8 TZ Morogoro Tomato 2008 Ms 8 75% 1 JF743197 JF743349 JF743501 Tanzani 4.1 TZ Arusha Tomato 2008 Ms 8 75% 1 JF743198 JF743350 JF743502 Ms 660 68 haric RE Bras de Ponto Bean 2010 T. vaporar. 10 100% 3 JF743116-18 JF743268-70 JF743420-22 Co_pl RE Tampon 14e Zucchini field 1 2011 T. vaporar. 10 100% 7 JF743088-94 JF743240-46 JF743392-98 Co_p2 RE Tampon 14e Zucchini field 2 2011 T. vaporar. 10 100% 7 JF743095-101 JF743247-253 see more JF743399-405 T. vaporar. 30 17 SaAubF53 RE St Andre
Eggplant 2010 B. afer 2 100% 1 JF743155 JF743307 JF743459 B. afer 2 1 152 T. vaporar. : Trialeurodes vaporariorum. B. afer : Bemisia afer. Country abbreviations stand for France (FR), Spain (ES), Israel (IL), Burkina Faso (BF), Togo (TG), Benin (BJ), Tanzania (TZ), Seychelles (SC), Comoros Grande Comore (KM), Mayotte (YT), Madagascar (MG), Mauritius (MU) and Reunion (RE). Gr.: greenhouse. Gen. gr. : Genetic group. ntot: number of individuals NVP-AUY922 clinical trial screened for Arsenophonus, n: number of individuals used for the phylogenetic analysis. Arsen. Prev.: Arsenophonus prevalence.
Accession numbers are given for fbaA, ftsK and yaeT sequences obtained in this study. Figure 1 Location of sampling sites indicating the presence of the genetic groups of Bemisia tabaci (Q2, Q3, AnSL, ASL, Ms), Bemisia afer and Trialeurodes vaporariorum. Samples were collected in mainland France (FR), Spain (ES), Israel (IL), Burkina Faso (BF), Togo (TG), Benin (BJ), Tanzania (TZ), Seychelles (SC), Comoros Grande Comore (KM), Mayotte (YT), Madagascar (MG), Mauritius (MU) and Reunion (RE). DNA extraction and PCR amplification Arsenophonus detection ifoxetine and identification of B. tabaci genetic groups Insects were sexed and DNA was extracted as previously described by Delatte et al. [49]. All samples were screened for Arsenophonus infection using the specific primers Ars-23S1/Ars-23S2 targeting the 23S RNA gene [50] (Table 2). To check for extracted DNA quality, all samples were also tested for the presence of the primary symbiont
P. aleyrodidarum using specific primers for the 16S rRNA genes described by Zchori-Fein and Brown [23]. When positive signals were recorded in both PCRs, insects were used in the analysis. B. tabaci genetic groups were identified by PCR-RFLP (random fragment length polymorphism) test based on the mitochondrial marker COI (Cytochrome Oxidase 1) gene as described by Gnankine et al. [35] for Q, ASL and AnSL individuals. A set of 10 microsatellite markers was used to identify Ms according to Delatte et al. [42]. Moreover, a portion of the COI gene was sequenced for five individuals from each of the different B. tabaci genetic groups, using the protocol described by Thierry et al. [37] and Gnankine et al.