Stephan Anja, Clausen Peter-Henning, Bauer Burkhard, Steuber Stephan
Institute for Parasitology and Tropical Veterinary Medicine, Freie Universitaet Berlin, Koenigsweg 67, 14163, Berlin, Germany.
Parasitol Res. 2009 Aug;105(2):367-71. doi: 10.1007/s00436-009-1407-z. Epub 2009 Mar 24.
Due to the severe outbreaks of bluetongue disease (BTD) in the years 2006/2007 in Germany in the absence of the main African vector Culicoides imicola, a rapid and easy applicable method for identification of autochthonous Culicoides spp. had to be developed. Morphological identification is time-consuming, rendering impossible the identification of large numbers of midges in a short period of time. A polymerase chain reaction (PCR)-based procedure in connection with a species-specific primer greatly simplifies the identification process. The region of internal transcribed spacer 1 (ITS-1) of the ribosomal DNA has shown great potential for developing a reliable PCR-based procedure. Culicoides midges were caught with ultraviolet-light traps installed on different farms in Germany during 2007 and 2008. The midges were mounted on slides and morphologically characterised. Midge DNA was extracted and the ITS-1 region amplified using conservative primers. Potential primer regions within ITS-1 were determined and a species-specific Culicoides dewulfi primer was developed to correctly identify autochthonous C. dewulfi, one of the suspected BTV vectors in northwestern Europe. The developed primer was used to identify C. dewulfi in a pool of Culicoides midges from a farm in the state of Brandenburg.
由于2006/2007年德国蓝舌病(BTD)严重暴发,而主要的非洲传播媒介库蠓不存在,因此必须开发一种快速且易于应用的方法来鉴定本地库蠓种类。形态学鉴定耗时,无法在短时间内鉴定大量蠓虫。基于聚合酶链反应(PCR)并结合物种特异性引物的方法极大地简化了鉴定过程。核糖体DNA的内部转录间隔区1(ITS-1)区域在开发可靠的基于PCR的方法方面显示出巨大潜力。2007年和2008年期间,在德国不同农场安装紫外线诱捕器捕获库蠓。将蠓虫固定在载玻片上并进行形态学特征描述。提取蠓虫DNA,使用保守引物扩增ITS-1区域。确定了ITS-1内的潜在引物区域,并开发了一种物种特异性的德氏库蠓引物,以正确鉴定本地的德氏库蠓,它是欧洲西北部疑似蓝舌病病毒载体之一。所开发的引物用于鉴定来自勃兰登堡州一个农场的库蠓池中的德氏库蠓。
