对图书馆员常态量化绩效管理的实践探索

图书馆在对馆员日常管理中,由于对其品德、业绩、能力等综合指数缺乏比较精确的量化评价,往往使部分馆员认为年度考核不公、流于形式或失真,常常在工作中引发消极情绪。分析馆员考核结果失真的原因,研究失真的对策,应成为图书馆界研究的一个重要课题。以东北林业大学图书馆为例,将图书馆试行一年来绩效管理的实践探索加以总结,以期对日后推动科学化管理有所助益。     

实时荧光PCR检测马铃薯白线虫技术研究

马铃薯胞囊线虫是马铃薯上最重要的有害生物之一,也是我国特别关注的重要植物检疫性线虫.针对马铃薯白线虫ITS序列,我们设计了引物和TaqMan探针,使用15种马铃薯胞囊线虫群体和4种其它胞囊线虫样品进行验证,可高度灵敏地检测单个马铃薯白线虫的胞囊或幼虫,最高检测灵敏度达到10fs;同时开展了混合样品和未知样品的检测,证明了引物的专化性和TaqMan探针特异性.该检测方法可自动化检测马铃薯白线虫并进行定量,适合进行标准化的常规检测.     

Use of real-time PCR to examine the relationship between disease severity in pea and <Emphasis Type="Italic">Aphanomyces euteiches</Emphasis> DNA content in roots

Aphanomyces euteiches causes severe root rot of peas. Resistance is limited in commercial pea cultivars. Real-time fluorescent PCR assay specific for A. euteiches was used to study the relationship between disease severity and pathogen DNA content in infected peas. Five pea genotypes ranging in levels of resistance were inoculated with five isolates of A. euteiches. Plants were visually rated for disease development and the amount of pathogen DNA in roots was determined using the PCR assay. The susceptible genotypes Genie, DSP and Bolero tended to have significantly more disease and more pathogen DNA than the resistant genotypes 90-2079 and PI 180693. PI 180693 consistently had less disease, while 90-2079 had the lowest amount of pathogen DNA. The Spearman correlation between pathogen DNA quantity and disease development was positive and significant (P < 0.05) for three isolates, but was not significant for two other isolates. This suggests that the real-time PCR assay may have limited application as a selection tool for resistance in pea to A. euteiches. Its utility as a selection tool would be dependent on the correlation between disease development and pathogen DNA content for a given pathogen isolate. The accuracy and specificity of the real-time PCR assay suggests considerable application for the assay in the study of mechanisms of disease resistance and the study of microbial population dynamics in plants.     

有害生物风险分析定量评估模型及其比较

全球化的进程使有害生物入侵问题日益严重,植物检疫工作备受重视。有害生物风险分析(pest risk analysis,PRA)是植物检疫的支撑技术之一,风险评估是其核心内容,定量评估模型的研究与应用成为近30年来该领域的热点。本文在收集、整理国内外PRA文献和相关信息的基础上,针对有害生物入侵风险半定量评估模型、定量评估模型及软件的发展进行了系统性的回顾和分析。同时,我们比较了主要模型和软件的特点、优势和局限性,归纳总结出了适用于不同起点的有害生物定量风险评估集成技术体系,并展望了我国有害生物风险分析技术的未来发展。本综述能够为我国生物入侵防控管理机构、推广部门、高等院校及科研单位提供重要的工作参考,对植物检疫工作具有理论和实践意义。     

单管实时荧光RT PCR方法同时检测大豆种子中的菜豆荚斑驳病毒和烟草环斑病毒

 本研究建立了大豆种子中菜豆荚斑驳病毒（BPMV）和烟草环斑病毒（TRSV）单管双重实时荧光PCR检测方法。将含有相同浓度的分别带有BPMV和TRSV CP基因的质粒溶液作为阳性对照,以受两种病毒侵染的大豆种子作为待测样品进行实时荧光PCR检测,结果表明能从同一管中同时检测出这两种病毒而不发生交叉反应。尽管在阳性对照中,二者的检测限相当,均可达到35 pg/mL,但在实际应用中,两种病毒由于在大豆种子中的浓度不一致而存在一定的差别。该方法快速、灵敏、简便,同时特异性更强,在出入境检验检疫中具有广泛的应用前景。     

Pathogenesis-related gene expression in rice is correlated with developmentally controlled Xa21-mediated resistance against Xanthomonas oryzae pv. oryzae

Disease resistance mediated by the resistance gene Xa21 is developmentally controlled in rice. We examined the relationship between Pathogenesis Related (PR) defense gene expression and Xa21-mediated developmental disease resistance induced by Xanthomonas oryzae pv. oryzae (Xoo). OsPR1a, OsPR1b, and OsPR1c genes were cloned and their induction was analyzed, in addition to the OsPR10a gene, at the juvenile and adult stages in response to a wildtype Xoo strain that induces a resistance response (incompatible interaction) and an isogenic mutant Xoo strain that does not (compatible interaction). We found that the adult stage leaves are more competent to express these OsPR1 genes and that the Xa21 locus is required for the highest levels of induction.     

利用绿色荧光蛋白GFP研究稻瘟病菌与水稻的互作

稻瘟病菌Magnaporthe oryzae严重威胁水稻的产量与质量,明确稻瘟病菌与水稻互作过程及机理,对防治稻瘟病具有重要意义。本研究利用稻瘟病菌常用致病菌株GUY11和ZB25,构建了绿色荧光蛋白GFP的过量表达菌株,并通过荧光显微观察菌株侵染寄主水稻过程中侵染结构的形成与发育,包括孢子萌发、附着胞形成、侵染钉形成、侵染菌丝增殖、坏死斑形成及产孢。另外,通过比较过量表达菌株对稻瘟病高抗水稻和易感水稻的侵染过程,发现侵染过程的差异主要集中于侵染钉的穿透和侵染菌丝的定殖。本研究为分析稻瘟病菌对寄主水稻的定殖规律提供了一种有效工具。     

Isolation and pathogenicity of Colletotrichum spp. causing anthracnose of strawberry in south west Spain

Anthracnose, caused by Colletotrichum spp., is a major disease of cultivated strawberry, Fragaria × ananassa. This study identifies the Colletotrichum spp. which causes strawberry anthracnose in the southwest of Spain. A survey of the region was carried out, and the strains isolated were identified as C. acutatum by using the polymerase chain reaction (PCR) with genus and species-specific primers, demonstrating that this species is currently the causal agent of strawberry anthracnose in the studied region. The pathogenicity of C. acutatum and C. gloeosporioides strains was evaluated on two principal strawberry cultivars (cvs Camarosa and Ventana) under field conditions, the latter being more pathogenic than the former.     

龙眼体胚发生早期miR166初级体的克隆与表达分析

为了解龙眼miR166初级体基因Pri-miR166 S53结构特点及其前体和成熟体在龙眼体胚发生早期的表达模式,采用SMART~(TM) RACE试剂盒和PCR扩增技术克隆龙眼体胚早期miR166基因的初级体(Pri-miR166 S53),确认其转录起始位点,并预测其含有的潜在ORF;利用龙眼基因组数据库提取其启动子序列,预测其含有的顺式作用元件;用实时荧光定量PCR对龙眼体胚发生早期及不同激素处理下的胚性愈伤组织中miR166基因的前体(Pre-miR166 S53)和成熟体(miR166a.2)表达模式进行分析。结果表明:获得长317 bp的Pri-miR166 S53基因初级体序列,对其进行翻译,得到一条长13个氨基酸序列的miPEP(MLCFVDALFLIST)。利用生物信息学软件分析Pri-miR166 S53基因的启动子序列发现,除了具有TATA/CAAT-box外,还含有生长素、脱落酸、乙烯、水杨酸、茉莉酸甲酯及spl、HSE等特异作用元件。实时荧光定量PCR分析表明,在2,4-D调控的龙眼体胚发生早期过程中,从胚性松散型愈伤组织发育到球形胚的过程中,Pri-miR166 S53基因的前体pre-miR166 S53和成熟体miR166a.2都表现为下调趋势;而在无2,4-D调控的龙眼体胚发生早期中,pre-miR166 S53和miR166a.2表达模式不同。此外,pre-miR166S53随ABA和乙烯处理浓度升高呈下调表达,而对不同浓度2,4-D处理无应答;miR166a.2随2,4-D、ABA处理浓度升高呈下调表达,而在乙烯处理下呈上调表达。上述研究结果提示miR166前体和成熟体在对外源激素应答的模式上并不呈简单线性相关,可能存在多层次、多方位的调控。     

山羊TNNT3基因可变剪切及其对骨骼肌细胞分化的作用

【目的】快速骨骼肌肌钙蛋白T(fast skeletal troponin T3,TNNT3)作为肌钙蛋白(troponin, Tn)家族成员,调节横纹肌收缩、参与骨骼肌的生长发育并影响家畜肉质性状。通过获得山羊TNNT3基因的可变剪切体,分析山羊TNNT3基因可变剪切的表达模式及其在肌细胞分化中的作用,深入解析TNNT3基因在山羊骨骼肌生长发育过程中的作用机制。【方法】基于NCBI已公布山羊TNNT3基因(NM₀01314210.1)和牛TNNT3基因(XM₀10821200)mRNA序列,使用软件Primer Premier6.0设计引物,以简州大耳羊胚胎期和出生后7个阶段骨骼肌为试验材料,克隆测序获得山羊TNNT3基因的CDS区可变剪切体,利用软件ORF Finder、EditSeq、DNAMAN、ClustalW和MEGA_X10.1.8等对序列进行生物信息学分析;进一步设计实时荧光定量(real-time PCR,RT-qPCR)及半定量引物,研究TNNT3基因剪切体在7个不同组织(背最长肌...