基于模糊识别和刺探电位技术鉴定小麦种质资源抗蚜性

利用田间抗蚜性鉴定模糊识别技术,结合室内刺探电位(EPG)植物抗性鉴定技术,比较分析了不同遗传背景的小麦种质资源的抗蚜性,为筛选新型小麦抗蚜种质材料提供依据。2年田间抗蚜性鉴定结果表明: 小偃麦多表现为中抗或低抗,而小黑麦多为中感或低感。选取抗性性状稳定且抗性级别不同的小偃麦21(中抗)、小偃麦22(低抗)、小黑麦31(中感)和小黑麦32(低感)进行麦长管蚜取食行为分析。对非刺探波(Np)、刺探波(P)、电势落差(Pd)、水溶性唾液分泌波(E1)、韧皮部取食波(E2)、细胞机械阻碍波(F)和木质部取食波(G)等基本波形的分析显示,麦长管蚜在小偃麦上首次开始刺探的时间显著长于小黑麦,且在小偃麦上的E1波的持续时间显著大于小黑麦;麦长管蚜在小偃麦21上的F波和小偃麦22上Np波的持续时间最长,在小黑麦31上的P波和小黑麦32上的G波的持续时间最长。以E1、F和Np波的持续时间为指标,基于刺探电位的小麦种质资源抗性水平鉴定结果与田间鉴定结果基本一致。因此,使用EPG技术筛选抗蚜小麦材料时,建议采用E1、F和Np波作为评价小麦抗性水平的指标。小偃麦21、22对麦长管蚜的抗性水平较高,可作为小麦抗蚜育种的种质材料。     

不同小麦基因型对γ射线辐照敏感性的分子解析

本研究以63份小麦品种(系)的风干种子为材料,分别利用0 Gy、100 Gy、150 Gy和250 Gy剂量的60Coγ射线辐照,通过种子发芽试验和基因表达等方法,探讨不同小麦基因型间辐射敏感性差异及辐射敏感性相关基因的表达模式。结果表明:根据苗高损伤效应,将63份不同小麦基因型分为敏感型(核优1号、中优206和太原703等)、较敏感型(旱选10号、济麦20和中麦175等)、较钝感型(德抗961、豫麦68和淮麦20等)和钝感型(衡观136、邯6172和偃展4110等)4类。所选材料γ射线辐照后,敏感型基因型中Ta Ku70和Ta Ku80基因诱导表达明显,钝感型基因型中Ta Ku70和Ta Ku80基因诱导表达不明显。本研究表明不同小麦基因型间辐射敏感性差异明显且与Ta Ku70和Ta Ku80基因表达模式有关。     

抗白粉病小麦-中间偃麦草种质的选育和SSR鉴定

在从抗白粉痛小麦砷间偃麦草异附加系Ⅱ-1—1与含杀3C配子染色体的农林26杂交井自交的后代中,通过人工接种鉴定,选出4个抗白粉病种质03012、04060、04112、04146。细胞学鉴定表明,4个种质的染色体数目均为2n=42条。花粉母细胞减数分裂中期Ⅰ多形成二价体。03012／烟农15杂种F1花粉母细胞减数分裂中期Ⅰ细胞中平均形成2个单价体,可能为异代换系。04060／烟农15、04112／烟农15和04146／烟农15的F1中均出现一定数量的单价体和多价体,可能为易位系。利用SSR标记鉴定表明,引物WMC327是含中间偃麦草抗白粉病基因所在染色体的特异标记;03012可能是一个2D染色体的异代换系。     

小偃麦衍生品系CH7086抗白粉基因的遗传及SSR分析

CH7086是兼抗白粉病、条锈病的小麦新品系,衍牛于来自十倍体长穗偃麦草的八倍体小偃麦与普通小麦的杂种后代.温室接种鉴定结果显示,CH7086对白粉病菌系E09、E21、E26均表现为免疫,且其抗件来自长穗偃麦草.抗性遗传分析表明CH7086的白粉病抗性由1对显性基因控制,暂定名为MlCH86.应用分离群体分组法(BSA)对从CH5241×CH7086的F2中随机选取的95个单株进行微卫星标记检测,发现位于2BL、2DL上的SSR位点Xbarc159在双亲和抗、感池间有特异性,并与抗性基因MlCH86连锁,其遗传距离为10.8 cM.用中国春第2部分同源群的缺体-四体系和双端体系进行验证,进一步将MlCH86定位在2BL上.用白粉病菌系E21、E26接种鉴定表明,MlCH86的抗性反应明显不同于2BL上已命名的抗性基因Pm6、Pm33.根据抗性基因的来源、染色体位置及抗性反应,初步推断存在于CH7086的抗性基因来自长穗偃麦草,它不同于已有的抗白粉病基因,可能是一个新基因.     

小麦新种质N9659抗白粉病基因的遗传分析

抗性种质N9659含有野生二粒小麦(资源编号:AS846)的抗白粉病基因,并对陕西关中地区白粉病优势小种表现为高抗.为了研究其抗白粉病基因的遗传规律,用高感品种辉县红、阿勃、陕160和阿勃21个缺(单)体系分别与N9659进行杂交,F1和F2苗期接种关中地区白粉病流行小种.结果显示,组合辉县红×N9659、阿勃×N9659、陕160×N9659及阿勃21个缺(单)体系和N9659杂交组合的所有F1均表现为高抗白粉病,F2的白粉病抗感比例除组合阿勃5BM×N9659偏离3∶ 1外,其他组合均符合3∶ 1,表明N9659苗期白粉病抗性由1对位于染色体5B上的完全显性基因控制.     

3个烤烟品系对TMV抗性的遗传规律分析

为更好地利用抗TMV烤烟种质资源,提高烤烟抗TMV育种效率,对烤烟品系CV87、FC8、抗88的TMV抗性遗传规律及抗性来源进行了研究。利用抗病烤烟品系CV87、FC8、抗88分别与感病品种云烟87、中烟100配置杂交组合,构建F1、F2群体,并利用TMV-C菌株进行抗性鉴定;同时,设计N基因引物对参试烤烟品种（系）的基因组DNA进行PCR扩增。经抗性鉴定,CV87、FC8、抗88及F1群体对TMV免疫,云烟87、中烟100感TMV,卡方（χ2）检验证明F2群体抗感分离比为3:1,符合显性单基因遗传;PCR结果表明,抗病品系CV87、FC8、抗88基因组内存在N基因序列,感病品种云烟87、中烟100基因组内未发现。本研究表明,CV87、FC8、抗88烤烟品系的TMV抗性来源于N基因。     

以小麦叶片壶氧化物酶同工酶p16．1酶带为生化标记研究小麦在各生长期对白粉病的敏感性

小麦白粉病以其多发性、普通性成为世界各地小麦生产的主要病害之一。在研究抗病品种对白粉病菌侵染的抗病机理中,采用等电聚焦凝胶电泳技术对抗、感白粉病小麦品种的叶片过氧化物酶同工酶酶谱进行的比较发现：两者的p16．1酶带（位于等电聚焦凝胶电泳酶谱p16．1）从拔节期至田间发病期之间的表现水平有很大差别。可以将其视为区别抗、感白粉病品种的特征性酶带。实验采用功能叶片（Fig.1),对50个小麦品种品系、抗、感病品种间4个组合的正反交F1代、119株F2代、65株抗病品种／感病品种／／感病品种的回交一代（BC1）材料,在pH5－8范围内进行过氧化酶同工酶的等电聚焦凝胶电泳分离。胶片于联苯胺染色液中显色。抗病品种中,p16．1酶带在小麦全生育期均有较强的活性,染色后着色深,多属一级酶带;感病品种中,p16．1酶带在拔节之间变得模糊不清、甚至消失踪迹,多为三级、零级酶带;然而、感染白粉病之后酶活性重新表现,并再次回升为一、二级酶带（Tab.1)。此结果在五年年份中均能很好地重复（Tab.2)。抗、感病品种间正反交F1代的p16．1酶带均正常（Fig.2),证明：p16．1酶带的活性是核基因的表达行为。进而在拔节期至发病期,分析抗、感病品种的杂交F2代,p16.1处为一级酶带者与其它类型之间的比值为3：1;而在抗病品种／感病品种／／感病品种的回交一代中,两者比例为1：1。表明：p16.1酶带由一单基因编码。由此推断：感病品种的p16．1酶带在拔节期至发病期还受到一隐性调控基因的影响,造成酶活性降低或丧失。     

普通小麦与长穗偃麦草杂种及其衍生材料的细胞遗传学特性

对十倍体长穗偃麦草(Thinopyrum ponticum)与普通小麦杂交F1及其与普通小麦回交BC1F1的形态学和细胞学特性进行了分析。结果表明,长穗偃麦草与普通小麦‘兰考矮早八’衍生F1(‘兰考小偃麦’)的根尖细胞染色体数为56条;花粉母细胞减数分裂中期Ⅰ染色体构型平均值为19.81Ⅰ+15.78Ⅱ+0.75Ⅲ+0.59Ⅳ;基因组荧光原位杂交(GISH)显示,兰考小偃麦中含有35条完整的长穗偃麦草和21条小麦染色体。‘兰考小偃麦’/‘科育818’和‘兰考小偃麦’/‘Cp02-3-5-5’杂交F1的根尖细胞染色体数及其所遗传的长穗偃麦草染色体数分别为50~52和16~22条,且存在染色体易位;花粉母细胞减数分裂中期Ⅰ平均染色体构型为14.54Ⅰ+17.40Ⅱ+0.55Ⅲ+0.14Ⅳ,平均49.4%的细胞出现多价体(三价体或四价体)。这些材料为创造小麦-长穗偃麦草新种质奠定了基础。     

精细定位甜瓜白粉病抗性基因Pm-M

以抗白粉病甜瓜品种MR1与感白粉病新疆地方品种新密1号为亲本,构建BC1P2和F2群体,研究白粉病菌Px1B(P.xanthii race 1B)的抗性遗传规律.以BC1P2与F2群体为试验材料,利用BSA(Bulked segregation analysis)结合分子标记技术发掘多态性信息,并开发分子标记进行抗性基...     

基于归一化法的小麦干物质积累动态预测模型

为探讨基于归一化法的不同分蘖力小麦品种干物质积累动态预测模型和参数特征,实现不同小麦品种干物质积累的有效预测,以3个分蘖力不同的小麦品种(豫麦49-198、兰考矮早8和偃展4110)为材料,对3个密度(75、225和375万株/hm2)下的干物质积累动态进行了研究。结果表明,高成穗率小麦品种(豫麦49-198和偃展4110)的干物质重均以375万株/hm2密度最高,而分蘖力高成穗率低的小麦品种(兰考矮早8)以225万株/hm2最高。建立的基于相对干物质积累量和相对积温的干物质积累预测模型中最佳模型方程式为y=1.1435/(1+e0.2776-4.6558 x)1/0.1130,r=0.9927,可较好地对小麦干物质积累动态进行模拟。通过对小麦干物质积累模型的特征参数分析发现,干物质积累过程可划分为前、中和后期3个阶段,且干物质积累平均速率与最终干物质重呈极显著正相关,较高的干物质积累平均速率对小麦干物质重的稳定和提高都有十分重要的作用。     

Akt phosphorylates Connexin43 on Ser373, a "mode-1" binding site for 14-3-3

Connexin43 (Cx43) is a membrane-spanning protein that forms channels that bridge the gap between adjacent cells and this allows for the intercellular exchange of information. Cx43 is regulated by phosphorylation and by interacting proteins. “Mode-1” interaction with 14-3-3 requires phosphorylation of Ser373 on Cx43 (Park et al. 2006). Akt phosphorylates and targets a number of proteins to interactions with 14-3-3. Here we demonstrate that Akt phosphorylates Cx43 on Ser373 and Ser369; antibodies recognizing Akt-phosphorylated sites or phospho-Ser “mode-1” 14-3-3-binding sites recognize a protein from EGF-treated cells that migrates as Cx43, and GST-14-3-3 binds to Cx43 phosphorylated endogenously in EGF-treated cells. Confocal microscopy supports the co-localization of Cx43 with Akt and with 14-3-3 at the outer edges of gap junctional plaques. These data suggest that Akt could target Cx43 to an interaction with 14-3-3 that may play a role in the forward trafficking of Cx43 multimers and/or their incorporation into existing gap junctional plaques.     

洋葱"昌激99-3"的激光诱变选育

采用CO2和He-Ne两种激光的三种剂量,分别辐照两个洋葱品种的湿种子,从He-Ne和CO2激光辐照元谋洋葱变异后代中选育出高产、优质、多抗、适应性较强的红皮洋新品种“昌激99-3”,经专家组实地验收亩产达9186.7Kg,是红皮洋葱经专家正式验收的全国最高产量。     

红皮洋葱"昌激99-3"的激光诱变选育

采用两种激光的三种剂量,分别辐照两个红皮洋葱品种的种子,从He-Ne和c02激光辐照云南元谋本地洋葱的变异后代中选育出高产、优质、多抗、适应性较强的红皮洋葱新品种“昌激99．3”,经专家组实地验收667m^2产量达9186．7kg,属红皮洋葱经专家正式验收的全国最高产量。     

Deciphering the role of 14-3-3 proteins

14-3-3 Proteins are found to bind to a growing number of eukaryotic proteins and evidence is accumulating that 14-3-3 proteins serve as modulators of enzyme activity. Several 14-3-3 protein recognition motifs have been identified and an increasing number of target proteins have been found to contain more than one binding site for a 14-3-3 protein. It is thus possible that 14-3-3 dimers function as clamps that simultaneously bind to two motifs within a single binding partner. Phosphorylation of a number of binding motifs has been shown to increase the affinity for 14-3-3 proteins but other mechanisms also regulate the association. It has recently been demonstrated that fusicoccin induces a tight association between 14-3-3 proteins and the plant plasma membrane H⁺-ATPase. Phorbol esters and other hydrophobic molecules may have a similar effect on the association between 14-3-3 proteins and specific binding partners.     

Overexpression of the Arabidopsis 14-3-3 protein GF14 lambda in cotton leads to a "stay-green" phenotype and improves stress tolerance under moderate drought conditions

The Arabidopsis gene GF14 lambda that encodes a 14-3-3 protein was introduced into cotton plants to explore the physiological roles that GF14 lambda might play in plants. The expression level of GF14 lambda under the control of the cauliflower mosaic virus 35S promoter varied in transgenic cotton plants, and lines that expressed GF14 lambda demonstrated a "stay-green" phenotype and improved water-stress tolerance. These lines wilted less and maintained higher photosynthesis than segregated non-transgenic control plants under water-deficit conditions. Stomatal conductance appears to be the major factor for the observed higher photosynthetic rates under water-deficit conditions. The stomatal aperture of transgenic plants might be regulated by GF14 lambda through some transporters such as H(+)-ATPase whose activities are controlled by their interaction with 14-3-3 proteins. However, since 14-3-3 proteins interact with numerous proteins in plant cells, many metabolic processes could be affected by the GF14 lambda overexpression. Whatever the mechanisms, the traits observed in the GF14 lambda-expressing cotton plants are beneficial to crops under certain water-deficit conditions.     

Cloning of Schistosoma japonicum 14-3-3 epsilon (Sj14-3-3 epsilon), a new member of the 14-3-3 family of proteins from schistosomes

A new member of the 14-3-3 protein family from Schistosoma japonicum has been identified. Phylogenetic analysis showed that this member belongs to the epsilon subfamily of the 14-3-3 proteins, and it is therefore named Sj14-3-3 epsilon. Consistent with the findings for the previously reported S. japonicum 14-3-3 protein (Sj14-3-3), Southern analysis suggested the presence of more than one gene, and/or introns or allelic polymorphism in this epsilon isoform. By RT-PCR, Sj14-3-3 epsilon was shown to be stage-specifically transcribed, being abundant in adults, present in sporocysts but absent in cercariae. Furthermore, mRNA of the epsilon isoform seemed to be much less abundant in the sporocyst stage, compared with Sj14-3-3. This suggests varying requirements of the different 14-3-3 isoforms at different stages of the life cycle.