pRb is required for MEF2-dependent gene expression as well as cell-cycle arrest during skeletal muscle differentiation

Background: The onset of differentiation-specific gene expression in skeletal muscle is coupled to permanent withdrawal from the cell cycle. The retinoblastoma tumor-suppressor protein (pRb) is a critical regulator of this process, required for both cell-cycle arrest in G0 phase and high-level expre...

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Bibliographic Details
Published in:Current biology 1999-05, Vol.9 (9), p.449-459
Main Authors: Novitch, Bennett G., Spicer, Douglas B., Kim, Paul S., Cheung, Wang L., Lassar, Andrew B.
Format: Article
Language:English
Subjects:
Animals
Binding Sites
Cell Cycle
Cell Differentiation
Cell Nucleus - metabolism
Creatine Kinase - genetics
DNA - metabolism
DNA-Binding Proteins - genetics
DNA-Binding Proteins - metabolism
Gene Expression Regulation
Herpes Simplex Virus Protein Vmw65 - genetics
Herpes Simplex Virus Protein Vmw65 - metabolism
MEF2 Transcription Factors
Mice
Muscle, Skeletal - cytology
MyoD Protein - metabolism
Myogenic Regulatory Factors - genetics
Myogenic Regulatory Factors - metabolism
Promoter Regions, Genetic
Recombinant Fusion Proteins - genetics
Recombinant Fusion Proteins - metabolism
Resting Phase, Cell Cycle
Retinoblastoma Protein - metabolism
Serine
Transcription Factors - genetics
Transcription Factors - metabolism
Transcriptional Activation
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Summary:Background: The onset of differentiation-specific gene expression in skeletal muscle is coupled to permanent withdrawal from the cell cycle. The retinoblastoma tumor-suppressor protein (pRb) is a critical regulator of this process, required for both cell-cycle arrest in G0 phase and high-level expression of late muscle-differentiation markers. Although the cell-cycle defects that are seen in pRb-deficient myocytes can be explained by the well-described function of pRb as a negative regulator of the transition from G1 to S phase, it remains unclear how pRb positively affects late muscle-gene expression. Results: Here, we show that the myogenic defect in Rb−/− cells corresponds to a deficiency in the activity of the transcription factor MEF2. Without pRb, MyoD induces the accumulation of nuclear-localized MEF2 that is competent to bind DNA yet transcriptionally inert. When pRb is present, MyoD stimulates the function of the MEF2C transcriptional activation domain and the activity of endogenous MEF2-type factors. Co-transfection of MyoD together with an activated form of MEF2C containing the Herpesvirus VP16 transcriptional activation domain partially bypasses the requirement for pRb and induces late muscle-gene expression in replicating cells. This ectopic myogenesis is nevertheless significantly augmented by co-expression of an E2F1–pRb chimeric protein that blocks the cell cycle. Conclusion: These findings indicate that pRb promotes the expression of late-stage muscle-differentiation markers by both inhibiting cell-cycle progression and cooperating with MyoD to promote the transcriptional activation activity of MEF2.
ISSN:0960-9822
1879-0445
DOI:10.1016/S0960-9822(99)80210-3