医学临床研究
醫學臨床研究
의학림상연구
JOURNAL OF CLINICAL RESEARCH
2014年
10期
1889-1891
,共3页
谢平丽%李峰%李跃辉%王宇环%罗晓玲%李官成
謝平麗%李峰%李躍輝%王宇環%囉曉玲%李官成
사평려%리봉%리약휘%왕우배%라효령%리관성
表皮生长因子/遗传学%大肠杆菌%基因扩增%遗传载体
錶皮生長因子/遺傳學%大腸桿菌%基因擴增%遺傳載體
표피생장인자/유전학%대장간균%기인확증%유전재체
Epidermal Grow th Factor/GE%Escherichia coli%Gene Amplification%Genetic Vectors
【目的】构建类表皮生长因子域7(EGFL7)原核表达载体,并诱导其表达、纯化及鉴定目的蛋白。【方法】以人肝癌细胞系 HepG2总RNA为模板,PCR扩增 EGFL7基因,克隆至原核表达载体pET‐21a(+)中,转化大肠杆菌 BL21(DE3),IPTG 诱导表达。 His‐tag 磁珠纯化重组蛋白 EGFL7,SDS‐PAGE 鉴定。【结果】克隆目的基因序列正确,未发生碱基突变;重组表达质粒pET21a(+)‐TRX‐EGFL7经双酶切鉴定构建正确;表达的重组蛋白相对分子量为80 kD ,与预期相符。【结论】成功在大肠杆菌BL21(DE3)中表达并纯化了EGFL7重组蛋白,为后续研究奠定了基础。
【目的】構建類錶皮生長因子域7(EGFL7)原覈錶達載體,併誘導其錶達、純化及鑒定目的蛋白。【方法】以人肝癌細胞繫 HepG2總RNA為模闆,PCR擴增 EGFL7基因,剋隆至原覈錶達載體pET‐21a(+)中,轉化大腸桿菌 BL21(DE3),IPTG 誘導錶達。 His‐tag 磁珠純化重組蛋白 EGFL7,SDS‐PAGE 鑒定。【結果】剋隆目的基因序列正確,未髮生堿基突變;重組錶達質粒pET21a(+)‐TRX‐EGFL7經雙酶切鑒定構建正確;錶達的重組蛋白相對分子量為80 kD ,與預期相符。【結論】成功在大腸桿菌BL21(DE3)中錶達併純化瞭EGFL7重組蛋白,為後續研究奠定瞭基礎。
【목적】구건류표피생장인자역7(EGFL7)원핵표체재체,병유도기표체、순화급감정목적단백。【방법】이인간암세포계 HepG2총RNA위모판,PCR확증 EGFL7기인,극륭지원핵표체재체pET‐21a(+)중,전화대장간균 BL21(DE3),IPTG 유도표체。 His‐tag 자주순화중조단백 EGFL7,SDS‐PAGE 감정。【결과】극륭목적기인서렬정학,미발생감기돌변;중조표체질립pET21a(+)‐TRX‐EGFL7경쌍매절감정구건정학;표체적중조단백상대분자량위80 kD ,여예기상부。【결론】성공재대장간균BL21(DE3)중표체병순화료EGFL7중조단백,위후속연구전정료기출。
[Objective]To construct the prokaryotic expression vector of EGFL 7 ,and to induce the expression and purification EGFL7 ,and to identify EGFL7 protein .[Methods]EGFL7 gene was amplified from human hepato‐ma cell HepG2 by PCR and cloned into prokaryotic expression vector pET 21a(+) ,and then transformed into Esche‐richia coli BL21(DE3) .The expression of EGFL7 was induced by isopropylβ‐D‐1‐thiogalactopyranoside(IPTG) ,and purified by His‐tag magnetic beads ,and identified by SDS‐PAGE .[Results] The sequence of the cloned target gene was correct and had no base mutation .Double enzyme digestion showed that the recombinant plasmid pET 21a (+)‐TRX‐EGFL7 was constructed correctly .The recombinant protein EGFL7 was expressed with an expected molecular weight of 80kD .[Conclusion]The recombinant protein EGFL7 is successfully expressed and purified in Escherichia coli BL21 (DE3) which sets up the foundation for the following study .
