早期断奶仔猪的断奶应激与腹泻研究

早期断奶仔猪一方面消化系统发育不成熟,吸收养分能力差,消化酶和胃酸分泌不足,正常的肠道微生物系统尚未建立;另一方面断绝了从母体获得被动免疫的来源,而自身的主动免疫发育尚未成熟。所以断奶应激造成早期断奶仔猪出现消化不良、生长迟滞、抗病力弱等“仔猪早期断奶综合症”。仔猪肠道对日粮抗原过敏从而导致肠道损伤是断奶后腹泻的根本原因。早期补饲、逐步断奶、去母留仔、合理饲喂可预防早期断奶仔猪腹泻。     

应用cDNA微阵列芯片技术筛选猪蛔虫性别差异表达基因的研究

采用cDNA微阵列芯片技术，从所构建的猪蛔虫雌、雄成虫cDNA消减文库分别挑取1044和1119个克隆，PCR扩增其插入片段，经纯化后点样于预先处理好的基片上（双点杂交），制备成cDNA微阵列芯片。将分别标记荧光素Cy3-dUTP和Cy5-dUTP的雌虫和雄虫cDNA探针，与制备好的cDNA芯片杂交（平行进行反标杂交试验）。根据每个点杂交后的Ratio值，筛选出双点杂交和正反标中都同时具有表达差异的基因克隆共1559个。将表达差异最明显的前831个克隆进行测序，获得720个有效序列，经生物信息学分析发现，雄虫特异表达的主要精于蛋白和雌虫特异表达的卵巢信息蛋白的基因序列多数与新杆属线虫存在同源性，有31个可能是新的ESTs。性别差异表达基因及其相关生物信息的获得为下一步研究基因功能奠定了基础。     

鸭源呼肠孤病毒DRV-GZ株S2基因的序列分析及其表达

采用RT-PCR方法从鸭源呼肠孤病毒DRV—GZ株中扩增出了S2基因片段,将其克隆到表达载体pET-28a（＋）中,测序验证后转化入表达宿主菌Rosetta^TM2（DE3）plysS,进行IPTG诱导表达。结果表明,重组菌可表达出相对分子质量约为50000的重组融合蛋白,在浓度为0．6mmol／L的IPTG诱导4h的情况下表达效果最好。表达的蛋白以包涵体的形式存在于菌体中。表达产物经Ni柱纯化后可得到纯度较高的目的蛋白。经Western-blot分析,所纯化的蛋白能与抗呼肠孤病毒DRV—GZ株阳性血清进行特异性的免疫印迹反应,证实表达的蛋白具有较好的反应原性。     

广西猪瘟病毒E0和E2基因的克隆及序列分析

通过分析目前广西猪瘟病毒(CSFV)的E0和E2基因特征,为了解广西地区CSFV的分子流行病学、遗传变异及综合防控提供科学依据。试验采用RT-PCR方法,对阳性猪瘟样品进行CSFV的E0及E2基因的扩增,经克隆、测序后,利用DNAStar软件对序列进行比对分析,同时绘制系统遗传进化树。结果表明,从阳性猪瘟样品中成功扩增CSFV的E0及E2基因。序列比对分析发现,GX2毒株与参考毒株的E0基因核苷酸同源性在83.1%~94.1%,其推导氨基酸同源性在85.9%~99.6%;与参考毒株的E2基因核苷酸同源性为81.7%~93.7%,其推导氨基酸同源性为89.0%~97.0%;E0与E2基因均属于基因Ⅱ群。氨基酸变异位点分析表明,E0蛋白的RNase活性区域氨基酸基序位点没有发生变异;E2蛋白中15个位点上的半胱氨酸均未发生变异,但单抗识别位点S734R发生变异。遗传进化分析显示测定的GX2毒株与近年来广西CSFV流行毒株的变异趋势相似,与中国传统疫苗株HCLV、经典强毒株Shimen的同源性较低,亲缘关系较远,与广西近年来的流行毒株GXWZ02株的同源性较高,亲缘关系较近。     

种蛋孵化死胚及孵化厅环境样本中铜绿假单胞菌的分离鉴定及其耐药性分析

本研究旨在了解种鸡场中种蛋孵化死胚和周围环境中感染或污染铜绿假单胞菌(Pseudomonas aerugino-sa,PA)的比率及分离株的耐药性.从广东省的5个规模化种鸡场采集孵化厅死胚及其周围环境样本进行PA的分离鉴定,采用K-B纸片扩散法分析其抗菌药物敏感性,并通过常规PCR检测对应的耐药基因.结果 显示,在采集...     

飞播种草综合配套技术研究及创新

飞播种草是沙化、退化草地治理的重要技术措施之一,近10年在财政部、农业部的大力支持下,全国开展了以"飞播种草 保护利用"为核心,对牧草筛选、草种组合、种子处理、地面处理、适时播种、机型选择、播后管护、合理利用8项关键技术进行组装和研究,集成应用在北方沙化退化草地区等6个不同生态区域中.在筛选以乡土草种为主的飞播草种、最佳播种时期、青藏高海拔利用直升机播种等方面实现了自主创新.在豆科草种接种根瘤菌与混合草种拌种增产菌、应用GPS导航技术、地面处理、组织管理等方面实现了集成创新.为改善草原生态环境、饲草饲料资源开发和保护生物多样性奠定了一定的基础.     

一例猫卵巢恶性颗粒细胞瘤的病理学分析

本文报道猫伴发腹腔种植性转移的卵巢恶性颗粒细胞瘤1例,较为罕见,国内外文献未见报道。1例15岁雌性家猫,因不食和腹围增大就诊。超声检查显示,左肾尾侧可见一大小约4.27 cm×2.63 cm的肿物。开腹探查,可见大网膜、肠壁及胃壁弥散性分布大量大小不等的球形肿物,左侧卵巢明显增大,表面形成坚实或柔软的结节。对肿物进行组织病理学检查,诊断为卵巢恶性颗粒细胞瘤。本文提供该病例临床和组织病理学资料,并回顾相关文献资料,希望对该肿瘤的诊疗和研究提供帮助。     

奶牛源MRSA菌株的分离鉴定和耐药性分析

本研究对部分奶牛场采集的502份隐性乳房炎试验（california mastitis test,CMT）检测呈阳性的奶样进行细菌分离、鉴定,运用多重PCR方法筛选出耐甲氧西林金黄色葡萄球菌（methicillin-resistant Staphylococcus aureus,MRSA）,并对分离出的MRSA用纸片扩散法进行药敏试验,检测其对19种抗菌药物的敏感性。结果显示,分离到细菌的奶样有452份,其中检出葡萄球菌338株,MRSA 89株;MRSA分离株主要对万古霉素、磷霉素、氯霉素和克拉霉素敏感,对青霉素、多黏菌素、大观霉素及头孢他啶具有较强的耐药性。本研究为指导奶牛乳房炎用药、MRSA菌株的快速鉴定及制定MRSA感染的防控措施提供参考。     

Analysis on Target Genes with Mutation in microRNA of Blue-shelled Chicken and White Leghorn

The study was conducted to explore the potential different characters between Blue-shelled chicken and White leghorn.Global genome microRNA was combined the identified microRNA with complementary lab-predicted microRNA.Then the two breed chicken's SNP data got by GGRS were mapped to the microRNA and focused on SNP that deliberately located in mature-microRNA.Bioinformatics method was adopted for target prediction on microRNA which had SNPs.By further gene enrichment analysis,the study found these genes enriched in 22 GO terms,10 KEGG pathways,and 3 IPA important networks.And they enriched in traits which associated with growth,such as mTOR signaling pathways,Wnt signaling pathways,growth hormone receptor networks and insulin-like growth factor Ⅰ receptor networks.And they also enriched in some laying traits,such as oocyte meiotic signaling pathways and progesterone mature oocytes signaling pathways.The methods and the results might provide references for further studies.     

Cloning and Expression of CMKLR1 Gene and Its Correlation with Intramuscular Fat in Goat (Capra hirus)

In order to enrich basic date in goat (Capra hirus) CMKLR1 gene and investigate the correlation between CMKLR1 gene expression and intramuscular fat (IMF) content in muscles, the CMKLR1 gene was cloned from the goat of subcutaneous adipose tissue by RT-PCR, characterized by bioinformatics methods. The expression profiles of CMKLR1 gene of goat in various tissues were constructed liver was benchmark, the GAPDH (GenBank accession No.: AJ431207.1) as a reference gene.Then, the correlation between CMKLR1 mRNA expression and IMF content in muscles was analyzed. The results showed that the CMKLR1 gene CDS of goat (GenBank accession No.: KT165374) was 1 089 bp. Real-time PCR indicated that CMKLR1 was widely expressed in various tissues, including heart, liver, spleen, lung, kidney, adipose, longissimus dorsi, biceps femoris and triceps brachii, and was the highest in lung (P< 0.05). Similar expression variation trend of CMKLR1 was observed between the muscles from 1 to 3 and 24 months old goat, and was the highest in biceps femoris. Reversely, in 8 to 10 months old CMKLR1 was the highest in triceps brachii. The IMF of longissimus dorsi from 24 months old was the highest. Correlation analysis demonstrated that different correlations were observed between expression of CMKLR1 mRNA and IMF content in longissimus dorsi, biceps femoris, and triceps brachii in goat. The CMKLR1 gene did not participate in the deposition of IMF in goats. The research built the theoretical basis for further studies about the CMKLR1 gene.