Egg quality and lipid composition of eggs from hens fed Camelina sativa

The present study was conducted to investigate the effect of feeding Camelina sativa to layer birds on egg production, egg quality characteristics, egg lipids, and fatty acid and lipid oxidation products. Fifty-eight-week-old ISA Brown Leghorn laying hens (n = 48) were kept in individual cages and were fed a corn- and soybean meal-based diet with added Camelina meal at 0%, (control), 5%, (CAM5), 10% (CAM10), and 15% (CAM15). The experimental diets were fed for a period of 80 d. Hen-day egg production was lowest for CAM15 (P < 0.05). A significant reduction in yolk weight was observed for CAM10 and CAM15 eggs when compared with control eggs (P < 0.05). Yolk weight, as a percentage of egg weight, was lower for CAM10 and CAM15 eggs, whereas albumen weight, as a percentage of egg weight, was higher in CAM10 and CAM15 eggs than in control eggs (P < 0.05). The yolk:albumen ratio was higher in control eggs than in CAM10 and CAM15 eggs (P < 0.05). Egg total fat content was lowest for CAM15 eggs and was 31.5, 31.9, 30.8, and 29.5 for control, CAM5, CAM10, and CAM15 eggs, respectively (P < 0.05). Total n-3 fatty acids constituted 0.32% in control eggs compared with 2.54, 2.69, and 2.99% in CAM5, CAM10, and CAM15 eggs (P < 0.05). An 8-fold increase in docosahexaenoic acid was observed in CAM15 eggs when compared with control eggs (P < 0.05). The n-6:n-3 ratio was 14.8, 5.6, 4.6, and 4.3 for control, CAM5, CAM10, and CAM15 eggs, respectively (P < 0.05). Total saturated fats were lowest for CAM5 and CAM10 eggs. Eggs from the CAM15 regimen had higher TBA-reactive substance values (P < 0.05) than those from the CAM5, CAM10, or control regimen. Camelina meal could be incorporated into poultry rations as a source of energy, protein, and essential n-3 and n-6 fatty acids. However, inclusion of more than 10% Camelina meal in the hen diet may affect egg lipid quality aspects. Therefore, measures for minimizing lipid peroxidation should be used to enhance egg quality and lipid stability.     

Effects of N-methyl-D, L-aspartate on secretion of growth hormone-releasing hormone from the boar hypothalamic-preoptic area and median eminence in vitro

N-methyl-D, L-aspartate (NMA) elicited secretion of growth hormone (GH)-releasing hormone from both the hypothalamic-preoptic area and the median eminence that were collected from boars. We suggest that the previously described increase in GH secretion that follows peripheral treatment of swine with NMA is attributable, at least in part, to NMA-stimulated secretion of GH-releasing hormone from the central nervous system.     

Identification of CD3+ T lymphocytes in the green turtle Chelonia mydas

To understand the role of the immune system with respect to disease in reptiles, there is the need to develop tools to assess the host's immune response. An important tool is the development of molecular markers to identify immune cells, and these are limited for reptiles. We developed a technique for the cryopreservation of peripheral blood mononuclear cells and showed that a commercially available anti-CD3 epsilon chain antibody detects a subpopulation of CD3 positive peripheral blood lymphocytes in the marine turtle Chelonia mydas. In the thymus and in skin inoculated with phytohemagglutinin, the same antibody showed the classical staining pattern observed in mammals and birds. For Western blot, the anti-CD3 antibodies identified a 17.6 kDa band in membrane proteins of peripheral blood mononuclear cell compatible in weight to previously described CD3 molecules. This is the first demostration of CD3+ cells in reptiles using specific antibodies.     

Antigenic Detection of Human Strain of Influenza Virus A (H3N2) in Swine Populations at Three Locations in Nigeria and Ghana during the Dry Early Months of 2014

Since the first detection of human H3N2 influenza virus in Taiwanese pigs in 1970, infection of pigs with wholly human viruses has been known to occur in other parts of the world. These viruses, referred to as human‐like H3N2 viruses, have been known to cause clinical and subclinical infections of swine populations. Due to the paucity and complete unavailability of information on transmission of influenza viruses from other species, especially humans, to swine in Nigeria and Ghana, respectively, this study was designed to investigate the presence and prevalence of a human strain of influenza A (H3N2) in swine populations at three locations in two cities within these two West African countries in January and February, 2014. Using stratified random technique, nasal swab specimens were collected from seventy‐five (75) pigs at two locations in Ibadan, Nigeria and from fifty (50) pigs in Kumasi, Ghana. These specimens were tested directly by a sensitive Quantitative Solid Phase Antigen‐detection Sandwich ELISA using anti‐A/Brisbane/10/2007 haemagglutinin monoclonal antibody. Influenza virus A/Brisbane/10/2007 (H3N2) was detected among pigs at the three study locations, with an aggregate prevalence of 4.0% for the two locations in Ibadan, Nigeria and also 4.0% for Kumasi, Ghana. Transmission of influenza viruses from other species to swine portends serious sinister prospects for genetic reassortment and evolvement of novel viruses. We therefore recommend that further studies should be carried out to investigate the presence of other circulating human and avian influenza viruses in swine populations in West Africa and also determine the extent of genetic reassortment of strains circulating among these pigs. This would provide an early warning system for detection of novel influenza viruses, which could have pandemic potentials.     

猪圆环病毒2型CC株ORF3基因序列分析及真核表达

根据GenBank中猪圆环病毒2型(PCV2)的核酸序列,设计了1对引物,采用PCR方法从疑似断奶仔猪多系统衰竭综合征(PMWS)的死亡仔猪病料中扩增出了ORF3基因,将其克隆到高效真核表达载体pEGFP- N2中,筛选出含有ORF3基因的重组质粒,命名为pEGFP-N2-ORF3.对此重组质粒进行测序分析,结果表明,克隆的ORF3基因与其他PCV2的ORF3核苷酸序列相似性为96.2％-99.0％,氨基酸序列同源性为90.5 ％～98.1％.将重组质粒纯化后转染COS-7细胞,用PCR方法扩增出了特征性的基因片段,并采用特异性单抗进行间接免疫荧光,结果转染pEGFP- N2-ORF3重组蛋白在细胞核和细胞浆中均有表达,尤其在细胞核中表达量较高,且对细胞有一定的毒性.本研究为进一步探讨ORF3的结构和功能提供理论依据.     

In vitro effect of recombinant human tumor necrosis factor-alpha on canine neutrophil apoptosis

Neutrophils (polymorphonuclear leukocytes: PMNs) are essential for the host defense against various infections and are often injurious to the host, causing inflammatory diseases where tumor necrosis factor-alpha (TNF-alpha) is suggested to play an important role. Since an effect of TNF-alpha on canine PMN apoptosis has not been studied, canine PMNs were stimulated with recombinant human (rh)TNF-alpha in the present study to investigate the effect of TNF-alpha on canine PMN apoptosis. PMN apoptosis and function to produce ROS were assessed by flow cytometry. Delayed apoptosis was observed in the PMNs treated with rhTNF-alpha at 100 ng/ml, accompanied by retention of capability to produce ROS. However, PMN apoptosis was accelerated by rhTNF-alpha combined with cycloheximide. Therefore, it is indicated that TNF-alpha is able to activate anti- and pro-apoptotic pathways in PMNs and that the inhibition of PMN apoptosis by TNF-alpha requires protein synthesis in the PMNs.     

Cyclopedic protein expression analysis of cultured canine mammary gland adenocarcinoma cells from six tumours

We characterised cultured canine mammary gland adenocarcinoma cells by exhaustive step protein expression analysis to identify factors associated with tumour progression or metastasis of canine mammary gland tumour. Cultured adenocarcinoma cells derived from a total of 3 primary and 3 metastatic lesions from 3 dogs (CHMp/m, CIPp/m and CNMp/m, where CHM, CIP, and CNM indicate the 3 animals) were used in this study. The expression of 24 proteins reported to be related to tumourigenesis or malignancy of human breast cancers were examined by Western blot analysis using 24 antibodies. The expression of sialyl Lewis X [sLe(x)] was only observed in CHMm cells, which were derived from pleural effusion. This expression was further confirmed by immunohistochemistry. The levels of some factors, such as 14-3-3sigma, cyclinD1 and Rb, differed among cells or between the primary and metastatic cells in the pair. Though the difference in their expression was not consistent within the cells from primary and metastatic origin, this characterisation should provide useful information for further molecular analysis of these cultured cells. Since some of the factors, such as sLe(x), 14-3-3sigma, cyclinD1 and Rb, showed different levels of expression in the pair, these cultured cells might be meaningful tools for clarification of distant metastasis in canine mammary gland tumours.     

Exogenous testosterone modulates tumor necrosis factor-alpha and acute phase protein responses to repeated endotoxin challenge in steers

Clinical responses to some disease agents differ between sexes and this dimorphism has been attributed to the immunomodulating effects of steroid hormones. Our objective was to determine in steers the effect of testosterone on circulating concentrations of immune response mediators (tumor necrosis factor-alpha, TNF-alpha; serum amyloid-A, SAA; haptoglobin, HG; xanthine oxidase, XO; nitric oxide, NO) after two consecutive endotoxin challenges (LPS1 and LPS2, 5 days apart; 0.25 microg/kg BW). Sixteen crossbred steers (328+/-6 kg) were assigned to control (CON, n=8) or testosterone cypionate treatment (TES, n=8; 100 mg/m2 body surface; i.m. injection 12 and 2 days before LPS1). The response to LPS was calculated as area under the timexconcentration curve (AUC) for the parameter measured. After LPS1, TNF-alpha AUC was greater in TES than CON (P<0.05). Plasma HG and SAA concentrations increased (P<0.01) after LPS1 and LPS2. In all steers SAA AUC was greater after LPS1 than LPS2 (P<0.01) but the response was augmented over CON with testosterone treatment (P<0.05). HG response to LPS1 within 24 h was not affected by testosterone. However, 5 days after LPS1 mean plasma HG concentration remained higher in TES than CON (P<0.01). HG response to LPS2 was greater in TES than CON (P<0.01). Plasma nitrate+nitrite concentration (NO production marker) and XO activity increased after each LPS challenge but responses were not affected by testosterone treatment. Results indicate that the presence of circulating testosterone increases the magnitude of the TNF-alpha response to LPS challenge as well as the subsequent increases in acute phase proteins (APP). Effects of testosterone on increases in TNF-alpha and APP may underlie a differential presentation of disease symptoms between sexes or between steers and bulls. The data also suggest a role for testosterone in the development of tolerance to repeated immune challenge through its effect on the increased magnitude and duration of HG response.     

张掖黑河灌区苜蓿高效灌溉模式研究

通过对黑河流域大满灌区灌溉试验,测定了不同生育年龄甘农3号苜蓿Medecago sativacv.GannongNo.3地上生物量,经统计分析建立了苜蓿地上生物量年际动态和不同生育年内各茬间动态变化规律,结果表明,不同年际间各茬产量在不同水分处理下水分利用效率存在明显差异。不同水分处理下产量的变化呈高-低-高的“S”型变化,确定了苜蓿地的高效灌溉时期为现蕾-开花期,优化灌溉定额为520 mm,为苜蓿高产节水灌溉模式提供了理论依据。     

弓形虫微线体蛋白MIC3基因的克隆及原核表达

根据编码MIC3的已知基因序列设计并合成一对引物,应用PCR技术从弓形虫RH株的基因组DNA中扩增编码MIC3的全长基因,克隆入pGEX-KG表达载体,转化入E.coli DH5α感受态细胞,经含氨苄青霉素琼脂平板筛选,小量抽提质粒进行酶切、PCR及DNA测序鉴定.然后阳性重组质粒转化入E.coli BL21-CodonPlus,IPTG诱导,表达产物经SDS-PAGE和Western-blot分析鉴定.结果显示,扩增的MIC3基因与GenBank中相应基因序列（AJ132530）的同源性达99.6 %,表达的MIC3融合蛋白表观分子量约为66 ku,且可被兔抗弓形虫免疫血清识别.说明所获得的表达蛋白质具有一定的反应原性,为下一步利用重组蛋白建立弓形虫的诊断方法和研制弓形虫的亚单位疫苗奠定了基础.