A new tool for the molecular identification of Culicoides species of the Obsoletus group: the glass slide microarray approach

被引:11
作者
DeBlauwe, I. [1 ]
De Witte, J. C. [1 ]
De Deken, G. [1 ]
De Deken, R. [1 ]
Madder, M. [1 ,2 ]
Van Erk, S. [1 ]
Hoza, F. A. [1 ]
Lathouwers, D. [1 ]
Geysen, D. [1 ]
机构
[1] Inst Trop Med, Dept Anim Hlth, B-2000 Antwerp, Belgium
[2] Univ Pretoria, Fac Vet Sci, Dept Vet Trop Dis, ZA-0002 Pretoria, South Africa
关键词
Culicoides obsoletus s; l; bluetongue; identification; internal transcribed spacer 1; microarray; molecular detection; probe hybridization; vector; HORSE SICKNESS AHS; BLUETONGUE VIRUS; CERATOPOGONIDAE; DIPTERA; IMICOLA; VECTOR; PCR; OUTBREAK; AFRICA; EUROPE;
D O I
10.1111/j.1365-2915.2011.00979.x
中图分类号
Q96 [昆虫学];
学科分类号
摘要
Culicoides species of the Obsoletus group (Diptera: Ceratopogonidae) are potential vectors of bluetongue virus serotype 8 (BTV 8), which was introduced into central Western Europe in 2006. Correct morphological species identification of Obsoletus group females is especially difficult and molecular identification is the method of choice. In this study we present a new molecular tool based on probe hybridization using a DNA microarray format to identify Culicoides species of the Obsoletus group. The internal transcribed spacer 1 (ITS1) gene sequences of 55 Culicoides belonging to 13 different species were determined and used, together with 19 Culicoides ITS1 sequences sourced from GenBank, to design species-specific probes for the microarray test. This test was evaluated using the amplified ITS1 sequences of another 85 Culicoides specimens, belonging to 11 species. The microarray test successfully identified all samples (100%) of the Obsoletus group, identifying each specimen to species level within the group. This test has several advantages over existing polymerase chain reaction (PCR)-based molecular tools, including possible capability for parallel analysis of many species, high sensitivity and specificity, and low background signal noise. Hand-spotting of the microarray slide and the use of detection chemistry make this alternative technique affordable and feasible for any diagnostic laboratory with PCR facilities.
引用
收藏
页码:83 / 91
页数:9
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