Tracking interactions that stabilize the dimer structure of starch phosphorylase from <i>Corynebacterium callunae</i>

Griessler, Richard; Schwarz, Alexandra; Mucha, Ján; Nidetzky, Bernd

doi:10.1046/j.1432-1033.2003.03562.x

Cited by 10 publications

(32 citation statements)

References 33 publications

(112 reference statements)

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“…Considering results of previous studies delineating the disruptive effect of individual site-directed substitutions of Arg 234 and Arg 242 by Ala (R234A, R242A) on orthophosphate-dependent stability of Cc GlgP [15], we here selected Arg 141 from the P-site for mutational analysis. Figure 1A shows that Arg 242 has indirect interactions with orthophosphate via the co-ordinating Glu 235 .…”

Section: Resultsmentioning

confidence: 99%

“…The plasmid pQE 30-GlgP harbouring the gene encoding wild-type Cc GlgP fused to an N-terminal metal affinity peptide (RGSHHHHHHGSA) [15] was used as template for site-directed mutagenesis. Mutations were introduced by employing a modified two-stage PCR protocol [18] in which the following pairs of oligonucleotide primers (Invitrogen) were used with mismatched codons underlined.…”

Section: Methodsmentioning

confidence: 99%

“…Phosphorylase activity was measured with a continuous coupled enzyme assay described elsewhere [15]. The Bio-Rad dye binding assay referenced against BSA was used for determination of protein concentrations.…”

Section: Methodsmentioning

confidence: 99%

“…Occupancy of the P-site was thought to result in substantially stabilized intersubunit contacts. Results of mutagenesis experiments located residues responsible for orthophosphate-dependent stability in the region of the so-called TOWER helix, a conserved secondary structural element of the dimer interface in GlgP enzymes [11,15,16]. The crystal structure of Cc GlgP at 1.9 Å resolution (PDB code: 2C4M) now reveals that not one but three orthophosphate sites are dispersed across the dimer contact region of the enzyme.…”

Section: Introductionmentioning

confidence: 99%

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Orthophosphate binding at the dimer interface of Corynebacterium callunae starch phosphorylase: mutational analysis of its role for activity and stability of the enzyme

Mueller

Nidetzky

2010

BMC Biochemistry

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BackgroundOrthophosphate recognition at allosteric binding sites is a key feature for the regulation of enzyme activity in mammalian glycogen phosphorylases. Protein residues co-ordinating orthophosphate in three binding sites distributed across the dimer interface of a non-regulated bacterial starch phosphorylase (from Corynebacterium callunae) were individually replaced by Ala to interrogate their unknown function for activity and stability of this enzyme.ResultsWhile the mutations affected neither content of pyridoxal 5'-phosphate cofactor nor specific activity in phosphorylase preparations as isolated, they disrupted (Thr28→Ala, Arg141→Ala) or decreased (Lys31→Ala, Ser174→Ala) the unusually strong protective effect of orthophosphate (10 or 100 mM) against inactivation at 45°C and subunit dissociation enforced by imidazole, as compared to wild-type enzyme. Loss of stability in the mutated phosphorylases appeared to be largely due to weakened affinity for orthophosphate binding. Binding of sulphate mimicking the crystallographically observed "non-covalent phosphorylation" of the phosphorylase at the dimer interface did not have an allosteric effect on the enzyme activity.ConclusionsThe phosphate sites at the subunit-subunit interface of C. callunae starch phosphorylase appear to be cooperatively functional in conferring extra kinetic stability to the native dimer structure of the active enzyme. The molecular strategy exploited for quaternary structure stabilization is to our knowledge novel among dimeric proteins. It can be distinguished clearly from the co-solute effect of orthophosphate on protein thermostability resulting from (relatively weak) interactions of the ligand with protein surface residues.

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Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Orthophosphate binding at the dimer interface of Corynebacterium callunae starch phosphorylase: mutational analysis of its role for activity and stability of the enzyme

Mueller

Nidetzky

2010

BMC Biochemistry

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“…Therefore, we investigate in this communication also the effects of the deletion of glgA and glgC on malP transcription and MalP activity. The well-characterized ␣-glucan phosphorylase CcStP from Corynebacterium callunae was described as a starch phosphorylase based on its substrate preference for the branched glucose-polymer starch over linear maltodextrins (13,(46)(47)(48)(49)(50)(51)(52). Based on the close relatedness of C. glutamicum MalP to CcStP, which probably acts as the glycogen phosphorylase in C. callunae, we also analyzed the substrate spectrum of C. glutamicum MalP as well as control of MalP activity by ATP, ADP, AMP, and ADP-glucose.…”

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The α-Glucan Phosphorylase MalP of Corynebacterium glutamicum Is Subject to Transcriptional Regulation and Competitive Inhibition by ADP-Glucose

et al. 2015

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ABSTRACT␣-Glucan phosphorylases contribute to degradation of glycogen and maltodextrins formed in the course of maltose metabolism in bacteria. Accordingly, bacterial ␣-glucan phosphorylases are classified as either glycogen or maltodextrin phosphorylase, GlgP or MalP, respectively. GlgP and MalP enzymes follow the same catalytic mechanism, and thus their substrate spectra overlap; however, they differ in their regulation: GlgP genes are constitutively expressed and the enzymes are controlled on the activity level, whereas expression of MalP genes are transcriptionally controlled in response to the carbon source used for cultivation. We characterize here the modes of control of the ␣-glucan phosphorylase MalP of the Gram-positive Corynebacterium glutamicum. In accordance to the proposed function of the malP gene product as MalP, we found transcription of malP to be regulated in response to the carbon source. Moreover, malP transcription is shown to depend on the growth phase and to occur independently of the cell glycogen content. Surprisingly, we also found MalP activity to be tightly regulated competitively by the presence of ADP-glucose, an intermediate of glycogen synthesis. Since the latter is considered a typical feature of GlgPs, we propose that C. glutamicum MalP acts as both maltodextrin and glycogen phosphorylase and, based on these findings, we question the current system for classification of bacterial ␣-glucan phosphorylases. IMPORTANCEBacterial ␣-glucan phosphorylases have been classified conferring to their purpose as either glycogen or maltodextrin phosphorylases. We found transcription of malP in C. glutamicum to be regulated in response to the carbon source, which is recognized as typical for maltodextrin phosphorylases. Surprisingly, we also found MalP activity to be tightly regulated competitively by the presence of ADP-glucose, an intermediate of glycogen synthesis. The latter is considered a typical feature of GlgPs. These findings, taken together, suggest that C. glutamicum MalP is the first ␣-glucan phosphorylase that does not fit into the current system for classification of bacterial ␣-glucan phosphorylases and exemplifies the complex mechanisms underlying the control of glycogen content and maltose metabolism in this model organism.T he ␣-glucan phosphorylases (EC 2.4.1.1) catalyze the reversible cleavage of ␣-1,4-glycosidic linkages in polysaccharides, thereby liberating ␣-glucose-1-phosphate. By this means, ␣-glucan phosphorylases participate in metabolic processes such as degradation of the intracellular storage polysaccharides glycogen and starch (1, 2), as well as the degradation of maltodextrins formed both in the course of the maltose metabolism of various bacteria (3, 4) and in the cytosol of plant leaves (5-7). Several ␣-glucan phosphorylases have been extensively studied, their crystal structures have been solved, and the catalytic mechanisms have been described (8-11). Although the catalytic mechanisms appear to be similar in all hitherto characterized phosphorylases (12-14)...

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Glucosylglycerol and glucosylglycerate as enzyme stabilizers

Sawangwan

Goedl

Nidetzky

2010

Biotechnology Journal

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Compatible solutes constitute a diverse class of low-molecular-mass organic molecules that are accumulated in high intracellular concentrations in response to the external stress of hyperosmolality or high temperature. Many of these compounds like alpha, alpha-trehalose are well known for their stabilizing effect on protein structure and could lead to development of more stable protein formulations. Negatively charged solutes like mannosylglycerate (R-2-O-alpha-D-mannopyranosyl-glycerate) are widespread among (hyper)thermophilic microorganisms and are thought to be exceptionally potent stabilizers of proteins under high-temperature denaturation conditions. To further inquire into the role of compound charge for protective function, we have compared two naturally occurring and structurally related solutes, glucosylglycerol (2-O-alpha-D-glucopyranosyl-sn-glycerol) and glucosylglycerate (R-2-O-alpha-D-glucopyranosyl-glycerate), as stabilizers of different enzymes undergoing inactivation through elevated temperature or freeze drying, and benchmarked their effects against that of alpha,alpha-trehalose. Glucosylglycerate in concentrations of >/=0.1 M was the most effective in preventing thermally induced loss of enzyme activity of lactate dehydrogenase, mannitol dehydrogenase, starch phosphorylase, and xylose reductase. alpha,alpha-Trehalose could usually be replaced by glucosylglycerol without compromising enzyme stability. Glucosylglycerol and glucosylglycerate afforded substantial (eightfold) protection to mannitol dehydrogenase during freeze drying.

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Tracking interactions that stabilize the dimer structure of starch phosphorylase from Corynebacterium callunae

Cited by 10 publications

References 33 publications

Orthophosphate binding at the dimer interface of Corynebacterium callunae starch phosphorylase: mutational analysis of its role for activity and stability of the enzyme

Orthophosphate binding at the dimer interface of Corynebacterium callunae starch phosphorylase: mutational analysis of its role for activity and stability of the enzyme

The α-Glucan Phosphorylase MalP of Corynebacterium glutamicum Is Subject to Transcriptional Regulation and Competitive Inhibition by ADP-Glucose

Glucosylglycerol and glucosylglycerate as enzyme stabilizers

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