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利用不同的信号肽在转基因烟草植物中表达和大规模生产人组织型纤溶酶原激活物(t-PA)。

Expression and large-scale production of human tissue plasminogen activator (t-PA) in transgenic tobacco plants using different signal peptides.

机构信息

Department of Plant Breeding and Biotechnology, Faculty of Agriculture, Tarbiat Modares University, Tehran, Iran.

出版信息

Appl Biochem Biotechnol. 2013 Mar;169(6):1940-51. doi: 10.1007/s12010-013-0115-4. Epub 2013 Jan 26.

DOI:10.1007/s12010-013-0115-4
PMID:23354501
Abstract

An attempt was made to assess the expression level and targeting of a human protein entitled recombinant tissue plasminogen activator (rt-PA) through accumulation in three cellular compartments including the endoplasmic reticulum and cytosolic and apoplastic spaces in transgenic tobacco plants. In this context, three chimeric constructs pBI-SP-tPA, pBI-tPA-KDEL, and pBI-Ext-tPA were employed and transferred into the tobacco plants through a popular transformation-based system called Agrobacterium tumefaciens. As an initial screening system, the incorporation of the rt-PA gene in the genomic DNA of tobacco transgenic plants and the possible existence of the rt-PA-specific transcript in the total RNAs of transgenic plant leaves were confirmed via PCR and reverse transcription (RT)-PCR, respectively. Southern blot analysis, in addition, was used to determine the copy number of the corresponding gene (i.e., t-PA) transformed into the each transgenic plant; one or more copies were detected regarding transformants derived from all three abovementioned constructs. According to the enzyme-linked immunosorbent assay, the mean values of t-PA expression were calculated as 0.50, 0.68, and 0.69 μg/mg of the total soluble protein when a collection containing 30 transgenic plants transformed with pBI-SP-tPA, pBI-tPA-KDEL, and pBI-Ext-tPA was taken into account, respectively. The zymography assay was lastly performed and concluded the expression of the properly folded rt-PA in this expression system. Our results, altogether, revealed that tobacco plants could be utilized as a bioreactor system for the large-scale production of enzymatically active t-PA and presumably other therapeutic recombinant proteins in large quantities.

摘要

人们试图通过在三种细胞区室(包括内质网、细胞质和质外体空间)中积累,来评估一种名为重组组织纤溶酶原激活剂(rt-PA)的人类蛋白的表达水平和靶向性。在这种情况下,使用了三种嵌合构建体 pBI-SP-tPA、pBI-tPA-KDEL 和 pBI-Ext-tPA,并通过一种名为根癌农杆菌的流行转化系统将其转入烟草植物中。作为初始筛选系统,通过 PCR 和逆转录(RT)-PCR 分别确认了 rt-PA 基因整合到烟草转基因植物的基因组 DNA 中和转基因植物叶片总 RNA 中可能存在 rt-PA 特异性转录本。此外,Southern 印迹分析用于确定转化到每个转基因植物中的相应基因(即 t-PA)的拷贝数;对于源自上述三种构建体的转化体,检测到一个或多个拷贝。根据酶联免疫吸附测定法,当考虑包含 30 个转化为 pBI-SP-tPA、pBI-tPA-KDEL 和 pBI-Ext-tPA 的转基因植物的集合时,分别计算 t-PA 表达的平均值为 0.50、0.68 和 0.69μg/mg 总可溶性蛋白。最后进行了酶谱分析,并得出结论,在该表达系统中可以表达正确折叠的 rt-PA。总的来说,我们的结果表明,烟草植物可以用作生物反应器系统,用于大规模生产具有酶活性的 t-PA 和可能的其他大量治疗性重组蛋白。

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