首页> 外文期刊>Bangladesh Journal of Veterinary Medicine >ISOLATION AND DETECTION OF NEWCASTLE DISEASE VIRUS FROM FIELD OUTBREAKS IN BROILER AND LAYER CHICKENS BY REVERSE TRANSCRIPTION?POLYMERASE CHAIN REACTION
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ISOLATION AND DETECTION OF NEWCASTLE DISEASE VIRUS FROM FIELD OUTBREAKS IN BROILER AND LAYER CHICKENS BY REVERSE TRANSCRIPTION?POLYMERASE CHAIN REACTION

机译:通过逆转录聚合酶链反应从肉鸡和层鸡的野外暴发中分离和检测新城疫病病毒

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The present research work was carried out to isolate and identify Newcastle disease virus (NDV) by using haemagglutination inhibition (HI) test and reverse transcription-polymerase chain reaction (RT-PCR) assay. A total of 160 clinical (blood, tracheal and cloacal swabs) and post-mortem (brain, lung, colon and spleen) samples were collected from chickens of two field outbreaks of Newcastle disease (ND) in 2006, one in a broiler (Cobb-500) farm of Mymensingh district and other one in a layer (Sonali) farm of Gazipur district. All the samples were inoculated onto 10-day-old embryonated chicken eggs through allantoic sac route and in the chicken embryo fibroblasts (CEFs) cell culture. The allantoic fluid (AF) of the dead embryos and the infected culture fluid (ICF) of the CEF were harvested at 48 and 96 hours of post-infection, respectively. The HI and RT-PCR were employed to detect NDV in tissue homogenates of all the clinical and post-mortem samples as well as laboratory samples (AF and ICF). Among the clinical samples, virus isolation rate was found higher from tracheal swab (90%) compared to those of cloacal swab (85%) and serum (65%). On the other hand, among the four different types of post-mortem samples, virus isolation rate was found higher in spleen (100%) compared to those of lungs (80%), colon (60%), and brain (80%) samples. In CEF cell culture system, the rate of virus isolation from all the aforesaid samples was found 100% with the exception of serum samples. The isolation rate of NDV was higher in CEF culture system (93.8%) compared to that of avian embryos (80%). Among the clinical and post-mortem samples, inoculum of only cloacal swab and colon showed HA and HI activities. The anti-NDV hyperimmune serum revealed complete inhibition of the 4 haemagglutination unit of each isolate of viruses isolated from broiler and layer chickens present in the laboratory samples (AF and ICF). The NDV specific primers used in the direct RT-PCR for genome detection of NDV showed equal sensitivity and specificity with the RNA extracted from the clinical, post-mortem and laboratory samples (AF and ICF) as with the genomic RNA of reference NDV. Higher rate of detection of NDV was recorded with RT-PCR assay than HI test. Therefore, the molecular method (RT-PCR) can be introduced for rapid and confirmatory detection of NDV from any form of outbreak of ND in the field level of Bangladesh.
机译:目前的研究工作是通过血凝抑制(HI)试验和逆转录-聚合酶链反应(RT-PCR)试验来分离和鉴定新城疫病毒(NDV)。 2006年,从两次新城疫暴发的鸡中收集了160份临床(血液,气管和泄殖腔拭子)和验尸(脑,肺,结肠和脾脏)样本,其中一只在肉鸡中(Cobb) -500)Mymensingh区的农场和Gazipur区的另一个分层(Sonali)农场。通过尿囊囊途径和鸡胚成纤维细胞(CEFs)细胞培养将所有样品接种到10天大的鸡胚鸡蛋上。分别在感染后48小时和96小时收获死胚的尿囊液(AF)和CEF的感染培养液(ICF)。 HI和RT-PCR用于检测所有临床和验尸样品以及实验室样品(AF和ICF)的组织匀浆中的NDV。在临床样本中,发现气管拭子的病毒分离率(90%)高于泄殖腔拭子(85%)和血清(65%)。另一方面,在四种不同类型的验尸样本中,发现脾脏中的病毒分离率更高(100%),而肺部(80%),结肠(60%)和大脑(80%)的病毒分离率更高样品。在CEF细胞培养系统中,除血清样品外,从所有上述样品中分离出病毒的比率均为100%。 CEF培养系统中NDV的分离率(93.8%)高于禽类胚胎(80%)。在临床和验尸样品中,只有泄殖腔拭子和结肠的接种物显示出HA和HI活性。抗NDV高免疫血清显示出对从实验室样品(AF和ICF)中的肉鸡和蛋鸡中分离出的每种病毒的4个血凝单位的完全抑制作用。直接RT-PCR中用于NDV基因组检测的NDV特异性引物与从临床,验尸和实验室样本(AF和ICF)提取的RNA以及参考NDV的基因组RNA一样,具有相同的敏感性和特异性。 RT-PCR法记录的NDV检出率高于HI法。因此,可以采用分子方法(RT-PCR)来从孟加拉国田间水平的任何形式的ND暴发中快速,确定性地检测NDV。

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