共查询到20条相似文献,搜索用时 687 毫秒
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旨在研究MSTN和p21基因在鸡、鹌鹑和杂交禽胚胎肌肉发育过程中的表达规律,比较这2个基因在杂交禽与亲本鸡和鹌鹑中的差异表达,探讨MSTN和p21基因与肌肉发育的关系。通过人工受精获得鸡(♂)与鹌鹑(♀)杂交禽蛋,与鸡蛋、鹌鹑蛋按照鸡标准孵化条件同批入孵,采集第7~17天活胚胸肌组织,应用实时荧光定量PCR技术检测MSTN和p21基因在3个物种中每一天mRNA的相对表达量。MSTN和p21基因在胚胎肌肉发育的第7~17天均有表达,这2个基因mRNA的表达在鸡胚中第9天到达第1次峰值,在鹌鹑中第7天到达第1次峰值,后都随胚胎的发育表达水平上升,并维持相对稳定的高水平表达。杂交禽的表达规律与鸡一致,也在第9天达到峰值,而p21mRNA表达极显著高于鸡和鹌鹑(P<0.01)。MSTN mRNA表达规律与成肌细胞退出细胞周期的时间规律一致;在胚胎肌肉发育过程中,MSTN基因特异性上调p21的表达。 相似文献
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J M Sharma 《Veterinary immunology and immunopathology》1988,19(1):51-66
Spleen cells but not the thymus or the bursa cells of chicken embryos suppressed the in vitro mitogenesis of spleen cells of adult syngeneic or allogeneic chickens. The natural suppressor cell activity of embryo spleen was present at embryonation day 16, reached peak levels at embryonation day 18 and disappeared at hatch. The embryo spleen cells did not by themselves respond to phytohemagglutinin stimulation in vitro. The suppressive effect of embryonic spleen cells on adult spleen cells was present when the embryonic cells were added at the time of or after initiation of the adult spleen mitogenic cultures. When the embryonic cells were added to the cultures of adult spleen cells after the blastogenic response of the adult cells had peaked, the embryonic cells inhibited the incorporation of the label into adult spleen cell blasts. The suppressive activity of the embryonic spleen cells was mediated by soluble suppressor product(s) secreted by these cells, and direct cell-to-cell contact between embryonic and adult spleen cells was not necessary for suppression to occur. Infection of embryos with turkey herpesvirus and Marek's disease virus reduced the suppressor cell activity of embryonic spleen, although substantial residual suppressor cell activity remained in virus-infected embryos. Several pathogenic or non-pathogenic isolates of infectious bursal disease virus did not appreciably alter the suppressor cell activity of embryonic spleen cells. 相似文献
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Production and characterization of monoclonal antibodies against chicken lymphocyte surface antigens
T Kondo M Hattori H Kodama M Onuma T Mikami 《Nippon juigaku zasshi. The Japanese journal of veterinary science》1990,52(1):97-103
A panel of monoclonal antibodies (mAbs) with specificity for chicken lymphocyte surface antigens was established and characterized based on their reactivities against chicken lymphoid cells and tumor cell lines on flow cytometry. Three mAbs (7-3G-2, 7-2E-8, and JB-2) reacted preferentially with thymocytes, however, none of them reacted with Marek's disease derived T lymphoblastoid cell lines. Four mAbs (6-27A-1, 4-5C-5, Lc-4, and Lc-6) reacted with spleen cells and peripheral blood leukocytes as well as thymocytes. All seven mAbs reacted with chicken embryonic thymocytes from day 12 of embryonic life onward. All mAbs showed no reactivity against bursal lymphocytes. 相似文献
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鸡脾脏中B淋巴细胞的发育及其定位分布 总被引:1,自引:0,他引:1
应用IgM、IgG和IgA单克隆抗体的免疫组织化学方法,研究IgM+、IgG+和IgA+B淋巴细胞在鸡脾脏中的出现、迁移、数量变化规律等一系列的发育过程以及组织定位分布特点。结果显示,IgM+和IgA+细胞在胚胎15日龄时开始出现,IgG+细胞在胚胎18日龄时出现,21日龄雏鸡脾脏的红髓和生发中心中出现以IgG型为主的浆细胞。各日龄IgM+、IgG+和IgA+细胞主要分布在脾脏的特征性组织结构—椭球周围淋巴鞘和生发中心中,这些结构也随着B淋巴细胞的增多而不断发育成熟。B淋巴细胞的数量随着日龄增长持续增加,直至21日龄时趋于稳定,各日龄B淋巴细胞数量始终以IgG+细胞最多,IgM+细胞次之,IgA+细胞最少。结果表明,鸡出壳初期,脾脏的体液免疫功能逐渐增强,并在21日龄时达到成熟水平。 相似文献
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We examined the susceptibility of late-stage chicken embryos to infection with oncogenic serotype 1 Marek's disease virus (MDV 1). Intravenous inoculation of MDV 1 at embryonic day (ED) 16 resulted in significant replication of the virus in embryonic tissues. Within 5 days of virus exposure, pp38 viral antigen (pp38) was detected in embryonic bursae and MDV 1 was isolated by plaque assay from the spleens, thymuses, and bursae of embryos. The pathogenesis of MDV 1 after intravenous inoculation at ED 16 was similar to that in chicks exposed to MDV 1 after hatching. In contrast to the response of the embryo to intravenous inoculation, embryos exposed to MDV 1 by the amniotic route did not develop detectable pp38, nor could the virus be isolated from the embryonic tissues by plaque assay. These results show that the route of inoculation of MDV 1 in the embryos is critical for allowing the virus to come in contact with target cells. 相似文献
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通过免疫组织化学法,应用CD3、CD4和CD8单克隆抗体研究了CD3+T淋巴细胞及CD4+和CD8+T淋巴细胞亚群在鸡盲肠扁桃体中的出现、迁移、组织定位分布及数量变化规律等一系列发育过程。结果显示:CD3+、CD8+T淋巴细胞最初于11胚龄时出现,而CD4+T淋巴细胞在15胚龄时出现。在定位分布变化上,CD3+主要分布在黏膜上皮中,CD4+主要分布在黏膜固有层中,CD8+在黏膜固有层和黏膜上皮内都有大量分布。在数量变化上,1~7日龄雏鸡各种阳性细胞的数量都骤然增加;而到7日龄时,雏鸡CD3+淋巴细胞的数量明显减少,CD4+、CD8+T细胞的数量无明显变化;从21日龄开始直到35日龄,雏鸡CD3+、CD4+和CD8+T淋巴细胞的数量持续增加。试验证明,鸡在出壳后初期十二指肠的细胞免疫功能增强。 相似文献
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Regan DP Aarnio MC Davis WS Carmichael KP Vandenplas ML Lauderdale JD Moore PA 《Veterinary ophthalmology》2012,15(3):145-152
Objective Equine recurrent uveitis (ERU) is a spontaneous disease that is the most common cause of blindness in horses, affecting up to 15% of the horse population. Th17 cells are a major cell population driving the pathogenesis in several mouse models of autoimmune inflammation, including experimental autoimmune uveitis. The purpose of this study is to investigate the role a Th17 cell‐mediated response plays in the pathogenesis of ERU. Procedure Banked, Davidson’s‐fixed equine globes histopathologically diagnosed with ERU (n = 7) were compared immunohistochemically with healthy control globes (n = 7). Immunohistochemical staining was performed using a pan‐Leptospira antibody and antibodies against IL‐6, IL‐17, and IL‐23. Additionally, immunostaining was performed for T‐cell (CD3) and B‐cell (CD79α) markers. Specificity of immunoreactivity was confirmed by western blot analysis. Results Immunohistochemical staining was positive for IL‐6, IL‐17, and IL‐23 within the cytoplasm of nonpigmented ciliary epithelial cells and mononuclear inflammatory cells infiltrating the iris, and ciliary body of ERU horses (n = 7) but negative in controls (n = 7). ERU‐affected eyes were CD3 positive (n = 7) and CD79α negative (n = 7). Staining for Leptospira was negative in all ERU and control globes. Conclusions Strong immunoreactivity for IL‐6, IL‐17, and IL‐23, in conjunction with the fact that T lymphocytes are the predominating inflammatory cells present in ERU, suggests that IL‐17‐secreting helper T‐cells play a role in the pathogenesis of ERU. These findings suggest that horses with ERU may serve as a naturally occurring animal model for autoimmune uveitis. 相似文献
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Many species of erythrocytes were investigated for their ability to form spontaneous rosette with bovine peripheral blood leukocytes and fetal thymocytes. Only sheep and chicken red blood cells gave rosettes. Using conditions shown optimum for the demonstration of human rosette forming cells, only low numbers of bovine rosettes were demonstrable. By changing culture conditions to include 100% fetal calf serum, neuraminidase treated erythrocytes and/or lymphocytes and optimizing the incubation times and temperature, up to 38% of peripheral blood leukocytes and 52% of thymocytes formed rosettes. A thymic origin of rosetting cells was ascribed to T cells for the following reasons: 1) thymocytes gave higher numbers than did peripheral blood leukocytes, 2) rosette forming cell numbers were increased in peripheral blood leukocyte subpopulations enriched in T cells by nylon column separation and 3) only very few rosette forming cells had surface immunoglobulin, a marker of B lymphocytes. The reasons why all T cells were not detected by the technique were discussed. 相似文献
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Yoo J Chang HH Bae YH Seong CN Choe NH Lillehoj HS Park JH Min W 《Veterinary immunology and immunopathology》2008,121(3-4):359-363
Chicken interleukin-17 (chIL-17) gene was previously characterized through cloning from a chicken intestinal expressed sequence tag (EST) cDNA library. To further investigate the biological properties of chIL-17, six monoclonal antibodies (mAbs) against a bacterially expressed chIL-17 recombinant protein were produced and their binding specificities characterized. Antibodies which were initially selected on the basis of their specific binding reactivity with recombinant chIL-17 in ELISA were further characterized by Western blot analysis. Monoclonal antibodies specific for chIL-17 identified 20 and 21kDa protein bands in the culture supernatant and cell lysate of CU205 cells. These mAbs also recognized specific bands for chIL-17 in the cell lysate from conconavalin A (Con A)-activated, but not from normal splenic lymphocytes. Furthermore, these mAbs detected a 16kDa protein in the lysate of CU205 cells treated with tunicamycin and stained an intracellular protein in CU205 cells in flow cytometric analysis. Together, these results indicate that these new mAbs are specific for chIL-17 and will be a useful tool for structural and immunological studies of IL-17 in poultry. 相似文献
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以增强型绿色荧光蛋白(Enhanced green fluorescent protein,EGFP)为报告基因体外转染鸡胚胎精原细胞(Chicken embryonic spermatogonial cells,CESCs),比较磷酸钙、脂质体(梭华-Sofast)、电穿孔3种方法转染EGFP的效率,以获得高效的体外转染方法。本研究分离孵化16d的鸡胚睾丸,获取CESCs,体外培养和传代扩增,传至第2代后进行碱性磷酸酶(AKP)活性和阶段特异性表面抗原-1(Stage specific embryonic antigen-1,SSEA-1)免疫荧光鉴定。运用磷酸钙、脂质体(梭华-Sofast)、电穿孔3种方法体外转染第2代CESCs,荧光细胞计数法分析转染效率。结果表明:与磷酸钙法、脂质体法相比,电穿孔法可获得更高的细胞成活率和转染率(68% vs 39%、65%,19.70% vs 2.92%、9.73%),差异显著(P〈0.05)。因此得出,电穿孔法是将外源基因导入鸡胚精原细胞的适宜方法。 相似文献
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Evaluation of embryonic age and the effects of different proteases on the isolation and primary culture of chicken intestinal epithelial cells in vitro 
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下载免费PDF全文 Chao Yuan Qiang He Jun‐ming Li Mahmoud Mostafa Azzam Jian‐jun Lu Xiao‐ting Zou 《Animal Science Journal》2015,86(6):588-594
The present study evaluates the effects of embryonic age and proteolytic enzymes on the isolation and primary culture of chicken enterocyte and to establish an effective technique for chicken intestinal epithelial cell (IEC) cultivation. Fourteen‐day‐old, 16‐day‐old and 18‐day‐old embryos (average weight: 52.23 ± 0.76 g, 50.86 ± 0.99 g, 48.98 ± 1.03 g) were the source for preparation of enterocyte culture, and trypsin‐ethylene diamine tetraacetic acid, collagenase, thermolysin and combination of collagenase and thermolysin were used for digestion medium. Optimal culture protocols were determined by qualitative assays of proliferation. Cells isolated by using 14‐day‐old embryo and collagenase obtain the best attachment and growth in culture, and the production of continuously growing IEC cultures. Thus, we conclude that the use of collagenase as a dissociating enzyme and 14‐day‐old embryo as a source can be advantageously applied to the isolation of chicken IEC and this method may be useful for various applications and basic studies of the intestinal tract concerning such objects as physiology, immunology and toxicology. 相似文献
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Changes in cell density and size in the ganglion cell layer (GCL) of the retina were studied in chick embryos and post-hatching chicks. The total number of cells in the GCL increased from 3.64 million at embryonic day 8 (E8) to the maximal 7.85 million at E14. After E14, the number of cells decreased to 6.08 million at post-hatching day 1 (P1) and 4.87 million at P8. Cell density in the GCL decreased unevenly according to retinal regions; cell density in the presumptive central area (pCA) of P8-chicks decreased to approximately 45% of that in E8-embryos. Densities of the nasal peripheral retina (NP) and temporal peripheral retina (TP) of P8-chicks decreased to 23 and 18% of E8-embryos, respectively. Differentiation of the central (44,000 cells/mm(2) in pCA) - peripheral (28,000 cells/mm(2) in TP) gradient in cell density was formed by E8. The presumptive dorsal area (pDA) was shaped by E11, but became obscure with age. Although ganglion cell sizes were basically uniform at E8, differentiation occurred with the appearance of larger ganglion cells after E14. Mean size of retinal ganglion cells increased 2.8-fold in the pCA and 3.8-fold in the TP between E8 and P8, accompanying a similar scale of decreases in cell densities. 相似文献
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Min W Lillehoj HS Li G Sohn EJ Miyamoto T 《Veterinary immunology and immunopathology》2002,88(1-2):49-56
The chicken IL-15 gene was recently cloned and shown to encode a polypeptide with T cell growth factor activity similar to IL-2. To further characterize the chemical and biological properties of chicken IL-15, we generated a panel of monoclonal antibodies against bacterially expressed protein and characterized their binding specificities. All antibodies were reactive by ELISA with recombinant IL-15, but not IL-2, and identified a 15kDa recombinant chicken IL-15 by Western blot analysis. Two antibodies inhibited IL-15-induced proliferation of splenic lymphoblast cells. These monoclonal antibodies will be useful for further structural and immunological studies of chicken IL-15. 相似文献
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本研究旨在探讨鸡胚盲肠上皮细胞传代培养条件及其特性,为E.tenella损伤机制及抗球虫药的研究提供体外模型。分别用胰酶-EDTA联合消化和分步消化2种方法分离纯化原代鸡胚盲肠上皮细胞,通过测定贴壁细胞覆盖率选择细胞传代的适宜消化方式;筛选了传代细胞培养液中L-GLN和胰岛素的最佳浓度,通过贴壁差进一步纯化盲肠上皮细胞,探索其合适的培养条件。通过形态学观察、透射电镜、免疫组织化学技术、组织化学技术、糖原染色、流式细胞术的方法对传代细胞特性进行了鉴定。结果表明:胰酶-EDTA联合消化、15min贴壁差纯化除去成纤维细胞,72.5mg.L-1 L-GLN、0.05mg.L-1胰岛素和5%FBS的传代细胞培养液更有利于盲肠上皮细胞的生长;经形态学和透射电镜观察,AKP、Vimentin及PAS染色,所培养的传代细胞具有典型的上皮细胞特征,在传代后24~72h盲肠上皮细胞纯度达95%以上,贴壁细胞覆盖率达85%以上;细胞凋亡测定表明,细胞连传5代,活性较好,第6代细胞凋亡率显著增加,贴壁细胞覆盖率降低。本研究提示用该法传代可获得稳定、数量大、活性高、纯度高的鸡胚盲肠上皮细胞。 相似文献
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试验旨在研究RNA m6A修饰相关基因去甲基化酶Alk B同源蛋白5(Alk B homologue 5,ALKBH5)、去甲基化酶肥胖相关蛋白(fat mass and obesity-associated protein,FTO)、甲基转移酶样蛋白3(methyltransferase like 3,METTL3)、甲基转移酶样蛋白14(methyltransferase like 14,METTL14)和成肾细胞瘤1-结合蛋白(Wilms’tumor 1-associating protein,WTAP)在鸡骨骼肌发育过程中的表达,分析其与骨骼肌m6A甲基化水平的相关性。首先,利用实时荧光定量PCR技术检测m6A甲基化相关基因在金茅花鸡12(E12)、14(E14)、16(E16)、18(E18)胚龄和1日龄腿肌和胸肌组织中mRNA表达水平,以及其在鸡成肌细胞50%、100%增殖期和1、2、3、4、5 d分化期的mRNA表达水平;随后,利用m6A甲基化试剂盒检测金茅花鸡E12和1日龄腿肌和胸肌组织中m6A甲基化修饰水平,与m6A甲基化相关基因表达水平进行相关性分析。结果显示,m6A去甲基化基因ALKBH5和FTO mRNA表达水平在骨骼肌发育过程中显著上调(P<0.05),即在E12、E14低表达,E16、E18逐渐上调,1日龄达到最高。m6A甲基化写入基因METTL14、METTL3和WTAP mRNA表达水平在E12、E14、E16逐渐上升,E18下降,随后至1日龄表达量回升。在细胞增殖过程中,ALKBH5、FTO、METTL14、METTL3和WTAP基因表达均上调;在细胞分化过程中ALKBH5和FTO基因表达水平显著上调(P<0.05),在分化第5天达到最高。METTL14、METTL3和WTAP基因mRNA表达水平在细胞诱导分化的1、2、3、4 d表达量呈下降趋势,而在诱导分化的第5天有所回升。甲基化水平检测结果显示,腿肌和胸肌m6A甲基化水平变化趋势一致,均在胚胎发育过程中显著下降(P<0.05),至1日龄达到最低。相关性分析结果显示,鸡骨骼肌RNA m6A甲基化水平与m6A去甲基化修饰基因ALKBH5、FTO mRNA表达水平呈显著负相关(P<0.05)。综合以上试验结果,推测m6A甲基化修饰与鸡骨骼肌发育相关,而去甲基化基因ALKBH5、FTO可能通过调控RNA m6A甲基化水平,影响鸡骨骼肌发育。本研究结果为进一步研究m6A甲基化修饰调控鸡骨骼肌生长发育的功能和分子机制提供理论依据。 相似文献
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We recently cloned the genes encoding chicken IL-15 and IL-15 receptor (R) alpha proteins. In this study, 12 monoclonal antibodies (mAbs) against recombinant chicken IL-15Ralpha were produced and characterized. By enzyme-linked immunosorbent assay (ELISA), all mAbs showed binding specificity for IL-15Ralpha, but not IL-2 or interferon-gamma, and identified a 25.0kDa protein by immunoblot analysis. Flow cytometric analysis revealed negligible expression of IL-15Ralpha on non-activated lymphocytes from the spleen, thymus or bursa, low but detectable expression on macrophages and high expression on concanavalin A-activated spleen lymphoblasts. Established chicken T cell (RP13) and macrophage (HD11) cell lines expressed substantially higher levels of IL-15Ralpha compared with a B cell line (RP9). Two mAbs inhibited IL-15 dependent proliferation of T cells suggesting that the tertiary structure of the protein domain of native IL-15Ralpha that binds to IL-15 is preserved in the recombinant receptor molecule. These mAbs will be useful reagents for further in vitro and in vivo studies of the biological functions of chicken IL-15 and its receptor. 相似文献
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Asar M Bayram Z Korgun ET Tertemiz F Akkoyunlu G Demir R 《Anatomia, histologia, embryologia》2004,33(3):135-140
Summary In this study, the localization and appearance of synaptophysin-immunoreactive (IR) nerve cells and their relationships with the developing gastric layers were studied by immunocytochemistry and light microscopy in the embryonic rat stomach. The stomachs of Wistar rat embryos aged 13-21 days were used. The first neuronal bodies and their processes containing synaptophysin-immunoreactivity were observed on embryonic day 13. In contrast, synaptophysin-IR nerve terminals were first observed between mesenchymal cells on embryonic day 14. These results indicate that synaptophysin is expressed in growing neurits and neuronal cell bodies before these neurones have established synaptic connections. The occurrences of mesenchymal cell condensation near synaptophysin-IR neuroblasts on embryonic day 15 reflect an active nerve element-specific mesenchymal cell induction resulting in the morphogenesis of muscle cells. Similarly, the appearance of glandular structures after synaptophysin-IR neuroblasts, on embryonic day 18, suggests that the epithelial differentiation may be closely related to the neuronal maturation as well as other factors. Finally, synaptophysin is functionally important in neuronal development and maturation, together with the establishment of neuroneuronal and neuromuscular contacts and in epithelial differentiation. 相似文献