MurJ is the flippase of lipid-linked precursors for peptidoglycan biogenesis

Sham, Lok‐To; Butler, Emily K.; Lebar, Matthew D.; Kahne, Daniel; Bernhardt, Thomas G.; Ruiz, Natividad

doi:10.1126/science.1254522

Cited by 276 publications

(313 citation statements)

References 28 publications

(25 reference statements)

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“…Collectively, our data lead us to propose that Amj is the founding member of a new family of lipid II flippases. An additional conclusion that emerges from our study and previous work (6,8) is that the MOP family member SpoVB required for synthesis of spore cortex PG (27) is a lipid II flippase. It is unclear why B. subtilis possesses a sporulation-specific flippase, but one possibility is that the spatial and temporal requirements for PG synthesis during development cannot be met by the vegetative enzymes.…”

Section: Discussionmentioning

confidence: 56%

“…Tn-seq was performed as described previously (38,39). Lipid II flippase activity in E. coli was measured as described previously (6). Detailed protocols; tables of strains, plasmids, and oligonucleotide primers; and a description of strain and plasmid construction are provided in SI Experimental Procedures and Table S1.…”

Section: Methodsmentioning

confidence: 99%

“…The enzymes that transport lipid II across the membrane have been the subject of extensive research and speculation (3)(4)(5)(6). Recent work in Escherichia coli has provided strong evidence that the polytopic membrane protein MurJ is required for lipid II transport across the membrane, and is likely to be a lipid II flippase (6). MurJ is a member of the multidrug/oligosaccharidyl-lipid/polysaccharide (MOP) exporter superfamily (7).…”

mentioning

confidence: 99%

“…The molecule is then translocated to the outer face of the membrane, where the disaccharide-peptide monomer is incorporated into the existing PG by cell wall synthetic machineries composed of penicillin-binding proteins and additional factors (2). The enzymes that transport lipid II across the membrane have been the subject of extensive research and speculation (3)(4)(5)(6). Recent work in Escherichia coli has provided strong evidence that the polytopic membrane protein MurJ is required for lipid II transport across the membrane, and is likely to be a lipid II flippase (6).…”

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confidence: 99%

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MurJ and a novel lipid II flippase are required for cell wall biogenesis inBacillus subtilis

Meeske

Sham

Kimsey

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

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171

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Bacterial surface polysaccharides are synthesized from lipid-linked precursors at the inner surface of the cytoplasmic membrane before being translocated across the bilayer for envelope assembly. Transport of the cell wall precursor lipid II in Escherichia coli requires the broadly conserved and essential multidrug/oligosaccharidyl-lipid/polysaccharide (MOP) exporter superfamily member MurJ. Here, we show that Bacillus subtilis cells lacking all 10 MOP superfamily members are viable with only minor morphological defects, arguing for the existence of an alternate lipid II flippase. To identify this factor, we screened for synthetic lethal partners of MOP family members using transposon sequencing. We discovered that an uncharacterized gene amj (alternate to MurJ; ydaH) and B. subtilis MurJ (murJ Bs ; formerly ytgP) are a synthetic lethal pair. Cells defective for both Amj and MurJ Bs exhibit cell shape defects and lyse. Furthermore, expression of Amj or MurJ Bs in E. coli supports lipid II flipping and viability in the absence of E. coli MurJ. Amj is present in a subset of gram-negative and gram-positive bacteria and is the founding member of a novel family of flippases. Finally, we show that Amj is expressed under the control of the cell envelope stress-response transcription factor σ M and cells lacking MurJ Bs increase amj transcription. These findings raise the possibility that antagonists of the canonical MurJ flippase trigger expression of an alternate translocase that can resist inhibition.T he bacterial cell wall or peptidoglycan (PG) is composed of glycan strands cross-linked together by short peptides. This 3D meshwork protects the cell from osmotic lysis and determines shape, and its assembly is the target of some of our most successful antibiotics. Cell wall synthesis begins in the cytoplasm, where a set of highly conserved enzymes catalyze the formation of the lipid-linked precursor lipid II, which is composed of undecaprenyl-pyrophosphate (UndPP) linked to N-acetylglucosamine-N-acetylmuramic acid pentapeptide. Lipid II is synthesized on the inner face of the cytoplasmic membrane (1). The molecule is then translocated to the outer face of the membrane, where the disaccharide-peptide monomer is incorporated into the existing PG by cell wall synthetic machineries composed of penicillin-binding proteins and additional factors (2). The enzymes that transport lipid II across the membrane have been the subject of extensive research and speculation (3-6). Recent work in Escherichia coli has provided strong evidence that the polytopic membrane protein MurJ is required for lipid II transport across the membrane, and is likely to be a lipid II flippase (6). MurJ is a member of the multidrug/oligosaccharidyl-lipid/polysaccharide (MOP) exporter superfamily (7). It is broadly conserved among Eubacteria and essential for viability in many organisms. Intriguingly, work in the model gram-positive bacterium Bacillus subtilis indicates that cells lacking four MOP superfamily members similar to MurJ are viable and have...

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Section: Discussionmentioning

confidence: 56%

Section: Methodsmentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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MurJ and a novel lipid II flippase are required for cell wall biogenesis inBacillus subtilis

Meeske

Sham

Kimsey

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

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“…Next, the FemXAB transpeptidases catalyse the coupling of a pentaglycin-moiety to the D-lysine of the pentapeptide u it a d fu the o e, the a idatio of the -D-glutamate of the pentapeptide unit by the MurT/GatD two-enzyme complex leading to the corresponding D-isoglutamin (Münch et al 2012;Zapun et al 2013). This modified lipid II now contains the complete peptidoglycan monomer linked via a pyrophosphate to the bactoprenol membrane anchor, which is translocated through the phospholipid membrane by the MurJ flippase and presented on the extracellular membrane surface (Mohammadi et al 2011;Butler et al 2013a;Sham et al 2014;Meeske et al 2015). On the extracellular membrane surface the peptidoglycan precursor is released, incorporated into the growing peptidoglycan layer and crosslinked (Zapun et al 2013) with each other catalyzed by the PBPs (Sauvage et al 2008).…”

Section: Lessons Learned From Druggable Targets In Bacteriamentioning

confidence: 99%

New Structural Templates for Clinically Validated and Novel Targets in Antimicrobial Drug Research and Development

Klahn

Brönstrup

2016

Current Topics in Microbiology and Immunology

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Abstract:The development of bacterial resistance against current antibiotic drugs necessitates a continuous renewal of the arsenal of efficacious drugs. This imperative has not been met by the output of antibiotic research and development of the past decades for various reasons, including the declining efforts of large pharma companies in this area. Moreover, the majority of novel antibiotics are chemical derivatives of existing structures that represent mostly step innovations, implying that the available chemical space may be exhausted. This review negates this impression by showcasing recent achievements in lead finding and optimization of antibiotics that have novel or unexplored chemical structures. Not surprisingly, many of the novel structural templates like teixobactins, lysocin, griselimycin, or the albicidin/cystobactamid pair were discovered from natural sources. Additional compounds were obtained from the screening of synthetic libraries and chemical synthesis, including the gyrase-inhibiting NTBI s a d spiropyrimidinetrione, the tarocin and targocil inhibitors of wall teichoic acid synthesis, or the boronates and diazabicyclo[3.2

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Mechanisms of bacterial morphogenesis: Evolutionary cell biology approaches provide new insights

2015

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How Darwin’s “endless forms most beautiful” have evolved remains one of the most exciting questions in biology. The significant variety of bacterial shapes is most likely due to the specific advantages they confer with respect to the diverse environments they occupy. While our understanding of the mechanisms generating relatively simple shapes has improved tremendously in the last few years, the molecular mechanisms underlying the generation of complex shapes and the evolution of shape diversity are largely unknown. The emerging field of bacterial evolutionary cell biology provides a novel strategy to answer this question in a comparative phylogenetic framework. This relatively novel approach provides hypotheses and insights into cell biological mechanisms, such as morphogenesis, and their evolution that would have been difficult to obtain by studying only model organisms. We discuss the necessary steps, challenges, and impact of integrating “evolutionary thinking” into bacterial cell biology in the genomic era.

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MurJ is the flippase of lipid-linked precursors for peptidoglycan biogenesis

Cited by 276 publications

References 28 publications

MurJ and a novel lipid II flippase are required for cell wall biogenesis inBacillus subtilis

MurJ and a novel lipid II flippase are required for cell wall biogenesis inBacillus subtilis

New Structural Templates for Clinically Validated and Novel Targets in Antimicrobial Drug Research and Development

Mechanisms of bacterial morphogenesis: Evolutionary cell biology approaches provide new insights

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