Role of the Periplasmic Chaperones Skp, SurA, and DegQ in Outer Membrane Protein Biogenesis in Neisseria meningitidis

147

194

Section: Resultsmentioning

confidence: 83%

Section: Discussionmentioning

confidence: 99%

Distinct Roles of Secreted HtrA Proteases from Gram-negative Pathogens in Cleaving the Junctional Protein and Tumor Suppressor E-cadherin

Hoy

Geppert

Boehm

et al. 2012

147

194

“…NspA is a small eight-stranded ␤-barrel OMP whose correctly folded form migrates more slowly in seminative SDS-PAGE than the denatured form (18). Using this assay, we found that all NspA was folded in the ⌬GNA2091 mutant (Fig.…”

Section: Role Of Gna2091 In Omp Assemblymentioning

confidence: 93%

“…The transformants were checked by PCR for the presence of the mutant allele using primer pair NMB2090-for and NMB2092-rev and for the absence of the wild-type allele using primer pair GNA2091-for1 and NMB2092-rev. Double skp::cat⌬GNA2091, ⌬surA⌬GNA2091 and ⌬bamC⌬GNA2091 mutants were obtained by introducing the ⌬GNA2091::kan allele into previously constructed ⌬surA::cat, ⌬bamC::cat, and insertional skp::cat mutants (11,18). For complementation purposes, GNA2091 was amplified by PCR using genomic DNA of HB-1 as template and primers GNA2091-for-NdeI and GNA2091-rev-AatII.…”

Section: Methodsmentioning

confidence: 99%

Involvement of Neisseria meningitidis Lipoprotein GNA2091 in the Assembly of a Subset of Outer Membrane Proteins

Bos

Grijpstra

Boxtel

et al. 2014

Self Cite

Background: Outer membrane protein assembly is an incompletely understood process in Gram-negative bacteria. Results: A Neisseria meningitidis mutant lacking the lipoprotein GNA2091 is affected in growth and accumulates unassembled outer membrane proteins. Conclusion:We identified a novel component involved in outer membrane biogenesis. Significance: Our findings contribute to the understanding of a fundamental process occurring in Gram-negative bacteria.

“…When neisserial cell envelopes are subjected to this procedure, LptD is detected as two high molecular weight (HMW) bands, indicating that the protein is present in complexes (32) (Fig. 5A).…”

Section: Assessment Of Cell Surface Localization Of Lps-tomentioning

confidence: 99%

The LptD Chaperone LptE Is Not Directly Involved in Lipopolysaccharide Transport in Neisseria meningitidis

Bos

Tommassen

2011

Self Cite

The biosynthesis of lipopolysaccharide (LPS) in Gram-negative bacteria is well understood, in contrast to the transport to its destination, the outer leaflet of the outer membrane. In Escherichia coli, synthesis and transport of LPS are essential processes. Neisseria meningitidis, conversely, can survive without LPS and tolerates inactivation of genes involved in LPS synthesis and transport. Here, we analyzed whether the LptA, LptB, LptC, LptE, LptF, and LptG proteins, recently implicated in LPS transport in E. coli, function similarly in N. meningitidis. None of the analyzed proteins was essential in N. meningitidis, consistent with their expected roles in LPS transport and additionally demonstrating that they are not required for an essential process such as phospholipid transport. As expected, the absence of most of the Lpt proteins resulted in a severe defect in LPS transport. However, the absence of LptE did not disturb transport of LPS to the cell surface. LptE was found to be associated with LptD, and its absence affected total levels of LptD, suggesting a chaperone-like role for LptE in LptD biogenesis. The absence of a direct role of LptE in LPS transport was substantiated by bioinformatic analyses showing a low conservation of LptE in LPSproducing bacteria. Apparently, the role of LptE in N. meningitidis deviates from that in E. coli, suggesting that the Lpt system does not function in a completely conserved manner in all Gram-negative bacteria.Lipopolysaccharide (LPS) is a glycolipid, uniquely present at the cell surface of Gram-negative bacteria. It consists of a hydrophobic membrane anchor, called lipid A, which is embedded in the outer membrane (OM), 2 and an extracellular oligosaccharide core extended in some bacteria with a polysaccharide moiety, the O-antigen. The lipid A part can evoke strong, often toxic, innate immune responses; hence, it is also known as endotoxin. LPS is an essential component of the OM of most Gram-negative bacteria. Therefore, molecules involved in its biogenesis may represent attractive antimicrobial targets, as demonstrated by the successful development of antibiotics targeting LpxC, an enzyme involved LPS biogenesis (1), and LptD, an OM protein involved in LPS transport (2). However, much of the LPS biogenesis is not understood yet. The complete lipid A biosynthetic pathway, which takes place in the cytoplasm and at the inner leaflet of the inner membrane, has been elucidated in Escherichia coli and Salmonella. The ubiquitous presence of the lipid A biosynthetic enzymes in most other Gram-negative organisms suggests that this process is well conserved (3). The transport process of LPS from its site of synthesis to the cell surface is much less well understood (4 -7).The ATP-binding cassette transporter MsbA is thought to transport the lipid A-core moiety of newly synthesized LPS over the inner membrane (8, 9). At the OM, two proteins have been shown to be involved in the transport of LPS to the cell surface: the integral OM protein designated LptD (formerly Imp/OstA) (...