猪源伪狂犬病病毒AH02LA株糖蛋白的基因序列测定与对比分析

为了分析猪源伪狂犬病病毒AH02LA株糖蛋白的基因序列特征,本研究设计了17对特异性引物,通过PCR扩增AH02LA株的11个糖蛋白基因并进行序列测定,然后将其与PRV变异株(TJ株与HeN1株)和PRV经典株(Bartha株与Kaplan株)作比对分析。结果:成功扩增了11个糖蛋白基因序列,序列比对发现,AH02LA株的gB、gD、gG、gK和gM基因与PRV变异株的同源性为100%,而与PRV经典株的同源性为98%~99%;AH02LA株的gC、gE和gI基因与PRV变异株的同源性为99%,而与经典株的同源性为95%~97%,而且AH02LA株的gB、gC、gD、gE、gI和gN基因的插入或缺失也与变异株完全一致。研究表明,AH02LA株的主要糖蛋白基因序列与变异株高度同源,该毒株是一株典型的变异株。     

山东地区三株鸽Ⅰ型副粘病毒的分离及鉴定

2005年在山东地区部分肉鸽养殖场出现鸽子大量死亡现象,从死亡鸽中分离到三株鸽Ⅰ型副粘病毒(SD05027,SD05028,SD05029),其鸡胚平均死亡时间(MDT)分别为69h,69.6h,81.6h;鸡脑内接种指数(ICPI)为1.31,1.43,1.48,证明此次分离的三株病毒株均属速发型新城疫病毒。应用RT-PCR技术对F基因重要功能区片段扩增后进行序列测定,分析表明,F蛋白裂解位点处的序列(112R/K-R-Q-K-R-117F)与新城疫强毒在这一区域的序列相符。与多株已报道的NDV参考株相应片段进行序列比对和基因进化树分析,将其鉴定为基因VIb型。     

水貂隐孢子虫病流行病学调查及虫种的初步鉴定

为初步了解水貂隐孢子虫病的流行情况,作者于2005年11月份用饱和蔗糖溶液漂浮法检查了河北省肃宁县某水貂养殖场的469份粪便样品。结果,8份粪便样品为隐孢子虫阳性,总感染率为1.71%(8/469)。其中,白貂感染率为2.15%(5/233)、灰貂感染率为2.08%(1/48)、黑貂感染率为1.06%(2/188)。所查的8份隐孢子虫阳性样品均来自5~6月龄的水貂,表明幼龄水貂容易感染隐孢子虫病而老龄水貂不易感染。另外,8份阳性样品多数来自雄性水貂,显示水貂的隐孢子虫感染可能存在性别的差异性。根据卵囊形态和大小将水貂隐孢子虫初步鉴定为小球隐孢子虫(Cryptosporidium parvum)。同时,利用所收集的隐孢子虫卵囊进行了小白鼠感染试验,结果表明水貂源隐孢子虫不感染免疫抑制状态下的昆明系小白鼠。     

一株山羊支原体山羊肺炎亚种的分离鉴定与分子特征

从送检的山羊肺炎肺脏中成功分离到一株支原体，经过3次克隆纯化后进行生化试验、电镜观察、PCR及酶切、基因特征鉴定，结果显示分离物SD3属于山羊支原体山羊肺炎亚种成员。将培养物经气管接种2只山羊可引起1只山羊典型发病，体温升高至41．5℃，IgG和IgM抗体效价明显升高，其中IgG抗体变化与临床表现基本同步。剖检发现肺脏发生严重病变，并从中再次分离到该病原体。     

Isolation and Identification of Erysipelothrix rhusiopathiae from Abattoirs in Shanghai Area

In order to comprehend the status of Erysipelothrix rhusiopathiae carried in swinery in Shanghai area, samples of pigs were collected from some standard abattoirs in Shanghai area, including nasal swab, lung, tonsil and mandibular lymph nodes. Strains were isolated from these samples for detecting the Erysipelothrix rhusiopathiae. Several kinds of methods were used, such as VITEK 2 Compact system and VITEK MS system. A pair of primers was designed to amplify the 16S rRNA gene. 16 PCR products selected randomly were sequenced and 16S rRNA homology analysis was conducted. As a result, strains were isolated from 49.07% (105/214) samples and were identified as Erysipelothrix rhusiopathiae.16S rRNA homology in strains of isolation and reference were 99.6% to 100.0%. The result indicated that the situation was very severe for so many carriers of Erysipelothrix rhusiopathiae in health group in nursery.     

Isolation and Identification of Variant HeNZK-2014 of Pseudorabies Virus and Sequence Analysis of gE Gene

In order to learn the situation of pig pseudorabies virus (PRV) variant in this study, tissue samples such as lymph nodes which were collected from clinical pigs with suspected PRV infection were identified by PCR. PRV positive sample were inoculated on PK-15 cells after grinding and degerming, with further experiment including virus isolation, plague purification, PCR and IFA identification, TCID₅₀ confirmed by Reed-Muench method, inoculation test and observation of clinical symptoms in mice. The gE gene of purified PRV and brain tissue samples of dead mice were identified by sequencing analysis. The results showed that the virus grown on PK-15 cells could produce typical cytopathic effect (CPE) after 24 h; After three rounds of plaque purification,the isolate was PRV positive identified by PCR and IFA, and nominated as HeNZK-2014; The TCID₅₀ of the isolate was 10^-9.77/0.1 mL; The virus in 1×10⁸ TCID₅₀ inoculation was able to cause itching, tearing, death in infected mice, and PRV could be detected in tissues of dead mice; The molecular genetic variation analysis of gE gene by PCR amplification and clone sequencing indicated that the gE gene from brain tissue of infected mice shared 100.0% homology with HeNZK-2014, and located in a relatively independent branch with newly pandemic isolates in recent years after 2011, but was far from the classical strains before 2011, and both had two insertion of aspartic acid (D) at sites of 48 and 496 amino acids, which were considered to be the typical characteristics of PRV variants. This study successfully isolated a PRV variant, which laid a foundation for further research on vaccine development, prevention and control against PRV variants.     

低聚木糖对不同阶段猪的生长抗病作用及效益分析

我部于2005年5月25日至6月24日,在琉璃河三街猪场对40头三元杂交育成猪进行了饲料添加低聚木糖的第一组试验,代号为050525-31C三40-001,其效果明显。为了进一步证实低聚木糖的应用原理和实用价值,我部接着又进行了第二组跟踪连续试验和第三组的多头试验。现将试验结果报道如下。     

鸭疫里默氏菌的分离鉴定

本研究经过菌落形态、染色形态、生化实验以及PCR实验,从来自湖北4个鸭场的81份病料中,分离到11株鸭疫里默氏茵。以5.0×10~8CFU/mL剂量感染健康昆明鼠和健康樱桃谷鸭,鼠和鸭分别在感染后7 h和12 h出现症状,直到感染后1周,实验动物均死亡,而对照组则未出现任何症状,表明该菌株为有毒力菌株,药物敏感实验结果显示部分细菌对某些药物已经产生耐药性。     

不同细胞因子对水牛原始生殖细胞传代培养的影响

为探讨不同细胞因子对水牛原始生殖细胞（PGCs）传代培养的影响，将PGCs分别采用A、B、C、D、E、F和G共7种培养基进行培养，即A组：基础液＋10ng／mL白血病抑制因子（LIF）＋10ng／mL碱性成纤维细胞生长因子（bFGF）；B组：基础液＋20ng／mL LIF＋20ng／mL bFGF；C组：基础液＋20ng／mL LIF＋10ng／mL bFGF；D组：基础液＋20ng／mL LIF；E组：基础液＋20ng／mL LIF＋20ng／mL bFGF＋20ng／mL干细胞因子（SCF）；F组：基础液＋20ng／mL LIF＋40ng／mL bFGF＋40ng／mL SCF；G组（对照组）：基础液。将机械法分离的PGCs小集落接种到水牛胎儿成纤维细胞（BEF）饲养层上进行传代培养。结果，原代时，A、B、C、D、E和F组的克隆数目都显著高于对照组（P％0．05），其中E和F组的克隆数目显著高于A组（P〈0．05），而与B、C、D组差异均不显著（P〉0．05）；1～8代时，B、C、D、E、F组的克隆数目显著高于A组（P〈0．05）；对照组传代数仅为2代，A组为5代，而B、C、D、E和F组均为8代以上。结果表明，在传代过程中，LIF起主要作用，20ng／mL的LIF浓度可以满足水牛PGCs传代培养的需要。     

把好养猪业的最后一关

随着养猪规模化、集约化程度的不断提高，阶段饲养也越来越明显．多数猪场采用四阶段饲养三次转群生产工艺。即配种妊娠阶段、产仔阶段、保育阶段、育肥阶段。一般认为这四阶段中．育肥阶段猪只体重较大．抗病能力较强。比较好饲养。而易于疏忽管理，让养猪企业感到“不必花太多的功夫”，