柯萨奇病毒A6型的分子鉴定及VP1区序列分析  被引量:2

Molecular identification of Coxsackievirus A6 and the sequence analysis of VP1 region

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作  者:赵虹[1] 林鸿波[1] 俞平达[1] 李平[1] 

机构地区:[1]宁波市鄞州区疾病预防控制中心,浙江宁波315100

出  处:《中国卫生检验杂志》2014年第24期3572-3574,共3页Chinese Journal of Health Laboratory Technology

基  金:宁波市鄞州区科技局第二批科技计划项目(鄞科[2012]90号)

摘  要:目的对2012年-2013年宁波鄞州地区柯萨奇病毒A6型(CA6)进行分子鉴定,并对其VP1部分序列进化分析。方法 RT-PCR对2012年-2013年手足口病人的标本进行病原检测;兼并引物222-292对部分CA6阳性标本VP1部分序列进行扩增、克隆和测序;经过BLAST比对确定病毒的基因型;通过Mega 4.0对VP1序列的差异进行同源性分析。结果 2012年-2013年,共检出CA6阳性230份,占非EV71和非CA16肠道病毒阳性病例的61.8%(230/372)。测序结果表明,CA6核酸检测阳性的标本所获得的序列均为CA6型,且VP1区核苷酸序列具有高度一致性,与周边国家或地区CA6的核苷酸同源性为94.3%~99.1%。结论兼并引物222-292对CA6有良好的基因扩增特异性;2012年-2013年宁波市鄞州区手足口病的病原除EV71和CA16外,CA6也是重要的病原。Objective To identify the pathogens Coxsackievirus A6 and to analyze the partial sequence of the VP1 region in Yinzhou,Ningbo between 2012 and 2013. Methods The specimens from patients with hand- foot- mouth disease( HFMD)collected from 2012 to 2013 were detected by RT- PCR. The partial sequence of the VP1 region was performed by primer pair222- 292. The virus type was identified with BLAST,and phylogenetic analyses were conducted by using MEGA4. 0 software.Results 230 specimens were positive for CA6 in 2012- 2013. The positive rate of non- EV71 and non- CA16 enteroviruses was 61. 8%( 230 /372). The results of the VP1 sequence showed that 10 virus strains were identified as CA6 shared higher identified. The homology of nucleotides was 94. 3% ~ 99. 1% between the CA6 isolates from Yinzhou and other areas. Conclusion The degenerate primer pair 222- 292 was highly specific for gene amplification of CA6. Except for EV71 and CA16,CA6 infections may be emerging as a new and major cause of epidemic HFMD.

关 键 词:手足口病 柯萨奇病毒A组6型 VP1基因 序列分析 

分 类 号:R373.23[医药卫生—病原生物学]

 

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