O型口蹄疫病毒VP1蛋白单克隆抗体的制备与生物学特性鉴定

目的为了获得针对O型口蹄疫病毒的单克隆抗体,本研究采用差速离心、半饱和硫酸铵沉淀和蔗糖密度梯度离心法提纯O型口蹄疫病毒液,免疫BALB/c小鼠,取脾细胞和SP2/0细胞融合,经ELISA方法筛选和3次亚克隆后获得2株稳定分泌表达的杂交瘤细胞株2C8和5G10,腹水抗体效价分别达到1∶6 400和1∶25 600。经亚类鉴定确定两株单抗均为IgM型,Western-blot、间接ELISA和IFA确定这2株单克隆抗体分别针对O型口蹄疫病毒VP1蛋白不同表位,从而,为研究FMDV的生物学特性和建立快速诊断方法的建立奠定了基础。

Establishment of Monoclonal Antibody Competitive ELISA Using Monoclonal Antibody Against VP1 Protein of Asia 1 Type Foot-and-Mouth Disease Virus

Using the purified VP1 protein of Asia 1 type foot-and-mouth disease virus as the antigen, the purified monoclonal antibody was labeled by the sodium periodate method and the monoclonal antibody competitive ELISA was established in this study. Ten positive porcine foot-and-mouth disease serums and more than two hundreds negative serum were tested, and the results were the same as the background of samples. The sensitivity test and replicate test indicated that this method was stable and sensitive, which was suitable for monitoring Asia 1 type porcine foot-and-mouth disease virus antibody.

B Cell Epitopes within VP1 of Type O Foot-and-mouth Disease Virus for Detection of Viral Antibodies

In this study, the coding region of type O FMDV capsid protein VP1 and a series of codon optimized DNA sequences coding for VP1 amino acid residues 141-160 （epitopel）, tandem repeat 200-213 （epitope2 （＋2）） and the combination of two epitopes （epitopel-2） was genetically cloned into the prokaryotic expression vector PPRoExHTb and pGEX4T-1, respectively. VP1 and the fused epitopes GST-E1, GST-E2 （＋2） and GST-E1-2 were successfully solubly expressed in the cytoplasm of Escherichia coli and Western blot analysis demonstrated they retained antigenicity. Indirect VP1-ELISA and epitope ELISAs were subsequently developed to screen a panel of 80 field pig sera using LPB-ELISA as a standard test. For VP1-ELISA and all the epitope ELISAs, there were clear distinctions between the FMDV-positive and the FMDV-negative samples. Cross-reactions with pig sera positive to the viruses of swine vesicular disease virus that produce clinically indistinguishable syndromes in pigs or guinea pig antisera to FMDV strains of type A, C and Asia1 did not occur. The relative sensitivity and specificity for the GST-E1 ELISA, GST-E2 （＋2）, GST-E1-2 ELISA and VP1-ELISA in comparison with LPB-ELISA were 93.3% and 85.0%, 95.0% and 90%, 100% and 81.8%, 96.6% and 80.9% respectively. This study shows the potential use of the aforementioned epitopes as alternatives to the complex antigens used in current detection for antibody to FMDV structural proteins.

张家口市猪口蹄疫免疫抗体水平监测与分析

为了解张家口市猪O型口蹄疫免疫效果,控制猪口蹄疫的发生和流行,提高猪产品质量安全。采用猪O型口蹄疫VP1-ELISA和3ABC-ELISA两种方法,监测张家口市各区县规模化养殖场及不同类群猪自然感染和免疫抗体水平。结果表明:张家口市各区县规模化养殖场猪O型口蹄疫VP1结构蛋白抗体水平,万全县猪场2和宣化县猪场2合格率最高为100%,而蔚县猪场1合格率最低为77%;不同类群猪O型口蹄疫VP1结构蛋白抗体水平,以妊娠母猪和哺乳母猪免疫效果最好,合格率均高达100%,而种公猪免疫合格率最低,仅为75%。不同养殖场和不同类群猪的O型口蹄疫3ABC抗体阴性率均为100%,说明张家口市猪群未发生自然感染O型口蹄疫情况。总之,猪口蹄疫O型合成肽疫苗免疫效果良好,抗体检测结果均达到国家规定的合格率要求。

不同方法检测猪O型口蹄疫疫苗抗体效价与攻毒保护相关性研究

为评价不同检测方法检测的口蹄疫疫苗抗体效价与免疫保护率的相关性,使用O型液相阻断ELISA、正向间接血凝试验、VP1结构蛋白抗体ELISA三种检测方法对免疫不同类型O型口蹄疫疫苗的60头猪进行血清抗体跟踪测定,免疫21 d后,分别用OZK/93和O/(XJ/10-11/MYA/98)毒株进行攻毒保护实验。数据统计和分析结果显示,O型液相阻断ELISA试验测定的抗体效价与攻毒保护率存在着极显著的正相关性(P<0.01),相关系数为0.75;正向间接血凝试验测定的抗体效价以及VP1结构蛋白抗体ELISA法测定的S/P值与攻毒保护率之间均不存在线性相关关系(P>0.05)。试验表明,O型液相阻断ELISA抗体检测方法可作为田间猪O型口蹄疫疫苗免疫效果的评价方法。

安顺市平坝区2020年春季散养户猪O型口蹄疫免疫抗体监测分析

为评估平坝区生猪散养户使用0型口蹄疫合成肽疫苗的免疫效果,采用间接酶联免疫吸附试验对全区9个乡镇送检的164份猪血清样品进行猪O型口蹄疫VP1结构蛋白抗体检测。结果:检测免疫抗体合格数154份,不合格数10份,合格率为93.9%,免疫抗体合格率达到农业农村部规定≥70%的要求。结论:O型口蹄疫合成肽疫苗能够诱导生猪产生高水平的免疫抗体,具有良好的免疫保护效果。

抗Ⅰ型鸭肝炎病毒VP1蛋白单克隆抗体表位的鉴定

为了筛选Ⅰ型鸭肝炎病毒(Duck viral hepatitis typeⅠ,DVH-Ⅰ)VP1蛋白的抗原表位,试验应用噬菌体展示随机12肽库试剂盒,以抗DHV-ⅠVP1蛋白单克隆抗体纯化IgG作为靶标,通过ELISA和竞争抑制ELISA鉴定筛选克隆的结合特性,并对阳性克隆提取DNA进行测序分析。结果表明:通过3轮生物淘洗后,目标噬菌体得到282倍富集;随机挑选15个克隆进行测序分析及ELISA和竞争抑制ELISA检测,其中有8个噬菌体克隆可以与抗DVH-ⅠVP1蛋白单克隆抗体高度特异性结合,8个克隆的共有氨基酸序列为GMMIP。说明共有序列GMMIP可能是单克隆抗体2D5所识别的VP1蛋白的线性表位。

ECMS对O-Asia Ⅰ型FMD疫苗免疫功能增强的初探

目的证实ECMS增强O-Asia I型FMDV疫苗免疫功能的有效性,选择ECMS使用的有效浓度及诱导抗体的维持时间。方法本文用ELISA法测定了免疫后3、6、14周O型FMDV VP1及AsiaI型FMDV抗体的滴度。结果与结论与疫苗组和阳性组对照,100μgECMS诱导O-Asia I型FMDV疫苗产生两种抗体的效价较高,维持时间较长。相对来讲,ECMS诱导O型FMDV疫苗的抗体含量较高,但下降较快;诱导Asia I型FMDV疫苗的抗体较低,但下降非常缓慢。100μgECMS的效果优于公认的皂树皂甙(QA)佐剂。

不同口蹄疫疫苗免疫效果及检测方法评估

为更好地了解猪口蹄疫O型合成肽疫苗与猪口蹄疫O型灭活疫苗的免疫效果与合理的检测方法,广西农垦永新畜牧集团有限公司良圻原种猪场在某肥育场进行了此次试验。试验猪分3组,分别注射不同厂家生产的猪口蹄疫O型合成肽疫苗和猪口蹄疫O型OS/99株灭活疫苗,并采用猪O型口蹄疫VP1抗体检测试剂盒和正向间接血凝试验(HI)分别对使用上述口蹄疫疫苗免疫效果进行检测。结果表明,猪注射口蹄疫O型合成肽疫苗后,用猪O型口蹄疫VP1抗体检测试剂盒检测,抗体阳性率达到100%;用正向间接血凝试验方法检测不到注射合成肽疫苗后产生的抗体效价。免疫猪口蹄疫O型OS/99株灭活疫苗后,用VP1抗体检测试剂盒检测,抗体阳性率只有30%;用HI方法进行检测,抗体阳性率为60%。