首页> 美国卫生研究院文献>International Journal of Molecular Sciences >Sequence Analysis and Potentials of the Native RbcS Promoter in the Development of an Alternative Eukaryotic Expression System Using Green Microalga Ankistrodesmus convolutus
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Sequence Analysis and Potentials of the Native RbcS Promoter in the Development of an Alternative Eukaryotic Expression System Using Green Microalga Ankistrodesmus convolutus

机译:天然RbcS启动子的序列分析和潜力的发展使用绿色微藻Ankistrodesmus卷积的另一种真核表达系统中。

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摘要

The availability of highly active homologous promoters is critical in the development of a transformation system and improvement of the transformation efficiency. To facilitate transformation of green microalga Ankistrodesmus convolutus which is considered as a potential candidate for many biotechnological applications, a highly-expressed native promoter sequence of ribulose-1,5-bisphosphate carboxylase/oxygenase small subunit (AcRbcS) has been used to drive the expression of β-glucuronidase (gusA) gene in this microalga. Besides the determination of the transcription start site by 5′-RACE, sequence analysis revealed that AcRbcS promoter contained consensus TATA-box and several putative cis-acting elements, including some representative light-regulatory elements (e.g., G-box, Sp1 motif and SORLIP2), which confer light responsiveness in plants, and several potential conserved motifs (e.g., CAGAC-motif, YCCYTGG-motifs and CACCACA-motif), which may be involved in light responsiveness of RbcS gene in green microalgae. Using AcRbcS promoter::gusA translational fusion, it was demonstrated that this promoter could function as a light-regulated promoter in transgenic A. convolutus, which suggested that the isolated AcRbcS promoter was a full and active promoter sequence that contained all cis-elements required for developmental and light-mediated control of gene expression, and this promoter can be used to drive the expression of heterologous genes in A. convolutus. This achievement therefore advances the development of A. convolutus as an alternative expression system for the production of recombinant proteins. This is the first report on development of gene manipulation system for unicellular green alga A. convolutus.
机译:高活性同源启动子的可用性对于转化系统的开发和转化效率的提高至关重要。为了促进被认为是许多生物技术应用潜在候选者的绿色微藻盘旋线虫的转化,已使用高度表达的核糖-1,5-双磷酸羧化酶/加氧酶小亚基(AcRbcS)的天然启动子序列来驱动表达微藻中β-葡萄糖醛酸苷酶(gusA)基因的表达除了通过5'-RACE确定转录起始位点外,序列分析还显示AcRbcS启动子还包含共有的TATA-box和几个假定的顺式作用元件,包括一些代表性的光调节元件(例如G-box,Sp1基序和SORLIP2),赋予植物光响应性,以及一些潜在的保守基序(例如CAGAC-motif,YCCYTGG-motifs和CACCACA-motif),可能与绿色微藻中RbcS基因的光响应性有关。使用AcRbcS启动子:: gusA翻译融合,表明该启动子可以在转基因曲霉中充当光调节启动子,这表明分离的AcRbcS启动子是一个完整且活跃的启动子序列,其中包含所需的所有顺式元件用于发育和光介导的基因表达控制,并且该启动子可用于驱动卷积曲霉中异源基因的表达。因此,该成就促进了卷积曲霉作为用于生产重组蛋白的替代表达系统的开发。这是关于单细胞绿藻曲霉基因操纵系统开发的第一份报告。

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