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通过TaqMan MGB实时荧光定量PCR法重新检测中欧北美小龙虾种群中嗜酸性卵甲藻的流行情况。

Re-examination of the prevalence of Aphanomyces astaci in North American crayfish populations in Central Europe by TaqMan MGB real-time PCR.

作者信息

Kozubíková Eva, Vrålstad Trude, Filipová Lenka, Petrusek Adam

机构信息

Department of Ecology, Faculty of Science, Charles University in Prague, 12844 Prague 2, Czech Republic.

出版信息

Dis Aquat Organ. 2011 Dec 6;97(2):113-25. doi: 10.3354/dao02411.

DOI:10.3354/dao02411
PMID:22303628
Abstract

We applied quantitative TaqMan minor groove binder real-time polymerase chain reaction (PCR) on DNA isolates from soft abdominal cuticle of 460 North American crayfish Orconectes limosus and Pacifastacus leniusculus, previously tested for Aphanomyces astaci presence by conventional semi-nested PCR. Both approaches target the internal transcribed spacers of the pathogen nuclear ribosomal DNA, but apply different specific sequence motifs and technologies. The real-time PCR approach seems to provide higher sensitivity; the number of crayfish that tested positive increased from 23 to 32%, and 10 additional crayfish populations were indicated as hosting the disease agent. However, the vast majority of newly recorded positives contained very low agent levels, from 5 to 50 PCR-forming units. An isolate producing a false positive result by the semi-nested PCR (apparently undescribed Aphanomyces related to A. astaci) remained negative using the real-time PCR. The present study shows that previous results based on the semi-nested PCR were not substantially influenced by false positives but might have suffered from some false negatives at low agent levels. Combining alternative methods may therefore provide more reliable conclusions on the pathogen's presence. Further, we found positive correlation between the prevalence of infection carriers in American crayfish populations and the average amounts of A. astaci DNA detected in infected local crayfish individuals.

摘要

我们对460只北美螯虾(奥氏原螯虾和美洲鳌虾)腹部软角质层的DNA分离物进行了定量TaqMan小沟结合物实时聚合酶链反应(PCR),这些螯虾之前已通过传统半巢式PCR检测过是否存在螯虾瘟病原菌。两种方法均针对病原体核糖体DNA的内转录间隔区,但应用了不同的特定序列基序和技术。实时PCR方法似乎具有更高的灵敏度;检测呈阳性的螯虾数量从23%增加到32%,另外有10个螯虾种群被指出携带有病原体。然而,绝大多数新记录的阳性样本中病原体水平非常低,为5到50个PCR形成单位。一个通过半巢式PCR产生假阳性结果的分离株(显然是一种未描述的与螯虾瘟病原菌相关的丝囊霉属真菌),使用实时PCR检测时呈阴性。本研究表明,基于半巢式PCR的先前结果并未受到假阳性的实质性影响,但在病原体水平较低时可能存在一些假阴性。因此,结合多种方法可能会对病原体的存在得出更可靠的结论。此外,我们发现美国螯虾种群中感染携带者的患病率与受感染的当地螯虾个体中检测到的螯虾瘟病原菌DNA平均含量之间存在正相关。

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