Characterization of microsatellite DNA libraries from three mealybug species and development of microsatellite markers for Pseudococcus viburni (Hemiptera: Pseudococcidae)

被引:0
|
作者
Correa, M. C. G. [1 ]
Zaviezo, T. [1 ]
Le Maguet, J. [2 ,3 ]
Herrbach, E. [2 ]
Malausa, T. [4 ]
机构
[1] Pontificia Univ Catolica Chile, Fac Agron & Ingn Forestal, Santiago, Chile
[2] INRA, UMR SVQV INRA UDS, Equipe ViVe, F-68000 Colmar, France
[3] Inst Francais Prod Cidricoles, F-61500 La Rangee Chesnel, Sees, France
[4] INRA, UMR ISA INRA UNSA CNRS, Equipe BPI, F-06903 Sophia Antipolis, France
关键词
Microsatellite; SSR; next-generation sequencing; 454; Comstock mealybug; Obscure mealybug; Bohemian mealybug; MOLECULAR-IDENTIFICATION; MORPHOLOGICAL CHARACTERIZATION; CITRUS; DIFFERENTIATION; POPULATIONS; MANAGEMENT; HOMOPTERA; SOFTWARE; TAXA;
D O I
10.1017/S0007485313000667
中图分类号
Q96 [昆虫学];
学科分类号
摘要
Mealybugs (Hemiptera: Pseudococcidae) are important pests for crops worldwide. Different species, cryptic taxa under the same species name or even populations within a species can differ in biological characteristics, such as phenology, resistance to insecticides, virus transmission and susceptibility to natural enemies. Therefore, their management efficacy depends on their accurate identification. Microsatellite genetic markers are efficient in revealing the fine-scale taxonomic status of insects, both at inter- and intra-specific level. Despite their potential uses, microsatellites have been developed only for one mealybug species so far. Hence, it is unclear whether microsatellites may be useful to assess mealybug population differentiation and structuring. In this work, we tested the feasibility of developing microsatellite markers in mealybugs by: (i) producing and characterizing microsatellite DNA libraries for three species: Pseudococcus viburni, Pseudococcus comstocki and Heliococcus bohemicus, and (ii) by developing and testing markers for Ps. viburni. The obtained libraries contained balanced percentages of dinucleotide (ranging from 15 to 25%) and trinucleotide (from 5 to 17%) motifs. The marker setup for Ps. viburni was successful, although 70% of the primers initially tested were discarded for a lack of polymorphism. Finally, 25 markers were combined in two multiplex polymerase chain reactions with 21 displaying no evidence of deviation from Hardy-Weinberg equilibrium. Ps. viburni markers were tested on one population from France and one from Chile. The markers revealed a significant genetic differentiation between the two populations with an Fst estimate of 0.266.
引用
收藏
页码:213 / 220
页数:8
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