吉林农业大学学报
吉林農業大學學報
길임농업대학학보
JOURNAL OF JILIN AGRICUL TURAL UNIVERSITY
2014年
1期
51-55,65
,共6页
王皓%徐立群%陈欢%孙旸%王刚%陈光
王皓%徐立群%陳歡%孫旸%王剛%陳光
왕호%서립군%진환%손양%왕강%진광
胶原蛋白%重组载体%大肠杆菌%克隆%纯化
膠原蛋白%重組載體%大腸桿菌%剋隆%純化
효원단백%중조재체%대장간균%극륭%순화
collagen%recombinant vector%Escherichia coli%cloning%purification
根据GenBank上查到的人胶原蛋白序列COL6A2(NM058175.2),利用Primer 5设计特异性引物,以吉林农业大学生物物理实验室构建的重组质粒pCMV-Sport6-COL6A2为模板进行目的基因的克隆,获得目的基因COL6A2,然后用双酶切的方法连接目的基因COL6A2和表达载体pET32a,将连接产物转化到大肠杆菌中构建原核表达载体pET32a-COL6A2。再将鉴定成功的重组质粒pET32a-COL6A2分别转化到大肠杆菌BL21、BL21(DE3)、BL21(BE3)plysS及Rosetta(DE3)中,采用1 mmol/L的异丙基-β-D-硫代半乳糖苷(IPTG)诱导重组蛋白表达,经12%SDS-PAGE电泳分析并筛选出重组蛋白表达量最高的菌株。利用Ni Sepharose 6 Fast Flow琼脂糖树脂亲和层析柱纯化重组蛋白。结果表明:获得了大小为570 bp的COL6A2片段,经测序鉴定序列正确;成功构建了pET32a-COL6A2原核表达载体并表达出约30 kD的目的蛋白;筛选出BL21(DE3)作为高效表达菌株,其重组蛋白表达量占菌体总蛋白的23.9%;经镍离子亲和层析纯化获得了纯度>90%的目的蛋白。
根據GenBank上查到的人膠原蛋白序列COL6A2(NM058175.2),利用Primer 5設計特異性引物,以吉林農業大學生物物理實驗室構建的重組質粒pCMV-Sport6-COL6A2為模闆進行目的基因的剋隆,穫得目的基因COL6A2,然後用雙酶切的方法連接目的基因COL6A2和錶達載體pET32a,將連接產物轉化到大腸桿菌中構建原覈錶達載體pET32a-COL6A2。再將鑒定成功的重組質粒pET32a-COL6A2分彆轉化到大腸桿菌BL21、BL21(DE3)、BL21(BE3)plysS及Rosetta(DE3)中,採用1 mmol/L的異丙基-β-D-硫代半乳糖苷(IPTG)誘導重組蛋白錶達,經12%SDS-PAGE電泳分析併篩選齣重組蛋白錶達量最高的菌株。利用Ni Sepharose 6 Fast Flow瓊脂糖樹脂親和層析柱純化重組蛋白。結果錶明:穫得瞭大小為570 bp的COL6A2片段,經測序鑒定序列正確;成功構建瞭pET32a-COL6A2原覈錶達載體併錶達齣約30 kD的目的蛋白;篩選齣BL21(DE3)作為高效錶達菌株,其重組蛋白錶達量佔菌體總蛋白的23.9%;經鎳離子親和層析純化穫得瞭純度>90%的目的蛋白。
근거GenBank상사도적인효원단백서렬COL6A2(NM058175.2),이용Primer 5설계특이성인물,이길임농업대학생물물리실험실구건적중조질립pCMV-Sport6-COL6A2위모판진행목적기인적극륭,획득목적기인COL6A2,연후용쌍매절적방법련접목적기인COL6A2화표체재체pET32a,장련접산물전화도대장간균중구건원핵표체재체pET32a-COL6A2。재장감정성공적중조질립pET32a-COL6A2분별전화도대장간균BL21、BL21(DE3)、BL21(BE3)plysS급Rosetta(DE3)중,채용1 mmol/L적이병기-β-D-류대반유당감(IPTG)유도중조단백표체,경12%SDS-PAGE전영분석병사선출중조단백표체량최고적균주。이용Ni Sepharose 6 Fast Flow경지당수지친화층석주순화중조단백。결과표명:획득료대소위570 bp적COL6A2편단,경측서감정서렬정학;성공구건료pET32a-COL6A2원핵표체재체병표체출약30 kD적목적단백;사선출BL21(DE3)작위고효표체균주,기중조단백표체량점균체총단백적23.9%;경얼리자친화층석순화획득료순도>90%적목적단백。
According to the sequence of COL6A2 gene(NM0581 75.2)from GenBank of NCBI,specific DNA primers were designed by primer 5 .Target gene COL6A2 was obtained by PCR from the recombi-nant plasmid of pCMV-Sport6-COL6A2 structured by laboratory,gene COL6A2 and pET32a vector were connected by restriction endonuclease digestion assay .The recombinant plasmids of pET32a-COL6A2 were transformed into E .coli BL21 ,BL21 (DE3),BL21 (BE3)plysS and Rosetta(DE3)respectively and induced by IPTG .Then the best efficient strain was selected by SDS-PAGE assay .The recombinant protein was purified by Ni Sepharose 6 Fast Flow.The results show that cDNA sequence of COL6A2 was cloned correctly .The vector of pET32a-COL6A2 was constructed and the target protein about 30 kD was expressed successfully .E .coli BL21 (DE3)was screened as efficient expression strain and the expression level of target protein was 23.9 %.The target protein whose purity is more than 90%was obtained by Ni Sepharose 6 Fast Flow .The results lay foundation for the research of recombinant collagen activity .
