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Detection of Brucella abortus DNA and RNA in different stages of development of the sucking louse Haematopinus tuberculatus

机译:在吮吸性虱子嗜血杆菌的不同发育阶段中检测布鲁氏菌流产DNA和RNA

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摘要

BackgroundBrucellosis is considered the world’s most widespread zoonotic infection. It causes abortion and sterility in livestock leading to serious economic losses and has even more serious medical impact in humans, since it can be a trigger to more than 500,000 infections per year worldwide. The aim of this study was to evaluate the role of Haematopinus tuberculatus, a louse that can parasitize several ruminants, as a new host of brucellosis. Louse specimens were collected from seropositive and seronegative water buffaloes and divided in 3 developmental stages: adults, nymphs and nits. All samples were separately screened for Brucella spp. DNA and RNA detection by Real Time PCR. In particular, primers and probes potentially targeting the 16S rRNA and the Brucella Cell Surface 31 kDalton Protein (bcsp31) genes were used for Real Time PCR and buffalo β actin was used as a housekeeping gene to quantify host DNA in the sample. A known amount of B. abortus purified DNA was utilized for standard curve preparation and the target DNA amount was divided by the housekeeping gene amount to obtain a normalized target value. A further molecular characterization was performed for Brucella strain typing and genotyping by the Bruce-ladder, AMOS-PCR and MLVA assays. Data were statistically analysed by ANOVA.
机译:背景布鲁氏菌病被认为是世界上最广泛的人畜共患病感染。它会导致牲畜的流产和不育,从而造成严重的经济损失,并给人类带来更严重的医学影响,因为它可以引发全球每年超过500,000的感染。这项研究的目的是评估布鲁氏菌(Haematopinus tuberculatus)(一种可以寄生几种反刍动物的虱子)作为布鲁氏菌病的新宿主的作用。从血清阳性和血清阴性的水牛中采集虱子标本,并将其分为三个发育阶段:成虫,若虫和幼虫。分别筛选所有样品的布鲁氏菌属。通过实时PCR检测DNA和RNA。特别地,潜在靶向16S rRNA和布鲁氏菌细胞表面31 kDalton蛋白(bcsp31)基因的引物和探针用于实时PCR,水牛β肌动蛋白用作管家基因来定量样品中的宿主DNA。将已知量的流产芽孢杆菌纯化的DNA用于标准曲线制备,并将目标DNA量除以管家基因量以获得标准化的目标值。通过布鲁斯梯,AMOS-PCR和MLVA分析对布鲁氏菌菌株的分型和基因分型进行了进一步的分子表征。数据通过ANOVA进行统计分析。

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