稻瘟菌无毒基因研究进展

稻瘟菌是引起水稻稻瘟病的病原物。水稻与稻瘟菌间存在广泛而特异的相互作用,是研究寄主与病原物互作的重要模式系统。本文对稻瘟菌与水稻互作最重要的激发子―无毒基因的研究现状进行了概括,讨论了无毒基因的定位、克隆方法以及已克隆无毒基因的功能及进化研究,同时对今后无毒基因研究的重要方向进行了探讨,为深入理解无毒基因的功能及与水稻可能的互作关系奠定了基础。     

稻瘟菌无毒基因研究进展

无毒基因编码的产物激发病原物与植物特异性相互作用。水稻与稻瘟菌之间的特异互作符合“基因对基因”关系。从研究稻瘟菌无毒基因的意义、已鉴定和克隆的稻瘟菌无毒基因、稻瘟菌无毒基因与其抗病基因的互作特点等几个方面,对稻瘟菌无毒基因研究进展作了简要评述 。     

稻瘟菌Magnaporthe oryzae P-ATPases基因家族分析

利用TCDB(Transporter Classification Database)网站数据库中的P-ATPases氨基酸序列对稻瘟菌全基因组表达序列(Coding Sequence,CDS)数据库进行搜索和分析,共发现23个P-ATPases基因,进化树分析表明这23个基因分属于4个家族和7个亚家族。构建了本地ESTs数据库,通过P-ATPases基因CDS序列与EST序列比对分析发现,在这些基因中有20个存在EST同源体,另外3个基因没有发现EST同源体,因此这20个基因是真实P-ATPases基因的可能性更高。运用MEME程序分析了这些P-ATPases蛋白结构域的基序,有6种基序在90%以上的基因氨基酸序列中出现,属保守基序。对这23个P-ATPases基因GC含量的分析表明,它们的平均GC含量在0.519-0.628之间,稍高于稻瘟菌整个基因组GC平均含量(0.516),同时这些基因内各区段GC含量变化不大,没有明显的梯度变化。本文结果为下一步深入研究稻瘟菌中P-ATPases基因家族的功能奠定了基础。     

稻瘟菌突变体T-DNA插入位点的精细定位和插入模式的研究

随机挑取已构建的37个稻瘟菌T-DNA突变株,利用TAIL-PCR技术扩增出T-DNA插入位点的侧翼序列,测序并进行比对分析。结果显示:成功获得扩增产物并测序的序列共有39条,T-DNA边界序列为稻瘟菌序列的有19条,其余20条为载体主干序列。在这有效扩增为稻瘟菌序列的19条中,有10条是T-DNA右侧翼序列与稻瘟菌序列,9条为左侧翼序列加稻瘟菌序列。分析T-DNA剪切位点,10条右侧翼序列中有9条的剪切位点相同,这与农杆菌介导T-DNA转化植物一样。而左边界的剪切位点就没有这种规律性。研究也精细确定了17个不同突变株的T-DNA插入位置,为后续的基因功能研究奠定基础。     

稻瘟菌MgORP1基因敲除突变株的构建及其表型分析

[目的]了解稻瘟病菌中氧固醇结合蛋白(oxysterol-binding proteins related proteins,缩写为ORPs)家族成员组成情况,构建MgORP1基因缺失突变株和互补株,对MgORP1基因功能进行初步研究.[方法]以ORPs家族的典型结构域"ORD"为靶标,对稻瘟病菌基因组数据库进行BlastP搜索.通过同源重组的策略,构建MgORP1基因缺失突变体,再通过重新导入该基因全长片段获得互补株.然后对野生型、突变体和互补株进行菌落、分生孢子和附着胞形态或形成情况、以及致病力进行比较分析.[结果]稻瘟病菌基因组中含有6个可能的ORPs族蛋白,其中MgORP1基因的破坏降低了稻瘟菌在完全培养基上的菌落生长速率和产孢量.但对菌丝、分生孢子和附着胞的形态,以及在水稻上的致病力没有明显影响.[结论]MgORP1基因可能与稻瘟病菌的菌落生长和产孢量相关.     

靛红衍生物的合成及其对稻瘟菌的生物活性

以靛红为原料合成了系列3-亚胺基/亚甲基-吲哚-2-酮化合物及其Mannich碱衍生物,研究了它们在抗稻瘟菌方面的活性,发现了这两种类型的若干化合物有较好的抑制稻瘟菌孢子萌发的活性,初步讨论了构效关系。认为1位的羟甲基和胺甲基、3位的亚甲基是药效团,芳基亚甲基苯环上对位取代基、羟基取代基和吸电子取代基不利于活性的提高,邻位的供电子取代基有利于活性的提高。     

稻瘟菌侵染诱导水稻凝集素基因的表达

利用mRNA差异显示技术(DDRT-PCR),从非亲和性稻瘟菌生理小种131侵染的水稻品种爱知旭(Oryza sati-va L. cv.Aichi-asahi)叶片中分离了8个诱导差异表达的cDNA片段.对这8个差示片段进行了回收、重扩增和克隆,以其中一个长度为321碱基并与甘露糖结合水稻凝集素和水稻盐诱导蛋白基因高度同源的差示片段为探针,筛选水稻非亲和性cDNA文库,获得12个阳性克隆.序列测定和数据库查询表明该基因的cDNA与水稻凝集素基因的cDNA及盐诱导蛋白基因的cDNA核苷酸同源性高达96%,推定的氨基酸序列与甘露糖结合水稻凝集素的氨基酸序列一致,与水稻盐诱导蛋白仅相差2个氨基酸.Southern杂交显示该基因在水稻基因组中有两个同源拷贝数,Northern杂交表明非亲和性稻瘟菌侵染可强烈诱导该基因表达.因此推测该基因参与了水稻对稻瘟菌侵染的防御反应.     

稻瘟菌侵染后水稻幼苗活性氧的产物与抗病性的关系

以对稻瘟菌ＺＢ１小种表现抗病（Ｈ８Ｒ）和感病反应（Ｈ８Ｓ）的两种水稻为材料接种稻瘟菌后,表现不亲和反应的水稻幼苗叶片中Ｏ＾－２产生速率提高,于２４ｈ和６０出现两个高峰;Ｈ２Ｏ２量在３ｈ和４８ｈ分别出现高峰;ＯＨ量在３６ｈ后略高于对照;过氧化物酶（ＰＯＤ）活性从６ｈ起显著升高。而在表现亲和反应的水稻中Ｏ２＾－、Ｈ２Ｏ２和．ＯＨ的产生及ＰＯＤ活性的增加均迟于现不亲和反应的,且强度也小。ＳＯＤ和过氧化氢     

水稻受稻瘟菌侵染后发病初期的细胞学反应

采用致病性不同的3个稻瘟菌株接种水稻IR64品种.结果显示在抗性反应中,病菌接种后水稻细胞中形成原生质颗粒,逐渐向病菌侵入部位聚集;原生质浓缩及沉积的形成、细胞坏死与病菌侵染菌丝的受抑制在时间和空间上是一致的.在中度抗性反应中,原生质颗粒化的时间延迟.在感病反应中,尚未观察到水稻细胞质浓缩现象.病菌侵染后寄主细胞在蓝光激发下的自发荧光表明,在寄主细胞中有多酚类物质的产生和积累.抗性反应中稻瘟菌接种后多酚类物质产生早,荧光范围大而强;中度抗性反应中,多酚类物质产生迟,荧光范围小而弱;而在感病反应中,难以观察到寄主细胞的自发荧光.胼胝质、磷脂酶Dγ(phospholipase Dγ,PLDγ)产生和积累的趋势与多酚类积累的情况大致是相似的.不同互作类型寄主细胞中多酚类物质、胼胝质和PLDγ产生和积累的差异表明,这些物质在水稻的抗病性中起了重要作用.     

稻瘟菌无毒基因的分子检测及其指纹类型分析

针对稻瘟菌中Avr-Pita与AvrPiz-t两个无毒基因,设计特异性引物,利用PCR方法对吉林省103株稻瘟菌菌株进行分子检测,并结合AVR-Pib、AVR-C039、PWL2和ACE1 4个无毒基因在其中85个菌株中的分布情况,绘制出基于这6个无毒基因的指纹类型.结果表明,Avr-Pita基因和AvrPiz-t基因在吉林省稻瘟菌中的分布频率分别为86.41%和62.14%;建立的指纹类型显示,85株稻瘟菌分布于9种类型中,其中类型1为主要类型,其分布频率为40.00%:根据30个已知生理小种的菌株在指纹类型中的分布情况,初步发现类型7与吉林省优势生理小种ZE1可能存在对应关系,并应用于稻瘟菌优势生理小种的特异性分子检测;其他指纹类型与中国生理小种并无明显对应关系.明确了无毒基因Avr-Pita与AvrPiz-t在吉林省稻瘟菌中的分布情况,构建了无毒基因的指纹类型,为水稻抗瘟育种和稻瘟菌优势小种的分子监测提供理论依据.     

Functional significance of conserved amino acid residues.

A systemic study of single amino acid substitutions in bacteriophage T4 lysozyme permitted a test of the concept that conserved amino acid residues are more functionally important than nonconserved residues. Substitutions of amino acid residues that are conserved among five bacteriophage-encoded lysozymes were found to lead more frequently to loss of function than substitutions of nonconserved residues. Of 163 residues tested, only 74 (45%) are sensitive to at least one substitution; however, all 14 residues that are fully conserved are sensitive to substitutions.     

Comparative proteomic analyses reveal that the regulators of G‐protein signaling proteins regulate amino acid metabolism of the rice blast fungus Magnaporthe oryzae

The rice blast fungus Magnaporthe oryzae encodes eight regulators of G‐protein (GTP‐binding protein) signaling (RGS) proteins MoRgs1–MoRgs8 that orchestrate the growth, asexual/sexual production, appressorium differentiation, and pathogenicity. To address the mechanisms by which MoRgs proteins function, we conducted a 2DE proteome study and identified 82 differentially expressed proteins by comparing five ?Morgs mutants with wild‐type Guy11 strain. We found that the abundances of eight amino acid (AA) biosynthesis or degradation associated proteins were markedly altered in five ?Morgs mutants, indicating one of the main collective roles for the MoRgs proteins is to influence AA metabolism. We showed that MoRgs proteins have distinct roles in AA metabolism and nutrient responses from growth assays. In addition, we characterized MoLys20 (Lys is lysine), a homocitrate synthase, whose abundance was significantly decreased in the ?Morgs mutants. The ?Molys20 mutant is auxotrophic for lys and exogenous lys could partially rescue its auxotrophic defects. Deletion of MoLYS20 resulted in defects in conidiation and infection, as well as pathogenicity on rice. Overall, our results indicate that one of the critical roles for MoRgs proteins is to regulate AA metabolism, and that MoLys20 may be directly or indirectly regulated by MoRgs and participated in lys biosynthesis, thereby affecting fungal development and pathogenicity.     

结合光谱法在DMIs类杀真菌剂筛选中的应用

为建立一种快捷和准确的方法用于新型杀真菌剂的筛选,以外源表达的稻瘟菌羊毛甾醇14α-去甲基化酶为靶酶,以市售烯唑醇、戊唑醇、三唑醇、三唑酮为DMIs类杀真菌剂代表,分析了靶酶活性、靶酶纯度和靶酶浓度对二者结合光谱的影响,并与生物测试结果比较分析其可靠性。结果表明靶酶的高活性、无其他P450干扰和合适的靶酶浓度是获得准确结合光谱的必要条件。烯唑醇、戊唑醇、三唑醇、三唑酮与靶酶结合常数(Kd)分别为0.143μmol/L、0.24μmol/L、0.257μmol/L、0.307μmol/L,该结果与其对稻瘟菌生长抑制能力(120h-EC50)显著相关,证明结合光谱法可作为一种简便可靠的DMIs类杀真菌剂筛选方法。     

结合光谱法在DMIs类杀真菌剂筛选中的应用

为建立一种快捷和准确的方法用于新型杀真菌剂的筛选,以外源表达的稻瘟菌羊毛甾醇14α-去甲基化酶为靶酶,以市售烯唑醇、戊唑醇、三唑醇、三唑酮为DMIs类杀真菌剂代表,分析了靶酶活性、靶酶纯度和靶酶浓度对二者结合光谱的影响,并与生物测试结果比较分析其可靠性。结果表明靶酶的高活性、无其他P450干扰和合适的靶酶浓度是获得准确结合光谱的必要条件。烯唑醇、戊唑醇、三唑醇、三唑酮与靶酶结合常数（K,/i>_d）分别为0.143μmol/L、0.24μmol/L、0.257μmol/L、0.307μmol/L,该结果与其对稻瘟菌生长抑制能力(120h-EC₅₀)显著相关,证明结合光谱法可作为一种简便可靠的DMIs类杀真菌剂筛选方法。     

A conserved acidic amino acid mediates the interaction between modulators and co-chaperones in enterobacteria

Hsp40-like co-chaperones are ubiquitous enzymes that stimulate the protein refolding activity of Hsp70 family chaperones. They are widespread in prokaryotic and eukaryotic systems. In bacteria, the best characterized co-chaperone is the Escherichia coli DnaJ protein. Many γ-proteobacteria encode a functional homologue of DnaJ, known as CbpA, which is expressed in response to starvation and environmental stress. The activity of CbpA is regulated by the “modulator” protein CbpM. Here, we have used a combination of genetics and biochemistry to identify the co-chaperone contact determinant of CbpM. We show that the nature of the interaction is conserved in enterobacteria.     

我国东北稻区稻瘟病的研究进展

东北水稻种植区是我国粳稻的主产区,长期以来稻瘟病是生产中危害最严重的病害之一。本研究就近30年来东北稻区稻瘟病菌优势种群和优势小种变迁,主栽品种抗性进行了综述,分析了已鉴定的稻瘟病抗性基因在东北稻区的利用价值,同时对该地区稻瘟病研究存在的问题与今后的研究方向进行了讨论,以期为水稻抗稻瘟病的育种提供参考。     

Interaction between rough phenotype and amino acid auxotrophy inSaccharomyces cerevisiae

InSaccharomyces cerevisiae a tryptophan requirement suppresses the rough colony phenotype that is produced by mutants at three separate loci. The suppression is strongly influenced by the genetic background and is excercised by both tested tryptophan loci. Very high concentrations of tryptophan in the growth medium relieve the suppression in some segregants. A similar suppression of the rough phenotype was observed in a mutant requiring lysine, while neither histidine nor adenine requirements were effective in that respect. A preliminary report of part of this paper was presented at the 3rd Internat. Symp. on Yeasts, Delft—The Hague, Netherlands, 1969.     

Inheritance of dsRNAs in the rice blast fungus, Magnaporthe grisea

The 1.6 and 1.8 kbp dsRNAs have been found in the rice blast fungus, Magnaporthe grisea strain MG01. These dsRNA molecules are located in cytoplasm of the fungal cells and maintained stably during vegetative growth. Three crosses between dsRNA free and dsRNA containing strains including a parental cross, sib-mating and back cross were made to follow the inheritance of dsRNAs during sexual reproduction. Approximately 10% of ascospore progenies (11 out of 105) contained dsRNAs from all three crosses. These data indicate that dsRNAs of M. grisea are inherited at a low frequency and not in a Mendelian fashion.     

Analysis of the Relationship between Blast Resistance Genes and Disease Resistance of Rice Germplasm via Functional Molecular Markers

Rice blast disease is one of the most devastating diseases of rice (Oryza sativa L.) caused by the fungus Magnaporthe oryzae (M. oryzae), and neck blast is the most destructive phase of this illness. The underlying molecular mechanisms of rice blast resistance are not well known. Thus, we collected 150 rice varieties from different ecotypes in China and assessed the rice blast resistances under the natural conditions that favoured disease development in Jining, Shandong Province, China in 2017. Results showed that 92 (61.3%) and 58 (38.7%) rice varieties were resistant and susceptible to M. oryzae, respectively. Among the 150 rice varieties screened for the presence of 13 major blast resistance (R) genes against M. oryzae by using functional markers, 147 contained one to eight R genes. The relationship between R genes and disease response was discussed by analysing the phenotype and genotype of functional markers. The results showed that the rice blast resistance gene Pita was significantly correlated with rice blast resistance. Our results provided a basis for the further understanding of the distribution of 13 major R genes of rice blast in the germplasm resources of the tested rice varieties, and were meaningful for rice disease resistance breeding.