Cyclic nucleotide specificity of the activator and catalytic sites of a cGMP‐stimulated cGMP phosphodiesterase from <i>Dictyostelium discoideum</i>

Kesbeke, Fanja; Baraniak, Janina; Bulgakov, Roman; Jastorff, Bernd; Morr, Michael; Petridis, Georg; Stec, Wojciech J.; Seela, Frank; Haastert, Peter J.M. van

doi:10.1111/j.1432-1033.1985.tb09083.x

Cited by 18 publications

(16 citation statements)

References 35 publications

(7 reference statements)

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“…The full-length protein was purified by immunoprecipitation with GFP antibodies. The purified PdeD showed cGMP-PDE activity that was stimulated by cGMP and by 8-Br-cGMP, as was previously described for the enzyme lacking in stmF mutants (Kesbeke et al, 1985). In our hands, the stimulation by cGMP was less pronounced than described by Kesbeke et al, which is perhaps a result of the use of different parental strains.…”

Section: The Pded Catalytic Activity Resides In Its Metallo-␤-lactamasupporting

confidence: 86%

“…The cGMP-PDE activity in the PdeD-YFP immunoprecipitate was ϳ5% of the lysate from which it was derived. The immunoprecipitated activity was slightly activated by submicromolar cGMP concentrations and more strongly by 8-Br-cGMP, which is a good activator but a poor substrate for the stmF cGMP-PDE (Kesbeke et al, 1985). cAMP was a very poor competitor for 3 H-cGMP hydrolyzing activity.…”

Section: Novel Cgmp-pde In Dictyosteliummentioning

confidence: 96%

“…In the original biochemical characterization of the enzyme, stimulation by cGMP was also not noted (Dicou and Brachet, 1980). 8-Br-cGMP induced a more significant stimulation, because it is a poor substrate (Kesbeke et al, 1985). cAMP was no competitor for 3 H-cGMP hydrolysis.…”

Section: The Pded Catalytic Activity Resides In Its Metallo-␤-lactamamentioning

confidence: 99%

“…Studies with cGMP analogues showed that cyclic nucleotide specificity of the activator and catalytic sites of the enzyme are not identical (Kesbeke et al, 1985). Both sites are specific for cGMP, do not bind cAMP, and do not tolerate modification of the exocyclic oxygens.…”

Section: The Cnmp-binding Domain a Of Pded May Mediate Allosteric Actmentioning

confidence: 99%

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Identification of a Novel Type of cGMP Phosphodiesterase That Is Defective in the ChemotacticstmFMutants

Meima

Biondi

Schaap

2002

MBoC

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StmF mutants are chemotactic mutants that are defective in a cGMP phosphodiesterase (PDE) activity. We identified a novel gene, PdeD, that harbors two cyclic nucleotide-binding domains and a metallo-␤-lactamase homology domain. Similar to stmF mutants, pdeD-null mutants displayed extensively streaming aggregates, prolonged elevation of cGMP levels after chemotactic stimulation, and reduced cGMP-PDE activity. PdeD transcripts were lacking in stmF mutant NP377, indicating that this mutant carries a PdeD lesion. Expression of a PdeD-YFP fusion protein in pdeD-null cells restored the normal cGMP response and showed that PdeD resides in the cytosol. When purified by immunoprecipitation, the PdeD-YFP fusion protein displayed cGMP-PDE activity, which was retained in a truncated construct that contained only the metallo-␤-lactamase domain. Newell, 1979, 1981;Kuwayama et al., 1993). Mutants KI8 and KI10 show no ligand-induced cGMP response and cannot chemotax (Kuwayama et al., 1993). Streamer F (stmF) mutants are defective in cGMP-PDE activity (Van Haastert et al., 1982). These mutants show an elevated and prolonged cGMP response and prolonged association of myosin with the cytoskeleton (Ross and Newell, 1981;Liu and Newell, 1988, 1994. When grown as colonies on dense bacterial lawns, stmF mutants form aggregates with very pronounced aggregation streams, a phenotype that under these conditions is not displayed by wild-type cells. INTRODUCTION Mutants in cGMP metabolism have implicated cGMP as intermediate for ligand-induced chemotaxis in DictyosteliumThree PDE genes have been identified in Dictyostelium; two of those, RegA (Shaulsky et al., 1996;Thomason et al., 1998) and PDE3 (Kuwayama et al., 2001), belong to the large class of HD-domain PDEs that is commonly found in vertebrates (Mehats et al., 2002). The third enzyme, PdsA (Lacombe et al., 1986), is a class II PDE that is also found in yeast (Nikawa et al., 1987). None of these genes are associated with the stmF locus.In our search for targets of cyclic nucleotides, we identified a gene, PdeD, with two putative cyclic nucleotide (cNMP)-binding domains and a binuclear Zn 2ϩ -binding domain. The latter domain forms the catalytic center of bacterial metallo-␤-lactamases, which hydrolyze an amide bond in the ␤-lactam ring of carbapenem antibiotics (Carfi et al., 1995) and are a major cause for widespread bacterial antibiotic resistance (Payne, 1993). We show that pdeD-null mutants phenocopy stmF mutants. One of the cNMP-binding domains of PdeD most likely functions as an allosteric activator of the enzyme, whereas the metallo-␤-lactamase homology domain catalyzes the hydrolysis of cGMP. MATERIALS AND METHODS Cell Growth and DevelopmentD. discoideum strains NC4, XP55, and NP377 were grown in association with Klebsiella aerogenes on SM agar plates, and all other strains were grown in HL5 medium, supplemented with 5 g/ml blasticidin or 20 -200 g/ml G418 for strains transformed with pBsr⌬Bam or neomycin selection markers, respectively. For developmental time courses, cells ...

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Section: The Pded Catalytic Activity Resides In Its Metallo-␤-lactamasupporting

confidence: 86%

Section: Novel Cgmp-pde In Dictyosteliummentioning

confidence: 96%

Section: The Pded Catalytic Activity Resides In Its Metallo-␤-lactamamentioning

confidence: 99%

Section: The Cnmp-binding Domain a Of Pded May Mediate Allosteric Actmentioning

confidence: 99%

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Identification of a Novel Type of cGMP Phosphodiesterase That Is Defective in the ChemotacticstmFMutants

Meima

Biondi

Schaap

2002

MBoC

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“…Furthermore, this result shows that substituting sulfur for oxygen at the cyclic phosphate position has a 10-fold greater destabilizing effect than was observed at the C-6 position of the purine ring (1). The small extent of stereospecificity (Ͻ3-fold) exhibited by the R p and S p diastereomers distinguishes the photoreceptor PDE from other cGMP binding sites (22,44). The small difference in binding affinities of the R p and S p analogs of cGMP suggest that either 1) there is a single residue in the binding pocket positioned nearly equidistant from the two exocyclic oxygens, or 2) there are two sites in the binding pocket, each one of which forms a similar interaction with the equatorial and axial exocyclic oxygens.…”

Section: Table II Substitutions In the C-2/n-3 Region Of The Purine Ringmentioning

confidence: 99%

Structural Features of the Noncatalytic cGMP Binding Sites of Frog Photoreceptor Phosphodiesterase Using cGMP Analogs

Hebert¹,

Schwede²,

Jastorff³

et al. 1998

Journal of Biological Chemistry

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The cGMP-specific phosphodiesterase (PDE) of retinal photoreceptors is a central regulatory enzyme in the visual transduction pathway of vertebrate vision. Although the mechanism of activation of PDE by transducin is well understood, the role of the noncatalytic cGMP binding sites located on the catalytic subunits of PDE remains obscure. We report here for the first time the molecular basis of the noncovalent interactions between cGMP and the high affinity, noncatalytic cGMP binding sites of frog photoreceptor PDE.None of the tested cGMP analogs were able to bind with greater affinity than cGMP itself, and the noncatalytic sites were unable to bind cAMP. The major determinant for discrimination of cGMP over cAMP is in the N-1/C-6 region of the purine ring of cGMP where hydrogen bonding probably stabilizes the selective binding of cGMP. Substitutions at the C-2 position demonstrate that this region of the molecule plays a secondary but significant role in stabilizing cGMP binding to PDE through hydrogen bond interactions. The unaltered hydrogen at the C-8 position is also important for high affinity binding. A significant interaction between the binding pocket and the ribose ring of cGMP occurs at the 2-hydroxyl position. Steric constraints were greatest in the C-8 and possibly the C-6/N-1 regions, whereas the C-2/N-3 and C-2 regions tolerated bulky substituents better. Several lines of evidence indicate that the noncatalytic site binds cGMP in the anti-conformation. The numerous noncovalent interactions between cGMP and the noncatalytic binding pocket of the photoreceptor PDE described in this study account for both the high affinity for cGMP and the high level of discrimination of cGMP from other cyclic nucleotides at the noncatalytic site.Visual excitation of vertebrate retinal photoreceptors begins with the absorption of light by the visual pigment (opsin) which is followed by activation of a G-protein, transducin. This results in activation of a photoreceptor-specific cGMP phosphodiesterase (PDE).1 Increased cGMP hydrolysis lowers the cytoplasmic cGMP concentration which is believed to cause closure of the cGMP-gated ion channel in the plasma membrane and the generation of an electrical response (for reviews, see Refs. 1-5).The rod photoreceptor PDE holoenzyme is a heterotetramer consisting of two non-identical catalytic subunits (␣ and ␤) and two small subunits (␥) that serve to inhibit catalytic activity. Cone photoreceptors have a highly homologous PDE that consists of two identical catalytic subunits (␣Ј) and two conespecific ␥Ј subunits. In addition to containing the active site for cGMP hydrolysis, the catalytic subunits of rod and cone PDEs also possess noncatalytic cGMP binding sites (6). Two other classes of PDEs, namely the cGMP-stimulated PDE (PDE2) and the cGMP-specific PDE (PDE5), are also known to contain noncatalytic binding sites for cGMP. In the case of PDE2, binding of cGMP at the noncatalytic site allosterically activates cyclic nucleotide hydrolysis at the active site (7,8). For PDE5, the...

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Regulation of Cell-Fate Determination in Dictyostelium

Brown

Firtel

1999

Developmental Biology

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A key step in the development of all multicellular organisms is the differentiation of specialized cell types. The eukaryotic microorganism Dictyostelium discoideum provides a unique experimental system for studying cell-type determination and spatial patterning in a developing multicellular organism. Unlike metazoans, which become multicellular by undergoing many rounds of cell division after fertilization of an egg, the social amoeba Dictyostelium achieves multicellularity by the aggregation of approximately 10(5) cells in response to nutrient depletion. Following aggregation, cell-type differentiation and morphogenesis result in a multicellular organism with only a few cell types that exhibit a defined patterning along the anterior-posterior axis of the organism. Analysis of the mechanisms that control these processes is facilitated by the relative simplicity of Dictyostelium development and the availability of molecular, genetic, and cell biological tools. Interestingly, analysis has shown that many molecules that play integral roles in the development of higher eukaryotes, such as PKA, STATs, and GSK-3, are also essential for cell-type differentiation and patterning in Dictyostelium. The role of these and other signaling pathways in the induction, maintenance, and patterning of cell types during Dictyostelium development is discussed.

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Cyclic nucleotide specificity of the activator and catalytic sites of a cGMP‐stimulated cGMP phosphodiesterase from Dictyostelium discoideum

Cited by 18 publications

References 35 publications

Identification of a Novel Type of cGMP Phosphodiesterase That Is Defective in the ChemotacticstmFMutants

Identification of a Novel Type of cGMP Phosphodiesterase That Is Defective in the ChemotacticstmFMutants

Structural Features of the Noncatalytic cGMP Binding Sites of Frog Photoreceptor Phosphodiesterase Using cGMP Analogs

Regulation of Cell-Fate Determination in Dictyostelium

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