A novel non-canonical mechanism of regulation of MST3 (mammalian Sterile20-related kinase 3)

The canonical pathway of regulation of the GCK (germinal centre kinase) III subgroup member, MST3 (mammalian Sterile20-related kinase 3), involves a caspase-mediated cleavage between N-terminal catalytic and C-terminal regulatory domains with possible concurrent autophosphorylation of the activation loop MST3(Thr178), induction of serine/threonine protein kinase activity and nuclear localization. We identified an alternative ‘non-canonical’ pathway of MST3 activation (regulated primarily through dephosphorylation) which may also be applicable to other GCKIII (and GCKVI) subgroup members. In the basal state, inactive MST3 co-immunoprecipitated with the Golgi protein GOLGA2/gm130 (golgin A2/Golgi matrix protein 130). Activation of MST3 by calyculin A (a protein serine/threonine phosphatase 1/2A inhibitor) stimulated (auto)phosphorylation of MST3(Thr178) in the catalytic domain with essentially simultaneous cis-autophosphorylation of MST3(Thr328) in the regulatory domain, an event also requiring the MST3(341–376) sequence which acts as a putative docking domain. MST3(Thr178) phosphorylation increased MST3 kinase activity, but this activity was independent of MST3(Thr328) phosphorylation. Interestingly, MST3(Thr328) lies immediately C-terminal to a STRAD (Sterile20-related adaptor) pseudokinase-like site identified recently as being involved in binding of GCKIII/GCKVI members to MO25 scaffolding proteins. MST3(Thr178/Thr328) phosphorylation was concurrent with dissociation of MST3 from GOLGA2/gm130 and association of MST3 with MO25, and MST3(Thr328) phosphorylation was necessary for formation of the activated MST3–MO25 holocomplex.

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Enzyme activity effects of N-terminal His-tag attached to catalytic sub-unit of phosphoinositide-3-kinase

Bioscience Reports ◽

10.1042/bsr20130075 ◽

2013 ◽

Vol 33 (6) ◽

Cited By ~ 15

Author(s):

James M. J. Dickson ◽

Woo-Jeong Lee ◽

Peter R. Shepherd ◽

Christina M. Buchanan

Keyword(s):

Protein Kinase ◽

Kinase Activity ◽

Catalytic Domain ◽

Cell Signalling ◽

Protein Kinase Activity ◽

Lipid Kinase ◽

His Tag ◽

The Impact

NTT (N-terminal tags) on the catalytic (p110) sub-unit of PI 3-K (phosphoinositol 3-kinase) have previously been shown to increase cell signalling and oncogenic transformation. Here we test the impact of an NT (N-terminal) His-tag on in vitro lipid and protein kinase activity of all class-1 PI 3-K isoforms and two representative oncogenic mutant forms (E545K and H1047R), in order to elucidate the mechanisms behind this elevated signalling and transformation observed in vivo. Our results show that an NT His-tag has no impact on lipid kinase activity as measured by enzyme titration, kinetics and inhibitor susceptibility. Conversely, the NT His-tag did result in a differential effect on protein kinase activity, further potentiating the elevated protein kinase activity of both the helical domain and catalytic domain oncogenic mutants with relation to p110 phosphorylation. All other isoforms also showed elevated p110 phosphorylation (although not statistically significant). We conclude that the previously reported increase in cell signalling and oncogenic-like transformation in response to p110 NTT is not mediated via an increase in the lipid kinase activity of PI 3-K, but may be mediated by increased p110 autophosphorylation and/or other, as yet unidentified, intracellular protein/protein interactions. We further observe that tagged recombinant protein is suitable for use in in vitro lipid kinase screens to identify PI 3-K inhibitors; however, we recommend that in vivo (including intracellular) experiments and investigations into the protein kinase activity of PI 3-K should be conducted with untagged constructs.

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Requirement of phosphatidylinositol-3 kinase modification for its association with p60src

Molecular and Cellular Biology ◽

10.1128/mcb.11.4.1972-1979.1991 ◽

1991 ◽

Vol 11 (4) ◽

pp. 1972-1979

Author(s):

Y Fukui ◽

H Hanafusa

Keyword(s):

Protein Kinase ◽

Tyrosine Phosphorylation ◽

Kinase Activity ◽

Catalytic Domain ◽

Sh2 Domain ◽

Protein Kinase Activity ◽

Phosphatidylinositol 3 Kinase ◽

Tyrosine Residues ◽

Phosphorylated Form ◽

Chicken Embryo Fibroblasts

When purified p60v-src was mixed with lysates of chicken embryo fibroblasts and immunoprecipitated with anti-Src antibody, phosphatidylinositol (PI)-3 kinase activity was found to be present in the Src protein immunoprecipitates. The level of bound PI-3 kinase activity was 5 to 10 times higher in lysates obtained from cells transformed by the src, fps, or yes oncogene than in lysates of uninfected cells. This increase in associated PI-3 kinase activity appears to be due to increased binding of this enzyme to p60v-src. This change most likely resulted from tyrosine phosphorylation of PI-3 kinase or an associated protein, since the PI-3 kinase activity that can bind to p60v-src was depleted by antiphosphotyrosine antibody. Binding of PI-3 kinase did not require either p60src protein kinase activity or autophosphorylation of p60v-src tyrosine residues. Furthermore, binding was markedly decreased by deletions in the N-terminal SH2 region but unchanged by deletion of the C-terminal half of p60v-src containing the catalytic domain. Taking these data together, it appears that PI-3 kinase or its associated protein is phosphorylated on tyrosine and that the phosphorylated form can bind to the N-terminal half of p60v-src, which contains the SH2 domain.

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Sumoylation of AMPKβ2 subunit enhances AMP-activated protein kinase activity

Molecular Biology of the Cell ◽

10.1091/mbc.e12-11-0806 ◽

2013 ◽

Vol 24 (11) ◽

pp. 1801-1811 ◽

Cited By ~ 24

Author(s):

Teresa Rubio ◽

Santiago Vernia ◽

Pascual Sanz

Keyword(s):

Protein Kinase ◽

Kinase Activity ◽

Catalytic Domain ◽

Protein Kinase Activity ◽

Energy Status ◽

Regulatory Subunits ◽

Cellular Energy ◽

Sumo Ligase ◽

Ampk Activity ◽

Amp Activated Protein Kinase

AMP-activated protein kinase (AMPK) is a sensor of cellular energy status. It is a heterotrimer composed of a catalytic α and two regulatory subunits (β and γ). AMPK activity is regulated allosterically by AMP and by the phosphorylation of residue Thr-172 within the catalytic domain of the AMPKα subunit by upstream kinases. We present evidence that the AMPKβ2 subunit may be posttranslationally modified by sumoylation. This process is carried out by the E3-small ubiquitin-like modifier (SUMO) ligase protein inhibitor of activated STAT PIASy, which modifies the AMPKβ2 subunit by the attachment of SUMO2 but not SUMO1 moieties. Of interest, AMPKβ1 is not a substrate for this modification. We also demonstrate that sumoylation of AMPKβ2 enhances the activity of the trimeric α2β2γ1 AMPK complex. In addition, our results indicate that sumoylation is antagonist and competes with the ubiquitination of the AMPKβ2 subunit. This adds a new layer of complexity to the regulation of the activity of the AMPK complex, since conditions that promote ubiquitination result in inactivation, whereas those that promote sumoylation result in the activation of the AMPK complex.

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Tyrosine phosphorylation of focal adhesion kinase at sites in the catalytic domain regulates kinase activity: a role for Src family kinases.

Molecular and Cellular Biology ◽

10.1128/mcb.15.2.954 ◽

1995 ◽

Vol 15 (2) ◽

pp. 954-963 ◽

Cited By ~ 645

Author(s):

M B Calalb ◽

T R Polte ◽

S K Hanks

Keyword(s):

Signal Transduction ◽

Cell Adhesion ◽

Focal Adhesion Kinase ◽

Focal Adhesion ◽

Kinase Activity ◽

Catalytic Domain ◽

Src Family Kinases ◽

Protein Kinase Activity ◽

Dependent Manner

Focal adhesion kinase (FAK) is a widely expressed nonreceptor protein-tyrosine kinase implicated in integrin-mediated signal transduction pathways and in the process of oncogenic transformation by v-Src. Elevation of FAK's phosphotyrosine content, following both cell adhesion to extracellular matrix substrata and cell transformation by Rous sarcoma virus, correlates directly with an increased kinase activity. To help elucidate the role of FAK phosphorylation in signal transduction events, we used a tryptic phosphopeptide mapping approach to identify tyrosine sites of phosphorylation responsive to both cell adhesion and Src transformation. We have identified four tyrosines, 397, 407, 576, and 577, which are phosphorylated in mouse BALB/3T3 fibroblasts in an adhesion-dependent manner. Tyrosine 397 has been previously recognized as the major site of FAK autophosphorylation. Phosphorylation of tyrosines 407, 576, and 577, which are previously unrecognized sites, is significantly elevated in the presence of c-Src in vitro and v-Src in vivo. Tyrosines 576 and 577 lie within catalytic subdomain VIII--a region recognized as a target for phosphorylation-mediated regulation of protein kinase activity. We found that maximal kinase activity of FAK immune complexes requires phosphorylation of both tyrosines 576 and 577. Our results indicate that phosphorylation of FAK by Src (or other Src family kinases) is an important step in the formation of an active signaling complex.

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Requirement of phosphatidylinositol-3 kinase modification for its association with p60src.

Molecular and Cellular Biology ◽

10.1128/mcb.11.4.1972 ◽

1991 ◽

Vol 11 (4) ◽

pp. 1972-1979 ◽

Cited By ~ 46

Author(s):

Y Fukui ◽

H Hanafusa

Keyword(s):

Protein Kinase ◽

Tyrosine Phosphorylation ◽

Kinase Activity ◽

Catalytic Domain ◽

Sh2 Domain ◽

Protein Kinase Activity ◽

Phosphatidylinositol 3 Kinase ◽

Tyrosine Residues ◽

Phosphorylated Form ◽

Chicken Embryo Fibroblasts

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Effect of Thrombin on Phosphorylation of Platelet Membrane Proteins

Thrombosis and Haemostasis ◽

10.1055/s-0038-1647962 ◽

1976 ◽

Vol 35 (03) ◽

pp. 635-642 ◽

Cited By ~ 4

Author(s):

M Steiner

Keyword(s):

Protein Kinase ◽

Kinase Activity ◽

Qualitative Change ◽

Protein Kinase Activity ◽

Protein Substrates ◽

Phosphoprotein Phosphatase ◽

Progressive Loss ◽

Platelet Membranes ◽

Endogenous Protein ◽

Considerable Loss

SummaryThe effect of thrombin on the phosphorylating activity of platelet membranes was compared to that of trypsin. Preincubation of non-32P phosphorylated platelet membranes with or without either of these two enzymes resulted in a considerable loss of membrane protein kinase activity which was most severe when trypsin was used. Protein kinase activity and endogenous protein acceptors decreased in parallel. 32P-phosphorylated membranes showed a slow but progressive loss of label which was accelerated by trypsin. Thrombin under these conditions prevented the loss of 32P-phosphate. These results are interpreted to indicate a thrombin-induced destruction of a phosphoprotein phosphatase. The protein kinase activity of phosphorylated platelet membranes using endogenous or exogenous protein substrates showed a significant reduction compared to non-phosphorylated membranes suggesting a deactivation of protein kinase by phosphorylation of platelet membranes. Neither thrombin nor trypsin caused a qualitative change in the membrane polypeptides accepting 32P-phosphate but resulted in quantitative alterations of their ability to become phosphorylated.

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