狂犬病快速诊断方法的建立和应用

根据狂犬病病毒核蛋白基因保守区序列设计1对引物，建立了用于狂犬病病毒特异性核酸检测的RT-PCR技术。该技术可从狂犬病病毒CVS株、8202株和SRV9株的含毒细胞培养物及鼠脑组织中，扩增出443bp的核酸片段，检出核酸的敏感性约为3pg。对30份不同种动物脑组织的检测结果与小鼠脑内接种试验(MIT)的测定结果完全吻合，但前者可在3h内直接对组织匀浆进行诊断，具有快速、简便和敏感的优点。     

出口禽肉风险分析研究

根据我国近十几年出口禽肉发生的有关案例与各主要进口国的兽医卫生要求，依据《国际动物卫生法典》的有关规定，对影响我国出口禽肉安全卫生质量的家禽疫病病原、各种食源性致病菌、农兽药物残留、放射性残留等因素进行风险分析，确定影响出口禽肉安全卫生的关键因素，由此制定保障出口禽肉安全卫生的管理措施。这是我国首次对出口禽肉进行风险分析研究。     

Combined microRNAome and transcriptome analysis of follicular phase and luteal phase in porcine ovaries

The aim of this study was to explore the expression difference of miRNAs and mRNAs between the follicular phase (FP) and luteal phase (LP) in porcine ovaries and provide a theoretical basis for the research on mammalian reproductive regulation. RNA‐Seq and miRNA‐Seq were used to identify differentially expressed genes (DEGs) and miRNAs (DEMs) between the FP and LP in ovaries of six sows (3‐year‐old Yorkshire pigs with similar weights and same parities). Bioinformatic analysis was used to screen potential genes and miRNAs related to porcine ovarian function. Real‐time qualitative PCR was used to validate the sequencing results. RNA‐Seq results showed that 3,078 genes were up‐regulated, and 1,444 genes were down‐regulated in the LP compared with the FP, and DEGs were significantly enriched in 242 Gene Ontology (GO) terms and 33 Kyoto Encyclopedia of Genes and Genomes (KEGG) pathways. miRNA‐Seq identified 112 DEMs, of which 25 were up‐regulated and 87 were down‐regulated in the LP compared with the FP. We obtained 186 intersection genes (IGs) between the 4,522 DEGs and 2,444 target genes predicted from the 112 DEMs. After constructing a miRNA‐gene‐pathway network, we identified key miRNAs and genes including miR‐17‐3p, miR‐214, miR‐221‐5p, miR‐125b, FGF1, YWHAG, YWHAZ, FDFT1 and DHCR24, which are enriched in Hippo and PI3K‐Akt signalling pathways, and various metabolic pathways. These results indicate that these key genes and miRNAs may play important roles in the developmental transition from FP to LP in porcine ovaries and represent candidate targets for further study.     

病毒性出血性败血症病毒液相芯片检测技术的建立

为建立检测病毒性出血性败血症病毒（VHSV）的液相芯片快速检测技术,用DNAStar软件对GenBank中VHSV的G基因进行序列分析,设计VHSV特异性引物并标记生物素。探针氨基化修饰并与荧光编码微球偶联后与VHSV RT-PCR产物杂交反应,用液相芯片仪器检测荧光信号。结果表明液相芯片检测体系能够正确检出VHSV。病毒核酸的最低检出量为10pg,检测特异性高,说明初步建立了检测VHSV的液相芯片技术,为VHSV的检测提供了新方法。     

Sampling and Investigating Zearalenone Contamination of Feeds and Feedstuffs of Pig Farms in Beijing Area

本研究采用免疫亲和柱高效液相色谱法测定了北京地区猪场饲料原料及全价饲料中玉米赤霉烯酮(ZEN)的含量,以了解北京地区饲料中ZEN的污染情况.试验抽样采集北京市昌平区、大兴区、延庆区、平谷区、顺义区5个区县15个猪场131份饲料样[55份玉米、豆粕、麸皮、干酒糟及其可溶物( DDGS)原料,76份猪全价饲料]进行ZEN含量的测定.结果表明:玉米、豆粕、麸皮、DDGS和全价饲料中ZEN的检出率分别为100.00％、54.45％、100.00％、100.00％和58.88％,超标率分别为0.00％、0.00％、0.00％、41.18％和0.00％,平均含量分别为109.08、9.19、14.92、882.68和58.88 μg/kg.结果提示,不同饲料原料中ZEN含量存在差异,DDGS中ZEN平均含量超标,猪全价饲料及玉米、豆粕等饲料原料中ZEN平均含量均未超标.     

12个微卫星DNA标记在江口萝卜猪群体中的遗传多样性研究

采用12对微卫星引物对江口萝卜猪群体的遗传多样性进行研究。结果发现12个微卫星位点在江口萝卜猪群体中均具有多态性,平均基因杂合度、多态信息含量和有效等位基因数分别为0.760 1、0.707 9和4.173 7。实验结果表明,江口萝卜猪群体具有较高的遗传多样性,群体内部变异较大,若通过家系育种有较大的选育潜力。     

PPARγ和PCNA在口腔鳞癌组织的表达及临床意义

目的 探讨过氧化物酶体增殖物激活受体(PPARγ)与增殖细胞核抗原(proliferating cell nuclear antigen,PCNA)在口腔鳞癌中(oral squamous-cell carcinoma,OSCC)的表达及其生物学意义.方法 采用免疫组织化学和流式细胞术检测50例口腔鳞状细胞癌、癌旁黏膜(距瘤缘2 cm)和切缘正常黏膜(距瘤缘≥5 cm,镜下未见癌浸润)标本中PPARγ和PCNA的表达.结果 PPARγ在癌组织中的阳性表达率为68.0% (34/50),高于癌旁组织(26.0%,13/50)和正常黏膜组织(2.0%,1/50) (P ＜0.05);PCNA在癌组织中的阳性表达率为72.0% (36/50),高于癌旁组织(26.0%,13/50)和正常黏膜组织(4.0%,2/50)(P＜0.05).流式细胞术检测PPARγ在鳞癌组织中的表达为(396.56±33.39),明显高于癌旁组织(333.36±15.93)及正常口腔黏膜组织(289.28±13.80)(P＜0.05).PCNA在鳞癌组织中的表达为(543.11±41.55),明显高于癌旁组织(456.97±23.86)和正常口腔黏膜组织(409.40±40.07) (P ＜0.05).PPARγ和PCNA的表达与细胞分化程度、淋巴结转移均有相关性(PPARγ,r分别为0.497、0.392,P＜0.05;PCNA,r分别为0.324、0.561,P＜0.05),且二者在口腔鳞癌中的表达呈正相关.结论 口腔鳞癌组织中PPARγ和PCNA的表达均升高,可能与口腔鳞癌的发生、发展相关.     

鹅DHRS7基因克隆、序列分析及其在鹅肥肝形成过程中的表达特点

为获得鹅DHRS7基因全长cDNA,并探讨该基因是否参与鹅肥肝的形成过程。本研究应用抑制消减杂交文库获得鹅DHRS7基因部分EST序列,采用RACE技术扩增了鹅该基因全长cDNA,并对其序列进行了生物信息分析;用荧光定量PCR技术检测了DHRS7在鹅肝脏、皮脂、腹脂等10个组织中的差异表达,以及填饲对鹅肝脏中DHRS7表达变化的影响。结果发现,鹅DHRS7基因cDNA全长1 279bp,含一个完整的开放阅读框1 011bp(可编码336个氨基酸),25bp的5′UTR和243bp的3′UTR序列;生物信息学分析结果显示,鹅DHRS7含有跨膜结构域以及NADP结合位点,且在这些功能区域变异较少;荧光定量结果显示,DHRS7在鹅肝脏和脂肪组织中都有较高表达,填饲后鹅肝脏中DHRS7的表达水平显著上调(P<0.05)。以上结果表明,DHRS7在鹅肥肝形成过程中具有重要的作用。     

猪瘟病毒E2蛋白与猪RACK1相互作用的鉴定

为筛选和鉴定与猪瘟病毒(CSFV)E2蛋白相互作用的猪宿主蛋白,我们采用酵母双杂交方法筛选猪肺泡巨噬细胞表达文库得到与CSFV E2蛋白相互作用的宿主细胞RACK1蛋白,经共转化试验和GST pull-down试验进一步证实两者可以特异性结合,并且共聚焦试验表明两者共定位于细胞的细胞浆。本研究显示E2蛋白与宿主细胞RACK1蛋白存在相互作用,RACK1在CSFV感染过程中所发挥的功能有待进一步研究。     

Effects of animal liver and bile extracts on biochemical values of rat ethanol‐induced fatty liver

The purposes of this study were to assess the improvement of fatty liver induced by ethanol with animal liver and bile extracts. This research aimed to increase the economic values of animal liver and bile extracts and used these to reduce damage of ethanol‐induced fatty liver. Extracts came from animal liver and bile, including pig bile powder, pig liver extract, a mixture of pig bile powder and pig liver extract, chicken bile powder, chicken liver extract, and a mixture of chicken bile powder and chicken liver extract, and these were fed to Long‐Evans rats. The results showed that rats fed ethanol for long terms could increase values of aspartate transaminase, cholesterol, γ‐glutamy‐transferase and alkaline phosphatase. Pig bile powder could decrease the values of aspartate transaminase, cholesterol and γ‐glutamy‐transferase. The significances also decreased on aspartate transaminase, γ‐glutamy‐transferase and aspartate transaminase, which were carried out with the pig liver extract treatment. These results suggest pig bile and liver extracts have high potential to improve rats' ethanol‐induced fatty liver with serum biochemical parameters.