抗大豆疫霉根腐病野生大豆资源的初步筛选

由大豆疫霉菌引起的大豆疫霉根腐病是严重影响大豆生产的毁灭性病害之一.防治该病唯一经济、有效和环境安全的方法是利用抗病品种.本研究对野生大豆资源进行抗大豆疫霉根腐病初步筛选,以期探讨野生大豆的抗性水平、分布和获得抗性野生大豆资源.通过苗期接种大豆疫霉菌对412份野生大豆资源进行抗病性鉴定,有13.4%的资源抗大豆疫霉根腐病,15.3%的资源表现为中间反应类型.对野生大豆资源的来源分析表明,抗大豆疫霉根腐病野生大豆资源在我国分布广泛,其中安徽省野生大豆资源抗性最丰富.     

黑龙江省主要栽培大豆品种(系)对大豆疫霉根腐病的多抗性评价

用下胚轴伤口接种方法接种鉴定黑龙江省60个栽培大豆品种和育成品系对5个具有不同毒力大豆疫霉菌菌株41-4、PMCl、USAR4、PSZJ6和USAR17的抗性.有50个品种(系)抗1个或1个以上茵株或表现中间类型,其中有5个、8个、16个和21个品种(系)分别对4个、3个、2个和1个菌株表现抗性或中间类型.60个品种(系)对5个菌株共产生12种反应模式,其中呈RRSSR反应类型的品种(系)可能含有Rpslα或Rpslc基因,品系农大3861可能含有Rps3c基因,呈SSSSS反应模式的品种(系)可能含有Rps7基因,或不含抗病基因;其它9种反应模式与含有已知单基因品种或单基因组合的反应模式不同,可能具有未知抗病基因.该研究结果表明,黑龙江省具有较丰富的抗大豆疫霉根腐病大豆品种(系),大部分品种(系)的抗性是有效的,可合理地用于大豆生产和抗疫霉根腐病育种.     

大豆品种早熟18抗疫霉根腐病基因的SSR分子标记

大豆品种早熟18是抗疫霉根腐病的有效抗源。本研究鉴定和分子标记早熟18的抗疫霉根腐病基因,以期为该品种的有效利用及分子辅助育种奠定基础。以感病大豆品种Williams与早熟18杂交建立分离群体。抗性遗传分析表明,早熟18对大豆疫霉菌抗性由1个显性单基因控制,该基因被定名为RpsZS18。SSR标记连锁分析表明,RpsZS18位于大豆分子遗传连锁群D1b上的SSR标记Sat_069和Sat_183之间,与这两个标记的遗传距离分别为10．0cM和8．3cM。RpsZS18是D1b连锁群上鉴定的第一个抗疫霉根腐病基因。     

一种土壤中大豆疫霉菌分离新方法

由于腐霉菌的干扰,土壤中大豆疫霉菌的分离十分困难。利用大豆疫霉菌的致病性和大豆对病原菌的选择作用排除腐霉菌,我们建立了一种简单、有效的土壤中大豆疫霉菌的分离方法。该方法用不含抗大豆疫霉根腐病基因的大豆叶碟诱钓大豆疫霉菌的游动孢子,将诱钓叶碟直接接种不含抗大豆疫霉菌基因的大豆植株,再对病株进行选择性或非选择性分离获得大豆疫霉菌。此方法能十分有效地排除腐霉菌干扰和细菌的污染,直接获得纯化菌株。应用该方法我们在以前未报道有大豆疫霉根腐病发生的山东、河南、安徽、江苏和浙江分离到大豆疫霉菌。     

用SSR标记分析抗疫霉根腐病大豆品种(系)的遗传多样性

利用50对SSR引物对抗疫霉根腐病大豆品种(系)进行遗传多样性分析。在166份品种(系)中,50个SSR座位共产生265个等位变异,平均每个座位5.3个。采用NTSYS-pc2.10计算品种(系)间遗传相似系数,平均相似系数为0.3124,表明抗疫霉根腐病大豆品种(系)间的遗传差异较大。用UPMGA进行聚类分析,166个品种(系)在相似系数为0.33时被聚为6类,地理来源相同的品种(系)大多聚类在一起。一些具有相同或相近抗病反应型的品种(系)被聚类在同一个类群中,表明这些抗病品种(系)的遗传关系较近,应有选择地利用。W illiam s和C lark抗疫霉根腐病近等基因系构成明显不同于中国大豆的基因源,可以用于拓宽我国大豆品种的遗传基础。     

一种土壤中大豆疫霉菌分离新方法*

由于腐霉菌的干扰,土壤中大豆疫霉菌的分离十分困难。利用大豆疫霉菌的致病性和大豆对病原菌的选择作用排除腐霉菌,我们建立了一种简单、有效的土壤中大豆疫霉菌的分离方法。该方法用不含抗大豆疫霉根腐病基因的大豆叶碟诱钓大豆疫霉菌的游动孢子,将诱钓叶碟直接接种不含抗大豆疫霉菌基因的大豆植株,再对病株进行选择性或非选择性分离获得大豆疫霉菌。此方法能十分有效地排除腐霉菌干扰和细菌的污染,直接获得纯化菌株。应用该方法我们在以前未报道有大豆疫霉根腐病发生的山东、河南、安徽、江苏和浙江分离到大豆疫霉菌。     

大豆疫霉菌无毒基因的快速检测

大豆疫霉菌Phytophthora sojae可引起大豆疫霉根腐病,是影响大豆生产的毁灭性病害。全球每年由于大豆疫霉根腐病导致的直接经济损失高达十几亿美元,该菌流行于我国东北大豆产区和福建等地并引起严重病害[1]。     

大豆疫霉菌的血清学研究

利用大豆疫霉菌（Phytophthoramegaspermaf.sp.glycinea）的菌丝可溶性蛋白,游动孢子悬浮液和培养液的浓缩物质作免疫原,获得三种抗血清。免疫双扩散测效价表明以菌丝可溶性蛋白作免疫原获得的抗血清效价最高,利用这种抗血清能够检测到4．4ng／ml的菌丝可溶性蛋白抗原,特异性试验表明大豆疫霉菌的抗血清与其它属真菌无交叉反应,但与测试的疫霉属真菌具有不同程度的交叉反应,由于疫霉属真菌只有大雄疫霉大豆专化型侵染大豆,故可用于对大豆疫霉菌的检测、诊断。     

大豆疫霉菌的分离与鉴定

采用叶碟诱捕法从2007年进口的美国大豆携带的土壤和2006年从黑龙江感病大豆田采集的土壤中分离出2株疫霉菌菌株,并对病原菌进行了形态特征、致病性、分子检测。结果表明:形态观察为疫霉属真菌;接种大豆后出现典型的大豆疫病症状;采用大豆疫霉的特异性引物PCR检测,2个菌株均能扩增出分子量为330 bp的特异性条带。结合形态、致病性测定和分子检测,2株病菌鉴定为大豆疫霉菌(Phytophthora sojaeKauf-mann et Gerdemann)。     

基于SSR标记分析大豆疫霉根腐病抗源的遗传多样性

丰富的遗传多样性可为大豆育种提供宽阔的遗传基础,本研究基于35对SSR标记,对60份东北地区大豆疫霉根腐病抗性品种进行了遗传多样性分析,共检测到189个等位基因,平均每个位点等位变异数5.4个,多态性信息含量指数(PIC)为0.1550~0.8195,平均为0.6636;遗传相似系数的变异范围为0.31~0.74。利用5对高多态性SSR引物构建了60份抗性材料的指纹图谱,这5对SSR引物构建的指纹图谱可以将60份疫霉根腐病抗性材料逐一区分开。采用NTSYS2.10基于遗传距离的聚类分析,将60份抗性材料分为7个类群,其中78.33%的抗性品种(系)的遗传相似系数在0.45~0.74间,表明遗传差异相对较窄,品种间遗传多样性水平较低。聚类分析与群体遗传结构分析结果有部分重合,均反映出不同地区的抗性材料间存在一定的渗透和交流。     

野生大豆资源对大豆疫病抗病性和耐病性鉴定

大豆疫病是大豆重要病害之一,在世界范围内导致严重经济损失。防治大豆疫病最有效方法是利用抗病或耐病品种。筛选抗性资源是发掘抗性基因和抗病育种的基础。本研究鉴定了野生大豆资源对大豆疫病的抗病性和耐病性,以期发掘优异抗源。苗期用子叶贴菌块方法鉴定104份野生大豆资源对两个不同毒力的大豆疫霉分离物PSJS2(毒力型:1a,1b,1c,1d,1k,2,3a,3b,3c,4,5,6,7,8)和PS41-1(毒力型:1a,1d,2,3b,3c,4,5,6,7,8)抗性,结果表明33份资源抗PS41-1,35份资源抗PSJS2,其中18份抗两个分离物。在抗病性鉴定基础性上,用菌层接种方法对选择的82份资源进行耐病性鉴定,发现7份高耐病性资源。这些结果表明,野生大豆中可能含有新的大豆疫病抗病和(或)耐病资源,这些抗病或耐病资源可以用于未来大豆抗病育种,以丰富大豆对大豆疫病的抗性遗传基础。     

大豆种质对疫霉根腐病抗性特点研究

对1027份中国和国外引进的大豆种质进行了大豆疫霉(Phytophthora sojae)根腐病的抗病性鉴定评价.结果表明,中国大豆种质的抗病性高于国外引进种质;中国南方的大豆种质抗病性较北方种质强,长江流域大豆中抗病种质比率最高,其次为黄淮海流域种质,而东北地区抗病种质较少;不同省份大豆种质的总体抗病性差异明显;育成品系的抗性好于改良品种和农家种,但不同省份来源的农家种、品系和品种抗性存在差异,黑龙江材料抗病性最低,这也是该省大豆疫霉根腐病严重发生的重要原因之一;在大豆籽粒脐色为黄色和褐色的材料中,抗病种质较多.     

Diversity among Single Zoospore Isolates Derived from Single-zoosporangia of Phytophthora sojae Kauf. and Gerd

Phytophthora sojae Kauf. and Gerd, a host specific pathogen to soybean, causes pre and postemergence damping-off and root and stem rot on soybean. The pathogen evokes severe yield losses in most soybean growing areas worldwide. The objective of this study was to determine phenotypic and genotypic diversity among single zoospore isolates (SZIs) originating from two single zoosporangia (Ps411-1 and Ps411-2) derived from the same parental isolate of P . sojae Ps411. Results showed that colony morphology and growth rate of 32 SZIs derived from sporangium Ps411-1 and 35 SZIs released from sporangium Ps411-2 did not significantly differ from the parental isolate Ps411. Pathogenicity of the SZIs was tested on three resistant and three susceptible Chinese soybean cultivars. While the majority of SZIs derived from sporangium Ps411-1(59.4%) and sporangium Ps411-2(71.4%) retained the same virulence spectrum as the parental isolate, the other SZIs of both progenies demonstrated either a higher or a lower level of virulence compared to that of parental isolate. A low level genetic variability in the populations of both single zoospore progenies was also demonstrated using the sequence-related amplified polymorphism (SRAP) technique. Cluster analysis separated the SZIs from both zoosporangia, Ps411-1 and Ps411-2, into four and three SRAP groups, respectively. No close correlation among SRAP and virulence could be established among SZIs. The results of this study suggest that virulence variability may be regarded as part of the total genetic changes among the zoospore progenies derived from single-zoosporangia. The pathogenic variability during asexual reproduction may play a role in changing the virulence structure of P . sojae .     

Soybean phytophthora resistance gene Rps8 maps closely to the Rps3 region

Root and stem rot is one of the major diseases of soybean. It is caused by the oomycete pathogen Phytophthora sojae. A series of resistance genes (Rps) have been providing soybean with reasonable protection against this pathogen. Among these genes, Rps8, which confers resistance to most P. sojae isolates, recently has been mapped. However, the most closely linked molecular marker was mapped at about 10 cM from Rps8. In this investigation, we attempted to develop a high-density genetic map of the Rps8 region and identify closely linked SSR markers for marker-assisted selection of this invaluable gene. Bulk segregant analysis was conducted for the identification of SSR markers that are tightly linked to Rps8. Polymorphic SSR markers selected from the Rps8 region failed to show cosegregation with Phytophthora resistance. Subsequently, bulk segregant analysis of the whole soybean genome and mapping experiments revealed that the Rps8 gene maps closely to the disease resistance gene-rich Rps3 region.     

Growth in microgravity increases susceptibility of soybean to a fungal pathogen.

The influence of microgravity on the susceptibility of soybean roots to Phytophthora sojae was studied during the Space Shuttle Mission STS-87. Seedlings of soybean cultivar Williams 82 grown in spaceflight or at unit gravity were untreated or inoculated with the soybean root rot pathogen P. sojae. At 3, 6 and 7 d after launch while still in microgravity, seedlings were photographed and then fixed for subsequent microscopic analysis. Post-landing analysis of the seedlings revealed that at harvest day 7 the length of untreated roots did not differ between flight and ground samples. However, the flight-grown roots infected with P. sojae showed more disease symptoms (percentage of brown and macerated areas) and the root tissues were more extensively colonized relative to the ground controls exposed to the fungus. Ethylene levels were higher in spaceflight when compared to ground samples. These data suggest that soybean seedlings grown in microgravity are more susceptible to colonization by a fungal pathogen relative to ground controls.