ABSTRACT
Repair of double-strand breaks (DSBs) in somatic cells is primarily accomplished by error-prone nonhomologous end joining and less frequently by precise homology-directed repair preferentially using the sister chromatid as a template. Here, a Drosophila system performs efficient somatic repair of both DSBs and single-strand breaks (SSBs) using intact sequences from the homologous chromosome in a process we refer to as homologous chromosome-templated repair (HTR). Unexpectedly, HTR-mediated allelic conversion at the white locus was more efficient (40 to 65%) in response to SSBs induced by Cas9-derived nickases D10A or H840A than to DSBs induced by fully active Cas9 (20 to 30%). Repair phenotypes elicited by Nickase versus Cas9 differ in both developmental timing (late versus early stages, respectively) and the production of undesired mutagenic events (rare versus frequent). Nickase-mediated HTR represents an efficient and unanticipated mechanism for allelic correction, with far-reaching potential applications in the field of gene editing.
Subject(s)
Deoxyribonuclease I , Drosophila , Alleles , Animals , CRISPR-Cas Systems , ChromatidsABSTRACT
A recurring target-site mutation identified in various pests and disease vectors alters the voltage gated sodium channel (vgsc) gene (often referred to as knockdown resistance or kdr) to confer resistance to commonly used insecticides, pyrethroids and DDT. The ubiquity of kdr mutations poses a major global threat to the continued use of insecticides as a means for vector control. In this study, we generate common kdr mutations in isogenic laboratory Drosophila strains using CRISPR/Cas9 editing. We identify differential sensitivities to permethrin and DDT versus deltamethrin among these mutants as well as contrasting physiological consequences of two different kdr mutations. Importantly, we apply a CRISPR-based allelic-drive to replace a resistant kdr mutation with a susceptible wild-type counterpart in population cages. This successful proof-of-principle opens-up numerous possibilities including targeted reversion of insecticide-resistant populations to a native susceptible state or replacement of malaria transmitting mosquitoes with those bearing naturally occurring parasite resistant alleles.
Subject(s)
Alleles , Drosophila melanogaster/genetics , Drosophila melanogaster/physiology , Insecticide Resistance/genetics , Animals , CRISPR-Cas Systems , Culicidae , Female , Genetic Engineering , Insecticides , Male , MutationABSTRACT
The neonicotinoid thiamethoxam is widely used in different agricultural crops, and it has a spectrum of action against insects, affecting both pests and pollinators, such as bees. In this study, the effects of exposure to sublethal concentrations of thiamethoxam on stingless bees Scaptotrigona bipunctata were evaluated. Foragers bees were exposed to the insecticide and subjected to genetic biochemical, histochemical, and morphological analyses after 24, 48, and 72 h of ingestion. Analysis of isoenzyme esterases revealed significant alterations in the relative activity of EST-4, a type II cholinesterase. Evaluation of the S. bipunctata brain revealed changes in the state of chromatin condensation according to the exposure time and concentration of neonicotinoid compared with the control. Morphological changes were observed in the midgut of this species at all concentrations and exposure times, which may interfere with various physiological processes of these insects. We can conclude that, although thiamethoxam at the concentrations evaluated did not cause high mortality, it induced concentration-dependent changes in bees by activating enzymes related with the protection for xenobiotic, internal morphology and probably these changes may lead to alterations in the activity of bees.
Subject(s)
Bees/drug effects , Insecticides/toxicity , Neonicotinoids/toxicity , Nitro Compounds/toxicity , Oxazines/toxicity , Thiazoles/toxicity , Animals , Bees/metabolism , Cholinesterases/metabolism , ThiamethoxamABSTRACT
Several recent studies have elucidated the molecular mechanisms that confer insecticide resistance on insect pests. However, little is known about multiple resistance in red flour beetle (Tribolium castaneum) at molecular level. The multiple resistance is characterized as resistance to different classes of insecticides that have different target sites, and is mediated by several enzymatic systems. In this study, we investigated the biochemical and molecular mechanisms involved in multiple resistance of T. castaneum to bifenthrin (pyrethroid [Pyr]) and pirimiphos-methyl (organophosphate [Org]). We used artificial selection, biochemical and in silico approaches including structural computational biology. After five generations of artificial selection in the presence of bifenthrin (F5Pyr) or pirimiphos-methyl (F5Org), we found high levels of multiple resistance. The hierarchical enzymatic cluster revealed a pool of esterases (E), lipases (LIPs) and laccase2 (LAC2) potentially contributing to the resistance in different ways throughout development, after one or more generations in the presence of insecticides. The enzyme-insecticide interaction network indicated that E2, E3, LIP3, and LAC2 are enzymes potentially required for multiple resistance phenotype. Kinetic analysis of esterases from F5Pyr and F5Org showed that pirimiphos-methyl and specially bifenthrin promote enzyme inhibition, indicating that esterases mediate resistance by sequestering bifenthrin and pirimiphos-methyl. Our computational data were in accordance with kinetic results, indicating that bifenthrin has higher affinity at the active site of esterase than pirimiphos-methyl. We also report the capability of these insecticides to modify the development in T. castaneum. Our study provide insights into the biochemical mechanisms employed by T. castaneum to acquire multiple resistance.
