Protein phosphatase 2A1 is the major enzyme in vertebrate cell extracts that dephosphorylates several physiological substrates for cyclin-dependent protein kinases.

Ferrigno, Paul Ko; Langan, Thomas A.; Cohen, Philip

doi:10.1091/mbc.4.7.669

Cited by 108 publications

(102 citation statements)

References 63 publications

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“…Because such hyperphosphorylated vimentin was completely insoluble, we were constrained to measure dephosphorylation on phosphovimentin adsorbed to nitrocellulose strips. In these assays recombinant B55 increased the specificity of dimeric PP2A by approximately fivefold, an increase similar to that measured with histone H1, which is a highly specific substrate for B55-containing PP2A (Ferrigno et al, 1993). Further confirmation that PP2A could act on native vimentin was derived from an in situ assay, which is based on the assumption that vimentin phosphorylation induces its disassembly and bundling, whereas dephosphorylation would induce reassembly into filaments (Inagaki et al, 1996).…”

supporting

confidence: 56%

“…The lack of functional B55 in yeast and Drosophila causes severe aberrations in mitotic transit (Healy et al, 1991;Mayer-Jaekel et al, 1993;Wang and Burke, 1997) presumably because of the lack of dephosphorylation of certain p34 cdc2 phosphorylated sites (Ferrigno et al, 1993;. It was recently also reported that B55 associates with the microtubule network (Sontag et al, 1995).…”

Section: Introductionmentioning

confidence: 99%

“…The 55-kDa regulatory subunit B55 (or PR55) was one of the first B-type regulators to be identified in skeletal muscle preparations of PP2A, and subsequent cDNA cloning revealed evolutionary conservation from yeast to human (Healy et al, 1991;Mayer et al, 1991;Pallas et al, 1992;Mayer-Jaekel et al, 1993). The lack of functional B55 in yeast and Drosophila causes severe aberrations in mitotic transit (Healy et al, 1991;Mayer-Jaekel et al, 1993;Wang and Burke, 1997) presumably because of the lack of dephosphorylation of certain p34 cdc2 phosphorylated sites (Ferrigno et al, 1993;. It was recently also reported that B55 associates with the microtubule network (Sontag et al, 1995).…”

Section: Introductionmentioning

confidence: 99%

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Vimentin Dephosphorylation by Protein Phosphatase 2A Is Modulated by the Targeting Subunit B55

Turowski

Myles

Hemmings

et al. 1999

MBoC

101

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The intermediate filament protein vimentin is a major phosphoprotein in mammalian fibroblasts, and reversible phosphorylation plays a key role in its dynamic rearrangement. Selective inhibition of type 2A but not type 1 protein phosphatases led to hyperphosphorylation and concomitant disassembly of vimentin, characterized by a collapse into bundles around the nucleus. We have analyzed the potential role of one of the major protein phosphatase 2A (PP2A) regulatory subunits, B55, in vimentin dephosphorylation. In mammalian fibroblasts, B55 protein was distributed ubiquitously throughout the cytoplasm with a fraction associated to vimentin. Specific depletion of B55 in living cells by antisense B55 RNA was accompanied by disassembly and increased phosphorylation of vimentin, as when type 2A phosphatases were inhibited using okadaic acid. The presence of B55 was a prerequisite for PP2A to efficiently dephosphorylate vimentin in vitro or to induce filament reassembly in situ. Both biochemical fractionation and immunofluorescence analysis of detergent-extracted cells revealed that fractions of PP2Ac, PR65, and B55 were tightly associated with vimentin. Furthermore, vimentinassociated PP2A catalytic subunit was displaced in B55-depleted cells. Taken together these data show that, in mammalian fibroblasts, the intermediate filament protein vimentin is dephosphorylated by PP2A, an event targeted by B55. INTRODUCTIONProtein phosphatase 2A (PP2A) is implicated in a significant array of cellular processes, including metabolism, DNA replication, transcription, translation, cell cycle progression, and membrane-to-nuclear signal transduction (for review, see Shenolikar, 1994;Wera and Hemmings, 1995). Regulatory flexibility is conferred by the association of a constant dimeric core of a 36-kDa catalytic (PP2Ac) and a 65-kDa (PR65 or A) subunit with a third, variable B subunit . To date three families of B subunits have been identified, which we will refer to as B55, B56, and B72, according to the predicted molecular weight of their founding member (Mayer et al., 1991;Hendrix et al., 1993a;McCright and Virshup, 1995). At least 10 individual genes code for B-type regulators, with this number being further increased by the additional presence of alternatively spliced forms of certain messages (Hendrix et al., 1993a;Csortos et al., 1996;McCright et al., 1996;Tanabe et al., 1996;Tehrani et al., 1996;Zolnierowicz et al., 1996). By analogy to PP1, in which associated noncatalytic subunits target the catalytic subunit to different subcellular compartments and/or substrates, it was proposed that the B-type regulators act as targeting subunits for PP2A (Hubbard and Cohen, 1993). Indeed, B subunits affect the substrate specificity of PP2A in vitro and in vivo (Agostinis et al., 1987;Cegielska et al., 1994;Kamibayashi et al., 1994;Zhao et al., 1997). Distinct subcellular localization has been reported for some B subunits (McCright et al., 1996;Tehrani et al., 1996). The 55-kDa regulatory subunit B55 (or PR55) was one of the first B-type re...

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supporting

confidence: 56%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Vimentin Dephosphorylation by Protein Phosphatase 2A Is Modulated by the Targeting Subunit B55

Turowski

Myles

Hemmings

et al. 1999

MBoC

101

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“…The alteration of the phosphorylation status of signaling molecules has been demonstrated to be the primary action of the ST antigen in cell transformation (Janssens and Goris, 2001; Moreno Sablina and Hahn, 2008). Indeed, PP2A complexes formed by various B subunits confer specificity of substrates dephosphorylation (Ferrigno et al, 1993;Cegielska et al, 1994). Among them, several members of the B56 family have been reported to have important roles in control of PP2A potential tumorsuppressive activity by dephosphorylation of its target oncogene (Arnold and Sears, 2006;Margolis et al, 2006;Grochola et al, 2009;Shouse et al, 2010).…”

Section: Discussionmentioning

confidence: 99%

Upregulation of miR-27a contributes to the malignant transformation of human bronchial epithelial cells induced by SV40 small T antigen

Wang

et al. 2011

Oncogene

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“…For example, the B subunit greatly increases PP2A activity towards cdc2 phosphorylated histone H1 (Sola et al, 1991;Agostinis et al, 1992;Ferrigno et al, 1993;Mayer-Jaekel et al, 1994). PP2A regulation during the development in di erent tissues may therefore occur in part through di erential expression of the various subunits (for review, see Mumby and Walter, 1993).…”

Section: Introductionmentioning

confidence: 99%

Protein phosphatase 2A subunit assembly: the catalytic subunit carboxy terminus is important for binding cellular B subunit but not polyomavirus middle tumor antigen

1997

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Protein phosphatase 2A1 is the major enzyme in vertebrate cell extracts that dephosphorylates several physiological substrates for cyclin-dependent protein kinases.

Cited by 108 publications

References 63 publications

Vimentin Dephosphorylation by Protein Phosphatase 2A Is Modulated by the Targeting Subunit B55

Vimentin Dephosphorylation by Protein Phosphatase 2A Is Modulated by the Targeting Subunit B55

Upregulation of miR-27a contributes to the malignant transformation of human bronchial epithelial cells induced by SV40 small T antigen

Protein phosphatase 2A subunit assembly: the catalytic subunit carboxy terminus is important for binding cellular B subunit but not polyomavirus middle tumor antigen

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