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双顺反子 IRES 报告基因使用的当前实践:系统评价。

Current Practice in Bicistronic IRES Reporter Use: A Systematic Review.

机构信息

Department of Orthopedic Surgery, Maastricht University, Medical Center+, 6229 ER Maastricht, The Netherlands.

Department of Experimental, Diagnostic and Specialty Medicine, Bologna University, I-40138 Bologna, Italy.

出版信息

Int J Mol Sci. 2021 May 14;22(10):5193. doi: 10.3390/ijms22105193.

Abstract

Bicistronic reporter assays have been instrumental for transgene expression, understanding of internal ribosomal entry site (IRES) translation, and identification of novel cap-independent translational elements (CITE). We observed a large methodological variability in the use of bicistronic reporter assays and data presentation or normalization procedures. Therefore, we systematically searched the literature for bicistronic IRES reporter studies and analyzed methodological details, data visualization, and normalization procedures. Two hundred fifty-seven publications were identified using our search strategy (published 1994-2020). Experimental studies on eukaryotic adherent cell systems and the cell-free translation assay were included for further analysis. We evaluated the following methodological details for 176 full text articles: the bicistronic reporter design, the cell line or type, transfection methods, and time point of analyses post-transfection. For the cell-free translation assay, we focused on methods of in vitro transcription, type of translation lysate, and incubation times and assay temperature. Data can be presented in multiple ways: raw data from individual cistrons, a ratio of the two, or fold changes thereof. In addition, many different control experiments have been suggested when studying IRES-mediated translation. In addition, many different normalization and control experiments have been suggested when studying IRES-mediated translation. Therefore, we also categorized and summarized their use. Our unbiased analyses provide a representative overview of bicistronic IRES reporter use. We identified parameters that were reported inconsistently or incompletely, which could hamper data reproduction and interpretation. On the basis of our analyses, we encourage adhering to a number of practices that should improve transparency of bicistronic reporter data presentation and improve methodological descriptions to facilitate data replication.

摘要

双顺反子报告基因检测在转基因表达、对内质网进入位点(IRES)翻译的理解以及新型帽非依赖性翻译元件(CITE)的鉴定中发挥了重要作用。我们观察到双顺反子报告基因检测在使用和数据呈现或归一化程序方面存在很大的方法学差异。因此,我们系统地搜索了双顺反子 IRES 报告基因研究的文献,并分析了方法学细节、数据可视化和归一化程序。使用我们的搜索策略确定了 257 篇出版物(发表于 1994 年至 2020 年)。将用于进一步分析的真核贴壁细胞系统和无细胞翻译测定的实验研究包括在内。我们评估了 176 篇全文文章的以下方法学细节:双顺反子报告基因设计、细胞系或类型、转染方法以及转染后分析的时间点。对于无细胞翻译测定,我们专注于体外转录方法、翻译裂解物类型以及孵育时间和测定温度。数据可以以多种方式呈现:来自两个顺式元件的原始数据、两者的比率或其倍数变化。此外,在研究 IRES 介导的翻译时,已经提出了许多不同的对照实验。此外,在研究 IRES 介导的翻译时,已经提出了许多不同的归一化和对照实验。因此,我们还对它们的使用进行了分类和总结。我们的无偏分析提供了双顺反子 IRES 报告基因检测使用的代表性概述。我们确定了报告不一致或不完整的参数,这可能会阻碍数据的再现和解释。基于我们的分析,我们鼓励遵守一些实践,这些实践应提高双顺反子报告基因数据呈现的透明度,并改进方法学描述,以促进数据复制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4b31/8156625/4e7861c6c39f/ijms-22-05193-g001.jpg

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