Pore-Forming Toxins During Bacterial Infection: Molecular Mechanisms and Potential Therapeutic Targets.

Bacterial infections are predominantly treated with antibiotics, and resistance to antibiotics is becoming an increasing threat to our health. Pore-forming toxins (PFTs) are virulence factors secreted by many pathogenic bacterial strains, both in acute and chronic infections. They are special membrane-targeting proteins that exert toxic effects by forming pores in the cell membrane. Recent studies have elucidated the structure of PFTs and the detailed molecular mechanisms of their pathogenicity. Here, we discuss recent findings that highlight the regulatory mechanisms and important roles of two types of PFTs, α-PFTs and β-PFTs, in mediating the virulence of bacteria, and the therapeutic potential of targeting PFTs for antibacterial treatment. Therapeutic strategies based on PFTs are highly specific and may alleviate the issue of increasing resistance to antibiotics.

Introduction

Currently, most bacterial infections are treated with one or more antibiotics, but antibiotic resistance has become a significant concern, and has led to the need for new therapy targets and strategies to combat bacterial infections. Pore-forming toxins (PFTs) are produced by a variety of organisms that are widely found in eukaryotes and prokaryotes, including pathogenic bacteria.1,2 They act as crucial virulence factors in the pathogenicity of bacteria by destroying the cell barrier and promoting the survival of pathogenic bacteria under various stimuli and harsh environmental pressures.3 PFTs also can attack the human innate and adaptive immune defense systems, enabling the pathogen to persistently attack the host. Reducing the production of PFTs or interrupting their pathogenesis are therefore important steps to reduce their pathogenicity. PFTs are divided into two categories, α-PFTs and β-PFTs, according to the secondary structure that binds to the cell membrane, namely α-helices or β-barrels.4 Both α-PFTs and β-PFTs are further divided into three families, respectively. The synthesis of various PFTs is regulated via co-ordination of a variety of transcriptional regulators,5,6 but the specific mechanisms of most PFTs are not clear. The PFT structure has recently been elucidated, which has provided the basis for a deeper understanding of its pathogenic mechanism.3,7 When initially secreted, PFTs are in the form of water-soluble monomers, and during the process of invasion, the monomers undergo specific assembly, and oligomerize into a polymer that forms a transmembrane structure, which is the pore.8–11 This oligomerization process may occur before the PFT inserts into the cell membrane, or during interaction of the monomers with membrane receptors.12 It has become necessary to continuously develop new treatments to cope with the toxin-producing pathogens.

In this review, we have focused on Bacillus cereus and Staphylococcus aureus as examples. They are both clinically significant pathogenic bacteria with secreted PFTs as their primary pathogenic factors during infection. We focus on recent studies on the toxicity characteristics of two α-PFTs predominantly produced by B. cereus, namely non-hemolytic enterotoxin (NHE) and hemolysin BL (HBL), and two β-PFTs predominantly produced by S. aureus, namely γ-hemolysin and leukocidin A/B (also named leukocidin G/H) (LukAB). We discuss their synthesis pathways, and corresponding regulatory and pathology mechanisms. With this information we hypothesize potential therapeutic targets to interfere with PFT toxicity.

Synthesis of PFTs

HBL toxin comprises three subunits: HBL-B, HBL-L1, and HBL-L2, encoded by the genes hblA, hblD, and hblC, respectively.13,14 These three genes are located on the operon hblCDAB, and the promoter is located upstream of hblC.15 Alignment of the deduced amino acid sequences of the three proteins indicates significant similarity (20 to 24% identical), and structural analysis of the HBL protein shows that all three components are almost entirely composed of α-helices. HBL-B and HBL-L1 contain predicted transmembrane fragments of 17 and 60 amino acid residues, respectively, at the same position, while HBL-L2 has no predicted transmembrane fragments. These observed similarities indicate that the HBL components are produced by duplication of common genes. Similar to HBL, the coding genes of the three components of NHE, namely NHE-A, NHE-B, and NHE-C, are nheA, nheB, and nheC, respectively, and in an operon containing the three open reading frames (ORFs).16 There is a high degree of homology between NHE and HBL, and similarities between NHE-A and HBL-C, NHE-B and HBL-D, and NHE-C and HBL-A, are the most significant.17,18 The gene encoding γ-hemolysin is present in more than 99.5% of human S. aureus isolates.12 γ-Hemolysin is composed of three subunits: two S components (HlgA and HlgC), and an F subunit (HlgB).19 Unlike hblCDAB and nheABC, hlgACB comprises two transcription units. The first transcription unit comprises a single ORF, hlgB, which encodes an F subunit (HlgB), and the second unit comprises two ORFs, hlgA and hlgC, encoding two S components (HlgA and HlgC), respectively.20 The gene encoding LukAB is a part of the core genome of S. aureus, which exists in most genomes. It is composed of the S component, LukA/H, and the F component, LukB/G, and the sequence homology between the two components is unlike that of other toxins.21

Regulation of PFT Synthesis in Pathogens

HBL and NHE expression is regulated by multiple factors. For example, expression of the primary virulence factors of B. cereus, hblCDAB and nheABC, is regulated by the pleiotropic regulatory factor PlcR, redox regulator Fnr, two-component system ResDE, and the catabolic control protein CcpA, on the promoter regions of the two operons. These transcriptional regulatory factors may regulate toxin expression via a synergistic effect.22–24

PlcR is a small transcriptional activator that participates in the regulation of various virulence factors.25 During the exponential phase of bacterial growth, PlcR promotes specific interactions with PapR quorum sensing peptides.26 PlcR expression reaches its highest level at the beginning of the stationary phase of bacterial growth.25 High levels of PlcR activate most of the virulence factors, including the three components of HBL. PlcR appears to be a key regulator of the effective adaptation of B. cereus to the host environment. The transcription of another virulence factor, cytotoxin K, is also regulated by PlcR.27 PapR is a quorum sensing system signal molecule that is an autoinducing small signal peptide. It is secreted by bacterial cells and reintroduced into cells after processing.28 A previous study showed that a set of synthetic PapR derived peptides could inhibit the activation of many virulence factors. These small artificial peptides interfere with the normal quorum sensing systems and are a potential target as anti-toxin agents.26,29 Thus, novel small molecules that interfere with the quorum sensing systems, or facilitate the quorum quenching systems, may be selected as anti-virulence agents.

ResDE and Fnr are both regulators of redox regulatory pathways, and Fnr is a member of the iron-sulfur protein Crp/Fnr superfamily.30 ResDE is a typical two-component system (TCS) consisting of a membrane-bound histidine receptor kinase (ResE) and a cytoplasmic response regulator (ResD). ResE senses signals inside and outside the cell, such as oxygen limitation and NO, and undergoes autophosphorylation of the conserved histidine residues.31 ResD phosphorylation is achieved by transphosphorylation with ResE as a phosphate donor. The phosphorylated ResD acts as a transcription activator for the transcription of hblCDAB and nheABC. Phosphorylated ResD also interacts with Fnr to form a transcriptionally active complex.30,31 Fnr plays an important role in the fermentation and metabolism of B. cereus and the transcriptional regulation of the enterotoxins, HBL and NHE.22,32,33 CcpA is a member of the LacI family of transcriptional regulators. CcpA binds to a histidine-containing phosphocarrier protein to enable it to function as an effector. CcpA acts as a repressor to inhibit transcription in the catabolic regulation of HBL and NHE. The expression of NHE and HBL in CcpA-deficient strains is higher than that of the wild-type.22,31

The expression of γ-hemolysin and LukAB are strictly regulated by a highly complex, and multifaceted, regulatory network. An important regulator, accessory gene regulator (AGR) and several TCSs, such as S. aureus exoprotein expression RS (SaeRS), autolysis-related locus ArlRS, and staphylococcal respiratory response AB (SrrAB), are all involved in the regulatory systems.34–37 AGR acts as an activator of toxin production. At the population level, AGR is an auto-inducing peptide, which produces an effector RNA molecule, called RNAIII, in the process of activating its own synthesis. RNAIII acts as a direct or indirect regulator of many virulence genes, either up- or down-regulating their transcription and protein production.7 The SaeRS system is a key switch that regulates the production of leukocidins.34 It plays an important role in protecting microbial cells from exposure to the cytotoxic concentration of intracellular heme.38 In the ArlRS TCS, ArlS is a membrane-anchored sensor protein, and ArlR is an intracellular response regulator.37 The ArlRS two-component system inhibits the transcription of the Staphylococcus AGR operon via interaction with the AGR promoter. SrrAB regulates the pathogenic factors of S. aureus by directly binding the corresponding promoter region, including TSST-1, RNAIII, and protein A. SrrAB TCS is the main regulator of the respiratory growth and virulence of S. aureus.36

Pathogenicity of PFTs

Hemolysin HBL has been identified as a three-component toxin. Recent studies have demonstrated that the formation of pores in macrophages by HBL leads to the outflow of potassium ions, which triggers rapid cell death, and the pyrin domain-containing protein, NLRP3 inflammasome.39 HBL also has a variety of toxic effects, such as enteric toxicity, hemolysis, cytotoxicity, vascular permeability, and skin necrosis.40–42 It is a heat-sensitive protein comprising binding component B and two soluble components, L1 and L2, which assemble on the cell membrane in a specific order; B-L1-L2.43,44 HBL-B is the component believed to bind to the cell. The binding of HBL-B to target cells is a key step in the formation of the membrane pore, and pores will not form if there is insufficient B binding to the cells, or if there are excess quantities of L2 or L1 (Figure 1). Optimal pore-forming activity occurs when the B:L1:L2 ratio is 10:10:1.45 Of the three components, only HBL-B binds to Chinese hamster CHO cells in vitro, and one study showed that only HBL-L1, and not HBL-L2, binds to HBL-B.45 The three components of HBL are essential for its cytotoxicity and pore formation. The combination of any two components will not produce cytotoxicity, and maximum activity can only be exerted when all three components are present at the same time, and in the correct ratio.46

Figure 1

A brief summary of the regulation and pathogenic mechanisms of two typical α-PFTs, non-hemolytic enterotoxin (NHE) and hemolysin BL (HBL) toxins. The promoter regions of hblCDAB and nheABC are regulated by pleiotropic regulatory factor PlcR (along with the quorum sensing system signal molecule PapR), redox regulator Fnr, catabolic control protein CcpA, and two-component system ResDE. The three components of HBL and NHE were secreted and assemble on the cell membrane to form the pore in a specific order; B-L1-L2 and C-B-A. NHE and HBL cooperate to influence the secretion of K+ and activate an inflammatory response.

The non-hemolytic enterotoxin, NHE, is a homolog of HBL, and another important toxin secreted by B. cereus. Single, or combinations of two NHE components cannot induce hemolysis; maximum activity is only achieved when all three subunits (NHE-A, NHE-B, and NHE-C) interact in a molar ratio of 10:10:1.44 This was confirmed in a eukaryotic, cell-free protein synthesis system using the three purified proteins, which showed that the toxicity of NHE was diminished when NHE-C was present at higher concentrations. NHE-B and NHE-C form a complex that was shown to directly bind to Vero kidney epithelial cells; however, only NHE-C was required to induce cytotoxicity.44 NHE-A is dispensable for initial cell binding, but necessary for cytotoxic effect.47,48 NHE was recently reported to induce rapid cell death via the NLRP3 inflammasome, and NHE and HBL cooperate to activate an inflammatory response.49 Compared with the wild-type, the cytotoxicity of the Δnhe mutant was shown to be reduced, and the B. cereus Δhbl and Δnhe mutant strain failed to activate the NLRP3 inflammasome.39,41,49 Based on this feature, screening small molecules to target one of these components, in particular HBL-B or NHE-C, may be an effective strategy to inhibit the cytotoxicity of HBL and NHE.

The pore-forming γ-hemolysin and LukAB secreted by S. aureus are members of the β‑PFT family and consist of two different monomeric protein components.50 According to their chromatographic elution characteristics, these are named the S and F subunits, where S and F represent slow elution and fast elution, respectively.51 The S component is responsible for recognizing and binding to the cell membrane receptors, and recruiting the F component to dimerize through conformational changes. These proteins bind to the host leukocyte membrane and form beta-barrel pores that span the phospholipid bilayer (Figure 2).52 γ-Hemolysin exhibits lytic activity on human and rabbit cells and recognizes and binds to the red blood cell membrane as an octamer through direct interaction with host lipids and glycolipid derivatives.19 γ-Hemolysin HlgCB targets the human complement membrane receptors, C5a anaphylatoxin chemotactic receptor 1 and C5a anaphylatoxin chemotactic receptor 2, to mediate interaction with the cell membrane.53 γ-Hemolysin HlgAB also induces human phagocyte cell death by interacting with the chemokine receptors, chemokines CXC chemokine receptor 1 (CXCR1), CXCR2 and CC-chemokine receptor 2 (CCR2).12 This interaction appears to be species specific as, in a mouse model, HlgAB did not bind to the mouse neutrophil CCR2 receptor. In addition to the formation of induction pores, HlgAB and HlgCB can also induce pro-inflammatory reactions, which have been shown to be related to the pathogenesis of septic arthritis.12,19,54 Studies show that the S. aureus USA300 strain, lacking hlgABC, has less ability to form pores in human neutrophils than wild-type strains, and the mutant strain can improve the survival rate in a mouse bacteremia model.55

Figure 2

The pore-forming process of two β-PFTs. The water-soluble monomers S subunits (HlgA and HlgC) and one F subunit (HlgB) of γ-hemolysin target the receptors C5aR and C5L2 on the cell membrane. These proteins form beta-barrel pores that span the phospholipid bilayer. LukAB are pre-assembled into heterodimers in solution. Four LukAB heterodimers form an octamer on the cell membrane through direct interact with the receptor CD11b. The potential therapeutic targets are highlight by pentagram.

LukAB, with a molecular weight of 75KDa, is a newly discovered member of the two-component interleukin family.56 LukAB fundamentally differs from the other two-component toxins in its mechanism of toxicity. The monomers are pre-assembled into heterodimers in solution, and these insert into the cell membrane and recruit other heterodimers to finally form an octamer β-barrel pore spanning the phospholipid bilayer (Figure 2).50 The individual subunits are not cytotoxic.57 Compared with other leukotoxins, this unique assembly method eliminates the pore formation process, and seems to increase the toxicity of LukAB. The ability of LukAB to cause disease in the body is largely due to its precise targeted killing of specific immune cells, including neutrophils, monocytes, macrophages, and lymphocytes, to avoid the hosts natural immunity.57,58 LukAB promotes bacterial survival by facilitating their escape from the neutrophils after phagocytosis.19,59 LukAB interacts directly with CD11b via the binding site in the I domain.60,61 As LukA and LukB are secreted as monomers and form heterodimers before recognizing and binding to receptors on the cell membrane, it would seem unlikely to be able to inhibit the toxic effect by inhibiting the dimerization of LukA and LukB. A better strategy may be to interfere with the binding of the LukAB complex to the cell, or with dimer oligomerization into the pore complexes. The I domain of mouse CD11b differs from human CD11b, which results in a weaker affinity of LukAB with mouse CD11b. Thus, even when mouse leukocytes express high levels of CD11b they have a greater tolerance to high doses of toxins.19

HlgAB, HlgCB, and LukAB can also activate NLRP3 inflammasomes in macrophages and monocytes, and promote their lysis and pro-inflammatory activity.62 These two types of pore-forming toxins mediate cell death by inserting into the cell membrane to “dissolve” the cell membrane.7 The formation of pores leads to a K+ efflux, considered to be the key factor for activation of the NLRP3 inflammasome. The NLRP3 inflammasome then initiates the release of caspase-1-dependent cytokines, IL-1β and IL-18, and induces cell necrosis.63

Potential PFT-Derived Strategies for the Treatment of Bacterial Infections

Antibiotics are, and have always been, the primary treatment for bacterial infections. However, with the continuous mutation of drug-resistant strains, and the overuse of antibiotics, the antibiotic-based treatment strategy needs to be challenged.64 It is worth noting that with the continuous progress of research, a variety of treatment methods have been explored and innovated. PFTs are a powerful tool in the pathogen’s armor to attack and resist the host organism. Potential treatment strategies based on PFTs can be divided into two parts: targeting the PFT-producing strains, and targeting the host cells after infection.

Strategies for Targeting PFT-Producing Strains

We put forward three possible avenues to reduce the virulence of PFTs-producing strains: toxin synthesis, toxin secretion, and the process of invasion. The coding genes of most PFTs are in an operon. siRNAs or microRNAs can be used to directly decrease the expression level of the PFTs. siRNAs are currently used in the treatment of cancer and present as a promising treatment for diseases caused by bacterial infections. However, it is a challenge to accurately deliver the siRNA into the PFTs producing strains, while avoiding the degradation and removal of siRNAs in the host cells. Therefore, the development of safe and effective delivery systems is crucial to the application of siRNAs as a treatment strategy to reduce toxin synthesis. Currently, various of siRNA delivery systems have been proposed, such as chemical modification of siRNA, lipid-based siRNA delivery systems, polymer-based siRNA delivery systems, and conjugate siRNA delivery systems.65 The conjugate siRNA delivery system involves covalently linking the siRNA with small molecules and antibodies to improve targeting to specific cells.66 Antibodies to bacterial cell wall components are the preferred choice to link to siRNAs, enabling far more accurate delivery of the siRNA. Research into effective delivery systems has room for innovation.

Many PFTs, such as HBL and NHE, contain Sec-type signal peptides that are necessary for secretion through the Sec pathway.67 SecA, the ATPase motor of the Sec pathway, is unique to bacteria, and is thus an ideal target for the development of novel antibacterial agents.68 Some in vitro studies have confirmed that certain antibacterial effects can be achieved using SecA inhibitors, and a variety of SecA inhibitors have been discovered and designed, such as azide compounds, imino-containing molecules, pannomycinan, 5-cyano-6-aryl-2-thiouracils derivatives, thiazolo [4,5-d] pyrimidine derivatives, and indole derivatives.69–71 However, whether these inhibitors can achieve the conditions and standards used for in vivo treatment need to be further explored.71 The Sec system is widely used in various strains and inhibiting this system may disrupt the normal metabolism and balance of beneficial gut microbiota. Thus, therapeutics that target PFTs themselves are a more effective alternative to inhibitors and antibiotics for the treatment of pathogenic infections.72,73 Thirdly, PFTs are cell-specific and recognize lipid, sugar, and protein receptors on the cell membrane. Surface binding to target cells leads to an increase in the concentration of PFTs and promotes the formation of oligomers. This is a key step in the formation of the pores in the cell membrane that destroy the epithelial barrier and cellular structure to promote bacterial growth. Interfering with the formation of these pores in an appropriate ratio may be an effective therapeutic strategy. In S. aureus some compounds, including Oroxylin A, Oroxylin A 7-O-glucuronide (OLG), Oroxin A (ORA), and Oroxin B (ORB), have been shown to bind to α-hemolysin and inhibit the self-assembly process, thus making it impossible to form pores in the membrane.74,75

Strategies for Targeting the Host Cell After Infection

Previous studies have shown that monoclonal antibodies (mAbs) are effective in the treatment of experimental models of infection by PFTs.76 For example, two cross-neutralizing leukocidin mAbs, SAN177 and SAN481 can cross-neutralize a variety of toxins, including HlgAB and HlgBC, by binding to the F subunit of the toxin.77 The human LukAB antibody can be combined with toxin monomers or dimers to neutralize cytotoxicity.78 Similarly, the use of monoclonal antibodies to neutralize α-PFTs is worthy of further investigation. Recent studies have also shown that nanoparticles and toxins coated with a biofilm can effectively neutralize toxins, and the development of this kind of nanotoxoid vaccine is expected to slow down the threat of many types of toxins.79,80 Furthermore, single-stranded DNA or RNA oligonucleotides, named aptamers, are screened against α-toxin-induced cell death. These aptamers inhibit toxin-mediated activation of the transcription factors TNF-α and IL-17. However, development of agents based on these aptamers for the treatment of infections need further exploration.74

Specific receptors on the cell surface are the key to the toxic effects of β-PFTs, and some receptors are shared by multiple toxins. Therefore, the inhibitors of specific receptors may be used to simultaneously slow the effects multiple toxins. Current studies have shown that the C5a receptor is the co-receptor of HlgCB and another β-PFT, Panton-Valentine Leukocidin (PVL), on the surface of human immune cells, and a variety of C5a receptor inhibitors have been demonstrated in in vitro experiments. This inhibition has a significant effect on neutralizing the PVL toxin, but the effect on the HlgCB toxin is not obvious.53 Therefore, it is feasible that an inhibitor may block the interaction between the toxin and the C5aR without interfering with the normal C5aR immune function. Further research to better understand the mechanism involved here is required.

PFTs form pores in the cell membrane and change the permeability of the cell, which results in increased Ca2+ inflows, and the stimulation of Ca2+-dependent repair mechanisms. Compared with the protein pores caused by mechanical damage of the cell membrane, the pores formed by PFTs are proteolipid pores which have certain boundaries. These proteolipid pores are considered to stimulate two main repair mechanisms; shedding and endocytosis,81 both of which remove damaged membranes through vesicles or endocytosis.81,82 Recent studies have shown that Ca2+-activated lipid scramblase TMEM16F can enhance the fluidity and plasticity of the membrane, and the release of damaged membrane bubbles, to promote the repair of the plasma membrane after pore formation.83 To treat cellular inflammation caused by Ca2+ outflow mediated by PFTs, some studies have proposed the use of DNA aptamers to inhibit toxin-mediated cytolysis and activation of transcription factors, but this protective mechanism needs further exploration.84

Conclusion

Pathogenic bacteria secrete various virulence factors to attack host cells; PFTs being one of the most complex of these. This review has highlighted the synthesis of two types of PFTs, α-PFTs and β-PFTs. The regulatory systems especially transcriptional regulatory factors have been concluded which provided several potential targets for therapeutic. The invasive mechanism of these two types PFTs are also discussed. Though PFTs are not very widely spread, these various toxins are mostly participated in destroying the host immune system in different ways to mediate different cellular responses, which leading to high levels of resistance to the innate and adaptive immune defenses.3,7 These effects lower the immunity of the host and trigger more infections. Though deletion of PFTs will not completely protect from disease in animal models, it will be helpful in enhancing the immunity. Therefore, an in-depth exploration of the structure of toxins secreted by these pathogens, and their pathogenic mechanisms have enabled us to understand the heterogeneity of pore formation more clearly.

Overall, we propose several potential strategies based on our understanding of PFTs, with particular emphasis on their biosynthesis and pathogenic features. The possible strategies are focused mainly on the synthesis, secretion, and invasion process of PFTs. Such as SecA inhibitors and some compound like Oroxylin A and its derivatives which can bind to α-hemolysin to inhibit the pore-forming process. Furthermore, targeting the host cell after infection are also important strategies that can decrease pathogenicity or facilitate recovery of the host cells. Here, we discussed the application of monoclonal antibodies, nanoparticles and DNA aptamers. Further studies are warranted for the application of these strategies to treat PFT-induced diseases. A better understanding of the mechanisms of action of PFTs may aid in the design of novel strategies for the prevention and treatment of bacterial PFT-induced diseases.