Harrington Noel P, Surujballi Om P, Prescott John F
Canadian Food Inspection Agency, Ottawa Laboratory Fallowfield, Ottawa, Ontario, K2H 8P9, Canada.
J Wildl Dis. 2006 Apr;42(2):219-33. doi: 10.7589/0090-3558-42.2.219.
It has been difficult to perform cytokine studies for many wildlife and nontraditional species because of a lack of immunologic reagents at the protein level. Recently, simple and rapid assays for quantifying mRNA expression by real-time reverse transcription-polymerase chain reaction (RT-PCR) have been used for analysis of cytokine profiles in humans and other mammalian species. This report describes the development and application of real time RT-PCR to measure the expression of several important elk (Cervus elaphus) cytokine mRNAs, including interleukin (IL)-2, IL-4, IL-10, IL-12p40, interferon-gamma, tumor necrosis factor (TNF)-alpha, and the enzyme-inducible nitric oxide synthase, all of which are involved in immune responses and regulation. For the broadest potential application of the assay, primers and probes were designed using consensus sequences from several species of interest. To obtain standardized quantitative results, external controls consisting of a DNA template for each target gene were used to generate linear standard curves over a 6 to 8 log range with detection of as few as 10 copies of amplicon per reaction. Sample-to-sample variation in the efficiency of the RT, as well as in the quantity and quality of the starting RNA, was compensated for by normalizing the results to the endogenous housekeeping gene beta(2)-microglobulin. The assay was evaluated by monitoring the kinetics of cytokine mRNA synthesis induced by mitogenic and antigenic stimulation of peripheral blood mononuclear cells (PBMCs) from Mycobacterium bovis-infected elk. Concanavalin A-stimulated PBMCs demonstrated a rapid but transient increase in cytokine mRNA expression following in vitro mitogenic activation with optimal mRNA induction observed after 4 to 16 hr. The PBMCs stimulated with the mycobacterial recall antigen, bovine-purified protein derivative (PPD-bovis), demonstrated variable mRNA induction kinetics for each cytokine. Whereas PPD-bovis optimally induced IL-2 mRNA after 8 hr of in vitro stimulation, longer in vitro stimulation times were necessary for the optimal induction of IL-4 and TNF-alpha mRNA (up to 48 hr). We demonstrate real-time RT-PCR to be a rapid, sensitive, and reproducible technique, which will make it a valuable tool in the study of immunologic responses and cytokine profiles of cervids and other nontraditional livestock and wildlife species.
由于缺乏蛋白质水平的免疫试剂,对许多野生动物和非传统物种进行细胞因子研究一直很困难。最近,通过实时逆转录-聚合酶链反应(RT-PCR)定量mRNA表达的简单快速检测方法已被用于分析人类和其他哺乳动物物种的细胞因子谱。本报告描述了实时RT-PCR的开发和应用,以测量几种重要的麋鹿(Cervus elaphus)细胞因子mRNA的表达,包括白细胞介素(IL)-2、IL-4、IL-10、IL-12p40、干扰素-γ、肿瘤坏死因子(TNF)-α和酶诱导型一氧化氮合酶,所有这些都参与免疫反应和调节。为了使该检测方法具有最广泛的潜在应用,使用来自几种目标物种的共有序列设计引物和探针。为了获得标准化的定量结果,使用由每个靶基因的DNA模板组成的外部对照在6至8个对数范围内生成线性标准曲线,每个反应检测低至10个拷贝的扩增子。通过将结果与内源性管家基因β2-微球蛋白进行归一化,补偿了RT效率以及起始RNA的数量和质量在样本间的差异。通过监测牛分枝杆菌感染的麋鹿外周血单核细胞(PBMC)的有丝分裂原和抗原刺激诱导的细胞因子mRNA合成动力学来评估该检测方法。伴刀豆球蛋白A刺激的PBMC在体外有丝分裂原激活后,细胞因子mRNA表达迅速但短暂增加,在4至16小时后观察到最佳mRNA诱导。用分枝杆菌回忆抗原牛纯化蛋白衍生物(PPD-bovis)刺激的PBMC对每种细胞因子表现出可变的mRNA诱导动力学。虽然PPD-bovis在体外刺激8小时后最佳诱导IL-2 mRNA,但对于IL-4和TNF-α mRNA的最佳诱导需要更长的体外刺激时间(长达48小时)。我们证明实时RT-PCR是一种快速、灵敏且可重复的技术,这将使其成为研究鹿科动物以及其他非传统家畜和野生动物物种免疫反应和细胞因子谱的有价值工具。
