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在从毛里塔尼亚牛身上采集的蜱虫(蜱螨亚纲:硬蜱科)中通过聚合酶链反应检测环形泰勒虫

Detection of Theileria annulata by the PCR in ticks (Acari:Ixodidae) collected from cattle in Mauritania.

作者信息

d'Oliveira C, van der Weide M, Jacquiet P, Jongejan F

机构信息

Department of Parasitology and Tropical Veterinary Medicine, Faculty of Veterinary Medicine, Utrecht University, The Netherlands.

出版信息

Exp Appl Acarol. 1997 May;21(5):279-91. doi: 10.1023/a:1018455223462.

Abstract

We report on the detection of Theileria annulata in infected Hyalomma ticks by the PCR using primers derived from the gene encoding the 30 kDa major merozoite surface antigen (TamsI-1). No inhibition of the PCR was observed and as little as 0.1 pg of parasite DNA, corresponding to 12 sporozoites, could be detected in non-infected tick DNA samples, spiked with T. annulata genomic DNA. Hyalomma dromedarii ticks, fed on a calf experimentally infected with T. annulata, were used to validate the PCR further. The infection rate in the adult ticks, fed as nymphs during the febrile reaction, was high (62%), dropped to zero for 1 day in tick batches that engorged after treatment with Butalex and increased to 30% 2 days later and 38% of the ticks acquired the infection after feeding as nymphs during a carrier state piroplasm parasitaemia of less than 0.1%. As an internal control, 16S tick rDNA sequences could be amplified from T. annulata-negative tick samples. Finally, 202 adult ticks from Mauritania, collected from zebu cattle carrying low levels of Theileria piroplasms, were tested by the PCR. Thirty-eight out of 52 (73%) and 17 out of 30 (57%) H. dromedarii from the Gorgol and Trarza regions, respectively and two out of 30 (7%) Hyalomma marginatum rufipes from the Gorgol region were positive. Hyalomma marginatum rufipes, Rhipicephalus evertsi evertsi and Rhipicephalus guilhoni from the Trarza region were negative. These findings confirm that H. dromedarii is the main vector of T. annulata in Mauritania and that the PCR is a useful method of determining the infection rates in ticks collected from cattle carrying low levels of T. annulata piroplasms.

摘要

我们报告了使用源自编码30 kDa主要裂殖子表面抗原(TamsI-1)的基因的引物,通过PCR在感染环形泰勒虫的璃眼蜱中检测到该病原体。未观察到PCR受到抑制,在加入环形泰勒虫基因组DNA的未感染蜱DNA样本中,可检测到低至0.1 pg的寄生虫DNA,相当于12个孢子体。用实验感染环形泰勒虫的小牛喂养的单峰驼璃眼蜱,用于进一步验证PCR。在发热反应期间以若虫形式进食的成年蜱中,感染率很高(62%),在用Butalex处理后饱血的蜱批次中,感染率在1天内降至零,2天后升至30%,在携带低于0.1%的梨形虫血症的带虫状态下以若虫形式进食后,38%的蜱感染。作为内部对照,可从环形泰勒虫阴性的蜱样本中扩增出16S蜱rDNA序列。最后,对从携带低水平泰勒梨形虫的瘤牛采集的202只来自毛里塔尼亚的成年蜱进行了PCR检测。分别来自戈尔戈尔和特拉扎地区的52只单峰驼璃眼蜱中的38只(73%)和30只中的17只(57%)呈阳性,来自戈尔戈尔地区的30只边缘璃眼蜱中的2只(7%)呈阳性。来自特拉扎地区的边缘璃眼蜱、埃氏扇头蜱和吉尔氏扇头蜱均为阴性。这些发现证实,单峰驼璃眼蜱是毛里塔尼亚环形泰勒虫的主要传播媒介,并且PCR是确定从携带低水平环形泰勒虫梨形虫的牛身上采集的蜱的感染率的有用方法。

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