雏鸡不同组织TLR3、TLR7和TLR21 mRNA转录水平研究

参考GenBank登录的ChTLRs基因序列设计实时定量PCR特异性引物,建立检测鸡T011样受体（ChTLR）mRNA相对转录水平的实时定量PCR方法,分析ChTLR3、ChTLR7和ChTLR21在雏鸡不同器官组织中的转录水平。3种ChTLRs在脾脏、法氏囊、胸腺和各段肠道组织中均有转录。其中,ChTLR3 mRNA在肾脏、胸腺、盲肠、空肠、肝脏和十二指肠转录水平较高,在皮肤中未检测到转录;chTLR7 mRNA在脾脏、肾脏、盲肠、胸腺和十二指肠转录水平较高,在肝脏和皮肤中转录水平很低;ChTLR21 mRNA在所检测组织中均有转录,其中在脾脏转录水平最高,其次为法氏囊、胸腺和十二指肠。结果表明,ChTLRs mRNA在雏鸡各器官组织中转录水平差异较大,可能与雏鸡各器官组织对病原的识别和抵抗能力有关。     

Differential expression of Toll-like receptor mRNA in White Leghorn and indigenous chicken of India

In the present experiment, the expression profile of Toll-like receptor mRNA in indigenous and pure line chickens was studied. The expression of TLR3, TLR4, TLR5 and TLR7 were quantified in heterophils of Aseel, Kadaknath, Naked neck, Dwarf and White Leghorn lines by Quantitative Real-time PCR. White Leghorns expressed significantly (P < 0.01) higher levels of TLR3 mRNA compared to other lines. TLR4 and TLR5 mRNA were significantly highly expressed in Kadaknath line. Among the TLRs investigated TLR5 was more expressed in all lines studied. TLR7 was highly expressed in indigenous chicken Aseel and Kadaknath than other lines. Dwarf chicken expressed significantly (P < 0.01) lower levels of all TLRs investigated. On the basis of the present study we conclude that the differential expression of TLR mRNA in the heterophils of indigenous and other chicken breeds might contribute to their variable disease resistance/susceptibility.     

胰岛素受体mRNA在新生犊牛组织中的表达

应用半定量RT-PCR方法检测了新生犊牛中枢神经系统和外周组织中胰岛素受体（insulin receptor，InsR）基因的表达。结果表明，InsR基因在肝、皮下脂肪、半腱肌、胰、肾皮质、脾、心、肺、下丘脑、肠系膜淋巴结、主动脉、十二指肠、结肠、垂体、大脑皮质、小脑皮质中都有表达。其中，肝、半腱肌、下丘脑、胰、主动脉、垂体中InsR基因的表达量显著多于其他组织（P〈0．05）。InsR基因在各组织中的广泛分布表明胰岛素在体内具有广泛的生理功能。     

鸡干扰素受体基因在外周血淋巴细胞和组织中的表达

提取惠阳胡须鸡脾脏、胸腺、盲肠扁桃体、胸肌、肝脏、肾脏、心脏、未刺激的外周血淋巴细胞（PBL）和ConA刺激后的PBL的总RNA,采用RT-PCR的方法检测IFN-α/β受体α链（IFNAR1）、IFN-α/β受体β链（IFNAR2）和IFN-γ受体β链（IFNGR2）基因的表达情况.在未经刺激的PBL中未检测到IFNAR1、IFNAR2的表达,ConA刺激后的淋巴细胞中IFNAR1、IFNAR2的表达量比较高;在组织中,仅在脾脏、盲肠扁桃体、肝脏和胸腺中检测到了IFNAR1、IFNAR2的表达.在未刺激的PBL、ConA刺激后的PBL、脾脏、盲肠扁桃体、肝脏、胸腺、胸肌中均检测到了IFNGR2的表达,在肾脏和心脏中未检测到IFNGR2的表达.IFNAR1、IFNAR2、IFNGR2在刺激后的PBL、免疫器官和肝脏中分布,表明IFNAR1、IFNAR2、IFNGR2可能参与机体的免疫调节和肝脏的代谢过程.不同的干扰素受体在PBL和各组织中分布情况的差异可能与其各自功能的差异有关.     

Toll-like receptor expression in feline lymphoid tissues

Toll-like receptors (TLRs) are germline-encoded pattern recognition receptors (PRRs) that activate the innate immune system. While it is clear that TLRs are important in the immune response against pathogens, they may also be exploited by some pathogens. Our objective is to determine whether feline immunodeficiency virus (FIV) infection affects TLR expression or function thereby resulting in innate immune dysfunction. To this end, we cloned partial sequences for feline TLRs 1--3, 5--8, and developed real-time PCR assays to quantify feline TLRs 1--9. TLR expression was quantified in normal cat lymphoid tissues, purified lymphocyte subsets, and FIV-infected cell lines. Different expression patterns of TLRs were found in spleen, mesenteric lymph node, retropharyngeal lymph node, thymus, intestinal intraepithelial lymphocytes, and lamina propria lymphocytes. B lymphocytes, CD4+ T cells, and CD8+ T cells all expressed TLRs 2--5, 7--9; however, the relative levels of expression varied among lymphocyte phenotypes. Infection of cell lines with FIV resulted in altered TLR expression levels that differed depending on cell type. These results demonstrate that tissue distribution of TLRs is associated with the immunological role of a particular tissue, that lymphocytes may also express these 'innate immune' receptors, and that FIV infection can alter TLR expression.     

Expression profiles of antiviral response genes in chicken bursal cells stimulated with Toll-like receptor ligands

Cells of the adaptive immune system express Toll-like receptors (TLRs) and are able to respond to TLR ligands. With this in mind, the goal of the current study was to determine the expression of antiviral response genes in the cells of the chicken bursa of Fabricius (BF) to stimulation with TLR ligands. We investigated initially the response of bursal B cells to CpG-ODN, lipopolysaccharide (LPS) and poly(I:C) treatment. The expression level of type I interferons (IFNs) and interferon regulatory factor 7 (IRF7) did not differ between CpG-ODN and LPS treated groups compared to the non-stimulated cells. Poly(I:C) was the only TLR ligand, which has induced significant expression of antiviral innate immune response genes from bursal cells. Further in vitro and in vivo studies need to examine the efficacy of these antiviral responses against avian viruses.     

Expression of toll-like receptor 2 (TLR2) in porcine leukocyte subsets and tissues

Toll-like receptors (TLR) are a group of pattern recognition molecules that play a crucial role in innate immunity. TLR2 recognises a variety of microbial components leading to the development of inflammatory and immune responses. To characterise the expression and functional properties of porcine TLR2 (pTLR2), we have raised a panel of monoclonal antibodies (mAb) against this molecule. Mouse 3T3 cell transfectants expressing pTLR2 were used for immunisation of mice. The specificity of these antibodies was confirmed by their reactivity with CHO cells transfected with pTLR2 but not with pTLR4 or with non-transfected cells. Using one of these mAbs, named 1H11, pTLR2 was found on cells of the innate immune system, including monocytes, macrophages, and granulocytes, but not on peripheral blood lymphocytes. Staining of tissue sections showed that pTLR2 is also expressed on epithelial cells lining the tracheobronchial and intestinal tracts, bile ducts in the liver and renal tubules, and on the basal layer of the epidermis. This distribution is consistent with a surveillance function at entry sites, allowing for early detection of microbial invasion.     

鸡Toll样受体的研究进展

Toll样受体是进化保守的模式识别受体家族成员之一,介导天然免疫反应,通过识别病原体相关分子模式激活信号转导途径,引起炎性因子、趋化因子以及共刺激分子等表达,产生快速免疫应答。禽类与哺乳动物的Toll样受体具有同源性,但是也存在一定的差异性。目前,已经发现10种鸡Toll样受体,在天然免疫中发挥不同的作用,并且鸡Toll样受体配体具有作为疫苗佐剂的潜力。本文主要是对鸡Toll样受体的结构、信号转导通路和鸡Toll样受体在天然免疫中的作用进行综述。     

鸡褪黑激素受体基因在开产前后不同组织中的表达差异

为了从分子水平上了解鸡褪黑激素受体（MTNR）基因在开产前后不同组织中的表达差异,以β-actin基因为内标基因,运用实时荧光定量PCR方法,比较了MTNR1A、MTNR1B和MTNR1C这3个受体基因在心脏、肝脏、输卵管、卵巢、脑和视交叉各组织及在鸡开产前后表达量的差异。结果表明,MTNR1A只在开产后各组织中的表达量存在差异,其中以卵巢组织表达量最高,心脏中表达量最低。MTNR1B和MTNR1C的表达量在开产前或开产后均表现出组织间的显著差异;在开产前后的各组织中,MTNR1B的表达量均以视交叉为最高,卵巢为最低;而MTNR1C的表达量在开产前以心脏中最高,开产后在视交叉中最高,在卵巢组织中的表达量开产前后均为最低。同一组织开产后与开产前比较,MTNR1C基因在心脏、输卵管和脑组织中的表达量呈显著下调趋势。因此,3个受体基因在鸡的不同组织和生理时期存在表达差异。     

蒙古马不同组织器官TLR1、TLR2、TLR4和TLR6 mRNA转录水平研究

根据GenBank中马Toll样受体基因序列设计特异性引物,建立检测马Toll样受体（TLRs）mRNA转录水平的SYBR GreenⅠ实时荧光定量PCR方法,检测TLR4、TLR2、TLR1和TLR6在蒙古马不同组织器官中的转录水平。4种TLRs在心脏、肝脏、脾脏、肺脏、肾脏、胃、十二指肠、空肠、盲肠和骨髓中均有转录。其中,TLR4mRNA除在空肠和肝脏外,在其他组织器官中的表达水平均高于TLR2、TLR1、TLR6。免疫器官中,TLR4、TLR1mRNA在骨髓中表达量高于脾脏,而TLR2、TLR6mRNA在脾脏中表达量高于骨髓。各肠段,TLR4、TLR2、TLR1、TLR6mRNA表达水平之间在空肠的差异不是很大,而在十二指肠和盲肠中差异很大。结果表明,TLRs mRNA在马各组织器官转录水平差异较大,可能与其对病原体的识别和抵抗能力有关。     

Expression and functional analysis of chemokine receptor 7 in canine lymphoma cell lines

C-C chemokine receptor 7 (CCR7) contributes to cell homing to lymph nodes (LNs). Recent studies reported that CCR7 is also expressed in tumor cells, which correlates with LN metastasis in various cancers. However, the expression of CCR7 in tumor cells is unknown in dogs due to the lack of appropriate antibodies. In the present study, a fusion protein of C-C chemokine ligand 19 (CCL19) was employed as an alternative method to CCR7 antibodies. The fusion CCL19 protein specifically detected CCR7 expressed in canine lymphoma cell lines, which showed active chemotaxis to both canine and mouse ligands. The present study will help further research on the involvement of canine CCR7 in LN metastasis.     

Cloning of canine Toll-like receptor 7 gene and its expression in dog tissues

Toll-like receptor 7 (TLR7) is activated by single strand RNA and imidazoquinoline compounds, and induces interferon production. In this study, canine TLR7 cDNA was cloned and sequenced. The full-length cDNA of canine TLR7 gene was 3419bp, encoding 1032 amino acids. The similarities of canine TLR7 with human and mouse TLR7 were 84 and 80% at the nucleotide sequence level, and 86 and 79% at amino acid sequence level, respectively. Further, the expression of TLR7 mRNA was investigated in canine normal tissues by semiquantitative RT-PCR analysis. The common expression level of TLR7 mRNA in tissues from three dogs examined was in large intestine, lung, pancreas, small intestine and skin, though the expression level in each tissue was varied among these healthy dogs. In other tissues (kidney, liver, lymph node, spleen, adrenal gland, and PBMCs), the level of TLR7 mRNA expression was different in individuals.     

Expression and function of Toll-like receptor 2 in canine blood phagocytes

Toll-like receptors (TLRs) are a family of highly conserved pattern recognition receptors (PRR) of mammals that participate in the activation of innate immune responses against microbial infections. Among these receptors, TLR2 is essential for the recognition of conserved structural components of bacteria, protozoa and fungi. Until now, expression of TLR2 in dogs has not been investigated. In this work we describe a partial sequence of the gene coding for canine TLR2 and show that TLR2 mRNA is constitutively expressed in canine blood PMNs. We also show that stimulation of purified PMNs with lipoteichoic acid (LTA), a ligand of TLR2, leads to the release of proinflammatory chemokine IL-8. Furthermore, TLR2 protein is easily detectable by flow cytometry on the canine peripheral blood granulocyte and monocyte cell surface, and slightly on lymphocytes. These findings suggest that, also in dogs as in humans the initial antibacterial response of PMNs could be elicited through engagement of TLR2.     

荧光定量RT-PCR检测雏鸡感染NDV强毒后胸腺和法氏囊中TLR2与TLR4 mRNA的表达

Toll样受体2(TLR2)和Toll样受体4(TLR4)在识别病原微生物过程中发挥重要作用。为了定量检测TLR2、TLR4 mRNA表达水平,研究病原与机体的相互作用,本研究建立了检测鸡TLR2、TLR4 mRNA表达水平的SYBR GreenⅠ荧光定量RT-PCR(RRT-PCR)方法,检测了新城疫病毒强毒(vNDV)感染SPF雏鸡后36h、48h时胸腺、法氏囊中TLR2、TLR4 mRNA表达量变化。结果显示该方法特异性好,RRT-PCR产物分别在85.5℃、83.3℃出现单特异峰,对TLR2、TLR4的扩增效率分别为105.91%和95.30%,相关系数分别为0.9980、0.9996,最低检测限分别为108拷贝/反应和461拷贝/反应。感染后36h vNDV显著抑制TLR2、TLR4基因在法氏囊、胸腺中的表达;感染后48h时,法氏囊、胸腺中TLR2基因的表达水平显著升高,胸腺中TLR4基因的表达显著升高,而法氏囊中TLR4基因的表达仍处于抑制状态。本研究证明TLR2和TLR4参与了鸡体对NDV的感染应答。     

Expression of SOCS1-7 and CIS mRNA in porcine tissues

The Suppressor Of Cytokine Signaling (SOCS) proteins are key physiological regulators of the immune system. Little is known about tissue expression of SOCS and data in pigs are extremely scarce. In order to further study SOCS in pigs, preliminary data must be collected. In the current report, we first identified the three most suitable reference genes in ten porcine tissues. The beta-2-microglobulin (B2MI) reference gene was most often particularly suitable in our conditions. Then, using three reference genes we determined the mRNA expression of SOCS1-7 and CIS in every selected tissue. Constitutive mRNA expression was identified for all the members of the SOCS family in the ten tissues. Interestingly, the constitutive mRNA expression of SOCS1, SOCS3, SOCS7 and CIS was rather heterogeneous between tissues while for SOCS2, SOCS4, SOCS5 and SOCS6 differences of expression were less obvious. Highest CIS and SOCS mRNA expressions were observed in large intestine (SOCS1, SOCS3, SOCS4, SOCS6, and CIS), small intestine (SOCS1, SOCS4, SOCS6, and CIS), spleen (SOCS2, SOCS3, SOCS5, SOCS7, and CIS), trachea (SOCS3) and thymus (SOCS1, SOCS2, SOCS4, SOCS7, and CIS). These data will help for further studies about the role of SOCS proteins in the control of porcine innate and adaptive responses.     

SIGIRR对奶牛乳腺上皮细胞TLR4致炎信号通路的负调控作用

旨在探究SIGIRR对奶牛乳腺上皮细胞(BMECs)TLR4信号通路的负调控作用。构建SIGIRR-pEGFP真核表达载体,脂质体法转染HEK293T及BMECs,荧光显微镜观察及Western blot验证融合蛋白SIGIRR-pEGFP的表达;LPS刺激转染后BMECs,检测TLR4及其信号通路分子IRAK1、IRAK4和TRAF6的变化,以及下游炎性因子IL-6、IL-8、IL-1β和TNF-α的表达量。结果显示,成功构建SIGIRR-pEGFP真核表达载体,荧光检测重组质粒转染到HEK293T和BMECs中;Western blot鉴定融合蛋白SIGIRR-pEGFP表达正确;重组质粒转染BMECs后,SIGIRR表达量较转染空载质粒组及空白未转染组显著升高(P0.01);炎性因子IL-6、IL-8、IL-1β、TNF-α、TLR4及下游信号分子IRAK1、IRAK4、TRAF6表达量显著降低(P0.01),转染空载质粒组与空白未转染组相比仅IRAK1表达量有差异(P0.05)。结果表明,本试验通过研究牛SIGIRR在BMECs中的作用,证实SIGIRR基因具有炎性负调控LPS-TLR4信号通路的作用,具有潜力成为临床治疗奶牛乳腺炎的新靶标。     

Long form leptin receptor mRNA expression in the brain, pituitary, and other tissues in the pig

Much effort has focused recently on understanding the role of leptin, the obese gene product secreted by adipocytes, in regulating growth and reproduction in rodents, humans and domestic animals. We previously demonstrated that leptin inhibited feed intake and stimulated growth hormone (GH) and luteinizing hormone (LH) secretion in the pig. This study was conducted to determine the location of long form leptin receptor (Ob-Rl) mRNA in various tissues of the pig. The leptin receptor has several splice variants in the human and mouse, but Ob-Rl is the major form capable of signal transduction. The Ob-Rl is expressed primarily in the hypothalamus of the human and rodents, but has been located in other tissues as well. In the present study, a partial porcine Ob-Rl cDNA, cloned in our laboratory and specific to the intracellular domain, was used to evaluate the Ob-Rl mRNA expression by RT-PCR in the brain and other tissues in three 105 d-old prepuberal gilts and in a 50 d-old fetus. In 105 d-old gilts, Ob-Rl mRNA was expressed in the hypothalamus, cerebral cortex, amygdala, thalamus, cerebellum, area postrema and anterior pituitary. In addition, Ob-Rl mRNA was expressed in ovary, uterine body, liver, kidney, pancreas, adrenal gland, heart, spleen, lung, intestine, bone marrow, muscle and adipose tissue. However, expression was absent in the thyroid, thymus, superior vena cava, aorta, spinal cord, uterine horn and oviduct. In the 50 d-old fetus, Ob-Rl mRNA was expressed in brain, intestine, muscle, fat, heart, liver and umbilical cord. These results support the idea that leptin might play a role in regulating numerous physiological functions.