Figure 3.
Figure 3. Characterizing the regions that are required for direct interaction between FANCB and FANCL. (A) Mammalian 2-hybrid assays coexpressing mutant fragments of BD-FANCL with full-length AD-FANCB. Fold induction of luciferase expression was measured relative to AD-FANCB alone. +++ indicates a strong activation of the luciferase reporter gene; –, no activation of the reporter gene. (B) FANCL constructs that failed to activate the luciferase reporter in the mammalian 2-hybrid experiments were transfected in 293 cells. Whole-cell extracts were immunoblotted with anti–GAL4-BD to show expression of the constructs. The fragments 219-375 and 275-375 are probably difficult to detect because of the presence of background bands. (C) BD-FANCL–containing point mutations of the RING domain were coexpressed with full-length AD-FANCB and fold induction was measured relative to AD-FANCB alone. +++ indicates a strong activation of the luciferase reporter gene; –, no activation of the reporter gene. (D) FANCL missense mutants were transfected in FA-L cell line EUFA868 and tested for their ability to restore the MMC hypersensitive phenotype of this cell line in an MMC growth inhibition test.

Characterizing the regions that are required for direct interaction between FANCB and FANCL. (A) Mammalian 2-hybrid assays coexpressing mutant fragments of BD-FANCL with full-length AD-FANCB. Fold induction of luciferase expression was measured relative to AD-FANCB alone. +++ indicates a strong activation of the luciferase reporter gene; –, no activation of the reporter gene. (B) FANCL constructs that failed to activate the luciferase reporter in the mammalian 2-hybrid experiments were transfected in 293 cells. Whole-cell extracts were immunoblotted with anti–GAL4-BD to show expression of the constructs. The fragments 219-375 and 275-375 are probably difficult to detect because of the presence of background bands. (C) BD-FANCL–containing point mutations of the RING domain were coexpressed with full-length AD-FANCB and fold induction was measured relative to AD-FANCB alone. +++ indicates a strong activation of the luciferase reporter gene; –, no activation of the reporter gene. (D) FANCL missense mutants were transfected in FA-L cell line EUFA868 and tested for their ability to restore the MMC hypersensitive phenotype of this cell line in an MMC growth inhibition test.

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