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Mutations on the Smad3 MH2 interfaces that mediate binding to Smad4 reduce binding to Smad4 or Smad3 but have differential effects on interactions with other Smad-binding proteins.

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Figshare2015-12-02 更新2026-04-29 收录
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https://figshare.com/articles/dataset/_Mutations_on_the_Smad3_MH2_interfaces_that_mediate_binding_to_Smad4_reduce_binding_to_Smad4_or_Smad3_but_have_differential_effects_on_interactions_with_other_Smad_binding_proteins_/404847
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Binding between wild-type or mutant Renilla-Smad3 fusion proteins and eight different Flag epitope-tagged Smad-binding proteins was quantified by pull-down of protein complexes from cell lysates and detection of the Renilla luciferase activity per well. The Renilla luciferase counts were normalized to the number of counts recovered with phosphorylated wild-type Smad3 (100%). The proteins were co-expressed with the constitutively active Alk5. The average of the data from at least four independent transfections is shown. Total Renilla luciferase activity was measured in each transfected cell lysate as a surrogate measure for the level of Renilla-Smad fusion protein; data is only reported for experiments where the level of each Renilla-Smad3 mutant was within two-fold of the level of the Renilla-Smad3 wild type protein in the same experiment. FL indicates that the full-length protein was used, e.g., full-length SARA [59]. The amino acids comprising the SARA [32], Smurf2 [52], Ski [22], and Sip1 [94] Smad3-binding motifs expressed on the Flag-epitope tagged thioredoxin scaffold are indicated below each gene. Standard deviations are indicated in parenthesis.
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2015-12-02
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