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库蠓属昆虫及非洲和欧洲蓝舌病(BT)和非洲马瘟(AHS)的主要传播媒介——伊氏库蠓的分子检测。

Molecular detection of Culicoides spp. and Culicoides imicola, the principal vector of bluetongue (BT) and African horse sickness (AHS) in Africa and Europe.

作者信息

Cêtre-Sossah Catherine, Baldet Thierry, Delécolle Jean-Claude, Mathieu Bruno, Perrin Aurélie, Grillet Colette, Albina Emmanuel

机构信息

CIRAD-EMVT, Campus international de Baillarguet, TA30/G, 34398 Montpellier Cedex 5, France.

出版信息

Vet Res. 2004 May-Jun;35(3):325-37. doi: 10.1051/vetres:2004015.

Abstract

Bluetongue (BT) and African Horse Sickness (AHS) are infectious arthropod-borne viral diseases affecting ruminants and horses, respectively. Culicoides imicola Kieffer, 1913, a biting midge, is the principal vector of these livestock diseases in Africa and Europe. Recently bluetongue disease has re-emerged in the Mediterranean Basin and has had a devastating effect on the sheep industry in Italy and on the islands of Sicily, Sardinia, Corsica and the Balearics, but fortunately, has not penetrated onto mainland France and Spain. To survey for the presence of C. imicola, an extensive light-trap network for the collection of Culicoides, was implemented in 2002 in southern mainland France. The morphological identification of Culicoides can be both tedious and time-consuming because its size ranges from 1.5 to 3 mm. Therefore, an ITS1 rDNA polymerase chain reaction (PCR)-based diagnostic assay was developed to rapidly and reliably identify Culicoides spp. and C. imicola. The aim of this work was to set up a rapid test for the detection of C. imicola amongst a pool of insects collected in areas at risk for BT. The sequence similarity of the rDNA (nuclear ribosomal DNA), which is greater within species than between species, is the foundation of its utilisation in species-diagnostic assays. The alignment of the 11 ITS1 sequences of Culicoides obtained from Genbank and EMBL databases helped us to identify one region in the 5' end and one in the 3' end that appear highly conserved. PCR primers were designed within these regions to amplify genus-specific fragments. In order to set up a C. imicola-specific PCR, another forward primer was designed and used in combination with the previously designed reverse primer. These primers proved to be highly specific and sensitive and permitted a rapid diagnostic separation of C. imicola from Culicoides spp.

摘要

蓝舌病(BT)和非洲马瘟(AHS)是分别影响反刍动物和马的传染性节肢动物传播的病毒性疾病。1913年的库蠓(Culicoides imicola Kieffer),一种吸血蠓,是非洲和欧洲这些家畜疾病的主要传播媒介。最近,蓝舌病在地中海盆地再次出现,对意大利的绵羊产业以及西西里岛、撒丁岛、科西嘉岛和巴利阿里群岛造成了毁灭性影响,但幸运的是,尚未蔓延到法国大陆和西班牙。为了调查库蠓的存在情况,2002年在法国大陆南部实施了一个用于收集库蠓的广泛的诱虫灯网络。库蠓的形态鉴定既繁琐又耗时,因为其大小在1.5至3毫米之间。因此,开发了一种基于内转录间隔区1核糖体DNA(ITS1 rDNA)聚合酶链反应(PCR)的诊断检测方法,以快速、可靠地鉴定库蠓属物种和库蠓。这项工作的目的是建立一种快速检测方法,用于在有蓝舌病风险地区收集的昆虫样本中检测库蠓。核糖体DNA(rDNA)的序列相似性在种内比种间更高,这是其在物种诊断检测中应用的基础。从Genbank和EMBL数据库获得的11个库蠓ITS1序列的比对帮助我们确定了5'端和3'端的一个区域,这些区域看起来高度保守。在这些区域内设计了PCR引物,以扩增属特异性片段。为了建立库蠓特异性PCR,设计了另一个正向引物,并与先前设计的反向引物结合使用。这些引物被证明具有高度特异性和敏感性,并允许快速诊断区分库蠓和库蠓属物种。

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