Molecular investigation on the presence of canine parvovirus in Egypt

Canine parvovirus type 2 (CPV-2) causes a highly contagious gastroenteritis disease of dogs and wild canids. To investigate the CPV-2 prevalence in Dakahlia Governorate, Egypt, a total of 50 fecal swabs were collected from suspected diseased dogs during 2016–2017. Out of 50 collected samples, 35 samples (70 %) presented positive results for CPV-2 using immuno-chromatography (IC) as a rapid test. CPV-2DNA was detected in 42 samples (84 %) by using polymerase chain reaction (PCR). The frequencies of CPV-2 were significantly higher in German shepherd breed (46 %; 23/50) and in age groups less than 6 months (76%; 38/50). We evaluated the breed, age, sex, rapid test results and clinical signs as predictors for classification of animal status into infected and not infected. The best predictors for classification process were rapid test result and clinical signs. Both CPV-2b and CPV-2c subtypes were detected by CPV2-VP2 gene sequences analysis. Deduced amino acid sequences alignment showed substitutions at 3 sites (Arg453Pro, Ala574Glu and Gln457Leu). Further investigations are needed to reveal the genetic and antigenic relation between field and vaccinal strains of CPV-2 in Egypt.     

Serologic and molecular survey of horses to Coxiella burnetii in East of Iran a highly endemic area

There are few reports about Q fever in horse populations worldwide. This study aimed to detect the C. burnetii infection by serologic and molecular confirmation using commercial ELISA kit and real-time PCR in the East of Iran a region highly endemic. A total of 177 blood samples and 115 vaginal swabs were randomly collected from horses in East of Iran. The sera samples were analyzed for anti C.burnetii Ig G antibodies by a commercial ELISA kit and nucleic acid extraxted from vaginal samples were used to determine the C. burnetii DNA by real-time PCR assay. Antibodies were detected in 5.64 % (10/177) of sera samples and C. burnetii DNA was detected in 7.82 % (9/115) of horse vaginal samples. There was no significant difference in seroprevalence in different sex, age and breed groups. Our study showed that horses could be considered as a mild potential reservoir of C. burnetii which may be effective on horse health status. However, additional studies are needed to assess whether the horse could be considered as a relevant transmission risk indicator for Q fever.     

甘蔗热带种金属硫蛋白家族基因的克隆及响应重金属胁迫的表达分析

金属硫蛋白是一类富含巯基的低分子量蛋白,在植物的重金属解毒及细胞氧化还原调控等方面起重要的作用。本研究以甘蔗热带种Badila组培苗为材料,分别测定了其在CdCl2、ZnSO4和CuCl2水溶液培养条件下地上部和地下部的重金属含量,结果显示其对上述3种重金属有较强的耐受与富集能力。继而克隆了ScMT1(登录号为KJ504373)、ScMT2-1-5(登录号为MH191346)和ScMT3(登录号为KJ5043704)3个金属硫蛋白家族基因,它们分别属于植物MT亚家族中的MT1、MT2和MT3型基因。ScMT1含有1个内含子和2个外显子,开放阅读框(Open Reading Frame,ORF)长228 bp,编码75个氨基酸;ScMT2-1-5含有2个内含子和3个外显子,ORF长246 bp,编码81个氨基酸;ScMT3含有1个内含子和2个外显子,ORF长198 bp,编码65个氨基酸。RT-qPCR显示,Cd2+胁迫下,在甘蔗地上部和地下部,ScMT2-1-5均连续显著上调表达,而ScMT1的上调应答出现延迟。ScMT3在地上部的上调应答出现延迟,在地下部呈“扬-抑”趋势,提示甘蔗响应Cd^2+胁迫过程中ScMT2-1-5起更积极的作用,ScMT1参与胁迫后期的分子响应,而ScMT3不起主导作用。Cu^2+胁迫下,地上部ScMT1连续显著上调表达,ScMT2-1-5和ScMT3呈总体上调的表达趋势;地下部,ScMT1和ScMT2-1-5的上调表答均出现延迟,仅在胁迫后期显著上调表达,而ScMT3仅在胁迫前期显著上调表达。该结果提示了ScMT1、ScMT2-1-5和ScMT3在Cu2+胁迫响应过程中的协作关系,三者共同参与了地上部的胁迫响应,其中ScMT1起更积极的作用;此外三者还先后参与了地下部对Cu^2+胁迫的分子响应。Zn^2+胁迫下,ScMT1和ScMT3分别仅在地上部和地下部显著上调表达;ScMT2-1-5在地上部和地下部均呈“扬-抑”的应答趋势;提示了在甘蔗响应Cd^2+胁迫应答过程中ScMT1和ScMT3分别在地上部和地下部起主要作用,ScMT2-1-5参与了胁迫前期的分子响应。ScMT1、ScMT2-1-5和ScMT3在甘蔗不同组织中及在重金属(Cd^2+、Zn^2+或Cu^2+)不同累积水平下呈现出相似或互补的应答特性,提示上述甘蔗MT家族不同成员在重金属解毒及细胞氧化还原调控等方面产生了功能分化,且三者在应对过量Cd^2+、Zn^2+或Cu^2+对甘蔗组织造成伤害的过程中存在时空上的协同作用。该研究为深入理解多倍体植物甘蔗中MT家族各成员基因在重金属耐受过程中的协同作用机制奠定了基础。     

Real-time RT-qPCR assay to detect sequences in the Piscine orthoreovirus-1 genome segment S1 associated with heart and skeletal muscle inflammation in Atlantic salmon

During the last decade, Piscine orthoreovirus was identified as the main causative agent of heart and skeletal muscle inflammation (HSMI) in Atlantic Salmon, Norway. A recent study showed that PRV-1 sequences from salmonid collected in North Atlantic Pacific Coast (NAPC) grouped separately from the Norwegian sequences found in Atlantic Salmon diagnosed with HSMI. Currently, the routine assay used to screen for PRV-1 in NAPC water and worldwide cannot differentiate between the two groups of PRV-1. Therefore, this study aimed at developing a real-time polymerase chain reaction (RT-qPCR) assay to target the PRV-1 genome segments specific for variants associated with HSMI. The assay was optimized and tested against 71 tissue samples collected from different regions including Norway, Chile and both coast of Canada and different hosts farmed Atlantic Salmon, wild Coho Salmon and escaped Atlantic Salmon collected in British Columbia, West Coast of Canada. This assay has the potential to be used for screening salmonids and non-salmonids that may carry PRV-1 potentially causing HSMI.     

基于qPCR和LAMP技术的马铃薯晚疫病菌快速检测方法

马铃薯晚疫病菌（Phytophthora infestans）能侵染多种茄科植物,它引起的马铃薯晚疫病,是马铃薯生产中的第一大病害。为了开发能在田间快速检测马铃薯晚疫病病原的方法,利用P. infestans T30-4基因组测序数据的contig 1.18131,设计qPCR和LAMP引物,优化扩增条件后得到引物的特异性和灵敏度,最后通过检测田间收获薯块,比较形态学传统方法、qPCR及LAMP的差异。特异性检测结果发现,qPCR和LAMP仅在含有P. infestans DNA模板的体系有阳性扩增,在寄主和其他微生物DNA中均无扩增;在优化的条件下,qPCR和LAMP的检测下限可达1×10 ^-6ng/μL,在有寄主和其他微生物DNA存在的条件下,引物的灵敏度没有显著差异。利用两种快速方法对在大理、丽江及昆明3个地区田间收获薯块上检测发现,qPCR和LAMP方法得到的检出率差异极为不显著（P=0.420）,两种快速检测方法和形态学鉴定方法检出率差异极显著（P=0.009）。在大理、丽江及昆明3个地区的薯块中,两种分子检测方法检出率均比形态学方法高。其中,qPCR检测方法比形态学方法分别提高了12.00%、2.00%、8.70%;LAMP检测方法比形态学方法分别提高了11.30%、2.00%、8.70%。     

不同地区楼葱栽培种的性状与品质分析

为了研究不同地区楼葱的特性,试验对我国不同地区12个楼葱栽培种的数量性状和品质性状进行了测定分析。14个数量性状的相关分析结果显示,主成分分析数量指标后,单株质量、株高、假茎质量、花葶高、叶形指数和假茎指数影响分类;相关性分析说明主要数量指标间具有极显著相关性(P<0.01)。聚类分析后,遗传距离为3.1时可将楼葱种质根据所得主要数量性状分为4个类群。测定不同地区楼葱6个品质指标后,相关性分析结果表明,紧实度与蛋白质含量、干物质率、香辛油含量、总糖含量、游离氨基酸总量存在着极显著正相关或相关性,主成分分析表明主成分反映了89.99%的原有信息量,楼葱的干物质率与紧实度为主要成分;应用灰色关联度分析了品质与数量性状的关系,假茎直径、出叶孔间距、单株质量这3个数量性状对楼葱品质的影响居前3位。研究表明楼葱种质材料具有极其丰富的遗传多样性,宁夏同心2个地区黄水桥HSQ、石羊圈SYJ的楼葱种质距其他种质资源间亲缘关系最远且干物质率含量及紧实度最高。     

High vegetative compatibility diversity of Cryphonectria parasitica infecting sweet chestnut (Castanea sativa) in Britain indicates multiple pathogen introductions

Chestnut blight, caused by Cryphonectria parasitica, was identified in Devon, UK, in December 2016. Intensive surveys detected the disease at further sites in Devon (seven), Berkshire (one), Dorset (one), Derbyshire (four) and a cluster of eight sites in southeast London. Over 570 survey samples were tested, and 227 were positive for C. parasitica by isolation and real-time PCR. A total of 227 isolates were tested for mating type, and 197 screened for vegetative compatibility group (VCG) and compared with VCGs known from mainland Europe. The same isolates were also screened for the presence of Cryphonectria hypovirus 1 (CHV-1). Eleven VCGs were identified within the UK population. Five corresponded to already known European VCGs but six were unique. The European VCGs mainly came from the Devon, Dorset, Berkshire and Derbyshire disease outbreaks, whilst unique VCGs were almost exclusively from the southeast London cluster. Both mating types were detected, but only one mating type was present at each site, with the exception of a single Devon site. Perithecia of C. parasitica were never observed at any site. CHV-1 was found in seven isolates from three different locations and was always subtype-I, which has limited hypovirulence. Therefore, although CHV-1 is associated with C. parasitica at some outbreaks, it probably has limited impact on virulence. The diversity of VCGs and their distribution at outbreak sites, together with findings of CHV-1, suggests C. parasitica has been introduced to the UK multiple times over at least two decades through international plant trade.     

小麦种子规模化DNA提取及检测体系的优化

以小麦种子分子检测农业行业标准(NY/T 2859-2015)为基础,开发小麦种子快速、规模化提取DNA方法,优化反应体系中各组分含量,为小麦真实性快速执法提供技术支撑。通过对SDS、CTAB、高盐低p H、快速提取和试剂盒5种方法提取的DNA质量、浓度和PCR扩增效果进行比较,发现改进的高盐低p H方法提取种子的DNA质量、浓度能够满足小麦真实性鉴定中42对SSR引物重复鉴定的需求,是利用96孔深孔板和自动化移液工作站规模化、高通量提取DNA的较优方法。进一步优化结果显示该方法在65℃温浴条件下比室温的浓度高出25%,但两种温度条件下提取的DNA质量及浓度均能够满足品种鉴定的需求;沉淀时用0.5倍提取液体积的预冷异丙醇沉淀浓度最高,用室温的异丙醇沉淀的最佳体积是提取液体积的0.6倍。对标准中42对引物的最佳引物浓度和模板浓度均进行了优化,综合所有42对引物的优化结果发现,反应体系为20μL时,引物终浓度为0.437 5μmol/L,模板终浓度为10 ng/μL时扩增效率相对较高,扩增产物稳定,能够满足多重电泳的需求。     

基于实时性优化的内燃机燃烧分析系统研究

采用缸压传感器、数据采集卡、光电编码器和Lab VIEW软件,搭建在线缸压采集和实时燃烧分析系统平台,研究HCCI和RCCI燃烧模式的循环波动特性。针对单循环缸压测量过程中的通道效应干扰,基于频谱分析,采用FFT、线性插值法和IFFT等方法相结合的滤波方式,实现共振峰的在线自适应识别与实时滤波,较好地减少了单循环缸压的干扰误差,使单循环的实时燃烧分析成为可能。随后,基于实时滤波后的缸压曲线,计算得到内燃机的最大压力升高率、燃烧放热率、爆发压力等重要燃烧参数。利用程序算法中同步性良好的生产者/消费者运算模式提高数据的共享能力,实现了数据实时运算与数据快速储存的并行处理,提高了燃烧计算的实时性;针对发动机不同工作阶段采用了不同精度层次的计算方法,减少了进排气、压缩和膨胀阶段的计算耗时,在计算量较大的燃烧放热率计算部分,通过适当简化计算公式和公式节点运算模块来提高燃烧系统的实时性。最后,分析了燃烧分析系统的实时性,并进行了燃烧分析系统的实验验证。     

多重PCR检测耐除草剂转基因作物

为建立耐除草剂转基因作物的高通量检测方法,本试验以目前生产上广泛应用的5种除草剂抗性基因dmo、pat、CP4EPSPS、bar和aad1为靶标进行多重PCR(MPCR)研究。通过引物适用性测试、反应体系中的不同引物浓度和反应程序中的退火温度测试、灵敏度和特异性验证等,建立了能同时检测5种除草剂抗性基因的MPCR检测方法。结果表明,当dmo、pat、CP4EPSPS、bar、aad1基因的检测引物终浓度分别为0.2、0.2、0.3、0.4、0.2 μmol·L^-1,退火温度为63℃时5种靶标扩增效果较好,且特异性条带清晰且均一。此外,MPCR检测方法具有较好的特异性,对每种靶标的检测灵敏度均可达到0.1%。适用性测试结果显示,MPCR检测方法可对含有5种除草剂抗性基因的多种转基因作物的单个品系或多个品系混合物进行筛选检测。无假阳性和假阴性结果表明,MPCR检测方法对实际样品具有很好的适用性。本试验结果为筛选高效耐除草剂转基因作物检测技术提供了一定的理论依据。