Project description:Induction Spodoptera midgut after induction by benzoxazinoids

Project description:Sf9 induction with 8 compounds

Project description:L6 larvae midgut expression after induction by either DIBOA or DIMBOA treatment1: DIBOA (13.5mM) versus DMSO (control) treatment2: DIMBOA (13.5mM) versus DMSO (control) DIBOA (2,4-Dihydroxy-1,4-benzoxazin-3-one glucoside) and DIMBOA (2,4-dihydroxy-7-methoxy-1,4-benzoxazin-3-one) are benzoxazinoids compounds

Project description:Midgut gene expression after induction by 11 compounds: each treatment was done in biological triplicate and using dye swap resulting in 6 microarrays per treatment. on each microarray a treated midgut RNA was compared to a DMSO treated midgut RNA. indole3carbinol, xanthotoxine, 2tridecanone, clofibrate, indole, phenobarbital, quercetine, methoprene, methoxyfenozide, deltamethrine and fipronil

Project description:Sf9 induction with phenobarbital

Project description:Sf9 induction with methoxyfenozide and methoprene

Project description:Accurate chromosome segregation requires assembly of the multiprotein kinetochore complex at centromeres. In most eukaryotes, kinetochore assembly is primed by the histone H3 variant CenH3, which physically interacts with components of the inner kinetochore constitutive-centromere-associated-network (CCAN). Unexpected to its critical function, previous work identified that select eukaryotic lineages, including several insects, have lost CenH3, while having retained homologs of the CCAN. These findings imply alternative CCAN assembly pathways in these organisms that function in CenH3-independent manners. Here, we study the composition and assembly of CenH3-independent kinetochores of Lepidoptera. We show that lepidopteran kinetochores consist of previously identified CCAN homologs as well as additional components including a divergent CENP-T homolog, which are required for accurate mitotic progression. Our study focuses on CENP-T that we find both necessary and sufficient to recruit the Mis12 outer kinetochore complex. In addition, CRISPR-mediated gene editing in Bombyx mori establishes an essential function of CENP-T in vivo. Finally, the retention of CENP-T homologs in other independently-derived CenH3-deficient insects indicates a conserved mechanism of kinetochore assembly between these lineages. Our study provides the first functional insights into CCAN-based kinetochore assembly pathways that function independently of CenH3, thus contributing to the emerging picture of an unexpected plasticity to build a kinetochore.

Project description:Spodoptera frugiperda Transcriptome or Gene expression

Project description:Spodoptera frugiperda Transcriptome or Gene expression

Project description:Spodoptera frugiperda Transcriptome or Gene expression