Odes and their hosts. Accurate color description is a major difficulty in taxonomic works (Aguiar 2005), and often its variation within and between species can lead to confusion. In Microgastrinae, as in many other groups, the color pattern of body regions seems to be more important and taxonomically informative than the definition of the color per se. Accordingly, in the Lucid dataset, we used a simplified convention to code color, considering it as purchase NVP-BEZ235 either pale (white, light yellow, orange-yellow, light brown-yellow) or dark (dark brown, black). For details on the exact color patterns on the body, we provide extensive illustrations for every species. When describing leg color (especially metacoxa, metafemur, and metatibia), we are referring to the outer side of the leg, e.g., sensu figure 1 of Goulet and Huber (1993). Most of the photos were taken with a Canon EOS 60D with MPE-65 lenses (aperture: 4.0, ISO: 100, CR2 format images), and a 600EX-RT Speedlight (manual) flash. The camera was mounted on a Kaiser copy stand with a Z-stepper (Stackshot) to allow for taking of multiple images. A dozen species were photographed with a Keyence VHX-1000 Digital Microscope, using a lens with a range of 13?30 ? Multiple images through the focal plane were taken of a structure and these were combined to produce a single in-focus image. For the pictures taken with the Canon camera, the Zerene Stacker program (http://zerenesystems.com/cms/stacker) was used; the software associated with the Keyence System produced the focused images taken with that camera. Plates for the illustrations were prepared using Adobe Photoshop CS4. Although the keys provided in this paper are based on morphological characters, in a few cases (mainly with species belonging to the leucostigmus group) we used molecular characters to differentiate species that are morphologically exceptionally similar to each other. In those cases we used characteristic loci in the DNA barcoding region in identification couplets. The bases are numbered from the start of the COI gene according to the reference sequence U37541 (Drosophila melanogaster). The bases noted are only diagnostic within the couplet and beneath that described split. A hypothetical example of the format used is: “A total of 11 diagnostic characters in the barcoding region: 12 A, 18 C, 22 A, 23 T, 44 C, 56 G, 120 G, 340 A, 488 T, 502 T, 601 A”. The letters A, C, G, and T order Biotin-VAD-FMK correspond to adenine, cytosine, guanine, and thymine respectively.Jose L. Fernandez-Triana et al. / ZooKeys 383: 1?65 (2014)Figure 1. Bayesian Maximum Clade Credibility Tree (MCCT) for 180 species of Mesoamerican Apanteles with over 500 bp in the barcoding region and 29 species from other genera used as outgroups. Posterior probabilities over 0.50 are shown on the left side of nodes. Scale bar indicates branch length, expressed as the expected number of substitutions per site.Review of Apanteles sensu stricto (Hymenoptera, Braconidae, Microgastrinae)…DNA barcodes for all ACG inventory Microgastrinae (Appendix 2) were obtained using DNA extracts prepared from single legs using a glass fibre protocol (Ivanova et al. 2006). Extracts were re-suspended in 30 l of dH2O, and a 658-bp region near the 5′ terminus of the COI gene was amplified using standard primers (LepF1 epR1) following established protocols (Smith et al. 2006, 2007, 2008). If the initial 658 bp amplification was not successful, composite sequences were generated using internal primers. Primer inf.Odes and their hosts. Accurate color description is a major difficulty in taxonomic works (Aguiar 2005), and often its variation within and between species can lead to confusion. In Microgastrinae, as in many other groups, the color pattern of body regions seems to be more important and taxonomically informative than the definition of the color per se. Accordingly, in the Lucid dataset, we used a simplified convention to code color, considering it as either pale (white, light yellow, orange-yellow, light brown-yellow) or dark (dark brown, black). For details on the exact color patterns on the body, we provide extensive illustrations for every species. When describing leg color (especially metacoxa, metafemur, and metatibia), we are referring to the outer side of the leg, e.g., sensu figure 1 of Goulet and Huber (1993). Most of the photos were taken with a Canon EOS 60D with MPE-65 lenses (aperture: 4.0, ISO: 100, CR2 format images), and a 600EX-RT Speedlight (manual) flash. The camera was mounted on a Kaiser copy stand with a Z-stepper (Stackshot) to allow for taking of multiple images. A dozen species were photographed with a Keyence VHX-1000 Digital Microscope, using a lens with a range of 13?30 ? Multiple images through the focal plane were taken of a structure and these were combined to produce a single in-focus image. For the pictures taken with the Canon camera, the Zerene Stacker program (http://zerenesystems.com/cms/stacker) was used; the software associated with the Keyence System produced the focused images taken with that camera. Plates for the illustrations were prepared using Adobe Photoshop CS4. Although the keys provided in this paper are based on morphological characters, in a few cases (mainly with species belonging to the leucostigmus group) we used molecular characters to differentiate species that are morphologically exceptionally similar to each other. In those cases we used characteristic loci in the DNA barcoding region in identification couplets. The bases are numbered from the start of the COI gene according to the reference sequence U37541 (Drosophila melanogaster). The bases noted are only diagnostic within the couplet and beneath that described split. A hypothetical example of the format used is: “A total of 11 diagnostic characters in the barcoding region: 12 A, 18 C, 22 A, 23 T, 44 C, 56 G, 120 G, 340 A, 488 T, 502 T, 601 A”. The letters A, C, G, and T correspond to adenine, cytosine, guanine, and thymine respectively.Jose L. Fernandez-Triana et al. / ZooKeys 383: 1?65 (2014)Figure 1. Bayesian Maximum Clade Credibility Tree (MCCT) for 180 species of Mesoamerican Apanteles with over 500 bp in the barcoding region and 29 species from other genera used as outgroups. Posterior probabilities over 0.50 are shown on the left side of nodes. Scale bar indicates branch length, expressed as the expected number of substitutions per site.Review of Apanteles sensu stricto (Hymenoptera, Braconidae, Microgastrinae)…DNA barcodes for all ACG inventory Microgastrinae (Appendix 2) were obtained using DNA extracts prepared from single legs using a glass fibre protocol (Ivanova et al. 2006). Extracts were re-suspended in 30 l of dH2O, and a 658-bp region near the 5′ terminus of the COI gene was amplified using standard primers (LepF1 epR1) following established protocols (Smith et al. 2006, 2007, 2008). If the initial 658 bp amplification was not successful, composite sequences were generated using internal primers. Primer inf.