Peptidoglycan synthesis drives an FtsZ-treadmilling-independent step of cytokinesis

João M. Monteiro; Ana R. Pereira; Nathalie T. Reichmann; Bruno M. Saraiva; Pedro B. Fernandes; Helena Veiga; Andreia C. Tavares; Margarida Santos; Maria T. Ferreira; Vânia Macário; Michael S. VanNieuwenhze; Sérgio R. Filipe; Mariana G. Pinho

doi:10.1038/nature25506

Peptidoglycan synthesis drives an FtsZ-treadmilling-independent step of cytokinesis

João M. Monteiro, Ana R. Pereira, Nathalie T. Reichmann, Bruno M. Saraiva, Pedro B. Fernandes, Helena Veiga, Andreia C. Tavares, Margarida Santos, Maria T. Ferreira, Vânia Macário, Michael S. VanNieuwenhze, Sérgio R. Filipe, Mariana G. Pinho

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114 Scopus citations

Abstract

Peptidoglycan is the main component of the bacterial wall and protects cells from the mechanical stress that results from high intracellular turgor. Peptidoglycan biosynthesis is very similar in all bacteria; bacterial shapes are therefore mainly determined by the spatial and temporal regulation of peptidoglycan synthesis rather than by the chemical composition of peptidoglycan. The form of rod-shaped bacteria, such as Bacillus subtilis or Escherichia coli, is generated by the action of two peptidoglycan synthesis machineries that act at the septum and at the lateral wall in processes coordinated by the cytoskeletal proteins FtsZ and MreB, respectively. The tubulin homologue FtsZ is the first protein recruited to the division site, where it assembles in filaments - forming the Z ring - that undergo treadmilling and recruit later divisome proteins. The rate of treadmilling in B. subtilis controls the rates of both peptidoglycan synthesis and cell division. The actin homologue MreB forms discrete patches that move circumferentially around the cell in tracks perpendicular to the long axis of the cell, and organize the insertion of new cell wall during elongation. Cocci such as Staphylococcus aureus possess only one type of peptidoglycan synthesis machinery, which is diverted from the cell periphery to the septum in preparation for division. The molecular cue that coordinates this transition has remained elusive. Here we investigate the localization of S. aureus peptidoglycan biosynthesis proteins and show that the recruitment of the putative lipid II flippase MurJ to the septum, by the DivIB-DivIC-FtsL complex, drives peptidoglycan incorporation to the midcell. MurJ recruitment corresponds to a turning point in cytokinesis, which is slow and dependent on FtsZ treadmilling before MurJ arrival but becomes faster and independent of FtsZ treadmilling after peptidoglycan synthesis activity is directed to the septum, where it provides additional force for cell envelope constriction.

Original language	English (US)
Pages (from-to)	528-532
Number of pages	5
Journal	Nature
Volume	554
Issue number	7693
DOIs	https://doi.org/10.1038/nature25506
State	Published - Feb 22 2018
Externally published	Yes

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@article{a31937a76c5f49beac470262e18d6bfb,

title = "Peptidoglycan synthesis drives an FtsZ-treadmilling-independent step of cytokinesis",

abstract = "Peptidoglycan is the main component of the bacterial wall and protects cells from the mechanical stress that results from high intracellular turgor. Peptidoglycan biosynthesis is very similar in all bacteria; bacterial shapes are therefore mainly determined by the spatial and temporal regulation of peptidoglycan synthesis rather than by the chemical composition of peptidoglycan. The form of rod-shaped bacteria, such as Bacillus subtilis or Escherichia coli, is generated by the action of two peptidoglycan synthesis machineries that act at the septum and at the lateral wall in processes coordinated by the cytoskeletal proteins FtsZ and MreB, respectively. The tubulin homologue FtsZ is the first protein recruited to the division site, where it assembles in filaments - forming the Z ring - that undergo treadmilling and recruit later divisome proteins. The rate of treadmilling in B. subtilis controls the rates of both peptidoglycan synthesis and cell division. The actin homologue MreB forms discrete patches that move circumferentially around the cell in tracks perpendicular to the long axis of the cell, and organize the insertion of new cell wall during elongation. Cocci such as Staphylococcus aureus possess only one type of peptidoglycan synthesis machinery, which is diverted from the cell periphery to the septum in preparation for division. The molecular cue that coordinates this transition has remained elusive. Here we investigate the localization of S. aureus peptidoglycan biosynthesis proteins and show that the recruitment of the putative lipid II flippase MurJ to the septum, by the DivIB-DivIC-FtsL complex, drives peptidoglycan incorporation to the midcell. MurJ recruitment corresponds to a turning point in cytokinesis, which is slow and dependent on FtsZ treadmilling before MurJ arrival but becomes faster and independent of FtsZ treadmilling after peptidoglycan synthesis activity is directed to the septum, where it provides additional force for cell envelope constriction.",

author = "Monteiro, {Jo{\~a}o M.} and Pereira, {Ana R.} and Reichmann, {Nathalie T.} and Saraiva, {Bruno M.} and Fernandes, {Pedro B.} and Helena Veiga and Tavares, {Andreia C.} and Margarida Santos and Ferreira, {Maria T.} and V{\^a}nia Mac{\'a}rio and VanNieuwenhze, {Michael S.} and Filipe, {S{\'e}rgio R.} and Pinho, {Mariana G.}",

note = "Funding Information: Acknowledgements We thank R. Sobral for the construction of pSG-murF plasmid; A. Jorge for the construction of the pSG-EzrA plasmid; T. Roemer for providing DMPI and strains AS-022 and AS-185; M. DeLisa for pTRC99a-P7; Richard Novick for pCN51; S. Foster for antibodies against DivIB and DivIC; A. Henriques for critical reading of the manuscript and L. Krippahl for help with image analysis tools. This study was funded by the European Research Council through grant ERC-2012-StG-310987 (to M.G.P.), by Project LISBOA-01-0145-FEDER-007660 Microbiologia Molecular, Estrutural e Celular (to ITQB-NOVA), by the National Institutes of Health through grant NIHGM113172 (to M.V.N.) and FCT fellowships SFRH/BD/71993/2010 (J.M.M.), SFRH/BD/86416/2012 (A.R.P.), SFRH/BPD/95031/2013 (N.T.R.), SFRH/BPD/87374/2012 (H.V.), SFRH/BD/52204/2013 (A.C.T.) and SFRH/BD/77849/2011 (M.T.F.). Publisher Copyright: {\textcopyright} 2018 Macmillan Publishers Limited, part of Springer Nature. All rights reserved.",

year = "2018",

month = feb,

day = "22",

doi = "10.1038/nature25506",

language = "English (US)",

volume = "554",

pages = "528--532",

journal = "Nature",

issn = "0028-0836",

publisher = "Nature Publishing Group",

number = "7693",

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TY - JOUR

T1 - Peptidoglycan synthesis drives an FtsZ-treadmilling-independent step of cytokinesis

AU - Monteiro, João M.

AU - Pereira, Ana R.

AU - Reichmann, Nathalie T.

AU - Saraiva, Bruno M.

AU - Fernandes, Pedro B.

AU - Veiga, Helena

AU - Tavares, Andreia C.

AU - Santos, Margarida

AU - Ferreira, Maria T.

AU - Macário, Vânia

AU - VanNieuwenhze, Michael S.

AU - Filipe, Sérgio R.

AU - Pinho, Mariana G.

N1 - Funding Information: Acknowledgements We thank R. Sobral for the construction of pSG-murF plasmid; A. Jorge for the construction of the pSG-EzrA plasmid; T. Roemer for providing DMPI and strains AS-022 and AS-185; M. DeLisa for pTRC99a-P7; Richard Novick for pCN51; S. Foster for antibodies against DivIB and DivIC; A. Henriques for critical reading of the manuscript and L. Krippahl for help with image analysis tools. This study was funded by the European Research Council through grant ERC-2012-StG-310987 (to M.G.P.), by Project LISBOA-01-0145-FEDER-007660 Microbiologia Molecular, Estrutural e Celular (to ITQB-NOVA), by the National Institutes of Health through grant NIHGM113172 (to M.V.N.) and FCT fellowships SFRH/BD/71993/2010 (J.M.M.), SFRH/BD/86416/2012 (A.R.P.), SFRH/BPD/95031/2013 (N.T.R.), SFRH/BPD/87374/2012 (H.V.), SFRH/BD/52204/2013 (A.C.T.) and SFRH/BD/77849/2011 (M.T.F.). Publisher Copyright: © 2018 Macmillan Publishers Limited, part of Springer Nature. All rights reserved.

PY - 2018/2/22

Y1 - 2018/2/22

N2 - Peptidoglycan is the main component of the bacterial wall and protects cells from the mechanical stress that results from high intracellular turgor. Peptidoglycan biosynthesis is very similar in all bacteria; bacterial shapes are therefore mainly determined by the spatial and temporal regulation of peptidoglycan synthesis rather than by the chemical composition of peptidoglycan. The form of rod-shaped bacteria, such as Bacillus subtilis or Escherichia coli, is generated by the action of two peptidoglycan synthesis machineries that act at the septum and at the lateral wall in processes coordinated by the cytoskeletal proteins FtsZ and MreB, respectively. The tubulin homologue FtsZ is the first protein recruited to the division site, where it assembles in filaments - forming the Z ring - that undergo treadmilling and recruit later divisome proteins. The rate of treadmilling in B. subtilis controls the rates of both peptidoglycan synthesis and cell division. The actin homologue MreB forms discrete patches that move circumferentially around the cell in tracks perpendicular to the long axis of the cell, and organize the insertion of new cell wall during elongation. Cocci such as Staphylococcus aureus possess only one type of peptidoglycan synthesis machinery, which is diverted from the cell periphery to the septum in preparation for division. The molecular cue that coordinates this transition has remained elusive. Here we investigate the localization of S. aureus peptidoglycan biosynthesis proteins and show that the recruitment of the putative lipid II flippase MurJ to the septum, by the DivIB-DivIC-FtsL complex, drives peptidoglycan incorporation to the midcell. MurJ recruitment corresponds to a turning point in cytokinesis, which is slow and dependent on FtsZ treadmilling before MurJ arrival but becomes faster and independent of FtsZ treadmilling after peptidoglycan synthesis activity is directed to the septum, where it provides additional force for cell envelope constriction.

AB - Peptidoglycan is the main component of the bacterial wall and protects cells from the mechanical stress that results from high intracellular turgor. Peptidoglycan biosynthesis is very similar in all bacteria; bacterial shapes are therefore mainly determined by the spatial and temporal regulation of peptidoglycan synthesis rather than by the chemical composition of peptidoglycan. The form of rod-shaped bacteria, such as Bacillus subtilis or Escherichia coli, is generated by the action of two peptidoglycan synthesis machineries that act at the septum and at the lateral wall in processes coordinated by the cytoskeletal proteins FtsZ and MreB, respectively. The tubulin homologue FtsZ is the first protein recruited to the division site, where it assembles in filaments - forming the Z ring - that undergo treadmilling and recruit later divisome proteins. The rate of treadmilling in B. subtilis controls the rates of both peptidoglycan synthesis and cell division. The actin homologue MreB forms discrete patches that move circumferentially around the cell in tracks perpendicular to the long axis of the cell, and organize the insertion of new cell wall during elongation. Cocci such as Staphylococcus aureus possess only one type of peptidoglycan synthesis machinery, which is diverted from the cell periphery to the septum in preparation for division. The molecular cue that coordinates this transition has remained elusive. Here we investigate the localization of S. aureus peptidoglycan biosynthesis proteins and show that the recruitment of the putative lipid II flippase MurJ to the septum, by the DivIB-DivIC-FtsL complex, drives peptidoglycan incorporation to the midcell. MurJ recruitment corresponds to a turning point in cytokinesis, which is slow and dependent on FtsZ treadmilling before MurJ arrival but becomes faster and independent of FtsZ treadmilling after peptidoglycan synthesis activity is directed to the septum, where it provides additional force for cell envelope constriction.

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JO - Nature

JF - Nature

IS - 7693

ER -

Peptidoglycan synthesis drives an FtsZ-treadmilling-independent step of cytokinesis

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