A novel and essential mechanism determining specificity and activity of protein phosphatase 2A (PP2A) in vivo

Fellner, Thomas; Lackner, Daniel H.; Hombauer, Hans; Piribauer, Patrick; Mudrak, Ingrid; Zaragoza, Katrin; Juno, Claudia; Ogris, Egon

doi:10.1101/gad.259903

Cited by 89 publications

(157 citation statements)

References 40 publications

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“…Nevertheless, PP2A can auto-dephosphorylate Tyr307 in an OA-sensitive reaction in vitro [48] and, in a YPA1/YPA2-null yeast strain, PP2A can dephosphorylate pNPP (a bulky phosphotyrosyl-mimic). This finding indicates the existence of a conformationally relaxed catalytic center that directs alterations in substrate specificity in the absence of PTPA [59]. Moreover, PTPA can activate the Ser/Thr phosphatase activity of a native inactive PP2A form isolated from tissues in complex with PME-1 [46] via a mechanism involving a peptidyl prolyl isomerase activity [57,58].…”

Section: Reviewmentioning

confidence: 87%

“…His59!Gln, His118!Gln, Asp85!Asn and Arg!88Ala) [45] or in vivo via a mechanism that remains poorly defined [46,[57][58][59][60], its interaction surface drastically changes, resulting in an increased affinity for several interacting proteins such as PME-1 [45,46], the PP2A phosphatase activator (PTPA) [45] (Box 4) and other, as yet unidentified proteins [45]. Activity of the native inactive PP2A (PP2A i ) in complex with PME-1 cannot be restored by LCMT1-mediated (re)methylation [46].…”

Section: Trends In Biochemical Sciencesmentioning

confidence: 99%

“…The mechanism of this activation has recently been partially solved by demonstrating that PTPA has an ATP-Mg 2+ -stimulated peptidyl prolyl cis/trans isomerase activity that targets Pro190 in PP2A C [57], which is essential for PP2A activation [58]. In a YPA1/YPA2-null yeast strain (yeast PP2A activator 1 and 2, encoding the yeast homologs of PTPA), PP2A C has decreased Ser/Thr phosphatase activity and is hypomethylated owing to its increased association with PME-1 [59,60]. The additional deletion of PPE1 (protein phosphatase methylesterase 1, encoding the yeast PME-1 homolog) in this strain restores PP2A C methylation but not Ser/Thr phosphatase activity, confirming that demethylation itself does not cause PP2A inactivation and that the inactive conformation does not prevent methylation.…”

Section: Trends In Biochemical Sciencesmentioning

confidence: 99%

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PP2A holoenzyme assembly: in cauda venenum (the sting is in the tail)

Janssens

Longin

Goris

2008

Trends in Biochemical Sciences

365

424

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Section: Reviewmentioning

confidence: 87%

Section: Trends In Biochemical Sciencesmentioning

confidence: 99%

Section: Trends In Biochemical Sciencesmentioning

confidence: 99%

See 1 more Smart Citation

PP2A holoenzyme assembly: in cauda venenum (the sting is in the tail)

Janssens

Longin

Goris

2008

Trends in Biochemical Sciences

365

424

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“…The reactivation of PP2Ac by PTPA in vitro was at first only identified as an increase in phosphotyrosyl phosphatase activity (11,12) when in fact it appears to activate the phosphoserine/threonine-specific activity of PP2Ac from a poorly active and substrate unspecific metal-dependent state (13,14). PTPA is an essential protein as revealed by its high evolutionary conservation as well as the lethality of the deletion of the two PTPA homologs in yeast, Rrd1 and Rrd2, in certain nutritional backgrounds (15).…”

mentioning

confidence: 99%

The Crystal Structure of a Human PP2A Phosphatase Activator Reveals a Novel Fold and Highly Conserved Cleft Implicated in Protein-Protein Interactions

Magnusdottir

Stenmark

Flodin

et al. 2006

Journal of Biological Chemistry

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Protein phosphatase 2A (PP2A) is a heterotrimeric Ser/Thr phosphatase that is involved in regulating a plethora of signaling pathways in the cell, making its regulation a critical part of the well being of the cell. For example, three of the non-catalytic PP2A subunits have been linked to carcinogenic events. Therefore, the molecular basis for the complicated protein-protein interaction pattern of PP2A and its regulators is of special interest. The PP2A phosphatase activator (PTPA) protein is highly conserved from humans to yeast. It is an activator of PP2A and has been shown to be essential for a fully functional PP2A, but its mechanism of activation is still not well defined. We have solved the crystal structure of human PTPA to 1.6 Å . It reveals a twodomain protein with a novel fold comprised of 13 ␣-helices. We have identified a highly conserved cleft as a potential region for interaction with peptide segments of other proteins. Binding studies with ATP and its analogs are not consistent with ATP being a cofactor/substrate for PTPA as had previously been proposed. The structure of PTPA can serve as a basis for structurefunction studies directed at elucidating its mechanism as an activator of PP2A.

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“…Most PP2A catalytic subunits in the cell form heterotrimeric complexes followed by the AC core dimer and, finally, numerous lower abundance complexes (22)(23)(24)(25)(26)(27). Highlighting the role of PP2A in growth control, several viruses encode proteins that subvert PP2A activity by binding to either dimeric or trimeric forms of the phosphatase (1).…”

mentioning

confidence: 99%

Critical Role for Protein Phosphatase 2A Heterotrimers in Mammalian Cell Survival

Strack

Cribbs

Gomez

2004

Journal of Biological Chemistry

141

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The predominant forms of protein phosphatase 2A (PP2A), one of the major Ser/Thr phosphatases, are dimers of catalytic (C) and scaffolding (A) subunits and trimers with an additional variable regulatory subunit. In mammals, catalytic and scaffolding subunits are encoded by two genes each (␣/␤), whereas three gene families (B, B , and B؆) with a total of 12 genes contribute PP2A regulatory subunits. We generated stable PC12 cell lines in which the major scaffolding A␣ subunit can be knocked down by inducible RNA interference (RNAi) to study its role in cell viability. A␣ RNAi decreased total PP2A activity as well as protein levels of C, B, and B but not B؆ subunits. Inhibitor experiments indicate that monomeric C and B subunits are degraded by the proteosome. Knock-down of A␣ triggered cell death by redundant apoptotic and non-apoptotic mechanisms because the inhibition of RNAi-associated caspase activation failed to stall cell death. PP2A holoenzymes positively regulate survival kinase signaling, because RNAi reduced basal and epidermal growth factor-stimulated Akt phosphorylation. RNAi-resistant A␣ cDNAs rescued RNAi-induced loss of the C subunit, and A␣ point mutants prevented regulatory subunit degradation as predicted from each mutant's binding specificity. In transient, stable, and stable-inducible rescue experiments, both wild-type A␤ and A␣ mutants capable of binding to at least one family of regulatory subunits were able to delay A␣ RNAi-induced death of PC12 cells. However, only the expression of wild-type A␣ restored viability completely. Thus, heterotrimeric PP2A holoenzymes containing the A␣ subunit and members of all three regulatory subunit families are necessary for mammalian cell viability.

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A novel and essential mechanism determining specificity and activity of protein phosphatase 2A (PP2A) in vivo

Cited by 89 publications

References 40 publications

PP2A holoenzyme assembly: in cauda venenum (the sting is in the tail)

PP2A holoenzyme assembly: in cauda venenum (the sting is in the tail)

The Crystal Structure of a Human PP2A Phosphatase Activator Reveals a Novel Fold and Highly Conserved Cleft Implicated in Protein-Protein Interactions

Critical Role for Protein Phosphatase 2A Heterotrimers in Mammalian Cell Survival

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