Bacterial Cell Wall Recycling

Mayer, Christoph

doi:10.1002/9780470015902.a0021974

Cited by 12 publications

(17 citation statements)

References 57 publications

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“…Generally, in bacteria about two‐thirds of peptidoglycan is degraded during cell wall turnover in cell division by lytic transglycosylases and endopeptidases, releasing GlcNAc‐1, 6‐anhydro‐MurNAc‐ l ‐Ala‐ d ‐Glu‐mesoDAP‐ d ‐Ala (anhydro‐muropeptide) as a major degradation product. In most Gram‐negative bacteria, the released muropeptides are then recycled into the cytoplasm via the AmpG‐like permeases . Orthologs of peptidoglycan recycling enzymes have been identified in some Gram‐positive bacteria as well, such as in Bacillus subtilis and Clostridium acetobutylicum .…”

Section: Survival Through Recycling Environmental Peptidoglycan Fragmmentioning

confidence: 99%

“…In many Gram‐negative bacteria, but not E. coli , muropeptide fragments entering the cytoplasm due to cell wall damage or cell wall recycling regulate induction of chromosomal AmpC‐type β‐lactamases, which can provide resistance to β‐lactam antibiotics . For the purpose of peptidoglycan synthesis, after entering the cytoplasm, muropeptides are further broken down by amidases and carboxypeptidases to release GlcNAc, anhMurNAc, murein tripeptides and d ‐Ala, which then enter the peptidoglycan biosynthetic pathway . In the oral cavity, peptidoglycan fragments released from the cohabiting bacteria as a result of their cell wall turnover or death are expected to be available to T. forsythia .…”

Section: Survival Through Recycling Environmental Peptidoglycan Fragmmentioning

confidence: 99%

“…In most Gram-negative bacteria, the released muropeptides are then recycled into the cytoplasm via the AmpG-like permeases. 6,27,28 Orthologs of peptidoglycan recycling enzymes have been identified in some Gram-positive bacteria as well, such as in Bacillus subtilis and Clostridium acetobutylicum. 34,36 In some bacteria, peptidoglycan fragments (muropeptides) function as important messengers in bacterial communication, and as antidormancy and spore resuscitation signals in some Gram-positive bacteria.…”

Section: Survival Through Recycling Environmental Peptidoglycan Framentioning

confidence: 99%

“…27 For the purpose of peptidoglycan synthesis, after entering the cytoplasm, muropeptides are further broken down by amidases and carboxypeptidases to release GlcNAc, anhMurNAc, murein tripeptides and d-Ala, which then enter the peptidoglycan biosynthetic pathway. 6,27,28 In the oral cavity, peptidoglycan fragments released from the cohabiting bacteria as a result of their cell wall turnover or death are expected to be available to T. forsythia. Importantly, scavenging on these fragments by T. forsythia is even more significant given that the human host does not make the peptidoglycan amino sugars.…”

Section: Survival Through Recycling Environmental Peptidoglycan Framentioning

confidence: 99%

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Peptidoglycan synthesis in Tannerella forsythia: Scavenging is the modus operandi

Ruscitto¹,

Sharma

2018

Molecular Oral Microbiology

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Tannerella forsythia is a Gram-negative oral pathogen strongly associated with periodontitis. This bacterium has an absolute requirement for exogenous N-acetylmuramic acid (MurNAc), an amino sugar that forms the repeating disaccharide unit with amino sugar N-acetylglucosamine (GlcNAc) of the peptidoglycan backbone. In silico genome analysis indicates that T. forsythia lacks the key biosynthetic enzymes needed for the de novo synthesis of MurNAc, and so relies on alternative ways to meet its requirement for peptidoglycan biosynthesis. In the subgingival niche, the bacterium can acquire MurNAc and peptidoglycan fragments (muropeptides) released by the cohabiting bacteria during their cell wall breakdown associated with cell division. Tannerella forsythia is able to also use host sialic acid (Neu5Ac) in lieu of MurNAc or muropeptides for its survival during the biofilm growth. Evidence suggests that the bacterium might be able to shunt sialic acid into a metabolic pathway leading to peptidoglycan synthesis. In this review, we explore the mechanisms by which T. forsythia is able to scavenge MurNAc, muropeptide and sialic acid for its peptidoglycan synthesis, and the impact of these scavenging activities on pathogenesis.

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Section: Survival Through Recycling Environmental Peptidoglycan Fragmmentioning

confidence: 99%

Section: Survival Through Recycling Environmental Peptidoglycan Fragmmentioning

confidence: 99%

Section: Survival Through Recycling Environmental Peptidoglycan Framentioning

confidence: 99%

Section: Survival Through Recycling Environmental Peptidoglycan Framentioning

confidence: 99%

See 2 more Smart Citations

Peptidoglycan synthesis in Tannerella forsythia: Scavenging is the modus operandi

Ruscitto¹,

Sharma

2018

Molecular Oral Microbiology

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“…The bacterial peptidoglycan is a large, meshlike macromolecule consisting of polysaccharide chains of alternating N-acetylglucosamine (GlcNAc) and N-acetylmuramic acid (MurNAc) 4 links that are connected via short oligopeptide bridges (1). The biosynthesis of peptidoglycan is highly conserved and essential for bacteria, and enzymes within this synthetic pathway therefore represent attractive targets for antibacterial drug design.…”

mentioning

confidence: 99%

Crystal Structure of the N-Acetylmuramic Acid α-1-Phosphate (MurNAc-α1-P) Uridylyltransferase MurU, a Minimal Sugar Nucleotidyltransferase and Potential Drug Target Enzyme in Gram-negative Pathogens

Renner-Schneck

Hinderberger

Gisin

et al. 2015

Journal of Biological Chemistry

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Background: N-Acetylmuramic acid ␣-1-phosphate (MurNAc-␣1-P) uridylyltransferase MurU contributes to a shortcut in Pseudomonas putida cell wall biosynthesis accounting for intrinsic fosfomycin resistance. Results: This work provides the first structural analysis of a MurNAc-␣1-P uridylyltransferase. Conclusion: MurNAc-␣1-P and UTP are coordinated at distinct sites in the active center. Significance: The presented structure represents a "minimal nucleotidyltransferase domain" and may provide structural guidelines for inhibitor design.

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Macromolecular Machineries in Cell‐Wall Recycling

Batuecas

Hermoso

2019

Encyclopedia of Life Sciences

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Peptidoglycan, the major constituent of bacterial cell wall, is a huge polymeric macromolecule composed of glycan strands covalently linked by interconnecting peptide stems and critical for survival of bacteria. Peptidoglycan is constantly edited, biosynthesised and degraded, during essential bacterial processes such as division, elongation or insertion of the cellular machinery (e.g. flagella, pili) into cell wall. Degradation fragments are recovered, especially in Gram‐negative bacteria, by active transport and recycled to rebuild the wall. In some important Gram‐negative pathogens, β‐lactam resistance is directly linked to peptidoglycan recycling. The recycling process requires orchestration of different lytic enzymes and transporters from periplasm, the inner membrane, to cytoplasm. Recent structural and functional studies have provided relevant insights into enzymatic regulation, substrate specificity and activity of the lytic machineries involved in recycling with relevant implications in antibiotics resistance. Key Concepts Peptidoglycan recycling is an essential process in Gram‐negative bacteria that recovers self‐degradation products of cell wall in the cytoplasm to reutilise them to rebuild the wall. PG recycling is important in cell‐wall biosynthesis and in bacterial communication in many bacteria, and in antibiotics resistance in some pathogens from Enterobacteriaceae and Pseudomonadaceae families. PG recycling involves a large number of enzymes and transporters spanning from periplasm, inner and outer membranes, and cytoplasm. Lytic transglycosylases (LTs) are periplasmic and, typically, modular enzymes that initiate PG recycling by non‐hydrolytic degradation of glycan chains. They are classified in six families. Several LTs are found in each Gram‐negative bacterium. The Slt structure reveals how, under the effect of β‐lactam antibiotics, the cell wall is repaired by degradation of aberrant nascent PG chains and how it initiates the resistance phenotype. MltF is a modular membrane‐bound LT that experiences allosteric activation triggered by muropeptides. PG amidases are present in periplasm and cytoplasm. Activity in periplasm is regulated by cellular location, protein–protein interactions and oligomeric state. An activation mechanism has been discovered for cytosolic enzymes. Anhydro‐muropeptides are the key molecules to activate the AmpR to induce AmpC β‐lactamase in response to β‐lactam challenge. Regulation (in space and time) of the catalytic processes as well as of interaction between different partners is essential in PG recycling enzymes.

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Bacterial Cell Wall Recycling

Cited by 12 publications

References 57 publications

Peptidoglycan synthesis in Tannerella forsythia: Scavenging is the modus operandi

Peptidoglycan synthesis in Tannerella forsythia: Scavenging is the modus operandi

Crystal Structure of the N-Acetylmuramic Acid α-1-Phosphate (MurNAc-α1-P) Uridylyltransferase MurU, a Minimal Sugar Nucleotidyltransferase and Potential Drug Target Enzyme in Gram-negative Pathogens

Macromolecular Machineries in Cell‐Wall Recycling

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