鲫和鳝红细胞C3b受体的研究

本文应用免疫花环试验对鲫和鳝红细胞进行了检测。结果表明，鲫红细胞可形成Ｃ_３ｂ受体花环，花环率为７．９５±２．３３和免疫复合物花环，花环率为３．０５±１．１２。而鳝红细胞主要形成Ｃ_ｂ受体花环，花环率为３．９０±１．４２，免疫复合物花环率仅为０．２０±０．４２。正常鲫和鳝红细胞Ｃ_３ｂ受体花环率均高于红细胞免疫复合物花环率，差异极显著。这证实了鲫和鳝红细胞表面均存在Ｃ_３ｂ受体，从而表明二者的红细胞也具有重要的免疫功能。     

沙拉沙星间接竞争化学发光酶联免疫检测方法的建立

为建立动物源性食品中沙拉沙星（SAR）残留的快速检测方法,本试验通过对盐酸沙拉沙星进行分子改造和偶联蛋白合成完全免疫原,免疫小鼠制备SAR单克隆抗体。通过棋盘法确定最佳包被原浓度及一抗稀释度,优化确定最佳反应条件,从而建立间接竞争化学发光酶联免疫（ic-CLEIA）检测方法,并通过灵敏度、精密度、交叉反应率、添加回收试验对该方法进行评价。紫外扫描结果显示,完全免疫原偶联成功;制备的SAR单克隆抗体效价达1：4×10⁶;包被原浓度为0.25 μg/mL,抗体稀释比为1：750 000,4 ℃包被过夜,5%脱脂乳封闭,竞争孵育1 h,酶标二抗稀释比为1：10 000,孵育1 h为ic-CLEIA最佳反应条件;建立的ic-CLEIA方法标准曲线呈线性,线性范围为0.0625~10 ng/mL,R²=0.995,灵敏度IC₅₀为1.45 ng/mL;其平均批内和批间变异系数均<10%;除与二氟沙星的交叉反应率达到98.08%以外,与其他氟喹诺酮类药物的交叉反应率均<8%,与其他非氟喹诺酮类药物均无交叉反应;SAR标准溶液的最低检测限（LOD）为0.32 ng/mL,SAR在鸡肉样品中的LOD为0.46 μg/kg;添加回收率在88.3%~106.7%范围内,其变异系数≤12.2%。结果表明,本研究建立的ic-CLEIA方法检测速度快、灵敏度高,适用于动物源性食品中SAR残留的大量检测,为SAR残留检测提供了新的方法。     

Estimation of deoxynivalenol (DON) content by symptom rating and exoantigen content for resistance selection in wheat and triticale

Fusarium head blight (FHB) in wheat and triticale leads to contamination of the grain with the mycotoxin deoxynivalenol (DON) that is harmful to animal and man. A fast, low-cost, and reliable method for quantification of the DON content in the grain is essential for selection. We analysed 113 wheat and 55 triticale genotypes for their symptom development on spikes, Fusarium exoantigen (ExAg) and DON content in the grain after artificial inoculation with a highly aggressive isolate of F. culmorum in three (wheat) and six (triticale) location-by-year combinations. Additionally, in triticale the amount of Fusarium damaged kernels (FDK) was assessed. ExAg content was analysed by a newly developed Fusarium-specific plate-trapped antigen enzyme-linked immunosorbent assay (PTA-ELISA) and DON content by an immunoassay. A moderate disease severity resulted in an ExAg content of 0.87 optical density (OD) units in wheat and 1.02 OD in triticale. DON content ranged from 12.0 to 105.2 mg kg^–1 in wheat and from 24.2 to 74.0 mg kg^–1 in triticale. Genotypic and genotype-by-environment interaction variances were significant (P < 0.01). Coefficient of phenotypic correlation between DON content analysed by the immunoassay and ExAg content was r = 0.86 for wheat and r = 0.60 for triticale. The highest correlation between DON content and symptom rating was found by FHB rating in wheat (r = 0.77) and by FDK rating in triticale (r = 0.71). In conclusion, selection for reduced FHB symptoms should lead to a correlated selection response in low fungal biomass and low DON content in the grain.     

Predation on walleye pollock (Theragra chakograrnma) eggs and yolk-sac larvae by pelagic crustacean invertebrates in the western Gulf of Alaska

Immunological detection of yolk protein was used to assess predation by pelagic amphipods (gammarid and hyperiid), mysids, and euphausiids on eggs and yolk-sac larvae of walleye pollock Theragra chalcogramma during 1988 and 1989. Consumption estimates were made on the basis of frequency of positive immunoassays, assay detection times (gut clearance time), predator abundance, and spatial overlap of predators and prey. From our results gammarid amphipods and euphausiids were important predators on eggs and yolk-sac larvae, respectively. Gammarid amphipods alone consumed about 14% of the standing stock of pollock eggs in 1989. These results were compared with those from clearance rate experiments of predators feeding on pollock eggs in 300-1 bags. In general, clearance rate estimates of egg consumption were lower than those determined from gut contents.     

2019—2021年伊吾县牛羊口蹄疫免疫抗体监测与分析

为掌握伊吾县牛羊口蹄疫免疫抗体水平,采用液相阻断ELISA抗体检测(LPB-ELISA)方法,收集6个乡镇2019—2021年抽检春秋两季牛1258头、羊2496只,进行时间、地域分布描述。实验显示,口蹄疫A型总体合格率90.86%、90.91%,O型口蹄疫免疫抗体总体合格率94.12%、94.03%,免疫抗体效价大于70%。不同区域前山乡口蹄疫整体免疫水平最高,吐葫芦乡牛A型口蹄疫免疫抗体较低仅为74.67%。结果表明,全县牛羊口蹄疫免疫抗体检测效果整体良好,部分乡镇免疫较低。需做好基层牛羊口蹄疫免疫调研,查找原因,提出了今后的工作方向,加强对防疫员开展从疫苗保存、免疫部位选择、免疫剂量技术指导,特别是动物检疫站监管,为伊吾县畜牧业高质量健康发展提供依据。     

二级竞争酶联免疫孕酮临界点判别分析在乳牛早期妊娠诊断上的应用

本文根据二级竞争酶联免疫定量测定的原理建立了用于乳牛早期妊娠诊断的二级竞争酶联免疫孕酮临界点判别分析法．本方法无需仪器比色和数学计算，反应结果清晰可辨、操作简便．根据对５２０头次配种后２１ｄ乳牛进行测试，其总正确率为８３．８％，其中阴性正确率为９０％，阳性正确率为７９％。     

Development and validation of a sensitive enzyme immunoassay (EIA) for blood plasma cortisol in female cattle,buffaloes, and goats

A highly sensitive enzyme immunoassay (EIA) that used the second antibody coating technique and the cortisol-horseradish peroxidase conjugate as a label for determination of free and total cortisol in blood plasma of dairy animals (cows, buffaloes, and goats) was developed. For biological validation of the EIA, blood samples were collected from the animals at 48 and 24 h before and 0, 12, 24, 36, 48, 60, 72, 84, 96, 108, 120, and 132 h after dexamethasone administration. The EIA was performed directly with 20 μL of fresh plasma (for free cortisol) and also with 20 μL of heat-treated plasma (for total cortisol) after 1:5 dilutions with PBS. Cortisol standards ranging from 0.39 to 200 pg/well/20 μL were used, and the sensitivity of the EIA procedure was found to be 0.39 pg/well/20 μL, which corresponded to 0.02 ng/mL. In comparison with RIA the EIA was at least 4 times more sensitive and required 5 times less cortisol antiserum. In female cattle, buffaloes, and goats, the total, free, and bound plasma cortisol before dexamethasone administration was significantly (P < 0.05) higher than the total, free, and bound cortisol after dexamethasone administration. It can be concluded from these studies that the direct, sensitive EIA validated for estimating the free and total cortisol concentrations was sufficiently reliable and quick for studying the dynamics of cortisol distribution in blood plasma of dairy animals.     

Evaluation of the PATHFAST Chemiluminescent Enzyme Immunoassay for Measuring Progesterone in Whole Blood and Serum of Mares

Evaluation of a new chemiluminescent enzyme immunoassay, the PATHFAST assay system (PATHFAST), for measurement of circulating progesterone in mares was performed. Five mares at the mid-luteal stage were administrated a single i.m. injection of prostaglandin F2α analog (PGF2α; cloprostenol 250 μg/ml), and then blood samples were collected from the jugular vein at 0, 15, 30 and 45 min, at one-hour intervals until 24 and at 48 hr via a catheter in the jugular vein. To monitor the physiological changes in circulating progesterone in mares after induced luteolysis, concentrations of progesterone in whole blood and serum samples were measured by PATHFAST. In addition, concentrations of progesterone in serum samples measured by PATHFAST were compared with those measured by radioimmunoassay (RIA) and enzyme immunoassay (EIA). Using PATHFAST, the serum concentrations of progesterone in mares correlated highly with those of whole blood samples (r=0.9672, n=88). The serum concentrations of progesterone as measured by PATHFAST correlated well with RIA (r=0.9654, n=88) and EIA (r=0.9323, n=112). An abrupt decline in circulating progesterone in whole blood samples was observed within 2 hr (50%), followed by a gradual decline until 48 hr later. The results for progesterone in whole blood samples correlated highly with those in serum samples, and the declining pattern paralleled that of the serum samples. These results demonstrated that PATHFAST is useful in the equine clinic as an accurate diagnostic tool for rapid assay of progesterone within 26 min, using unextracted whole blood.