Molecular Identification of a New Member of the Clover Proliferation Phytoplasma Group (16SrVI) Associated with Centaurea Solstitialis Virescence in Italy

In the United States, yellow starthistle (Centaurea solstitialis) is an annual invasive weed with Mediterranean origins. Malformed plants displaying witches' broom, fasciations, abortion of buds and flower virescence symptoms were observed in central Italy. Attempts to transmit the causal agent from the natural yellow starthistle host to periwinkle by grafting, resulted in typical symptoms of a phytoplasma, i.e. yellowing and shortening of internodes. The detection of phytoplasmas was obtained from both symptomatic yellow starthistle and periwinkle by the specific amplification of their 16S-23S rRNA genes. PCR amplification of extracted DNA from symptomatic plant samples gave a product of expected size. Asymptomatic plants did not give positive results. An amplicon obtained by direct PCR with universal primers P1/P7 was cloned and sequenced. The homology search using CLUSTALW program showed more than 99% similarity with Illinois elm yellows (ILEY) phytoplasma from Illinois (United States) and 97% with Brinjal little leaf (BLL) phytoplasma from India. Digestion of the nested-PCR products with restriction enzymes led to restriction fragment length polymorphism patterns referable to those described for phytoplasmas belonging to the clover proliferation (16S-VI) group. Since this is a previously undescribed disease, the name Centaurea solstitialis virescence has been tentatively assigned to it. This is a new phytoplasma with closest relationships to ILEY and BLL, but distinguishable from them on the basis of 16S rDNA homology, the different associated plant hosts and their geographical origin.     

Sources of resistance to septoria tritici blotch and implications for wheat breeding

Twenty-four wheat cultivars and breeding lines were screened for isolate-specific resistance to septoria tritici blotch (STB) caused by 12 isolates of Mycosphaerella graminicola. New isolate-specific resistances that could be used in wheat breeding were identified. Major sources of resistance to STB used in world breeding programmes for decades, such as Kavkaz-K4500, Veranopolis, Catbird and TE9111, have several isolate-specific resistances. This suggests that 'pyramiding' several resistance genes in one cultivar may be an effective and durable strategy for breeding for resistance to STB in wheat. Several cultivars, including Arina, Milan and Senat, had high levels of partial resistance to most isolates tested as well as isolate-specific resistances. Resistance to isolate IPO323 was common, present in all but one of the major sources of resistance tested. This suggests that resistance to IPO323 may be an indicator of varietal resistance to STB in the field.     

透明颤菌血红蛋白基因(vgb)在大肠杆菌中的高效表达

利用PCR技术将透明颠菌血红蛋白基因（vgb）克隆到融合表达载体pET28a，在大肠杆菌BL21（DE3）表达。重组蛋白在30℃诱导获得可溶表达。利用Ni^2＋亲和层析对重组蛋白进行了纯化，得到重组的透明颠菌血红蛋白，蛋白呈红色。实验现象显示重组蛋白与血红索相结合。紫外光区和可见光区波长扫描分析显示：蛋白粗提物和纯化后的血红蛋白在230nm和413nm都有强吸收峰，初步表明，尽管重组蛋白比天然蛋白多36个氨基酸，重组蛋白仍然具有生理活性。诱导后4h和6h的培养液氨基乙酰丙酸含量分别达到17mg／L和21mg／L。说明重组蛋白的表达明显促进了体内heme合成途径。     

西安荷斯坦奶牛群5个基因座位遗传多态性的PCR-RFLP分析

应用PCR-RFLP方法对西安荷斯坦牛的κ-en、β-lg、β-lg5′侧翼区、CSN1S2、IGFBP-3共5个基因座位进行了多态性分析。结果表明，在西安荷斯坦牛群中，没有发现携带CSN1S2^P等位基因的个体，其多态信息含量为0。κ-en基因座位呈现低度多态(PIC=0．2366)，β-lg、β-lg5′侧翼区、IGFBP-3基因座位的多态信息含量分别为0．3168、0．3689、0．4439，均呈现中度多态。κ-en、β-lg、β-lg5′侧翼区、IGFBP-3、CSNIS2基因座位的杂合度和DNA多态度分别为0．2742、0．3947、0．4879、0．4891、0和0．0255、0．0116、0．0333、0．0112、0。而且，在西安荷斯坦牛群中，κ-en、β-lg、β-lg5′侧翼区、IGFBP-3共4个基因座位均处于Hardy-Weinberg平衡状态，CSN1S2基因座位处于纯合状态。     

以催乳素受体基因作为撒坝猪部分生产性能候选基因的研究

此文运用PCR-RFLP技术检测催乳素受体(PRLR)基因在撒坝猪群体中的多态性分布,并采用最小二乘分析模型初步统计分析基因多态性与部分生产性能的相关性。结果表明,PRLR基因等位基因B及其基因型BB在群体中占优势,频率分别为0.6594和0.4438;PRLR基因在群体中处于Hardy-Weinberg平衡状态;头胎繁殖性状有利等位基因B对生长性状无不利影响。     

西尼罗热病毒RT-PCR检测方法的建立

参考Genebank发表的西尼罗热病毒(West Nile virus，WNV)E糖蛋白基因序列，自行设计合成一对引物，对WNV进行RT—PCR扩增，产物经琼脂糖电泳分析，呈现一条约400bp的条带，将其克隆入pMD18-T—Vector载体中，并进行序列测定，与已发表的WNV基因比较发现，核苷酸的同源性为99．7％，证实为WNV的E基因，通过对样品多次检测，都能扩增出一条约400bp的条带，表明该方法比较稳定。     

我国部分地区猪繁殖与呼吸综合征病毒分离株ORF5基因的遗传变异分析

参考Genbank发表的猪繁殖与呼吸综合征病毒（PKRSV）ATCC VR-2332的ORF5基因序列，设计并合成了一对引物．对来自福建、浙江、山东等地的PRRSV分离毒株进行RT-PCR扩增．获得约748bp的DNA片断，将其分别克隆入pMD18-T载体中，并进行测序。应用DNAStar软件分析所测序列，并与ATCCVR-2332、CH-1a、MLV、Lv等毒株的ORF5序列进行比较，结果表明：SHDl与F114、MLV、ATCCVR-2332同源性高达98．5％，与CH-1a同源性为91．0％，与其它毒株同源性为86．6％~88．4％；F114与MLV、ATCCVR-2332同源性为99．3％～99．7％．其余分离毒株在遗传关系上和CH-1a又分为明显的两个群．显示近年来各地PRRSV分离毒株与cH-1a株的遗传差异越来越大。     

复方中草药"毒菌杀"对禽大肠杆菌及鸡白痢沙门氏菌的体外抑菌试验

观察了复方中草药“毒菌杀”的安全性及其对禽大肠杆菌及鸡白痢沙门氏菌的体外抑菌情况。结果发现“毒菌杀”安全性高，组成“毒菌杀”的各单味中药及其合剂对大肠杆菌的最低抑菌浓度MIC(g/mL)分别为板蓝根0．05、穿心莲0．05、黄芪0．025、黄柏0．05、柴胡0．05、生地0．05、甘草0．05、当归0．025，“毒菌杀”方剂为0．05；对沙门氏菌的MIC分别为板蓝根0．05、穿心莲0．025、黄芪0．025、黄柏0．05、柴胡0．025、生地0．05、甘草0．025、当归0．05，“毒菌杀”方剂为0．025；而牛胆汁对这两种致病菌的最低抑菌浓度分别为2％和1％。说明“毒菌杀”方剂对大肠杆菌、沙门氏菌具有明显的抑制作用。     

土耳其斯坦东毕吸虫肌动蛋白基因的克隆及其序列分析

目的利用RT-PCR和RACE技术克隆土耳其斯坦东毕吸虫肌动蛋白基因全长序列并进行序列分析.方法根据日本血吸虫和曼氏血吸虫肌动蛋白基因的保守区设计引物,利用RT-PCR扩增出土耳其斯坦东毕吸虫的肌动蛋白基因的大片段,再结合RACE技术分别得到肌动蛋白的3＇端和5＇端,将三部分序列拼接后获得肌动蛋白基因的全长cDNA序列并进行序列分析.结果成功克隆了土耳其斯坦东毕吸虫肌动蛋白的全长cDNA并提交GenBank,登录号为DQ017265,核酸序列比对表明东毕吸虫肌动蛋白基因的核苷酸序列和日本血吸虫、曼氏血吸虫的同源性分别为90%和91%.结论土耳其斯坦东毕吸虫肌动蛋白的全长cDNA的克隆为进一步表达及其生物学性能的分析提供了理论基础.     

隐性白肉鸡羽速自别雌雄系的选育(1)

本研究根据现代遗传学基因测交理论,共用32只表型慢羽公鸡与245只快羽母鸡组成测交试验.结果表明,所测的32只公鸡无一只为纯合慢羽基因型.但发现测交后代的快慢羽分布比例与孟德尔遗传上的分离定律完全吻合.同时通过混合精液输精,实施扩群繁育,其中选留慢羽种母雏1460只,表型慢羽种公雏150只,从而为建立隐性白鸡慢羽系奠定了基础.