The glgB-encoded glycogen branching enzyme is essential for glycogen accumulation in Corynebacterium glutamicum

Seibold, Gerd M.; Breitinger, Katrin J.; Kempkes, Raoul; Both, Leonard; M, Kramer; Dempf, Stefan; Eikmanns, Bernhard J.

doi:10.1099/mic.0.051565-0

Cited by 19 publications

(18 citation statements)

References 40 publications

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“…(16)(17)(18)(19)(20) It has also been suggested that bacteria make distinct forms of glycogen depending on their environment. Bacteria like Enterobacteria, that live primarily in other organisms where food is relatively plentiful, tend to have glycogen made up of longer average glucan chains, while organisms that must survive for extended periods outside of a host, in relatively hostile environments, tend to produce glycogen with much shorter average glucan chains.…”

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Crystal Structures of Escherichia coli Branching Enzyme in Complex with Linear Oligosaccharides

et al. 2015

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Branching enzyme is responsible for all branching of glycogen and starch. It is an unusual member of the α-amylase family because it has both α-1,4-amylase activity and α-1,6-transferase activity [Drummond, G. S., et al. (1972) Eur. J. Biochem. 26, 168-176]. It also does not react with shorter glucans, though it will bind much longer substrates and substrate mimics [Binderup, K., et al. (2002) Arch. Biochem. Biophys. 397, 279-285]. In an effort to better understand how branching enzyme interacts with its polymeric substrate, we have determined the structure of Δ112 Escherichia coli branching enzyme bound to maltoheptaose and maltohexaose. Together, these structures define six distinct oligosaccharide binding sites on the surface of E. coli branching enzyme. Most of these binding sites surround the edge of the β-barrel domain and are quite far from the active site. Surprisingly, there is no evidence of oligosaccharide binding in the active site of the enzyme. The closest bound oligosaccharide resides almost 18 Å from the active site. Mutations to conserved residues in binding sites I and VI had a debilitating effect on the activity of the enzyme.

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confidence: 99%

Crystal Structures of Escherichia coli Branching Enzyme in Complex with Linear Oligosaccharides

et al. 2015

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“…In a similar manner, transcription of the genes glgC, glgA, and glgB for glycogen synthesis is induced in cultivations with glucose and repressed in cultivations with acetate (42,44). The two global regulators RamA and RamB are involved in the control of glgC and/or glgA transcription; however, the substrate-dependent transcriptional control of these two genes is brought about by an as-yet-unknown regulator (44).…”

Section: Discussionmentioning

confidence: 84%

“…For quantification of ␣-glucan degradation products, the bicinchoninic acid assay was used as described previously (42). Glucose solutions (0 to 25 M) were used for the calibration.…”

Section: Methodsmentioning

confidence: 99%

“…In cultivations of C. glutamicum on glucose, large amounts of glycogen are synthesized in the early exponential growth phase from glc-6-P by the consecutive action of phosphoglucomutase (Pgm), ADP-glucose pyrophosphorylase (GlgC), glycogen synthase (GlgA), and glycogen branching enzyme (GlgB) (34,40,42,43). Degradation of glycogen takes place in C. glutamicum before the entry of the stationary phase and proceeds by the concerted action of the glycogen debranching enzyme (GlgX) and the two ␣-glucan phosphorylases designated MalP and GlgP (41,43).…”

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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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“…Branching enzymes have been described in a variety of organisms, including plants [Carciofi et al, 2012;Huang et al, 2013;Kang et al, 2013;Yandeau-Nelson et al, 2011], animals [Lee et al, 2011;Ward et al, 2004;Ziemssen et al, 2000], fungi [Matsumoto et al, 1990] and bacteria [Roussel et al, 2013;Seibold et al, 2011]. However, only a few of these branching enzymes have been shown to be active at high temperatures.…”

Section: Introductionmentioning

confidence: 99%

Expression and Biochemical Characterization of a Thermostable Branching Enzyme from <b><i>Geobacillus thermoglucosidans</i></b>

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et al. 2016

Microb Physiol

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The branching enzyme (EC 2.4.1.18) catalyzes the formation of α-1,6 branch points in starch. In this study, the Geobacillus thermoglucosidans gene-encoding branching enzyme was expressed in Escherichia coli BL21 (DE3) and the protein was isolated and characterized. G. thermoglucosidans branching enzyme is a thermostable enzyme with an optimal reaction temperature of nearly 60°C and a half-life at 65°C of approximately 1.1 h. The activity of the recombinant enzyme is optimal at pH 7.5, with broad stability between pH 5.5 and 9.0. Its thermostability, relatively broad pH stability and optimal temperature near the temperature at which starch begins to gelatinize may make it easy to use in industrial production. Furthermore, the enzyme is activated by Mg²⁺, Ba²⁺, K⁺ and Na⁺ in a concentration-dependent manner and dramatically inhibited by Ni²⁺ and Co²⁺. Its substrate dependence, using amylopectin as the substrate, could be adequately fitted using the Michaelis-Menten equation, yielding a K_m of 0.99 mg/ml. High-performance anion exchange chromatography results showed that the chain length distribution of branching enzyme-treated waxy corn starch is indistinguishable from that of the branching enzyme-treated common corn starch. This enzyme may therefore be a promising tool for the enzymatic modification of starch.

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The glgB-encoded glycogen branching enzyme is essential for glycogen accumulation in Corynebacterium glutamicum

Cited by 19 publications

References 40 publications

Crystal Structures of Escherichia coli Branching Enzyme in Complex with Linear Oligosaccharides

Crystal Structures of Escherichia coli Branching Enzyme in Complex with Linear Oligosaccharides

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

Expression and Biochemical Characterization of a Thermostable Branching Enzyme from <b><i>Geobacillus thermoglucosidans</i></b>

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