Systematic in vivo RNAi analysis of putative components of the Drosophila cell death machinery
pmid: 16485033
Systematic in vivo RNAi analysis of putative components of the Drosophila cell death machinery
Despite the identification of numerous key players of the cell death machinery, little is known about their physiological role. Using RNA interference (RNAi) in vivo, we have studied the requirement of all Drosophila caspases and caspase-adaptors in different paradigms of apoptosis. Of the seven caspases, Dronc, drICE, Strica and Decay are rate limiting for apoptosis. Surprisingly, Hid-mediated apoptosis requires a broader range of caspases than apoptosis initiated by loss of the caspase inhibitor DIAP1, suggesting that Hid causes apoptosis not only by antagonizing DIAP1 but also by activating DIAP1-independent caspase cascades. While Hid killing requires Strica, Decay, Dronc/Dark and drICE, apoptosis triggered by DIAP1 depletion merely relied upon Dronc/Dark and drICE. Furthermore, we found that overexpression of DIAP2 can rescue diap1-RNAi-mediated apoptosis, suggesting that DIAP2 regulates caspases directly. Consistently, we show that DIAP2 binds active drICE. Since DIAP2 associates with Hid, we propose a model whereby Hid co-ordinately targets both DIAP1 and DIAP2 to unleash drICE.
- National Institute of Genetics Japan
- Gulbenkian Institute for Molecular Medicine Portugal
- University College London United Kingdom
- Institute of Cancer Research United Kingdom
- Breast Cancer Over Time United States
Apoptosis, Genes, Insect, Eye, Caspase Inhibitors, Models, Biological, Inhibitor of Apoptosis Proteins, Animals, Genetically Modified, Phenotype, Caspases, Animals, Drosophila Proteins, Drosophila, RNA Interference, Signal Transduction
Apoptosis, Genes, Insect, Eye, Caspase Inhibitors, Models, Biological, Inhibitor of Apoptosis Proteins, Animals, Genetically Modified, Phenotype, Caspases, Animals, Drosophila Proteins, Drosophila, RNA Interference, Signal Transduction
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