中华微生物学和免疫学杂志
中華微生物學和免疫學雜誌
중화미생물학화면역학잡지
CHINESE JOURNAL OF MICROBIOLOGY AND IMMUNOLOGY
2012年
5期
399-402
,共4页
范秀华%刘海楠%郑艳%张玲%姚智燕%李文建%邢艳超%宋小天%马翠卿
範秀華%劉海楠%鄭豔%張玲%姚智燕%李文建%邢豔超%宋小天%馬翠卿
범수화%류해남%정염%장령%요지연%리문건%형염초%송소천%마취경
A族链球菌%Fba蛋白%单克隆抗体%补体调节蛋白%H因子
A族鏈毬菌%Fba蛋白%單剋隆抗體%補體調節蛋白%H因子
A족련구균%Fba단백%단극륭항체%보체조절단백%H인자
Group A Streptococcus%Fba protein%Monoclonal antibody%Complement regulatory proteins%Factor H
目的 通过侵袭抑制及攻毒试验检测A族链球菌表面蛋白FbaA的单克隆抗体FbaAmAb2的免疫功能,为进一步探索A族链球菌的致病机制和感染后的治疗策略奠定基础.方法 通过亚克隆、全菌ELISA方法筛选稳定分泌高效价FbaAmAb2的杂交瘤细胞,并将其接种子小鼠腹腔制备腹水.通过侵袭试验对FbaAmAb2能否阻止H因子与A族链球菌的结合进行研究.而后将获得的腹水倍比稀释为1:1、1:2、1:4、1:8、1:16行试管凝集试验,选定合适的稀释度被动免疫动物后用致死量A族链球菌(FbaA+)标准菌株(7.5×107个)攻击,连续观察15 d计算保护率.结果 侵袭试验中FbaAmAb2能够竞争性抑制H因子与A族链球菌表面蛋白FbaA的结合,减少了H因子介导的A族链球菌侵入上皮细胞的数量.与全菌结合的ELISA效价为1:1600,试管凝集效价为1:8.在单抗被动免疫试验中,腹水原液、1:2稀释组的动物保护率高达66.67%,1:4稀释组保护率为50%,经SPSS10.0统计软件分析各实验组与PBS组保护牢差异有统计学意义(P<0.05).结论 FbaAmAb2有望用于紧急预防及治疗A族链球菌感染,并为深入研究A族链球菌的致病机制、治疗策略及疫苗预防方面提供新的靶标.
目的 通過侵襲抑製及攻毒試驗檢測A族鏈毬菌錶麵蛋白FbaA的單剋隆抗體FbaAmAb2的免疫功能,為進一步探索A族鏈毬菌的緻病機製和感染後的治療策略奠定基礎.方法 通過亞剋隆、全菌ELISA方法篩選穩定分泌高效價FbaAmAb2的雜交瘤細胞,併將其接種子小鼠腹腔製備腹水.通過侵襲試驗對FbaAmAb2能否阻止H因子與A族鏈毬菌的結閤進行研究.而後將穫得的腹水倍比稀釋為1:1、1:2、1:4、1:8、1:16行試管凝集試驗,選定閤適的稀釋度被動免疫動物後用緻死量A族鏈毬菌(FbaA+)標準菌株(7.5×107箇)攻擊,連續觀察15 d計算保護率.結果 侵襲試驗中FbaAmAb2能夠競爭性抑製H因子與A族鏈毬菌錶麵蛋白FbaA的結閤,減少瞭H因子介導的A族鏈毬菌侵入上皮細胞的數量.與全菌結閤的ELISA效價為1:1600,試管凝集效價為1:8.在單抗被動免疫試驗中,腹水原液、1:2稀釋組的動物保護率高達66.67%,1:4稀釋組保護率為50%,經SPSS10.0統計軟件分析各實驗組與PBS組保護牢差異有統計學意義(P<0.05).結論 FbaAmAb2有望用于緊急預防及治療A族鏈毬菌感染,併為深入研究A族鏈毬菌的緻病機製、治療策略及疫苗預防方麵提供新的靶標.
목적 통과침습억제급공독시험검측A족련구균표면단백FbaA적단극륭항체FbaAmAb2적면역공능,위진일보탐색A족련구균적치병궤제화감염후적치료책략전정기출.방법 통과아극륭、전균ELISA방법사선은정분비고효개FbaAmAb2적잡교류세포,병장기접충자소서복강제비복수.통과침습시험대FbaAmAb2능부조지H인자여A족련구균적결합진행연구.이후장획득적복수배비희석위1:1、1:2、1:4、1:8、1:16행시관응집시험,선정합괄적희석도피동면역동물후용치사량A족련구균(FbaA+)표준균주(7.5×107개)공격,련속관찰15 d계산보호솔.결과 침습시험중FbaAmAb2능구경쟁성억제H인자여A족련구균표면단백FbaA적결합,감소료H인자개도적A족련구균침입상피세포적수량.여전균결합적ELISA효개위1:1600,시관응집효개위1:8.재단항피동면역시험중,복수원액、1:2희석조적동물보호솔고체66.67%,1:4희석조보호솔위50%,경SPSS10.0통계연건분석각실험조여PBS조보호뢰차이유통계학의의(P<0.05).결론 FbaAmAb2유망용우긴급예방급치료A족련구균감염,병위심입연구A족련구균적치병궤제、치료책략급역묘예방방면제공신적파표.
Objective To detect the immune effect of FbaAmAb2 against the surface protein of group A Straptococcus (GAS),and explore the pathogenesis and therapy of GAS infections.Methods By subclonal and bacterial ELISA,the positive hybridoma cells were screened that can produce better titers of FbaAmAb2 against GAS-surface FbaA protein,and were injected into the peritoneal cavities of BALB/c mice to produce ascites.The collected ascites were performed to dilute,as follows,original ascite,1:2,1:4,1:8,and 1:16 to test tube agglutination.Based on the results,we selected appropriate dilution to passively immunize mice,and then challenged the mice with GAS,evaluating FbaAmAb2 neutralizing ability with GAS in mice by the survival rate of the immunized mice.Whether FbaAmAb2 could inhibit the binding of factor H to GAS was confirmed by the invasive inhibition assay.Results The IgG titer of bacteria solution ELISA is 1:160 and the titer of tube agglutination is 1∶8.The protect rates of FbaAmAb2 on preventing mice with GAS infections are as follows:66.67% in original ascite and 1:2 diluted groups,and 50% in 1:4 diluted group.Mice in each experimental group were evoked significantly protective immune responses compared with the PBS control by SPSS analysis.FbaAmAb2 can competitively inhibit factor H binding to the surface proteins FbaA of GAS,which decreased the entry of GAS into the cytoplasm of human epithelial cells through the binding of factor H.Conclusion FbaAmAb2 is promising to be used in emergent prevention or the clinical therapy for GAS infection and it is promising starting points for pharmacologic targeting and further development of new therapeutic agents for GAS.
