From the
Lehrstuhl für Biotechnologie, Biozentrum der Universität Würzburg, Am Hubland, D-97074 Würzburg, Germany and the ¶Zentrum für Infektionsforschung, Universität Würzburg, Röntgenring 11, D-97070 Würzburg, Germany
Received for publication, December 23, 2002 , and in revised form, April 8, 2003.
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ABSTRACT |
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INTRODUCTION |
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Early biochemical investigations have established that NMN1 and nicotinamide riboside (NR) can substitute for NAD, whereas nicotinamide, niacin, or other nicotine-based intermediates of the Preiss-Handler pathway cannot (68). The NAD dependence of H. influenzae was confirmed by the absence of genes encoding the enzymes necessary for the de novo biosynthesis of NAD (9). Accumulation of nicotinamide nucleotides derived from NAD or NR has been demonstrated in H. influenzae and Haemophilus parainfluenzae (10, 11). For H. parainfluenzae, the Km for transport is 0.55 µM for NAD and 0.14 µM for NR, and the Vmax for NR is about four times that of NAD (11). This implies that NR is the substrate for an as yet unidentified inner membrane transporter.
Recently, we presented data showing that two gene products appear to be involved in the NAD utilization pathway of H. influenzae (1214). The gene products were identified as the hel-encoded outer membrane lipoprotein e(P4) and a periplasmic protein termed NadN. Knockout mutations of both genes resulted in growth-deficient phenotypes depending on the NAD concentrations provided in the growth medium. The enzymatic activities of both proteins were characterized. NadN has the ability to act as an NAD pyrophosphatase as well as an NMN 5'-nucleotidase. Furthermore, for e(P4), we showed that it acts as an NMN 5'-nucleotidase and that deletion or point mutants in hel affect the growth of H. influenzae and the uptake of NAD and NMN. Finally, an nadN hel double mutant was constructed, which was unable to utilize NAD or NMN and could grow only in the presence of NR (13).
It becomes more and more apparent that specialized outer membrane proteins (OMPs) play a key role in bacterial adaptation in host niches (15). In H. influenzae, a number of OMPs have been characterized, but none of them have been assigned as facilitators for specific substrates. Of the major OMPs, OmpP2, with a molecular mass of 40 kDa, was described previously (1618). It was found that ompP2 knockout mutants are viable under laboratory conditions, but are deleterious in an animal model, thus indicating an important role for bacterial physiology and infection under in vivo conditions. Through investigation of permeability channels of outer membrane (OM) samples of H. influenzae type b, a 40-kDa OMP was described previously as a diffusion porin with an exclusion size of
1400 Da (19), which was then found to correspond to OmpP2 (16). Variations in OmpP2 porins of different non-typeable H. influenzae isolates were found to cluster in a surface-exposed protein domain (20). OmpP2 porins of different non-typeable H. influenzae isolates from antibiotic-treated cystic fibrosis patients have been collected and tested for antibiotic permeability and channel properties (21). The OmpP2 variants have different properties due to variation and accumulation of point mutations in distinct protein domains (21). In addition, it was shown that OmpP2 is involved in binding between bacterial cells and human nasopharyngeal mucin (22).
In this study, we show that OmpP2 has an additional property that can be best described as specialized porin for the nicotinamide ribonucleotides NMN and NAD, but not for the nucleoside NR. An ompP2 knockout mutant showed an uptake deficiency for NAD and NMN substrates, but NR uptake was even higher than the wild-type level. Furthermore, purified OmpP2 porin was utilized in artificial lipid membrane systems, and conductivity was determined in the presence of different nucleotides and nucleosides. We found that only NAD and NMN caused a decrease in conductivity. This indicates that not only is OmpP2 a general diffusion pore, but it also has a similar function as the carbohydrate-specific porins of the OMs of enteric bacteria such as LamB and ScrY (2325).
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EXPERIMENTAL PROCEDURES |
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Construction and Characterization of the H. influenzae Mutant Strain ompP2::catTo generate an ompP2 knockout mutant, PCR-constructed DNA fragments containing 500 bp of the immediate upstream sequence and 400 bp of the immediate downstream sequence flanking the ompP2 gene were generated (see Fig. 1A). Synthesis of these PCR fragments was carried out according to Mullis and Faloona (26) using the following synthetic oligonucleotides (synthesized by MWG Biotech, Ebersberg, Germany): 2P2-3 (5'-CCAGAACTAGAAAGTTTTAC-3') and 3P2SnaBI (5'-AAATACGTAAAAGCAAGGGCGAATCGAAAGA-3'); and 5P2-5 (5'-CACGCTTTATAGTGATAGCC-3') and 5P2PstI (5'-AACTGCAGCTCCAATAGAATTGTCCAATCGCC-3'), respectively. In addition, an 1-kbp cat gene, encoding chloramphenicol acetyltransferase, was obtained by fragment isolation via gel separation using QIAGEN-Quick (QIAGEN, Frankfurt, Germany) and was derived from plasmid pAKcat (27) digested with SnaBI and PstI. A ligation reaction was performed with the two PCR DNA fragments (treated with restriction enzymes SnaBI and PstI) and the cat gene fragment according to Maniatis et al. (28). The ligation mixture was used as template in PCRs utilizing oligonucleotides 2P2-3 and 5P2-5. As a result, a 1.9-kbp DNA fragment was amplified. Upon restriction analysis, this fragment was identified as a DNA fragment containing the cat gene flanked by 500 bp of ompP2 upstream sequence and 400 bp of ompP2 downstream sequence (data not shown). Next, this DNA fragment was used and transformed into H. influenzae strain Rd, which was made competent for DNA uptake according to the method of Barcak et al. (29). The transformed cells were plated onto BHI agar containing chloramphenicol. After 2 days, chloramphenicol-resistant H. influenzae colonies were observed and purified. Chromosomal DNA was prepared; and utilizing the chromosomal DNA as template and oligonucleotides 2P2-3 and 5P2-5, we verified the cat insertion onto the chromosome by PCR analysis (data not shown). The data indicated that the cat gene had been acquired by double crossover and therefore had replaced ompP2 on the chromosome (see Fig. 1).
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Uptake StudiesH. influenzae strain Rd and mutant strain Rd ompP2::cat from overnight cultures were inoculated in BHI agar (3.8%) supplemented with NAD (10 µM) and hemin chloride (20 µg/ml) and grown to A490 = 2. Cells were then harvested; washed with BHI; resuspended to A490 = 2 (corresponding to 1.5 x 109 colony-forming units/ml); and used for the uptake of [14C]NAD, [14C]NMN, and [14C]NR as described previously (13). To determine the Vmax and Km values for NAD and NMN uptake, substrate concentrations ranging from 0.1 to 8 µM were used, and wild-type and mutant ompP2 strains were tested. For the wild-type Rd strain, a Lineweaver-Burk fit by least-squares linear regression analysis could be applied for NAD and NMN uptake. The specific activity of [carbonyl-14C]NAD was 81,000 cpm/nmol. NMN and NAD uptake was monitored at time points ranging from 0.5 to 2.5 min and from 2 to 18 min, respectively.
OmpP2 ExtractionOmpP2 was isolated and purified starting from 1 liter of culture of the H. influenzae Rd KW20 strain grown to A490 = 1 under the conditions described above. Cells were harvested by centrifugation at 8000 x g for 10 min in a Sorvall RC5 B centrifuge and washed once with buffer containing 100 mM NaCl. Subsequently, the cells were resuspended in 25 ml of 10 mM Hepes (pH 7.4) supplemented with proteinase inhibitor (Roche Diagnostics GmbH, Mannheim, Germany) and were passed three times through a French pressure cell. Unbroken cells were removed by centrifugation at 8000 x g for 15 min. The supernatant containing the broken cells was portioned in 2-ml aliquots, and the cell membrane was pelleted by centrifugation in an Eppendorf centrifuge at 13,000 rpm for 30 min at 4 °C. OM preparation was carried out according to Carlone et al. (30). In brief, the cell membrane pellets were resuspended in 1% sodium N-lauryl sarcosinate and 10 mM Hepes (pH 7.4) and incubated for 30 min at room temperature to remove most of the soluble inner membrane components. The pellets of the subsequent centrifugation were washed once with 10 mM Hepes (pH 7.4) and resuspended in 50 µl of the same buffer supplemented with proteinase inhibitor (Bio-Rad). The probes contained 1 mg/ml protein from OM components, including the channel-forming activity.
The probes were pooled, and the OM was pelleted by a subsequent centrifugation at 48,000 rpm for 30 min at 4 °C (Beckman Optima Ti-70.1 rotor). The pellet was resuspended in 2 ml of 0.05% Zwittergent 312 (Calbiochem) and 10 mM Tris-HCl (pH 8.0) and pelleted by centrifugation. The pellet was resuspended in 2 ml of the same buffer, and the mixture was centrifuged again. To solubilize OmpP2, the pellet was resuspended in 2 ml of 0.4% Zwittergent, 10 mM Tris-HCl (pH 8.0), and 10 mM EDTA and incubated for 30 min on ice. The OM was pelleted by centrifugation at 48,000 rpm for 30 min at 4 °C (Beckman Optima, Ti-70.1 rotor). The pellet was subjected to the same procedure again. The supernatants of both extractions were pooled and used for preparative SDS-PAGE or subjected to anion-exchange chromatography.
SDS-PAGESDS-PAGE was performed according to Laemmli (31) as described previously (13). The gels were stained with Coomassie Brilliant Blue or silver. Preparative SDS-PAGE was used for identification and purification of the channel-forming activity from the extracts of OM fractions obtained by sodium N-lauryl sarcosinate treatment of the cell envelopes. 15 µl of the 0.4% Zwittergent supernatant (protein concentration of 0.2 mg/ml) were mixed with 7 µl of colorless sample buffer and added to one pocket of the preparative SDS-polyacrylamide gel. One lane of the gel was stained with Coomassie Blue to localize the different protein bands. Unstained lanes with different molecular mass ranges were cut into slices and eluted overnight with 10 mM Tris-HCl (pH 8) and 1% Genapol X-80.
Anion-exchange ChromatographyThe supernatant from the extraction with 0.4% Zwittergent was loaded onto a Q-Sepharose anion-exchange column (1-ml HiTrap Q, Amersham Biosciences, Freiburg, Germany). Bound OmpP2 protein was eluted by a linear NaCl gradient in 0.05% Zwittergent and 10 mM Tris-HCl (pH 8.0). The fractions were collected and checked for purity by SDS-PAGE. Fractions collected at 550 mM NaCl contained pure OmpP2 protein and were used for reconstitution in black lipid bilayer membranes.
Determination of Conductivity and Titration Experiments with Nicotinamide CompoundsThe methods used for the lipid bilayer experiments have been described in detail previously (32). Black lipid bilayer membranes were obtained from a 1% (w/v) solution of diphytanoylphosphatidylcholine (Avanti Polar Lipids, Alabaster, AL) in n-decane. The single-channel records were performed using Ag/AgCl electrodes (with salt bridges) connected in series to a voltage source and a current-to-voltage converter made with a Burr Brown operational amplifier. OmpP2 was added from the concentrated stock solution either to the aqueous phase bathing a membrane in the black state or immediately prior to membrane formation. The temperature was kept at 20 °C throughout.
Binding of nucleosides and nucleotides to OmpP2 was investigated in the same way as the binding of malto-oligosaccharides to carbohydrate-specific porins (24, 33). Binding of the substrate to a binding site inside the channel could be detected by a reduced ion flux through the channel. After the membrane turned black, the protein was added to the aqueous compartment (final concentration of 100 ng/ml). The membrane conductance increased upon reconstitution of channels. After 2030 min, the increase slowed down; and when the conductance was nearly constant, the titration experiment was started. Nucleosides or nucleotides were added in defined concentrations to both sides of the membrane. If the compounds bound to the OmpP2 channel, the membrane conductance decreased in a dose-dependent manner as result of the reduced ion flux. The stability constant (K) of the binding could be analyzed using Equation 1 (24),
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RESULTS |
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However, by analyzing the uptake of [14C]NAD, [14C]NMN, and [14C]NR, we found a significant uptake deficiency for NAD and NMN (Fig. 2, A and B). In contrast, if NR was used as substrate, the mutant ompP2 strain showed at least the same level of accumulation compared with the wild-type strain (Fig. 2C). In addition, we determined the Vmax and Km values for substrates NMN and NAD (Table I). For the wild-type strain, it was possible to obtain the absolute values according to Michaelis-Menten kinetics. In contrast, for the ompP2 mutant, no absolute values for Vmax and Km could be determined. This was because up to the highest possible amount of labeled substrate (8 µM), the uptake rates still increased linearly, and no saturation could be observed. This indicated that the concentration range used in the experiments was below the Km; and therefore, the Michaelis-Menten equation can be reduced to V = Vmax·c/Km, indicating that the slope of the linear dependence between the uptake rate and the substrate concentration is Vmax/Km. This procedure allowed quantitative comparison with the wild-type strain. We found that the Vmax/Km ratios were 10-fold lower for the ompP2 mutant (Table I).
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Conductivity of OMPs of the Wild-type and Mutant ompP2 StrainsWe studied the OM fractions of wild-type H. influenzae (strain Rd KW20) and the ompP2 deletion mutant for channel formation in lipid bilayer membranes. The OMs were dissolved in buffer containing 10 mM Tris-HCl (pH 8) and 1% Genapol X-80. Lipid bilayer experiments demonstrated that the OM of the wild-type strain contained a channel-forming protein with a single-channel conductance of 1.6 nS in 1 M KCl. Only small amounts of the dissolved membrane fraction had to be added for high reconstitution rates. In contrast, the probability for channel formation observed with the dissolved OM fraction of the ompP2 deletion strain was very low. Here, the channel-forming protein with a conductance of 1.6 nS was absent. The majority of channels observed with the ompP2 deletion strain had a single-channel conductance of
2.5 nS in 1 M KCl. We conclude that OmpP2 protein is the origin of the 1.6-nS conductance steps.
Purification of OmpP2Many porins expressed by enteric bacteria are firmly attached to the peptidoglycan layer (34), indicating that they can be isolated starting from the peptidoglycan-protein complex. OmpP2 represents an exception because it is only loosely associated with the peptidoglycan (19), and different solubilization and isolation procedures have been used starting from whole cells or the cell envelope (19, 35). To purify OmpP2, we started from the OM fraction obtained by N-lauryl sarcosinate treatment of the cell envelope. The OM pellet was resuspended twice in buffer containing 0.05% Zwittergent, followed by centrifugation. The supernatants from the 0.05% Zwittergent treatments contained only very low channel-forming activity, indicating that OmpP2 porin was not dissolved by this procedure and was retained in the pellet. In the next step, the pellet was resuspended in buffer containing 0.4% Zwittergent and 10 mM EDTA and was kept on ice for 30 min. The mixture was centrifuged, and the pellet was subjected to the same procedure again. The supernatants of both extractions contained high channel-forming activity in the lipid bilayer assay.
SDS-PAGE demonstrated that the 0.4% Zwittergent extracts contained OmpP2 as the major band (Fig. 3, lane 2). Final purification of OmpP2 was achieved by preparative SDS-PAGE or by anion-exchange chromatography. For purification by preparative SDS-PAGE, the supernatant was loaded onto a 10% SDS-polyacrylamide gel. Different molecular mass bands were excised and eluted overnight with 10 mM Tris-HCl (pH 8) and 1% Genapol-X80 at 4 °C. The fraction with the highest channel-forming activity contained pure OmpP2 protein essentially free of contaminants as proven by SDS-PAGE (data not shown). Alternatively, OmpP2 was purified by anion-exchange chromatography. The supernatant was loaded onto a HiTrap Q column, and a linear salt gradient was used to elute bound protein. Fractions collected at 550 mM NaCl contained pure protein, which was identified as OmpP2 by SDS-PAGE (Fig. 3, lane 3). OmpP2 protein purified by ion-exchange chromatography formed the same channels as Genapol X-80 extracts of the OM and the protein derived from preparative SDS-PAGE. This shows that purification by preparative SDS-PAGE does not affect the channel-forming ability of OmpP2.
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Characterization of OmpP2OmpP2 has been characterized previously in experiments using lipid bilayer membranes (36). To verify that the channel properties of purified OmpP2 used in this study are similar to those described in the previous work, we performed single-channel and multichannel measurements using lipid bilayer membranes from diphytanoylphosphatidylcholine/n-decane. The addition of pure OmpP2 at a very low concentration (100 ng/ml) to a black lipid membrane caused a substantial conductance increase over several orders of magnitude similar to that caused by other bacterial porins (37). Under conditions of appropriate amplification and low protein concentration, the recording of single events of pore integration into the membrane could be resolved as conductance steps (see Fig. 4 for a single-channel recording in 1 M KCl). Fig. 5 shows a histogram of all current fluctuations observed with OmpP2 in 1 M KCl. The data suggest that the current fluctuations are fairly homogeneous.
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The single-channel conductance was independent of the applied voltage within a range of 100 to +100 mV, indicating that OmpP2 pores are not voltage-gated. This corresponds with the observations of Vachon et al. (36). The average single-channel conductance of OmpP2 in 1 M KCl was 1.6 nS. This value is similar to that derived previously by Vachon et al. (36) under otherwise similar conditions. By statistical analysis of at least 100 of these integration steps, the single-channel conductance of OmpP2 as a function of different salts and different concentrations was evaluated. The results are summarized in Table II. The investigation of different KCl concentrations from 0.03 to 3 M demonstrated that the channel conductance was an almost linear function of the salt concentration. This is again in good agreement with the previous study (36). The linear correlation between channel conductance and salt concentration excluded the possibility of an ion-binding site inside the OmpP2 channel because we would expect saturation at high salt concentrations.
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Potassium and chloride ions have a similar mobility in aqueous solutions (38). Replacement of potassium with lithium ions led to a decrease in the single-channel conductance from 0.2 nS (at 0.1 M KCl) to 0.1 nS. On the other hand, when chloride was replaced with the large and less mobile acetate, the single-channel conductance decreased also to 0.1 nS. This indicates that the influence of cations and anions on the single-channel conductance is approximately the same, suggesting that the OmpP2 channel has very low ion selectivity.
Ion Selectivity of OmpP2The presumed low selectivity of OmpP2 was checked by multichannel experiments under zero-current conditions. For a 5-fold salt gradient, the potential on the more dilute side of the membrane was positive for KCl and potassium acetate, suggesting preferential movement of cations through the OmpP2 channel for these salts. However, the zero-current membrane potential was slightly negative using LiCl as electrolyte, suggesting preferential movement of chloride over lithium ions. The calculation of the permeability ratios of cations and anions through OmpP2 using the Goldman-Hodgkin-Katz equation (39) is given in Table III together with the zero-current membrane potential. The results suggest that the selectivity of the OmpP2 channel is indeed very low, in agreement with the study of Vachon et al. (36). The channel showed a small preference for cations over anions for KCl and potassium acetate (Pc/Pa = 1.5 and 2.5, respectively), whereas it was slightly anion-selective for LiCl (Pc/Pa = 0.8).
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The OmpP2 Channel Binds NAD and NMNThe in vivo uptake experiments revealed that OmpP2 is necessary for the transport of certain nicotinamide compounds such as NAD and NMN, but not NR, across the OM. This result suggests that OmpP2 could be a channel specific for nicotinamide compounds containing a binding site for NAD and NMN in a similar way as LamB and ScrY are carbohydrate-specific channels with a binding site for malto-oligosaccharides (25, 40, 41). To test this hypothesis, we performed similar titration experiments as described previously for specific porins of Escherichia coli (24, 33). OmpP2 was reconstituted into lipid bilayer membranes. After the insertion process had slowed down considerably, concentrated solutions of different nicotinamide compounds were added to the aqueous solutions at both sides of the membrane while stirring to allow equilibration. Fig. 6 shows the experiment using NMN as a prospective substrate of OmpP2. Interestingly, the addition of NMN led to a dose-dependent block of OmpP2-mediated membrane conductance, which decreased by 40% at 7.4 mM NMN.
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The titration experiments with OmpP2 were analyzed in a way similar to that previously used with the carbohydrate-binding channels of Gram-negative bacteria (25, 33), which means that the stability constants could be calculated by a direct fit of the experimental data using Equation 1 or 2. Fig. 7 shows the fit of the experimental data of Fig. 6 using Equation 1(dashed line), which resulted in a stability constant (K)of 108 M1 (KS = 9.2 mM). Unfortunately, the fit of the titration data of Fig. 6 using Equation 1 was not satisfactory, as the dashed line in Fig. 7 clearly indicates. This could be explained by the assumption either that OmpP2 did not close completely when it was occupied by NMN or that the OmpP2 probe contained another highly active channel-forming protein that could not be detected by SDS-PAGE and that did not respond to NMN. A much better fit was possible with Equation 2, which took this problem into account. Fig. 7 shows also the fit of the data of Fig. 6 using Equation 2 (solid line). It was much better and yielded a stability constant (K) of 330 M1 (KS = 3.0 mM). The average of six titration experiments of the same type yielded, on average, a stability constant of 260 M1 (KS = 3.8 mM), and we found that 45% of the OmpP2-mediated conductance was not blocked by NMN (Table IV). As pointed out above, this could mean that 45% of the initial conductance was ascribed to channels that did not react to NMN or, as a second possibility, that OmpP2 channels occupied by NMN could still conduct KCl at
45% of the conductance in the open state (without NMN).
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To investigate the two possibilities, we performed single-channel conductance experiments with OmpP2 in the presence of different concentrations of NMN. The results (summarized in Table V) indicate that OmpP2 does not contain a channel-forming impurity because the conductance of the 1.6-nS channel at 1 M KCl and that of the 0.2-nS channel at 0.1 M KCl were found to be dependent on the presence of NMN. Analysis of the single-channel conductance as a function of NMN concentration using Equation 2 resulted in a similar half-saturation constant as derived above from the titration experiments (KS = 3.8 mM). Interestingly, the ionic strength of the aqueous phase had a substantial effect on the binding of NMN to OmpP2. An increase in potassium chloride concentration from 0.1 to 1 M resulted in a 2.6-fold increase in the half-saturation constant for NMN binding from 3.8 to 10.0 mM (Table IV). Again, the channels were not completely blocked by NMN and conducted by 70% at very high concentrations of NMN, similar to the situation at 0.1 M KCl. The dependence of NMN binding on the electrolyte concentration indicates a possible ion-ion interaction between OmpP2 and the substrate NMN.
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We also performed current inhibition measurements with other nicotinamide compounds to investigate whether the interaction between NMN and OmpP2 is specific and if special structural requirements of the molecules are necessary for binding. As demonstrated above, the stability constant (K) for binding of these molecules to the binding site inside the OmpP2 channel was derived from a direct fit of the experimental data using Equation 2. The results for K and the half-saturation constant KS (1/K) are listed in Table IV. They suggest that, besides NMN, also NAD binds to the binding site inside OmpP2. On the other hand, we did not observe binding of ATP, ADP, AMP, GTP, GMP, and NR to OmpP2 within the concentration range that could be used here. This indicates that the half-saturation constant for binding of these molecules, if it exists, is at least above 100 mM, which is above the physiologically relevant concentration.
The influence of the different nicotinamide compounds was also tested on the single-channel conductance of OmpP2 in 0.1 and 1 M KCl. As described above, the conductance of the channel was decreased by the addition of NAD. The molecules, which had no effect in titration experiments, showed also no effect on channel conductance. The results of the single-channel experiments are summarized in Table V.
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DISCUSSION |
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So far, we have excluded the possibility that NAD nucleotidase or NMN phosphatase activities are associated with OmpP2 because the purified OmpP2 samples (data not shown) and whole OMP preparations of hel knockout mutants do not show either of these activities (13). Because the accumulation of NR in the ompP2 deletion strain was comparable to that in the wild-type strain, we suggest that OmpP2 provides the hydrophilic pathway for NAD and NMN and that NR is able to cross the OM through a different or additional pathway, most likely through a yet not identified pore-forming protein. It should be mentioned that the knockout of ompP2 strongly affects the growth rate of H. influenzae (16), even in the presence of NR in the growth medium (data not shown).
In wild-type bacteria, OmpP2 protein was expressed in high copy number, as it was responsible for one of the major bands on an SDS gel of OMP preparations. The knockout of OmpP2 indicates a strong reduction of the OM permeability concomitant with limited nutrient uptake. A reduced growth rate can be observed also in other Gram-negative bacteria with a knockout of major porins such as OmpF and OmpC in E. coli (42, 43). Lack of the major porins stimulates the cells to promote the increased expression of other pore-forming proteins (34). In the case of H. influenzae, this could be a pore-forming protein with the ability to transport NR across the OM, explaining the observed ompP2-independent uptake rate for NR. We observed pore activity of the OM extract from the ompP2 knockout strain. Further characterization of the responsible proteins will be part of future studies.
Upon revealing that OmpP2 provides the hydrophilic pathway for NAD and NMN across the OM, we tested whether OmpP2 is a specific channel for these nicotinamide compounds. Therefore, we purified OmpP2 from H. influenzae Rd KW20 and reconstituted the porin in black lipid bilayers. Detergent extracts of the OM fractions showed a high reconstitution rate of pores with a single-channel conductance of 1.6 nS in 1 M KCl, which was not observed in OM extracts of the OmpP2-deficient strain. OmpP2 was further purified by preparative SDS-PAGE or ion-exchange chromatography. Preparative SDS-PAGE has been previously used for purification of other pore-forming proteins (4446). One should mention that OmpP2 forms trimers, which are not stable in SDS. Therefore, only the monomeric form could be cut out of the gel. Nevertheless, this preparation was active, and pores showed no difference compared with those seen before SDS-PAGE. One can assume that OmpP2 trimers assemble properly in vitro, as shown previously and as also known for E. coli porin (47, 48). Alternatively, OmpP2 was also purified by ion-exchange chromatography to exclude that SDS treatment changes channel characteristics. Either purification protocol resulted in channels with the same characteristics, which are similar to those determined in a previous study (36). The single-channel conductance of OmpP2 measured in our study was a little higher than in the previous study, which could be explained by the use of different H. influenzae strains. The primary sequence of the different OmpP2 proteins varies within the region of loop 4, which is known to influence single-channel conductance (49). The reconstituted pores were voltage-independent up to a range of ±100 mV, and single-channel conductance showed a linear dependence on the electrolyte concentration, revealing that there is no ion-binding site inside the channel. Concerning ion selectivity, the OmpP2 pores showed a small preference for cations over anions for KCl and potassium acetate (Pc/Pa = 1.5 and 2.5, respectively) and were slightly anion-selective for LiCl (Pc/Pa = 0.8). Compared with the partially highly cation-selective general diffusion pores of enteric bacteria such as E. coli and Salmonella typhimurium with Pc/Pa ratios between 4 and
20 for KCl, the selectivity of OmpP2 porin is not very pronounced (40, 50). Although, in enteric bacteria, the OM acts as a filter against negatively charged harmful compounds such as bile salts, OmpP2 porin might not select passing compounds according to their charge. This is underscored by the observation that the OM of H. influenzae shows a higher permeability for anionic
-lactam antibiotics than the OM of E. coli (51). The two substrates NAD and NMN, which enter the periplasmic space via OmpP2, carry no net charge, but are zwitterionic with a positively charged nicotinamide and a negatively charged phosphate group. The addition of these substances to a membrane with reconstituted OmpP2 channels resulted in a dose-dependent decrease in the membrane conductance. This indicates that NAD and NMN block the flow of the electrolyte by binding reversibly to a binding site inside the channel. Thus, it is possible to perform titration experiments similar to those performed to study the malto-oligosaccharide binding of carbohydrate-specific channels and to calculate the stability constant of the binding process. The binding constant of NMN was double that of NAD (260 and 125 M1 in 0.1 M KCl, respectively), corresponding to half-saturation concentrations of 3.8 and 8.0 mM, respectively. Compared with the binding of maltooligosaccharides to sugar-specific channels (e.g. the binding constant (K) for binding of maltopentaose to maltoporin is
14,000 M1) (24), these values appear to be low. One has to consider that the number and strength of interactions between the protein and the substrates determine the stability constant. In the case of maltoporin, the stability constant for maltose binding (Kmaltose = 110 M1) is 2 orders of magnitude lower compared with that for maltopentaose binding, and that for glucose binding is even lower (Kglucose = 9.5 M1) (24). An important question that results from these studies is what parts of the substrates are involved in binding to the binding site of OmpP2? Comparing the structures of NAD and NMN, one has to assume that the adenosine monophosphate group of the NAD molecule does not contribute to the binding. Otherwise, one would expect a higher stability constant for NAD compared with NMN. This was confirmed using AMP as substrate for titration experiments. No binding of AMP was observed, as the conductance remained unchanged up to 100 mM AMP in the aqueous solution. Also, ADP and ATP had no effect, showing that a nicotinamide ribosyl group is necessary for binding. However, titration experiments with NR failed, revealing that this group is not able to interact with the binding site. This shows that a combination of the nicotinamide ribosyl group and the phosphate group may be necessary to become a target for the specific binding site of OmpP2. Both groups are charged, and one can assume that ionic interactions play a role in the binding of the substrates to the binding site.
By measuring the binding affinities of NMN in different electrolyte concentrations, we showed that binding depends on the ionic strength of the aqueous solution. Binding was significantly reduced in 1 M KCl compared with that in 100 mM KCl (260 and 100 M1, respectively). Charges (which might be involved in the binding process) are shielded more at higher ionic strength. This reduces the strength of interaction between the binding site and substrate and leads to a lower binding constant. Another indication that point charges are involved in binding is the observation that NAD in its reduced form (NADH) lacking the positive charge at the nicotinamide group did not bind to OmpP2.
In contrast to the carbohydrate-specific porins, binding of NAD and NMN to OmpP2 does not completely block the passage of electrolytes. The remaining conductance is the result of partially blocked OmpP2 channels and not of impurities, as we showed by single-channel measurements in the presence of substrate. The maximal percent inhibition depends of the size of the substrate. In the case of NMN (334.2 Da), the conductance is reduced by 55%; for NAD (663.4 Da), this value is 70%. One can imagine that NMN, when bound to the binding site, does not block the channel constriction completely and leaves a gap for ions passing through. The additional adenosine monophosphate group in the NAD molecule leads to a further reduction of the remaining open channel diameter, explaining the higher maximal inhibition of the channel conductance.
The in vivo uptake study revealed that NMN is taken up somehow faster than NAD (Fig. 2, A and B). For NMN, the Vmax is 0.59 µM min1 (1.5 x 109 colony-forming units/ml), and the Km is 6.4 µM, compared with 0.13 µM min1 and 5.5 µM measured for NAD, respectively. In a previous study, it was calculated and experimentally proven that, at low substrate concentrations, the OM is rate-limiting for uptake (52). The substrate concentration in our uptake experiment was 1 µM; thus, it is possible that passage through OmpP2 is the limiting step for NAD and NMN uptake. The stability constants for NAD and NMN binding to OmpP2 measured by in vitro titration experiments reflect the ratios of the on- and off-rates of the binding process. We assume that the off-rates of the NMN- and NAD-binding processes, reflecting the strength and duration of binding, are similar because interaction between the substrates and the binding site should be the same. Therefore, the difference in stability constants must be a result of different on-rates for NAD and NMN. This is in good agreement with the uptake study because, at low concentrations, uptake depends on the on-rate, and the binding constant and the uptake rate of NMN are higher than those of NAD.
In conclusion, we have shown that OmpP2 reveals the hydrophilic pathway for NAD and NMN into the periplasmic space. Uptake of these vital substances through OmpP2 seems to be further improved by the presence of a binding site inside the channel. Our study is the first step in the further characterization of the binding site in the future.
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FOOTNOTES |
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Recipient of an Emmy-Noether fellowship.
|| To whom correspondence should be addressed. Tel.: 49-931-888-4501; Fax: 49-931-888-4509; E-mail: roland.benz{at}mail.uni-wuerzburg.de.
1 The abbreviations used are: NMN, nicotinamide mononucleotides; NR, nicotinamide riboside; OMPs, outer membrane proteins; OM, outer membrane; BHI, brain-heart infusion; nS, nanosiemens.
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