ARTICLE
Received 23 Jul 2015 | Accepted 15 Dec 2015 | Published 25 Jan 2016
DOI: 10.1038/ncomms10515 OPEN
A novel mechanism for the biogenesis of outer membrane vesicles in Gram-negative bacteria
Sandro Roier1, Franz G. Zingl1, Fatih Cakar1, Sanel Durakovic1, Paul Kohl1, Thomas O. Eichmann1, Lisa Klug2, Bernhard Gadermaier1, Katharina Weinzerl1, Ruth Prassl3, Achim Lass1, Gnther Daum2, Joachim Reidl1, Mario F. Feldman4 & Stefan Schild1
Bacterial outer membrane vesicles (OMVs) have important biological roles in pathogenesis and intercellular interactions, but a general mechanism of OMV formation is lacking. Here we show that the VacJ/Yrb ABC (ATP-binding cassette) transport system, a proposed phospholipid transporter, is involved in OMV formation. Deletion or repression of VacJ/Yrb increases OMV production in two distantly related Gram-negative bacteria, Haemophilus inuenzae and Vibrio cholerae. Lipidome analyses demonstrate that OMVs from VacJ/Yrb-defective mutants inH. inuenzae are enriched in phospholipids and certain fatty acids. Furthermore, we demonstrate that OMV production and regulation of the VacJ/Yrb ABC transport system respond to iron starvation. Our results suggest a new general mechanism of OMV biogenesis based on phospholipid accumulation in the outer leaet of the outer membrane. This mechanism is highly conserved among Gram-negative bacteria, provides a means for regulation, can account for OMV formation under all growth conditions, and might have important pathophysiological roles in vivo.
1 Institute of Molecular Biosciences, University of Graz, NAWI Graz, BioTechMed-Graz, Humboldtstra 50, A-8010 Graz, Austria. 2 Institute of Biochemistry, Graz University of Technology, NAWI Graz, BioTechMed-Graz, Petersgasse 12/2, A-8010 Graz, Austria. 3 Institute of Biophysics, Medical Universityof Graz, BioTechMed-Graz, Harrachgasse 21, A-8010 Graz, Austria. 4 Department of Biological Sciences, University of Alberta, CW405 Biological Sciences Building, Edmonton, Alberta, Canada T6G 2E9. Correspondence and requests for materials should be addressed to S.S. (email: mailto:[email protected]
Web End [email protected] ).
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ARTICLE NATURE COMMUNICATIONS | DOI: 10.1038/ncomms10515
Outer membrane vesicles (OMVs) are spherical, bilayered, membranous structures that are released naturally from the outer membrane (OM) of Gram-negative bacteria1.
These small particles (B10300 nm in diameter) are primarily composed of phospholipids (PLs), OM proteins (OMPs), and lipopolysaccharides or lipooligosaccharides, but also contain periplasmic proteins and cell wall components, which get trapped in the vesicle lumen during the release process. However, OMVs may also comprise proteins of the inner membrane, cytoplasmic proteins, DNA, RNA, ions, metabolites and signalling molecules24. The secretion of OMVs seems to be an evolutionary conserved process, as OMV production has been observed under various growth conditions and in different natural environments in all pathogenic and non-pathogenic Gram-negative bacteria investigated so far. Since OMV production requires a signicant energy cost, the benets in certain environmental conditions must have been sufcient to allow OMV secretion to evolve1,2,5,6. Based on their metabolic cost, ubiquity and interesting cargo material, it is likely that OMVs have vital biological functions and, as a consequence of intense research, it was soon found that OMVs play important roles in bacterial physiology and pathogenesis. They are proposed to be involved in horizontal gene transfer, biolm formation, intra- and interspecies communication, stress response, delivery of toxins and other biomolecules, killing of competing microbial cells, resistance to antibiotics, adherence to host cells, complement absorption and immunomodulation13,5,7. In addition, many studies focused on vesicle-based vaccines and demonstrated that OMVs are promising vaccine candidates against bacterial infections caused by, for example, Haemophilus inuenzae, Pasteurella multocida, Vibrio cholerae, enterotoxigenic Escherichia coli, Neisseria meningitidis, Bordetella pertussis and Salmonella typhimurium813.
Despite these important biological roles and applications of OMVs, research has only just begun to understand the mechanism of OMV biogenesis. Currently, three major models are discussed within the scientic community. The rst model is based on either loss or relocation of covalent linkages (for example, via lipoproteins) between the OM and the underlying peptidoglycan layer. These missing cross-links in combination with an OM that grows faster than the underlying cell wall allow the OM to protrude and thus initiate vesiculation2,3,7,1416. A second model proposes that an accumulation of peptidoglycan fragments or misfolded proteins in the periplasmic space exerts a turgor pressure on the OM causing the OM to bulge and nally to pinch off. Such accumulations can be triggered by, for example, defects in cell wall remodelling or temperature stress2,3,7,17,18. The third model is based on the enrichment of membrane curvature-inducing molecules, such as the B-band lipopolysaccharide and the quinolone PQS of Pseudomonas aeruginosa. It is hypothesized that PQS enhances anionic repulsions between lipopolysaccharide molecules resulting in membrane blebbing by sequestering divalent cations, which are important in forming stabilizing salt bridges between the negatively charged B-band lipopolysaccharide molecules. Recently, it was proposed that PQS induces OMV formation through a mechanism of asymmetric expansion of the outer leaet of the OM2,3,7,1922. Although the PQS-based model is one of the best studied so far, it is limited by the fact that PQS is only produced by P. aeruginosa and therefore species specic. In summary, all these proposed models of OMV formation require either genetic manipulations, the presence of stress, or are thus far only applicable to a single bacterial species. It is currently unknown whether Gram-negative bacteria share a conserved general mechanism of OMV biogenesis that is amenable to regulation.
Here we show that disruptions within the VacJ/Yrb ABC (ATP-binding cassette) transport system increase OMV production in the human pathogens H. inuenzae and V. cholerae without compromising OM integrity. Concordantly, mutations in homo-logues of E. coli also exhibit increased vesiculation, as independently demonstrated by other groups (ref. 23 and Thomas J. Silhavy, Princeton University, personal communication). Since this system is proposed to function as a PL transporter in maintaining the lipid asymmetry in the OM24, we performed lipidome analyses to demonstrate that OMVs from PL transporter mutants in H. inuenzae are enriched in PLs, which are likely to be incorporated into the outer leaet of the vesicle membrane. Furthermore, we report that iron limitation leads to a ferric uptake regulator (Fur)-dependent downregulation of the VacJ/Yrb ABC transport system correlating with an increased OMV production in H. inuenzae, V. cholerae and E. coli. Our results indicate that the disadvantage of an increased serum sensitivity caused by this downregulation can be overcome in vivo by an increased OMV production suggesting an important pathophysiological role of this system. We propose a novel and potentially highly conserved bacterial OMV biogenesis mechanism, which provides the opportunity of regulation and may represent a rst general mechanism applicable to all Gram-negative bacteria.
ResultsIdentication of mutants with altered OMV production. In an attempt to discover a general mechanism of OMV formation, we used H. inuenzae, an opportunistic pathogen of the human respiratory tract25, as a model organism. We conducted a transposon mutagenesis and a dot blot screen to identify 20 gene disruptions that led to altered OMV production based on immunological detection of several OMV associated proteins (Supplementary Table 1). For this analysis OMPs P1, P2, P4, P5 and P6 were chosen, since these represent highly abundant OMPs of H. inuenzae and have recently shown to be present in OMVs in detectable levels26. Representative examples for dot blots as well as examples for the evaluation of relative signal intensities are provided in Supplementary Fig. 1. In most cases the observed trends generally correlated with an increase or decrease of the surveyed OMPs P1, P2, P4, P5 or P6 in OMVs indicating no differential protein sorting. Notably, the majority of transposon insertion mutants showed markedly and consistently increased relative OMV and OMP dot blot signals suggesting an overall increase in vesiculation, while only four mutants exhibited decreased dot blot signals indicating hypovesiculation. A similar trend has also been reported for E. coli in a previous screen for alterations in OMV production16. The most pronounced phenotypes for hypovesiculation were observed for insertion mutants in HI_0572 and HI_0854 encoding for a peroxiredoxin hybrid Prx5 and a haem iron utilization protein, respectively. Strong hypervesiculation phenotypes were observed for insertion mutants in HI_0037 (rod shape-determining protein MreB), HI_0528 (tyrosine-specic transport protein TyrP), HI_1083 (NTP-binding protein YrbB), HI_1086 (ABC transporter permease YrbE), HI_1164 (OMP P5), HI_1181 (phosphoheptose isomerase GmhA) and HI_1213 (thiol-disulde interchange protein DsbC). An increased vesiculation due to deletion or truncation of OmpA, representing the OMP P5 homologue and an abundant protein linking the OM and peptidoglycan layer, has already been reported in E. coli, Salmonella, and V. cholerae15,27,28. Other mutants, including those in mreB, dsbC and gmhA can be linked to OM stability or stress response, which have been previously implicated in OMV secretion2,7,15,18. In this study we focused on adjacent mutations in HI_1083 (yrbB) and HI_1086 (yrbE),
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NATURE COMMUNICATIONS | DOI: 10.1038/ncomms10515 ARTICLE
a b
Bacterium
H. influenzaeP. multocidaE. coliV. choleraeP. aeruginosaS. typhimuriumY. enterocoliticaN. meningitidisC. crescentusD. vulgarisH. pylori
VacJ
100%
HI_0718
57%
PM_1501
42%
b_2346
42%
VC_2048
33%
PA_2800
42%
STM_2392
40%
YE_1272
34%
NMB_1961
30%
CC_3692
29%
DVU_1242
NA
YrbB
100%
HI_1083
57%
PM_0178
32%
b_3191
29%
VC_2516
23%
PA_4452
28%
STM_3309
39%
YE_3748
25%
NMB_1962
NA
20%
DVU_1241
NA
YrbC
100%
HI_1084
47%
PM_0177
42%
b_3192
37%
VC_2517
26%
PA_4453
41%
STM_3310
43%
YE_3749
19%
NMB_1963
27%
CC_3693
22%
DVU_1243
a.c.
HP_1463
YrbD
100%
HI_1085
73%
PM_0176
60%
b_3193
55%
VC_2518
50%
PA_4454
61%
STM_3311
58%
YE_3750
48%
NMB_1964
31%
CC_3694
37%
DVU_1244
21%
HP_1464
YrbE
100%
HI_1086
86%
PM_0175
73%
b_3194
74%
VC_2519
65%
PA_4455
74%
STM_3312
71%
YE_3751
54%
NMB_1965
34%
CC_3695
41%
DVU_1246
31%
HP_1466
YrbF
100%
HI_1087
86%
PM_0174
67%
b_3195
68%
VC_2520
60%
PA_4456
67%
STM_3313
69%
YE_3752
53%
NMB_1966
36%
CC_3696
38%
DVU_1245
34%
HP_1465
OM
IM
Lipooligosaccharide
Lipoprotein
Substrate binding protein
Phospholipid
Periplasmic binding protein
Permease
NTP binding protein
YrbC
Periplasm
Cytoplasm
VacJ
YrbD
YrbE YrbE
ATP
ADP + Pi
YrbB
YrbB
YrbF YrbF
ATPase
Figure 1 | A conserved ABC transport system putatively prevents PL accumulation in the outer leaet of the OM. (a) The VacJ and Yrb proteinsof H. inuenzae are homologous to members of the E. coli Mla pathway, which has been proposed to maintain the lipid asymmetry in the Gram-negative OM by retrograde trafcking of PLs from the OM to the inner membrane (IM)24. The model is derived from the Mla pathway model proposed by Malinverni and Silhavy24. (b) Conservation of H. inuenzae VacJ and Yrb proteins among Gram-negative bacteria. The respective genes or gene clusters were identied via the SSEARCH programme in combination with the SSDB (Similarity Sequence DataBase) using the KEGG database resource. Shown are the corresponding gene numbers and the respective amino acid sequence identities (in percentage), which were determined by BLASTp and/or Clustal Omega. Adjacent genes located in gene clusters are highlighted in yellow, genes located outside of the yrb gene clusters are coloured orange. In case of a single dash and NA (not applicable) no conserved homologous protein was identied. In Helicobacter pylori an auxiliary component (a.c.) with no homology to any other component is encoded within the yrb gene cluster. Genomes analysed were: H. inuenzae Rd KW20 (g), P. multocida Pm70 (g), E. coli K-12
MG1655 (g), V. cholerae O1 El Tor N16961 (g), P. aeruginosa PAO1 (g), Salmonella enterica serovar Typhimurium LT2 (g), Yersinia enterocolitica 8081 (g),N. meningitidis MC58 (b), Caulobacter crescentus CB15 (a), Desulfovibrio vulgaris Hildenborough (d) and H. pylori 26695 (e). The symbols a, b, g, d and e refer to the class of the respective bacterium within the phylum Proteobacteria.
which showed strong OMV and OMP dot blot signals suggesting an overall increase in vesiculation. These were the most promising candidates for further evaluation, as they have not been previously implicated in OMV formation and both genes are located within a gene cluster comprising three additional genes (yrbC, yrbD and yrbF). In E. coli, homologues of these ve gene products, together with the VacJ protein, have been implicated in maintaining the lipid asymmetry in the Gram-negative OM24. This ABC transport system was termed the Mla pathway and is thought to prevent PL accumulation in the outer leaet of the OM by retrograde trafcking of PLs from the OM to the inner membrane24. Recent studies reported that this PL transport system also contributes to serum resistance among pulmonary isolates of nontypeable H. inuenzae (NTHi)29 and is required for intercellular spread of Shigella exneri30. Figure 1a illustrates the putative VacJ/Yrb ABC transport system in H. inuenzae based on the E. coli Mla pathway model24. Notably, the VacJ and Yrb proteins of H. inuenzae as well as the overall genomic organization of their corresponding genes are conserved among Gram-negative bacteria (Fig. 1b). In representatives of b-, g- and d-Proteobacteria all components are highly conserved, while a- and e-Proteobacteria are lacking the smallest component annotated as NTP-binding protein YrbB. In addition, e-Proteobacteria have an auxiliary periplasmic substrate-binding component instead of the periplasmic binding protein YrbC and the OM lipoprotein VacJ. The integral components of the transport system including the substrate-binding protein YrbD, the inner membrane permease YrbE and the ATPase YrbF are highly conserved in all representatives. Indeed, the conservation of core components of the VacJ/Yrb ABC transport system in Gram-negative bacteria and in the chloroplasts of plants has also been previously reported by others24,31.
VacJ/Yrb ABC transport system mutants produce more OMVs. To conrm that disruptions within the VacJ/Yrb ABC transport system increase OMV production in H. inuenzae, we constructed gene-specic vacJ and yrbE deletion mutants and quantied the protein and lipooligosaccharide content of their derived OMVs using established methodologies16,26 (Fig. 2a). Compared with the wild-type, deletions of the OM lipoprotein VacJ or the inner membrane permease YrbE revealed signicant increases in OMV production with, on average, 1.6-fold and 2.2-fold higher vesiculation levels, respectively. The hypervesiculation phenotypes of nonpolar deletion mutants were complementable. To ensure that the higher amounts of protein and lipooligosaccharide as well as the elevated dot blot signals detected in OMV preparations were really due to increased vesiculation levels and not due to increased vesicle sizes, we performed a nanoparticle tracking analysis (Fig. 2b) and conrmed these results by transmission electron microscopy (Fig. 2c). We found no differences in the OMV size distribution between the strains conrming that the deletion of vacJ or yrbE indeed increases the amount of OMVs produced by H. inuenzae. Sensitivity of the mutant strains to cell lysis, SDS and polymyxin B treatment was comparable to the wild-type indicating that the OM integrity remains largely intact (Supplementary Fig. 2). Similar observations were also reported for related genes24,29, strengthening the conclusion that the hypervesiculation phenotypes are not caused by a compromised OM integrity. To determine whether these ndings also hold true in a distantly related Gram-negative species, we constructed vacJ and yrbE deletion mutants inV. cholerae and determined their vesiculation levels and OMV size distributions (Fig. 3a,b). Hypervesiculation phenotypes similar to those of H. inuenzae were observed. PL transporter mutants in V. cholerae revealed, on average, 3.9-fold (DvacJ) and
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ARTICLE NATURE COMMUNICATIONS | DOI: 10.1038/ncomms10515
a
*
*
* *
Bradford Purpald Dot blot
*
*
*
*
* 10
8 6 4 2 0
5
2
1
0
*
*
1
4 3
1
1
mg l1 OD 490 unit
mg l1 OD 490 unit
a.u. OD 490unit
2 1 0
Rd KW20
Rd vacJ
Rd yrbE
Rd vacJ::vacJ
Rd yrbE::yrbE
Rd KW20
Rd vacJ
Rd yrbE
Rd vacJ::vacJ
Rd yrbE::yrbE
Rd KW20
Rd vacJ
Rd yrbE
Rd vacJ::vacJ
Rd yrbE::yrbE
b
120
100
OMV diameter (nm)
80
60
40
20
0 Rd KW20 Rd vacJ Rd yrbE Rd vacJ::vacJ Rd yrbE::yrbE
Mean
Mode
c
Rd KW20 Rd yrbE
Rd vacJ
Figure 2 | H. inuenzae PL transporter mutants produce excessive OMVs. (a) OMV preparations derived from equivalent OD490 units of cultured wild-type (Rd KW20), deletion mutants (Rd DvacJ and Rd DyrbE) and complementation strains (Rd DvacJ::vacJ and Rd DyrbE::yrbE) were analysed for total protein (Bradford), lipooligosaccharide (Purpald) or OMV specic proteins (Dot blot). Mean values with standard error of the mean (s.e.m.) are shown (n 6 biological replicates). Signicant differences between the data sets are marked by asterisks (Po0.05; one-way ANOVA followed by Sidaks multiple
comparison post test). (b) Distributions of OMV sizes produced by the strains were determined by nanoparticle tracking analysis. Mean values with standard deviation (s.d.) of mean and mode OMV diameter sizes within each OMV preparation are shown (n 6 biological replicates). (c) Visualization of
density gradient puried OMVs by transmission electron microscopy. Shown are representative micrographs. Scale bars, 100 nm.
4.3-fold (DyrbE) higher vesiculation levels but similar OMV sizes compared with the wild-type. Similar to the complementation analysis in H. inuenzae, the hypervesiculation phenotypes of the DvacJ and DyrbE mutants in V. cholerae were restored to wild-type levels by expression of the respective gene in trans (Fig. 3c,d). Concordantly, mutations in the E. coli Mla pathway exhibit increased vesiculation, as independently demonstrated by another group (Thomas J. Silhavy, Princeton University, personal communication). This observation is reinforced by a recent genome wide assessment of OMV production in E. coli indicating an increased vesiculation of mlaA (vacJ) as well as mlaE (yrbE) mutants, which was not further investigated23. Furthermore, we used the arabinose-inducible vector system pBAD to overexpress the mla gene cluster (comprising mlaF to B) in the E. coli wild-type. Consistent, with the increase in vesiculation upon deletion of the Mla pathway, the over-expression resulted in decreased vesiculation compared with the empty vector control (Supplementary Fig. 3). Taken together, these ndings indicate a conserved role of the VacJ/Yrb ABC transport system in OMV formation of distantly related Gram-negative bacteria.
OMVs from PL transporter mutants have an altered lipidome. To evaluate the OMV and OM compositions of the H. inuenzae wild-type and PL transporter mutants DvacJ and DyrbE, we performed proteome and lipidome analyses. Comparison of protein proles generated by SDSPAGE (Supplementary Fig. 4) and proteome analysis by mass spectrometry (Supplementary Table 2) revealed very similar OMV or OM protein compositions for each strain, in good agreement with the dot blot results (Supplementary Table 1). Although the PL transporter mutants showed a slight alteration in the high molecular weight OMV protein band pattern in the SDSPAGE, we did not follow this observation, since it was not restored by complementation (Supplementary Fig. 4). Additionally, the protein mass spectrometry results (Supplementary Table 2) of the OMVs revealed no relevant hits in the PL transporter mutant OMVs compared with the wild-type OMVs, which could explain this alteration in protein band patterns. Therefore, we conclude that the PL transporter mutants closely resemble the wild-type regarding OMV or OM protein compositions, respectively.
Analysis of the PL composition conrmed the results of our recent study26, which demonstrated that phosphatidylethanolamine (PE) is by far the most dominant PL species identied in OMVs
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a b
Bradford
Bradford
Purpald
Purpald
Mean
Mean
Mode
Mode
4.5
1.5 150 125 100
75 50 25
0
* *
* *
*
*
OMV diameter (nm) OMV diameter (nm)
1
mg l1 OD 600 unit
1
mg l1 OD 600 unit
mg l1 OD 600 unit
mg l1 OD 600 unit
3.0
1.5
1.0
0.5
0.0
0.0
12 1.0 125 100
75 50 25
1 0.80.60.40.20.0
Vc AC53
Vc AC53 p
Vc vacJ
Vc yrbE
Vc fur
Vc AC53
Vc vacJ
Vc yrbE
Vc fur
Vc AC53
Vc vacJ
Vc yrbE
Vc fur
c d
*
*
**
**
*
*
10 8 6 4 2 0
1
Vc vacJ p
Vc vacJ pvacJ
Vc yrbE p
Vc yrbE pyrbE
Vc AC53 p
Vc vacJ p
Vc vacJ pvacJ
Vc yrbE p
Vc yrbE pyrbE
Vc AC53 p
0 Vc vacJ p
Vc vacJ pvacJ
Vc yrbE p
Vc yrbE pyrbE
e
vacJ expression yrbE expression
*
*
Relative gene expression
1.5
1.0
0.5
0.0
Relative gene expression
1.5
1.0
0.5
0.0
Vc AC53 Vc fur Vc AC53 Vc fur
Figure 3 | Excessive OMV production by PL transporter mutants, and regulation of vacJ and yrbE expression in V. cholerae. (a,c) OMV preparations derived from equivalent OD600 units of cultured wild-type (Vc AC53) and deletion mutants (Vc DvacJ, Vc DyrbE and Vc Dfur) as well as wild-type containing vector control (Vc Ac53 p) and deletion mutants containing either vector control (Vc DvacJ p, Vc DyrbE p) or expression plasmids (Vc DvacJ pvacJ and Vc DyrbE pyrbE) were analysed for total protein (Bradford) and lipopolysaccharide (Purpald). Mean values with s.e.m. are shown (n 12
biological replicates for Vc AC53 and n 6 biological replicates for all other strains). (b,d) Distributions of OMV sizes produced by the strains were
determined by nanoparticle tracking analysis. Mean values with s.d. of mean and mode OMV diameter sizes within respective OMV preparations are shown (n 12 biological replicates for Vc AC53 and n 6 biological replicates for all other strains). (e) Relative expressions of vacJ and yrbE in Vc AC53 and Vc
Dfur were determined by qRT-PCR. Horizontal bars highlight the mean of each data set (n 6 biological replicates). Dotted lines indicate a relative gene
expression of 1. (a,c,e) Signicant differences between the data sets are marked by asterisks (Po0.05; one-way ANOVA followed by Sidaks multiple comparison post test (a,c) or unpaired t test (e)).
and the OM of H. inuenzae (Fig. 4a). Only minor alterations in phosphatidylcholine and phosphatidylserine levels in OM preparations of the strains were observed, which did not correlate with increased or decreased vesiculation and were therefore not further investigated. Other differences in OMV or OM PL compositions between the strains were negligible. In contrast, analysis of fatty acid (FA) composition revealed that the OMVs of PL transporter mutants show signicant 10 percentage point decreases in C16:0 FA levels compared with the wild-type, which generally goes along with signicant 8 to 15 percentage point increases of C14:0 FA levels (Fig. 4b). By using a complementary mass spectrometry-based lipidome analysis and by analysing
identical amounts (protein equivalents) of respective preparations, we were able to compare quantitatively the total PE contents of all OMV and OM preparations (Fig. 4c). Total OM PE contents were not altered among the strains, whereas the total PE contents of OMVs derived from the PL transporter mutants were signicantly twofold increased compared with wild-type OMVs. Similar trends of slightly increased PL levels were already visible in the wild-type OMVs compared with the wild-type OM, but became more pronounced in the mutant strains (Fig. 4c). In consideration of the similar OMV size distributions, these results indicate that OMVs from PL transporter mutants are enriched in PLs, which are likely to be incorporated into the outer leaet of the vesicle membrane.
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ARTICLE NATURE COMMUNICATIONS | DOI: 10.1038/ncomms10515
a b
*
*
100
80
Rd KW20: OMV
Rd vacJ: OMV
Rd vacJ: OM
Rd yrbE: OMV
Rd yrbE: OM
Rd KW20: OM
50 40 30
% of total phospholipids
Total PE content [fold change]
60 40 20
*
*
% of total fatty acids
20 10
*
*
*
0 PE PC PS
0 C14:0
C14:1 C16:0 C16:1 C18:0 C18:1 C18:2
Rd KW20: OMV
Rd vacJ: OMV
Rd vacJ: OM
Rd yrbE: OMV
Rd yrbE: OM
Rd KW20: OM
C26:0
c
d
**
3.02.52.01.51.00.50.0
*
*
Rd KW20: OMV
Rd vacJ: OMV
**
Rd yrbE: OMV
Rd yrbE: OM
Rd KW20: OM
% of total PE species
20
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Rd KW20: OMV
Rd vacJ: OMV
Rd vacJ: OM
Rd yrbE: OMV
Rd yrbE: OM
Rd KW20: OM
Rd vacJ: OM
*
*
*
*
10 * *
*
*
OMV
OM
FAs
0 C24:0 C14:0
C10:0
C26:0 C14:0
C12:0
C26:1 C14:0
C12:1
C28:0 C14:0
C14:0
C28:1 C14:1
C14:0
C30:0 C16:0
C14:0
C30:1 C16:1
C14:0
C32:0 C16:0
C16:0
C32:1 C16:1
C16:0
C32:2 C16:1
C16:1
C34:1 C18:0
C16:1
C34:2 C18:1
C16:1
Figure 4 | Lipidome analyses of H. inuenzae density gradient puried OMVs and OM. (a,b) PL (a) and FA (b) compositions of OMV and OM preparations derived from Rd KW20, Rd DvacJ, and Rd DyrbE were analysed by thin-layer chromatography and by gas liquid chromatography in combination with ame-ionization detection, respectively. Mean percentage values with s.e.m. of total PLs (a) and FAs (b) within a given preparation are shown (n 3 biological replicates). Detected PLs and FAs were: phosphatidylethanolamine (PE), phosphatidylcholine (PC), phosphatidylserine (PS),
myristic acid (C14:0), myristoleic acid (C14:1), palmitic acid (C16:0), palmitoleic acid (C16:1), stearic acid (C18:0), oleic acid (C18:1), linoleic acid (C18:2), and cerotic acid (C26:0). (c,d) Total PE contents (c) and PE species compositions (d) of respective OMV and OM preparations were determined by LC/ESI-MS. Total PE contents (c) are given in x-fold changes normalized to Rd KW20 OMV preparations and PE species compositions (d) are given in percentage of total PE species within a respective preparation. Mean values with s.e.m. are shown (n 3 biological replicates). For PE composition analysis
(d), only PE species over 1% (at least in one preparation) are shown. The main FAs of a given PE species are indicated below each species. Additional detected FAs: capric acid (C10:0), lauric acid (C12:0), and lauroleic acid (C12:1). (b,c,d) Signicant differences between the data sets are marked by asterisks (Po0.05; one-way ANOVA followed by Sidaks multiple comparison post test).
To exclude the possibility that the observed alterations in PL levels result from increased expression of FA biosynthesis genes in the PL transporter mutants, we performed qRT-PCR analyses of the genes fabB, fabD and fabH. These genes encode for the 3-oxoacyl-ACP synthase I, the acyl carrier protein S-malonyltransferase, and the 3-oxoacyl-ACP synthase III representing three key enzymes in the FA biosynthesis pathway. TheH. inuenzae DyrbE mutant was chosen for direct comparison to the wild-type, since it showed the most pronounced alterations in the lipidome. As DyrbE and the wild-type exhibited similar transcriptional levels for all three genes (Supplementary Fig. 5), the observed PL accumulation in PL transporter mutants is not due to increased FA biosynthesis.
PE species composition analysis (Fig. 4d) conrmed the results of the FA analysis (Fig. 4b) by showing reduced PE species containing C16:0 and enriched PE species containing C14:0 in OMVs derived from PL transporter mutants compared with the wild-type. Notably, the C16:0/C14:0 FA shift (Fig. 4b,d) as well as the difference in total PE contents (Fig. 4c) between OMVs and the OM were already present in the wild-type and were just more pronounced in the PL transporter mutants. Since these changes in the PL content correlate with increased OMV formation, we hypothesize that dened PL rearrangements promote OMV formation in H. inuenzae.
Fur regulates expression of the PL transporter. By comparing the OMV quantication results of our H. inuenzae wild-type strain Rd KW20 with those of our previous study26, it became
obvious that cultures containing protoporphyrin IX instead of hemin solution produce more OMVs. Besides presence of
L-histidine and triethanolamine in the hemin solution, the only other difference between cultures containing protoporphyrin IX and hemin solution is the presence of iron contained in hemin32. Thus, we considered whether iron availability might be involved in the regulation of OMV formation in H. inuenzae. To address this question, we rst determined the vesiculation levels and OMV size distributions of Rd KW20 grown in hemin medium supplemented with or without the iron chelator 2,20-dipyridyl33 (Fig. 5a,b). We found that Rd KW20 produces 35% more, but similarly sized, OMVs in the presence of 2,20-dipyridyl. qRT-PCR experiments revealed that vacJ and yrbE expression levels were signicantly decreased (Btwo-fold) in Rd KW20 grown under iron-restricted conditions mediated by addition of 2,20-dipyridyl (Fig. 5c). This indicates that iron limitation leads to a downregulation of the VacJ/Yrb ABC transport system, which ultimately results in increased OMV production in H. inuenzae. Furthermore, we asked whether OMV production and the expression of the PL transporter genes is inuenced by Fur, a global transcriptional repressor or activator of iron-regulated genes in most bacteria3436. Indeed, a Dfur mutant grown under iron-replete conditions produces at least 70% more, but similarly sized OMVs (Fig. 5a,b). Additional qRT-PCR experiments performed with the Dfur mutant revealed that vacJ and yrbE expression levels were signicantly decreased (B10-fold and twofold, respectively) compared with Rd KW20 grown under the same conditions (Fig. 5c). This suggests that Fur activates vacJ and yrbE expression and that the downregulation of the PL
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Figure 5 | Regulation of vacJ and yrbE expression in H. inuenzae. (a) OMV preparations derived from equivalent OD490 units of cultured Rd KW20 or Rd Dfur grown in BHINADhemin supplemented without ( dip) or with ( dip) 2,20-dipyridyl were analysed for total protein (Bradford) and
lipooligosaccharide (Purpald). Mean values with s.e.m. are shown (n 6 biological replicates). (b) Distributions of OMV sizes produced by the strains in
different culture conditions were determined by nanoparticle tracking analysis. Mean values with s.d. of mean and mode OMV diameter sizes within respective OMV preparations are shown (n 6 biological replicates). (c) Relative expressions of vacJ and yrbE in Rd KW20 or Rd Dfur grown in BHINAD
hemin supplemented without ( dip) or with ( dip) 2,20-dipyridyl as well as in Rd KW20 after colonization of the mouse nasopharynx for 4 h (in vivo)
were determined by qRT-PCR. (d) Relative expressions of vacJ and yrbE in NTHi 2019-R and NTHi 1479-R grown in BHINADhemin were determined by qRT-PCR. (c,d) Horizontal bars highlight the mean of each data set (n 6 biological replicates). Dotted lines indicate a relative gene expression of 1. (a,c,d)
Signicant differences between the data sets are marked by asterisks (Po0.05; one-way ANOVA followed by Sidaks multiple comparison post test (a,c) or unpaired t-test (d)).
transporter genes in a Dfur mutant correlates with increased OMV production in H. inuenzae. To investigate whether this also holds true in distantly related Gram-negative bacteria, we analysed the OMV production and expression levels of PL transporter genes in Dfur mutants of V. cholerae and E. coli. In accordance with the observations in H. inuenzae (Fig. 5), Dfur mutants of V. cholerae and E. coli exhibited a signicant increase in vesiculation of about twofold and a signicant twofold decrease in vacJ and yrbE transcription compared with the respective wild-type (Figs 3a,b,e; 6). Thus, hypervesiculation phenotypes of Dfur mutants correlate with downregulation of vacJ and yrbE in all three bacterial species. Furthermore, in silico analyses revealed putative Fur binding sites in the upstream regions of vacJ and the yrb gene clusters of H. inuenzae, V. cholerae and E. coli,
respectively (Supplementary Fig. 6). Although this provides a rst hint that Fur might interact directly with the respective upstream regions, we cannot exclude that the Fur-dependent activation observed in this study may also be indirect via a yet unknown factor. In summary, these results indicate that the observed increase in vesiculation correlates with a downregulation of the PL transporter genes via a Fur-dependent manner, which is conserved in distantly related Gram-negative bacteria.
As iron limitation is commonly observed for bacterial pathogens in the host37,38, we analysed the expression levels of the PL transporter genes in H. inuenzae Rd KW20 during the initial stages of nasopharyngeal colonization. Compared with the in vitro condition using BHINADhemin as a growth medium, Rd KW20 revealed signicantly and at least sevenfold decreased
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Figure 6 | Regulation of vacJ and yrbE expression in E. coli. (a) OMV preparations derived from equivalent OD600 units of cultured wild-type (Ec BW) and deletion mutant (Ec Dfur) were analysed for total protein (Bradford) and lipooligosaccharide (Purpald). Mean values with s.e.m. are shown (n 6 biological
replicates). (b) Distributions of OMV sizes produced by the strains were determined by nanoparticle tracking analysis. Mean values with s.d. of mean and mode OMV diameter sizes within respective OMV preparations are shown (n 6 biological replicates). (c) Relative expressions of vacJ and yrbE in Ec BW
and Ec Dfur were determined by qRT-PCR. Horizontal bars highlight the mean of each data set (n 6 biological replicates). Dotted lines indicate a relative
gene expression of 1. (a,c) Signicant differences between the data sets are marked by asterisks (Po0.05; unpaired t-test).
% of survival
vacJ and yrbE expression levels after colonization of the mouse nasopharynx for 4 h (Fig. 5c). The reduced PL transporter gene expression in vivo suggests an increased OMV production by bacterial pathogens during initial colonization of the host. Furthermore, we recently observed different levels of OMV production for clinical NTHi isolate 2019-R and 1479-R, with the latter generating about twofold more OMVs26. In the light of the data presented herein, we investigated the PL transporter gene expressions in these two clinical NTHi isolates and observed that vacJ expression levels were signicantly 100-fold decreased in NTHi 1479-R compared with those in NTHi 2019-R (Fig. 5d), which is consistent with the observation that NTHi 1479-R generates more OMVs compared with NTHi 2019-R (ref. 26).
Hypervesiculation correlates with serum resistance. Interestingly, a recent study revealed that many clinical isolates of NTHi have surprisingly low vacJ and yrbE expression levels and these correlate with increased serum sensitivity29. Consistent with this previous report for NTHi, the H. inuenzae Rd DvacJ mutant showed a reduced survival rate in presence of human serum compared with the wild-type Rd KW20, which was restored by complementation (Fig. 7). Here we demonstrated that serum resistance was also signicantly 4,000-fold increased to a DvacJ mutant in vitro by the addition of physiological concentrations of OMVs derived from a DvacJ mutant. Likewise, the wild-type showed a signicant 10-fold increase in serum resistance, when physiological concentrations of OMVs derived from the wild-type were added. To exclude differences in the capacity to resist complement-mediated attacks, we also performed an assay using twofold higher wild-type OMV concentrations added to the DvacJ mutant. As the DvacJ mutant produces approximately twice as many OMVs compared with the wild-type (Fig. 2), the double
amount of wild-type OMVs reect a physiological concentration of DvacJ OMVs. Since the survival rate of the DvacJ mutant in presence of DvacJ OMVs and in presence of the same amount of wild-type OMVs is quite similar, we can exclude a differential
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Figure 7 | OMVs increase the serum resistance of H. inuenzae. Serum bactericidal assays were used to determine the serum resistance of Rd KW20, Rd DvacJ, and Rd DvacJ::vacJ to normal human serum. Groups tagged with Rd-OMVs, DvacJ-OMVs, and 2x Rd-OMVs
indicate assays, where Rd KW20 or Rd DvacJ OMV preparations were added to corresponding assays using respective physiological nal in vitro concentrations or a twofold higher concentration (2 Rd-OMVs). For
details please see the respective method section (serum bactericidal assay). Horizontal bars highlight the mean percentage of survival of each group (n 56 biological replicates). The dotted line indicates 100%
survival. Signicant differences between the data sets are marked by asterisks (Po0.05; one-way ANOVA followed by Sidaks multiple comparison post test).
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Outer membrane vesicle
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Figure 8 | A new model of OMV formation in Gram-negative bacteria. Step 1: Decreased expression or deletion of vacJ and/or yrb genes results in PL accumulation in the outer leaet of the OM. This asymmetric expansion of the outer leaet initiates an outward bulging of the OM. Step 2: Further enrichment of positive and negative curvature-inducing PLs in both leaets supports the budding of the OM, which nally pinches off to form an OMV. Step 3: The released OMV is enriched in PLs incorporated into the outer leaet of the vesicle membrane.
capacity between wild-type and mutant OMVs to resist complement activation. These data suggest that the disadvantage of an increased serum sensitivity caused by a downregulation of the VacJ/Yrb ABC transport system can be overcome in vivo by an increased OMV production.
DiscussionTaken together, our ndings allow us to propose a novel and potentially highly conserved OMV biogenesis mechanism in Gram-negative bacteria (Fig. 8). According to this model, deletion of vacJ and/or yrb genes, or their reduced expression, results in PL accumulation in the OM. As DvacJ and DyrbE mutants do not exhibit higher PL contents in their OM compared with the wild-type, accumulated PLs are likely to be directly secreted via OMVs. Concordantly, OMVs derived from the PL transporter mutants contain higher PL levels compared with wild-type OMVs. Notably, all hypervesiculating strains as well as the wild-type investigated in this study secrete OMVs of comparable size distribution, indicating a similar amount of PLs in the inner leaet of the vesicle membrane. Thus, the observed enrichment of PLs in OMVs derived from PL transporter mutants implicates a PL incorporation in the outer leaet of the vesicle membrane. Since the PL transporter genes are highly conserved among Gram-negative bacteria and the hypervesiculation phenotype of PL transporter mutants can be observed in distantly related Gram-negative bacteria (for example, H. inuenzae, V. cholerae and E. coli), this model of OMV formation could be a general mechanism applicable to a variety of Gram-negative bacteria.
Moreover, we show that this mechanism can be regulated by iron availability in a Fur-dependent manner. Although additional regulatory pathways may act on the PL transporter genes, it is likely that iron limitation causes the observed downregulation of the respective genes in vivo, which might impact the bacterial pathophysiology. One example could be the transmission ofH. inuenzae into a new host. Upon initial colonization of the nasopharynx, H. inuenzae must overcome mucosal immune defence mechanisms, including the protective effects of
complement factors and secretory IgA antibodies39,40. Based on our ndings, it can be hypothesized that the iron-limiting conditions in vivo cause a downregulation of the VacJ/Yrb ABC transport system resulting in increased OMV production, which counteracts antibody and complement attacks. The importance of OMVs in bacterial serum resistance is also highlighted by a recent study by Tan et al.41 demonstrating that Moraxella catarrhalis OMVs are involved in the complement resistance of nasopharyngeal bacteria by binding and depleting complement factors. One could speculate that this might also be a protective feature of H. inuenzae OMVs within the human nasopharynx. The hypervesiculation during initial colonization of a new host could provide an advantage for H. inuenzae by lowering the selective pressure of local immune defence mechanisms and thereby facilitating proliferation in the nasopharynx. In this sense, our proposed OMV biogenesis mechanism could be very important for bacterial adaptation to a new host.
It should be emphasized that this OMV biogenesis mechanism based on PL accumulation can act in concert with all other OMV formation models proposed so far. As already briey discussed in the introduction, previously reported OMV formation models are species-specic, require the presence of stress or depend on mutations affecting OM integrity. In contrast, the model proposed herein overcomes these limitations as it represents a rst general mechanism that can account for OMV formation under all growth conditions, is applicable for a broad range of Gram-negative bacteria, and can be regulated by the microorganisms.
Methods
Ethics statement. Female BALB/c (Charles River Laboratories) were used for all immunization experiments and female CD-1 IGS mice (Charles River Laboratories) were used for colonization studies in strict accordance with the recommendations in the Guide for the Care and Use of Laboratory Animals of the National Institutes of Health, the national Bundesgesetzblatt fr die Republiksterreich. The corresponding animal protocol (39/53/00 ex 2012/13) has been approved by the Austrian Federal Ministry of Science and Research Ref. II/10b and the local Committee on the Ethics of Animal Experiments of the University of Graz. Mice were housed with food and water ad libitum and monitored under the care of
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full-time staff and in accordance with the rules of the Institute of Molecular Biosciences at the University of Graz. All animals were acclimated for 1 week before any procedures were carried out and were 911 weeks old at the start of the experiment. Normal human serum was obtained and pooled from ve healthy adult volunteers according to an approval of the University of Graz Ethics Commission (GZ. 39/31/63 ex 2012/13). All volunteers provided written consent.
Bacterial strains, plasmids and growth conditions. All bacterial strains and plasmids used in this study are listed in Supplementary Table 3. Unless stated otherwise, bacteria were grown at 37 C with aeration in LuriaBertani (LB) broth or on LB agar in the case of E. coli and V. cholerae, or in brain heart infusion (BHI) broth or on BHI agar supplemented with NAD and either protoporphyrin IX (PPIX) or hemin solution (stock-solution containing a mixture of hemin,
L-histidine and triethanolamine) in the case of H. inuenzae. BHINADPPIX served as standard growth medium for H. inuenzae. BHINADhemin was used only for the following experiments: construction of transposon insertion mutants, deletion mutants and complementation strains; quantication of OMVs under conditions of iron excess or depletion; and quantitative real-time RT-PCR experiments. Supplements were used in the following nal concentrations: NAD, 10 mg ml 1; hemin, 20 mg ml 1; L-histidine, 20 mg ml 1; triethanolamine, 0.08%;
and PPIX, 20 mg ml 1. When appropriate, streptomycin (Sm, 100 mg ml 1), chloramphenicol (Cm, 2 mg ml 1), kanamycin (Km, 10 mg ml 1), or 2,20-dipyridyl (100 mM) were added to H. inuenzae growth media. E. coli and V. cholerae growth media were supplemented with streptomycin (Sm, 100 mg ml 1), kanamycin (Km, 50 mg ml 1), ampicillin (Ap, 100 or 50 mg ml 1 in combination with other antibiotics), sucrose (10%), arabinose (0.0002%), or isopropyl-b-D-thiogalactopyranoside (IPTG, 0.5 mM), if appropriate.
Purication of OMVs and OM. For H. inuenzae, OMVs as well as density gradient puried OMVs and OM were prepared as described previously26.V. cholerae and E. coli OMVs were isolated according to Schild et al.10 and Leitner et al.11, respectively. Briey, OMVs were isolated from cultures grown to late exponential phase for 13 h (H. inuenzae) or 8 h (V. cholerae and E. coli). Bacterial cells were removed from the supernatants containing the OMVs by centrifugation and subsequent ltration through 0.45 and 0.2 mm pore size lters. OMVs were pelleted from the ltrate by ultracentrifugation (144,000 g, 4 h, 4 C) using a
Beckman Coulter Optima L-100 XP ultracentrifuge. In case of lipidome and proteome analyses as well as transmission electron microscopy, H. inuenzae OMVs were further puried by density gradient ultracentrifugation using an isopycnic OptiPrep-iodixanol (Sigma-Aldrich) density gradient26. OM preparations were isolated from French press lysates obtained from H. inuenzae cultures grown to late exponential phase for 13 h followed by purication steps via ultracentrifugation using a sucrose cushion and an isopycnic sucrose density gradient26. Protein concentrations of OMV and OM preparations were either determined by photometric TrayCell measurements of the absorbances at 260 and 280 nm using a Beckman Coulter DU730 spectrophotometer in combination with a TrayCell (Hellma) and the Warburg-Christian equation or by Bradford assays (Bio-Rad Laboratories, Protein Assay Dye Reagent) according to the manufacturers manual. For all H. inuenzae, V. cholerae or E. coli Bradford assays, an OMV preparation of Rd KW20, Vc AC53, or Ec BW whose protein concentration had been determined by a TrayCell measurement was used as a protein standard, respectively.
SDSPAGE and immunoblot analysis. The protein content of OMV and OM preparations was analysed by SDSPAGE42 in combination with 12% polyacrylamide gels using the Prestained Protein Marker Broad Range (New England Biolabs) as a molecular mass standard. Protein bands were visualized by a colloidal Coomassie brilliant blue G250 staining according to Kang et al.43. Immunoblot analysis was performed as described previously26. The following primary antibodies and dilutions were used: anti-OMV mouse antiserum (see below), as well as anti-P1, -P2, -P4, -P5, or -P6 mouse antisera26 were diluted 1:500, the monoclonal antibody to the a-subunit of the E. coli RNA polymerase (NeoClone Biotechnology) was diluted 1:2,000. The horseradish peroxidaseconjugated goat anti-mouse IgG antibody (Dianova), diluted 1:7,500, served as secondary antibody. Chemiluminescence detection was performed by incubating each membrane in an ECL solution26 for 2 min with subsequent exposure in a ChemiDoc XRS system (Bio-Rad Laboratories) in combination with Quantity One software (Bio-Rad Laboratories).
Generation of an antiserum against H. inuenzae OMVs. To generate a specic polyclonal antiserum against H. inuenzae OMVs, ve female BALB/c mice were intraperitoneally immunized at days 0, 14 and 28 with approximately2 mg of an OMV preparation derived from Rd KW20 dissolved in 0.1 ml PBS (pH 7.4). Sera were isolated from blood samples collected between day 38 and46 as described previously10. Each serum was evaluated by immunoblot analysis against Rd KW20 OMVs before they were combined to generate the nal polyclonal antiserum.
Transposon mutagenesis and dot blot screen. Transposon mutagenesis inH. inuenzae was accomplished according to a method described by Schlr et al.44. For this purpose, 480 independent transformations with pAKcat carrying the transposon Tn10d-cat were performed in Rd AK01. Cm-resistant colonies were pooled and extracted chromosomal DNA was cut with XmaI. The digested DNA was retransformed into Rd KW20 resulting in 2,820 chloramphenicol-resistant transposon insertion mutants, which were subsequently screened by dot blot for altered OMV production and amounts of the OMPs P1, P2, P4, P5 or P6 in OMVs. According to Akerley et al.45 the number of non-essential ORFs, which can be targeted by transposon mutagenesis is B1,300. Thus, the screen presented herein represents an at least twofold coverage, which may not achieve saturation. To this end, transposon insertion mutants were grown for 16 h in 200 ml of BHINAD
PPIXchloramphenicol broth in quintuplicate in 96-well U-bottom plates (BD-falcon). The optical densities at 490 nm (OD490) were measured and cells were subsequently pelleted (2,000g, 10 min, room temperature). About 1 ml of pooled supernatant per transposon insertion mutant culture was ltered through a 0.2 mm pore size Supor (polyethersulfone) lter (Pall AcroPrep Advance 96-well lter plate) by centrifugation (2,000g, 2 min, room temperature) and each ltrate was stored at 20 C until dot blots were performed. For dot blot analysis, ltrates were thawed and appropriate volumes were blotted onto six Amersham Hybond ECL nitrocellulose membranes (GE Healthcare) using a 96-well Whatman Minifold I Dot-Blot System (GE Healthcare). In addition, each membrane was spotted with the respective volume of a prior made and aliquoted wild-type (Rd KW20) ltrate (prepared in the same manner as the transposon insertion mutant ltrates) as a positive control and a sterile control ltrate as a negative control. Then, each membrane was dried, incubated in Tris-buffered saline (TBS) (20 mM Tris/HCl, pH 7.5, 150 mM NaCl) for 2 min, and blocked in 10% skim milk in TBS for 2 h. Afterwards, the six membranes were incubated with either anti-OMV, -P1, -P2, -P4, -P5, or -P6 mouse antiserum (primary antibodies, see above) diluted 1:500 in 10% skim milk in TBS overnight. The next day, membranes were washed three times in TBS for 10 min, incubated with the secondary antibody (horseradish peroxidase-conjugated goat anti-mouse IgG antibody from Dianova, diluted 1:10,000 in 10% skim milk in TBS) for 2 h, washed once in TBS-T (20 mM Tris/ HCl, pH 7.5, 250 mM NaCl, 0,05% Tween-20), and twice in TBS for 10 min each. Finally, chemiluminescence detection was performed as described above. Relative intensities of dot blot signals derived from transposon insertion mutants were evaluated by eye through comparison with the respective wild-type signals in combination with the respective OD490 values. Representative examples for dot blots as well as the evaluation of relative signal intensities are provided in Supplementary Fig. 1. Interesting mutants with stronger or weaker OMV, OMPP1, -P2, -P4, -P5 and/or -P6 signals compared with the wild-type were validated once. Then, chromosomal Tn10d-cat insertions were located by DNA sequencing of junction fragments generated by PCR using the transposon mutagenesis oligonucleotide primers, which are listed in Supplementary Table 4, and a previously described method44,46.
Construction of deletion mutants and complementation strains. For construction of deletion mutants and complementation strains in H. inuenzae, overlap extension PCRs in combination with a Rd KW20 transformation protocol were performed as described previously26. Corresponding oligonucleotide primers for amplication of up- and downstream fragments, the cat gene of pAKcat, and the npt gene of pACYC177, as well as primers for validation of correct construction are listed in Supplementary Table 4. In cis complementations were achieved by replacing the cat gene of a deletion mutant with the respective gene (upstream fragment containing upstream sequence and gene of interest) and the npt gene due to homologous recombination. For construction of deletion mutants in V. cholerae, isolation of chromosomal DNA, PCRs, purication of plasmids or PCR products, construction of suicide plasmids, as well as subsequent generation of deletion mutants were carried out as described previously47. For this purpose, the plasmid pCVD442, as well as the strains DH5alpir, SM10lpir and Vc AC53 were used to construct the suicide plasmids pCVDDvacJ, pCVDDyrbE, pCVDDfur, as well as the respective deletion mutants. The expression plasmids pvacJ and pyrbE were constructed in a similar manner. PCR fragments of the respective genes containing their own ribosomal binding sites were generated using oligonucleotide primer pairs digested with the respective restriction enzymes indicated by the name of the oligonucleotide primer, and ligated into the similarly digested IPTG-inducible expression vector pMMB67EH. To construct expression plasmids for the E. coli mlaF-B genes, a PCR fragment containing the respective genes generated using oligonucleotide primer pairs digested with the respective restriction enzymes indicated by the name of the oligonucleotide primer, was ligated into the similarly digested IPTG-inducible expression vector pTRC99A. From there, a fragment containing the mla gene cluster was cut by NcoI and XbaI and ligated into a similarly digested pBAD24 to generate the arabinose-inducible expression plasmid pBADmlaF-B. Expression constructs were transformed into DH5alpir, and Apr colonies were characterized by PCR. All mutants and plasmids described herein were conrmed by PCR (data not shown). Used oligonucleotide primers are listed in Supplementary Table 4.
Quantication of OMVs. To compare the amount of OMVs produced by differentH. inuenzae, V. cholerae and E. coli strains, OMVs were puried essentially as
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described above with slight modications. Cultures were grown to late exponential phase, OD were measured, and 70 ml (H. inuenzae and V. cholerae) or 140 ml (E. coli) of the sterile-ltered supernatant was ultracentrifuged (150,000g, 4 h, 4 C) using a Type 45 Ti rotor (Beckman Coulter). The pellet comprising the OMVs was immediately resuspended in 100110 ml PBS (pH 7.4) and stored at 20 C. To quantify the protein content of OMVs, Bradford assays as described above were used. To quantify the lipooligosaccharide or lipopolysaccharide content of OMVs, purpald assays were performed as described previously48 using 3-deoxy-D-mannooctulosonic acid (Kdo) (Sigma-Aldrich) as a standard. OMVs were quantied by back-calculating the respective protein and lipooligosaccharide/lipopolysaccharide content to 1 l original culture volume per OD unit (mg l 1 OD unit 1). In case of
H. inuenzae cultivated with BHINADPPIX an additional method for OMV quantication based on dot blot analysis as described above was used. To this end, the same volume of sterile-ltered supernatants derived from all strains to be tested were dot blotted on the same membrane and anti-OMV mouse antiserum was used as primary antibody. Dot blots were developed as described above and OMV signal intensities of dots were determined using the Quantity One software (Bio-Rad Laboratories) to calculate the respective articial units (a.u.) per OD490 unit (a.u.
OD490 unit-1).
Size distribution and visualization of OMVs. Nanoparticle tracking analysis was used to measure the respective OMV size distribution of H. inuenzae, V. cholerae or E. coli OMV preparations and transmission electron microscopy was applied for OMV visualization using H. inuenzae density gradient puried OMV preparations as described previously26. Briey, respective OMV preparations were examined via nanoparticle tracking analysis using a NanoSight LM10-HS instrument (Malvern Instruments) in combination with the nanoparticle tracking analysis software suite (version 2.3). For this analysis, a monochromatic laser beam at 405 nm was applied to the diluted suspension of OMVs and a video of 90 s duration was taken with a frame rate of 25 frames per s. Measurements were performed with ambient temperatures ranging from 22 to 24 C. Particle movement was analysed by nanoparticle tracking analysis software with the minimal expected particle size, minimum track length and blur setting all set to automatic. Each video was then analysed to determine the respective mean and mode (particle size that appears most often within a given preparation) OMV size. To visualize H. inuenzae OMVs by transmission electron microscopy, preparations were diluted to 0.1 mg ml 1 (protein equivalent) in PBS (pH 7.4) and 3 ml thereof was allowed to adsorb onto a carbon-coated copper grid for 15 s. After removal of excess liquid, samples were negatively stained with 2% uranyl acetate for 15 s followed by a further removal of excess liquid. Micrographs were recorded using a Morgagni 268 (FEI) transmission electron microscope.
OM integrity assays. To compare the OM stability between different H. inuenzae strains, the degree of cell lysis was assessed by dot blot analysis and minimal inhibitory concentrations of SDS and polymyxin B were determined. Dot blot analysis was performed as described above for the quantication of OMVs, except that a monoclonal antibody to the a-subunit of the E. coli RNA polymerase (RpoA,
NeoClone Biotechnology, diluted 1:2,000) was used as primary antibody to detect RpoA in the sterile-ltered supernatants. RpoA detection has previously been used as a cytoplasmic contamination and lysis control in H. inuenzae26. Minimal inhibitory concentrations were determined by using respective mid-log phase grown cultures to inoculate each well of a 96-well plate to a nal OD490 of 0.1.
Appropriate serial dilutions of SDS and polymyxin B were added and the plate was incubated at 37 C for 16 h. Afterwards, the OD490 of each well was measured and
compared with wells not containing bacteria (negative control). The minimal inhibitory concentration was dened as the lowest concentration of SDS or polymyxin B that inhibited bacterial growth (OD490o0.3).
Proteome analysis. Mass spectrometry was used to identify proteins from density gradient puried OMV and OM preparations. Sample preparation, mass spectrometry, and protein identication by the Mascot search engine (version 2.3.02, Matrix Science) were performed as described previously26. Briey, 0.7 mg (protein equivalent) of respective preparations were subjected to trypsin in-solution digestion. Therefore, samples were subjected to lipid extraction and resuspended in ammonium bicarbonate. Addition of DTT ensured reduction of disulphides in the samples, which were alkylated via iodoacetamide treatment. After trypsin digestion, samples were lyophilized, resuspended in 10 ml 0.1% triuoroacetic acid, desalted using ZipTip C18 microcolumns (Millipore) according to the manufacturers manual, and resuspended in 8 ml 0.1% formic acid. Finally, samples were analysed using a hybrid quadrupole orthogonal acceleration time-of-ight (Q-TOF) mass spectrometer (Waters) equipped with a nanoACQUITY ultra performance liquid chromatography system (Waters). The resulting MS/MS spectra were used for the identication of proteins by the Mascot search engine using the NCBInr database with the bacteria (eubacteria) taxonomy selected. Searches were carried out with the xed modication carbamidomethyl (C), the enzyme selected as trypsin allowing up to 1 missed cleavages, a peptide tolerance of 1.2 Da, a MS/MS tolerance of 0.6 Da, a peptide charge of 1 , 2 and 3 , monoisotopic mass values, and the
instrument setting selected as ESI-QUAD-TOF. All data were searched with the signicance threshold set to a P value of o0.05 resulting in an identity ion score
threshold between 58 and 61. Only results with ion scores greater than or equal to the identity threshold were considered signicant.
Lipidome analyses. Lipids from density gradient puried OMV and OM preparations were extracted according to Folch et al.49 with minor modications. For phosphatidylethanolamine composition analysis, lipids were extracted twice with a solvent containing 1% acetic acid, 500 nM butylated hydroxyl toluene, and 4 nM C17:0 phosphatidylcholine per sample as internal standard (ISTD). For determination of FAs, PLs, and phosphatidylethanolamine composition, lipids were extracted from samples containing 300 mg, 1,000 mg, and 50 mg protein, respectively. All lipid extracts were dried under a stream of nitrogen and stored at 20 C until analysis. For FA analysis, dried lipid extracts were transesteried to fatty acid methyl esters (FAMEs) by methanolysis containing 2.5% sulphuric acid at 85 C for 90 min. FAMEs were extracted into light petroleum ether/water (3/1, vol/vol) and analysed by gas liquid chromatography and ame-ionization detection (Hewlett-Packard 6890) using a HP-INNOWax capillary column(15 m 0.25 mm i.d. 0.50 mm lm thickness) with helium as carrier. FAME
species were identied by comparison to the FAME standard mix GLC-68B (Nu-Chek, Inc) and C26:0 FAME (Sigma-Aldrich). For PL analysis, lipid extracts and, for comparison, a PL mix were separated by one-dimensional thin-layer chromatography on Silica gel 60 plates (Sigma-Aldrich) using chloroform/acetone/ methanol/acetic acid/water (50/20/10/10/5, per vol.). Lipids were stained with iodine vapour, stained spots were scraped off and phosphate residues of PLs were liberated by treatment with H2SO4 (72%)/HClO4 (9/1, vol/vol), which were subsequently quantied colourimetrically as phosphomolybdate measured at820 nm according to the standard procedure described by Broekhuyse50. For phosphatidylethanolamine species analysis, dried lipids were dissolved in 2-propanol/chloroform/methanol (7/2/1, per vol.) and analysed by LC/ESI-MS using an Acquity UPLC HSS T3 column (100 , 1.8 mm, 2.1 100 mm, Waters)51.
Extraction efcacy and lipid recovery were normalized using ISTD.
Quantitative real-time RT-PCR. Expression of vacJ, yrbE, fabB, fabD or fabH was determined by quantitative real-time RT-PCR (qRT-PCR). For this purpose, respective strains were grown to an OD490 of 0.8-1 in BHINADhemin medium supplemented with or without 100 mM 2,20-dipyridyl in case of H. inuenzae or to an OD600 of 0.70.9 in LB medium in case of V. cholerae and E. coli. Bacterial RNA extraction, DNase digestion, cDNA synthesis and qRT-PCR were performed as described previously52. To determine the gene expression of vacJ and yrbE inH. inuenzae under in vivo conditions, CD-1 mice were intranasally inoculated with Rd KW20 essentially as described previously8 with an inoculum of approximately 5 108 c.f.u. per mouse. After 4 h, the mice were sacriced,
the nasopharynx of each mouse was removed by dissection and mechanically homogenized in 2 ml Trizol. RNA was subsequently extracted using chloroform extraction and precipitated with isopropanol. DNase digestion, cDNA synthesis and qRT-PCR were performed as described previously53. Corresponding oligonucleotide primers are listed in Supplementary Table 4. Relative gene expression comparisons were obtained through the DDCT method by normalizing the mean cycle threshold of each investigated transcript to the housekeeping gene rpoB and to one randomly selected reference sample.
Serum bactericidal assay. To test H. inuenzae strains in serum bactericidal assays, cells were grown to an OD490 of 0.81 and diluted in Hanks buffer (HBSS from Gibco, with Ca2 and Mg2 , no phenol red) to an OD490 of 0.1. About 100 ml of this suspension were mixed with 5 ml normal human serum (2% nal concentration) and optionally with 5 ml of appropriate dilutions of respective OMV preparations. This resulted in the following physiological nal in vitro concentrations of OMVs based on the OMV quantication via purpald assays (lipooligosaccharide equivalent) of B0.6 mg l 1 OD490 unit 1 for Rd KW20-derived OMVs and 1.2 mg l 1 OD490 unit-1 for Rd DvacJ derived OMVs. In case of two-fold amounts of Rd KW20-derived OMVs, 10 ml were added, which result in a nal concentration of approximately 1.2 mg l 1 OD490 unit 1. Hanks buffer was added beforehand to obtain a nal reaction volume of 250 ml. The mixture was incubated at 37 C for 45 min with rotation, the assay was stopped by coolingto 4 C, and appropriate dilutions were plated on agar plates to determine viable counts. To calculate the percentage of survival, viable counts were compared with control samples in absence of normal human serum.
Statistical analysis. Data were analysed using GraphPad Prism version 6.0f for Mac OS X (GraphPad Software). The statistical signicance of differences between groups was examined using the unpaired t test or an ordinary one-way ANOVA followed by Sidaks multiple comparison post test. Differences were considered signicant at P values of o0.05.
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Acknowledgements
We thank Wael Elhenawy as well as Bela Reiz (University of Alberta, Edmonton,
Canada) for assistance with protein mass spectrometry, Arlene Oatway (University of
Alberta, Edmonton, Canada) for assistance with transmission electron microscopy, and
Gebhard Schratter (Medical University of Graz, Austria) for assistance with nanoparticle
tracking analysis. We are grateful to Klaus Hantke (University of Tbingen, Germany)
for providing the Ec BW and Ec Dfur strains. Furthermore, we thank Lydia Mausser for
help with artwork design as well as Ellen L. Zechner and Rudolf Zechner (University of
Graz, Austria) for critically reading the manuscript. This work was supported by
the Austrian FWF grants P25691 to S.S., P25193 to A.L., P27346 to G.D., as well as
W901-B12 (DK Molecular Enzymology) to S.R, F.G.Z., F.C., G.D. and S.S. We
acknowledge the Alberta Glycomics Centre and the Natural Sciences and Engineering
Research Council of Canada (NSERC) for funding to M.F.F. M.F.F. is a Canadian
Institutes of Health Research (CIHR) new investigator.
Author contributions
S.R. and S.S. conceived the study, designed the experiments, and wrote the manuscript
with input from all authors. S.R., F.G.Z., F.C., S.D., P.K., T.O.E., L.K., B.G., K.W., J.R. and
12 NATURE COMMUNICATIONS | 7:10515 | DOI: 10.1038/ncomms10515 | http://www.nature.com/naturecommunications
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NATURE COMMUNICATIONS | DOI: 10.1038/ncomms10515 ARTICLE
S.S. performed the experiments. S.R., F.G.Z., F.C., R.P., A.L., G.D., J.R., M.F.F. and S.S.
Analysed and interpreted the data. R.P., A.L., G.D., J.R., M.F.F. and S.S. provided
reagents, materials, and analysis tools.
Additional information
Accession codes: The mass spectrometry proteomics data have been deposited to the
ProteomeXchange Consortium via the PRIDE partner repository with the data set
identier PXD003249.
Supplementary Information accompanies this paper at http://www.nature.com/naturecommunications
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Abstract
Bacterial outer membrane vesicles (OMVs) have important biological roles in pathogenesis and intercellular interactions, but a general mechanism of OMV formation is lacking. Here we show that the VacJ/Yrb ABC (ATP-binding cassette) transport system, a proposed phospholipid transporter, is involved in OMV formation. Deletion or repression of VacJ/Yrb increases OMV production in two distantly related Gram-negative bacteria, Haemophilus influenzae and Vibrio cholerae. Lipidome analyses demonstrate that OMVs from VacJ/Yrb-defective mutants in H. influenzae are enriched in phospholipids and certain fatty acids. Furthermore, we demonstrate that OMV production and regulation of the VacJ/Yrb ABC transport system respond to iron starvation. Our results suggest a new general mechanism of OMV biogenesis based on phospholipid accumulation in the outer leaflet of the outer membrane. This mechanism is highly conserved among Gram-negative bacteria, provides a means for regulation, can account for OMV formation under all growth conditions, and might have important pathophysiological roles in vivo.
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