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Diagnosis of iridovirus in large yellow croaker by PCR

机译:PCR诊断大黄鱼中的虹膜病毒。

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A rapid and sensitive PCR-based method for the detection of the large yellow croaker iridovirus (LYCIV) is described, which involves the amplification of a 295 bp fragment of the LYCIV ATPase gene from DNA isolated from naturally infected fish spleen. Sequencing of LYCIV ATPase gene fragment showed it shared 100% nucleotide sequence homology with the corresponding region of the ATPase gene of red sea bream iridovirus (RSIV) and sea bass iridovirus (SBIV), suggesting that LYCIV was homologous with RSIV and SBIV at least in part of the gemone. The specificity and sensitivity of the PCR procedure were tested on the iridovirus-infected fishes, the expected fragment was detected from spleen DNA samples of infected fishes, whereas no fragments were amplified from healthy fish spleen DNA, white spot syndrome baculoviruses (WSBV) DNA and pseudorabies virus (PRV) DNA.Detection limit of this method was 10-7 ng positive plasmid DNA containing target sequence, equal to about 100 virions. In the infected experiment, first positive detection (1/4) appeared at Day 3 post-infection, all fish (4/4) tested positive at Day 7, however obvious symptoms were observed at Day 8, so LYCIV infection could be detected prior to the appearance of obvious symptoms. These results indicate that this PCR method could be used for early, rapid and specific detection of LYCIV infection.
机译:描述了一种基于PCR的快速灵敏的方法来检测大黄鱼虹膜病毒(LYCIV),该方法涉及从天然感染鱼脾脏分离的DNA中扩增LYCIV ATPase基因的295 bp片段。 LYCIV ATPase基因片段的测序表明,它与红鲷鱼虹膜病毒(RSIV)和鲈鱼虹膜病毒(SBIV)的ATPase基因的相应区域具有100%的核苷酸序列同源性,这表明LYCIV至少与RSIV和SBIV同源。宝石的一部分。在感染了虹膜病毒的鱼类上测试了PCR方法的特异性和敏感性,从受感染鱼类的脾DNA样本中检测到了预期的片段,而从健康鱼类脾DNA,白斑综合症杆状病毒(WSBV)DNA和伪狂犬病病毒(PRV)DNA。此方法的检测极限是10-7 ng阳性质粒DNA,含有靶序列,约等于100个病毒粒子。在受感染的实验中,感染后第3天首次检测出阳性(1/4),所有鱼类(4/4)在第7天检测为阳性,但是在第8天观察到明显的症状,因此可以在之前检测到LYCIV感染出现明显的症状。这些结果表明该PCR方法可用于早期,快速和特异性检测LYCIV感染。

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