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Ribonuclease selection for ribosome profiling

机译:核糖核酸酶选择对核糖体分析

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Ribosome profiling has emerged as a powerful method to assess global gene translation, but methodological and analytical challenges often lead to inconsistencies across labs and model organisms. A critical issue in ribosome profiling is nuclease treatment of ribosome-mRNA complexes, as it is important to ensure both stability of ribosomal particles and complete conversion of polysomes to monosomes. We performed comparative ribosome profiling in yeast and mice with various ribonucleases including I, A, S7 and T1, characterized their cutting preferences, trinucleotide periodicity patterns and coverage similarities across coding sequences, and showed that they yield comparable estimations of gene expression when ribosome integrity is not compromised. However, ribosome coverage patterns of individual transcripts had little in common between the ribonucleases. We further examined their potency at converting polysomes to monosomes across other commonly used model organisms, including bacteria, nematodes and fruit flies. In some cases, ribonuclease treatment completely degraded ribosome populations. Ribonuclease T1 was the only enzyme that preserved ribosomal integrity while thoroughly converting polysomes to monosomes in all examined species. This study provides a guide for ribonuclease selection in ribosome profiling experiments across most common model systems.
机译:核糖体分析已经成为评估全球基因翻译的强大方法,但方法论和分析挑战往往导致实验室和模型生物体的不一致。核糖体分析中的一个关键问题是核糖体-mRNA配合物的核酸酶处理,因为重要的是确保核糖体颗粒的稳定性并完全转化为单体粒子。我们在酵母和小鼠中进行了比较核糖体分析,其中包含I,A,S7和T1,其特征在于它们在编码序列中的切割偏好,三核苷酸周期性模式和覆盖相似性,并且显示它们在核糖体完整性时产生基因表达的相当估计没有妥协。然而,核糖核酸酶之间的个体转录物的核糖体覆盖范围几乎没有常见。我们进一步研究了他们在其他常用模型生物体上转换多种多组织的效力,包括细菌,线虫和果蝇。在一些情况下,核糖核酸酶处理完全降解了核糖体群体。 Ribonuclease T1是保存核糖体完整性的唯一酶,同时将多变地转化为所有检查物种中的单体。本研究提供了核糖核酸核糖核酸酶选择的指南,这些核糖体分析实验在大多数常见的模型系统上。

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