Engagement of certain cell surface receptors by the their cognate ligands leads to the rapid induction of cell death by an intracellular suicide program known as apoptosis (1). The signaling pathways employed by these “death receptors” appear to involve the sequential activation of the caspase group of cysteine proteases in an ordered and hierarchical manner (2). A well-described cofactor in this process is FADD, a key adapter protein that mediates the recruitment of proximal caspases to the cell surface receptor (3). However, a recent report by Bannerman et al. in the JCI (4) reveals an intriguing additional function for FADD as a regulator of the transcription factor NF-κB. FADD is best known as an intracellular factor that, upon ligand binding, is recruited to the cytoplasmic domain of Fas (also known as Apo-1 and CD95), a member of the TNF receptor (TNFR) superfamily (5, 6). Fas and FADD associate through a conserved motif known as the death domain (DD), which is found in both the Fas cytoplasmic tail and the FADD protein (7). In turn, FADD can recruit certain caspases, notably caspase-8, through a second element known as the death effector domain, present in FADD and in the prodomain of the caspase. How might FADD control the apparently unrelated NF-κB pathway? A complex relationship exists between the control of apoptosis and NF-κB. Studies of signaling through the type 1 TNFR (TNFR1) have demonstrated the activation of both a proapoptotic pathway (similar to the Fas mechanism) and NF-κB (8); in this case activation of NF-κB appears to provide a prosurvival signal whose mechanism is still unclear but that is presumed to involve the transcriptional induction of various apoptotic suppressors (9). As reviewed recently by Budd (10), variations on this theme are numerous and may be cell type–specific. The existence of these two opposing signals may explain why many cells bearing TNF receptors do not undergo apoptosis upon TNF binding. Similarly, the proinflammatory molecule lipopolysaccharide (LPS) can act through the Toll-like receptor Tlr-4 to induce caspase and NF-κB activation. Some of the intracellular components involved in Tlr-4 signaling are different (the adapters MyD88, FADD, and the NF-κB–activating kinase IRAK are recruited to the Tlr-4 cytoplasmic domain in the latter pathway), but the paradigm is the same: caspases are activated, but so is NF-κB (11). The report by Bannerman et al.(4) shows that FADD can function in both pathways to activate apical caspases while at the same time suppressing NF-κB signaling (Figure 1). The precise manner in which FADD achieves this is still unclear. The authors speculate that through binding to MyD88, FADD might competitively displace IRAK from the complex. An alternative mechanism would be the direct binding of FADD to IRAK. As pointed out by Bannerman et al.(4), previous studies have found that

FADD can act as a suppressor—and not, as in this report, an inducer—of NF-κB (12–14). One of the most significant experimental differences between these reports is the use by Bannerman et al. of lines containing stably overexpressed FADD, as well as lines derived from FADD-deficient mice. In contrast, the earlier studies employed transient overexpression of FADD. Differences in cell type and the nature of the stimulus may also have a profound influence. Indeed, Bannerman et al. found that, whereas FADD-deficient embryonic fibroblasts show heightened induction of NF-κB following LPS treatment, their response to TNF is normal (4). Perhaps the most fascinating question arising from these studies concerns the physiologic advantage of coordinating caspase induction …