Figure 4
Figure 4. SBDS interacts directly with the GTPase EFL1 to jointly trigger eIF6 eviction. (A) In vivo interaction between endogenous SBDS and EFL1FLAG. Lyzates from eflAFLAG cells treated with DSP (+) or vehicle (DMSO) alone (-DSP) were immunoprecipitated with isotype control (IgG), anti-SBDS or anti-FLAG antibodies and the indicated proteins visualized by immunoblotting. Input represents 5% material used for immunoprecipitations. (B) In vivo interaction between endogenous SBDS and EFL1FLAG is RNA-dependent. Lyzates were immunoprecipitated as in panel A after treatment with ribonuclease (RNase) before (bottom) or after (top) incubation with DSP. (C) Direct interaction between SBDS and EFL1FLAG in vivo. Lyzates from eflAFLAG cells treated with the crosslinker DSS were immunoprecipitated as in panel A. Native (arrowheads) and crosslinked (brackets) SBDS and EFL1FLAG were visualized by immunoblotting (IB). Cell lysate untreated with DSS (1% of input) was loaded as a control (left). *Indicates mouse IgG heavy chain. (D) Human SBDS and EFL1 jointly catalyze eIF6 release. The indicated combinations of recombinant human SBDS and EFL1 (wild-type or the catalytically inactive mutants EFL1T33A and EFL1H96A) were incubated with pre-60S subunits purified from sbdSint(ts) cells in the presence of GTP, GDP or the nonhydrolysable analog GDPNP. “Free” and “bound” fractions from sucrose cushions were immunoblotted to detect eIF6 and Rpl8.

SBDS interacts directly with the GTPase EFL1 to jointly trigger eIF6 eviction. (A) In vivo interaction between endogenous SBDS and EFL1FLAG. Lyzates from eflAFLAG cells treated with DSP (+) or vehicle (DMSO) alone (-DSP) were immunoprecipitated with isotype control (IgG), anti-SBDS or anti-FLAG antibodies and the indicated proteins visualized by immunoblotting. Input represents 5% material used for immunoprecipitations. (B) In vivo interaction between endogenous SBDS and EFL1FLAG is RNA-dependent. Lyzates were immunoprecipitated as in panel A after treatment with ribonuclease (RNase) before (bottom) or after (top) incubation with DSP. (C) Direct interaction between SBDS and EFL1FLAG in vivo. Lyzates from eflAFLAG cells treated with the crosslinker DSS were immunoprecipitated as in panel A. Native (arrowheads) and crosslinked (brackets) SBDS and EFL1FLAG were visualized by immunoblotting (IB). Cell lysate untreated with DSS (1% of input) was loaded as a control (left). *Indicates mouse IgG heavy chain. (D) Human SBDS and EFL1 jointly catalyze eIF6 release. The indicated combinations of recombinant human SBDS and EFL1 (wild-type or the catalytically inactive mutants EFL1T33A and EFL1H96A) were incubated with pre-60S subunits purified from sbdSint(ts) cells in the presence of GTP, GDP or the nonhydrolysable analog GDPNP. “Free” and “bound” fractions from sucrose cushions were immunoblotted to detect eIF6 and Rpl8.

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