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1.
本试验借助透射电镜技术、琼脂糖凝胶电泳、流式细胞术和荧光染色技术对传染性法氏囊病病毒变异 E 株人工感染诱导的雏鸡法氏囊淋巴细胞和体外培养法氏囊细胞的细胞凋亡进行了较为详细的研究。结果表明, I B D V 感染后早期阶段,雏鸡法氏囊淋巴细胞和体外培养法氏囊细胞呈现典型细胞凋亡的形态学特征和生化特 征。 I B D V 感染雏鸡后24~48 h 和感染法氏囊培养细胞后4~24 h,法氏囊淋巴细胞凋亡细胞数量显著增加,而正常淋巴细胞数量相应减少,揭示 I B D V 人工感染可以诱导雏鸡法氏囊淋巴细胞和体外培养法氏囊淋巴细胞的细胞凋亡。  相似文献   

2.
本研究用新城疫病毒(NDV)参考强毒株F48E8感染鸡,通过光镜和电镜观察鸡的胸腺和法氏囊淋巴绌胞凋亡的形态学特征,并进行统计学分析。NDV感染鸡后,其胸腺和法氏囊淋巴细胞凋亡数量显著增加(P<0.01)。实验结果说明NDV参考强毒株F48E8人工感染鸡后可以诱导胸腺和法氏囊淋巴绌胞凋亡。  相似文献   

3.
传染性法氏囊病病毒(IBDV)为dsRNA病毒,可造成雏鸡法氏囊损伤进而发生免疫抑制;MDA5是能够特异性识别dsRNA病毒的模式识别受体。为研究鸡MDA5(chMDA5)信号通路在IBDV致雏鸡法氏囊病理损伤中的作用,试验选取50只14日龄SPF雏鸡随机分为IBDV感染组和空白对照组,每组25只,IBDV感染组雏鸡通过点眼、滴鼻感染IBDV JIC7株病毒液,0.6 mL·只-1,空白对照组雏鸡经相同途径给予相同剂量无菌PBS,感染IBDV后第1、4、7、21及35天采集雏鸡法氏囊。采用qRT-PCR方法检测法氏囊中IBDV载量,chMDA5及chMDA5信号通路衔接蛋白(chIPS-1)、转录因子(chIRF3和chNF-κB)、下游产物细胞因子(chIFN-βchTNF-αchIL-1βchIL-6) mRNA水平变化;间接免疫荧光法检测chMDA5蛋白表达变化,传统病理学方法检查法氏囊病理组织学变化。结果发现,雏鸡感染IBDV后,其法氏囊中chMDA5、chIPS-1、chIRF3、chNF-κBchIFN-βchTNF-αchIL-1βchIL-6的表达量均显著高于对照组,且法氏囊组织发生形态损伤,上述变化趋势与IBDV载量变化基本一致。结果表明,雏鸡法氏囊chMDA5及其信号转导通路可被IBDV激活,参与到IBDV感染雏鸡法氏囊损伤与抗损伤过程中。  相似文献   

4.
本研究鸡传染性法氏囊病冻干卵黄抗体和市售精制液体卵黄抗体分别以10羽份和3 mL超剂量肌肉注射各10只18日龄SPF雏鸡,观察14 d均安全。两种抗体以1羽份剂量分别肌肉注射各20只18日龄SPF雏鸡24 h后,用IBDV强毒TL株攻击,连续观察144 h,2个试验组分别有20/20、17/20的雏鸡健活,剖检没有发现法氏囊病变;二者分别以1羽份剂量连续2 d肌肉注射各20只18日龄已经被IBDV强毒TL株攻击12 h的SPF雏鸡,连续观察96 h,2个试验组有19/20、17/20的雏鸡健活,而预防和治疗试验中的阳性对照组中20只鸡均有法氏囊特征性病变发生(20/20),且死亡率在85%(17/20)以上,阴性对照组雏鸡均正常。  相似文献   

5.
利用光镜、透射电镜、凝胶电泳和原位末端标记技术(TUNEL)对鸡新城疫病毒(NDV)F48E8株在体内诱导鸡胸腺淋巴细胞的凋亡情况进行了观察和检测,以期探讨NDV的致病机制。经NDV感染后,鸡胸腺淋巴细胞呈现典型的凋亡特征,感染组胸腺的淋巴细胞凋亡率显著高于对照组(P<0.01)。结果表明:NDV标准强毒F48E8株可以在体内诱导胸腺淋巴细胞凋亡,由此所致的免疫抑制可能是NDV致病的重要原因。  相似文献   

6.
观察中药对人工感染传染性囊病(IBD)雏鸡的死亡率、器官出血率、增重效果的影响,以及抑制人工感染的传染性囊病病毒(IBDV)致死鸡胚试验。结果表明:中药对人工感染传染性囊病雏鸡的治愈率为83.3%,降低死亡率61.1%(P<0.05);法氏囊、脾脏出血率显著降低;适量中药明显控制感染,提高增重,抑制IBDV致死鸡胚效果明显。  相似文献   

7.
以SPF雏鸡为研究对象,应用细胞培养、MTT及流式细胞检测技术,通过T淋巴细胞对刀豆蛋白A的增殖能力及其CD4+和CD8+T淋巴细胞亚型数量的检测,较全面系统的研究了传染性法氏囊病病毒(IBDV)感染21日龄SPF雏鸡后,其免疫器官(胸腺、脾脏、法氏囊)T细胞增殖能力及其亚型的动态变化,结果发现:IBDV感染SPF雏鸡后,其胸腺和脾脏T淋巴细胞增殖能力于病毒感染后3~7 d显著降低,CD4+和CD8+T淋巴细胞数量于病毒感染初期明显低于对照雏鸡;法氏囊中CD4+和CD8+T淋巴细胞数量在病毒感染初期迅速增加,而后持续低于对照雏鸡.表明SPF雏鸡感染IBDV后,其免疫器官细胞免疫功能受抑制,而作为病毒侵袭的主要靶器官,法氏囊在病毒感染初期有大量T细胞浸润,该项研究为进一步阐明IBDV的免疫致病机制提供了重要的参考依据.  相似文献   

8.
Mx蛋白是由干扰素诱导产生的在多种脊椎动物中发挥抗病毒作用的效应分子。为探究雏鸡感染传染性法氏囊病病毒(IBDV)后鸡抗病毒基因Mx m RNA在法氏囊和脾脏中的表达变化,采用IBDV感染雏鸡70只,分别于感染后0、24、72、120、168、192 h随机选取6只,收集法氏囊和脾脏,利用q RT-PCR技术检测IBDV感染后不同时间点鸡Mx m RNA表达变化。结果显示,雏鸡感染IBDV后,法氏囊和脾脏中Mx m RNA表达水平均极显著高于对照组(P0.01),对照组各时间点之间几乎无变化;且随着感染时间延长,法氏囊和脾脏中Mx m RNA表达量呈先增高后降低的趋势,法氏囊和脾脏分别在72和24 h Mx表达量达到最高,是对照组的66.13和25.40倍。结果表明,法氏囊和脾脏中Mx的转录水平随着IBDV在法氏囊中的增殖而迅速升高,而IBDV减少后Mx的转录水平下降;脾脏中Mx对IBDV感染的转录水平变化比法氏囊更为快速。  相似文献   

9.
为了研究感染IBDV雏鸡外周血液变化,采用白细胞分类计数和针挑血滴法,对人工感染IBDV30日龄雏鸡后72h、96h、120h外周血液变化进行研究。结果表明:嗜中性WBC、淋巴细胞减少,嗜碱性WBC增加,血凝时间延长。并有一定的变化规律;而嗜酸性WBC、单核细胞无明显变化。说明人工感染IBDV后,对雏鸡外周血液确有影响。  相似文献   

10.
曹永长  毕英佐 《动物保健》2009,(7):14-16,39
鸡传染性法氏囊病(IBD)是由传染性法氏囊病病毒(IBDV)引起的一种急性、高度接触性传染病。IBDV主要侵害3~12周龄雏鸡的免疫器官-法氏囊,在孵化后3~6周,当法氏囊生长成熟时,此时鸡群极易感染病毒。该病不但会使感染鸡致病死亡,生产性能下降,而且还会引起免疫抑制和免疫缺陷,导致其他疫苗免疫失败,因而常继发和混合感染多种疾病。  相似文献   

11.
传染性囊病病毒诱导细胞凋亡的初步观察   总被引:5,自引:0,他引:5  
用1株IBDV强毒株感染易感小鸡,对病鸡法氏囊进行电镜观察及DNA电泳分析,直接观察到病鸡法氏囊中B淋巴细胞凋亡的典型形态学特征和生化变化:染色质凝聚成团,集于核膜旁,胞膜与核膜出现凹陷,细胞拉长变形,最后细胞裂解成由膜包围着的小团,被网状细胞和巨噬细胞吞噬;感染IBDV24~48h的法氏囊细胞总DNA在电泳谱上呈梯状条带,而从正常的法氏囊提取的总DNA在电泳谱上只有1条带。结果表明,IBDV感染小鸡之后,导致了法氏囊中B淋巴细胞的凋亡。作者据此推断,细胞凋亡是造成B淋巴细胞数量减少,从而导致小鸡免疫抑制的原因  相似文献   

12.
100只SPF鸡均分为5组,A、B、c3组免疫后攻毒,接种3批次自制的IBD基因工程重组亚单位油乳剂疫苗;D组不免疫不攻毒,E组不免疫而攻毒。免疫后第22天,感染IBDV强毒株BC-6/85。攻毒后第4天,将所有存活的鸡只以颈脱臼致死,收集法氏囊,以3种方法和指标(法氏囊眼观病变;法氏囊显微病变;法氏囊中IBDV抗原检测)进行分析,以评定免疫保护率。结果显示,以这3种方法和指标评定,A组免疫保护率为90%,B、C组免疫保护率均为95%;试验鸡A3、A14、B7、C16、E1~E20,法氏囊眼观病变明显,法氏囊显微病理损伤评分为3~5分,琼脂免疫扩散试验检测法氏囊中IBDV抗原均为阳性;其他试验鸡,法氏囊眼观无明显异常,法氏囊显微病理损伤评分在3分以下,琼脂免疫扩散试验检测法氏囊中IBDV抗原均为阴性。结果表明,这3种方法和指标在IBD疫苗免疫保护试验评定中具有很好的一致性。  相似文献   

13.
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14.
The Australian strain of infectious bursal disease virus (IBDV), 002/73, affected the response of chickens to Newcastle disease virus (NDV). The titre of serum antibodies to NDV in chickens infected with IBDV was significantly lower than that of birds infected with NDV alone. It also appeared that IBDV affected NDV excretion from chickens as NDV was more frequently isolated from chickens infected with IBDV, IBDV infection did not alter the pathogenicity of NDV in chickens. This Australian strain of IBDV therefore appeared to be immunodepressive in one-day-old chickens.  相似文献   

15.
Primary and secondary immune responses to Newcastle disease virus (NDV) was evaluated in chickens infected with infectious bursal disease virus (IBDV) at one and 28 days of age. The geometric mean primary hemagglutination-inhibition antibody titers (GMT) of chickens infected with IBDV at one day of age was significantly lower (P less than or equal to 0.01) than those infected at 28 days of age. Infection with IBDV had no influence on secondary immune response to NDV. The effect of IBDV infection at one day of age on the cell-mediated immunity of chickens was evaluated by skin allograft acceptance or survival time. There was no significant difference between the percentage of grafts accepted in IBDV infected and noninfected control chickens. However, the mean graft survival time in the IBDV infected chickens was significantly longer (P less than or equal to 0.05) than those in the control group. This suggested a suppression of cell-mediated immunity due to IBDV infection.  相似文献   

16.
Variations of B lymphocytes bearing surface immunoglobulin (SIg) M [SIg(M)] and G [SIg(G)] were studied in the spleen and peripheral blood of chickens infected with infectious bursal disease virus (IBDV). The proportion of SIg-bearing B lymphocytes and SIg(M)- and SIg(G)-bearing B cells in chickens infected at one day of age decreased from 1 week postinfection (p.i.) onward and was significantly lower at 8 weeks p.i. In chickens infected at 4 weeks, the percentage of SIg-bearing B cells decreased severely during the first 2 weeks p.i. The decrease of SIg(M)-bearing B cells preceded that of SIg (G)-bearing B cells: the lowest percentage of SIg(M)-bearing B cells has observed 2 to 3 days p.i., and that of SIg(G)-bearing B cells was seen 4 days p.i. The results suggest that SIg(M)-bearing B cells are the major target for IBDV infection.  相似文献   

17.
Infectious bursal disease virus and proventriculitis in broiler chickens   总被引:2,自引:0,他引:2  
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18.
The role of cell-mediated immunity (CMI) in pathogenesis of infectious bursal disease virus (IBDV) was investigated. One-day-old specific pathogen-free chickens were treated with 3mg of cyclophosphamide (Cy) per chicken for 4 consecutive days and, 3 weeks later, infected with the IBDV-IM strain. Chickens were examined for: (a) mitogenic response of splenocytes to ConA, as an indicator of T-cell functions in vitro, (b) antibody against IBDV by ELISA, (c) IBDV genome in various tissues by RT-PCR and (d) immunological memory. At the time of IBDV infection, Cy-treated chickens had depleted bursal tissue (an avian primary B-cell lymphoid organ), severely compromised antibody-producing ability, but normal T-cell response to ConA. In primary infection, no detectable antibody against IBDV antigen in Cy-treated, IBDV-infected chickens was observed up to 28 days post-infection (PI), while IBDV genome was detected by RT-PCR in spleen, thymus, liver and blood until 10 days PI. Like intact control chickens infected with IBDV, Cy-treated, IBDV-infected chickens suppressed splenocytes responses to ConA from 5 to 10 days PI, suggesting that intact control as well as Cy-treated chickens responded similarly to IBDV infection in the early phase. Following re-infection with IBDV, no detectable secondary antibody response to IBDV as well as IBDV genome in tissues were observed in Cy-treated chickens, while intact control chickens developed vigorous secondary antibody response. Similar to intact control chickens infected with IBDV, Cy-treated chickens after second infection with IBDV did not suppress splenocyte response to ConA. These results suggested that in the absence of detectable anti-IBDV antibodies, protection of Cy-treated chickens from IBDV infection may occur via immunological memory mediated by CMI. We concluded that under normal conditions, IBDV induces a protective antibody response, however, in the absence of antibody, CMI alone is adequate in protecting birds against virulent IBDV.  相似文献   

19.
人工感染IBDV鸡法氏囊的电镜研究   总被引:7,自引:0,他引:7  
通过透射电镜系统观察了人工感染传染性法氏囊病病毒(IBDV)后鸡法氏囊各类细胞的病理变化。感染后12 ̄24h,病毒粒子主要见于髓质淋巴细胞中,细胞中可见到大量纤维样病毒发生基质及无囊膜包围的大型病毒晶格,细胞核染色质浓缩,核中出现纤维样结构。感染后36h,淋巴细胞开始大量裂解死亡。无囊膜包围的病毒晶格也出现于髓质网状细胞中,被感染的网状细胞并不裂解,而表现出细胞凋亡的特征:染色质固缩呈颗粒块状,胞  相似文献   

20.
取320只30~40H龄SPF鸡,经滴鼻和点眼接种传染性法氏囊病病毒(IBDV),接种后24~72h出现死亡,病死率51.25%,死亡鸡剖检变化主要为法氏囊肿胀、出血,甚至呈紫葡萄样,脾脏肿大、出血,骨骼肌出血,腺胃肌胃交界处出血。病理组织学变化,呈现以法氏囊淋巴滤泡内髓质淋巴细胞坏死为主的特征性病变,并可在巨噬细胞浆内发现病毒包涵体。电镜观察,在法氏囊内淋巴细胞、异染性细胞、巨噬细胞浆内,见大量晶格状排列的病毒粒子和包涵体,表明IBDV首先损害法氏囊淋巴滤泡髓质内未成熟的B淋巴细胞,病毒在淋巴细胞内以包涵体方式增殖。  相似文献   

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