1. Introduction
Invasion of host cells by the facultative pathogen
Serratia proteamaculans 94 arises at the stationary growth phase when the density of the bacterial population is maximal [
1]. In response to changes in the density of the population, the Quorum Sensing System (QS) regulates gene expression involved in controlling the lifestyle and activity of bacteria, including the activity of their virulence factors.
S. proteamaculans 94 has a LuxI/LuxR type QS system consisting of AHL synthase SprI and regulatory receptor protein SprR. In a classical
Aliivibrio fischeri [
2] LuxI/LuxR QS model, AHLs’ binding stabilize the LuxR-type proteins, allowing them to bind DNA and activate transcription of target genes [
3], including the LuxI-type AHL synthase gene. In this QS model, expression of the AHL synthase gene requires AHL activation of the LuxR protein. However, the QS system of
S. proteamaculans 94 is different from the
A. fischeri QS system: the AHL synthase
sprI gene and the
sprR gene encoding a receptor protein are convergently transcribed and overlapped in their terminal areas [
4]. In contrast to the classical QS system of
A. fischeri, AHL synthesis by the
S. proteamaculans 94 does not depend on the SprR regulatory receptor protein [
5]. Accordingly, only a mutation in the AHL synthase
sprI gene, but not a mutation in the receptor
sprR gene, led to a decrease in exoprotease and chitinolytic activities and the ability to form biofilms by
S. proteamaculans 94 [
5].
Previously, we have shown that inactivation of the AHL synthase
sprI gene resulted in the increase in invasive activity of
S. proteamaculans preceded by the increased bacterial adhesion to the cell surface [
6]. By our data, the increased adhesion of
S. proteamaculans SprI(-) could be caused by both an increase in the expression of the surface protein OmpX responsible for adhesion [
6,
7,
8] and a decrease in the activity of protease protealysin, whose substrate is OmpX [
7,
8]. On the other hand, the AHL signaling molecules can directly affect host cells and their multiple signaling pathways by triggering calcium mobilization, activation of Rho GTPases, MAPK, and NFκB that control diverse host cells functions and behaviors, including cytoskeleton remodeling [
9]. In epithelial cells, AHL interacts with the GTPase-activating proteins which lead to phosphorylation of Rac1 and Cdc42 [
10]. Phosphorylation of these Rho GTPases leads to their activation, and this may be a necessary stage of bacterial invasion [
11]. Therefore, bacteria
S. proteamaculans SprR(-) with an inactivated SprR receptor that does not affect the AHL synthesis have become an excellent model for assessing the direct effect of signaling AHL molecules on the host cell. The aim of the present work is to unravel the effect of inactivation of the regulatory AHL-receptor SprR on the
S. proteamaculans invasive activity and the activity of known virulence factors.
Our results show that, in contrast to the inactivation of the AHL synthase
sprI gene [
6], inactivation of the regulatory receptor protein
sprR gene does not lead to an increase in the expression of the surface protein OmpX, which is responsible for adhesion, and does not affect the activity of protease protealysin, the substrate of which is OmpX. Despite the absence of an effect on adhesion, inactivation of the
sprR gene leads to an increase in the invasive activity of
S. proteamaculans correlated with the increase in the activity of extracellular metalloprotease serralysin, which is cytotoxic to mammalian cells. In addition, the inactivation of the
sprR gene as well as inactivation of the
sprI gene [
6] results in a loss of the
S. proteamaculans’ ability to adapt to iron-limiting conditions. This can be a key factor in influencing the spread of infection in the body, because iron content in the body is limited during infections due to sequestration by host proteins such as lactoferrin, transferrin, and haemoglobin. These results indicate that inactivation of both proteins of the LuxI/LuxR-type QS system through independent mechanisms leads to a similar increase in the invasive activity of
S. proteamaculans and prevents this effect under iron-limited conditions typical of the human body.
2. Materials and Method
2.1. Cell Cultures, Bacterial Strains, and Growth Conditions
Human cervical carcinoma cells M-HeLa and embryonic mouse fibroblasts transformed with SV40 virus (Balb 3T3-SV40) were obtained from the Vertebrate Cell Culture Collection (Institute of Cytology, St. Petersburg, Russia) supported by the Ministry of Science and Higher Education of the Russian Federation (Agreement №075-15-2021-683). M-HeLa cells were grown in α-MEM (Minimum Essential Medium α) supplemented with 1% NEAA (Non-Essential Amino Acids) medium, and 3T3-SV40 cells were grown in DMEM (Dulbecco’s Modified Eagle Medium). The cells were grown in the antibiotic-free media supplemented with 10% fetal bovine serum (Sigma, Darmstadt, Germany) at 37 °C under 5% CO2 atmosphere, for the time required to get 70–90% confluent (usually 18–40 h).
The wild-type
Serratia proteamaculans strain 94 (
S. proteamaculans (w.t.)) was isolated as described earlier [
12].
S. proteamaculans SprR(-) carrying the inactivated receptor gene was obtained by inserting a suicide vector into the
S. proteamaculans 94
rif-r chromosome by homologous recombination using the sacB-based strategy [
13], as described earlier [
5]. This suicidal vector for the
sprR gene contained the full-length 750 bp
sprR gene with the insert 865-bp fragment from the p34S-Gm plasmid bearing the gentamicin resistance [
5]. To replace the native sprR gene in
S. proteamaculans with the defective gene, the vector was transferred to the
S. proteamaculans strain by conjugation of
S. proteamaculans and
Escherichia coli S-17 strains carrying the pEX18Tc plasmid with an inactivated
sprR gene. Rifamycin resistance was necessary for the subsequent separation of
S. proteamaculans from
E. coli. PCR was used to test the insertion of the gentamicin resistance gene into the
sprR gene. After inactivation of the
sprR gene, bacteria acquired the gentamicin resistance gene and the size of the
sprR PCR product increased as a result of the insertion of the gentamicin resistance gene. We have verified that
S. proteamaculans 94
rif-r carrying an additional spontaneous mutation of rifampicin resistance did not have higher invasive activity than the wild-type
S. proteamaculans 94. Inactivation of the
sprR gene did not affect the expression of the
sprI gene (not shown), synthesis of AHL, chitinolytic activity, or swimming mobility [
5].
S. proteamaculans were grown in Luria broth (LB medium) in the absence or presence of 0.3 mM 2,2′-bipyridyl at 30 °C with agitation speed controlled at 150 rpm for 21 h or 44–48 h until actinase activity on the
S. proteamaculans extract could be determined [
1]. The aliquots of every bacterial culture were diluted with growth medium to the equal optical densities at 600 nm.
2.2. Limited Proteolysis Assay
Rabbit skeletal muscle actin used as a substrate for protealysin was isolated by a standard procedure of Spudich and Watt [
14]. G-actin in buffer G (0.2 mM ATP, 0.1 mM CaCl
2, 5 mM Tris-HCl, pH 7.5, 0.02% NaN
3) was stored as aliquots (1–3 mg/mL) at −20 °C for a single use. To determine the ability of bacterial extracts to cleave actin, bacteria were pelleted by centrifugation at 12,000×
g for 10 min, the pellets were re-suspended in buffer G, and the bacteria were lysed by seven cycles of freezing and thawing. The bacterial extracts were clarified by centrifugation at 12,000×
g for 10 min. The clarified bacterial extracts were mixed with an equal volume of actin and incubated for 18 h at 4 °C. The reaction was stopped by the addition of an equal volume of the electrophoresis sample buffer containing 4% SDS, 125 mM Tris-HCl, pH 6.8, followed by a 5 min boiling. The digestion products were analyzed by SDS PAGE [
15]. The actinase activity was determined by the appearance of the 36 kDa fragment resulting from the cleavage of actin by protealysin.
2.3. Hemolysis Assay
To determine hemolytic activity of
S. proteamaculans, the standard hemolysis assay with erythrocytes was used [
16], with modifications [
17]. Horse erythrocytes were a generous gift from Maria Sergeeva (Research Institute of Influenza, Saint Petersburg, Russia). Washed erythrocytes were suspended in PBS to a final concentration of 2%.
S. proteamaculans were grown for 48 h, and their extracts were tested for the actinase activity [
1]. The aliquots of every bacterial culture were diluted with growth medium to the equal optical densities at 600 nm. Bacteria were pelleted by centrifugation at 12,000×
g for 10 min, resuspended in 100 µL PBS, and the bacteria suspension was added to 1 mL of erythrocyte suspension for 1 h at 37 °C and then centrifuged for 3 min at 2000×
g. The absorbance of released hemoglobin was measured at 405 nm. Hemolytic activities are presented as the percentage of the total erythrocytes lysed by 4% SDS.
2.4. Zymography with Gelatin
The ability of extracellular bacterial protease to cleave gelatin was performed by zymography. Bacteria were grown in the LB medium for 48 h, then the growth medium (conditioned medium) was clarified, incubated with electrophoresis sample solution (62.5 mM Tris–HCl, pH 6.8, 0.1% SDS) for 30 min at the room temperature, and analyzed by SDS-PAGE, which is different from a regular SDS-PAGE due to the presence of 0.3% gelatin in the resolving gel. After electrophoresis, the gel was washed twice with 2.5% Triton X-100 to remove SDS and incubated in 5 mM CaCl2, 50 mM Tris–HCl, pH 7.2–7.4, for 18 h at 37 °C to renature the proteases and carry out proteolysis. Finally, the gel was fixed in 25% isopropanol with 10% acetic acid for 30 min and stained with Coomassie brilliant blue G-250.
2.5. Proteolysis of Azocasein
The reaction mixture consisted of 100 µL of azocasein (10 mg/mL) in 50 mM Tris–HCl, pH 7.2, and 50 µL of the conditioned media of S. proteamaculans (grown for 48 h) was incubated at 37 °C for 60 min. The reaction was quenched by the addition of 200 µL 10% trichloroacetic acid for 10 min at 20 °C. After centrifugation at 12,000× g for 5 min, 250 µL of supernatant was mixed with 50 µL 4 M NaOH, and the absorbance was determined at 450 nm.
2.6. Fluorescence Microscopy
Bacteria were grown as described above until the actinase activity of
S. proteamaculans extracts could be detected [
1]. Thirty minutes before the experiment, bacteria (1 mL) were pelleted at 9600 g for 10 min; the pellets were resuspended in FITC (1 mg/mL) of the bacterial culture to visualize the bacteria. Bacteria were pelleted at 9600 g for 10 min; the pellets were resuspended in 100 µL DMEM and added to the host cells in a 1 mL fresh portion of DMEM. The host cells and bacteria were co-cultivated at 37 °C in 5% CO
2 for 3 h. Cells were washed three times with PBS solution at each staining step. The preparations were fixed with 3.7% formaldehyde solution (Sigma, Darmstadt, Germany) for 10 min, incubated for 5 min with 0.1% Triton X100 and stained with rhodamine-phalloidin (Sigma, Darmstadt, Germany) for 15 min to visualize the actin cytoskeleton. The samples were mounted in the mounting medium and analyzed with a confocal fluorescence Leica SP5 TCS microscope using dual 488 nm (green fluorescence) and 543 nm (red fluorescence) laser system to visualize the FITC-stained bacteria and the rhodamine–phalloidin-stained cytoskeleton, respectively.
2.7. Quantitative Adhesion and Invasion Assay
Efficiency of invasion and adhesion was evaluated by the quantitative invasion assay [
8,
18]. Bacteria (1 mL) were pelleted at 9600×
g for 10 min; the pellets were then resuspended in 100 µL DMEM and added to the host cells in a 1 mL fresh portion of DMEM. After co-cultivating host cells and bacteria at 37 °C in 5% CO
2 for 1–2.5 h, unattached bacteria were washed out twice with PBS and the infected cells were suspended in 0.25% trypsin–versene solution. To quantify the effectiveness of adhesion, suspension of the infected cells was quickly diluted and plated out on LB agar to determine the number of colony forming units (CFU) of adherent bacteria. To quantify the effectiveness of invasion, suspension of the infected cells was incubated in DMEM containing kanamycin to kill extracellular bacteria and then the cells were lysed with 1.5% sodium deoxycholate, quickly diluted with cold LB medium, and the aliquots of the resulting suspension were plated on LB agar to determine the number of colony forming units (CFU) of intracellular bacteria [
8]. The results for each experiment are the average of an assay performed in triplicate and independently repeated three times.
2.8. PCR Analysis
Genes’ expression was analyzed by semi-quantitative RT-PCR. Bacteria were grown for 21 h and pelleted by centrifugation at 12,000× g for 10 min. Total RNA was extracted from the bacterial pellet using an extraction kit (DiaM, Russia) according to the manufacturer’s instructions. Reverse transcription was performed with the RevertAid First Strand cDNA Synthesis Kit (Thermo Fisher Scientific, Waltham, MA, USA) and the resulting cDNA was diluted in H2O to 20 ng/mL. Gene-specific primer pairs designed using BLAST-primer software were as follows: for ompX gene, 5′-GCAGTAGCAGCCTGTGTATTA-3′ and 5′- TTGGGCGTTGTCGATGTT-3′; for serralysin gene, 5′-AGGCAACCCAACCTACAA-3′ and 5′-AACCGGAGAAGTCGAAAGT-3′; for protealysin gene, 5′-GGTGAAGTCATCCGCGATATT-3′ and 5′-ATCAGCCAGTCGGCTTTATC-3′; for ShlA gene, 5′-GCACAACGGACAGCTACTAT-3′ and 5′-GGATCTCGTCACCCTGAATATC-3′; and for S12 ribosomal protein gene, 5′-CAGAAACGTGGCGTATGTACT-3′ and 5′-CGAGCTTGCTTACGGTCTTTA-3′. The PCRs were optimized independently for each set of primers as follows: primary melting at 94 °C for 3 min, 30 amplification cycles (94 °C for 1 min, annealing temperature of 62 °C for 1 min, 72 °C for 1 min), and a final elongation step of 10 min at 72 °C. Amplified products were resolved on 1% agarose gels and visualized with SYBR Safe (Thermo Fischer Scientific) staining. Gene expression was evaluated relative to the constitutive expression of a S12 ribosomal protein gene. Three biological replicates were analyzed.
2.9. Statistical Analysis
Data were analyzed statistically using one-way analysis of variance (ANOVA) with the Excel Data Analysis Pack. A difference was considered significant at the p < 0.05 level.
4. Discussion
Bacteria coordinate gene expression by quorum sensing (QS) through the production of signal molecules. The N-acyl-L-homoserine lactones (AHL) signal molecules are used by LuxI/LuxR-type QS systems functioning in gram-negative bacteria [
19], and the autoinducer-2 (AI-2) signal molecules are used by LuxS-type QS systems in both gram-negative and in gram-positive bacteria [
20]. The synthesis of AHL and AI-2 depends on the LuxI and LuxS-type proteins, respectively. QS systems had been demonstrated to play a pivotal role in bacterial pathogenesis by regulating the expression of different virulence factors affecting adhesion, invasion, and survival within a tissue [
21]. Strategies aimed at manipulating QS regulation of bacterial virulence are viewed as especially promising. Nevertheless, the effect of the QS system on bacterial invasion, which is a key stage of virulence, has been shown only for LuxS type QS systems and is controversial both for different bacteria and for different host cells. The inactivation of the QS system significantly increased the internalization of
Pseudomonas aeruginosa [
22] and
Streptococcus pyogenes [
23], but reduced the invasiveness of pathogenic
Escherichia coli (APEC) [
24] and
Salmonella [
25]. Inactivation of the QS system of
Campylobacter jejuni had virtually no effect on invasion in Caco-2 cells [
26], but reduced invasion in INT407 cells [
27].
S. proteamaculans 94 has both the LuxS type QS system and the LuxI/LuxR type QS system consisting of AHL synthase SprI and regulatory protein SprR. Previously published data have indicated that the
luxS gene inactivation results in a mutant
S. proteamaculans 94 phenotype are very similar to AHL synthase gene inactivation phenotype [
4]. This indicates that both AHLs and AI-2 signal molecules in the
S. proteamaculans 94 strain could be involved in QS control of the same physiological and metabolic processes. We have shown that inactivation of the AHL synthase
sprI gene led to a more than fourfold increase in the invasive activity of
S. proteamaculans as a result of increased adhesion [
6]. This increase in the adhesion of
S. proteamaculans with inactivated AHL synthase gene can be caused by an increase in the amount of the surface protein OmpX and a decrease in the activity of the protease protealysin, the substrate of which is OmpX [
6,
7,
8]. These results allowed us to suggest that synthesis of AHLs controls the invasion of
S. proteamaculans by accumulation on the bacterial surface of full-length OmpX not cleaved by protealysin [
6].
Our present results show that inactivation of the
sprR gene led to a more than twofold increase in the invasive activity of
S. proteamaculans SprR(-). Thus, the direct effect of AHL signaling molecules on the host cells is not critical in regulating the intensity of
S. proteamaculans invasion. Moreover, the results of the present work show that inactivation of the
sprR receptor gene does not affect the amount of the outer membrane protein OmpX and the activity of protease protealysin cleaving OmpX which, in turn, does not lead to an increase in adhesion. Thereby, inactivation of the
sprR receptor gene led to an increase in the activity of the extracellular metalloprotease serralysin. Serralysin-like proteases secreted by
S. marcescens not only suppress cellular immunity by decreasing the adhesive properties of immunosurveillance cells [
28], but are also cytotoxic to mammalian cells [
29,
30,
31], thus contributing to bacterial pathogenesis. At the same time, inactivation of the AHL synthase
sprI gene did not lead to an increase in the activity of serralysin [
6]. Thus, inactivation of the
sprI and
sprR genes leads to an increase in the intensity of bacterial invasion as a result of the activation of different virulence factors.
The key point for the spread of infection is the regulation of the intensity of the invasion of opportunistic bacteria when they enter the human body. One of the factors signaling the entry of bacteria into the body is a decrease in the concentration of iron in the medium. Because the body’s environmental iron content is limited during infections due to sequestration by host proteins such as lactoferrin, transferrin, and hemoglobin, a decrease in the concentration of iron in the medium leads to the activation of the pore-forming toxin ShlA and an increase in the invasion of
S. proteamaculans [
17]. The pore-forming toxin ShlA not only has a cytotoxic effect on epithelial cells in a culture [
32], but is also necessary for invasion by
S. marcescens [
16]. The inactivation of both the
sprI gene and the
sprR gene resulted in the loss of the ability of
S. proteamaculans to adapt to iron-limiting conditions. The iron deficiency in the growth medium of bacteria with an inactivated QS system leads to the decrease in the invasive activity in the absence of an increase in toxin activity. These results indicate that inactivation of either of the LuxI/LuxR-type QS system proteins through different mechanisms leads to the increase in the invasive activity of
S. proteamaculans, but prevents an increase in invasion under iron-limited conditions typical of the human body.