Sonawane Ganesh G, Tripathi Bhupendra Nath
Animal Health Division, Indian Council of Agricultural Research-Central Sheep and Wool Research Institute, Avikanagar, Malpura, District Tonk-304501, Rajasthan, India.
Indian Council of Agricultural Research-National Research Centre on Equines, Hisar, Haryana, India.
Int J Mycobacteriol. 2016 Dec;5 Suppl 1:S77-S78. doi: 10.1016/j.ijmyco.2016.09.042. Epub 2016 Nov 11.
OBJECTIVE/BACKGROUND: Paratuberculosis (Johne's disease) is a chronic infectious granulomatous enteritis, primarily affecting ruminants, and caused by Mycobacterium avium ssp. paratuberculosis (MAP). The disease is widely prevalent throughout the world with significant economic losses. MAP has also been implicated with human Crohn's disease. There exists a strong correlation between the immune response and development of various types of pathologies in ruminants. The polarization of the immune response, which is critical to clinical outcome of the paratuberculosis infection, is controlled by the differential expression of certain cytokines and inducible nitric oxide synthase (iNOS) in Johne's disease. In previous studies, the role of different cytokines (Th1 and Th2) has been occasionally studied in sheep paratuberculosis. In the present study, we studied differential expression of interferon (IFN)-γ, interleukin (IL)-1α, IL-10, transforming growth factor (TGF)-β, iNOS, and TRAF1 genes in MAP-infected sheep and established relationship with distinct pathologies.
Tissue sections (small intestine, ileocecal junction, and mesenteric lymph nodes) were collected from sheep suspected for Johne's disease and appropriately preserved for RNA extraction, polymerase chain reaction (PCR) analysis, and histopathology. Pathologic grading was done on the basis of nature and extent of cellular infiltration, granuloma formation and abundance of acid-fast bacilli. Six sheep each with pauci (PB)- and multibacillary (MB) lesions and six healthy control sheep were selected for cytokine studies. MAP in tissue extracted genomic DNA of sheep was quantified by a quantitative PCR assay. Tissue extracted RNA was reversed transcribed to prepare c-DNA from which quantitative reverse transcription PCR (qRT-PCR) was performed to amplify IFN-γ, IL-1β, IL-10, TGF-β, β-actin, TRAF1, and iNOS with Quantitect SYBR Green Master Mix. qRT-PCR data were analyzed using 2 method using β-actin gene as a control. All qRT-PCR results were compared by using one-way analysis of variance (least significance difference and Duncan tests) for p-value using SPSS (version 7.5) for expression of each gene in tissues from infected and control sheep.
In the small intestine, PB sheep showed significant enhancements in the expression of IL-10, TGF-β, iNOS, and IFN-γ in comparison to similar tissues from uninfected control sheep. IL-1α expression was significantly reduced (p<0.01). The expression of IL-10 in the mesenteric lymph node (MLN) tissue of PB sheep was significantly increased (p<0.01) as compared with the control sheep. MB sheep revealed significantly enhanced expression of TGF-β mRNA and reduction in the expression of IL-1α in comparison to control sheep. In the MLN of MB sheep, the expressions of IL-10 and TGF-β were significantly (p<0.01) increased, and IFN-γ was significantly downregulated in comparison to uninfected control sheep. When the cytokine expression was compared between two distinctly infected groups, the MB sheep showed highly significant decrease (p<0.01) in the expression of iNOS and IFN-γ in the small intestine and IFN-γ in the MLN tissues.
The present study indicated that IFN-γ and iNOS were found to play important role in the induction of Th1 type immune response in PB sheep. MB sheep had significant reduction in expression of IFN-γ and iNOS and elevation of IL-10 and TGF-β, which was typical of Th2 cytokine pattern. Elevated expression of IL-10 and TGF-β in PB cases possibly suggests the role of T-regulatory cells and may follow an independent mechanism not typical of Th1 pattern. In view of significantly reduced expression in both forms of the disease, IL-1α may not be an important cytokine in ovine paratuberculosis.
目的/背景:副结核病(约翰氏病)是一种慢性感染性肉芽肿性肠炎,主要影响反刍动物,由副结核分枝杆菌(MAP)引起。该病在全球广泛流行,造成重大经济损失。MAP也与人类克罗恩病有关。反刍动物的免疫反应与各种病理类型的发展之间存在很强的相关性。免疫反应的极化对副结核病感染的临床结果至关重要,它由约翰氏病中某些细胞因子和诱导型一氧化氮合酶(iNOS)的差异表达控制。在先前的研究中,不同细胞因子(Th1和Th2)在绵羊副结核病中的作用偶尔被研究。在本研究中,我们研究了MAP感染绵羊中干扰素(IFN)-γ、白细胞介素(IL)-1α、IL-10、转化生长因子(TGF)-β、iNOS和TRAF1基因的差异表达,并建立了与不同病理的关系。
从疑似患有约翰氏病的绵羊收集组织切片(小肠、回盲交界处和肠系膜淋巴结),并妥善保存用于RNA提取、聚合酶链反应(PCR)分析和组织病理学检查。根据细胞浸润的性质和程度、肉芽肿形成以及抗酸杆菌的丰度进行病理分级。选择6只患有少菌(PB)和多菌(MB)病变的绵羊以及6只健康对照绵羊进行细胞因子研究。通过定量PCR测定法对绵羊组织提取的基因组DNA中的MAP进行定量。将组织提取的RNA逆转录以制备cDNA,然后使用Quantitect SYBR Green Master Mix进行定量逆转录PCR(qRT-PCR)以扩增IFN-γ、IL-1β、IL-10、TGF-β、β-肌动蛋白、TRAF1和iNOS。使用2−ΔΔCT方法以β-肌动蛋白基因为对照分析qRT-PCR数据。使用单因素方差分析(最小显著差异和邓肯检验)通过SPSS(7.5版)比较所有qRT-PCR结果,以确定感染和对照绵羊组织中每个基因表达的p值。
在小肠中,与未感染对照绵羊的相似组织相比,PB绵羊的IL-10、TGF-β、iNOS和IFN-γ表达显著增强。IL-1α表达显著降低(p<0.01)。与对照绵羊相比,PB绵羊肠系膜淋巴结(MLN)组织中IL-10的表达显著增加(p<0.01)。与对照绵羊相比,MB绵羊的TGF-β mRNA表达显著增强,IL-1α表达降低。在MB绵羊的MLN中,与未感染对照绵羊相比,IL-10和TGF-β的表达显著(p<0.01)增加,IFN-γ显著下调。当比较两个明显感染组之间的细胞因子表达时,MB绵羊小肠中iNOS和IFN-γ的表达以及MLN组织中IFN-γ的表达显著降低(p<0.01)。
本研究表明,IFN-γ和iNOS在PB绵羊Th1型免疫反应的诱导中起重要作用。MB绵羊的IFN-γ和iNOS表达显著降低,IL-10和TGF-β升高,这是Th2细胞因子模式的典型特征。PB病例中IL-10和TGF-β的表达升高可能表明T调节细胞的作用,并且可能遵循一种不同于Th1模式的独立机制。鉴于两种疾病形式中IL-1α的表达均显著降低,IL-1α可能不是绵羊副结核病中的重要细胞因子。
