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PpiD is a player in the network of periplasmic chaperones in Escherichia coli

Abstract

Background

The inner membrane-anchored periplasmic folding factor PpiD is described as a parvulin-like peptidyl prolyl isomerase (PPIase) that assists in the maturation of the major beta-barrel outer membrane proteins (OMPs) of Escherichia coli. More recent work however, calls these findings into question. Here, we re-examined the role of PpiD in the E. coli periplasm by analyzing its functional interplay with other folding factors that influence OMP maturation as well as general protein folding in the periplasmic compartment of the cell, such as SurA, Skp, and DegP.

Results

The analysis of the effects of both deletion and overexpression of ppiD on cell envelope phenotypes revealed that PpiD in contrast to prior observations plays only a minor role, if any, in the maturation of OMPs and cannot compensate for the lack of SurA in the periplasm. On the other hand, our results show that overproduction of PpiD rescues a surA skp double mutant from lethality. In the presence of increased PpiD levels surA skp cells show reduced activities of both the SigmaE-dependent and the Cpx envelope stress responses, and contain increased amounts of folded species of the major OMP OmpA. These effects require the anchoring of PpiD in the inner membrane but are independent of its parvulin-like PPIase domain. Moreover, a PpiD protein lacking the PPIase domain also complements the growth defects of an fkpA ppiD surA triple PPIase mutant and exhibits chaperone activity in vitro. In addition, PpiD appears to collaborate with DegP, as deletion of ppiD confers a temperature-dependent conditional synthetic phenotype in a degP mutant.

Conclusions

This study provides first direct evidence that PpiD functions as a chaperone and contributes to the network of periplasmic chaperone activities without being specifically involved in OMP maturation. Consistent with previous work, our data support a model in which the chaperone function of PpiD is used to aid in the early periplasmic folding of many newly translocated proteins.

Background

It is well established that numerous chaperones, folding catalysts and proteases exist in the periplasm of E. coli and cooperate in protein folding and protein quality control in this cellular compartment of the cell. At least three of these factors, SurA, Skp and DegP, assist in the maturation of integral β-barrel outer membrane proteins (OMPs), a major class of proteins in the E. coli outer membrane, and are thought to be responsible for the transport of OMP folding intermediates through the periplasm to the OMP assembly site, a multi-protein complex in the outer membrane [1].

The chaperone and peptidyl-prolyl isomerase (PPIase) SurA is specialized for the biogenesis of OMPs. SurA preferentially interacts with newly-synthesized OMPs in vitro[2] by specifically recognizing and binding to peptide sequences that are characteristic of OMPs [3, 4]. Only a subset of OMPs however, appears to directly depend on SurA for maturation [5]. The two biochemical activities of SurA reside in distinct regions of the protein [2]. The PPIase activity is carried in the second of two iterative parvulin-like domains (domain I and domain II) located in the C-terminal half of the protein [2, 6]. The chaperone activity, which is required and sufficient for the so far known biological role of SurA, is contained in a module formed by its N-terminal region and a short C-terminal sequence [2]. Lack of SurA gives phenotypes that are indicative of disturbances in OMP biogenesis and of a defective cell envelope. Such phenotypes are reduced levels of the major OMPs OmpA, LamB, and OmpC in the outer membranes of the cells, increased sensitivity to hydrophobic agents, such as SDS/EDTA, bile salts, and the antibiotic novobiocin, and a constitutively induced σE-dependent envelope stress response [6–8]. The σE pathway together with the Cpx signal transduction pathway monitors and controls the protein folding state in the cell envelope [9].

The small periplasmic chaperone Skp and the protease-chaperone DegP affect general protein folding in the periplasm and assist in the biogenesis of OMPs. A skp mutant shows phenotypes that are similar to but less severe than those of a surA mutant [7]. Moreover, deletion of skp confers synthetic lethality in a surA mutant, as does deletion of degP[2, 10]. degP skp double mutants on the other hand are viable. It has therefore been proposed that DegP and Skp act together in one pathway of OMP maturation whereas SurA acts in a separate parallel pathway [5, 10]. Skp has been shown to interact with early OMP folding intermediates at the periplasmic side of the inner membrane [11, 12] and to keep immature OMPs in a soluble state [13, 14]. DegP on the other hand, was found to bind to and stabilize folded OMP monomers [15] and thus appears to act downstream of Skp in the proposed Skp/DegP pathway for OMP maturation.

Conflicting results have been reported regarding the involvement of the periplasmic PpiD protein in the biogenesis of OMPs. PpiD is anchored to the inner membrane by an N-terminal transmembrane segment and consists of a single parvulin domain flanked by large N- and C-terminal protein regions. The N-terminal region shares sequence similarity with the N-terminal region of SurA, which comprises the major part of the SurA chaperone module ([16–19]; see additional file 1). Several previous findings suggested that PpiD and SurA have overlapping functions in OMP biogenesis [18]. First, a ppiD mutant was documented to have phenotypes that are similar to those of a surA mutant and are suppressed by multicopy surA. Second, the simultaneous deletion of ppiD and surA was reported to cause lethality. More recently however, surA ppiD mutants were shown to display no visible growth defects [20]. Finally and most importantly, ppiD was isolated as a multicopy suppressor in a surA mutant. Remarkably however, whereas the surA phenotypes result from loss of chaperone function [2], a high PPIase activity of PpiD was identified as the complementing biochemical activity [18]. Most recently, this result was disputed by the finding that the isolated parvulin domain of PpiD is devoid of detectable PPIase activity [19]. Here, we analyzed the functional interplay of PpiD with SurA, Skp, and DegP to define its role in the E. coli periplasm.

Results

Re-examination of PpiD function in the biogenesis of OMPs

To resurvey the role of PpiD in OMP maturation we analyzed the physiological consequences of both inactivation and overexpression of ppiD in wild-type cells and in the surA and skp mutants, respectively, using phenotypes known to report on OMP biogenesis and outer membrane integrity, such as σE activity, resistance of the cells to SDS/EDTA and to the antibiotic novobiocin, as well as the levels of major OMPs in their outer membranes. In contrast to previous work [18] we found that expression of multicopy ppiD from the IPTG-inducible Ptrc promoter does not suppress the surA mutant phenotypes but rather interferes with cell growth (data not shown). We therefore used a plasmid (pPpiD) that carries ppiD under control of its natural promoter, which is positively regulated by the classical cytoplasmic σ32-dependent heat-shock response and by the Cpx two-component system [18, 21].

Consistent with recent observations [20], the inactivation of ppiD in a surA strain did not cause lethality. Also, neither the inactivation nor the overexpression of ppiD in the tested strains had major effects on the activity of σE (Figure 1), on the plating efficiencies on 0.5% SDS/0.5 mM EDTA (Table 1), on the sensitivities of the cells to novobiocin, or on the levels of major OMPs in their outer membranes (data not shown). However, as is also the case for strains lacking Skp, PpiD-deficient strains showed slightly retarded growth on plates containing 0.5% SDS and 0.5 mM EDTA. At increased concentrations of SDS (2%) a ppiD skp double mutant even revealed a small (3-to 4-fold) plating defect (Table 1), but showed no major changes in the activity of σE and in the amounts of OMPs in the outer membranes of the cells relative to the Δskp single mutant (Figure 1 and data not shown). Thus, loss of PpiD appears to slightly interfere with outer membrane integrity without notably affecting the assembly of OMPs. Together these results suggest that PpiD plays only a minor role, if any, in the biogenesis of OMPs in the strain background used here.

Figure 1
figure 1

Response of the σE-dependent and the CpxA/R-regulated envelope stress pathways to inactivation and overexpression of ppiD. EσE (A) and Cpx (B) activities in the indicated strains carrying SurA (light gray bars), PpiD (dark gray bars), and Skp (black bars) encoding plasmids or an empty vector (pASK75; white bars) were assayed by monitoring the accumulation of β-galactosidase resulting from σE-dependent rpoH P3::lacZ and from Cpx-meditated cpxP-lacZ reporter expression, respectively. Cells were grown in LB (σE) or in LB buffered at pH 7.0 (Cpx) at 37°C and β-galactosidase activities were determined as described in Methods and compared to that of wild-type cells. Results represent the average of at least two independent experiments (*P ≤ 0.05; **P ≤ 0.01 Student's t-test). Qualitatively similar results were obtained from cells grown at 30°C (data not shown). (C) Western blot analysis of crude extracts derived from cells with (+) and without (-) pPpiD. A volume of sample equivalent to 4 × 107 cells was loaded onto each lane. The anti-PpiD antiserum showed a weak unspecific cross-reaction with a similar sized unknown protein. The intensity of the PpiD signal relative to that in the wild-type strain (rel. Int.) was calculated using MalE as the internal standard for each lane.

Table 1 Plating efficiencies on SDS/EDTA

Effects of inactivation and overexpression of ppiD on the Cpx envelope stress response

The σE signal transduction pathway partially overlaps with the CpxA/R pathway in sensing and responding to folding stress in the cell envelope [9]. Since ppiD is a member of the Cpx regulon [18] we asked whether the Cpx system would respond to inactivation or increased expression of ppiD. As shown in Figure 1B, inactivation of ppiD had no significant effect on Cpx activity in any of the tested strains, indicating that PpiD is not specifically involved in cell envelope functions that are monitored by the Cpx stress response pathway. In contrast, lack of SurA induced the Cpx response ~4-fold, as is consistent with the involvement of SurA in OMP and pilus biogenesis [20] and with misfolding pilus subunits being sensed by the Cpx signaling system [22]. The presence of ppiD in multicopy led to an about 2-fold induction of the Cpx response in all strains but the surA single and the surA ppiD double mutants. In the surA ppiD double mutant increased expression of ppiD from pPpiD slightly reduced Cpx activity, whereas it showed no significant effect on Cpx activity in the surA single mutant.

ppiD is a multicopy suppressor of the lethal surA skp phenotype

We also asked whether ppiD in multicopy would suppress the synthetic lethality of a surA skp mutant. SurA-depletion strains were constructed by placing the chromosomal surA gene under the control of the IPTG-inducible promoter P Llac-O1 [23], so that expression of surA could be shut off in the absence of IPTG. As expected, P Llac-O1 -surA Δskp cells grew poorly without IPTG but normal growth was restored by providing copies of either surA or skp on a plasmid (Figure 2B). Unexpectedly, growth in the absence of IPTG was also restored by ppiD in multicopy (pPpiD), although the colonies grew up slower and remained smaller than those grown in the presence of IPTG. The growth-promoting effect of pPpiD was abolished by the introduction of a frameshift mutation that results in a premature stop at codon 173 of the plasmid-borne ppiD gene (pPpiDfs601). Thus, suppression of surA skp lethality elicited by pPpiD requires the intact ppiD gene. Multicopy ppiD also restored viability of surA skp cells in liquid media (Figure 2C). The P Llac-O1 -surA Δskp strain ceased growth approximately 3.5 h after transfer into non-permissive media (LB without IPTG) but continued to grow when it carried pPpiD, although with slower rates during the mid- to late logarithmic phase. Western blot analysis indicated that PpiD is present in these cells at levels greater than that of chromosomally encoded PpiD (Figure 2D, lane 3 versus lanes 1 and 2). Thus, increased production of PpiD restores viability of surA skp cells but it does not completely compensate for the growth defect caused by the simultaneous lack of the SurA and Skp chaperones.

Figure 2
figure 2

Suppression of the lethal phenotype of surA skp cells by multicopy ppiD. (A) Schematic representation of PpiD and its variants used in this study, with amino acid residues numbered as in the full-length PpiD polypeptide. Diagonally striped box: transmembrane segment; white box: N-terminal region; Gray box: parvulin domain, with alanine substitutions indicated by black bars. PpiDΔTM was preceded by the SurA signal peptide so that it would be secreted into the periplasm (see Methods). (B) Growth of the SurA-depletion strain P Llac-O1 -surA Δskp (SB44452) carrying pASK75 (empty vector), pSurA, pSkp, and pPpiD, respectively. Cells were grown overnight in the presence of IPTG, after dilution spotted on LB plates ± IPTG, and incubated at 37°C for 16-24 h. (C) Growth of the strains P Llac-O1 -surA (SB44454) and P Llac-O1 -surA Δskp (SB44452) at 37°C in liquid LB with (solid lines) and without (dotted lines) IPTG, resulting in the indicated "genotypes" wild-type (WT), surA, skp, and surA skp. The asterisk marks the point of sub-culturing (see Methods). Within the framed interval samples were taken for further analysis. Note that the Δskp surA strain containing pASK75 or pPpiDΔTM resumed growth after ~360-minute cultivation without IPTG. Western blotting revealed that at this point the cells also resumed production of SurA (see additional file 3). In contrast, SurA levels remained low in Δskp surA pPpiD cells during the entire course of growth, indicating that increased PpiD levels compensate for the simultaneous lack of SurA and Skp. (D) PpiD proteins in P Llac-O1 -surA Δskp cells after 240-minute growth in LB without IPTG. Extracts from 4 × 107 cells were loaded in each lane and analyzed by western blotting. Lane 8 shows lane 6 after prolonged development of the blot to visualize the protein. Cytoplasmic Hsc66 served as a loading control. Data for one representative experiment are shown.

Suppression of surA skp lethality does not require the parvulin domain but the membrane-localization of PpiD

The lethal phenotype of surA skp cells has been suggested to result from loss of periplasmic chaperone activity [10]. Consistent with this assumption, we found that the chaperone module of SurA (SurAN-Ct), which is devoid of any PPIase activity [2], is sufficient to fully complement the growth defect of the P Llac-O1 -surA Δskp strain in the absence of IPTG (Figure 2B). To also dissect the activities and regions of PpiD required for complementation of surA skp lethality, we substituted amino acids G347 and I350 in its parvulin domain with alanine, generating the proteins PpiDG347A and PpiDI350A, respectively. These mutations had originally been reported to effectively eliminate PPIase activity of PpiD and to result in the loss of its reported surA complementing function [18]. In addition, we completely deleted the parvulin domain from the protein, resulting in PpiDΔParv (Figure 2A). Only most recently, while this manuscript was in preparation, PpiD and its isolated parvulin domain have been shown to be devoid of PPIase activity [19]. However, because G347 and I350 are located at the peptide binding site of the parvulin domain, it was suggested that substrate binding to this domain is important for the in vivo function of PpiD.

Both mutant proteins, PpiDG347A and PpiDI350A, complemented the growth defect of surA skp cells just as well as wild-type PpiD, whereas PpiDΔParv complemented slightly less well in these assays (Figure 2B and 2C). Western blot analysis indicated however, that PpiDΔParv was present in the cells at significant lower levels than plasmid-encoded wild-type PpiD (Figure 2D, lane 5 versus lane 3), suggesting that the protein is less stable. We have confirmed that all three mutant PpiD proteins also restore growth of a ppiD skp surA triple mutant (additional file 2), demonstrating that the surA skp complementing activity does not depend on some residual function provided by chromosomally encoded wild-type PpiD. Together, these results show that the parvulin domain is not required for PpiD to function in rescuing surA skp cells from lethality. Unfortunately, we were unable to assess meaningfully if the N-terminal region of PpiD which shows sequence similarity to a substantial portion of the chaperone domain of SurA ([16–18] and additional file 1) contributes to this function, as a protein lacking the respective region (PpiDΔ69-201, Figure 3A) was present in the cells at even lower levels than PpiDΔParv (Figure 3D, lanes 7 and 8).

Figure 3
figure 3

Increased PpiD levels reduce σE and Cpx activity in surA skp cells. (A) SurA-depletion strains carrying either the chromosomal σE-dependent rpoH P3::lacZ or the Cpx-regulated cpxP-lacZ reporter fusions were cultivated at 37°C in LB buffered at pH 7.0 ± IPTG as described in Methods. Once growth of P Llac-O1 -surA Δskp cells ceased in the absence of IPTG, samples were taken and assayed for σE and Cpx activities, respectively, by determining β-galactosidase activity. The strains contained either an empty vector (pASK75) or a plasmid encoding wild-type PpiD, PpiDI350A, PpiDΔParv, and PpiDΔTM (soluble His6-PpiD), respectively. The data shown are representative of at least two independent experiments. (B) Western blot detection of SurA and of DegP in crude extracts of cells after 240-minute growth at 37°C in LB ± IPTG. A volume of extracts equivalent to 4 × 107 cells was loaded onto each lane. Signal intensities were calculated using Hsc66 as the internal standard for each lane and are shown relative to those in the wild-type strain (rel. Int.). Western analysis was performed a minimum of two times for each σE and Cpx reporter assay, and data for one representative experiment are shown.

Finally, we asked if PpiD must be anchored to the inner membrane to function in vivo. Neither production of soluble N-terminally His6-tagged PpiD (PpiDΔTM) at a level similar to that of PpiDΔParv nor its production from pASKssPpiD at different inducer concentrations restored growth of surA skp cells (Figure 2, and data not shown). pASKssPpiD has also been used to produce and purify soluble His6-PpiD from the periplasmic fraction of E. coli, thus confirming the periplasmic location of the protein. As soluble His6-PpiD is functional in vitro (see below and [24]), these results suggest that the function of PpiD in vivo requires the protein to be anchored in the inner membrane.

Overproduction of PpiD lowers folding stress in the cell envelope of surA skp cells

Previous studies suggested that the lethal phenotype of a surA skp mutant is caused by severe protein folding stress in the periplasmic compartment of the cells [10, 25]. To determine whether increased PpiD levels restore viability of surA skp cells by counteracting folding stress in the cell envelope, we monitored the activities of the σE and Cpx stress pathways over time once growth of P Llac-O1 -surA Δskp cells had leveled off in the absence of IPTG (time interval indicated in Figure 2C). At this time point, SurA was hardly detectable in the cells (Figure 3B), indicating that SurA had efficiently been depleted from the cells. During the course of the depletion of SurA in Δskp cells both the Cpx pathway and, as also reported previously [26], the σE-dependent pathway were strongly induced (Figure 3A). The σE and Cpx activities were 4- to 6-fold increased in SurA-depleted Δskp cells (surA skp pASK75) relative to those of SurA-depleted wild-type cells (surA pASK75). This is also reflected in further increased levels of DegP (Figure 3B, lane 4 versus lane 2), whose gene is positively controlled by the σE and Cpx stress responses [27, 28]. In Δskp cells that overproduced PpiD during the course of SurA depletion, σE and Cpx activities were significantly lower, being only 1.5- to 3-fold induced relative to the respective activities in surA cells. Consistent herewith, the level of DegP was lower in these cells than in surA skp cells that not overproduced PpiD but slightly higher than the DegP level in surA cells (Figure 3B, lane 5 versus lanes 4 and 2, respectively). Production of PpiDΔParv during the course of SurA depletion in Δskp cells reduced the σE and Cpx activities slightly less effectively and production of soluble His6-PpiD (PpiDΔTM), which does not rescue surA skp cells from lethality, further induced both stress responses (Figure 3A). Thus, only increased levels of membrane-anchored PpiD proteins dampen the strong response of the σE and the Cpx envelope stress signal transduction pathways to the simultaneous loss of SurA and Skp chaperone activity.

Taking advantage of the fact that overproduction of the outer membrane lipoprotein NlpE specifically induces the Cpx response [29] and that the Cpx pathway negatively controls expression of the σE regulatory components [30] we also asked whether down-regulation of σE activity alone would be sufficient to restore growth of surA skp cells. Indeed, the presence of multicopy nlpE during the course of SurA depletion in Δskp cells led to a further induction of the Cpx response and down-regulated σE activity to a similar extent as overproduction of PpiD (see additional files 3 and 4). Overexpression of nlpE even slightly improved cell growth in liquid media but it did not restore growth of surA skp cells on solid plates. Thus, Cpx-mediated repression of σE alone is not sufficient to restore surA skp cell viability.

Effect of PpiD overproduction in surA skp cells on OMP biogenesis

The reduction of σE activity in surA skp cells elicited by higher levels of PpiD suggests that PpiD in these cells directly or indirectly affects OMP biogenesis. σE positively controls the production of small non-coding RNAs, which down-regulate OMP synthesis by translational repression [31], and decreased levels of OMPs in SurA-deficient cells therefore reflect defects in both OMP synthesis and assembly [6]. We asked if conversely, the decrease in σE activity in PpiD overproducing surA skp cells correlated with increased levels of the major OMP OmpA. Western blot analysis of crude cell extracts confirmed a slight increase in the level of OmpA in these cells as compared to surA skp cells (Figure 4A lane 5 versus lanes 4 and 6, respectively), suggesting that in the absence of SurA and Skp increased levels of PpiD stimulate OmpA synthesis and/or stability. To substantiate this result and to explore a possible influence of PpiD on OmpA folding in surA skp cells, we examined the consequence of PpiD overproduction on the OmpA folding state during the course of SurA depletion in Δskp cells. The OmpA folding state can be conveniently followed by a shift in the apparent mass on SDS polyacrylamide gels. The folded β-barrel domain of OmpA is stable in 2% SDS and migrates faster than unfolded OmpA if not heat-denatured prior to electrophoresis [32]. OMPs were prepared by gentle lysis to preserve their native conformation [33] and OmpA folding intermediates were detected by western blotting (Figure 4B). In contrast to previous work showing that unfolded OmpA accumulates in surA skp double null cells [26], we found the conditional surA skp mutant to contain significantly reduced levels of both, folded and unfolded forms of OmpA (lanes 4 and 5). This difference may reflect the use of a different SurA depletion strategy or the presence of higher levels of DegP protease activity in the strain used here, or both. In any case, the amount of folded OmpA was clearly increased in surA skp cells that overproduced PpiD (lane 3) and was almost as high as that in surA cells (lane 1). Thus, in surA skp cells both synthesis and folding of OmpA is stimulated by increased PpiD levels. Together, these results suggest that in the absence of both chaperones, SurA and Skp, overproduction of PpiD can, at least in part, counteract the defects in the biogenesis of OmpA and possibly of other OMPs.

Figure 4
figure 4

Overproduction of PpiD in surA skp cells stimulates synthesis and folding of OmpA. The SurA- depletion strains P Llac-O1 -surA (SB44454) and P Llac-O1 -surA Δskp (SB44452; Δskp) were grown at 37°C in LB buffered at pH 7.0 supplemented with 0.2% maltose ±of IPTG. Cells contained either pPpiD (+) or the empty vector pASK75 (-). The data shown are representative for a minimum of two independent experiments. (A) Total cellular levels of SurA and of OmpA in SurA-depletion strains grown for 240 min as described above. Extracts corresponding to 8 × 107 cells were loaded onto each lane and analyzed by western blotting. Signal intensities were calculated using cytoplasmic Hsc66 as the internal standard for each lane and are shown relative to those in the SurA-depleted P Llac-O1 -surA strain (rel. Int.). (B) Levels of unfolded OmpA (u-OmpA) and folded OmpA (f-OmpA) species in SurA-depletion strains grown as described above. Culture samples corresponding to an equal number of cells were taken at the indicated time points and cell extracts prepared by gentle lysis. Samples of cell extracts corresponding to 1.3 × 108 cells were loaded onto each lane and analyzed by western blotting. Relative signal intensities (rel. Int.) for u-OmpA (u) and f-OmpA (f) were calculated as in A.

PpiD has in vitro chaperone activity

The above findings suggest that suppression of the lethal surA skp phenotype by overproduction of PpiD does not simply result from regulatory events in response to increased PpiD levels but rather from functional complementation of the surA skp caused deficiency. As the defects of the surA skp double mutant are thought to result from lack of periplasmic chaperone activity [10], we asked whether the PpiD and PpiDΔParv proteins provide such an activity by examining their capability to prevent aggregation of thermally denatured citrate synthase, a classic in vitro assay for chaperone function [34]. SurA had previously been shown to possesses this activity [2] and was used as a control. When citrate synthase was thermally denatured in the presence of an 8-fold molar excess of SurA (based on citrate synthase monomer) aggregation was significantly reduced (Figure 5). Chymotrypsinogen A, which served as a negative control, showed no or only minor effects at this concentration. In contrast, an 8-fold excess of PpiD reduced aggregation of citrate synthase significantly, although less effectively than SurA, requiring 2-fold higher concentrations to have roughly the same effect. PpiDΔParv finally, which lacks the PPIase domain (Figure 2A), protected citrate synthase about 2-fold more effectively from aggregation than intact PpiD, being almost as effective as SurA. The observed chaperone effects are not caused by protease contamination, as the same amount of citrate synthase was present in samples taken throughout a 1200 s incubation period with a 16-fold excess of PpiD proteins (as judged by SDS-PAGE and silver stain; data not shown). Thus, PpiD exhibits a chaperone activity that is carried in the non-PPIase regions of the protein. The finding that PpiDΔParv complements the growth defect of a surA skp mutant less well than full-length PpiD (Figure 2C) although it exhibits stronger in vitro chaperone activity (Figure 5) likely relates to the presence of lower levels of PpiDΔParv than of plasmid-encoded intact PpiD in these cells (Figure 2D). The overall chaperone activity provided by PpiDΔParv in the cells may thus be weaker than that provided by the overproduced intact PpiD.

Figure 5
figure 5

The PpiD and PpiDΔParv proteins exhibit chaperone activity in vitro. Thermal aggregation of citrate synthase (0.15 μM monomer) at 43°C in the presence of SurA (positive control), Chymotrypsinogen A (negative control), and the soluble PpiD and PpiDΔParv proteins was observed by light scattering at 500 nm.

PpiDΔParv complements the growth defect of an fkpA ppiD surA triple mutant

To provide further in vivo evidence for the existence of a chaperone activity of PpiD we took advantage of a phenotype that has previously been shown to be associated with inactivation of ppiD. Such a phenotype is exhibited by an fkpA ppiD surA triple mutant, which displays growth defects during mid- to late exponential phase in liquid culture, while all double mutant combinations including these genes grow normally [20]. The fkpA gene codes for the periplasmic folding factor FkpA, which like SurA exhibits PPIase and chaperone activity [35, 36]. Our complementation analysis showed that both the SurAN-Ct protein, which only exhibits chaperone activity [2], and PpiDΔParv restore growth of the fkpA ppiD surA mutant as well as intact PpiD (Figure 6). This demonstrates that the growth phenotype of the triple PPIase mutant is not due to loss of PPIase activity but to loss of chaperone function. It also shows that PpiD shares this function with SurA and FkpA. As in SurA, the chaperone activity is carried solely in the non-parvulin regions of the protein (PpiDΔParv).

Figure 6
figure 6

Growth complementation of an fkpA ppiD surA triple mutant. Growth of the fkpA ppiD surA (SB11116; triple), fkpA surA (SB11114), and surA (CAG24029) PPIase mutants and of wild-type (CAG16037) in LB at 37°C was assayed by monitoring the OD600 during shaking culture.

Lack of PpiD confers increased temperature-sensitivity in a degP mutant

The periplasmic protease DegP also acts as a chaperone [15, 37] and the simultaneous lack of DegP and SurA gives a synthetically lethal phenotype [10]. We therefore asked whether similarly a chaperone function of PpiD may be disclosed by the combined deletion of ppiD and degP. DegP-deficient strains display a temperature-sensitive phenotype at temperatures above 37°C [38]. Accordingly, we compared the growth of degP and ppiD single mutants with that of a degP ppiD double mutant at 30, 37, and 42°C (Figure 7). As expected, lack of DegP compromised cell growth above 37°C. In contrast, the ppiD single mutant showed wild-type growth at all temperatures. However, the degP ppiD double mutant was more temperature sensitive than the degP single mutant and grew normally only at 30°C. Thus, degP ppiD mutants show a synthetic conditional phenotype at temperatures greater than 30°C.

Figure 7
figure 7

Inactivation of ppiD confers increased temperature sensitivity in a degP mutant. Growth analysis of wild-type (CAG16037), degP::kan (SB44964), ppiD:: Tn10 (SB44741), and degP::kan ppiD:: Tn10 (SB44970) cells. Cells were grown overnight at 30°C and after dilution spotted on LB plates. Plates were incubated overnight at the indicated temperature.

Discussion

PpiD is a SurA-like multidomain chaperone

To date, four representatives of the three major families of PPIases are known to exist in the periplasm of E. coli: the cyclophilin PpiA [39], the FKBP-like protein FkpA [35], and the parvulin-like proteins PpiD [18] and SurA [6–8]. In addition to PPIase activity, SurA and FkpA also exhibit prolyl isomerase-independent chaperone activity [2, 36] and the major function of SurA in the maturation of the integral β-barrel OMPs actually is that of a chaperone [2]. While PpiD has also been implicated in OMP biogenesis, the biochemical activity required for this function was reported to be a PPIase activity carried in its parvulin domain [40]. A chaperone activity has so far not been demonstrated for either PpiD or PpiA.

In this study we for the first time directly demonstrate, both in vitro and in vivo, that PpiD exhibits a PPIase-independent chaperone activity that resides in the N- and/or C-terminal regions of the protein. The parvulin domain of PpiD is neither required for function in vivo nor for chaperone activity in vitro, as a PpiD protein lacking this domain fully complements the growth defect of an fkpA ppiD surA triple mutant and protects citrate synthase from thermal aggregation even more effectively than wild-type PpiD. In addition, these results show that a catalytic prolyl isomerase activity plays no major role for the function of PpiD in vivo. This conflicts with previous results [40] but is consistent with most recent data showing that the parvulin domain of PpiD is devoid of detectable PPIase activity in vitro[19].

The chaperone function of PpiD is most likely carried in its N-terminal region, which shares sequence similarity with the N-terminal region of SurA (see additional file 1A; [16–18]) and thus with a substantial part of the SurA chaperone module [2]. Model structures of this region of PpiD generated by alignment based as well as by automated three-dimensional homology modeling (see additional file 1, C and D) show some deviation from the crystal structure of the SurA chaperone module mainly in the helix 1-helix 2 and the helix 3-helix 4 interconnecting loop regions. Interestingly, whereas the chaperone module of SurA lacks sequence similarity with the structurally homologous chaperone domain of the E. coli cytosolic Trigger factor (TF) [41], the predicted helix 1-loop-helix 2 region of PpiD shows similarity on the amino acid level with the corresponding region of TF (24.1% identity between regions 43-121 and 295-371 of PpiD and TF, respectively; see additional file 1, B and E).

The similarities in sequence and predicted structure between PpiD, SurA and TF suggest that PpiD contains a conserved SurA-like chaperone module. However, for a complete chaperone active module the region of PpiD that would correspond to the C-terminal helix of SurA still needs to be identified. As an integral element of the conserved module structure this helix is indispensable for the stability and activity of SurA [2, 42] and presumably also of other members of this family of chaperones. The C-terminal helix of SurA was originally identified as the stabilizing region of the protein as it is very basic (predicted isoelectric points of 10.5) as compared to the rather acidic N-terminal region (predicted isoelectric point 5.3) [2]. Similarly, the corresponding helix in the chaperone domain of TF is rather basic as opposed to the rest of the module (predicted isoelectric points of 8.4 and 4.7, respectively). Finally, the N-terminal region of PpiD is acidic too (predicted isoelectric point of 4.7) and therefore the single basic region of the protein which is located in the C-terminal domain (amino acids 511-560, predicted isoelectric point of 10) and is predicted to be rich in α-helical secondary structure, would be a primary candidate for the stabilizing region. Taken together, all indications are that PpiD is a membrane-anchored SurA-like multidomain chaperone, which like SurA combines a conserved chaperone module with an inactive parvulin domain. Different from SurA however, PpiD lacks a second active parvulin domain and instead contains a C-terminal domain, whose function remains to be determined.

Role of PpiD in the periplasm

PpiD was previously reported to be redundant in function with SurA in the maturation of OMPs [18]. Our results however, establish that PpiD plays no major role in the biogenesis of OMPs and that it cannot compensate for lack of SurA in the periplasm. In addition, PpiD differs from SurA in that it requires to be anchored in the inner membrane to function in vivo whereas SurA is functional both in a soluble and in a membrane-anchored state (S. Behrens-Kneip, unpublished results). Then again, ppiD in multicopy suppresses the surA skp caused deficiencies. The strong induction of the σE and Cpx stress pathways during the course of depletion of SurA from Δskp cells is significantly reduced by simultaneous overproduction of PpiD. This suggests that increased levels of PpiD rescue surA skp cells from lethality by counteracting the severe folding stress in the cell envelope which results from the loss of periplasmic chaperone activity. We cannot formally eliminate the possibility that the observed effects result from a response of (an)other known or still to be identified regulatory pathway(s) to increased levels of PpiD in the inner membrane. Such regulatory mechanisms may, for instance, induce periplasmic protease activity that reduces folding stress by protein degradation. However, they would not readily explain our observation that PpiD overproducing surA skp cells contain higher levels of folded forms of OmpA even though they lack two of three chaperones critical for OMP folding. The third OMP chaperone, DegP, appears to interact preferentially with OMPs that already contain substantial levels of folded structure [15] and would thus be expected to predominantly assist in late steps of OMP folding. Moreover, since DegP levels in surA skp cells are reduced by overproduction of PpiD it seems implausible that DegP is responsible for the observed effect on OmpA folding. This, together with our finding that PpiD has chaperone activity in vitro leads us to suggest that PpiD, when present at sufficient levels, is able to partially compensate for the simultaneous loss of SurA and Skp chaperone function.

But why would PpiD promote the folding of OmpA in a surA skp double mutant but have no discernable impact on OMP folding in the respective surA and skp single mutants? We believe that this effect is due to overlapping substrate specificities but yet distinct roles of these chaperones in the periplasm, as has also been suggested for the SurA and Skp chaperones [5, 26]. Both SurA and Skp interact with unfolded major OMPs [2, 43] and facilitate their biogenesis, yet they cannot functionally substitute one another in the cell (Figure 1 and our unpublished data) and are thought to act in parallel pathways of OMP folding [5, 26]. The peptide binding specificity of PpiD has been shown to overlap with that of SurA but to be less specific [44], suggesting that PpiD is capable of interacting with a broader range of substrates. Thus, while unfolded major OMPs obviously are no preferred substrates of PpiD, they may still effectively interact with PpiD for folding in the absence of the competing chaperones SurA and Skp. In this context it is important to mention, that overproduction of PpiD does not restore viability of a surA degP double mutant (S. Behrens-Kneip, unpublished results). This suggests that, when overproduced in surA skp cells, PpiD compensates for the lack of Skp upstream of DegP in the proposed Skp/DegP branch of protein folding rather than for the lack of SurA. The magnitude of suppression of the surA skp phenotypes elicited by multicopy ppiD and the additive phenotypes of the ppiD degP and skp ppiD double mutants described in this work are in support of this notion. Moreover, direct evidence for partially overlapping functions of the membrane-anchored PpiD and the soluble Skp comes from the recent finding that both proteins interact with OMP polypeptides very early during translocation and promote their release from the SecYEG translocation channel [12, 14, 24].

It has recently been proposed that PpiD is a periplasmic gatekeeper of the Sec translocon responsible for newly translocated OMPs [24]. Our work agrees with and refines this assumption, as it shows that PpiD exhibits the requisite chaperone activity for such a function, that this function is not preferentially directed at folding of OMPs, and that PpiD cooperates with SurA, Skp, FkpA and DegP in mediating protein folding in the periplasmic compartment of the cell. We suggest that the role of PpiD is to assist in the initial periplasmic folding events of many newly secreted envelope proteins.

In the cytosol, the folding of newly synthesized proteins is initiated by the ribosome-associated chaperone TF [45, 46]. Of note, PpiD and TF show some interesting analogies. First, similar to PpiD TF is composed of three domains: an N-terminal ribosome-binding domain, a central FKBP-like PPIase domain, and a C-terminal chaperone module which is structurally homologous to the chaperone module of SurA [41, 47] and, as outlined above, shows sequence similarity with the N-terminal putative chaperone region of PpiD. Second, TF associates with the ribosome to sequester and protect polypeptides just as they emerge from the peptide exit tunnel [46] and this association is crucial for its in vivo function [48]. PpiD on the other hand, is anchored in the inner membrane and interacts with newly translocated polypeptides that emerge from the periplasmic exit site of the Sec translocon [24] and according to our data, the anchoring of PpiD in the membrane is required for its function in vivo. Third, TF is dispensable for cell viability and a deletion of the tig gene confers a discernable phenotype only in combination with a mutation of the dnaK gene for the cytosolic chaperone DnaK [45]. Likewise, lack of PpiD gives a discernable phenotype only in cells with already compromised periplasmic chaperone activity, such as in the fkpA ppiD surA triple mutant and in the degP ppiD and ppiD skp double mutants. Finally, the amino acid sequence pattern of known PpiD binding peptides [44] resembles that of the peptide binding motifs identified for the cytosolic chaperones TF and DnaK, consisting of a central patch of hydrophobic amino acids flanked by positively charged amino acids [49]. Altogether, we speculate that PpiD may represent the periplasmic counterpart of TF. Its fixed localization in the inner membrane not necessarily conflicts with such a function, as it may provide a local enrichment of the binding partners but still allows PpiD to dynamically interact with and cycle on and off its interaction partners by lateral diffusion in the membrane, just as it is the hallmark of TF function on translating ribosomes [50]. Further detailed studies on the interaction of PpiD with both the Sec translocation machinery and translocating polypeptides as well as the analysis of the structure-function relationship in PpiD are needed to ascertain its real function in the periplasm.

Conclusions

This study for the first time directly demonstrates that PpiD functions as a chaperone and that its previous classification as a folding factor for OMPs must be revised. PpiD appears to belong to the SurA-like family of chaperones but different from SurA it plays no major role in the maturation of OMPs. A biochemical capability of PpiD to also assist the folding of OMPs becomes relevant only in the absence of both chaperones for unfolded OMPs, SurA and Skp. In addition, the role of PpiD in the periplasm appears to be restricted to folding events that take place in close proximity to the inner membrane, as only membrane-anchored PpiD functions in vivo. Taken together, our data are in line with the recently proposed role of PpiD as a periplasmic gatekeeper of the Sec translocon [24], as they suggest that it acts as a chaperone for initial folding events of many newly exported proteins. We speculate that PpiD may have a role at the periplasmic exit site of the Sec translocon similar to that of TF at the exit site of the translating ribosome.

Methods

Media and growth conditions

Luria-Bertani (LB) media were prepared as described [51]. Ampicillin (Ap), chloramphenicol (Cm), kanamycin (Kan), spectinomycin (Spec), and tetracycline (Tc) were used at final concentrations of 100, 20, 30, 50 and 10 μg ml-1, respectively. For assaying β-galactosidase activity in cpxP-lacZ reporter strains the medium was buffered with 100 mM sodium phosphate to a pH of 7.0, at which cpxP transcription, which is affected by extracellular alkaline pH, is induced to a medium level [57]. Strains were grown at 37°C with aeration unless noted otherwise.

Strains

Strains used in this work are listed in Table 2. Mutant alleles were moved into the appropriate strains either by general transduction using phage T4-GT7[52] or by P1 transduction [53]. The presence of the mutant alleles in recombinants was verified by PCR. To generate SurA-depletion strains the chromosomal surA gene was placed under the control of the IPTG-inducible promoter P Llac-O1 [23] by gene replacement as described previously [54]. A ~3.1 kb DNA fragment bearing an Ω:: spectinomycin-P Llac-O1 fusion flanked by approximately 500 bp of imp and surA sequence, respectively, was obtained from pΩSurA by cleavage with Eco RI and partial digest with Hin dIII. E. coli KM22 was electroporated with the purified fragment. Recombinants were selected on LB/Spec and used as donors for transduction of the Ω::spec-P Llac-O1 -surA locus into the appropriate strains. The final Ω::spec-P Llac-O1 -surA strains were transformed with pPLT13 to provide the LacI repressor protein.

Table 2 Strains used in this study

Plasmids

Plasmids used in this study are listed in Table 3. To make pΩSurA, the sequences flanking the Ω::spec-P Llac-O1 cassette in plasmid pBA106 [55] were replaced by portions of the imp-surA locus corresponding to nucleotides -581 to -35 (imp3', 497 bp) and nucleotides -26 to 508 (surAN, 534 bp), respectively, relative to the surA translational start codon. Fragment imp3' was amplified by PCR from purified MC1061 genomic DNA using the primers 5'-GGATTGCGTGGCGGAATTCAGTACG-3' and 5'-ACCGCACTGCGGATCCCGTGGTAAATC-3'. The Eco RI/Bam HI-cleaved product was ligated into the corresponding sites of pBA106. Subsequently, the surAN fragment was obtained from pSurAN [2] by Nco I/Hin dIII cleavage and cloned into the corresponding sites downstream of Ω::spec-P Llac-O1 in the above intermediate. pASKSurAN-Ct was constructed by cloning a Pst I/Bgl II fragment of pSurAN-Ct [2] into the corresponding sites of pASKSurA [2]. To yield pPpiD, the ppiD gene and its promoter region was PCR amplified from the MC1061 chromosome using the primers 5'-GTGCTGCCCATATGGGCCGCAACCCG-3'and 5'-TTTTGCGAGGAAGCTTCAGGA TTATTGC-3'. The PCR fragment was cleaved with Nde I/Hin dIII and cloned into the Nde I and Hin dIII sites of pTrc99a, thereby removing the plasmid encoded lacIq gene and P trc promoter sequences. Plasmids pPpiDG347A and pPpiDI350A were created by replacing the codons 347 and 350 of ppiD to codons for alanine by QuikChange site directed mutagenesis (Stratagene, La Jolla, CA) using the primer pair 5'-CAAATCTTCGGTCGCTTTCCTG-3'/5'-CAGGAAAGCGACCGAAGATTTG-3' and 5'-CGGTTTCCTGGCTGTACGTCTGG-3'/5'-CCAGACGTACAGCCAGGAAACC-3', respectively. Plasmid pPpiDΔ69-201 was made by deletion of a Pvu I/Hpa I fragment from pPpiD. pPpiDΔParv was constructed as follows: a second Eco RV site was introduced at nucleotides 1062-1068 of ppiD by QuikChange mutagenesis of pPpiD using primers 5'-GTCTGGACGATATCCAGCCAGCGAAAG-3' and 5'-CTTTCGCTGGCTGGATATCGTCCAGAC-3'. In the resulting plasmid, the parvulin domain encoding sequence of ppiD was flanked by Eco RV sites. Deletion of the Eco RV fragment resulted in pPpiDΔParv. Plasmid pPpiDfs601 was made by cleavage of pPpiD with Kpn I, removal of the resulting 3'-overhangs with DNA polymerase I Klenow fragment, and subsequent ligation. Plasmid pASKssPpiD for the production of a soluble periplasmic N-terminally hexa-His-tagged PpiD protein was constructed in three steps. First, a Bam HI site was introduced at codons 33-34 of ppiD by QuikChange mutagenesis of pPpiD using primers 5'-GCGTGAGTGGATCCCTGATTGGCGGA-3' and 5'-TCCGCCAATCAGGGATCCACTCACGC-3'. Second, the Bam HI/Hin dIII fragment of the resulting plasmid, encoding PpiD without the transmembrane segment, was cloned into the Bam HI/Hin dIII sites of a pASKSurA plasmid that carried a Sac I site at codons 22-23 of surA[2]. Third, the 5'-phosphorylated oligonucleotides 5'-CCATCACCATCACCATCACG-3' and 5'-GATCCGTGATGGTGATGGTGATGGAGCT-3' were annealed and cloned into Sac I/Bam HI of the above intermediate, thereby placing a hexa-His sequence between the signal peptide sequence of surA and codons 34 to 623 of ppiD. To make pASKssPpiDΔParv, the Sph I/Pst I fragment of pASKssPpiD bearing the parvulin domain encoding sequence was replaced by a Sph I/Pst I fragment derived from plasmid pPpiDΔParv. To make pPpiDΔTM, a 1350 bp-fragment carrying the surA signal sequence-his 6 -ppiD fusion was PCR amplified from pASKssPpiD using primers 5'-CATTGATAGAGTTACGTAACCACTCCC-3' and 5'-CACTTTCTGCTGCAGCGCG-3'. The product was cleaved with Sna BI/Pst I and cloned into the Stu I and Pst I sites of pPpiD. To create plasmid pSkp, a 1722 bp Xho I/Nde I fragment derived from plasmid pMP1 was cloned into the corresponding sites of pQE60 thereby removing the plasmid-encoded P T5 /O lac promoter/operator sequences. All plasmid sequences were confirmed by DNA sequencing.

Table 3 Plasmids used in this study

Assay of susceptibility to SDS/EDTA

The sensitivity of the strains to SDS/EDTA was determined in plating assays as previously described [2]. The efficiency of plating was calculated from the colony count after incubation at 37°C for 24-48 h. A minimum of three experiments were performed for each strain and condition.

Spot dilution assays

SurA-depletion strains were freshly transformed with the required plasmids and were grown overnight at 37°C in selective LB containing 1 mM IPTG. Overnight cultures were adjusted to an optical density at 600 nm (OD600) of 4.0 and 10-fold serially diluted with IPTG-free LB. Ten microlitres of the 10-1, 10-3, 10-5, and 10-7 dilutions were spotted on LB ± 1 mM IPTG plates supplemented with the appropriate antibiotics and incubated at 37°C for 16-24 h. To test for temperature sensitivity, strains were grown overnight at 30°C in LB and were diluted and spotted on LB plates as described above.

SurA depletion in vivo

SB44452 or SB44997 were freshly transformed with the appropriate plasmids and grown overnight at 37°C in LB/Ap/Kan/Spec (buffered at a pH of 7.0, if required) supplemented with 1 mM IPTG and 0.2% (w/v) maltose to induce expression of the maltoporin LamB. Two milliliters of each overnight culture were pelleted in a microcentrifuge and were washed three times in 2 ml of LB to remove IPTG from the cells. The washed cultures were then diluted to an OD600 of 0.01 into 50 ml of LB/Ap/Kan ± 1 mM IPTG. These pre-cultures were grown for 4-5 cell generations with shaking in a gyratory water bath at 37°C and diluted into fresh LB/Ap/Kan ± 1 mM IPTG to an OD600 of 0.005. Aliquots were sampled for β-galactosidase assays, for western blot analysis, and for the preparation of OmpA folding intermediates at the indicated time points after the second sub-culturing and processed as described below.

β-galactosidase assays

EσE and Cpx pathway activities were assayed by monitoring the β-galactosidase activity resulting from the expression of the chromosomal σE- and Cpx-dependent reporter fusions rpoH P3::lacZ[56] and cpxP-lacZ[57], respectively, in cells growing in LB medium (buffered at pH 7.0 for Cpx assays) at 37°C. Overnight cultures were diluted to an OD600 of 0.005 into fresh media and grown with shaking in a gyratory water bath at 37°C. Duplicate samples (0.5 ml) were taken throughout the early exponential phase of the growth curve (OD600 = 0.08-0.4) and β-galactosidase activity was measured by the standard assay [53]. EσE and Cpx activities shown in Figure 1 were determined from the slope on the line of a differential plot of β-galactosidase activity in 0.5 ml of culture versus OD600 and normalized to the wild-type case. In Figure 3, the average β-galactosidase activity/OD600 (Miller Units) was calculated and normalized to that of wild-type. Statistical analysis was performed using a Student's t-test.

Western blot analysis

Whole cell extracts were prepared by resuspending cells in urea protein sample buffer (8 M urea, 200 mM Tris-Base, 200 mM DTT, 2% SDS, 0.02% bromphenol blue) followed by short sonication and heating of the sample to 95°C for 10 min. Extracts from equal numbers of cells were run on SDS-polyacrylamide gels and transferred to nitrocellulose membranes. The membranes were probed with dilutions of rabbit polyclonal antisera raised against SurA (1:10 000), PpiD (1:10 000), DegP (1:20 000), Hsc66 (1:20 000), LamB (1:3000), and with mouse monoclonal antibodies raised against OmpA (1:500), respectively. Alkaline phosphatase conjugated goat anti-rabbit and anti-mouse IgGs (Sigma, 1.10 000 dilutions), respectively, served as secondary antibodies. They were visualized by incubating the blots in reaction buffer (100 mM Tris-HCl, pH 8.8, 100 mM NaCl, 5 mM MgCl2, 37.5 μg/ml nitro blue tetrazolium, 150 μg/ml 5-bromo-4-chloro-3-indolyl phosphate). Signal intensities were quantified using ImageJ software http://rsb.info.nih.gov/ij/. Hsc66 and MalE were used as the internal standard for each lane. Experiments were repeated a minimum of two times for each strain and condition, and data for one representative experiment are shown.

Preparation of OmpA folding intermediates

During the course of SurA depletion, samples corresponding to an equal number of cells were harvested by centrifugation and immediately frozen in a dry ice/ethanol bath. Folded and unfolded OmpA folding intermediates were isolated by gentle lysis as previously described [33]. Samples were mixed with protein sample buffer (3% SDS, 10% glycerol, 5% β-mercaptoethanol in 70 mM Tris, HCl, pH 6.8), heated to 37°C for 10 min and loaded onto 12.5% SDS-polyacrylamide gels. Electrophoresis was performed at 50 V and OmpA intermediates were detected by Western blot analysis as described above.

Protein purification

N-terminally His6-tagged PpiD proteins and C-terminally His6-tagged SurA were produced in E. coli CAG44102 from pASKssPpiD, pASKssPpiDΔParv and pASKSurA, respectively, and purified from the periplasmic fraction by affinity chromatography on Ni2+-chelating sepharose as previously described [2]. Protein concentrations were determined by UV absorbance at 280 nm using absorption coefficients of 36 270 M-1 cm-1, 26 740 M-1 cm-1 and 29 450 M-1 cm-1 for His6-PpiD, His6-PpiDΔParv and SurA-His6, respectively, as calculated according to [58].

Analysis of chaperone function in vitro

Effects of PpiD proteins on the thermal aggregation of citrate synthase were determined according to [34]. Aggregation was monitored on a Hitachi F-4500 spectrofluorometer with both excitation and emission wavelengths set to 500 nm at a spectral bandwidth of 2.5 nm. Data points were recorded every 0.5 s.

References

  1. Wu T, Malinverni J, Ruiz N, Kim S, Silhavy TJ, Kahne D: Identification of a multicomponent complex required for outer membrane biogenesis in Escherichia coli. Cell. 2005, 121 (2): 235-245. 10.1016/j.cell.2005.02.015.

    Article  CAS  PubMed  Google Scholar 

  2. Behrens S, Maier R, de Cock H, Schmid FX, Gross CA: The SurA periplasmic PPIase lacking its parvulin domains functions in vivo and has chaperone activity. The EMBO journal. 2001, 20 (1-2): 285-294. 10.1093/emboj/20.1.285.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  3. Bitto E, McKay DB: The periplasmic molecular chaperone protein SurA binds a peptide motif that is characteristic of integral outer membrane proteins. The Journal of biological chemistry. 2003, 278 (49): 49316-49322. 10.1074/jbc.M308853200.

    Article  CAS  PubMed  Google Scholar 

  4. Hennecke G, Nolte J, Volkmer-Engert R, Schneider-Mergener J, Behrens S: The periplasmic chaperone SurA exploits two features characteristic of integral outer membrane proteins for selective substrate recognition. The Journal of biological chemistry. 2005, 280 (25): 23540-23548. 10.1074/jbc.M413742200.

    Article  CAS  PubMed  Google Scholar 

  5. Vertommen D, Ruiz N, Leverrier P, Silhavy TJ, Collet JF: Characterization of the role of the Escherichia coli periplasmic chaperone SurA using differential proteomics. Proteomics. 2009, 9 (9): 2432-2443. 10.1002/pmic.200800794.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  6. Rouviére PE, Gross CA: SurA, a periplasmic protein with peptidyl-prolyl isomerase activity, participates in the assembly of outer membrane porins. Genes & development. 1996, 10 (24): 3170-3182.

    Article  Google Scholar 

  7. Missiakas D, Betton JM, Raina S: New components of protein folding in extracytoplasmic compartments of Escherichia coli SurA, FkpA and Skp/OmpH. Molecular microbiology. 1996, 21 (4): 871-884. 10.1046/j.1365-2958.1996.561412.x.

    Article  CAS  PubMed  Google Scholar 

  8. Lazar SW, Kolter R: SurA assists the folding of Escherichia coli outer membrane proteins. Journal of Bacteriology. 1996, 178 (6): 1770-1773.

    PubMed Central  CAS  PubMed  Google Scholar 

  9. Raivio TL, Silhavy TJ: The sigmaE and Cpx regulatory pathways: overlapping but distinct envelope stress responses. Current opinion in microbiology. 1999, 2 (2): 159-165. 10.1016/S1369-5274(99)80028-9.

    Article  CAS  PubMed  Google Scholar 

  10. Rizzitello AE, Harper JR, Silhavy TJ: Genetic evidence for parallel pathways of chaperone activity in the periplasm of Escherichia coli. Journal of Bacteriology. 2001, 183 (23): 6794-6800. 10.1128/JB.183.23.6794-6800.2001.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  11. De Cock H, Schafer U, Potgeter M, Demel R, Muller M, Tommassen J: Affinity of the periplasmic chaperone Skp of Escherichia coli for phospholipids, lipopolysaccharides and non-native outer membrane proteins. Role of Skp in the biogenesis of outer membrane protein. European journal of biochemistry/FEBS. 1999, 259 (1-2): 96-103. 10.1046/j.1432-1327.1999.00010.x.

    Article  CAS  PubMed  Google Scholar 

  12. Schäfer U, Beck K, Müller M: Skp, a molecular chaperone of gram-negative bacteria, is required for the formation of soluble periplasmic intermediates of outer membrane proteins. The Journal of biological chemistry. 1999, 274 (35): 24567-24574. 10.1074/jbc.274.35.24567.

    Article  PubMed  Google Scholar 

  13. Bulieris PV, Behrens S, Holst O, Kleinschmidt JH: Folding and insertion of the outer membrane protein OmpA is assisted by the chaperone Skp and by lipopolysaccharide. The Journal of biological chemistry. 2003, 278 (11): 9092-9099. 10.1074/jbc.M211177200.

    Article  CAS  PubMed  Google Scholar 

  14. Harms N, Koningstein G, Dontje W, Muller M, Oudega B, Luirink J, de Cock H: The early interaction of the outer membrane protein PhoE with the periplasmic chaperone Skp occurs at the cytoplasmic membrane. The Journal of biological chemistry. 2001, 276 (22): 18804-18811. 10.1074/jbc.M011194200.

    Article  CAS  PubMed  Google Scholar 

  15. Krojer T, Sawa J, Schafer E, Saibil HR, Ehrmann M, Clausen T: Structural basis for the regulated protease and chaperone function of DegP. Nature. 2008, 453 (7197): 885-890. 10.1038/nature07004.

    Article  CAS  PubMed  Google Scholar 

  16. Matern Y, Barion B, Behrens-Kneip S: The Escherichia coli peptidyl-prolyl isomerase PpiD - the periplasmic trigger factor for newly-translocated proteins?. BioSpectrum, Abstracts Annual meeting of the VAAM. 2009

    Google Scholar 

  17. Matern Y, Behrens-Kneip S: Genetic analysis of the functional interplay between SurA, Skp and PpiD in the maturation of outer membrane proteins in Escherichia coli. BioSpectrum, Abstracts Annual meeting of the VAAM. 2007

    Google Scholar 

  18. Dartigalongue C, Raina S: A new heat-shock gene, ppiD, encodes a peptidyl-prolyl isomerase required for folding of outer membrane proteins in Escherichia coli. The EMBO journal. 1998, 17 (14): 3968-3980. 10.1093/emboj/17.14.3968.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  19. Weininger U, Jakob RP, Kovermann M, Balbach J, Schmid FX: The prolyl isomerase domain of PpiD from Escherichia coli shows a parvulin fold but is devoid of catalytic activity. Protein Sci. 19 (1): 6-18.

  20. Justice SS, Hunstad DA, Harper JR, Duguay AR, Pinkner JS, Bann J, Frieden C, Silhavy TJ, Hultgren SJ: Periplasmic peptidyl prolyl cis-trans isomerases are not essential for viability, but SurA is required for pilus biogenesis in Escherichia coli. Journal of Bacteriology. 2005, 187 (22): 7680-7686. 10.1128/JB.187.22.7680-7686.2005.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  21. Price NL, Raivio TL: Characterization of the Cpx regulon in Escherichia coli strain MC4100. Journal of Bacteriology. 2009, 191 (6): 1798-1815. 10.1128/JB.00798-08.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  22. Hung DL, Raivio TL, Jones CH, Silhavy TJ, Hultgren SJ: Cpx signaling pathway monitors biogenesis and affects assembly and expression of P pili. The EMBO journal. 2001, 20 (7): 1508-1518. 10.1093/emboj/20.7.1508.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  23. Lutz R, Bujard H: Independent and tight regulation of transcriptional units in Escherichia coli via the LacR/O, the TetR/O and AraC/I1-I2 regulatory elements. Nucleic acids research. 1997, 25 (6): 1203-1210. 10.1093/nar/25.6.1203.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  24. Antonoaea R, Furst M, Nishiyama K, Müller M: The periplasmic chaperone PpiD interacts with secretory proteins exiting from the SecYEG translocon. Biochemistry. 2008, 47 (20): 5649-5656. 10.1021/bi800233w.

    Article  CAS  PubMed  Google Scholar 

  25. Sklar JG, Wu T, Gronenberg LS, Malinverni JC, Kahne D, Silhavy TJ: Lipoprotein SmpA is a component of the YaeT complex that assembles outer membrane proteins in Escherichia coli. Proceedings of the National Academy of Sciences of the United States of America. 2007, 104 (15): 6400-6405. 10.1073/pnas.0701579104.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  26. Sklar JG, Wu T, Kahne D, Silhavy TJ: Defining the roles of the periplasmic chaperones SurA, Skp, and DegP in Escherichia coli. Genes & development. 2007, 21 (19): 2473-2484.

    Article  CAS  Google Scholar 

  27. Danese PN, Snyder WB, Cosma CL, Davis LJ, Silhavy TJ: The Cpx two-component signal transduction pathway of Escherichia coli regulates transcription of the gene specifying the stress-inducible periplasmic protease, DegP. Genes & development. 1995, 9 (4): 387-398.

    Article  CAS  Google Scholar 

  28. Raina S, Missiakas D, Georgopoulos C: The rpoE gene encoding the sigma E (sigma 24) heat shock sigma factor of Escherichia coli. The EMBO journal. 1995, 14 (5): 1043-1055.

    PubMed Central  CAS  PubMed  Google Scholar 

  29. Snyder WB, Davis LJ, Danese PN, Cosma CL, Silhavy TJ: Overproduction of NlpE, a new outer membrane lipoprotein, suppresses the toxicity of periplasmic LacZ by activation of the Cpx signal transduction pathway. Journal of Bacteriology. 1995, 177 (15): 4216-4223.

    PubMed Central  CAS  PubMed  Google Scholar 

  30. De Wulf P, McGuire AM, Liu X, Lin EC: Genome-wide profiling of promoter recognition by the two-component response regulator CpxR-P in Escherichia coli. The Journal of biological chemistry. 2002, 277 (29): 26652-26661. 10.1074/jbc.M203487200.

    Article  CAS  PubMed  Google Scholar 

  31. Vogel J, Papenfort K: Small non-coding RNAs and the bacterial outer membrane. Current opinion in microbiology. 2006, 9 (6): 605-611. 10.1016/j.mib.2006.10.006.

    Article  CAS  PubMed  Google Scholar 

  32. Schweizer M, Hindennach I, Garten W, Henning U: Major proteins of the Escherichia coli outer cell envelope membrane. Interaction of protein II with lipopolysaccharide. European journal of biochemistry/FEBS. 1978, 82 (1): 211-217. 10.1111/j.1432-1033.1978.tb12013.x.

    Article  CAS  PubMed  Google Scholar 

  33. Misra R, Peterson A, Ferenci T, Silhavy TJ: A genetic approach for analyzing the pathway of LamB assembly into the outer membrane of Escherichia coli. The Journal of biological chemistry. 1991, 266 (21): 13592-13597.

    CAS  PubMed  Google Scholar 

  34. Buchner J, Grallert H, Jakob U: Analysis of chaperone function using citrate synthase as nonnative substrate protein. Methods in enzymology. 1998, 290: 323-338. full_text.

    Article  CAS  PubMed  Google Scholar 

  35. Horne SM, Young KD: Escherichia coli and other species of the Enterobacteriaceae encode a protein similar to the family of Mip-like FK506-binding proteins. Archives of microbiology. 1995, 163 (5): 357-365. 10.1007/BF00404209.

    Article  CAS  PubMed  Google Scholar 

  36. Ramm K, Plückthun A: The periplasmic Escherichia coli peptidylprolyl cis,trans-isomerase FkpA. II. Isomerase-independent chaperone activity in vitro. The Journal of biological chemistry. 2000, 275 (22): 17106-17113. 10.1074/jbc.M910234199.

    Article  CAS  PubMed  Google Scholar 

  37. Spiess C, Beil A, Ehrmann M: A temperature-dependent switch from chaperone to protease in a widely conserved heat shock protein. Cell. 1999, 97 (3): 339-347. 10.1016/S0092-8674(00)80743-6.

    Article  CAS  PubMed  Google Scholar 

  38. Lipinska B, Fayet O, Baird L, Georgopoulos C: Identification, characterization, and mapping of the Escherichia coli htrA gene, whose product is essential for bacterial growth only at elevated temperatures. Journal of Bacteriology. 1989, 171 (3): 1574-1584.

    PubMed Central  CAS  PubMed  Google Scholar 

  39. Liu J, Walsh CT: Peptidyl-prolyl cis-trans-isomerase from Escherichia col i: a periplasmic homolog of cyclophilin that is not inhibited by cyclosporin A. Proceedings of the National Academy of Sciences of the United States of America. 1990, 87 (11): 4028-4032. 10.1073/pnas.87.11.4028.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  40. Dartigalongue C, Missiakas D, Raina S: Characterization of the Escherichia coli sigma E regulon. The Journal of biological chemistry. 2001, 276 (24): 20866-20875. 10.1074/jbc.M100464200.

    Article  CAS  PubMed  Google Scholar 

  41. Merz F, Hoffmann A, Rutkowska A, Zachmann-Brand B, Bukau B, Deuerling E: The C-terminal domain of Escherichia coli trigger factor represents the central module of its chaperone activity. The Journal of biological chemistry. 2006, 281 (42): 31963-31971. 10.1074/jbc.M605164200.

    Article  CAS  PubMed  Google Scholar 

  42. Bitto E, McKay DB: Crystallographic structure of SurA, a molecular chaperone that facilitates folding of outer membrane porins. Structure. 2002, 10 (11): 1489-1498. 10.1016/S0969-2126(02)00877-8.

    Article  CAS  PubMed  Google Scholar 

  43. Chen R, Henning U: A periplasmic protein (Skp) of Escherichia coli selectively binds a class of outer membrane proteins. Molecular microbiology. 1996, 19 (6): 1287-1294. 10.1111/j.1365-2958.1996.tb02473.x.

    Article  CAS  PubMed  Google Scholar 

  44. Stymest KH, Klappa P: The periplasmic peptidyl prolyl cis-trans isomerases PpiD and SurA have partially overlapping substrate specificities. The FEBS journal. 2008, 275 (13): 3470-3479. 10.1111/j.1742-4658.2008.06493.x.

    Article  CAS  PubMed  Google Scholar 

  45. Deuerling E, Schulze-Specking A, Tomoyasu T, Mogk A, Bukau B: Trigger factor and DnaK cooperate in folding of newly synthesized proteins. Nature. 1999, 400 (6745): 693-696. 10.1038/23301.

    Article  CAS  PubMed  Google Scholar 

  46. Maier T, Ferbitz L, Deuerling E, Ban N: A cradle for new proteins: trigger factor at the ribosome. Current opinion in structural biology. 2005, 15 (2): 204-212. 10.1016/j.sbi.2005.03.005.

    Article  CAS  PubMed  Google Scholar 

  47. Hesterkamp T, Deuerling E, Bukau B: The amino-terminal 118 amino acids of Escherichia coli trigger factor constitute a domain that is necessary and sufficient for binding to ribosomes. The Journal of biological chemistry. 1997, 272 (35): 21865-21871. 10.1074/jbc.272.35.21865.

    Article  CAS  PubMed  Google Scholar 

  48. Kramer G, Rauch T, Rist W, Vorderwulbecke S, Patzelt H, Schulze-Specking A, Ban N, Deuerling E, Bukau B: L23 protein functions as a chaperone docking site on the ribosome. Nature. 2002, 419 (6903): 171-174. 10.1038/nature01047.

    Article  CAS  PubMed  Google Scholar 

  49. Deuerling E, Patzelt H, Vorderwulbecke S, Rauch T, Kramer G, Schaffitzel E, Mogk A, Schulze-Specking A, Langen H, Bukau B: Trigger Factor and DnaK possess overlapping substrate pools and binding specificities. Molecular microbiology. 2003, 47 (5): 1317-1328. 10.1046/j.1365-2958.2003.03370.x.

    Article  CAS  PubMed  Google Scholar 

  50. Kaiser CM, Chang HC, Agashe VR, Lakshmipathy SK, Etchells SA, Hayer-Hartl M, Hartl FU, Barral JM: Real-time observation of trigger factor function on translating ribosomes. Nature. 2006, 444 (7118): 455-460. 10.1038/nature05225.

    Article  CAS  PubMed  Google Scholar 

  51. Sambrook J, Fritsch E, Maniatis T:Molecular Cloning: A Laboratory Manual. Cold Spring Harbor. 1989, New York: Cold Spring Harbor Laboratory Press,

    Google Scholar 

  52. Wilson GG, Young KY, Edlin GJ, Konigsberg W: High-frequency generalised transduction by bacteriophage T4. Nature. 1979, 280 (5717): 80-82. 10.1038/280080a0.

    Article  CAS  PubMed  Google Scholar 

  53. Miller JH, (ed): Experiments in Molecular Genetics. Cold Spring Harbor. 1972, New York: Cold Spring Harbor Laboratory Press

  54. Murphy KC: Use of bacteriophage lambda recombination functions to promote gene replacement in Escherichia coli. Journal of Bacteriology. 1998, 180 (8): 2063-2071.

    PubMed Central  CAS  PubMed  Google Scholar 

  55. Alba BM, Zhong HJ, Pelayo JC, Gross CA: degS (hhoB) is an essential Escherichia coli gene whose indispensable function is to provide sigma (E) activity. Molecular microbiology. 2001, 40 (6): 1323-1333. 10.1046/j.1365-2958.2001.02475.x.

    Article  CAS  PubMed  Google Scholar 

  56. Mecsas J, Rouviere PE, Erickson JW, Donohue TJ, Gross CA: The activity of sigma E, an Escherichia coli heat-inducible sigma-factor, is modulated by expression of outer membrane proteins. Genes & development. 1993, 7 (12B): 2618-2628.

    Article  CAS  Google Scholar 

  57. Danese PN, Silhavy TJ: CpxP, a stress-combative member of the Cpx regulon. Journal of Bacteriology. 1998, 180 (4): 831-839.

    PubMed Central  CAS  PubMed  Google Scholar 

  58. Pace CN, Vajdos F, Fee L, Grimsley G, Gray T: How to measure and predict the molar absorption coefficient of a protein. Protein Sci. 1995, 4 (11): 2411-2423. 10.1002/pro.5560041120.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  59. Baba T, Ara T, Hasegawa M, Takai Y, Okumura Y, Baba M, Datsenko KA, Tomita M, Wanner BL, Mori H: Construction of Escherichia coli K-12 in-frame, single-gene knockout mutants: the Keio collection. Molecular systems biology. 2006, 2: 10.1038/msb4100050. 2006 0008

    Google Scholar 

  60. Skerra A: Use of the tetracycline promoter for the tightly regulated production of a murine antibody fragment in Escherichia coli. Gene. 1994, 151 (1-2): 131-135. 10.1016/0378-1119(94)90643-2.

    Article  CAS  PubMed  Google Scholar 

  61. Tavormina PL, Reznikoff WS, Gross CA: Identifying interacting regions in the beta subunit of Escherichia coli RNA polymerase. Journal of molecular biology. 1996, 258 (2): 213-223. 10.1006/jmbi.1996.0244.

    Article  CAS  PubMed  Google Scholar 

  62. Blattner FR, Plunkett G, Bloch CA, Perna NT, Burland V, Riley M, Collado-Vides J, Glasner JD, Rode CK, Mayhew GF: The complete genome sequence of Escherichia coli K-12. Science (New York, NY). 1997, 277 (5331): 1453-1474. 10.1126/science.277.5331.1453.

    Article  CAS  Google Scholar 

  63. Larkin MA, Blackshields G, Brown NP, Chenna R, McGettigan PA, McWilliam H, Valentin F, Wallace IM, Wilm A, Lopez R: Clustal W and Clustal X version 2.0. Bioinformatics (Oxford, England). 2007, 23 (21): 2947-2948. 10.1093/bioinformatics/btm404.

    Article  CAS  Google Scholar 

  64. Huang XQ, Miller W: A Time-Efficient, Linear-Space Local Similarity Algorithm. Advances in Applied Mathematics. 1991, 12 (3): 337-357. 10.1016/0196-8858(91)90017-D.

    Article  Google Scholar 

  65. Arnold K, Bordoli L, Kopp J, Schwede T: The SWISS-MODEL workspace: a web-based environment for protein structure homology modelling. Bioinformatics (Oxford, England). 2006, 22 (2): 195-201. 10.1093/bioinformatics/bti770.

    Article  CAS  Google Scholar 

  66. Bates PA, Kelley LA, MacCallum RM, Sternberg MJ: Enhancement of protein modeling by human intervention in applying the automatic programs 3D-JIGSAW and 3D-PSSM. Proteins. 2001, 39-46. 10.1002/prot.1168. Suppl 5

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Acknowledgements

We thank C.A. Gross for providing strains and plasmids, D. Kahne and T. Silhavy for sharing strains, M. Ehrmann for the gift of plasmids and antibodies, and A. Charbit, E. Deuerling, B. Bukau, and K. Williams for providing antibodies. We also thank W. Kramer for helpful discussions. The work was supported by grants of the DFG to S.B.

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Correspondence to Susanne Behrens-Kneip.

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Authors' contributions

YM analyzed the effect of a ppiD deletion and of multicopy ppiD on cell envelope phenotypes. BB constructed SurA-depletion strains and performed first depletion experiments. SB designed and conceived the study, conducted the SurA depletion studies, analyzed results and wrote the manuscript. All authors read and approved the final manuscript.

Yvonne Matern, Birgitta Barion contributed equally to this work.

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12866_2010_1207_MOESM1_ESM.PDF

Additional file 1:Similarity between the N-terminal region of PpiD and the chaperone modules of SurA and Trigger factor (TF). (A and B) The N-terminal region of PpiD shows sequence similarity with the N- and C-terminal regions of SurA (A, 25.2% identity) and TF (B, 19.9% identity), respectively. The sequence alignments were generated with CLUSTALW2 [63]. Gray shaded regions indicate the regions of high similarity that were initially identified with LALIGN [64] (31.1% (A) and 24.1% (B) identity, respectively). Identical amino acid residues are indicated by asterisks; conserved and semi-conserved residues are marked with colons and dots, respectively. (C-E) Three-dimensional homology modeling suggests structural similarity of the N-terminal region of PpiD with the chaperone modules of SurA and TF. All structures were visualized in PyMol and are depicted in ribbon representation. (C) Comparative model structure of the N-terminal region of PpiD (red colored) and the N-Ct chaperone module of SurA (blue colored) based on the sequence alignment shown in (A). The model was generated in the Swiss-Model workspace [65] using the structure coordinates of SurA (PDB 1m5y; [42]) as a template. Helices of the N-terminal region of SurA are numbered. A region of PpiD that corresponds to the C-terminal helix ("C helix") of SurA has not yet been identified. (D) Model structure of the N-terminal region of PpiD generated by the automatic program 3D-JIGSAW [66]. (E) Fold of the C-terminal chaperone domain of TF (PDB code 1w26; [41]). The region that shares similarity with PpiD is highlighted in red (corresponding to the gray shaded sequence in (B)). (PDF 257 KB)

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Additional file 2:Complementation of the growth defect of ppiD skp surA cells by wild-type PpiD and its PPIase domain mutants. Growth of the SurA-depletion strain P Llac-O1 -surA Δskp ppiD::kan (SB44961) carrying the empty vector pASK75 or plasmids encoding wild-type proteins and variants of SurA, Skp, and PpiD, respectively. Cells were grown overnight in the presence of IPTG and after dilution spotted on LB plates ± 1 mM IPTG. Plates were incubated at 37°C for 16-24 h. (PDF 88 KB)

12866_2010_1207_MOESM3_ESM.PDF

Additional file 3:Effects of NlpE overproduction in surA skp cells. (A) Growth of the SurA-depletion strains P Llac-O1 -surA (SB11019) and P Llac-O1 -surA Δskp (SB44997) at 37°C in buffered LB (pH 7.0) with (solid lines) and without (dotted lines) IPTG, resulting in the indicated wild-type (WT), surA, skp and surA skp "genotypes". Strains carried pASK75 (empty vector) or plasmids encoding PpiD and NlpE, respectively. (B) Within the indicated interval (box in panel A) samples were taken and assayed for the activities of σE and Cpx by monitoring β-galactosidase activity resulting from chromosomal rpoH P3::lacZ and cpxP-lacZ reporter fusions, respectively (see Methods). Results represent the average of at least two independent experiments. (C) Western blot detection of SurA in P Llac-O1 -surA strains after 265- and 360-minute growth as described in A. Extracts from 4 × 107 cells were loaded onto each lane. Signal intensities were calculated using Hsc66 as the internal standard for each lane and are shown relative to those in the wild-type strain (rel. Int.). P Llac-O1 -surA Δskp cells that carried pASK75 or pNlpE resumed production of SurA after 265-minute growth without IPTG. At about the same time, these cultures also resumed growth (see panel A). The onset of regained SurA production and revived growth varied between growth experiments (data not shown), suggesting that the cultures contained a small population of the cells that was still capable of producing SurA, possibly due to a promoter mutation, and that eventually outgrew the SurA-depleted Δskp cell population. In contrast, SurA was hardly detectable during the entire course of growth of PpiD overproducing surA Δskp cells. (D) Growth of the strain P Llac-O1 -surA Δskp (SB44997) carrying pASK75 or plasmids encoding SurA, PpiD, and NlpE, respectively. Cells were grown overnight in the presence of IPTG, after dilution spotted on LB plates ± 1 mM IPTG, and incubated at 37°C for 16-24 h. (PDF 143 KB)

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Additional file 4:Effects of ppiD and nlpE overexpression on the surA skp growth and stress response phenotypes. Table summarizing the levels of suppression of the growth defect and the σE and Cpx phenotypes of surA skp cells caused by multicopy ppiD and nlpE, respectively. (PDF 12 KB)

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Matern, Y., Barion, B. & Behrens-Kneip, S. PpiD is a player in the network of periplasmic chaperones in Escherichia coli. BMC Microbiol 10, 251 (2010). https://0-doi-org.brum.beds.ac.uk/10.1186/1471-2180-10-251

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