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In vivo co-localization of enzymes on RNA scaffolds increases metabolic production in a geometrically dependent manner

机译:酶在RNA支架上的体内共定位以几何依赖方式增加代谢产生

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Co-localization of biochemical processes plays a key role in the directional control of metabolic fluxes toward specific products in cells. Here, we employ in vivo scaffolds made of RNA that can bind engineered proteins fused to specific RNA binding domains. This allows proteins to be co-localized on RNA scaffolds inside living Escherichia coli. We assembled a library of eight aptamers and corresponding RNA binding domains fused to partial fragments of fluorescent proteins. New scaffold designs could co-localize split green fluorescent protein fragments to produce activity as measured by cell-based fluorescence. The scaffolds consisted of either single bivalent RNAs or RNAs designed to polymerize in one or two dimensions. The new scaffolds were used to increase metabolic output from a two-enzyme pentadecane production pathway that contains a fatty aldehyde intermediate, as well as three and four enzymes in the succinate production pathway. Pentadecane synthesis depended on the geometry of enzymes on the scaffold, as determined through systematic reorientation of the acyl-ACP reductase fusion by rotation via addition of base pairs to its cognate RNA aptamer. Together, these data suggest that intra-cellular scaffolding of enzymatic reactions may enhance the direct channeling of a variety of substrates.
机译:生化过程的共定位在代谢通量向细胞中特定产物的方向控制中起着关键作用。在这里,我们采用由RNA制成的体内支架,该支架可以结合融合到特定RNA结合结构域的工程蛋白。这使蛋白质可以共定位在活大肠杆菌内部的RNA支架上。我们组装了八个适体和与荧光蛋白部分片段融合的相应RNA结合结构域的文库。新的支架设计可以共定位分裂的绿色荧光蛋白片段,从而产生基于细胞荧光的活性。支架由单个二价RNA或设计用于在一维或二维聚合的RNA组成。新的支架用于增加包含脂肪醛中间体以及琥珀酸生产途径中的三种和四种酶的二酶十五烷生产途径的代谢输出。十五烷的合成取决于支架上酶的几何形状,这是通过对酰基-ACP还原酶融合物进行系统性重新定向而确定的,方法是通过向其关联的RNA适体中添加碱基对进行旋转来实现。总之,这些数据表明酶促反应的细胞内支架可以增强多种底物的直接通道。

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