埃及吉萨省临床病例中绵羊痘病毒和山羊痘病毒的检测、鉴定与区分
Detection, identification, and differentiation of sheep pox virus and goat pox virus from clinical cases in Giza Governorate, Egypt.
作者信息
Mahmoud M A, Khafagi M H
机构信息
Department of Parasitology and Animal Diseases, Veterinary Research Division, National Research Centre, Dokki 12622, Giza, Egypt.
出版信息
Vet World. 2016 Dec;9(12):1445-1449. doi: 10.14202/vetworld.2016.1445-1449. Epub 2016 Dec 18.
AIM
To isolate, identify, and differentiate (CaPV) (sheep pox virus and goat pox virus) infections by egg inoculation, transmission electron microscopy (TEM), and 30 kDa RNA polymerase subunit gene-based polymerase chain reaction (PCR) (RPO30) in clinically affected animals in Hawamdia township of Giza Governorate, Egypt.
MATERIALS AND METHODS
A total of 37 scab samples were collected from clinically suspected field cases of sheep pox and goat pox. These samples were collected during (2014-2015) during different outbreaks of sheep pox and goat pox from Hawamdia township of Giza Governorate, Egypt. The samples were subjected to egg inoculation, TEM, and (RPO30) gene-based PCR. By using the egg inoculation: Previously prepared 37 scab samples (n=23 sheep and n=14 goats) were inoculated on the chorioallantoic membrane of specific pathogen free (SPF) embryonated chicken eggs (12 days old age). In the presence of the suitable percentage of humidity and candling, the inoculated eggs were incubated at 37°C. By using the TEM: Samples showed positive pock lesions on the chorioallantoic membranes, were fixed in glutaraldehyde, then processed and sectioned for TEM. Using the (RPO30) gene-based PCR assay, 30 of positive samples after egg inoculation (n=19 sheep and n=11 goats) were screened.
RESULTS
Using the egg inoculation, a characteristic pock lesions for poxviruses were seen in 30/37 (n=19 sheep and n=11 goats) (81.08%). Using the TEM, examination of the positive samples after egg inoculation revealed positive result in 23/30 (n=15 sheep and n=8 goats) (76.66%). The positive results represented by the presence of negatively stained oval-shape virus particles. Using the (RPO30) gene-based PCR assay, out of 30 total of positive samples after egg inoculation (n=19 sheep and n=11 goats) were screened, 27 (90%) samples (n=17 sheep and n=10 goats) were positive. The given band sizes of sheep and goats were 172 and 152 bp, respectively.
CONCLUSION
PCR assay depended on RPO30 gene can be used lonely for the detection, identification, and differentiation of CaPVs. RPO30 gene-based PCR assay in combination with gene sequencing helps in molecular epidemiological studies of CaPV infection.
目的
通过卵接种、透射电子显微镜(TEM)以及基于30 kDa RNA聚合酶亚基基因的聚合酶链反应(PCR)(RPO30),对埃及吉萨省哈瓦姆迪亚镇临床患病动物中的绵羊痘病毒和山羊痘病毒(CaPV)感染进行分离、鉴定和区分。
材料与方法
从绵羊痘和山羊痘临床疑似现场病例中总共采集了37份痂皮样本。这些样本于2014 - 2015年期间,在埃及吉萨省哈瓦姆迪亚镇不同的绵羊痘和山羊痘疫情爆发时采集。样本进行了卵接种、TEM以及基于(RPO30)基因的PCR检测。通过卵接种:先前准备好的37份痂皮样本(n = 23只绵羊和n = 14只山羊)接种到无特定病原体(SPF)的12日龄鸡胚的绒毛尿囊膜上。在适宜湿度和照蛋条件下,接种后的鸡蛋在37°C孵育。通过TEM:在绒毛尿囊膜上显示出阳性痘疱病变的样本,用戊二醛固定,然后进行处理和切片用于TEM观察。使用基于(RPO30)基因的PCR检测方法,对卵接种后30份阳性样本(n = 19只绵羊和n = 11只山羊)进行筛查。
结果
通过卵接种,在30/37(n = 19只绵羊和n = 11只山羊)(81.08%)样本中观察到痘病毒特有的痘疱病变。通过TEM,对卵接种后的阳性样本检查发现,23/30(n = 15只绵羊和n = 8只山羊)(76.66%)样本呈阳性结果。阳性结果表现为存在负染的椭圆形病毒颗粒。使用基于(RPO30)基因的PCR检测方法,在卵接种后总共30份阳性样本(n = 19只绵羊和n = 11只山羊)中进行筛查,27份(90%)样本(n = 17只绵羊和n = 10只山羊)呈阳性。绵羊和山羊的给定条带大小分别为172和152 bp。
结论
基于RPO30基因的PCR检测方法可单独用于CaPVs的检测、鉴定和区分。基于RPO30基因的PCR检测方法与基因测序相结合有助于CaPV感染的分子流行病学研究。
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