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草莓的根和茎部分:功能性人胰岛素原的生产工厂。

Root and shoot parts of strawberry: factories for production of functional human pro-insulin.

作者信息

Tavizi Ashkan, Javaran Mokhtar Jalali, Moieni Ahmad, Mohammadi-Dehcheshmeh Manijeh, Mohebodini Mehdi, Ebrahimie Esmaeil

机构信息

Institute of Biotechnology, Shiraz University, Shiraz, Iran.

出版信息

Mol Biol Rep. 2015 May;42(5):1013-23. doi: 10.1007/s11033-014-3837-7. Epub 2014 Nov 18.

Abstract

Diabetes, a disease caused by excessive blood sugar, is caused by the lack of insulin. For commercial production, insulin is made in bacteria or yeast by protein recombinant technology. The focus of this research is evaluating another resource and producing of recombinant insulin protein in as strawberry as this plant has high potential in production of pharmaceutical proteins. Strawberry is a suitable bioreactor for production of recombinant proteins especially edible vaccines. In this research, human pro-insulin gene was cloned in pCAMBIA1304 vector under CaMV35S promoter and NOS terminator. Agrobacterium tumefaciens LBA4404, AGL1, EHA105, EHA101, C58, C58 (pGV2260) and C58 (pGV3101) strains were used for transformation of pro-insulin gene into strawberry cv. Camarosa, Selva, Sarian Hybrid, Pajaro, Paros, Gaviota, Alpine. Additionally, Agrobacterium rhizogenes K599, R1000, A4 and MSU440 strains were utilized for gene transformation into hairy roots. PCR analysis indicated the presence of transformed human pro-insulin gene in the strawberry and hairy roots. Also, its transcription was confirmed using RT-PCR. Furthermore, the analysis of plants, fruits and hairy roots at the level of proteins using dot blot, ELISA, SDS-PAGE and ECL tests re-confirmed the expression of this protein in the transgenic plants as well as hairy roots. Protein purification of human pro-insulin from transgenic tissues was performed using affinity chromatography. Finally, the bioassay of recombinant pro-insulin was performed. The analysis of second generations of transgenic plants (T1) at DNA and protein levels was also performed as a complementary experiment. This study opens a new avenue in molecular farming of human pro-insulin through its mass production in roots and shoots of strawberry.

摘要

糖尿病是一种由血糖过高引起的疾病,是由于胰岛素缺乏所致。在商业生产中,胰岛素是通过蛋白质重组技术在细菌或酵母中制造的。本研究的重点是评估另一种资源,并在草莓中生产重组胰岛素蛋白,因为这种植物在药用蛋白生产方面具有很高的潜力。草莓是生产重组蛋白尤其是可食用疫苗的合适生物反应器。在本研究中,人胰岛素原基因在CaMV35S启动子和NOS终止子的控制下克隆到pCAMBIA1304载体中。使用根癌农杆菌LBA4404、AGL1、EHA105、EHA101、C58、C58(pGV2260)和C58(pGV3101)菌株将胰岛素原基因转化到草莓品种Camarosa、Selva、Sarian Hybrid、Pajaro、Paros、Gaviota、Alpine中。此外,利用发根农杆菌K599、R1000、A4和MSU440菌株将基因转化到毛状根中。PCR分析表明草莓和毛状根中存在转化的人胰岛素原基因。此外,通过RT-PCR证实了其转录。此外,使用斑点印迹、ELISA、SDS-PAGE和ECL试验在蛋白质水平上对植物、果实和毛状根进行分析,再次证实了该蛋白在转基因植物以及毛状根中的表达。使用亲和色谱法从转基因组织中纯化人胰岛素原蛋白。最后,对重组胰岛素原进行了生物测定。作为补充实验,还对第二代转基因植物(T1)进行了DNA和蛋白质水平的分析。这项研究通过在草莓的根和芽中大量生产人胰岛素原,为其分子农业开辟了一条新途径。

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