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Massively parallel gene expression variation measurement of a synonymous codon library

机译:同义密码子文库的大规模平行基因表达变异测量

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Cell-to-cell variation in gene expression strongly affects population behavior and is key to multiple biological processes. While codon usage is known to affect ensemble gene expression, how codon usage influences variation in gene expression between single cells is not well understood. Here, we used a Sort-seq based massively parallel strategy to quantify gene expression variation from a green fluorescent protein (GFP) library containing synonymous codons in Escherichia coli. We found that sequences containing codons with higher tRNA Adaptation Index (TAI) scores, and higher codon adaptation index (CAI) scores, have higher GFP variance. This trend is not observed for codons with high Normalized Translation Efficiency Index (nTE) scores nor from the free energy of folding of the mRNA secondary structure. GFP noise, or squared coefficient of variance (CV2), scales with mean protein abundance for low-abundant proteins but does not change at high mean protein abundance. Our results suggest that the main source of noise for high-abundance proteins is likely not originating at translation elongation. Additionally, the drastic change in mean protein abundance with small changes in protein noise seen from our library implies that codon optimization can be performed without concerning gene expression noise for biotechnology applications.
机译:基因表达中的细胞对细胞变异强烈影响人口行为,并且是多种生物过程的关键。虽然已知密码子使用会影响集合基因表达,但是如何利用单细胞之间的基因表达的变异的措施。这里,我们使用基于SEQ基于SEQ的大规模并行策略来量化来自含有大肠杆菌中的同义密码子的绿色荧光蛋白(GFP)文库的基因表达变化。我们发现,含有具有较高TRNA适配指数(TAI)分数的密码子和更高的密码子适应指数(CAI)评分的序列具有更高的GFP方差。对于具有高标准化翻译效率指数(NTE)评分的密码子未观察到这种趋势,也不是来自MRNA二级结构的折叠的自由能量。 GFP噪声或平方差异(CV2),具有平均蛋白质的平均蛋白质的蛋白质,但在高平均蛋白质丰度下不会改变。我们的研究结果表明,高丰纹蛋白的主要噪声来源可能不会源于翻译伸长率。另外,从我们的图书馆看到的蛋白质噪声的小变化的平均蛋白质丰度的激烈变化意味着可以在没有关于生物技术应用的基因表达噪声进行密码子优化。

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