中国兽药杂志
中國獸藥雜誌
중국수약잡지
CHINESE JOURNAL OF VETERINARY DRUG
2011年
10期
7-9,27
,共4页
李润%李宁%印春生%薛青红%支海兵
李潤%李寧%印春生%薛青紅%支海兵
리윤%리저%인춘생%설청홍%지해병
犬细小病毒%VP2%分离%鉴定
犬細小病毒%VP2%分離%鑒定
견세소병독%VP2%분리%감정
canine parvovirus%VP2%isolation%identification
本实验室对从疑似犬细小病毒感染的发病犬分离的病毒采用同步培养法接种猫肾细胞(CRFK)增殖,通过PCR试验、IFA试验和VP2基因测序分析等方法进行鉴定并分型,获得一株犬细小病毒强毒株,命名为CPV-DD株。对分离病毒进行PCR扩增,可扩增出特异性DNA片段(1 163 bp);盲传至第6代时,病毒液的HA效价为1∶1024,其血凝性能被特异性抗体抑制;IFA可见特异性亮绿色荧光,TCID50为105.5/0.1 mL;电镜观察可见20 nm左右的病毒颗粒,VP2蛋白氨基酸序列分析显示该毒株为CPV-2a型,氨基酸序列分析在324位出现Try→Ile替换,该位点处于病毒潜在的抗原表位。
本實驗室對從疑似犬細小病毒感染的髮病犬分離的病毒採用同步培養法接種貓腎細胞(CRFK)增殖,通過PCR試驗、IFA試驗和VP2基因測序分析等方法進行鑒定併分型,穫得一株犬細小病毒彊毒株,命名為CPV-DD株。對分離病毒進行PCR擴增,可擴增齣特異性DNA片段(1 163 bp);盲傳至第6代時,病毒液的HA效價為1∶1024,其血凝性能被特異性抗體抑製;IFA可見特異性亮綠色熒光,TCID50為105.5/0.1 mL;電鏡觀察可見20 nm左右的病毒顆粒,VP2蛋白氨基痠序列分析顯示該毒株為CPV-2a型,氨基痠序列分析在324位齣現Try→Ile替換,該位點處于病毒潛在的抗原錶位。
본실험실대종의사견세소병독감염적발병견분리적병독채용동보배양법접충묘신세포(CRFK)증식,통과PCR시험、IFA시험화VP2기인측서분석등방법진행감정병분형,획득일주견세소병독강독주,명명위CPV-DD주。대분리병독진행PCR확증,가확증출특이성DNA편단(1 163 bp);맹전지제6대시,병독액적HA효개위1∶1024,기혈응성능피특이성항체억제;IFA가견특이성량록색형광,TCID50위105.5/0.1 mL;전경관찰가견20 nm좌우적병독과립,VP2단백안기산서렬분석현시해독주위CPV-2a형,안기산서렬분석재324위출현Try→Ile체환,해위점처우병독잠재적항원표위。
A strain of canine parvovirus(CPV)was isolated from bloody feces of an ill puppy suspected of parvovirus infections in Beijing.The strain,designated as CPV-DD,was isolated by inoculating CRFK cells in synchronism and was identified as serotype CPV-2a by PCR,the HA,IFA,electron microscopy observation and sequencing of VP2 gene.A unique Ile-324 in VP2 of DD strain was found,contrasting to a Try-324 in the VP2 of other strains.After 6 passages in CRFK cells,the infected cell cultures could agglutinate red blood cells of pigs at the titer of 1∶ 1024.The haemagglutination could be inhibited by monoclonal antibody specific to CPV.Specific fluorescent in the nucleus of the infected cells was observed by IFA assay and the TCID50 of virus fluid was titred as 105.5/0.1mL.Concentrated virus particles with a diameter of 20nm were observed by transmission electron microscope.
