Fig. 1: NLRP1^CARD interacts with ASC^CARD by homotypic CARD–CARD interaction in solution and cells.

a Size-exclusion chromatograph of the MBP-ASC^CARD/NLRP1^CARD complex. ASC^CARD was fused with an N-terminal His-tag and incubated with untagged NLRP1^CARD, which was first purified by Ni-affinity chromatography. The complex eluted in the void position on a Superdex^TM 24 gel filtration column. b A negative-stain EM image of MBP-ASC^CARD/NLRP1^CARD complex. c Size-exclusion chromatograph of the MBP-ASC^CARD/NLRP1^CARD complex in different salt concentrations. d High salt significantly disrupted filament formation. e Y2H analysis of the NLRP1^CARD and ASC^CARD interaction. Yeast cells co-expressing GAL4 DNA-binding domain (BD)-ASC ^CARD fusion and GAL4 activation domain (AD)-NLRP1^CARD fusion were grown on agar plates lacking leucine and tryptophan (-Leu/-Trp) for transformant growth and lacking histidine, leucine, and tryptophan (-His/-Leu/-Trp) for detecting CARD–CARD interaction. Three individual clones for each combination were plated. (–) denotes empty vector control. f Measurement of the protein–protein interaction of wild-type NLRP1^CARD with ASC^CARD by the M2H experiment. Luciferase activity in the HEK293T cells was normalized to Renilla and data were presented as the fold of negative control. Mean values ± SEM are representative of three independent experiments. g Structure-based sequence alignment of NLRP1^CARD (NP_127497.1) and ASC^CARD (NP_037390.2). Different colors are highlighted to show the interfacial residues involved in the three asymmetric interactions of death domain superfamily. The secondary structure of NLRP1^CARD and ASC^CARD are labeled on the top and bottom, respectively.