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定量实时 PCR 方法评估斑马鱼胚胎中的基因表达。

Quantitative Real-Time PCR Method to Evaluate Gene Expression in Zebrafish Embryos.

机构信息

Department of Biochemistry, Institute of Health Sciences, Marmara University, Istanbul, Turkey.

Department of Biochemistry, Faculty of Medicine, Istanbul Medipol University, Istanbul, Turkey.

出版信息

Methods Mol Biol. 2024;2753:553-561. doi: 10.1007/978-1-0716-3625-1_36.

Abstract

The fast zebrafish embryonic development offers an opportunity for the study of genes crucial for developmental processes. Several genes associated with human diseases have orthologs in zebrafish. Enhanced comprehension of a gene's function can be achieved by knowing when and where it is expressed. This knowledge also makes it possible to alter a gene-by-gene knockdown in a time- and place-specific manner. Moreover, gene expression analyses contribute greatly to teratogenicity studies in zebrafish embryos. Therefore, the importance of examining the differences between the expressions of these genes has increased day by day. The incorporation of reverse transcription (RT) as the initial step prior to thermal cycling in quantitative real-time polymerase chain reaction (RT-qPCR) has made a significant contribution to RNA research. RT-qPCR is the gold standard and an effective method for gene expression analysis. Quick readout, high sensitivity, reproducibility, as well as high potential throughput, along with reliable quantification, are just a few advantages of RT-qPCR. However, there are drawbacks to its application, such as RNA's inherent variability, impurities during RNA extraction, and variations in reverse transcription and PCR efficiencies. Implementing a precise normalization technique is crucial to account for these inaccuracies. In this chapter, the protocol for gene expression analysis by RT-qPCR for zebrafish embryos is explained.

摘要

快速的斑马鱼胚胎发育为研究对发育过程至关重要的基因提供了机会。几种与人类疾病相关的基因在斑马鱼中有同源基因。通过了解基因何时何地表达,可以更好地理解其功能。这一知识还使得以时间和空间特异性的方式逐个基因敲低成为可能。此外,基因表达分析对斑马鱼胚胎的致畸性研究有很大的贡献。因此,检查这些基因表达差异的重要性与日俱增。在定量实时聚合酶链反应 (RT-qPCR) 中,将逆转录 (RT) 作为热循环之前的初始步骤纳入其中,为 RNA 研究做出了重大贡献。RT-qPCR 是 RNA 研究的金标准和有效方法。快速读取、高灵敏度、重现性以及高潜在通量,以及可靠的定量,只是 RT-qPCR 的几个优点。然而,其应用也存在一些缺点,例如 RNA 的固有变异性、RNA 提取过程中的杂质以及逆转录和 PCR 效率的变化。实施精确的归一化技术对于纠正这些误差至关重要。本章介绍了用于斑马鱼胚胎基因表达分析的 RT-qPCR 方案。

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