首都医科大学学报
首都醫科大學學報
수도의과대학학보
JOURNAL OF CAPITAL UNIVERSITY OF MEDICAL SCIENCES
2015年
2期
232-238
,共7页
毕阔%秦佳佳%杨静%诸欣平
畢闊%秦佳佳%楊靜%諸訢平
필활%진가가%양정%제흔평
旋毛虫%cDNA文库%膜蛋白%表达
鏇毛蟲%cDNA文庫%膜蛋白%錶達
선모충%cDNA문고%막단백%표체
Trichinella spiralis%cDNA library%membrane protein%expression
目的:免疫筛选旋毛虫成虫cDNA文库,寻找抗旋毛虫病的疫苗候选抗原或诊断抗原。方法应用旋毛虫感染的猪血清免疫筛选旋毛虫成虫cDNA文库,获得阳性克隆。将一阳性克隆与原核表达载体pET-28a(+)构建重组质粒,异丙醇硫代-β-D-半乳糖苷( isopropyl β-D-thiogalactoside,IPTG)诱导后,利用亲和层析柱纯化目的蛋白,并通过酶联免疫吸附实验( enzyme-linked immunosorbent assay,ELISA)和Western blotting鉴定其抗原特异性和免疫原性。结果免疫筛选旋毛虫成虫cDNA文库获得42个阳性克隆,选取一个新基因Tmp10,成功构建了重组质粒pET-28a(+)/ Tmp10,诱导表达后获得的重组蛋白(rTmp10)的相对分子质量约为40000。 Western blotting检测结果显示,该重组蛋白可被旋毛虫感染小鼠和猪血清所识别,具有抗原特异性。rTmp10免疫小鼠可诱导产生高滴度的抗体,显示其具有较好的免疫原性。结论免疫筛选旋毛虫成虫cDNA文库获得一个新基因Tmp10,生物信息学分析预测其为膜蛋白,其重组蛋白(rTmp10)具有较好的抗原特异性和免疫原性。
目的:免疫篩選鏇毛蟲成蟲cDNA文庫,尋找抗鏇毛蟲病的疫苗候選抗原或診斷抗原。方法應用鏇毛蟲感染的豬血清免疫篩選鏇毛蟲成蟲cDNA文庫,穫得暘性剋隆。將一暘性剋隆與原覈錶達載體pET-28a(+)構建重組質粒,異丙醇硫代-β-D-半乳糖苷( isopropyl β-D-thiogalactoside,IPTG)誘導後,利用親和層析柱純化目的蛋白,併通過酶聯免疫吸附實驗( enzyme-linked immunosorbent assay,ELISA)和Western blotting鑒定其抗原特異性和免疫原性。結果免疫篩選鏇毛蟲成蟲cDNA文庫穫得42箇暘性剋隆,選取一箇新基因Tmp10,成功構建瞭重組質粒pET-28a(+)/ Tmp10,誘導錶達後穫得的重組蛋白(rTmp10)的相對分子質量約為40000。 Western blotting檢測結果顯示,該重組蛋白可被鏇毛蟲感染小鼠和豬血清所識彆,具有抗原特異性。rTmp10免疫小鼠可誘導產生高滴度的抗體,顯示其具有較好的免疫原性。結論免疫篩選鏇毛蟲成蟲cDNA文庫穫得一箇新基因Tmp10,生物信息學分析預測其為膜蛋白,其重組蛋白(rTmp10)具有較好的抗原特異性和免疫原性。
목적:면역사선선모충성충cDNA문고,심조항선모충병적역묘후선항원혹진단항원。방법응용선모충감염적저혈청면역사선선모충성충cDNA문고,획득양성극륭。장일양성극륭여원핵표체재체pET-28a(+)구건중조질립,이병순류대-β-D-반유당감( isopropyl β-D-thiogalactoside,IPTG)유도후,이용친화층석주순화목적단백,병통과매련면역흡부실험( enzyme-linked immunosorbent assay,ELISA)화Western blotting감정기항원특이성화면역원성。결과면역사선선모충성충cDNA문고획득42개양성극륭,선취일개신기인Tmp10,성공구건료중조질립pET-28a(+)/ Tmp10,유도표체후획득적중조단백(rTmp10)적상대분자질량약위40000。 Western blotting검측결과현시,해중조단백가피선모충감염소서화저혈청소식별,구유항원특이성。rTmp10면역소서가유도산생고적도적항체,현시기구유교호적면역원성。결론면역사선선모충성충cDNA문고획득일개신기인Tmp10,생물신식학분석예측기위막단백,기중조단백(rTmp10)구유교호적항원특이성화면역원성。
Objective In order to obtain vaccine or diagnostic candidate antigens for trichinellosis, the adult cDNA library of T. spiralis was immunoscreened. Methods The adult cDNA library of T. spiralis was screened using the swine sera infected with T. spiralis. The cDNA sequence of the positive clone was analyzed and the recombinant protein was expressed and purified. The antigenicity and immunogenicity of the recombinant protein was analyzed with ELISA and Western blotting. Results Forty-two positive clones were identified by immunscreened. A novel gene Tmp10 of T. spiralis was sequenced and recombinant plasmid pET-28a (+)/Tmp10 was successfully constructed. The recombinant protein(rTmp10) was expressed and the molecular weight was about 40 000. The results of Western blotting showed that the rTmp10 could be recognized by sera from the mice and swine infected with T. spiralis respectively, which showed that the rTmp10 had the specific antigenicity. The rTmp10 could induce a high level of specific anti-Tmp10 IgG antibodies, which showed that the rTmp10 had the immunogenicity. Conclusion The novel gene Tmp10 of T. spiralis was obtained by immunoscreening and predicted to be a membrane protein. The recombinant protein Tmp10 had the high specific antigenicity and immunogenicity.