中国免疫学杂志
中國免疫學雜誌
중국면역학잡지
CHINESE JOURNAL OF IMMUNOLOGY
2015年
6期
790-794
,共5页
康月茜%张春燕%穆柳青%卢楠%杨春%李岱容
康月茜%張春燕%穆柳青%盧楠%楊春%李岱容
강월천%장춘연%목류청%로남%양춘%리대용
结核分枝杆菌%重组蛋白ClpP2%免疫原性
結覈分枝桿菌%重組蛋白ClpP2%免疫原性
결핵분지간균%중조단백ClpP2%면역원성
Mycobacterium tuberculosis%Recombinant ClpP2 protein%Immunogenicity
目的::对结核分枝杆菌Rv2460c基因(编码ClpP2蛋白)进行克隆,表达,并评价其编码产物的免疫原性。方法:扩增结核分枝杆菌(Mycobacterium tuberculosis,Mtb)H37Rv 的Rv2460c基因,构建重组质粒pET32a(+)-ClpP2,用IPTG诱导表达,利用亲和层析法进行纯化。用SDS-PAGE和Western blot分析重组蛋白ClpP2的表达和鉴定。用生物信息学对Mtb ClpP2的免疫原性分析和表位预测。酶联免疫吸附法( ELISA)测定兔和TB病人血清anti-ClpP2滴度。结果:重组ClpP2蛋白酶在大肠杆菌中以包涵体形式表达,经 bandscan 软件分析纯化蛋白的纯度为93%。生物信息学分析Mtb ClpP2蛋白具有多个优势B细胞表位和T细胞表位。 ELISA法测定兔抗血清效价为1∶64000;检测肺结核病人血清中anti-ClpP2抗体水平高于健康对照人群。结论:成功纯化了重组蛋白ClpP2和制备了特异性兔抗ClpP2多克隆抗体,实验和信息学均表明Mtb ClpP2蛋白酶有较强的免疫原性。
目的::對結覈分枝桿菌Rv2460c基因(編碼ClpP2蛋白)進行剋隆,錶達,併評價其編碼產物的免疫原性。方法:擴增結覈分枝桿菌(Mycobacterium tuberculosis,Mtb)H37Rv 的Rv2460c基因,構建重組質粒pET32a(+)-ClpP2,用IPTG誘導錶達,利用親和層析法進行純化。用SDS-PAGE和Western blot分析重組蛋白ClpP2的錶達和鑒定。用生物信息學對Mtb ClpP2的免疫原性分析和錶位預測。酶聯免疫吸附法( ELISA)測定兔和TB病人血清anti-ClpP2滴度。結果:重組ClpP2蛋白酶在大腸桿菌中以包涵體形式錶達,經 bandscan 軟件分析純化蛋白的純度為93%。生物信息學分析Mtb ClpP2蛋白具有多箇優勢B細胞錶位和T細胞錶位。 ELISA法測定兔抗血清效價為1∶64000;檢測肺結覈病人血清中anti-ClpP2抗體水平高于健康對照人群。結論:成功純化瞭重組蛋白ClpP2和製備瞭特異性兔抗ClpP2多剋隆抗體,實驗和信息學均錶明Mtb ClpP2蛋白酶有較彊的免疫原性。
목적::대결핵분지간균Rv2460c기인(편마ClpP2단백)진행극륭,표체,병평개기편마산물적면역원성。방법:확증결핵분지간균(Mycobacterium tuberculosis,Mtb)H37Rv 적Rv2460c기인,구건중조질립pET32a(+)-ClpP2,용IPTG유도표체,이용친화층석법진행순화。용SDS-PAGE화Western blot분석중조단백ClpP2적표체화감정。용생물신식학대Mtb ClpP2적면역원성분석화표위예측。매련면역흡부법( ELISA)측정토화TB병인혈청anti-ClpP2적도。결과:중조ClpP2단백매재대장간균중이포함체형식표체,경 bandscan 연건분석순화단백적순도위93%。생물신식학분석Mtb ClpP2단백구유다개우세B세포표위화T세포표위。 ELISA법측정토항혈청효개위1∶64000;검측폐결핵병인혈청중anti-ClpP2항체수평고우건강대조인군。결론:성공순화료중조단백ClpP2화제비료특이성토항ClpP2다극륭항체,실험화신식학균표명Mtb ClpP2단백매유교강적면역원성。
Objective:To clone and express Mycobacterium tuberculosis(Mtb) Rv2460c gene(encoding ClpP2 protein),and evaluate the immunogenicity of its coding product. Methods: The recombinant plasmid of pET32a (+) vector-ClpP2 that H37Rv Rv2460c gene was cloned into the plasmid pET32a(+)vector,was transformed into E. coli BL21(DE3)and induced expression by IPTG,then purified by affinity chromatography. The recombinant protein was confirmed by SDS-PAGE and Western blot. The analysis of immunogenicity of Mtb ClpP2 and its epitope prediction were performed by bioinformatic methods. The antibody levels of polyclonal antibody titer against ClpP2 protein in rabbits and TB patients′ serum were detected by ELISA. Results: The recombinant ClpP2 protease was expressed as inclusion bodies in E. coli. The purity of purified protein was 93% by bandscan software analysis. The bioin-formatics analysis shows Mtb ClpP2 protein has multiple preponderant B cell and T cell epitopes. Rabbit antiserum titer was 1∶64 000;Serum anti-ClpP2 antibody levels in TB patients was higher than that in healthy control subjects. Conclusion:The recombinant ClpP2 protein was purified, and specific Rabbit anti-ClpP2 polyclonal antibody was prepared successfully. Experiment and bioinformatic information studies showed that Mtb ClpP2 protease has strong immunogenicity.