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1.
为了解鸡马立克病病毒(MDV)、禽白血病病毒(ALV)和禽网状内皮组织增生症病毒(REV)在鲁北地区鸡群中的感染情况,对来自21个鸡群的送检病例进行了病原核酸的PCR检测.结果显示,MDV阳性率为28.5%,ALV-J阳性率为23.8%,REV阳性率为14.3%,肿瘤病毒的二重感染率为28.6%.结果表明,3种肿瘤病毒在鲁北地区蛋鸡和地方品种鸡群中的感染严重,病毒的混合感染较多.因此,做好MD的疫苗防护,对ALV-J及REV的感染状况要进行定期检测,控制好养殖环境,尽量避免3种肿瘤病毒的继发感染.  相似文献   

2.
1禽肿瘤病病毒禽肿瘤病病毒包括疱疹病毒、马立克氏病病毒(MDV)、网状内皮组织增生病病毒(REV)、禽白血病和禽白血病病毒J亚群(ALV-J)。火鸡对MDV、REV以及相对罕见的反转录病毒——淋巴细胞增殖病病毒(LPDV)易感。MDV为双股DNA病毒,  相似文献   

3.
为调查山东省家禽肿瘤性疾病的流行情况,本研究以血清学、病理组织学、免疫组织化学、病原学等检测手段,在山东省境内17家AA种鸡场进行检测.血清学试验结果显示:马立克氏病病毒(MDV)平均抗原阳性率为1.87%;禽白血病病毒J亚群(ALV-J)和网状内皮组织增生症病毒(REV)平均抗体阳性率分别为9.52%和39.78%;双重及三重感染,MDV+ALV-J、MDV+REV、ALV-J+REV及MDV+ALV-J+REV感染率分别为1.12%、1.21%、3.92%和0.65%.对57羽疑似肿瘤病的病鸡检测显示:MDV、ALV-J和REV的抗体阳性率分别为19.3%、47.37%和57.89%;MDV+ALV-J、MDV+REV和ALV-J+REV的双阳性率分别为1.75%、3.5%和19.3%;无三重感染.病理组织学观察显示:病鸡体内既有各病毒引起的单纯肿瘤,也有双重肿瘤共存的现象.免疫组织化学检测显示,MDV、ALV-J和REV抗原阳性信号在病鸡中的比例分别为38.6%、54.39%和28.07%.PCR检测结果表明:MDV、ALV-J和REV的阳性率分别为43.86%、64.91%和33.33%;MDV+ALV-J、MDV+REV、ALV-J+REV和MDV+ALV-J+REV阳性率分别为15.79%、10.53%、12.28%和7.02%.本研究结果表明,山东省境内AA肉鸡群中仍存在较高的肿瘤性病毒感染率.  相似文献   

4.
为调查云南省禽流感病毒、新城疫病毒与免疫抑制性病毒混合感染的情况,对云南省2007年1月~2009年10月期间145份禽流感阳性及30份新城疫阳性样品进行禽网状内皮增生病病毒(REV)、J亚群禽白血病病毒(ALV-J)及鸡传染性贫血病毒(CIAV)的检测。禽流感阳性样品中ALV-J的感染阳性率为15.9%,REV的感染阳性率为22.8%,CIAV的感染阳性率为26.9%;新城疫阳性样品中ALV-J的感染阳性率为13.3%,REV的感染阳性率为23.3%,CIAV的感染阳性率为26.7%;共有30份样品发生多重感染,多重感染率为17.1%。对不同区域的4份禽白血病病毒阳性样品、10份禽网状内皮增生病病毒阳性样品、10份禽传染性贫血病毒阳性样品进行了序列比对和系统发育分析。结果表明,云南ALV-J毒株gp85基因与国内外毒株核苷酸及氨基酸同源性分别介于80.4%~96.7%、85.2%~94.5%;REV毒株env基因核苷酸及氨基酸之间的同源性为98.8%~99.8%、97.7%~99.5%;CIAV毒株vp2基因核苷酸及氨基酸之间的同源性为92.4%~100.0%、93.7%~100.0%。  相似文献   

5.
山东省白羽肉鸡中MDV、REV、CAV和ARV感染状况的病原学调查   总被引:2,自引:0,他引:2  
为了解鸡马立克氏病病毒(MDV)、鸡传染性贫血病毒(CAV)、禽网状内皮增生病病毒(REV)和禽呼肠孤病毒(ARV)在山东省白羽肉用型鸡中的流行情况,试验采用地高辛标记的核酸探针-斑点杂交法对淘汰的商品肉鸡、病死商品肉鸡及淘汰肉种鸡进行了上述4种病毒病原的检测。结果表明:ARV主要以单一形式感染,在病死商品肉鸡中感染率最高(30.07%),在3种类型鸡中ARV感染率高于MDV,REV,CAV。MDV在淘汰肉种鸡中感染率(12.82%)高于其他2种鸡群,而REV,CAV,ARV感染率在病死商品肉鸡中最高。混合感染亦相当普遍,以淘汰肉种鸡最高(混合感染率达10.25%),高于任一病毒单独感染率,其次为病死商品肉鸡。  相似文献   

6.
肉种鸡肿瘤病料中MDV、REV和CAV共感染的检测   总被引:3,自引:0,他引:3  
从山东省东营、日照、潍坊、聊城等地区肉种鸡群采集102份有肿瘤病变的病、死鸡肝脏样品,用特异性核酸探针对样品进行马立克氏病病毒(Mareks disease virus,MDV)、网状内皮组织增生症病毒(Reticuloendotheliosis virus,REV)、鸡传染性贫血病病毒(chicken anemia virus,CAV)检测.结果显示,MDV、REV、CAV的检出率分别为88.24%、79.41%、47.06%,且存在严重的共感染现象,三重感染检出率达30.39%;二重感染检出率为59.80%,以MDV和REV共感染检出率最高,为44.12%;单一感染和阴性个体仅占3.92%和1.96%.结果表明,多种免疫抑制性病毒的共感染已普遍存在,是目前肿瘤性疾病发病率日趋上升的重要流行病学因素之一.  相似文献   

7.
2018年以来,某进口品种肉种鸡发生疑似禽白血病病例,流行范围广,危害严重,为确定该次疫情的病原,本研究从辽宁、山东等地发病鸡场采集55份疑似禽白血病病料样品。病理组织切片观察显示,病料样品肝脏和脾脏均有髓细胞样肿瘤细胞增生。针对禽白血病病毒(ALV)、鸡马立克氏病病毒(MDV)和网状内皮组织增生症病毒(REV)的特异性PCR检测结果显示,55份病料样品中ALV阳性样品12份(21.8%),MDV阳性样品1份(1.82%),REV均为阴性。将12份ALV阳性病料样品经处理后接种DF-1细胞进行病毒分离,ELISA检测结果显示有8份ALV群特异性抗原阳性。ALV多重PCR检测结果表明,8个分离株均为J亚群ALV (ALV-J),测序结果显示,8个分离株之间核苷酸序列同源性为99.5%~100%,与A、B、C、D、E亚群ALV的同源性仅为56. 5%~58.8%,与ALV-J的同源性为90.7%~96.6%,进一步表明所有分离株均为ALV-J。上述结果表明,引起该次进口白羽父母代肉种鸡发生禽白血病的病原主要以ALV-J为主,该研究结果为疫情的溯源和有效防控奠定了基础。  相似文献   

8.
禽网状内皮组织增生症(Reticuloendotheliosis,RE)是禽类一种重要的致瘤性和免疫抑制性疾病.近年来,鸡群中REV流行比较严重;REV与马立克氏病病毒(Marek's disease virus,MDV)、鸡贫血病病毒((Chicken infectious anemia,CAV)和J亚群禽白血病病毒(Subgroup J Avian Leuko-sis Virus,ALV-J)等几种免疫抑制性病毒的混合感染也比较普遍.鉴于REV正越来越受到重视.本文就RE的诊断和综合防制作一综述.  相似文献   

9.
为了解禽白血病、禽网状内皮组织增生症和鸡传染性贫血在本地鸡群的感染情况,对宁波市7个区、县的15个鸡群进行了3种疫病4种抗体的血清学检测。结果显示:362份被检血清中,AB亚群禽白血病病毒(ALV-AB)抗体阳性率为55.0%,J亚群禽白血病病毒(ALV-J)抗体阳性率为21.5%,禽网状内皮组织增生症病毒(REV)抗体阳性率为32.0%,鸡传染性贫血病毒(CAV)抗体阳性率为66.8%;15个鸡场AB亚群禽白血病和鸡传染性贫血共感染率为100.0%;12个鸡场共感染了3种免疫抑制性疫病,混合感染率高达80.0%。调查结果表明免疫抑制病在宁波市鸡群中非常普遍。  相似文献   

10.
为确诊疑似J亚群禽白血病病例,试验从湖北某养殖户送检的散养淮南王土鸡典型病变组织中,提取DNA,用分别针对A、B、J亚群禽白血病病毒(ALV)和针对马立克氏病病毒(MDV)、网状内皮增生症病毒(REV)的Multi-PCR方法进行检测,结果只扩增出与ALV-J对应的条带,而无MDV、REV、ALV-A、ALV-B对应条带,表明鸡群感染ALV-J。用DF-1细胞进行病毒分离培养,以抗ALV-J的单克隆抗体JE9为一抗进行间接免疫荧光试验结果显示DF-1细胞呈现亮绿荧光,表明从病料中分离到的病毒为ALV-J,这也是首次从淮南王土鸡分离到ALV-J。  相似文献   

11.
2009年我国部分地区禽白血病分子流行病学调查   总被引:12,自引:3,他引:9  
为了解自2009年年初以来国内一些地区禽白血病流行情况及流行毒株的分子特征,我们从湖北、黑龙江、山东、辽宁、吉林、广东、宁夏、安徽8个省区39个鸡场采集疑似禽白血病病料样品178份,用ALV-A、ALV-B和ALV-J特异性引物,通过PCR方法进行检测。结果表明,8个省的35个鸡场的124份病料中检出了ALV-J(69.7%);25份病料中检出了ALV-A(13.9%);7份病料中检出了ALV-B(3.9%)。14个分离毒株env基因氨基酸同源性为84.3%~99%;与J亚群原型毒株HPRS-103的氨基酸序列同源性为87.3%~98.2%;与其它J亚群env基因氨基酸序列同源性为83%~97.4%。遗传进化分析表明,14个ALV-J分离株分别分属于不同的分支。其中,LJL09DH02分离株与其它分离株及参考毒株的的亲缘关系最远,与HPRS-103的氨基酸同源性仅为87.3%。另外4个分离株的env基因与HPRS-103的氨基酸同源性低于93%,其余9株与HPRS-103的同源性较高(96.6%以上)。该调查结果表明,我国目前ALV的感染主要以J亚群为主,ALV-A和B同时存在。  相似文献   

12.
2009年8月,山东省邹城市某海兰褐蛋鸡群,160日龄发病,死亡率为7%.患鸡经大体剖检、病理组织学、PCR和免疫组织化学等检测,确诊为禽白血病病毒J亚群(ALV-J)感染.病理组织学检测发现,病鸡单独患血管瘤,或髓细胞瘤和纤维肉瘤多发性出现,由ALV-J自然感染引起同一鸡体出现髓细胞瘤和纤维肉瘤尚属国内外首次报道.肝脏研磨接种DF-1细胞培养7d后传3代,细胞无病变,ELISA检测感染细胞上清ALV p27抗原阳性,进一步确诊此鸡群为ALV感染.对病变严重的鸡进行病毒分离及ALV-J gp85基因同源性比较显示与原型株HPRS-103的同源性最高,达94.1%.本研究丰富了ALV-J感染的临床诊断依据,并为ALV-J在我国蛋鸡群中多潜能致瘤机制的研究提供了科学基础.  相似文献   

13.
对不同种鸡场不同周龄肉种鸡进行REV、CAV和ALV(A、B亚群)抗体检测。在572份血清样品中,除了一个8.1周龄和15周龄鸡群CAV抗体阳性率分别为13.3%和75%外,其它鸡群无论是否进行CAV疫苗免疫,抗体阳性率均为100%。在212份血清样品中,REV抗体阳性率在16.7%~62.5%之间;ALV(A、B亚群)抗体阳性率在0%~75%之间。本研究结果表明,所检测种鸡群中存在3种免疫抑制性病毒的感染或混合感染。  相似文献   

14.
为研究HR土鸡中存在的不同亚型禽白血病病毒(ALV)共感染的情况,本实验分别采集46只HR土公鸡的泄殖腔棉拭子和455枚鸡蛋卵白样品,采用ELISA试剂盒检测p27抗原;并采用相应的ELISA试剂盒分别检测卵黄中J亚型ALV(ALV-J)和AB亚型ALV(ALV-AB)抗体。结果表明:HR土公鸡泄殖腔棉拭子样品中p27检出阳性率为87%(40/46),卵白检出率为74.7%(340/455);而卵黄中ALV-J和ALV-AB抗体阳性率分别为0(0/30)和80%(24/30)。无菌采集初步筛选p27抗原检测为阳性的5只HR土公鸡的抗凝血接种CEF,采用抗ALV-J和ALV-A的单克隆抗体进行IFA检测,结果显示5份样品中ALV-A和ALV-J的阳性率均为100%(5/5)。同时选取HR土鸡分离株HR332进行PCR扩增鉴定,结果表明分离株HR332存在ALV-J(HR332J)和ALV-A(HR332A)。其中,HR332J与11株ALV-J国内外参考株的同源性为92.4%~97.9%;HR332A与ALV-A参考株RSA-A、MQNCSU的同源性分别为90.1%和89.7%,与国内分离株SDAU09E2的同源性为99.0%。本研究显示,地方品种HR土鸡存在不同亚型ALV共感染,同时ALV-A和ALV-J共感染同一个鸡的现象已经存在。  相似文献   

15.
16.
OBJECTIVE: To determine the extent of avian leukosis virus subgroup J (ALV-J) infection in Australian broiler breeder flocks, using virus isolation and molecular biological detection. Any resultant ALV-J viral isolates to be characterised by neutralisation cross testing in order to determine antigenic relationships to overseas isolates of ALV-J. STUDY DESIGN: Samples of blood, feather pulp, albumen and tumours were obtained from broiler breeder flocks which represented four genetic strains of meat chickens being grown in Victoria, South Australia, NSW and Queensland. Dead and ailing birds were necropsied on farm and samples were collected for microscopic and virological examinations. Virus isolation was carried out in C/O and DF-1 CEF cultures and ALV group specific antigen was detected in culture lysates using AC-ELISA. Micro-neutralisation assay was used for antigenic characterisation of selected isolates. Genomic DNA was isolated from cultured cells, tumours and feather pulp. ALV-J envelope sequences were amplified by PCR using specific ALV-J primers while antibodies against ALV-J were detected by ELISA. RESULTS: A total of 62 ALV-J isolates were recovered and confirmed by PCR from 15 (31.3%) of 48 breeder flocks tested. Antibody to ALV-J was detected in 20 (47.6%) of the 42 flocks tested. Characteristic lesions of myeloid leukosis caused by ALV-J were found in affected flocks. The gross pathological lesions were characterised by skeletal myelocytomas located on the inner sternum and ribs, neoplastic enlargement of the liver, and in some cases gross tumour involvement of the spleen, kidney, trachea, skeletal muscles, bone marrow, skin and gonads. Microscopically, the tumours consisted of immature granulated myelocytes, and were present as focal or diffuse infiltrations in the affected organs. Virus micro-neutralisation assays demonstrated antigenic variation among Australian isolates and to overseas strains of ALV-J. CONCLUSION: ALV-J infection was prevalent in Australian broiler breeder flocks during 2001 to 2003. Australian isolates of ALV-J show a degree of antigenic variation when compared to overseas isolates.  相似文献   

17.
随机抽取安徽省3个肉种鸡场种鸡及3个地市农贸市场商品鸡的血清样本和泄殖腔拭子,采用ELISA进行鸡白血病检测,并对J亚群鸡白血病病毒抗体阳性鸡群中病鸡的肝组织、全血及上毒细胞提取DNA进行PCR扩增和基因测序。检测结果表明,3个肉种鸡场中J亚群鸡白血病抗体阳性检出率分别为:0、73.50%和15.22%;3个农贸市场商品鸡抗体阳性检出率分别为:12.00%、2.22%和9.10%。3个肉种鸡场A、B亚群鸡白血病的抗体阳性率分别为0、17.93%和1.08%,ALV抗原阳性率分别为2.17%、17.93%和15.22%。PCR检测结果表明,从可疑发病鸡的肝组织和全血中均能扩增出ALV-J gp85特异性片段。结果证实安徽省鸡群中有ALV-J感染,并呈不同程度的流行,应引起高度重视。  相似文献   

18.
Chickens from seven different parental lines of commercial White Leghorn layer flocks from three independent breeders were inoculated with a naturally occurring avian leukosis virus (ALV) containing an ALV-B envelope and an ALV-J long terminal repeat (LTR) termed ALV-B/J. Additional groups of chickens from the same seven parental lines were inoculated with ALV-B. Chickens were tested for ALV viremia and antibody at 0, 4, 8, 16, and 32 wk postinfection. Chickens from all parental lines studied were susceptible to infection with ALV-B with 40%-100% of inoculated chickens positive for ALV at hatch following embryo infection. Similarly, infection of egg layer flocks with the ALV-B/J recombinant virus at 8 days of embryonation induced tolerance to ALV with 86%-100% of the chickens viremic, 40%-75% of the chickens shedding virus, and only 2/125 (2%) of the chickens producing serum-neutralizing antibodies against homologous ALV-B/J recombinant virus at 32 wk postinfection. In contrast, when infected with the ALV-B/J recombinant virus at hatch, 33%-82% of the chickens were viremic, 28%-47% shed virus, and 0%-56% produced serum-neutralizing antibodies against homologous ALV-B/J recombinant virus at 32 wk postinfection. Infection with the ALV-B/J recombinant virus at embryonation and at hatch induced predominately lymphoid leukosis (LL), along with other common ALV neoplasms, including erythroblastosis, osteopetrosis, nephroblastomas, and rhabdosarcomas. No incidence of myeloid leukosis (ML) was observed in any of the commercial White Leghorn egg layer flocks infected with ALV-B/J in the present study. Data suggest that the parental line of commercial layers may influence development of ALV-B/J-induced viremia and antibody, but not tumor type. Differences in type of tumors noted in the present study and those noted in the field case where the ALV-B/J was first isolated may be attributed to differences in the genetics of the commercial layer flock in which ML was first diagnosed and the present commercial layer flocks tested in the present study.  相似文献   

19.
广西凭祥斗鸡禽白血病病毒检测及分离株env基因分析   总被引:1,自引:0,他引:1  
为了解广西凭祥市特有家禽品种斗鸡禽白血病病毒(ALV)的感染情况,采集了该市3个鸡场斗鸡的肛拭子、血清、血浆样品共344份,用禽白血病ELISA检测试剂盒进行检测。结果显示,斗鸡ALV感染情况严重,其中肛拭样品ALV-p27抗原阳性率高达39.13%,血清样品病毒分离阳性率为12.97%,ALV-J和ALV-A/B抗体阳性率分别为22.39%和7.46%;对从2只斗鸡获得的病毒分离株DJ-3-18和DJ-45进行病毒囊膜蛋白基因env的扩增、序列测定及比较分析,结果显示2株病毒的gp85基因与ALV-A亚群参考株之间氨基酸的同源性为88.2%~96.5%,gp37基因与ALV-A亚群参考株之间氨基酸的同源性为91.4%~98.0%,其中与台湾A亚群蛋鸡源分离株TW-3577的亲缘关系最近,而与ALV其他亚群毒株的同源性则较低。结果表明,首次获得的2株斗鸡源ALV分离株属A亚群。  相似文献   

20.
Several subgroup J-like avian leukosis viruses (ALV-Js) were isolated from broiler breeder (BB) and commercial broiler flocks experiencing myeloid leukosis (ML) at 4 wk of age or older. In all cases, diagnosis of ML was based on the presence of typical gross and microscopic lesions in affected tissues. The isolates were classified as ALV-J by 1) their ability to propagate in chicken embryo fibroblasts (CEF) that are resistant to avian leukosis virus (ALV) subgroups A and E (C/AE) and 2) positive reaction in a polymerase chain reaction with primers specific for ALV-J. The prototype strain of these isolates, an isolate termed ADOL-Hc1, was obtained from an adult BB flock that had a history of ML. The ADOL-Hc1 was isolated and propagated on C/AE CEF and was distinct antigenically from ALV of subgroups A, B, C, D, and E, as determined by virus neutralization tests. Antibody to ADOL-Hc1 neutralized strain HPRS-103, the prototype of ALV-J isolated from meat-type chickens in the United Kingdom, but antibody to HPRS-103 did not neutralize strain ADOL-Hc1. On the basis of both viremia and antibody, prevalence of ALV-J infection in affected flocks was as high as 87%. Viremia in day-old chicks of three different hatches from a BB flock naturally infected with ALV-J varied from 4% to 25%; in two of the three hatches, 100% of chicks that tested negative for virus at hatch had evidence of viremia by 8 wk of age. The data document the isolation of ALV-J from meat-type chickens experiencing ML as young as 4 wk of age. The data also suggest that strain ADOL-Hc1 is antigenically related, but not identical, to strain HPRS-103 and that contact transmission of ALV-J is efficient and can lead to tolerant infection.  相似文献   

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