Loss of YhcB results in dysregulation of coordinated peptidoglycan, LPS and phospholipid synthesis during Escherichia coli cell growth

Goodall, Emily C. A.; Isom, Georgia L.; Rooke, Jessica L.; Pullela, Karthik; Icke, Christopher; Yang, Zihao; Boelter, Gabriela; Jones, Alun; Warner, Isabel; Costa, Rochelle Da; Zhang, Bing; Rae, James; Tan, Wee Boon; Winkle, Matthias; Delhaye, Antoine; Heinz, Eva; Collet, Jean-François; Cunningham, Adam F.; Blaskovich, Mark A. T.; Parton, Robert G.; Cole, Jeff; Banzhaf, Manuel; Chng, Shu‐Sin; Vollmer, Waldemar; Bryant, Jack A.; Henderson, Ian R.

doi:10.1371/journal.pgen.1009586

Cited by 20 publications

(12 citation statements)

References 142 publications

(186 reference statements)

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“…However, the molecular basis of such a lethality remained unknown. Although LapD has recently been implicated in cell division or the maintenance of cell envelope homeostasis, its function has remained unknown [ 36 , 37 ].…”

Section: Resultsmentioning

confidence: 99%

“…Our studies do not rule out a direct link between LapD and cell division machinery; however, our suppressor approach clearly shows suppressors that either increase LpxC amounts (mutations in lpxC , ftsH and lapB ) or enhance LPS translocation ( msbA suppressor mutations) support direct participation of LapD in LPS assembly. Another study using whole genome transposon mutagenesis approaches also proposes that LapD (YhcB) functions at the junction of several envelope biosynthetic pathways including peptidoglycan biogenesis [ 36 ]. Some phenotypes, such as defects in biofilm formation of Δ lapD mutant bacteria [ 72 ], can be explained as an indirect consequence of the alteration in LPS amounts.…”

Section: Discussionmentioning

confidence: 99%

“…We have previously shown that the lapD gene is required for the growth of E. coli at critical high temperatures [ 34 ]. LapD (YhcB) is an inner membrane protein and has recently been implicated in either the cell division process or the cell envelope homeostasis; although, molecular mechanisms in either of these functions remain unknown [ 35 , 36 , 37 , 38 ]. In this work, we show that in the absence of LapD, LpxL and LpxM acyl transferases become essential and the synthetic lethality of either Δ( lpxL lapD ) or Δ( lpxM lapD ) can be overcome by extragenic suppressor mutations mapping to the essential msbA gene ( Figure 2 B).…”

Section: Introductionmentioning

confidence: 99%

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A New Factor LapD Is Required for the Regulation of LpxC Amounts and Lipopolysaccharide Trafficking

Wieczorek

Sendobra

Maniyeri

et al. 2022

IJMS

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Lipopolysaccharide (LPS) constitutes the major component of the outer membrane and is essential for bacteria, such as Escherichia coli. Recent work has revealed the essential roles of LapB and LapC proteins in regulating LPS amounts; although, if any additional partners are involved is unknown. Examination of proteins co-purifying with LapB identified LapD as a new partner. The purification of LapD reveals that it forms a complex with several proteins involved in LPS and phospholipid biosynthesis, including FtsH-LapA/B and Fab enzymes. Loss of LapD causes a reduction in LpxC amounts and vancomycin sensitivity, which can be restored by mutations that stabilize LpxC (mutations in lapB, ftsH and lpxC genes), revealing that LapD acts upstream of LapB-FtsH in regulating LpxC amounts. Interestingly, LapD absence results in the substantial retention of LPS in the inner membranes and synthetic lethality when either the lauroyl or the myristoyl acyl transferase is absent, which can be overcome by single-amino acid suppressor mutations in LPS flippase MsbA, suggesting LPS translocation defects in ΔlapD bacteria. Several genes whose products are involved in cell envelope homeostasis, including clsA, waaC, tig and micA, become essential in LapD’s absence. Furthermore, the overproduction of acyl carrier protein AcpP or transcriptional factors DksA, SrrA can overcome certain defects of the LapD-lacking strain.

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Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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A New Factor LapD Is Required for the Regulation of LpxC Amounts and Lipopolysaccharide Trafficking

Wieczorek

Sendobra

Maniyeri

et al. 2022

IJMS

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“…A limitation of this method is that it only informs whether a mutant is present within the total pool of mutants, the nature of the method cannot distinguish whether the mutant of a given well is correct; further validation checks are required to test this. One caveat to consider is that the presence of a correctly positioned kanamycin resistance cassette is not sufficient evidence for the correct construction of a mutant, as is seen with yciM, yhcB, hda and holD mutants (Mahalakshmi et al 2014; Goodall et al 2021). In each of these examples, the kanamycin cassette is in the correct location, but secondary mutations have been reported elsewhere in the genome.…”

Section: Discussionmentioning

confidence: 99%

“…One caveat to consider is that the presence of a correctly positioned kanamycin resistance cassette is not sufficient evidence for the correct construction of a mutant, as is seen with yciM, yhcB, hda and holD mutants Goodall et al 2021). In each of these examples, the kanamycin cassette is in the correct location, but secondary mutations have been reported elsewhere in the genome.…”

Section: Discussionmentioning

confidence: 99%

TraDIS-validate: a method for curating ordered gene-replacement libraries

Goodall

Morris

McKeand

et al. 2022

Preprint

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In recent years the availability of genome sequence information has grown logarithmically resulting in the identification of a plethora of uncharacterised genes. To address this gap in functional annotation, many high-throughput screens have been devised with the goal of uncovering novel gene functions. Gene-replacement libraries are one such tool that can be screened in a high-throughput way to link genotype and phenotype and are key community resources. However, for a phenotype to be attributed to a specific gene, there needs to be confidence in the genotype. Construction of large libraries can be laborious and occasionally errors will arise. Here, we present a rapid and accurate method for the validation of any ordered gene-replacement library. We applied our method (TraDIS-Validate) to the well-known Keio library of Escherichia coli gene-deletion mutants. Our method identified 3,718 constructed mutants out of a total of 3,728 confirmed isolates. TraDIS-validate therefore had a success rate of 99.7% for identifying the correct kanamycin cassette position. This dataset provides a benchmark for the purity of the Keio mutants and a screening method for mapping the position of an antibiotic resistance cassette in any ordered library.

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Common and varied molecular responses of Escherichia coli to five different inhibitors of the lipopolysaccharide biosynthetic enzyme LpxC

Möller,

Vázquez-Hernández,

Kutscher

et al. 2024

Journal of Biological Chemistry

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Loss of YhcB results in dysregulation of coordinated peptidoglycan, LPS and phospholipid synthesis during Escherichia coli cell growth

Cited by 20 publications

References 142 publications

A New Factor LapD Is Required for the Regulation of LpxC Amounts and Lipopolysaccharide Trafficking

A New Factor LapD Is Required for the Regulation of LpxC Amounts and Lipopolysaccharide Trafficking

TraDIS-validate: a method for curating ordered gene-replacement libraries

Common and varied molecular responses of Escherichia coli to five different inhibitors of the lipopolysaccharide biosynthetic enzyme LpxC

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