Shirole Nitin, Balasubramanian Sreeram, Yanofsky Charles, Cruz-Vera Luis
Department of Biological Sciences, University of Alabama Huntsville, USA.
J Vis Exp. 2011 Feb 25(48):2498. doi: 10.3791/2498.
Recently, structural and biochemical studies have detailed many of the molecular events that occur in the ribosome during inhibition of protein synthesis by antibiotics and during nascent polypeptide synthesis. Some of these antibiotics, and regulatory nascent polypeptides mostly in the form of peptidyl-tRNAs, inhibit either peptide bond formation or translation termination. These inhibitory events can stop the movement of the ribosome, a phenomenon termed "translational arrest". Translation arrest induced by either an antibiotic or a nascent polypeptide has been shown to regulate the expression of genes involved in diverse cellular functions such as cell growth, antibiotic resistance, protein translocation and cell metabolism. Knowledge of how antibiotics and regulatory nascent polypeptides alter ribosome function is essential if we are to understand the complete role of the ribosome in translation, in every organism. Here, we describe a simple methodology that can be used to purify, exclusively, for analysis, those ribosomes translating a specific mRNA and containing a specific peptidyl-tRNA. This procedure is based on selective isolation of translating ribosomes bound to a biotin-labeled mRNA. These translational complexes are separated from other ribosomes in the same mixture, using streptavidin paramagnetic beads (SMB) and a magnetic field (MF). Biotin-labeled mRNAs are synthesized by run-off transcription assays using as templates PCR-generated DNA fragments that contain T7 transcriptional promoters. T7 RNA polymerase incorporates biotin-16-UMP from biotin-UTP; under our conditions approximately ten biotin-16-UMP molecules are incorporated in a 600 nt mRNA with a 25% UMP content. These biotin-labeled mRNAs are then isolated, and used in in vitro translation assays performed with release factor 2 (RF2)-depleted cell-free extracts obtained from Escherichia coli strains containing wild type or mutant ribosomes. Ribosomes translating the biotin-labeled mRNA sequences are stalled at the stop codon region, due to the absence of the RF2 protein, which normally accomplishes translation termination. Stalled ribosomes containing the newly synthesized peptidyl-tRNA are isolated and removed from the translation reactions using SMB and an MF. These beads only bind biotin-containing messages. The isolated, translational complexes, can be used to analyze the structural and functional features of wild type or mutant ribosomal components, or peptidyl-tRNA sequences, as well as determining ribosome interaction with antibiotics or other molecular factors. To examine the function of these isolated ribosome complexes, peptidyl-transferase assays can be performed in the presence of the antibiotic puromycin. To study structural changes in translational complexes, well established procedures can be used, such as i) crosslinking to specific amino acids and/or ii) alkylation protection assays.
最近,结构和生化研究详细阐述了在抗生素抑制蛋白质合成过程中以及新生多肽合成过程中核糖体发生的许多分子事件。其中一些抗生素以及主要以肽基 - tRNA形式存在的调节性新生多肽,会抑制肽键形成或翻译终止。这些抑制事件会阻止核糖体的移动,这种现象称为“翻译停滞”。由抗生素或新生多肽诱导的翻译停滞已被证明可调节参与多种细胞功能的基因表达,如细胞生长、抗生素抗性、蛋白质转运和细胞代谢。如果我们要了解核糖体在每个生物体翻译过程中的完整作用,那么了解抗生素和调节性新生多肽如何改变核糖体功能至关重要。在此,我们描述一种简单的方法,该方法可专门用于纯化用于分析的那些翻译特定mRNA并包含特定肽基 - tRNA的核糖体。此过程基于选择性分离与生物素标记的mRNA结合的翻译核糖体。使用链霉亲和素顺磁珠(SMB)和磁场(MF),将这些翻译复合物与同一混合物中的其他核糖体分离。生物素标记的mRNA通过使用含有T7转录启动子的PCR产生的DNA片段作为模板的径流转录测定法合成。T7 RNA聚合酶从生物素 - UTP掺入生物素 - 16 - UMP;在我们的条件下,在UMP含量为25% 的600 nt mRNA中大约掺入十个生物素 - 16 - UMP分子。然后分离这些生物素标记的mRNA,并用于从含有野生型或突变核糖体的大肠杆菌菌株获得的无释放因子2(RF2)的无细胞提取物中进行的体外翻译测定。由于缺乏通常完成翻译终止的RF2蛋白,翻译生物素标记的mRNA序列的核糖体在终止密码子区域停滞。使用SMB和MF从翻译反应中分离并去除含有新合成的肽基 - tRNA的停滞核糖体。这些珠子仅结合含生物素的信息。分离出的翻译复合物可用于分析野生型或突变核糖体组分或肽基 - tRNA序列的结构和功能特征,以及确定核糖体与抗生素或其他分子因子的相互作用。为了检查这些分离的核糖体复合物的功能,可以在抗生素嘌呤霉素存在的情况下进行肽基转移酶测定。为了研究翻译复合物中的结构变化,可以使用成熟的程序,如i)与特定氨基酸交联和/或ii)烷基化保护测定。
