表明,该基因cDNA长1 668 bp,5′非编码区为119 bp,3′非编码区为442 bp,CDS长1 107 bp,编码368个氨基酸.Blast比对发现,该基因核苷酸序列与已报道的番茄和番木瓜PG基因具有84%和85%的相似性.聚类分析表明,该基因与番茄和番木瓜的亲缘关系较近,与拟南芥PG基因的亲缘关系较远.     

病程相关基因非表达子1（NPR1）：植物抗病信号网络中的关键节点

最早从拟南芥（Arabidopsis thaliana）中克隆到的NPR1（nonexpressor of pathogenesis-related genes 1）基因是调控植物病害抗性的一个关键基因。它不仅对植物系统获得抗性（systemic acquired resistance,SAR）和诱导系统抗性（induced systemic resistance, ISR）起核心调控作用,而且是植物基础抗性（basic resistance）以及由抗病基因（resistance gene,R）决定的抗性的重要调控因子。氧化突发（oxidative burst）造成的强还原势导致NPR1蛋白还原成单体,以及NPR1单体在细胞核内的积累是诱导水杨酸（salicylic acid,SA）介导的PR（pathogenesis-related）基因表达和SAR产生的充分必要条件。NPR1通过与TGA转录因子的相互作用调控PR基因表达。NPR1作为多种信号途径的交叉点,与某些WRKY转录因子和NPR4一起,在调节和平衡SA和茉莉酸信号传导途径中起关键作用。NPR1的这种调控作用在细胞质内进行,通过遗传工程将其用于植物保护有很好的应用前景。     

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.     

病程相关基因启动子片段与GUS的融合基因在拟南芥中的表达

PR1是拟南芥 (Arabidopsis thaliana L.) 系统获得抗性的一个标志基因。利用PCR技术,从拟南芥中扩增并克隆了PR1基因的启动子片段。将该启动子片段与GUS报告基因拼接,构建成含有PR1-GUS融合基因的重组表达质粒。经根癌农杆菌介导转化,得到了转基因的拟南芥植株。用已知的系统获得抗性激活剂处理转基因植物,检测到GUS活性。因此,这一转基因体系可以作为一种简便、灵敏的实验体系以筛选激活植物系统获得抗性的化合物。     

香蕉NPR1基因家族的鉴定及在枯萎病菌胁迫下表达分析

以拟南芥NPR1基因家族成员蛋白序列为查询序列,在香蕉基因组数据库中鉴定香蕉NPR1基因家族成员,并对其进行生物信息学分析及在枯萎病菌侵染下的表达分析。共鉴定得到15个成员,将其命名为MaNPR1～MaNPR15。理化性质、保守功能结构域、重要的氨基酸残基及motif分析结果与其他物种所报道的有较高的一致度。香蕉NPR1基因家族成员种内进化树、基因结构及结构域的分类情况呈现出高度一致,表明了香蕉NPR1基因家族成员间有着明确的分工。种间进化树显示香蕉的NPR1基因分为3个分组,每个分组都含有拟南芥NPR1成员。主栽品种巴西蕉(Musa acuminata Colla. AAA group′Brazilian′)易感香蕉枯萎病,从巴西蕉CK及巴西蕉受枯萎病侵染2 d的根系转录组数据中综合表达量及表达趋势选定8个成员,并在巴西蕉与抗(耐)Foc TR4品种GCTCV-119中验证其表达模式。基因MaNPR4及MaNPR11在抗感品种中表现出明显的差异表达,在抗病品种GCTCV-119中随着Foc TR4侵染时间延长表达量不断增加,而在感病品种巴西蕉中表达量呈下降趋势。表明MaNPR4及MaNPR11参与香蕉抗枯萎病过程。本研究结果为进一步利用香蕉NPR1基因进行香蕉抗枯萎病遗传改良奠定基础。     

病程相关基因启动子片段与GUS的融合基因在拟南芥中的表达

PR1是拟南芥(Arabidopsisis thaliana L.)系统获得抗性的一个标志基因.利用PCR技术,从拟南芥中扩增并克隆了PR1基因的启动子片段.将该启动子片段与GUS报告基因拼接,构建成含有PR1-GUS融合基因的重组表达质粒.经根癌农杆菌介导转化,得到了转基因的拟南芥植株.用已知的系统获得抗性激活剂处理转基因植物,检测到GUS活性.因此,这一转基因体系可以作为一种简便、灵敏的实验体系以筛选激活植物系统获得抗性的化合物.     

对增强辣椒疫霉菌抗性的研究

病原物诱导型启动子能精确控制抗病基因在侵染位点的表达,是抗病基因工程的有效工具。prp1-1是来自马铃薯谷胱甘肽巯基转移酶基因启动子的一个273bp的片段,能够快速准确地启动被侵染位点抗病基因的表达;Rs-AFP2是具有对致病性丝状真菌的广谱抗性。该研究构建prp1-1调控Rs-AFP2基因表达的载体,经农杆菌介导转化法导入辣椒。逆转录PCR检测发现,转基因辣椒只在受到疫霉菌孢子侵染时,才由prp1-1启动Rs-AFP2基因的转录。用疫霉菌孢子灌根接种转基因辣椒T1代植株,35株T1代辣椒中有29株表现出明显的疫霉菌抗性。另将23株T1代辣椒种于人工气候箱,发现其形态和发育特征与相同条件下的非转基因植株无明显区别。研究表明,prp1-1调控Rs-AFP2的诱导表达达到了增强辣椒疫霉菌抗性的目的,而且避免了负面效应的发生。     

离体筛选抗枯萎病辣椒新种质

以2个辣椒(Capsicum annuum L.)自交系子叶诱导产生的愈伤组织为材料,辣椒枯萎菌粗毒素为选择剂,筛选抗枯萎病辣椒新种质.结果表明,枯萎菌粗毒素对辣椒子叶愈伤组织诱导、生长及不定芽分化具有明显的抑制作用,且随着粗毒素浓度的增加,抑制作用增强;在枯萎菌粗毒素质量浓度为0.60 g·L-1条件下,筛选、鉴定并获得了抗枯萎病辣椒体细胞变异无性系,且成功再生抗性植株.从而证明,离体筛选抗枯萎病辣椒新种质的方法是可行的.     

不同氮素水平辣椒幼苗对低温响应的差异

为研究低温对不同氮素水平辣椒幼苗生长的影响,在2228℃条件下分别用0.00g·L-1,2.00g·L-1和3.00g·L-13个浓度尿素水溶液培养的3个品种辣椒4叶1心期幼苗在人工气候箱内进行低温处理。结果显示:3个辣椒品种幼苗对相同低温的响应存在差异,其受低温危害由轻到重依次为中椒四号、市祥206和红龙。3个氮素水平下培养的3个品种辣椒幼苗进行连续3d11.0/5.0℃(Ⅲ)低温处理后,均危害严重,各项生理指标与对照差异显著,不能恢复正常生长,危害的程度因品种和氮素水平高低存在差异,氮素水平愈低受害愈重。连续3d15.0/9.0℃(Ⅰ)或13/7℃(Ⅱ)对辣椒幼苗处理后,受危害的程度仍因品种和氮素水平高低存在明显差异,但各项生理指标与对照差异显著减小,均能恢复生长,且氮素水平愈高,与对照的差异愈小。氮素水平影响辣椒幼苗对低温的响应,浓度较高时(3.00g·L-1)辣椒幼苗抵御低温的能力较强,较高的氮素水平虽能减轻低温对辣椒幼苗的影响程度,却不能完全抵消低温的危害。     

Evaluation of maize/pepper intercropping model in the management of pepper veinal mottle virus,genus Potyvirus,family Potyviridae on cultivated pepper (Capsicum annuum L.) in Nigeria

Three pepper cultivars obtained from National Horticultural Research Institute (NIHORT) Idi-Ishin, Ibadan were intercropped with maize for two planting seasons between March and September in each year. These pepper cultivars were NHV1-D96, and NHV1-E96 and NHV1-F96. A 90-day maturing maize variety (DMSR-1) was used as the intercropping companion plant. The pepper seedlings were raised in a greenhouse. A randomised complete block design was used for this experiment. Each variety was intercropped with maize and replicated three times including the sole plot. The results obtained for each year were not significantly different from each other. There was a significant difference in pepper veinal mottle virus (PVMV) disease incidence and severity at a probability of less than 5% in the treatment used. PVMV disease incidence and severity was relatively higher in the sole pepper crop compared with pepper intercropped with maize. In the three varieties of peppers intercropped with maize, less than 17% disease incidence and 15% disease severity were recorded in all the varieties with a minimum yield of 4 tons per hectare compared with the sole pepper cropping of the same variety that recorded as high as 75% disease incidence and 72% disease severity with a maximum yield of 3.3 tons per hectare. There was a significant negative correlation at probability less than 0.05 between disease incidence, severity and the fruit yield of pepper. Variety NHV1-F96 in the maize intercrop recorded the highest yield of 15.99 tons/ha with a land equivalent ratio of 2.4 tons/ha. The success of the PVMV disease management evaluated in this study was judged by the extent of reduction in number of diseased plants and by an increase in vigor of the cultivated pepper crop, with an increase in fruit yield and quality. This signifies that for devising effective viral disease management for any crop it is important that the vectors of the virus present in the particular area are exactly controlled from having contact with the target plant. The reduction of pest incidence with intercropping of non-host plants should be carefully considered.     

Qualitative and quantitative analysis of genetically modified pepper

For the development of qualitative and quantitative PCR methods of genetically modified (GM) pepper developed in Korea, a capsanthin-capsorubin synthase (CCS) gene was used as the endogenous reference gene. The primer pair ccs-F/R amplifying the pepper endogenous gene gave rise to an amplicon of 102 bp. No amplified product was observed when DNA samples from 16 different plants were used as templates. The construct-specific primer pairs amplifying the junction region of the bar gene and Ti7 introduced in GM pepper gave rise to an amplicon of 182 bp. Quantitative PCR assay was performed using a TaqMan probe and a standard plasmid as a reference molecule, which contained both an endogenous and event-specific sequence. For the validation of this method, the test samples containing 0.1, 1, 3, 5, and 10% GM pepper were quantified.     

辣椒疫霉菌侵染模型和侵染条件定量研究

在生长箱内控制条件下分析测定了土壤温度、水分含量对辣椒疫病死苗率的影响.结果表明:土壤温度和水分状况是决定辣椒疫病菌侵染的重要因子,病菌侵染的最适土壤温度为22 ℃～28 ℃,最适土壤含水量为40%,土壤过于干燥和过饱和都不利于病菌侵染发病;辣椒疫病死苗率与土壤温度、水分含量及其互作可用数学模式描述.田间调查发现,辣椒疫病田间流行趋势可用Gompertz模型描述,发病率与初始发病率、土壤温度、水分含量以及空气温度密切相关.建立了田间辣椒疫病发病率预测模型.     

己二酸二异丁酯对辣椒种子萌发及枯萎菌的化感效应

采用模拟的方式,利用生物测定和室内培养的方法,研究了不同浓度的己二酸二异丁酯对辣椒种子萌发、幼苗生长及辣椒枯萎菌的化感效应.结果表明:己二酸二异丁酯对辣椒种子萌发和幼苗生长具有低浓度促进、高浓度抑制的化感效应;己二酸二异丁酯对辣椒和茄子种子的化感效应存在较大差异,在低浓度时对辣椒种子萌发和幼苗生长的促进作用强于茄子种子,而高浓度时对辣椒种子萌发和幼苗生长的抑制强度弱于茄子种子;各浓度己二酸二异丁酯对辣椒枯萎菌菌丝生长有极显著的抑制作用,且作用强度随着浓度增加而增强,当浓度为1 mnol·L~(-1)时抑制作用最强,抑制率为10.75%;在田间抗病性调查期间内各浓度处理均提高了辣椒幼苗的抗病性,其中以1 mmol·L~(-1)处理抗病性最好,病情指数比对照降低了49.88%.

Abstract：

By the methods of laboratory incubation and bioassay, a simulation test was conducted to study the allelopathic effects of different concentration diisobutyl adipate on pepper seed germi-nation and its seedling growth and Fusarium oxysporum f. sp. vasinfectum. For the pepper seed germination and seedling growth, diisobutyl adipate exhibited allelopathic promotion at low con-centration, but allelopathic inhibition at high concentration. There existed greater differences in the allelopathic effects of diisobutyl adipate on the seed germination and seedling growth of pepper and eggplant. The promotion effects of low concentration diisobutyl adipate on pepper were stron-ger than those on eggplant, while the inhibition effects of high concentration diisobutyl adipate on pepper were weaker than those on eggplant. All test concentration diisobutyl adipate had signifi-cant inhibition effects on the mycelium growth of Fusarium oxysporum f. sp. vasinfectum, and the effects increased with increasing diisobutyl adipate concentration, being the strongest (an inhibi-tory rate of 10. 75%) at 1 mnol·L~(-1). Field text indicated that diisobutyl adipate at all test con-centrations enhanced the disease resistance of pepper seedlings. The best effect was observed at 1 mmol·L~(-1) of diisobutyl adipate, with the disease index decreased by 49.88%, compared to the control.     

甜椒育种材料N1345的疫病抗性遗传分析

阐明了以甜椒N1345为抗原的疫病抗性遗传机制,为甜辣椒抗疫病新品种选育提供依据。通过稳定高抗疫病甜椒育种材料N1345,与高感疫病辣椒材料N1308构建的P1、P2、F1、B1、B2、F2六个联合世代,应用植物数量性状主基因+多基因联合分离分析方法,进行了疫病抗性遗传分析。结果显示,以甜椒N1345为抗原的疫病抗性由2对加性-显性-上位性主基因控制（B-1-1）,两主基因加性效应、显性效应均相等,主基因遗传率在B1、B2和F2世代分别为63.43%、82.32%和83.46%。     

拮抗辣椒疫霉菌海洋细菌菌株SH-27的筛选鉴定及其防病促生作用

【背景】由辣椒疫霉引起的辣椒疫病是全球辣椒生产中一种毁灭性的病害。近年来生物防治因其具有对环境友好、对人畜安全的特性而倍受关注。【目的】筛选对辣椒具有防病促生作用的海洋细菌菌株SH-27并鉴定其分类地位。【方法】采用稀释分离法和平板对峙法筛选拮抗辣椒疫霉菌的海洋细菌菌株,以发酵液灌根法测定海洋细菌SH-27菌株对辣椒盆栽的防病促生作用;通过形态特征、生理生化测试及多基因序列分析对海洋细菌SH-27菌株进行鉴定。【结果】从分离的142株海洋细菌中筛选获得11株对辣椒疫霉菌具有较强抑制作用的细菌菌株,其中以来自珊瑚的SH-27菌株的抑菌作用最强、抑菌谱广;室内盆栽试验结果表明,SH-27菌株发酵液处理后的辣椒植株根长、株高、茎粗、鲜重、干重均显著高于对照处理。SH-27菌株发酵液灌根处理后,对辣椒疫病4、6和9 d的防效分别为70.81%、66.55%和48.20%。经形态特征、生理生化测试及16S rRNA、gyrA基因序列分析,鉴定SH-27菌株为解淀粉芽孢杆菌(Bacillus amyloliquefaciens)。【结论】海洋细菌SH-27菌株对辣椒具有较好的防病促生效果,具有开发为微生物农药及菌肥的潜力。     

Construction and characterization of a bacterial artificial chromosome library from chili pepper

A library of the bacterial artificial chromosome (BAC) that consisted of a total of 78,336 clones with an average insert size of 80 kb was constructed from Capsicum annuum, 'CM334', which is resistant to Phytophthora capsici and PVY. Based on a haploid genome size of pepper of 2,702 Mbp/C, the BAC library was estimated to contain approximately three genome equivalents and represented at least 90% of the pepper genome. In order to determine the percentage of BAC clones that contained mitochondrial DNAs, the entire library was screened with probes of chili pepper mitochondrial DNAs. The result showed that only twenty-five clones, which is 0.03% of the total BAC clones, were hybridized to mitochondrial gene probes. This indicates that the library is comprised predominantly of the nuclear sequences. The library was also tested for isolating specific clones by screening with a few known genes from the chili pepper, phytoene synthase gene, and two MADS genes--HpMADS1 and HpMADS3. The result showed that the three clones for phytoene synthase and the two clones for each MADS gene were positively hybridized to the specific probes. This indicates that the library is highly reliable and represents a resource for initiating map-based cloning and contig mapping in chili pepper.