抗黄矮病小麦新品系的分子标记检测研究

本研究对以小麦-中间偃麦草异附加系L1和小麦-中间偃麦草部分双二倍体‘无芒中4’为抗源选育出的抗黄矮病小麦新品系进行分子检测和抗病性鉴定.通过应用RAPD、SSR、SCAR 3种分子标记OPF15、Xgwm37、SC-W37进行分子检测,并采用人工接种和大田自然感病的方式进行抗黄矮病鉴定,筛选到了‘93646’、‘2003-2’等高抗黄矮病的小麦新品系.分子检测抗黄矮病基因与田间抗病鉴定结果基本一致,应用的3种PCR标记都可以检测出抗病材料,但SCAR标记SC-W37特异性强、稳定性好,可在小麦抗黄矮病育种早代选择过程中发挥重要作用.     

马铃薯晚疫病菌抗甲霜灵的SCAR标记

建立马铃薯晚疫病菌抗甲霜灵SCAR(sequenced characterized amplified region,序列特征扩增区域)标记,以马铃薯晚疫病菌对甲霜灵高抗菌株HD01-3和对甲霜灵高感菌株DK98-1为亲本,通过无性单游动孢子分离和有性杂交获得菌株HD01-3无性后代群体、菌株DK98-1无性后代群体以及F1代分离群体,以此为试验材料,利用BSA法(bulked segregant analysis,分离群体分组分析法)构建抗感基因池对后代菌系的甲霜灵抗性进行RAPD(random amplified polymorphic DNA,随机扩增多态性DNA)分析。从178条RAPD随机引物中找到一条特异性引物S2054,其可以扩增出一个与晚疫病菌对甲霜灵抗性相关的遗传标记,将该特异条带回收、克隆、测序,发现此标记大小为457bp,根据测序结果设计特异PCR引物,用于扩增抗感基因池,成功地将特异RAPD标记转化为SCAR标记。初步建立了马铃薯晚疫病菌抗甲霜灵SCAR标记,辅助监测晚疫病菌对甲霜灵的抗性。     

小麦品种(系)抗白粉病基因推导及分子标记鉴定

利用基因推导法和分子标记对我国主要麦区的小麦品种(系)进行了抗白粉病基因的鉴定。结果表明,南30-10等15个品种(系)含有Pm8,新麦2号等9个品种(系)含有Pm4,中植4号等9个品种(系)含有Pm21,郑麦113含有Pm4b+5b,杨09-111和新紫1号含有Pm2+mld。研究发现,基因推导和分子标记相结合,可大大提高小麦品种(系)抗白粉病基因鉴定结果的准确性,鉴定结果可为抗病育种和品种布局及白粉病的防治提供依据。     

番茄突变体再生植株抗晚疫病田间鉴定及抗病遗传规律

以番茄栽培品种为基础,开展用细胞育种方法筛选抗晚疫病突变体及抗晚疫病性状遗传规律的研究是培育抗晚疫病番茄优良品种行之有效的方法。而所获得的突变体再生植株的田间抗病性及其遗传力又是获得抗病品种的关键。同时,番茄抗晚疫病突变体的选择过程又是开展抗病生理生化机制研究的基础,因此具有重要的理论和实际意义。     

番茄抗晚疫病基因Ph-3的分子标记开发及应用

正番茄晚疫病由卵菌疫霉属的致病疫霉菌(Phytophthora infestans)侵染引起。病菌对番茄致病性强,侵染寄主后通过气流散发孢子,多次重复侵染植株,引起晚疫病爆发,对番茄生产造成严重危害[1]。利用抗晚疫病资源,培育番茄抗病品种是降低晚疫病危害的有效途径。在野生番茄中发现     

番茄抗黄化曲叶病基因Ty-2的分子标记及种质资源初步鉴定

以抗番茄黄化曲叶病毒病材料‘CLN2498D’为父本,感病材料‘早粉2号’为母本,以其F2代为研究对象,采用AFLP及SSR两种标记方法,筛选与Ty-2基因连锁的标记。通过对256对AFLP引物及30对SSR引物的筛选,共获得5个AFLP标记和2个SSR标记与Ty-2基因连锁,其中标记E02M11距离目标基因5.8cM,另有3个标记距离均在10cM以内。将标记E02M11用于30份番茄材料的种质资源筛选,获得12个含有该标记的番茄材料,为番茄抗黄化曲叶病毒育种工作提供基础。     

西瓜抗小西葫芦黄花叶病毒基因的连锁分子标记研究

 小西葫芦黄花叶病毒中国株系(Zucchini yellow mosaic virus Chinese strain,ZYMV-CH)是危害我国西瓜的主要病毒。本实验以抗病毒病西瓜野生种质P.I.595203与感病的普通西瓜自交系98R为亲本,采用单粒传方式得到109个E代株系,分别对亲本、F₁及109个F₃代株系群体进行了苗期抗ZYMV-CH接种鉴定,通过F₃代群体的抗感分离情况,推测得到F₂代各单株的基因型,采用集团分离分析法(bulked segregant analysis,BSA)在F₂代建立抗感基因池,以亲本、F₁和抗感基因池为模板,对640条RAPD引物进行PCR扩增筛选,其中引物AK13在亲本、F₁和抗感基因池之间扩增出一条多态性片段(644bp),在F₂代群体上验证该多态性条带与ZYMV-CH的抗性基因呈现连锁关系,遗传连锁距离为8cM,定名为AK13_-644,该连锁标记在ZYMV-CH抗性转育后代自交系上得到了验证。最终将此RAPD标记成功转化成SCAR标记SCAK13_-644,该标记可以作为西瓜抗病毒病辅助选择的分子标记。     

番木瓜抗环斑病毒突变体抗性遗传及RAPD标记

 ⁶⁰Coγ-射线处理番木瓜种子,从诱变一代中筛选到1株耐环斑病毒(PRSV)的变异植株(M₁),其侧芽组培后代(VM₁)部分植株也表现出了耐病性,以VM₁为母本进行回交,人工接种病毒鉴定回交后代(BM₂)的抗病性,结果为:在出自部分回交果实的BM₂群体中,包含有对PRSV Ys和Vb株系具抗性的植株,抗感分离比为1:1,但未发现抗Sm株系的植株;BM₂抗病两性株自交或以其为母本进行回交,分别获得诱变第三代(M₃)及回交诱变第三代(BM₃),人工接种PRSVYs株系,结果表明,BM₃抗感分离比也为1:1,因而认为辐射处理突变产生了具PRSV株系专化性的显性抗病基因,命名为Rys;但M₃抗感分离比不符合显性单基因3:1理论值,认为是单倍体选择的结果。运用BSA法,在BM₂中寻找到一个与抗病性密切相关的RAPD标记,经在BM₂、M₃及BM₃抗感群体中检验,可作为抗病育种的辅助选择标记。Rys是番木瓜栽培种中发现的第一个抗PRSV基因。     

用无菌苗法鉴定油菜对菌核病的抗(耐)病性

快速、准确、有效的抗病性鉴定方法是抗病育种的基础和保障.目前,国内外鉴定油菜菌核病的抗(耐)病性的方法归纳起来主要有草酸鉴定法、人工气候室盆栽苗接种鉴定、大田成株期人工辅助接种鉴定和大田病圃或非病圃自然侵染鉴定法等.草酸鉴定法对鉴定材料的破坏性大,育种中应用仅供筛选抗草酸的单株或材料,且不能鉴定抗菌核病菌侵入的材料.人工气候室盆栽苗接种鉴定受空间或成本的限制,难以用于大量的筛选工作,大田成株期人工辅助接种鉴定和大田自然侵染鉴定既受季节的限制,也受环境因素的影响.因此,探寻更高效、准确的抗(耐)病性鉴定方法,仍是抗病育种的迫切需要.本文介绍了一种准确、快速、高效的鉴定新方法.     

大豆品种(系)抗疫霉根腐病基因的连锁SSR标记分析

 大豆疫霉根腐病是大豆破坏性病害之一。利用抗病品种是防治该病的唯一有效的方法。迄今,已经鉴定了15个抗大豆疫霉根腐病基因(Rps基因),而且大豆部分基因都获得了不同类型的分子标记。本研究根据以前抗病基因推导结果选择26个可能含有Rps1基因座位等位基因或(和)Rps4基因的大豆品种(系),利用分别与Rps1a和Rps4紧密连锁的SSR标记进行抗病基因的分子检测,通过比较含有已知抗病基因对照大豆品种(系)分子标记检测结果并综合以往基因推导结果推断检测品种(系)的Rps基因。在选择的26个品种(系)中,长农14号被证明含有Rps1a,周豆13和铁95068-5含有Rps1a与Rps4基因组合,品系50794、科8924-3和合豆1号含有Rps4;有11个品种(系)存在含有Rps1a的证据、品系50052被推断含有Rps1c与Rps3b基因组合,但不排除这些品种(系)在Rps1座位含有一个新等位基因的可能性。另外,有7个品种(系)的所含抗病基因不能确定,它们可能含有新的Rps基因。     

亚麻品系9801-1抗白粉病基因的RAPD标记

 F2 populations were obtained from the cross between 9801-1 and DIANE.Bulked segregate and RAPD analyses were employed to identify molecules linked to the resistance to powdery mildew.OPP02 amplified about 792 bp polymorphic band in all individuals from 9801-1 and resistant bulk,but absent in all individuals from DIANE and susceptible bulk.By further analysis in F2 segregating population,the polymorphic band was found to be cosegregated with the resistant gene possibly.The fragment was sequenced,     

不同猕猴桃品种RAPD分析及其与抗溃疡病的关系

对不同猕猴桃品种的分子生物学试验表明：猕猴桃的DNA浓度在920 μg/mL符合RAPD分析的要求。通过60个随机引物的PCR扩增,报道了6个不同品种和类型猕猴桃种质资源的RAPD多态性,计算了它们之间的遗传距离,构建了聚类图,并讨论了其亲缘关系。聚类分析图反映出来源于安徽省主要猕猴桃产区的6个样品可以分为3组,其中抗病与感病的相对较为集中,由此可推断出现这种聚类的原因可能是由于它们基因组中有相同的DNA片段。抗病品系都有一条1 458 bp DNA片段,而感病品系均没有该带。故该片段可能与猕猴桃植株抗溃疡病相关。RAPD多态性从分子水平上反映出了猕猴桃种质资源不同品种及不同类型间复杂的遗传背景,为抗病育种的亲本选配提供了依据,也为合成猕猴桃抗溃疡病探针并用于检测猕猴桃抗溃疡病种质和分子标记辅助育种奠定了基础。     

Identification of a maize kernel stress-related protein and its effect on aflatoxin accumulation

ABSTRACT Aflatoxins are carcinogens produced mainly by Aspergillus flavus during infection of susceptible crops such as maize. Through proteomic comparisons of maize kernel embryo proteins of resistant and susceptible genotypes, several protein spots previously were found to be unique or upregulated in resistant embryos. In the present study, one of these protein spots was sequenced and identified as glyoxalase I (GLX-I; EC 4.4.1.5). The full-length cDNA of the glyoxalase I gene (glx-I) was cloned. GLX-I constitutive activity was found to be significantly higher in the resistant maize lines compared with susceptible ones. After kernel infection by A. flavus, GLX-I activity remained lower in susceptible genotypes than in resistant genotypes. However, fungal infection significantly increased methylglyoxal (MG) levels in two of three susceptible genotypes. Further, MG was found to induce aflatoxin production in A. flavus culture at a concentration as low as 5.0 muM. The mode of action of MG may be to stimulate the expression of aflR, an aflatoxin biosynthesis regulatory gene, which was found to be significantly upregulated in the presence of 5 to 20 muM MG. These data suggest that GLX-I may play an important role in controlling MG levels inside kernels, thereby contributing to the lower levels of aflatoxins found in resistant maize genotypes.     

Structural changes of homogalacturonan,rhamnogalacturonan I and arabinogalactan protein in xylem cell walls of tomato genotypes in reaction to Ralstonia solanacearum

Healthy and Ralstonia solanacearum-inoculated tomato genotypes susceptible or resistant to bacterial wilt including recombinant inbred lines (RILs) deriving from a cross between the resistant genotype Hawaii7996 and the susceptible Wva700 were compared for symptom and bacterial population development, and for the composition and structure of pectic polysaccharides and arabinogalactan proteins (AGPs) of xylem cell walls by immunological staining of tissue prints. Constitutive differences were observed between resistant and susceptible RILs, with a higher degree of methyl-esterification of homogalacturonan (HG) detected by antibody JIM7 in the resistant plants. After inoculation, decreased methyl-esterification of HG indicated by stronger labeling with antibody JIM5 was observed in all susceptible genotypes and in five of eleven resistant genotypes, with a clear increase in the non-blockwise de-esterification pattern of HG (LM7) only in the susceptible lines, indicating the mode of action of the pectinmethylesterase of R. solanacearum. In the susceptible lines infection generally leads to increased branching of rhamnogalacturonan I indicated by the detection of arabinan (LM6) and galactan (LM5) side chains, and of arabinogalactan protein (LM2), while only few of the resistant genotypes reacted with changes in these epitopes. All the resistant, symptomless genotypes contained relatively high pathogen populations in stems. A clear relation between cell wall composition and degree of latent infection of resistant genotypes was not found.     

Molecular mapping of the crown rust resistance gene rpc1 in barley

ABSTRACT Crown rust of barley, caused by Puccinia coronata var. hordei, occurs sporadically and sometimes may cause yield and quality reductions in the Great Plains region of the United States and Canada. The incompletely dominant resistance allele Rpc1 confers resistance to P. coronata in barley. Two generations, F(2) and F(2:3), developed from a cross between the resistant line Hor2596 (CIho 1243) and the susceptible line Bowman (PI 483237), were used in this study. Bulked segregant analysis combined with random amplified polymorphic DNA (RAPD) primers were used to identify molecular markers linked to Rpc1. DNA genotypes produced by 500 RAPD primers, 200 microsatellites (SSRs), and 71 restriction fragment length polymorphism (RFLP) probes were applied to map Rpc1. Of these, 15 RAPD primers identified polymorphisms between resistant and susceptible bulks, and 62 SSR markers and 32 RFLP markers identified polymorphisms between the resistant and susceptible parents. The polymorphic markers were applied to 97 F(2) individuals and F(2:3) families. These markers identified 112 polymorphisms and were used for primary linkage mapping to Rpc1 using Map Manager QT. Two RFLP and five SSR markers spanning the centromere on chromosome 3H and one RAPD marker (OPO08-700) were linked with Rpc1 and, thus, used to construct a 30-centimorgan (cM) linkage map containing the Rpc1 locus. The genetic distance between Rpc1 and the closest marker, RAPD OPO08-700, was 2.5 cM. The linked markers will be useful for incorporating this crown rust resistance gene into barley breeding lines.     

Elucidating resistance in cotton genotypes to whitefly, <Emphasis Type="Italic">Bemisia tabaci,</Emphasis> by population buildup studies

Plant resistance has become an important component of integrated pest management (IPM) for management of whitefly, Bemisia tabaci (Gennadius) (Homoptera: Aleyrodidae), an important pest of cotton in India. The present studies were undertaken to standardize the plant stage and identify resistant cotton genotypes against whitefly. Nine plant stages of F846, a susceptible cotton genotype, were exposed to whitefly for 25 days under no-choice conditions. The population buildup (eggs, nymphs, pupae and adults) was recorded. The 12-, 14- and 16-leaf stages were suitable for plant resistance studies against whitefly, and the 14-leaf stage was taken for further studies. Ten cotton genotypes of Gossypium hirsutum and two of G. arboreum were covered with split cages in which five pairs of B. tabaci (F₁) were released. The population buildup was recorded to categorize genotypes as resistant, moderately resistant, moderately susceptible or susceptible. The experiment was repeated with F₂ and F₃ generation whiteflies. Based on overall average score of three experiments, LD694 was rated as resistant; LK861, Supriya, RS2013, CNH911 and PA183 as moderately resistant; IS-376/4/1/20/72, NHH44, TxMaroon2-78, Bt 6304 and RS2098 as moderately susceptible; and F846 as susceptible. LD694 was found to be resistant in three consecutive generations of whitefly.     

Pathogenic diversity within field populations of Orobanche cumana and different reactions on sunflower genotypes

Different races of the parasitic Orobanche cumana (sunflower broomrape) have been reported in Spain, race F being the most virulent. Full resistance in sunflower to races A–E is achieved with each of the single major genes Or₁ to Or₅ respectively. However, parasitised hybrids allegedly resistant to race F were observed in early 2002. The purpose of this study was to verify broomrape incidences (BI) on resistant sunflower genotypes, to assess the mixture of races within field populations and to test for partial resistance to race F in the sunflower hybrids showing a low degree of attack (DA) by the weed. Tests were conducted under field conditions in two locations of southern Spain. While no significant differences were found for yield and BI between locations, the DA on the cultivars depended on the location. With high infection levels and significantly lower yield in susceptible controls, marked differences in BI and DA were found within resistant cultivars, but all of them showed similar crop yield. When artificially inoculated with several populations of race F, line P96 and mainly line L86, were consistently slightly infected, suggesting they were inbred lines responsible for horizontal resistance in infested fields. L86 was extremely susceptible to race E populations, which is unusual as sunflower resistance to one race provided resistance to all the previously described races of O. cumana. No different virulences were detected within two groups of subpopulations (races E and F) inoculated onto resistant sunflower genotypes. However, race F subpopulations showed significant differences in aggressiveness, which seems to be related to horizontal (multigenic) resistance of the crop to the parasitic weed.     

Infection process of Phoma koolunga on stem and leaf tissue of resistant and susceptible field pea (Pisum sativum)

This study investigates the infection process of Phoma koolunga on field pea (Pisum sativum) stems and leaves using different susceptible and resistant pea genotypes for each tissue, viz. 05P778‐BSR‐701 (resistant) and 06P830‐(F5)‐BSR‐5 (susceptible) for stems and ATC 866 (resistant) and ATC 5347 (susceptible) for leaves. On both resistant and susceptible genotypes, light and scanning electron microscopy showed P. koolunga conidia infect stem and leaf tissues directly via appressoria or stomatal penetration, but with more infections involving formation of appressoria on stems than on leaves. On leaves of the resistant genotype, at 72 h post‐inoculation, P. koolunga penetrated more frequently via stomata (5.2 conidia per 36 893 μm²) than by formation of appressoria (1.8 conidia); yet no such difference was observed on stems of the resistant genotype. In contrast, at the same time point, the number of conidia infecting the susceptible genotype by formation of appressoria on either stems (135 conidia) or leaves (11.3 conidia) was significantly greater than via stomata (8 and 7.3 conidia, stems and leaves, respectively). Mean germ tube length of germinating P. koolunga conidia on both stems (29.8 μm) and leaves (32.9 μm) of the resistant genotype was less than on the susceptible genotype (40.5 and 63.7 μm, stem and leaves, respectively). In addition, there were differences in the number of germ tubes emerging from conidia on resistant and susceptible genotypes. These are the first insights into the nature of leaf and stem resistance mechanisms operating in field pea against P. koolunga.     

Development and Comparison of Symptom Indices for Quantifying Grapevine Resistance to Pierce's Disease

ABSTRACT Symptoms of Pierce's disease (PD) were assessed under greenhouse conditions on field-resistant and field-susceptible grapevines in order to characterize the PD resistance phenotype in the genus Vitis. A cane maturation index (CMI) was developed to quantify the green-islands symptom, which was measured at 12 weeks post-bacterial inoculation, along with leaf scorch and percentage of xylem vessels blocked by occlusions. Canes of resistant genotypes matured normally and had a significantly lower CMI score of 0.9 (on a 0-to-6 scale) compared with 5.1 for the susceptible genotypes. The CMI scoring method had a high correlation (R(2) = 0.91) with previously characterized field performance, whereas leaf scorch had only a moderate correlation (R(2) = 0.51) with field performance. Average scorched area on leaves of the susceptible and resistant genotypes was 80 and 48%, respectively, demonstrating that leaf scorch can be extensive in resistant genotypes under the presented screening conditions, and suggesting that systemic infection can occur in all evaluated genotypes. Occlusions within both stem and petiole vessels were composed principally of tyloses and were significantly higher in petioles than in stems of either resistant or susceptible backgrounds. Susceptible genotypes displayed a higher level of stem tylose occlusions relative to resistant genotypes, but correlation to field performance was low (R(2) = 0.13). Ease of use and high correlation to field performance makes CMI scoring a better choice for PD resistance evaluations relative to other phenotypic symptom assessments.