堆型艾美耳球虫早熟株免疫雏鸡后血清抗体水平动态变化的研究

用堆型艾美耳球虫早熟株对雏鸡进行一次免疫和二次免疫试验 ,研究雏鸡血清抗体的动态变化。试验结果显示 ,在一次免疫试验中 ,各剂量组雏鸡均在免疫后 2天血清抗体出现较高的 OD值 ,之后呈下降趋势 ,11天后逐渐上升 ,到 12～ 13天时出现第 2个峰值 ,各组间的血清抗体 OD值比较 ,3 0 0 0个卵囊 /只剂量组极显著 (P<0 .0 1)高于 10 0 0个 /只、2 0 0 0个 /只和 5 0 0 0个 /只剂量组。在二次免疫试验中 ,8日龄首免、14日龄二免组雏鸡的抗体水平动态变化整体呈上升趋势 ,峰值 (0 .3 75 )出现在二免后第 10天 ,其后稳定地维持在较高水平 (平均 OD值为 0 .3 5 ) ,并且其抗体水平显著地高于 6日龄首免、12日龄二免组 (P<0 .0 5 )。抗体水平动态变化表明 ,堆型艾美耳球虫早熟株有较强的免疫保护力 ,其免疫方式可选用一次免疫 ,剂量为 3 0 0 0个卵囊 /只 ,也可采用二次免疫 ,即 8日龄首免 (15 0 0个 /只 ) ,14日龄二免 (15 0 0个 /只 ) ,从抗体动态变化的稳定性看 ,二次免疫更佳     

不同包被液对ELISA检测五号病病毒抗体的比较试验

０．０５ＭｐＨ９．６碳酸盐缓冲液和０．０５ＭＰＨ１３ＮａＯＨ溶液作为包被液，分别用于间接ＥＬＩＳＡ检测乙型五号病病毒抗体。结果表明，用０．０５ＭＰＨ１３ＮａＯＨ溶泡包被可完全灭活五号病病毒抗原而用０．０５ＭＰＨ９．６碳酸盐缓冲液却有８７％的五号病病毒抗原未被杀灭；用于检测时，以０．０５ＭＰＨ１３ＮａＯＨ溶液为包被液在敏感性及检测结果的梯度方面都优于用０．０５ＭＰＨ９．６碳酸盐缓冲液。     

H5亚型禽流感灭活疫苗免疫后鸡血凝抑制抗体动态变化观察

选择国家指定的两个厂家生产的禽流感灭活疫苗(H5亚型,N28株)进行无母源抗体来航鸡的免疫试验.通过鸡免疫后血凝抑制(HI)抗体的动态性检测,对两个疫苗的免疫效果进行了观察.研究结果表明,两个疫苗均具有良好的免疫效果,但也存在一定程度的差异;加强免疫可以明显提高抗体水平,延长免疫保护时间.     

破壁蜂花粉对蛋鸡免疫功能及肠道菌群的影响

试验将槐花蜂花粉进行振动磨超微粉碎破壁,分别按1 g/kg、5 g/kg、10 g/kg三个不同剂量混到蛋鸡饲料中,从7日龄开始饲喂至50日龄,每个剂量分两个试验,试验一用新城疫Ⅳ系疫苗免疫雏鸡,利用β-微量法监测血清中的血凝抑制抗体效价的动态变化;试验二用大肠杆菌油乳苗免疫雏鸡,利用间接血凝法监测血清中大肠杆菌抗体效价的动态变化。分别定期称重捕杀取脾、胸腺、法氏囊,计算免疫器官指数,取肠道内容物计数大肠杆菌和乳酸菌,测定肠道内pH值。结果表明,不同剂量的破壁蜂花粉均能不同程度地提高病毒抗原性抗体效价和菌体抗原性抗体效价,对雏鸡免疫器官的发育以及肠道内环境、菌群的平衡也有一定影响。     

Preparation and characterization of anti-hBLyS monoclonal antibody by DNA immunization

AIM:To establish the monoclonal antibody against human B lymphocyte stimulator (hBLyS) by DNA immunization and analyse its characterization. METHODS:The 858 bp DNA fragment of hBLyS was cloned into pcDNA3 plasmids. The cloned insert was identified by both sequence analysis and double digestion of the recombinant plasmid with restriction enzymesXho Iand EcoR I. After the splenocytes from BALB/c mice immunized with the recombinant plasmid of pcDNA3/hBLyS were fused with myeloma cells SP2/0,the hybridoma which can produce monoclonal antibodies against hBLyS were obtained. The specificity of anti-BLyS monoclonal antibody from hybridoma was verified by ELISA, Western blot and flow cytometry. RESULTS:The recombinant mammalian cell expression vector of pcDNA3/hBLyS was constructed,the sequence of the insert gene was identified to be the sequence encoding hBLy S antigen. The culture supernatants of hybridoma 9c10 were tested to be the monoclonal antibody with specificity against hBLyS on human peripheral blood CD3⁺T cell activated by hIFN-γ by ELISA,Western blot and flow cytometry.CONCLUSION:The monoclonal antibodies against hBLyS with high activity and specificity have been established successfully, and will be an useful tool in the studies of relationship between hBLyS and human autoimmunity diseases.     

Phylogeny of the frosty pod rot pathogen of cocoa

Morphological, cytological and molecular evidence is presented which confirms that the frosty pod rot pathogen of cocoa, formerly classified as the mitosporic fungus Moniliophthora roreri (Deuteromycota), belongs to the hymenomycetous genus Crinipellis (Basidiomycota) and that two varieties should now be recognized: Crinipellis roreri var. roreri and the new variety C. roreri var. gileri . The latter was collected on Theobroma gileri , an endemic tree of submontane forests in north-west Ecuador, and can be distinguished from Ecuadorian and Peruvian isolates from cocoa ( T. cacao ) on the basis of spore morphology, incompatibility and nucleotide sequence data. As with var. roreri , meiosis is shown to occur within the dispersive and infective spore stage of var. gileri and these meiospores are interpreted to represent a much modified probasidium. In addition, in a field inoculation experiment, an isolate from T. gileri proved to be noninfective to cocoa pods when compared with positive control strains isolated from T. cacao in western Ecuador and T. bicolor in eastern Ecuador. It is concluded that var. gileri is the vestigial progenitor of the frosty pod rot pathogen of cocoa, with a host range and distribution restricted to T. gileri in the mesic forests of north-west South America.     

Production and characterization of a monoclonal antibody specific to the M serotype of plum pox potyvirus

A monoclonal antibody to an Albanian isolate of plum pox potyvirus (PPV) was obtained (MAbAL), that specifically recognized strain M of this virus. The specificity of MAbAL, assessed by comparative ELISA on 130 PPV isolates of different geographical origin, 22 of which were also tested by comparative IC-PCR, gave consistent and highly reproducible results. MAbAL seems to be elicited by a stable surface determinant that makes it particularly suitable for successful use under a wide range of conditions. MAbAL is an useful addition to the panel of PPV-specific MAbs available to date.     

重组鸡IL-2增强鸡四联灭活苗免疫效果的研究

使用在原核表达系统中表达的重组鸡白细胞介素 2 (IL 2 )蛋白 ,经过初步的分离纯化 ,与鸡新城疫 禽流感 法氏囊 传染性支气管炎四联油乳剂灭活苗同时使用 ,检测其对疫苗的免疫增强效果。试验共分 5组 ,每组 1 0只鸡。其中对照组只注射四联油乳剂灭活苗 ;4个试验组 ,在注射疫苗的同时分别注射重组鸡IL 2蛋白 0 0 5mg、 0 0 1mg、 0 1 5mg、 0 2 0mg。试验组与对照组同时各注射新城疫等多联油苗 0 5mL。采用HA、HI试验测定鸡新城疫、禽流感抗体滴度。结果表明 :重组鸡IL 2对该四联油乳剂灭活苗有较强的免疫增强作用。以第 3、 4组的增强效果较为明显 ,其中对鸡新城疫病毒和禽流感抗原的抗体效价 ,与对照组相比分别提高 2 42 8和 2 2 3 0个滴度。重组鸡IL 2在使用的过程中 ,没有发现任何毒副作用 ,证明是一种安全高效的免疫增强剂。     

不同营养水平对种公鸡新城疫抗体水平的影响

研究选择21周龄新扬州鸡种公鸡135只,随机分成9组。采用两因子析因设计,分别设粗蛋白质水平为17%、14%和11%,钙水平为3.3%、2.3%和1.3%,构成9种日粮处理。比较在繁殖期全程饲喂不同粗蛋白质和钙水平日粮对种公鸡新城疫水平的影响,结果表明:日粮粗蛋白质水平对免疫后15、30天公鸡体内的抗体水平有显著影响(P<0.05),对免疫90天的水平有极显著影响(P<0.01);日粮钙对免疫后30天的抗体水平有极显著的影响(P<0.01);二者的交互作用对它影响不显著(P>0.05);低蛋白低钙组抗体水平显著高于高蛋白高钙组(P<0.05)。     

抗鸡传染性腺胃炎酶标抗体的制备和应用

在前期从患病鸡腺胃内分离到呼肠孤病毒的基础上，以该病毒为免疫原对兔进行免疫制备高免血清，分离纯化IgG，进行辣根过氧化物酶（HRP）标记，并用ELISA双抗体夹心法对山东省青岛、枣庄、泰安等地区采集的传染性腺胃炎的腺胃样品进行检测，结果表明制备的抗鸡传染性腺胃炎呼肠孤病毒的酶标抗体检测传染性腺胃炎特异性强、灵敏度高、较简便。