国际检验医学杂志
國際檢驗醫學雜誌
국제검험의학잡지
INTERNATIONAL JOURNAL OF LABORATORY MEDICINE
2014年
13期
1665-1666,1669
,共3页
夏剑波%席金瓯%刘贽%王维鹏
夏劍波%席金甌%劉贄%王維鵬
하검파%석금구%류지%왕유붕
人细胞空泡蛋白分选因子4A%基因克隆%真核表达
人細胞空泡蛋白分選因子4A%基因剋隆%真覈錶達
인세포공포단백분선인자4A%기인극륭%진핵표체
human vacuolar protein sorting 4A%gene clone%eukaryotic expression
目的:克隆人细胞空泡蛋白分选因子4A(human vacuolar protein sorting 4A,hVPS4A)基因,构建其真核表达质粒。方法以 Huh7细胞 cDNA 为模板,设计引物扩增全长 hVPS4A 基因,再将目的基因插入到真核载体 pRK5中。重组质粒经PCR、酶切和 DNA 测序确认。结果从 Huh7细胞 cDNA 中扩增得到约1350 bp 大小的目的片段,经回收、纯化、酶切后与载体pRK5连接,转化 DH5α大肠杆菌。选择 PCR 鉴定阳性的重组质粒,经 EcoRⅠ单酶切可见约一条5900 bp 片段;经 EcoRⅠ和HindⅢ双酶切可得到4600 bp 和1350 bp 两个片段,分别与载体 pRK5和目的片段 hVPS4A 预期大小一致;DNA 测序结果显示插入片段与 hVPS4A 参考序列一致。结论成功构建了含 hVPS4A 基因的真核表达载体,为进一步研究 hVPS4A 的生物学功能提供了条件。
目的:剋隆人細胞空泡蛋白分選因子4A(human vacuolar protein sorting 4A,hVPS4A)基因,構建其真覈錶達質粒。方法以 Huh7細胞 cDNA 為模闆,設計引物擴增全長 hVPS4A 基因,再將目的基因插入到真覈載體 pRK5中。重組質粒經PCR、酶切和 DNA 測序確認。結果從 Huh7細胞 cDNA 中擴增得到約1350 bp 大小的目的片段,經迴收、純化、酶切後與載體pRK5連接,轉化 DH5α大腸桿菌。選擇 PCR 鑒定暘性的重組質粒,經 EcoRⅠ單酶切可見約一條5900 bp 片段;經 EcoRⅠ和HindⅢ雙酶切可得到4600 bp 和1350 bp 兩箇片段,分彆與載體 pRK5和目的片段 hVPS4A 預期大小一緻;DNA 測序結果顯示插入片段與 hVPS4A 參攷序列一緻。結論成功構建瞭含 hVPS4A 基因的真覈錶達載體,為進一步研究 hVPS4A 的生物學功能提供瞭條件。
목적:극륭인세포공포단백분선인자4A(human vacuolar protein sorting 4A,hVPS4A)기인,구건기진핵표체질립。방법이 Huh7세포 cDNA 위모판,설계인물확증전장 hVPS4A 기인,재장목적기인삽입도진핵재체 pRK5중。중조질립경PCR、매절화 DNA 측서학인。결과종 Huh7세포 cDNA 중확증득도약1350 bp 대소적목적편단,경회수、순화、매절후여재체pRK5련접,전화 DH5α대장간균。선택 PCR 감정양성적중조질립,경 EcoRⅠ단매절가견약일조5900 bp 편단;경 EcoRⅠ화HindⅢ쌍매절가득도4600 bp 화1350 bp 량개편단,분별여재체 pRK5화목적편단 hVPS4A 예기대소일치;DNA 측서결과현시삽입편단여 hVPS4A 삼고서렬일치。결론성공구건료함 hVPS4A 기인적진핵표체재체,위진일보연구 hVPS4A 적생물학공능제공료조건。
Objective To clone human vacuolar protein sorting 4A gene(hVPS4A)and to construct its eukaryotic expressive plasmid.Methods Primers were designed to amplify the full length hVPS4A by PCR using cDNA of Huh7 cell as a template,then the target DNA was inserted into the eukaryotic vector pRK5.The recombinant plasmid was confirmed by PCR,restriction enzyme digestion and DNA sequencing.Results A 1 300 bp fragment was successfully amplified by PCR from the cDNA of Huh7 cells.Af-ter recycled,purified and ligated with the vector pRK5,the recombinant plasmid was transformed into E.coli DH5α.The positive re-combinant plasmid identified by PCR was selectred and digested by EcoRⅠto get a 5 900 bp fragment;and two fragments including 4 600 bp and 1 350 bp were obtained using EcoRⅠand HindⅢ digestion;the size of these two fragments were consistent with the pRK5 target fragment and the inserted hVPS4A as expected.Moreover,DNA sequencing results confirmed that the inserted frag-ment was in accordance with the hVPS4A reference sequence.Conclusion The eukaryotic expression vector containing hVPS4A gene is constructed successfully,which provides the condition for further study on the hVPS4A biological functions.
