Mfa4, an Accessory Protein of Mfa1 Fimbriae, Modulates Fimbrial Biogenesis, Cell Auto-Aggregation, and Biofilm Formation in Porphyromonas gingivalis

Porphyromonas gingivalis, a gram-negative obligate anaerobic bacterium, is considered to be a key pathogen in periodontal disease. The bacterium expresses Mfa1 fimbriae, which are composed of polymers of Mfa1. The minor accessory components Mfa3, Mfa4, and Mfa5 are incorporated into these fimbriae. In this study, we characterized Mfa4 using genetically modified strains. Deficiency in the mfa4 gene decreased, but did not eliminate, expression of Mfa1 fimbriae. However, Mfa3 and Mfa5 were not incorporated because of defects in posttranslational processing and leakage into the culture supernatant, respectively. Furthermore, the mfa4-deficient mutant had an increased tendency to auto-aggregate and form biofilms, reminiscent of a mutant completely lacking Mfa1. Notably, complementation of mfa4 restored expression of structurally intact and functional Mfa1 fimbriae. Taken together, these results indicate that the accessory proteins Mfa3, Mfa4, and Mfa5 are necessary for assembly of Mfa1 fimbriae and regulation of auto-aggregation and biofilm formation of P. gingivalis. In addition, we found that Mfa3 and Mfa4 are processed to maturity by the same RgpA/B protease that processes Mfa1 subunits prior to polymerization.


Introduction
Porphyromonas gingivalis, a gram-negative obligate anaerobic bacterium, is a component of dental plaque biofilms in humans and plays a key role in the initiation and progression of chronic periodontitis [1]. It is also thought to be associated with systemic diseases such as cardiovascular disease [2], rheumatoid arthritis [3], and nonalcoholic fatty liver disease [4]. The organism expresses a number of potential virulence factors, including fimbriae and gingipain It was also reported that Mfa1 fimbriae are essential for coadhesion and community formation with oral commensal bacteria such as Streptococcus gordonii [11] and for survival within human myeloid dendritic cells [15]. Indeed, we recently reported that an mfa3 mutant, which lacks all accessory proteins in the fimbriae, strongly auto-aggregates and forms biofilms, indicating that accessory proteins restrict auto-aggregation and biofilm formation [13].
Mfa3, with molecular weight 43 kDa, temporarily accumulates in the inner membrane and is then proteolytically processed. The 40-kDa mature Mfa3 redistributes to the outer membrane, where it is finally incorporated into fimbriae [13]. N-terminal sequencing suggests that Mfa3 is processed by gingipains. Therefore, it has been proposed that this accessory protein is processed and transported from the cytoplasm to the outer membrane in the same manner as the major structural proteins FimA and Mfa1 [16,17], which are also processed by the gingipain RgpA/B to yield mature forms [18,19].
In this study, we characterize Mfa4 and its role in the biogenesis and assembly of functional Mfa1 fimbriae. Furthermore, we show that RgpA/B is involved in the maturation of the accessory proteins Mfa3 and Mfa4.

DNA manipulations
Restriction endonucleases and DNA ligase were purchased from Takara Bio Inc. (Otsu, Japan) or New England Biolabs (Ipswich, MA, USA). PCR primers ( Table 2) were synthesized by Sigma Genosys (Ishikari, Japan) and were used in standard PCR using PCR Thermal Cycler Dice™ (Takara Bio Inc.) and Pyrobest (Takara Bio Inc.), a high-fidelity DNA polymerase.

Construction of gene-deficient and complemented strains
To construct the mfa4-deficient mutant, an internal fragment of the mfa4 gene was amplified by PCR with primers Mfa4F and Mfa4R (Table 2), the sequences of which were designed based on the P. gingivalis ATCC 33277 genome (NC_010729) [25]. The amplified 2.0-kbp fragment was ligated into a pCR-Blunt II-TOPO plasmid vector (Thermo Fisher Scientific Inc. Carlsbad, CA) and propagated in E. coli TOP10 (Thermo Fisher Scientific Inc.). The mfa4 gene was disrupted by inserting into the BalI site a fragment containing ermF, which is expressed in Porphyromonas and Bacteroides spp., and ermAM, which is expressed in E. coli. This fragment was excised from plasmid pVA2198 [23] by digestion with KpnI and BamHI. The plasmid containing disrupted mfa4 was linearized with KpnI, and then delivered by electroporation into P. gingivalis JI-1, a fimA-deficient strain (Table 1). After 12 h of anaerobic incubation in sTSB, cells were spread on Brucella HK agar supplemented with 20 μg/mL erythromycin and grown anaerobically at 37°C for 7 days.
The mfa5 disruption mutant was constructed in a similar manner. In brief, an internal sequence of mfa5 was amplified by PCR with primers Mfa5F and Mfa5R (Table 2), ligated into pCR-BluntII-TOPO, and amplified in E. coli TOP10. The erythromycin-resistance cassette as described was inserted into the SacI site in the mfa5 fragment. The resulting plasmid was linearized and then delivered by electroporation into P. gingivalis JI-1. Specific gene disruptions in mfa4 and mfa5 were confirmed by PCR and Southern blotting (data not shown).

Purification of Mfa1 fimbriae
Mfa1 fimbriae were purified from P. gingivalis JI-1, FMFA4, and FMFA5 as described previously [13]. Briefly, cells were lysed by French press. The soluble fraction was cleared by ultracentrifugation and precipitated with ammonium sulfate at 50% saturation. Mfa1 fimbriae were purified by ion exchange and size exclusion chromatography. Purity and identity were verified by SDS-PAGE and mass spectrometry.

Subcellular fractionation
P. gingivalis strains were cultivated in sTSB until the early stationary phase. The culture supernatant was separated from bacterial cells by centrifugation and proteins were concentrated by ammonium sulfate precipitation at 70% saturation, as described previously [27]. Cells were resuspended in 10 mM HEPES-NaOH pH 7.4 containing 0.1 mM N-α-p-tosyl-L-lysine chloromethyl ketone, 0.2 mM phenylmethylsulfonyl fluoride, and 0.1 mM leupeptin, and then lysed by French press. Residual intact cells were removed by centrifugation at 1,000 ×g for 10 min. The whole-cell lysate was then fractionated as previously described [28]. Briefly, the soluble fraction was separated from the envelope fraction by centrifugation at 100,000 ×g for 60 min at 4°C. The envelope fraction was suspended for 30 min at 20°C in HEPES buffer pH 7.4 containing 1% Triton X-100 and 20 mM MgCl 2 and then centrifuged at 100,000 ×g for 60 min at 4°C. The resulting supernatant contained the inner membrane fraction, while the sediment contained the outer membrane fraction and was subsequently homogenized in HEPES buffer.

SDS-PAGE and immunoblotting
Samples containing 5 μg total protein were solubilized in a buffer containing SDS and 2-mercaptoethanol and then heated at 100°C for 5 min, 80°C for 10 min, or 60°C for 10 min. Subsequently, samples were separated using SDS-PAGE, and were either stained with Coomassie brilliant blue R-250 or blotted on PVDF membranes. Membranes were blocked with 5% skim milk in 20 mM Tris-HCl pH 7.4 with 300 mM NaCl and 0.05% Tween 20. Membranes were then probed with primary rabbit polyclonal antibodies against purified Mfa1 fimbriae, Mfa2, Mfa3, Mfa4, or Mfa5 [12,13], and labeled with secondary HRP-conjugated goat anti-rabbit IgG (MP Biomedicals, Santa Ana, CA). Finally, bands were visualized with ECL-prime (GE Healthcare, Buckinghamshire, UK).

N-terminal sequencing
Proteins separated by SDS-PAGE were electrophoretically transferred to PVDF membranes and stained with Coomassie brilliant blue R-250. Mfa4 bands were excised and analyzed by Nterminal sequencing on an ABI 477 A automatic peptide sequence analyzer at Center for Instrumental Analysis, Hokkaido University.

Mass spectrometry
After SDS-PAGE, proteins of interest were analyzed using matrix-assisted laser desorption ionization time-of-flight mass spectrometry (MALDI-TOF MS) as described previously [29]. Briefly, bands were digested with trypsin in-gel, and digestion products were extracted, concentrated, and analyzed using a 4800 MALDI TOF/TOF Analyzer (AB Sciex, Framingham, MA).
Proteins were identified from MS peaks using MS-Fit peptide mass fingerprinting methods in the Mascot program (http://www.matrixscience.com/).

Preparation of antiserum against Mfa1-only fimbriae
Antiserum against Mfa1 fimbriae consisting of Mfa1 only and without accessory proteins was prepared according to published methods [13]. Briefly, Mfa1 fimbriae that lack all accessory proteins (Hasegawa, unpublished data) were purified from strain FMFA5, mixed with Freund's complete adjuvant, and subcutaneously injected into rabbits three times at 2-week intervals. A rabbit was housed (36 cm x 35 cm x 48 cm) in the climate-controlled room (23.3 ± 0.2°C, relative humidity of 58 ± 9%) maintained on a light/dark cycle with lights on from 07:00 to 19:00 with free access to food and water. During procedures, health monitoring was conducted every day. Animal work was performed in strict accordance with Regulations on Animal Experimentation at Aichi Gakuin University including humane endpoints. Protocols were approved by the Aichi Gakuin University Animal Research Committee (Permit No. AGUD113). All efforts were made to minimize animal suffering, and animals were sacrificed under sodium pentobarbital anesthesia.

Filtration ELISA
To detect Mfa1 fimbriae exposed on the cell surface, filtration ELISA was performed using intact cells as antigen [30]. A 100 μL cell suspension containing 5×10 6 cells was applied over filters in a 96-well MultiScreen-GV filtration plate with pore size 0.22 μm (EMD Millipore, MA). Subsequently, wells were washed with a buffer consisting of 20 mM Tris pH 7.5, 150 mM NaCl, and 0.05% Tween 20 (TBST), and blocked with 3% bovine serum albumin in TBST. Wells were then probed with a 1,000-fold dilution of antiserum against Mfa1-only fimbriae, washed, and then labeled with HRP-conjugated polyclonal goat anti-rabbit IgG (Dako, Glostrup, Denmark). Subsequently, o-phenylenediamine and H 2 O 2 in citrate buffer pH 5.0 were added as substrate.
Reactions were terminated with 1 M H 2 SO 4 and absorbance at 490 nm (OD 490 ) was measured.
To normalize Mfa1 expression to the amount of intact cells, filtration ELISA was also performed using antibodies raised against P. gingivalis whole cells [31].

Auto-aggregation activity of P. gingivalis
Auto-aggregation activity was measured according to published methods [13,32]. Cells were harvested by centrifugation at 8,000 ×g for 10 min and gently washed twice with, and resuspended in, 20 mM PBS pH 6.0. The OD 600 of the resulting cell suspension was measured and adjusted to 1.0 by dilution with PBS. Cells were then aliquoted into 13-mm culture tubes at 2 mL per tube, and shaken at 120 strokes/min at room temperature. The OD 660 of the cell suspension was measured at various time points with a Mini Photo 518R spectrophotometer (Taitec, Saitama, Japan).

Biofilm assay
Homotypic biofilm formation was quantified using a microtiter plate assay specifically adapted for P. gingivalis [13,31]

Statistics
Data are reported as mean ± standard deviation (SD). One-way analysis of variance and Dunnett multiple-comparison test were used to evaluate differences between groups. Significance was defined as p value < 0.01.

Processing of Mfa4 and its incorporation into Mfa1 fimbriae
We constructed the mfa4-deficient mutant FMFA4 from the fimA-deletion strain JI-1 to avoid potential confounding effects from FimA fimbriae. We also constructed FMFA4C, a complemented strain that expresses wild-type mfa4 in trans. Immunoblotting with antibodies against Mfa4 [13] showed a clear band with molecular weight 30 kDa in JI-1 and FMFA4C, but not in FMFA4 (Fig 1B). These results indicate that Mfa4 is lost upon disruption of mfa4, and is overwhelmingly regained upon complementation. We examined the subcellular localization of Mfa4 to follow the intracellular processing events that lead to its maturation. As shown in Fig 1C, Mfa4 was detected as a 30-kDa protein in the whole-cell lysate and accumulated predominantly in the envelope fraction. Upon separation of the envelope fraction into inner and outer membranes, Mfa4 was detected mainly in the inner membrane, suggesting that while Mfa4 is a minor fimbrial component, it is predominantly an inner-membrane protein. Nevertheless, some Mfa4 fractionates with the outer membrane, confirming a previous observation that Mfa4 co-purifies with fimbriae recovered from the outer membrane [28].
Effect of mfa4 mutation on assembly of Mfa1 fimbriae Mfa1 expression and polymerization were examined by immunoblotting using a specific antiserum against Mfa1 fimbriae purified from JI-1 [13]. No difference was observed in between the band pattern of the blot using anti-Mfa1 fimbriae from JI-1 and FMFA5. Whole-cell lysates from all strains except SMF-fimA, a Mfa1-deficient mutant, contained Mfa1 monomers of comparable molecular weight when completely denatured by heating at 100°C (Fig 2A). In contrast, heating whole-cell lysates from JI-1 and FMFA4C at 80°C generated a ladder, indicating partial dissociation of Mfa1 fimbriae (Fig 2A). We presume that the laddering is due to the effect of molecular shape and incomplete binding of SDS to polymerized Mfa1. However, FMFA4 did not show laddering, except when lysates were heat-denatured at 60°C (Fig 2A). Thus, the two fimbriae differ in temperature-dependent dissociability and it is likely that Mfa1 subunits are held together less strongly in the absence of mfa4.
Subsequently, Mfa1 fimbriae expression on the cell surface was determined by ELISA analysis of intact bacterial cells. As shown in Fig 2B, Mfa1 expression on the surface of FMFA4 is 43% of JI-1. Complementation of the mutant with a copy of mfa4 in trans significantly increased cell surface display to 79% of JI-1. Nevertheless, expression of Mfa1 fimbriae in FMFA4C is still significantly lower than in J1-1, even though Mfa4 is expressed much more abundantly (Fig 1B). Nevertheless, the data imply that Mfa4 facilitates the display of Mfa1 fimbriae on the cell surface.

Effect of mfa4 mutation on other fimbrial proteins
In JI-1 whole-cell lysates, Mfa3 was detected as bands of size 40 and 43 kDa, as shown in Fig 3. Only the 40-kDa band, which corresponds to the mature protein, was detected in the soluble fraction, which also contains Mfa1 fimbriae. The envelope fraction had both forms of Mfa3 in comparable amounts. However, the unprocessed and mature forms were enriched in inner and outer membranes, respectively, indicating that Mfa3 matures as it redistributes from the inner to the outer membrane. Finally, Mfa3 in any form was undetectable in the culture supernatant. In contrast, mature 40-kDa Mfa3 was not detected at all in FMFA4 (Fig 3). Notably, complementation completely rescues processing (Fig 3). These results strongly indicate that Mfa4 is required for maturation of Mfa3 in P. gingivalis. In contrast, Mfa4 deficiency did not alter the expression and cellular localization of Mfa2, and equivalent amounts of Mfa2 were detected in the outer membrane of FMFA4 and JI-1 (S1 Fig). On the other hand, Mfa5 was detected at 130 kDa in whole-cell lysates from JI-1, but not from FMFA4 (Fig 4). In addition, full-length Mfa5, as well as degradation products with molecular weight 100 and 78 kDa, were observed in the culture supernatant from FMFA4. Complementation reverses this leakage, and results in accumulation of Mfa5 in whole-cell lysates of FMFA4C. These results strongly suggest that Mfa4 is required to anchor and stabilize Mfa5 in FMFA4, FMFA4C, SMF-fimA, and rgpA/B-deficient KDP112 were applied over filters in a filtration plate at 5×10 6 cells/well. Bacterial cells were probed with antibodies against Mfa1-only fimbriae purified from FMFA5, and then with peroxidase-conjugated goat anti-rabbit IgG at a dilution of 1:1000. Data are mean ± SD from two experiments with triplicates. *, statistically significant difference from JI-1 based on Dunnett's test (p < 0.01).

Composition of Mfa1 fimbriae in FMFA4
Mfa1 fimbriae were purified from FMFA4 and JI-1 to examine the effect of mfa4 deficiency on composition and assembly. As shown in Fig 5A, JI-1 fimbriae (lane 1), contain several proteins, and bands at corresponding molecular weights were identified by mass spectrometry to be Mfa1 and Mfa3-5 [12]. Notably, N-terminal sequencing indicates that Mfa4 incorporated into Mfa1 fimbriae begins at Asn 54 (Fig 5D).
Mfa1 fimbriae purified from FMFA4 contained a ladder of Mfa1 between 50 and 75 kDa, as observed in JI-1, but did not contain the accessory components Mfa3, Mfa5, and Mfa4 (Fig 5A,  lane 2). The absence of accessory components was confirmed by immunoblotting (Fig 5B and 5C).

Auto-aggregation and biofilm formation in FMFA4
Because P. gingivalis ATCC 33277 contains a mutation in fimB that leads to the production of unusual FimA fimbriae [31], and to avoid possible confounding effects from FimA fimbriae, auto-aggregation and biofilm formation were analyzed in strains from which fimA had been deleted.
Wild type P. gingivalis auto-aggregates in shaking cultures, an event captured by a drastic decline in OD 660 , a measure of turbidity (Fig 6A) [13]. FimA fimbriae are known to accelerate auto-aggregation, whereas Mfa1 fimbriae suppress it [13]. Control experiments confirm that the OD 600 of liquid cultures of wild type P. gingivalis declines rapidly over 40-60 min, reaching approximately 20% of the initial value. In contrast, the turbidity of cultures of the fimA-deficient strain JI-1 decreased only 10% after 60 minutes (Fig 6A). However, the mfa1and fimAdeficient strain SMF-fimA auto-aggregates with kinetics comparable to wild type, also reaching 19% of the initial value after 1 h (Fig 6A). Interestingly, the mfa4and fimA-deficient strain FMFA4, which still produces Mfa1 fimbriae, albeit ones without Mfa3 and Mfa5, strongly auto-aggregates like SMF-fimA. Finally, FMA4C auto-aggregates with kinetics similar to JI-1, presumably because complementation of mfa4 in this strain restores the structure and function of Mfa1 fimbriae.
Crystal violet assays showed that strains SMF-fimA and FMFA4 form biofilms robustly ( Fig  6B). However, the complemented strain FMFA4C, which has functional Mfa1 fimbriae, but  Role of Accessory Protein Mfa4 in Mfa1 Fimbriae not FimA fimbriae, has diminished capacity to form biofilms, and resembles JI-1. Indeed, strains that auto-aggregate also form more robust biofilms.

Expression of the mfa gene cluster in P. gingivalis KDP112
It has been shown that FimA and Mfa1 are processed to maturity by Rgp [18,19], which specifically cleaves substrates on the carboxyl side of arginine residues. The N-terminal amino acids of Mfa1 and Mfa3 incorporated into Mfa1 fimbriae were reported to be Ala 50 [16] and Ala 44 [13], respectively. In this study, we determined the N-terminus of mature Mfa4 to be Asn 54 (Fig 5D). In all cases, the prior residue was arginine, suggesting that these proteins are also processed by RgpA/B. Therefore, we used KDP112, a double mutant lacking rgpA/B [21], to examine whether RgpA/B is involved in processing Mfa1-4.
Mfa2 in KDP112 is of similar size as in the parental strain (Fig 7B), but the other fimbrial proteins were found to be of higher molecular weight than those in strain JI-1, which expresses Rgp enzymes (Fig 7A, 7C and 7D, lanes 1-2). In KDP112, the molecular weights of these proteins were 78 kDa, 43 kDa, and 38 kDa, respectively. Consistent with defects in the maturation of fimbrial components, quantitative ELISA revealed that KDP112 expressed 50% less Mfa1 fimbriae than wild type (Fig 2B).

Discussion
Mfa4 is one of the accessory proteins incorporated into Mfa1 fimbriae [12,13], but its role has remained unclear. In this report, we describe genetic and biochemical approaches to investigate the role of the mfa4 gene in the assembly, structure, and function of Mfa1 fimbriae.
Incorporation of accessory components into mature fimbriae is common among gram-negative pathogenic bacteria such as uropathogenic E. coli, Neisseria meningitidis, and Pseudomonas aeruginosa [33][34][35][36]. The roles of some of these components are known. For example, accessory components that cap fimbrial tips facilitate adhesion, as in type I fimbriae and P pili in E. coli [37,38]. In P. gingivalis, a recent study demonstrated that the accessory proteins FimC-E are essential to maintain the structure and adhesive properties of FimA fimbriae [39].
Inactivation of mfa4 altered the cellular distribution of other accessory proteins. Immature Mfa3 accumulated in the inner membrane, whereas Mfa5 appeared to leak out into the culture supernatant. These effects reduce the amount of fimbriae displayed on the cell surface. The fimbriae themselves have altered composition when mfa4 is disrupted, contain only polymerized Mfa1, and are without accessory proteins. The control of fimbrial polymerization by CsgB, a minor component of an E. coli fimbrial structure known as curli, provides precedent. Specifically, CsgB is crucial for efficient polymerization of CsgA, the major subunit in curli [40].
Analysis of cell fractions from the fimA-deficient strain JI-1 shows that Mfa4 accumulates in the inner membrane. Because immature Mfa3 also accumulates in this fraction when mfa4 is absent, as in the strain FMFA4, it is tempting to speculate that Mfa4 regulates the transport of immature Mfa3, perhaps via a mechanism that resembles the chaperone-usher pathway, which is typically required to assemble various adhesive pili. In this system, individual pilus subunits reach the periplasm via the general secretory pathway, and are then folded by specific periplasmic chaperones and delivered to the outer membrane. At the outer membrane, subunits are assembled into pili by an usher [41]. However, a periplasmic chaperone-usher system for fimbrial proteins has not been found so far in P. gingivalis. Nevertheless, it has been shown that FimA and Mfa1 are trafficked via a unique transport and assembly mechanism that generates a lipoprotein intermediate. A leader peptide is also cleaved off by signal peptidase II and RgpA/B prior to polymerization at the cell surface [16,42].
Mfa5 is thought to belong to a family of C-terminal domain proteins secreted via the Por secretion system [43], a unique secretion apparatus in P. gingivalis [44,45]. Thus, Mfa5 may be secreted to the outer membrane via mechanisms not used for other proteins in the mfa gene cluster. Notably, C-terminal domain proteins are extensively modified with A-LPS and migrate as diffuse bands in SDS-PAGE with molecular mass generally 20 kDa higher than would be expected from the sequence [46,47]. In this study, Mfa5 incorporated into Mfa1 fimbriae was found to migrate as two bands with molecular weight 130 kDa and 150 kDa (Fig 4, lane F). As the first corresponds to the calculated molecular mass of 134495.35 Da, the second therefore appears to be Mfa5 decorated with A-LPS. Because modified Mfa5 was not detected in cellular fractions of FMFA4, and was released to the culture media (Fig 4), it is likely that A-LPS anchors Mfa5 to the extracellular side of the outer membrane. However, the direct role of Mfa4 in these processes is still unclear.
FMFA4, which expresses defective Mfa1 fimbriae lacking Mfa3-5, strongly auto-aggregates and robustly forms biofilms compared to JI-1. Notably, these activities are similar to levels in SMF-fimA, even though Mfa1 fimbriae are still expressed on the cell surface at 43% of JI-1 ( Fig  2B). On the other hand, auto-aggregation and biofilm formation are diminished to the same extent as JI-1 in the complemented strain FMFA4C, which expresses structurally intact Mfa1. These data demonstrate that accessory proteins strongly influence fimbrial structure and function.
Similarly, the adhesive properties of P. gingivalis FimA fimbriae depend crucially on the accessory proteins FimC-E [32,48]. In addition, Wang et al. [39] proposed that these accessory proteins are essential for virulence in experimentally induced periodontitis. A very recent study also found FimC-D to be involved in invasion of human oral keratinocytes and gingival fibroblasts [49]. It is obvious from these reports that FimA accessory proteins are functionally significant. Therefore, further work may also find critical roles for Mfa1 accessory proteins, perhaps in co-aggregation with oral streptococci or in interaction with host cells.
In the strain KDP112, from which there is complete loss of Rgp protease activity, unprocessed and immature Mfa1, Mfa3, and Mfa4 were detected. The defect in fimbrial protein processing decreases the expression of surface Mfa1 fimbriae by 42.5% (Fig 2B). Note that unprocessed Mfa1 could be detected at the cell surface by filtration ELISA because the antiserum against Mfa1-only fimbriae reacted with both Mfa1 monomers and oligomers. However, electron microscopy of KDP112 indicates that fimbriae are hardly observed on the cell surface [19], suggesting that RgpA/B is important for the formation of structurally sound fimbriae.
In conclusion, Mfa4 facilitates the incorporation of accessory proteins into Mfa1 fimbriae, not only by promoting maturation of Mfa3 but also by stabilizing Mfa5 at the cell surface. In this manner, Mfa4 mediates the formation of Mfa1 fimbriae and ultimately modulates biofilm formation. Furthermore, Rgp proteases process Mfa1, Mfa3, and Mfa4 to maturity.
Supporting Information S1 Fig. Expression and subcellular distribution of Mfa2. Cultures of P. gingivalis JI-1 and FMFA4 were harvested by centrifugation and fractionated into whole-cell lysate (W), soluble (Sol), envelope (Env), inner membrane (IM), and outer membrane (OM) fractions. The culture supernatant (CS) was also analyzed after ammonium sulfate precipitation. Samples were boiled at 100°C for 5 min in a buffer containing SDS and 2-mercaptoethanol, and were then subjected to western blot using antibodies raised against Mfa2. (TIFF)