| A Small RNA Isolation and Sequencing Protocol and Its Application to Assay CRISPR RNA Biogenesis in Bacteria
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Author:
Date:
2018-02-20
[Abstract] Next generation high-throughput sequencing has enabled sensitive and unambiguous analysis of RNA populations in cells. Here, we describe a method for isolation and strand-specific sequencing of small RNA pools from bacteria that can be multiplexed to accommodate multiple biological samples in a single experiment. Small RNAs are isolated by polyacrylamide gel electrophoresis and treated with T4 polynucleotide kinase. This allows for 3’ adapter ligation to CRISPR RNAs, which don’t have pre-existing 3’-OH ends. Pre-adenylated adapters are then ligated using T4 RNA ligase 1 in the absence of ATP and with a high concentration of polyethylene glycol (PEG). The 3’ capture step enables precise determination of the 3’ ends of diverse RNA molecules. Additionally, a random hexamer in the ligated ...
[摘要] 新一代高通量测序技术能够对细胞中的RNA群体进行敏感和明确的分析。在这里,我们描述了一种从细菌中分离和链特异性测序小RNA池的方法,所述细菌可以在单个实验中多路复用以容纳多个生物样品。小RNA通过聚丙烯酰胺凝胶电泳分离并用T4多核苷酸激酶处理。这允许3'衔接头连接至CRISPR RNA,其不具有预先存在的3'-OH末端。然后使用T4 RNA连接酶1在不存在ATP和高浓度聚乙二醇(PEG)的情况下将前腺苷酸化的衔接子连接。 3'捕获步骤能够精确测定不同RNA分子的3'末端。此外,连接适配器中的随机六聚体有助于控制潜在的下游扩增偏差。逆转录后,将cDNA产物环化并通过PCR制备文库。我们显示扩增的文库不需要通过凝胶电泳可见,以期望产物的有效测序。使用这种方法,我们通常从少量纯化的小RNA制备RNA测序文库。该协议适合于通过对成熟的CRISPR RNA进行测序来测定细菌中的CRISPR RNA生物合成,但可以用于测序不同类型的小RNA。我们还提供了一个完整的数据处理管道示例,并提供了运行所提供脚本的说明。
【背景】与聚集的经常散布的短回文重复序列(CRISPR)相关的遗传模块赋予不同的原核宿主适应性免疫(Barrangou et ...
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| Immunoprecipitation of Tri-methylated Capped RNA
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Author:
Date:
2018-02-05
[Abstract] Cellular quiescence (also known as G0 arrest) is characterized by reduced DNA replication, increased autophagy, and increased expression of cyclin-dependent kinase p27Kip1. Quiescence is essential for wound healing, organ regeneration, and preventing neoplasia. Previous findings indicate that microRNAs (miRNAs) play an important role in regulating cellular quiescence. Our recent publication demonstrated the existence of an alternative miRNA biogenesis pathway in primary human foreskin fibroblast (HFF) cells during quiescence. Indeed, we have identified a group of pri-miRNAs (whose mature miRNAs were found induced during quiescence) modified with a 2,2,7-trimethylguanosine (TMG)-cap by the trimethylguanosine synthase 1 (TGS1) protein and transported to the cytoplasm ...
[摘要] 蜂窝静止(因此已知为G <子> 0 骤停)是由降低的DNA复制,增加自噬表征,并且增加的细胞周期蛋白依赖性激酶p27蛋白上标kip1 表达。静止对伤口愈合,器官再生和瘤形成是必不可少的。先前的发现表明微小RNA(miRNA)在调节细胞静止过程中起重要作用。我们最近的出版物静止期间以实例阐述在原代人替代miRNA生物途径包皮成纤维(HFF)细胞的存在。实际上,我们已经发现了一组与由trimethylguanosine合酶1(TGS1)蛋白的2,2,7- trimethylguanosine(TMG)带肩改性PRI-的miRNA(其成熟miRNA发现静止期期间诱导的)的并运输到细胞质通过Exportin-1(XPO1)蛋白质。我们用来抗体针对(TMG)兴趣盖(不与第(m交叉反应 7 G)兴趣帽了大部分PRI-的miRNA或mRNA的含有[鲁曼等人的,1982]),以从增殖或静态HFFS的总RNA提取RNA进行免疫沉淀。该测定的新颖性是PRI-miRNA的以及含有一个TMG-帽修改以外的非编码RNA的特异性分离。
【背景】蜂窝静止,类型可逆生长停滞的,是在伤口愈合,器官再生,和预防瘤形成涉及一种重要的细胞状态(科勒,2011;瓦尔古等人 2012)。已发现小的非编码RNA如miRNA参与细胞静止的调节。 ...
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| ACE-score-based Analysis of Temporal miRNA Targetomes During Human Cytomegalovirus Infection Using AGO-CLIP-seq
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Author:
Date:
2016-04-20
[Abstract] Although temporal regulation of gene expression during the course of infection is known to be critical for determining the outcome of host-virus interactions, systematic temporal analysis of the miRNA targetomes during productive viral infection has been technically challenging due to the large range of miRNA-mRNA cross-talks at the host-virus interface. High-confidence quantifying models of the suppression efficacy in targeting sites by integrating bioinformatics with Argonaute-crosslinking and immunoprecipitation followed by high-throughput sequencing (AGO-CLIP-seq) (Chi et al., 2009) data have been poorly developed. To accurately identify miRNA target sites and calculate the targeting efficacy of miRNA-target interactions, we developed a new bioinformatic quantitation method, ...
[摘要] 尽管已知在感染过程中基因表达的时间调节对于确定宿主 - 病毒相互作用的结果是至关重要的,但是在生产性病毒感染期间对miRNA targetomes的系统时间分析在技术上是具有挑战性的,因为大范围的miRNA- mRNA在主机 - 病毒接口交叉对话。数据通过将生物信息学与Argonaute-交联和免疫沉淀接着高通量测序(AGO-CLIP-seq)数据(Chi等人,2009)数据结合,已经不发达。为了准确地鉴定miRNA靶位点并计算miRNA-靶相互作用的靶向效果,我们开发了新的生物信息学定量方法,即AGO-CLIP-seq富集(ACE) - 评分算法(Kim等, 2015)。在我们的AGO-CLIP-seq分析中包括未感染的对照可以显着提高病毒或人miRNA的真实靶位点识别的准确性,并且在我们的ACE评分方法中提取生产性人巨细胞病毒(HCMV)感染期间的生理学显着变化。因此,我们建议我们新的基于ACE评分的方法可以应用于各种miRNA targetome研究,这将在其他类型的时间背景下进行,如发展阶段,细胞因子或病原体的免疫刺激和其他病毒。
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