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应用实时 PCR 技术对鹌鹑脾细胞中干扰素、白细胞介素和 Toll 样受体 7 mRNA 的定量检测。

Quantification of interferon, interleukin, and Toll-like receptor 7 mRNA in quail splenocytes using real-time PCR.

机构信息

Department of Veterinary Medicine, Tottori University, Tottori, Japan.

出版信息

Poult Sci. 2012 Oct;91(10):2496-501. doi: 10.3382/ps.2012-02283.

Abstract

Japanese quail (Coturnix japonica) are farmed worldwide as poultry. Quail have been used as experimental animals in various scientific fields, but their immunological characteristics have not been well characterized. In this study, to develop a method for analyzing the innate immune response of quail to infectious pathogens, we determined the nucleotide sequences of major interleukins (IL) and Toll-like receptor (TLR)-7 of quail and developed quantitative real-time PCR assays. The nucleotide sequences of quail IL-1β, IL-4, IL-6, IL-8, IL-10, IL-12a, IL-12b, IL-13, IL-18, and TLR-7 were determined based on the sequences of the chicken genes. Specific primers for each of these genes and previously reported interferon (IFN)-α, IFN-γ, and IL-2 genes were designed for quantitative real-time PCR. Standard curves for quantification were established using serial dilutions of external standard plasmids containing real-time PCR products. Then, real-time PCR was performed to monitor the kinetics of quail immune-related gene expression induced in splenocytes stimulated with concanavalin A. After amplification, the r(2) values of the standard curves for all target genes were above 0.980. Melting analysis of real-time PCR revealed specific amplification of each gene that could be visualized clearly as a single peak of melting temperature in a melt peak chart. These data show that the mRNA expressions of quail immune-related genes can be accurately quantified using this real-time PCR assay. In this study, we showed the nucleotide sequences of several quail cytokine mRNA and constructed the quantitative real-time PCR for quail immune-related genes.

摘要

日本鹌鹑(Coturnix japonica)在世界各地被作为家禽养殖。鹌鹑已被用于各种科学领域的实验动物,但它们的免疫学特性尚未得到很好的描述。在这项研究中,为了开发一种分析鹌鹑对传染性病原体固有免疫反应的方法,我们确定了鹌鹑主要白细胞介素(IL)和 Toll 样受体(TLR)-7 的核苷酸序列,并开发了定量实时 PCR 检测。根据鸡基因的序列,确定了鹌鹑 IL-1β、IL-4、IL-6、IL-8、IL-10、IL-12a、IL-12b、IL-13、IL-18 和 TLR-7 的核苷酸序列。为每个基因设计了特异性引物,并报道了干扰素(IFN)-α、IFN-γ 和 IL-2 基因。使用包含实时 PCR 产物的外部标准质粒的系列稀释液建立定量标准曲线。然后,通过用刀豆蛋白 A 刺激脾细胞来监测鹌鹑免疫相关基因表达的动力学,进行实时 PCR。扩增后,所有靶基因标准曲线的 r(2)值均高于 0.980。实时 PCR 的熔解分析显示了每个基因的特异性扩增,在熔解峰图中可以清楚地看到作为单一峰的熔解温度。这些数据表明,使用这种实时 PCR 检测可以准确地定量鹌鹑免疫相关基因的 mRNA 表达。在这项研究中,我们展示了几种鹌鹑细胞因子 mRNA 的核苷酸序列,并构建了用于定量检测鹌鹑免疫相关基因的实时 PCR。

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