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采用黄芪多糖、葡聚糖作为免疫佐剂,与迟缓爱德华氏菌灭活疫苗配伍后注射免疫大菱鲆,测定免疫28d后血清中溶菌酶活力、SOD活力、抗体效价和各免疫组的相对保护率(RPS)。结果表明,添加多糖免疫佐剂能提高疫苗免疫的大菱鲆的各免疫指标,添加佐剂的免疫组的血清溶菌酶活力、SOD活力和血清效价比单纯的疫苗免疫组显著提高(P<0.05),2.5mg/ml黄芪多糖混合疫苗免疫组和5mg/ml葡聚糖混合疫苗免疫组的相对保护率最高,分别达(78.7±1.3)%和(64.0±8.9)%,且溶菌酶活力、SOD活力及血清效价等指标较其他各组有提高。 相似文献
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Edwardsiella tarda has become one of the most important emerging pathogens in aquaculture industry.Therefore,a rapid,reproducible,and sensitive method for detection and quantification of this pathogen is needed urgently.To achieve this purpose,we developed a TaqMan-based real-time PCR assay for detection and quantification of E.tarda.The assay targets the hemolysin activator HlyB domain protein of E.tarda.Our optimized TaqMan assay is capable of detecting as little as 40 fg of genomic DNA per reaction.A standard curve was generated from the threshold cycle values(y) against log10(E.tarda genomic DNA concentration) as x.The intra-and inter-assay coefficient of variation(CV) values were less than 2.06% and 1.05% respectively,indicating that the assay had good reproducibility.This method is highly specific to E.tarda strains,as it shows no cross-reactivity to Edwardsiella ictaluri,a member of the same genus,or to nine other fish-pathogenic bacteria species belonging to three other genera.This sensitive and specific real-time PCR assay provides a valuable tool for diagnostic quantitation of E.tarda in clinical samples. 相似文献
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3种水产病原菌简型基因芯片检测技术的建立 总被引:1,自引:0,他引:1
根据水产养殖中常见的3种病原菌鳗弧菌(Vibrio anguillarum)、嗜水气单胞菌(Aeromonas hydrophila)及迟缓爱德华氏菌(Edwardsiella tarda)的研究资料,筛选3个毒力相关基因toxR、aerA、evpA设计引物和探针,构建简型基因芯片,并使用对虾白斑病综合征病毒(WSSV)variable region的PCR荧光标记产物作为表面化学质控。通过已构建和优化的多重PCR反应条件,获得了3个目的基因的PCR产物;经过芯片制作过程的优化,将探针以终浓度20μmol/L溶于50%DMSO,在室温、相对湿度45%的条件下点印于醛基基片表面。扩增的PCR产物与杂交液混合后,在42℃杂交2 h就可检测到理想的杂交信号。芯片的灵敏度试验结果表明,可以检测到的3种水产病原菌的最低模板DNA为:鳗弧菌3×102拷贝、嗜水气单胞菌5×103拷贝、迟缓爱德华氏菌6×101拷贝。该芯片可成功应用于患病大菱鲆内脏的细菌分离物的鉴定。 相似文献
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Edwardsiella tarda is a major pathogen in aquatic environments that can cause heavy economic losses. An improved method for quick and accurate detection of E. tarda by loop-mediated isothermal amplification (LAMP) with two additional loop primers was developed by targeting the EsrB gene (EsrB-LAMP). In this method, the Mg 2+ concentration, reaction temperature, and reaction time were optimized to 8 mmol/L, 61°C, and 40 min, respectively. The detection limit with the EsrB gene was as low as 10 copies, which is 100 times more sensitive than that of conventional polymerase chain reaction (PCR). The EsrB-LAMP assay was shown more sensitive and rapid than previously reported LAMP assays targeting the hemolysin gene (hemolysin-LAMP) for detection of E. tarda. The EsrB-LAMP was also highly specific to E. tarda and had no cross-reaction with 13 other strains of bacteria. The assay can be carried out in a simple heating device and the EsrB-LAMP products can be visually detected by adding fluorescent dye to the reaction mixture. Taken together, the improved EsrB-LAMP diagnostic protocol has the potential for detection of E. tarda from indoor and outdoor samples. 相似文献
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