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Improvement of the pBI121 plant expression vector by leader replacement with a sequence combining a poly(CAA) and a CT motif

机译:通过前导序列替换poly(CAA)和CT基序的序列改进pBI121植物表达载体

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摘要

To improve expression levels of recombinant proteins in plants, a new leader sequence was designed. Several elements known to enhance gene translation and/or transcription were considered, including the CaMV 35S Inr site, a CT-rich motif often shared by highly expressed plant genes and a poly(CAA) region widespread in tobamovirus and plant leaders. The effect of the synthetic leader on gusA expression was evaluated in genetically modified tobacco plants by measuring the β-glucuronidase activity and the mRNA level. When compared to the gusA leader of pBI121, the new sequence determined a 8.6-fold and a 12.5-fold increase of enzyme concentration taking into account the whole plant population or the above-average expressors, respectively. Since most pCAMBIA vectors harbour a very short 5′-UTR, identical to a fragment of the pBI121 leader, leader replacement with the sequence herein described is strongly suggested.
机译:为了提高重组蛋白在植物中的表达水平,设计了一种新的前导序列。考虑了几种已知可增强基因翻译和/或转录的元件,包括CaMV 35S Inr位点,高表达植物基因通常共有的富含CT的基序,以及在烟草花叶病毒和植物前导物中广泛分布的poly(CAA)区。通过测量β-葡萄糖醛酸苷酶活性和mRNA水平,评估了转基因烟草植物中合成前导蛋白对gusA表达的影响。与pBI121的gusA前导序列相比,新序列分别考虑了整个植物种群或平均水平以上的表达体,确定了8.6倍和12.5倍的酶浓度增加。由于大多数pCAMBIA载体都带有非常短的5'-UTR,与pBI121前导序列的片段相同,因此强烈建议用本文所述的序列替换前导序列。

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