Direct Interaction of Polar Scaffolding Protein Wag31 with Nucleoid-Associated Protein Rv3852 Regulates Its Polar Localization

Rv3852 is a unique nucleoid-associated protein (NAP) found exclusively in Mycobacterium tuberculosis (Mtb) and closely related species. Although annotated as H-NS, we showed previously that it is very different from H-NS in its properties and is distinct from other NAPs, anchoring to cell membrane by virtue of possessing a C-terminal transmembrane helix. Here, we investigated the role of Rv3852 in Mtb in organizing architecture or synthesis machinery of cell wall by protein–protein interaction approach. We demonstrated a direct physical interaction of Rv3852 with Wag31, an important cell shape and cell wall integrity determinant essential in Mtb. Wag31 localizes to the cell poles and possibly acts as a scaffold for cell wall synthesis proteins, resulting in polar cell growth in Mtb. Ectopic expression of Rv3852 in M. smegmatis resulted in its interaction with Wag31 orthologue DivIVAMsm. Binding of the NAP to Wag31 appears to be necessary for fine-tuning Wag31 localization to the cell poles, enabling complex cell wall synthesis in Mtb. In Rv3852 knockout background, Wag31 is mislocalized resulting in disturbed nascent peptidoglycan synthesis, suggesting that the NAP acts as a driver for localization of Wag31 to the cell poles. While this novel association between these two proteins presents one of the mechanisms to structure the elaborate multi-layered cell envelope of Mtb, it also exemplifies a new function for a NAP in mycobacteria.

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CsiA is a bacterial cell wall synthesis inhibitor contributing to DNA translocation through the cell envelope

Molecular Microbiology ◽

10.1111/j.1365-2958.2009.06683.x ◽

2009 ◽

Vol 72 (3) ◽

pp. 779-794 ◽

Cited By ~ 8

Author(s):

Régis Stentz ◽

Udo Wegmann ◽

Mary Parker ◽

Roy Bongaerts ◽

Laurie Lesaint ◽

...

Keyword(s):

Cell Wall ◽

Bacterial Cell ◽

Cell Envelope ◽

Bacterial Cell Wall ◽

Cell Wall Synthesis ◽

Dna Translocation ◽

Synthesis Inhibitor ◽

Cell Wall Synthesis Inhibitor

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A cell wall damage response mediated by a sensor kinase/response regulator pair enables beta-lactam tolerance

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1520333113 ◽

2015 ◽

Vol 113 (2) ◽

pp. 404-409 ◽

Cited By ~ 34

Author(s):

Tobias Dörr ◽

Laura Alvarez ◽

Fernanda Delgado ◽

Brigid M. Davis ◽

Felipe Cava ◽

...

Keyword(s):

Cell Wall ◽

Response Regulator ◽

Cell Envelope ◽

Normal Growth ◽

Cell Diameter ◽

Cell Wall Synthesis ◽

Beta Lactam ◽

Cell Wall Damage ◽

A Cell

The bacterial cell wall is critical for maintenance of cell shape and survival. Following exposure to antibiotics that target enzymes required for cell wall synthesis, bacteria typically lyse. Although several cell envelope stress response systems have been well described, there is little knowledge of systems that modulate cell wall synthesis in response to cell wall damage, particularly in Gram-negative bacteria. Here we describe WigK/WigR, a histidine kinase/response regulator pair that enablesVibrio cholerae, the cholera pathogen, to survive exposure to antibiotics targeting cell wall synthesis in vitro and during infection. Unlike wild-typeV. cholerae, mutants lackingwigRfail to recover following exposure to cell-wall–acting antibiotics, and they exhibit a drastically increased cell diameter in the absence of such antibiotics. Conversely, overexpression ofwigRleads to cell slimming. Overexpression of activated WigR also results in increased expression of the full set of cell wall synthesis genes and to elevated cell wall content. WigKR-dependent expression of cell wall synthesis genes is induced by various cell-wall–acting antibiotics as well as by overexpression of an endogenous cell wall hydrolase. Thus, WigKR appears to monitor cell wall integrity and to enhance the capacity for increased cell wall production in response to damage. Taken together, these findings implicate WigKR as a regulator of cell wall synthesis that controls cell wall homeostasis in response to antibiotics and likely during normal growth as well.

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Modulation of the enzymatic activity of the flagellar lytic transglycosylase SltF by rod components, and the scaffolding protein FlgJ in Rhodobacter sphaeroides .

Journal of Bacteriology ◽

10.1128/jb.00372-21 ◽

2021 ◽

Author(s):

Mariela García-Ramos ◽

Javier de la Mora ◽

Teresa Ballado ◽

Laura Camarena ◽

Georges Dreyfus

Keyword(s):

Cell Wall ◽

Enzymatic Activity ◽

Rhodobacter Sphaeroides ◽

Cell Envelope ◽

Scaffold Protein ◽

Scaffolding Protein ◽

Lytic Enzyme ◽

Periplasmic Space ◽

Bacterial Flagellum ◽

Lytic Transglycosylase

Macromolecular cell-envelope-spanning structures such as the bacterial flagellum must traverse the cell wall. Lytic transglycosylases enzymes are capable of enlarging gaps in the peptidoglycan meshwork to allow the efficient assembly of supramolecular complexes. In the periplasmic space, the assembly of the flagellar rod requires the scaffold protein FlgJ, which includes a muramidase domain in the canonical models Salmonella enterica and Escherichia coli . In contrast, in Rhodobacter sphaeroides , FlgJ and the dedicated flagellar lytic transglycosylase SltF are separate entities that interact in the periplasm. In this study we show that sltF is expressed along with the genes encoding the early components of the flagellar hierarchy that include the hook-basal body proteins, making SltF available during the rod assembly. Protein-protein interaction experiments demonstrated that SltF interacts with the rod proteins FliE, FlgB, FlgC, FlgF and FlgG through its C-terminal region. A deletion analysis that divides the C-terminus in two halves revealed that the interacting regions for most of the rod proteins are not redundant. Our results also show that the presence of the rod proteins FliE, FlgB, FlgC, and FlgF displace the previously reported SltF-FlgJ interaction. In addition, we observed modulation of the transglycosylase activity of SltF mediated by FlgB and FlgJ that could be relevant to coordinate rod assembly with cell wall remodeling. In summary, different mechanisms regulate the flagellar lytic transglycosylase, SltF ensuring a timely transcription, a proper localization and a controlled enzymatic activity. Importance Several mechanisms participate in the assembly of cell-envelope-spanning macromolecular structures. The sequential expression of substrates to be exported, selective export, and a specific order of incorporation are some of the mechanisms that stand out to drive an efficient assembly process. In this work we analyze how the structural rod proteins, the scaffold protein FlgJ and the flagellar lytic enzyme SltF, interact in an orderly fashion to assemble the flagellar rod into the periplasmic space. A complex arrangement of transient interactions directs a dedicated flagellar muramidase towards the flagellar rod. All these interactions bring this protein to the proximity of the peptidoglycan wall while also modulating its enzymatic activity. This study suggests how a dynamic network of interactions participates in controlling SltF, a prominent component for flagellar formation.

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The transpeptidase PBP2 governs initial localization and activity of the major cell-wall synthesis machinery in E. coli

eLife ◽

10.7554/elife.50629 ◽

2020 ◽

Vol 9 ◽

Cited By ~ 4

Author(s):

Gizem Özbaykal ◽

Eva Wollrab ◽

Francois Simon ◽

Antoine Vigouroux ◽

Baptiste Cordier ◽

...

Keyword(s):

Cell Wall ◽

Cell Envelope ◽

Cylindrical Part ◽

Single Particle Tracking ◽

Cell Wall Synthesis ◽

E Coli ◽

Peptidoglycan Cell Wall ◽

Direct Binding ◽

Local Cell ◽

Residual Correlations

Bacterial shape is physically determined by the peptidoglycan cell wall. The cell-wall-synthesis machinery responsible for rod shape in Escherichia coli is the processive 'Rod complex'. Previously, cytoplasmic MreB filaments were thought to govern formation and localization of Rod complexes based on local cell-envelope curvature. Using single-particle tracking of the transpeptidase and Rod-complex component PBP2, we found that PBP2 binds to a substrate different from MreB. Depletion and localization experiments of other putative Rod-complex components provide evidence that none of those provide the sole rate-limiting substrate for PBP2 binding. Consistently, we found only weak correlations between MreB and envelope curvature in the cylindrical part of cells. Residual correlations do not require curvature-based Rod-complex initiation but can be attributed to persistent rotational motion. We therefore speculate that the local cell-wall architecture provides the cue for Rod-complex initiation, either through direct binding by PBP2 or through an unknown intermediate.

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Ectopic expression of LBD15 affects lateral branch development and secondary cell wall synthesis in Arabidopsis thaliana

Plant Growth Regulation ◽

10.1007/s10725-013-9873-9 ◽

2013 ◽

Vol 73 (2) ◽

pp. 111-120 ◽

Cited By ~ 4

Author(s):

Lin Zhu ◽

Jiansheng Guo ◽

Cheng Zhou ◽

Jian Zhu

Keyword(s):

Arabidopsis Thaliana ◽

Cell Wall ◽

Secondary Cell Wall ◽

Ectopic Expression ◽

Lateral Branch ◽

Cell Wall Synthesis ◽

Branch Development ◽

Secondary Cell Wall Synthesis

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Transpeptidase PBP2 governs initial localization and activity of major cell-wall synthesis machinery in Escherichia coli

10.1101/716407 ◽

2019 ◽

Cited By ~ 2

Author(s):

Eva Wollrab ◽

Gizem Özbaykal ◽

Antoine Vigouroux ◽

Baptiste Cordier ◽

Francois Simon ◽

...

Keyword(s):

Escherichia Coli ◽

Cell Wall ◽

Cell Envelope ◽

Cylindrical Part ◽

Single Particle Tracking ◽

Cell Wall Synthesis ◽

Complex Activity ◽

Peptidoglycan Cell Wall ◽

Local Cell ◽

Residual Correlations

AbstractBacterial shape is physically determined by the peptidoglycan cell wall. The cell-wall-synthesis machinery responsible for rod shape in Escherichia coli is the processive ‘Rod complex’. Previously, cytoplasmic MreB filaments were thought to govern formation and localization of Rod complexes based on local cell-envelope curvature. However, using single-particle tracking of the transpeptidase PBP2, we found strong evidence that PBP2 initiates new Rod complexes by binding to a substrate different from MreB or any known Rod-complex component. This substrate is likely the cell wall. Consistently, we found only weak correlations between MreB and envelope curvature in the cylindrical part of cells. Residual correlations do not require any curvature-based Rod-complex initiation but can be attributed to persistent rotational motion. Therefore, local cell-wall architecture likely provides the cue for PBP2 binding and subsequent Rod-complex initiation. We also found that PBP2 has a limiting role for Rod-complex activity, thus supporting its central role.

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Esx Systems and the Mycobacterial Cell Envelope: What's the Connection?

Journal of Bacteriology ◽

10.1128/jb.00131-17 ◽

2017 ◽

Vol 199 (17) ◽

Cited By ~ 20

Author(s):

Rachel E. Bosserman ◽

Patricia A. Champion

Keyword(s):

Cell Wall ◽

Outer Membrane ◽

Protein Transport ◽

Cytoplasmic Membrane ◽

Cell Envelope ◽

Transport Proteins ◽

Cell Wall Synthesis ◽

Mycobacterial Cell ◽

Genes Encoding ◽

Associated Proteins

ABSTRACT Mycobacterial 6-kDa early secreted antigenic target (ESAT-6) system (ESX) exporters transport proteins across the cytoplasmic membrane. Many proteins transported by ESX systems are then translocated across the mycobacterial cell envelope and secreted from the cell. Although the mechanism underlying protein transport across the mycolate outer membrane remains elusive, the ESX systems are closely connected with and localize to the cell envelope. Links between ESX-associated proteins, cell wall synthesis, and the maintenance of cell envelope integrity have been reported. Genes encoding the ESX systems and those required for biosynthesis of the mycobacterial envelope are coregulated. Here, we review the interplay between ESX systems and the mycobacterial cell envelope.

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In vitro assembly of 2-D crystals from partially purified EA1 protein secreted by Bacillus anthracis strain Delta Sterne-1

Proceedings, annual meeting, Electron Microscopy Society of America ◽

10.1017/s0424820100169110 ◽

1994 ◽

Vol 52 ◽

pp. 276-277

Author(s):

Mary Beth Downs ◽

Wilson Ribot ◽

Joseph W. Farchaus

Keyword(s):

Cell Wall ◽

Molecular Sieves ◽

Cell Envelope ◽

Single Species ◽

Supporting Cell ◽

Surface Layers ◽

Rabbit Igg ◽

In Vitro Assembly ◽

Covalently Linked

Many bacteria possess surface layers (S-layers) that consist of a two-dimensional protein lattice external to the cell envelope. These S-layer arrays are usually composed of a single species of protein or glycoprotein and are not covalently linked to the underlying cell wall. When removed from the cell, S-layer proteins often reassemble into a lattice identical to that found on the cell, even without supporting cell wall fragments. S-layers exist at the interface between the cell and its environment and probably serve as molecular sieves that exclude destructive macromolecules while allowing passage of small nutrients and secreted proteins. Some S-layers are refractory to ingestion by macrophages and, generally, bacteria are more virulent when S-layers are present.When grown in rich medium under aerobic conditions, B. anthracis strain Delta Sterne-1 secretes large amounts of a proteinaceous extractable antigen 1 (EA1) into the growth medium. Immunocytochemistry with rabbit polyclonal anti-EAl antibody made against the secreted protein and gold-conjugated goat anti-rabbit IgG showed that EAI was localized at the cell surface (fig 1), which suggests its role as an S-layer protein.

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