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Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes
Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes
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Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes
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Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes
Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes

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Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes
Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes
Journal Article

Analysis of the composition, assembly kinetics and activity of native Apaf-1 apoptosomes

2004
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Overview
The Apaf‐1 apoptosome is a multi‐subunit caspase‐activating scaffold that is assembled in response to diverse forms of cellular stress that culminate in apoptosis. To date, most studies on apoptosome composition and function have used apoptosomes reassembled from recombinant or purified proteins. Thus, the precise composition of native apoptosomes remains unresolved. Here, we have used a one‐step immunopurification approach to isolate catalytically active Apaf‐1/caspase‐9 apoptosomes, and have identified the major constituents of these complexes using mass spectrometry methods. Using this approach, we have also assessed the ability of putative apoptosome regulatory proteins, such as Smac/DIABLO and PHAPI, to regulate the activity of native apoptosomes. We show that Apaf‐1, caspase‐9, caspase‐3 and XIAP are the major constituents of native apoptosomes and that cytochrome c is not stably associated with the active complex. We also demonstrate that the IAP‐neutralizing protein Smac/DIABLO and the tumor‐suppressor protein PHAPI can enhance the catalytic activity of apoptosome complexes in distinct ways. Surprisingly, PHAPI also enhanced the activity of purified caspase‐3, suggesting that it may act as a co‐factor for this protease.