Physical interaction between CDK9 and B-Myb results in suppression of B-Myb gene autoregulation

Falco, Giulia De; Bagella, Luigi; Claudio, Pier Paolo; Luca, Antonio De; Fu, Yan; Calabretta, Bruno; Sala, Arturo; Giordano, Antonio

doi:10.1038/sj.onc.1203305

Cited by 43 publications

(40 citation statements)

References 38 publications

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“…While the generation of transiently active truncated B-Myb species in response to cyclin Amediated phosphorylation would clearly provide a rationale for the presence of an inhibitory C-terminal domain, it also remains possible that B-Myb hyperphosphorylation a ects interactions with as yet unrecognized regulatory proteins. In this regard, several B-Myb-binding proteins have now been identi®ed which inhibit its transactivation function, for example p107, Cdk9 and cyclin D1 (Sala et al, 1996;De Falco et al, 2000;Horstmann et al, 2000), and it will be of further interest to determine whether phosphorylation counteracts these e ects.…”

Section: Discussionmentioning

confidence: 99%

Inhibition of cyclin A/Cdk2 phosphorylation impairs B-Myb transactivation function without affecting interactions with DNA or the CBP coactivator

2001

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Expression of the B-Myb transcription factor is directed by an E2F-dependent transcriptional mechanism to late G1 and S phases of the cell cycle, where its transactivation properties are enhanced post-translationally by cyclin A/Cdk2-mediated phosphorylation. Other experiments have shown that removal of the B-Myb Cterminus constitutively activates both transactivation and DNA-binding activities, suggesting that autoregulation by this inhibitory domain is counteracted by phosphorylation. We report here on further experiments to examine this hypothesis. The importance of this modi®cation was ®rst emphasized by showing that cotransfected dominant-negative Cdk2 (Cdk2DN) substantially reduced B-Myb transactivation activity. We then attempted to map the autoregulatory domain by analysing a series of progressively deleted C-terminal B-Myb mutants. Removal of just 29 C-terminal aa increased transactivation appreciably, however, maximal activity required removal of 143 amino acids (as in BMyb+561). Enhanced B-Myb+561 function correlated with the acquisition of DNA binding activity to a single Myb binding site (MBS) oligonucleotide as determined by bandshift assays, however, further assays showed that even wt B-Myb could bind a DNA fragment containing three MBS. Although transactivation by B-Myb was severely dependent on hyperphosphorylation, neither inhibiting this activity by co-transfecting Cdk2DN nor augmenting it with cyclin A resulted in signi®cant e ects on DNA-binding. We also found that B-Myb could synergize with the CBP coactivator and that this cooperativity was cyclin A/Cdk2-dependent. Despite this, the physical association between these proteins was not in¯uenced by the B-Myb phosphorylation status. We discuss these ®ndings in relation to the autoregulation of B-Myb by the C-terminal domain. Oncogene (2001) 20, 3376 ± 3386.

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Section: Discussionmentioning

confidence: 99%

Inhibition of cyclin A/Cdk2 phosphorylation impairs B-Myb transactivation function without affecting interactions with DNA or the CBP coactivator

2001

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“…The polyclonal anti-HA Tag (Santacruz) was used at a dilution 1 : 3000 in Western blot. Immunoprecipitation and Western blotting conditions have been described (De Falco et al, 2000).…”

Section: Immunoprecipitation and Western Blotmentioning

confidence: 99%

“…The antibody (Ab) was used at a dilution of 1 : 1000 in Western blot. Anti-Cdk9 has already been described (De Falco et al, 2000). The antibody was affinity purified and used at a dilution 1 : 300 in Western blot.…”

Section: Immunoprecipitation and Western Blotmentioning

confidence: 99%

Cdk9, a member of the cdc2-like family of kinases, binds to gp130, the receptor of the IL-6 family of cytokines

et al. 2002

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“…These data indicate functional di erences between cycT1 and cycT2, even if cycT2 function remains less understood. The catalytic activity of the cdk9 immunocomplexes results only from cdk9 and it is abolished using a dominant negative form (kinase inactive mutant, cdk9dn) (De Falco et al, 2000), which consists of a point mutation within the ATP-binding domain that changes the Asp to Asn at residue 167.…”

Section: Introductionmentioning

confidence: 99%

Physical interaction between pRb and cdk9/cyclinT2 complex

et al. 2002

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Cyclin-dependent kinase 9 (cdk9) is a multifunctional kinase with roles in di erent cellular pathways such as transcriptional elongation, di erentiation and apoptosis. Cdk9/cyclin T di ers functionally from other cdk/cyclin complexes that regulate cell cycle progression, but maintains structural a nity with those complexes. In addition, previous reports have demonstrated that the cdk9 complex is able to phosphorylate p56/pRb in vitro.In this report we show in vitro and in vivo interaction between cdk9/cyclinT2 and the protein product of the retinoblastoma gene (pRb) in human cell lines. The interaction involves the region composed of residues 129 ± 195 of cdk9, cyclinT2 (1 ± 642 aa) and the Cterminal domain of pRb (835 ± 928 aa). We located the minimal region of cdk9 phosphorylation on the Cterminus of pRb, by identifying the residues between 793 and 834. This region contains at least three prolinedirected serines (sp), S795, S807 and S811, which have been reported to be phosphorylated in vivo and which could be targeted by the cdk9 complex. These data suggest that, in logarithmically growing cells, cdk9/ cyclin T2 and pRb are located in a nuclear multiprotein complex probably involved in transduction of cellular signals to the basal transcription machinery and that one of these signals could be the cdk9 phosphorylation of pRb.

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Physical interaction between CDK9 and B-Myb results in suppression of B-Myb gene autoregulation

Cited by 43 publications

References 38 publications

Inhibition of cyclin A/Cdk2 phosphorylation impairs B-Myb transactivation function without affecting interactions with DNA or the CBP coactivator

Inhibition of cyclin A/Cdk2 phosphorylation impairs B-Myb transactivation function without affecting interactions with DNA or the CBP coactivator

Cdk9, a member of the cdc2-like family of kinases, binds to gp130, the receptor of the IL-6 family of cytokines

Physical interaction between pRb and cdk9/cyclinT2 complex

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