Likewise, when we looked at the sections by fluorescence microscopy we observed that the number of calcein-labelled surfaces, as well as the distance between calcein labelling fronts was dramatically reduced in Col blasts, which were isolated from calvariae and differentiated ex vivo

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llagenase treatment. Dissociated cells were fixed and stained for DNA synthesis and nucleus following manufacturer’s protocol. Cells were counted in a fluorescence microscope. In order to determine whether exposure to XentariTM modulated the cell proliferation rate, last instar larvae from FRA were previously exposed to XentariTM at two different concentrations by surface contamination. 24195657 After two h exposure larvae were injected with EdU and processed as described above. Analysis of the correlation between gene expression and resistance For correlation experiments, 2nd instar larvae from Xen-RU were exposed to a sublethal dose of XentariTM using surface contamination. Briefly, a total of two hundred synchronous larvae were selected and fed for 6 d on artificial diet containing XentariTM at 25 mg/cm2. At the end of the assay, larvae were weighed individually, midguts dissected, and immediately stored at 280uC for further analysis. Subsequently, final weights of tested larvae were distributed in 5 mg intervals. Midguts from individual insects highly affected and from insects hardly affected by Xentari were used 17888033 for measuring the expression level of the candidate genes. RNA from midguts were isolated and transcript abundance was obtained by qRT-PCR as described above. Expression ratios were calculated in relation to the FRA colony using different pools of FRA larvae with similar mean wt than the S- and B-group, respectively. Correlation between gene expression level and larval wt was analyzed using the Pearson correlation coefficient using the GraphPad Prism program. Supporting Information Aminopeptidase activity in the midgut lumen Last instar FRA and Xen-R larvae were exposed to Cry1Ca protoxin in 50 mM carbonate buffer for 12 hours using diet surface contamination. Non exposed insects were treated side-by-side with the same buffer. Midguts were isolated and their contents were obtained by manually discarding of the midgut tissues. The contents were then transferred into 50 mM Tris-HCl pH 8 buffer containing 1 mM PMSF. For each BMS-345541 measurement, contents from at least 5 midguts were pooled, vortex mixed for 30 s, centrifuged at maximum speed for 5 min at 4uC and the supernatant was used Acknowledgments We are grateful to the people from the DNA-array facilities at the SCSIE, Universitat de Valencia. We also want to thank Manuela Barneo for her excellent help with insect rearing. Author Contributions Conceived and designed the experiments: PHM GNC SC RAdM WJM JF BE SH. Performed the experiments: PHM GNC SC SH. Analyzed the data: PHM GNC SC SH. Contributed reagents/materials/analysis tools: RAdM WJM. Wrote the paper: PHM RAdM WJM JF SH. 9 September 2010 | Volume 5 | Issue 9 | e12795 Bt-Resistance in S. exigua 13. Gunning RV, Dang HT, Kemp FC, Nicholson IC, Moores GD New resistance mechanism in Helicoverpa armigera threatens transgenic crops expressing Bacillus thuringiensis Cry1Ac toxin. Appl Environ Microbiol 71: 2558563. 14. Ma G, Roberts H, Sarjan M, Featherstone N, Lahnstein J, et al. Is the mature endotoxin Cry1Ac from Bacillus thuringiensis inactivated by a coagulation reaction in the gut lumen of resistant Helicoverpa armigera larvae Insect Biochem Mol Biol 35: 72939. 15. Martinez-Ramirez AC, Gould F, Ferre J Histopathological effects and growth reduction in a susceptible and a resistant strain of heliothis virescens caused by sublethal doses of pure Cry1A Crystal proteins from Bacillus thuringiensis. Biocontrol Science and Technology 9: