Kovalenko et al.
Supplementary information
Figures Legends:
Supplementary Fig. 1: «IKK is not the CYLD kinase»
HEK 293T cells were transfected and analyzed as described in Fig. 2a. A dominant negative version of IKK2 which is catalytically defective (IKK2 SS/AA) but still able to interact with NEMO (data not shown) was used to determine whether endogenous IKK was directly or indirectly responsible for CYLD phosphorylation.
Supplementary Fig. 2:«NEMO ubiquitination does not induce proteasome-dependent degradation»
a. HEK 293T cells were transfected with 500 ng of HA-NEMO. Twenty-four hours later, cells were treated for 6 hours with 20 M of the proteasome inhibitor MG132. Cytoplasmic extracts were prepared and NEMO expression was assessed with anti-NEMO. b. Same protocol as in a but NEMO was co-transfected with control vector (Pc) or HA-Ubiquitin (Ub) in the absence (lane 2) or presence (lane 3) of MG132.
Supplementary Fig. 3: «(N393)CYLD exhibits restricted substrate specificity and behaves as a specific negative regulator of TRAF2/NF-B signaling»
a. Deubiquitinating activity of (N393)CYLD. HEK 293T were transfected with 500 ng of TRAF2, 500 ng of HA-Ubiquitin and either 2ug of pcDNA3 (lanes 1,2), wt CYLD-Flag (lanes 3,4) or (N393)CYLD (lanes 5,6). TRAF2 ubiquitination was assessed after Western blotting with anti-TRAF2 and CYLD expression with anti-Flag. b. Same as in a., except that 500 ng of HA-NEMO were transfected instead of TRAF2 and NEMO ubiquitination was analyzed with anti-NEMO. c. Same as in a. except that 500 ng of Flag-TRAF6 were transfected instead of TRAF2 and TRAF6 ubiquitination was analyzed with anti-Flag. d. Same as in a. except that ubiquitination of total cytoplasmic proteins was analyzed with anti-HA after transfecting 500 ng of HA(K48R)ubiquitin.e. Luciferase assay of NF-B activation. HEK 293T cells were transfected with TRAF2 or TRAF6 and the effect of co-transfecting wt CYLD or (N393)CYLD analyzed.
Supplementary Fig. 4: «CYLD acts upstreamof IKK»
a. CYLD overexpression inhibits IKK activation by TNF. HEK 293T cells were transfected with 10 ng of VSV-IKK2 and 2 g of PcDNA3 (Pc) or wt CYLD (CYLD). After 24hours, cells were treated or not with TNF (10 ng/ml for 10 min), the cytoplasmic extracts prepared and immunoprecipitated with anti-VSV. The IKK kinase assay was carried out as described in Yamaoka et al.4. b. CYLD overexpression inhibits TNF-induced IB degradation. HEK 293T cells were transfected with PcDNA3, Myc-IB0.5 gor Myc-IB plus CYLD (2g). Twenty-four hours later cells were stimulated or not with 10 ng/ml TNF for the times indicated and IB degradation was analyzed by Western blotting with anti-IB. IB on the right of the figure indicates the endogenous molecule. c. CYLD does not inhibit the IB degradation step. HEK 293T cells were transfected with Myc IB (0.5 g) and the indicated combinations of the empty vector (Pc), IKK2 SS/EE (a constitutively active form of IKK2; IKK2*, 0.5 g) and wild-type CYLD (2g). Twenty four hours later, cells were treated or not with 20 M of MG132 for 6 hours, as indicated. Cytoplasmic extracts were analyzed with anti-IB. In this setting, CYLD overexpression did not affect IB induced phosphorylation (as shown here using MG132), IB ubiquitination (as shown in Fig. 3e) or IB degradation (as shown here in the absence of MG132).