Multiplex PCR assay for the accurate and rapid detection and differentiation of Lactococcus garvieae and L. petauri

IF 2.2 3区 农林科学 Q2 FISHERIES
Dilek Ustaoglu, Rafet Çağrı Öztürk, Mustafa Ture, Silvia Colussi, Paolo Pastorino, Ana Isabel Vela, Charalampos Kotzamanidis, Donatella Volpatti, Pier Luigi Acutis, Ilhan Altinok
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Abstract

Lactococcosis is a common bacterial fish disease caused by Lactococcus garvieae, L. petauri and L. formosensis. Although there are different PCR-based techniques to identify the etiological agent, none of these can differentiate these two bacteria without sequencing PCR-amplified fragments. In the present study, we developed a multiplex PCR assay for simultaneous detection and differentiation of L. garvieae and L. petauri. The specificity of the primers was validated against the bacterial DNA of the targeted and non-targeted bacteria. The sizes of the PCR amplicons were obtained as 204 bp for the DUF1430 domain-containing protein gene of L. garvieae, 465 bp for the Lichenan permease IIC component gene of L. petauri, and 302 bp for the teichoic acid biosynthesis protein F gene of both L. garvieae and L. petauri. The PCR amplicons were clearly separated by agarose gel electrophoresis. The multiplex PCR assay did not produce any amplification products with the DNA of the non-targeted bacteria. The multiplex PCR detection limits for L. garvieae and L. petauri were 5 and 4 CFU in pure culture and 50 and 40 CFU/g in spiked tissue samples, respectively. It takes less than 2 h from plate-cultured bacteria and 3 h from tissue samples to get results. In conclusion, the developed multiplex PCR assay is a rapid, specific, accurate, and cost-effective method for the detection and differentiation of L. garvieae and L. petauri and is suitable to be used for routine laboratory diagnosis of L. garvieae and L. petauri.

Abstract Image

用于准确、快速检测和区分 Garvieae 乳球菌和 Petauri 乳球菌的多重 PCR 法。
乳球菌病是一种常见的细菌性鱼病,由 Lactococcus garvieae、L. petauri 和 L. formosensis 引起。虽然有不同的基于 PCR 的技术来确定病原体,但如果不对 PCR 扩增片段进行测序,这些技术都无法区分这两种细菌。在本研究中,我们开发了一种多重 PCR 检测方法,用于同时检测和区分 L. garvieae 和 L. petauri。针对目标细菌和非目标细菌的细菌 DNA 验证了引物的特异性。PCR扩增子的大小分别为:L. garvieae的含DUF1430结构域的蛋白基因为204 bp,L. petauri的Lichenan渗透酶IIC成分基因为465 bp,L. garvieae和L. petauri的茶色酸生物合成蛋白F基因均为302 bp。PCR 扩增子在琼脂糖凝胶电泳中被清楚地分离出来。多重 PCR 检测未与非目标细菌的 DNA 产生任何扩增产物。在纯培养物中,L. garvieae 和 L. petauri 的多重 PCR 检测限分别为 5 CFU 和 4 CFU,在加标组织样本中分别为 50 CFU 和 40 CFU/g。平板培养细菌和组织样本的检测结果分别需要不到 2 小时和 3 小时。总之,所开发的多重 PCR 法是一种快速、特异、准确且经济有效的方法,可用于检测和鉴别 L. garvieae 和 L. petauri,适合用于 L. garvieae 和 L. petauri 的常规实验室诊断。
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来源期刊
Journal of fish diseases
Journal of fish diseases 农林科学-海洋与淡水生物学
CiteScore
4.60
自引率
12.00%
发文量
170
审稿时长
6 months
期刊介绍: Journal of Fish Diseases enjoys an international reputation as the medium for the exchange of information on original research into all aspects of disease in both wild and cultured fish and shellfish. Areas of interest regularly covered by the journal include: -host-pathogen relationships- studies of fish pathogens- pathophysiology- diagnostic methods- therapy- epidemiology- descriptions of new diseases
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