Abstract
The emerging pathogen, Borrelia miyamotoi, is a relapsing fever spirochete vectored by the same species of Ixodes ticks that carry the causative agents of Lyme disease in the US, Europe, and Asia. Symptoms caused by infection with B. miyamotoi are similar to a relapsing fever infection. However, B. miyamotoi has adapted to different vectors and reservoirs, which could result in unique physiology, including immune evasion mechanisms. Lyme Borrelia utilize a combination of Ixodes-produced inhibitors and native proteins [i.e., factor H-binding proteins (FHBPs)/complement regulator-acquiring surface proteins, p43, BBK32, BGA66, BGA71, CD59-like protein] to inhibit complement, while some relapsing fever spirochetes use C4b-binding protein and likely Ornithodoros-produced inhibitors. To evade the humoral response, Borrelia utilize antigenic variation of either outer surface proteins (Osps) and the Vmp-like sequences (Vls) system (Lyme borreliae) or variable membrane proteins (Vmps, relapsing fever borreliae). B. miyamotoi possesses putative FHBPs and antigenic variation of Vmps has been demonstrated. This review summarizes and compares the common mechanisms utilized by Lyme and relapsing fever spirochetes, as well as the current state of understanding immune evasion by B. miyamotoi.
Introduction
Tick-borne diseases are among the top reported diseases to the US Centers for Disease Control and Prevention. This group of diseases include an array of viral, bacterial, and parasitic pathogens (e.g., Lyme disease, tick-borne relapsing fever, anaplasmosis, rickettsiosis, Powassan virus, tick-borne encephalitis virus, Colorado tick fever, Heartland virus, babesisosis) transmitted by the bite of certain species of hard and soft shell ticks from four genera (Ixodes, Dermacentor, Amblyomma, Ornithodoros) (1–3).
Intense research efforts are occurring worldwide in an attempt to understand, detect, control, treat, and eradicate these pathogens and their diseases. One step toward preventing and treating infectious diseases is to understand how pathogens evade host defenses to establish infection. Pathogenic Lyme and relapsing fever borreliae establish infection through one or more of the following mechanisms: physical barriers (e.g., slime layer of glycoproteins), migration to immunoprivileged sites, and hijacking host processes [e.g., inactivation of complement with factor H-binding proteins (FHBPs)]. The mechanisms utilized by the emerging relapsing fever pathogen, Borrelia miyamotoi, are currently uncharacterized. Herein, we review some mechanisms Lyme and relapsing fever Borrelia utilize to inhibit and evade host complement and humoral immune responses and relate these to mechanisms that might be used by B. miyamotoi.
Lyme Disease and Tick-Borne Relapsing Fever: Spirochetes, Vectors, and Diseases
Approximately 20 closely related pathogenic and non-pathogenic species of Borrelia form the B. burgdorferi sensu lato complex. Of these 20 species, at least five are classified as causative agents of Lyme disease (US: B. burgdorferi sensu stricto; Europe and Asia: B. afzelii, B. garinii, B. spielmanii, B. bavariensis) (4–10). Lyme borreliae are carried and transmitted by several species of Ixodes ticks (Ixodidae, hard shell) though the most common species are I. scapularis and I. pacificus in the US and I. ricinus and I. persulcatus in Europe and Asia.
Species of Ornithodoros ticks (Argasidae, soft shell) carry and transmit relapsing fever spirochetes. Several Borrelia spp. cause relapsing fever but B. hermsii, B. turicatae, B. crocidurae, B. hispanica, B. duttonii are more commonly encountered.
While the general rule is Ixodes transmit spirochetes of the B. burgdorferi s.l. complex and Ornithodoros transmit relapsing fever borreliae, there are exceptions. B. recurrentis is a louse-borne relapsing fever spirochete endemic mainly to sub-Saharan Africa. B. theileri causes bovine borreliosis and is transmitted by Rhipicephalus microplus, a hard shell tick that parasitizes livestock (11). B. lonestari and B. turcica, spirochetes genetically similar to relapsing fever borreliae, are found in the hard shell ticks, Amblyomma americanum and Hyalomma aegyptium, respectively (12, 13). Finally, B. miyamotoi is a relapsing fever spirochete vectored by the same Ixodes spp. that transmit species of the B. burgdorferi s.l. complex.
In terms of disease, several tick-borne diseases are associated with non-specific symptoms (i.e., a possibly self-limiting “influenza-like” illness characterized by malaise, fatigue, aches, fever, and chills) (Table 1). While infection with Borrelia spp. generally results in similar symptoms, some species-specific symptoms can arise (14, 15). Erythema migrans and arthritis are commonly associated with a B. burgdorferi s.s. infection but rarely with B. afzelii infection, which more commonly manifests in the dermatological condition, acrodermatitis chronica atrophicans. B. garinii is more commonly associated with neurological symptoms. Relapsing fever is characterized by recurring spirochetemia corresponding to recurrent episodes of high fever not seen with B. burgdorferi s.l. infections.
Table 1
| Disease | Vectora | Causative agent(s)a | Clinical symptom(s) |
|---|---|---|---|
| Lyme disease | I. scapularis (USA) I. pacificus (USA) I. ricinus (Europe, Asia) I. persulcatus (Europe, Asia) | B. burgdorferi sensu stricto (USA) B. afzelii (Europe, Asia) B. bavariensis (Europe, Asia; formerly B. garinii OspA serotype 4) B. garinii (Europe, Asia) B. spielmanii (Europe, Asia) | Symptom onset after exposure: early stage generally 3–30 days Influenza-like (e.g., mild fever, malaise, myalgia/arthralgia; B. burgdorferi s.s.) Erythema migrans (B. burgdorferi s.s., B. afzelii) Symptom onset after exposure: late stage generally >30 days Arthritis Acrodermatitis chronica atrophicans (B. afzelii) Neurological (Lyme neuroborreliosis, e.g., numbness, Bell’s palsy, stiffness of neck, declining memory, sleep disorders; B. burgdorferi s.s., B. bavariensis) |
| Tick-borne relapsing fever | O. hermsi O. turicata O. parkeri O. moubata | B. hermsiiB. turicatae B. parkerii B. duttonii | Symptom onset: ca. 7 days Influenza-like Recurring high fever Headache Myalgia Arthritis Approximately 3–10 febrile episodes (relapses) occur; mortality rates are variable but generally less than 5% |
| Hard tick-borne relapsing fever/Borrelia miyamotoi disease | I. scapularisI pacificus I ricinus I. persulcatus | B. miyamotoi | Symptom onset after exposure: ca. 15 days (85) Influenza-like Most common: Fever Malaise Headache Chills Arthritis/arthralgia Meningoencephalitis (immunocompromised patients) Rare (less than 10% of patients): Rash/erythema migrans Gastrointestinal (e.g., vomiting, nausea, diarrhea) Cardiac/respiratory (shortness of breath) Neurological (e.g., dizziness, confusion) Stiffness of neck |
| Louse-borne relapsing fever | P. humanus humanus | B. recurrentis | Symptom onset after exposure: ca. 4–8 days Recurring high fever Malaise Headache Chills Meningism Myalgia Nausea Vomiting Approximately 3–5 relapses occur; mortality rate varies greatly (30–70% without treatment during outbreaks) |
Overview of Borrelia diseases.
aCommonly encountered and studied vectors and causative agents are listed.
Borreliamiyamotoi
Borrelia miyamotoi s.s. strains were first isolated and cultured in Japan in 1995 from I. persulcatus and the blood of Apodemus argenteus (small Japanese field mouse) (16). Since this initial isolation, B. miyamotoi DNA has been identified in I. scapularis, I. pacificus, I. ricinus, and I. persulcatus across the Northern hemisphere (17–84). B. miyamotoi DNA has also been identified in humans with a suspected tick-borne disease; while B. miyamotoi is associated with disease, teasing out the details of an infection with this spirochete has proven difficult for several reasons (85–92).
First, diagnoses based on serology can be problematic and lead to false-negative diagnoses. Several antigens, including 4 of the 10 assayed in a Lyme Western blot, are shared among Lyme, relapsing fever, and B. miyamotoi spirochetes (93, 94). Although Lyme and relapsing fever Borrelia cause different diseases and occupy different niches, species in this genus share a high degree of genetic homology (95–98). Therefore, some degree of cross-reactivity occurs between B. miyamotoi antibodies and B. burgdorferi s.l. antigens (91).
Second, an adequate and appropriate immunocompetent animal model to study B. miyamotoi infection is only now beginning to take shape. Without an optimal animal model to identify characteristic symptoms and pathologies, we are left to interpret and extrapolate symptoms from complex human cases where disease pathology can be complicated by underlying or unreported medical conditions or coinfections. Previous attempts to infect immunocompetent Peromyscus leucopus mice (a common reservoir for B. burgdorferi in the US) with B. miyamotoi s.l. LB-2001 (US strain) had been unsuccessful leaving severe combined immune deficient (SCID) mice as the only available animal model (17). SCID mice infected with B. miyamotoi exhibit sustained spirochetemia, similar to infection with relapsing fever spirochetes (99). Recently, however, Wagemakers et al. (100) were able to successfully infect immunocompetent C3H/HeN mice with LB-2001 and demonstrate spirochetemia 2 days post infection (dpi). Three of the eight mice infected exhibited relapsing spirochetemia at 5 and 6 dpi. More studies are required to determine the optimal animal model for B. miyamotoi infection (101–103).
Finally, B. miyamotoi’s status as a pathogen has only recently been established. The first confirmed human infections were reported in Russia in 2011 (85) with more cases subsequently described in the US, Europe, and Japan (86–91, 104–107).
B. miyamotoi Infection and Disease
Much of the data available on B. miyamotoi infections come from retrospective serological analyses of banked patient samples, which provide valuable epidemiological information but can lack the detailed patient history or clinical aspects required to sufficiently define a disease. The available data depict an illness, currently termed B. miyamotoi disease or hard tick-borne relapsing fever that is similar to relapsing fever.
The patients described by Platonov et al. (85) reported tick bites, developed moderate or severe disease, and were hospitalized as a precautionary measure against more severe tick-borne diseases, particularly viral tick-borne encephalitis. In total, 46 patients were classified as having a confirmed B. miyamotoi infection with no detected current B. burgdorferi s.l. coinfection by PCR. Sera from all 46 patients reacted with whole cell lysates of B. burgdorferi, B. afzelii, and B. garinii. The most common symptoms were fever, headache, and malaise or fatigue (Table 2). Five patients reported recurrent fever with an average duration of 3.4 days, and 9 days between relapses, similar to infections with relapsing fever spirochetes. All patients were successfully treated with ceftriaxone or doxycycline.
Table 2
| Symptom | US (n = 51) | Russia (n = 46) |
|---|---|---|
| Fever, chills | 96% | 98%, 35%a |
| Headache | 96%b | 89% |
| Myalgia | 84% | 59% |
| Arthralgia | 76% | 28% |
| Malaise/fatigue | 82% | 98% |
| Rash/EMc | 8% | 9% |
| Gastrointestinal symptomsd | 6% | 30% (nausea) |
| 7% (vomiting) | ||
| Respiratory symptomse | 6% | naf |
| Neurological symptoms (dizziness, confusion, vertigo) | 8% | na |
| Stiff neck | na | 2% |
aFever and chills were reported in separate categories.
bAuthors noted in most patients the headaches were severe.
cUS patients were described as having a rash. Russian patients were noted for having a single erythema migrans.
dFor US patients, GI symptoms included nausea, abdominal pain, diarrhea, anorexia. For Russian patients, GI symptoms included nausea and vomiting.
eLabored breathing or short of breath.
fNot reported.
A similar series of cases were reported in the US in 2015 (91). Ninety-seven of 11,515 patient samples submitted by clinical laboratories for tick-borne disease analysis were PCR-positive for B. miyamotoi. Patients with known or suspected B. burgdorferi coinfection or a history of Lyme disease were omitted from further analysis. Fever, headache, and malaise were commonly reported among US patients with two patients reporting recurrent fever (Table 2). The duration of febrile episodes and the time between relapses were not reported. Spirochetemia was noted in US patients but was either not reported or documented in Russian patients. Strikingly, a rash or single erythema migrans of unknown origin was reported in 8 and 9% of US and Russian patients, respectively.
Some symptoms were different between the US and Russia patients, which suggest clinical manifestations vary by B. miyamotoi strain, similar to that seen with B. burgdorferi s.l. strains (Table 2) (108). Arthralgia was more common in US (76%) compared to Russian patients (28%), and leukopenia, thrombocytopenia, and elevated liver enzymes were found in some US patients but in none of the Russian patients. These differences may be explained by genetic differences between American and Asian type B. miyamotoi. Genetic analyses of B. miyamotoi isolates have revealed heterogeneity between, and a high degree of homology among, strains from the US (American types; I. scapularis, I. pacificus), Europe (European type; I. ricinus), and Asia (Asian type; I. persulcatus) (59, 109).
Detailed case reports are currently available for nine patients in the US, Europe, and Japan. For immunocompetent patients, symptoms were similar to those observed in the aforementioned studies (e.g., fever, headache, malaise) (86, 89, 90, 106, 107). One US patient did not seek treatment, providing additional evidence that B. miyamotoi can result in recurrent fever and be self-resolving, similar to other relapsing fever infections (92, 110). This patient experienced two episodes of fever separated by 3 weeks, significantly longer than in other B. miyamotoi or relapsing fever patients, with each episode lasting 4–5 days, on par with B. miyamotoi or relapsing fever patients.
The pathology of B. miyamotoi infection is dramatically different in immunocompromised patients, specifically those treated for non-Hodgkin’s lymphoma (NHL) with rituximab. Two patients treated with rituximab for NHL, one from the US (88) and one from the Netherlands (87), with reported recent tick bites developed meningoencephalitis. Motile spirochetes were detected in cerebral spinal fluid in both cases. Interestingly, glpQ was amplified and sequenced from both patient’s samples yet no anti-GlpQ antibodies were detected in the blood or cerebral spinal fluid of the European patient. IgM against B. burgdorferi was negative for both patients. Neither patient reported any of the commonly associated symptoms of a B. miyamotoi infection (e.g., fever, headache, myalgia, malaise). Instead, both patients exhibited neurological symptoms (cognitive processing defects, disturbed gait). A third patient from Germany, also treated with rituximab for NHL, developed Lyme neuroborreliosis-like symptoms (dizziness, vomiting, and headache) (111).
The Complement System
The complement system, composed of the classical, lectin, and alternative branches, is a crucial component of the immune system (Figure 1). Components of complement continuously circulate in blood making complement one of the first lines of defense against pathogens. Complement initiates an immune response by: (1) triggering phagocytosis through opsonization, (2) mediating inflammation through the release of chemotactic peptides, and (3) lysing cells via the membrane attack complex (MAC, also called the terminal complement complex or TCC) (Figure 1) (112).
Figure 1
The classical pathway is generally mediated by non-specific antibodies, immunoglobulin G (IgG) or IgM, binding a bacterial antigen. Importantly, recent studies have shown Borrelia-specific IgM is produced by a subset of B cells during infection and plays a crucial role in clearing Borrelia (113–121). The C1 complex, composed of C1q, C1r, and C1s, forms upon recognition of bound IgG or IgM. C1 cleaves C2 (C2a, C2b) and C4 (C4a, C4b). C4b covalently binds the target’s cell surface and complexes with C2a to form C3 convertase, which cleaves C3 into C3a and C3b. C3b covalently binds the target cell surface (opsonization, facilitates phagocytosis of foreign cells and cellular debris), while C3a remains soluble to act as a mediator of inflammation. C5 convertase forms when C3b binds C3 convertase. Not surprisingly, C5 convertase cleaves C5 into C5a, a soluble inflammatory mediator, and C5b. C5b binds the target cell surface and C6 forming C5b6, which binds C7 (C5b–7) then C8. The C5b–8 complex binds C9 (C5b–9) and facilitates polymerization of several additional C9 proteins. These polymerized C9 proteins form the transmembrane pore of the MAC allowing an influx of extracellular fluid and subsequent lysis of the target cell.
The lectin pathway is very similar to the classical pathway, differing only in the initiation steps. The lectin pathway is typically initiated through mannose-binding lectins, a group of pattern recognition receptors (PRRs) on host cells, binding specific sets of carbohydrates on foreign cells (pathogen-associated molecular patterns, PAMPs). The lectin and classical pathways converge at the cleavage of C2 and C4 by different mechanisms. In the lectin pathway, C4 and C2 cleavage occurs through mannose-binding lectin-associated serine proteases (112).
Like the classical and lectin pathways, the alternative pathway forms a C3 convertase, C5 convertase, and results in the formation of the MAC. Unlike the classical and lectin pathways, the alternative pathway may not require antibody–antigen or PAMP–PRR interactions for activation. Rather, this pathway is initiated through hydrolysis of C3 to C3(H2O), which is thought to occur continuously at low levels. The pathway is propagated through interactions with bacterial antigens or a lack of host surface markers (e.g., sialic acid, glycosaminoglycans, sulfated polysaccharides) (112).
Factor B, after binding C3(H2O), is cleaved by factor D into Ba and Bb resulting in C3(H2O)Bb, the fluid-phase C3 convertase (cleaves C3 to C3a and C3b). C3b binds the bacterial cell surface where it complexes with additional factor B. Factor D again cleaves factor B, which results in the second, predominant and cell-bound C3 convertase (C3bBb). This cell-bound C3 convertase is stabilized by properdin (C3bBbP). Binding of additional C3b to C3 convertase results in the formation of C5 convertase (C3bBbC3b), which cleaves C5 and initiates the formation of the MAC as described above.
Inhibition of the Mammalian Complement System by Borrelia and Ixodes
Regulation of complement is critical for survival of host cells (122, 123). Numerous mechanisms have evolved in hosts to prevent aberrant activation of complement on host cells including the use of complement regulatory factors and host cell surface components (e.g., sialic acid). Pathogens that inhibit host complement use mechanisms that are inextricably tied to host regulatory processes. Borrelia use several native proteins to inhibit complement [i.e., FHBPs or complement regulator-acquiring surface proteins (CRASPs), p43, BBK32, BGA66, BGA71, CD59-like protein] (124). The following sections focus on the complement regulators factor H (FH), factor H-like protein-1 (FHL-1), factor I (FI), C4b-binding protein (C4BP), and CD59.
At least for Lyme borreliae, resistance to complement varies by strain and species (125–130). Roughly, 10% of B. burgdorferi s.s. are serum resistant, and 90% are intermediately resistant to serum; 75% of B. afzelii isolates are resistant, and 25% are intermediate; 100% of B. garinii isolates are sensitive (specifically, OspA serotypes 3, 5, 6, 7); B. bavariensis (formerly B. garinii OspA serotype 4) is intermediately resistant. To the best of our knowledge, similar comparisons of multiple strains and species have not been published for relapsing fever Borrelia, though complement resistance is not universal among relapsing fever species among the strains observed. Resistance to complement is important for the transmission, survival, and dissemination of some Borrelia spp. in mammalian and rodent hosts and reservoirs (131). Many Borrelia spp., particularly Lyme borreliae, are masters of complement evasion due to the native anticomplement proteins some possess and the ability all infectious strains possess to co-opt tick and host complement regulatory proteins.
FH, FHL-1, and FI
Factor H is an ubiquitous 150-kDa soluble protein produced by diverse cell types throughout the human body (e.g., hepatic cells, fibroblasts, monocytes, endothelial cells) (132). FH consists of 20 short consensus repeats, while FHL-1 is a truncated variant of FH consisting of the FH N-terminal short consensus repeats 1 through 7. Both FH and FHL-1 are major direct regulators of the alternative complement pathway. In addition, FH and FHL-1 can directly regulate the classical and lectin pathways, though the regulatory roles in these pathways are minor compared to other classical and lectin regulatory mechanisms. Regulation is achieved through the recognition of self and non-self molecules via domains located on the C- and N-terminals, respectively (133–135). The C-terminal discriminates self from non-self through interactions with sialic acids, glycosaminoglycans, and sulfated polysaccharides, which are typically found only on host cells (136–140). FH binds self molecules with high affinity to prevent activation of complement. FH regulates the classical and lectin pathways by acting as a co-factor for FI. In this capacity, FH facilitates the serine protease activity of FI in cleaving and inactivating C3b. The alternative pathway is regulated through FH targeting factor Bb, which prevents the formation of fluid-phase C3 convertase and promotes decay (“decay acceleration activity”) of C3 and C5 convertases (141). For comprehensive reviews of FH and FHL-1, see Ref. (132, 141, 142).
FHBPs and CRASPs
Interactions with FH are the best-studied mechanism for Borrelia complement inactivation, and complement resistance is correlated with binding FH (143). Borrelia spp. bind FH and/or FHL-1 through various native proteins collectively termed FHBPs or CRASPs (125, 144, 145). CRASPs can be grouped by their ability to bind only FH or both FH and FHL-1 as well as the species specificity of binding (that is, whether a FHBP can bind FH from only one or several host species) (125, 145): CRASP-1 (CspA) and CRASP-2 (CspZ) bind both FH and FHL-1, while CRASP-3 (ErpP), CRASP-4 (ErpC), and CRASP-5 (ErpA) bind only FH. CRASPs bind soluble FH and maintain it in an active conformation thereby allowing FH to inhibit completion of the complement response (i.e., MAC formation).
Several relapsing fever spirochetes bind FH in vitro (125, 146–151). Two FHBPs, FhbA and BhCRASP-1, have been identified in B. hermsii strains YOR and HS1, respectively (152, 153). However, binding FH is not as important for relapsing fever spirochetes to establish infection as it is for Lyme disease Borrelia (154, 155). Further supporting the non-essential nature of binding FH, Woodman et al. (154) found that despite FhbA being surface exposed and strongly binding FH in vitro, only 16% of B. hermsii recovered from the blood of infected mice had detectable levels of bound FH.
C4b-Binding Protein
C4b-binding protein (C4BP) has regulatory roles in all three pathways, though is the major regulator of the classical and lectin pathways. C4BP facilitates inactivation of C4b (classical, lectin) and fluid-phase C3b (alternative) by binding C4b, displacing C2a, and facilitating FI-mediated inactivation of C3 and C5 convertases (156).
Some Lyme and relapsing fever Borrelia spp. bind human and various animal C4BP (143, 148, 149, 157, 158). A comprehensive analysis identified outer surface proteins (Osps) associated with C4BP including OspA, Vlps, variable membrane proteins (Vmps), and several unidentified Osps (159). However, other studies have observed no binding of C4BP by Borrelia spp (143, 150, 160). These contradictory data may be due to differences in experimental design including the use of different strains, growth medium, temperatures, growth phases, and the use of recombinant versus native human C4BP. A putative C4BP receptor, p43, has been identified in B. burgdorferi s.l. (157). The relapsing fever spirochetes B. recurrentis and B. duttonii produce CihC, a surface lipoprotein homologous in sequence and function to fibronectin-binding proteins of other relapsing fever spirochetes, which also binds C4BP (148).
FHBP, C4BP, and Borrelia Niche
Resistance to complement is positively correlated to the infectivity of some Borrelia strains (130). With a higher resistance to complement, the more likely a bacterium can survive, disseminate, and proliferate. Co-opting tick proteins will protect spirochetes during the initial stages of transmission and dissemination but sustained dissemination requires Borrelia to resist complement via its own native mechanisms.
This leads to the question of how complement sensitive strains can cause infection. An interesting hypothesis was developed regarding complement resistance and spirochete niche when a relationship was noted between binding of the complement inhibitors, C4BP and FH (157, 158, 161). Neurotropic strains (e.g., B. bavariensis, B. garinii, B. turicatae, B. duttonii, and to a lesser extent B. hermsii) do not have to be highly resistant to complement in immunoprivileged sites, such as the central nervous system. Finding neurotropic species strongly bind C4BP and very weakly bind FH and FHL-1, while species that are not neurotropic bind C4BP but preferentially bind FH and/or FHL-1 supports this hypothesis (157). Alitalo et al. (162) did find B. garinii strains isolated from neuroborreliosis patients not only express FHBPs not expressed by strains cultured in vitro for an extended time but the FHBPs also bind FH. This implies complement resistance, though this was not reported and one of the isolates (LU59) was later reported to be highly but not completely sensitive to complement (163). It is possible that strong binding of FH is an artifact seen in vitro, similar to that observed with relapsing fever spirochetes (see FHBPs and CRASPs). Thus, binding FH is not required for neurotropic strains. Perhaps C4BP is sufficient to prevent complement activation during migration of neurotropic species from the site of inoculation to immunoprivileged sites. On the other hand, binding FH may be important for neurotropic strains to resist complement during migration and the incomplete sensitivity observed by Sandholm et al. (158) may be due to in vitro culturing resulting in the population losing its ability to bind FH. It could also be that neither C4BP nor FHBPs play a role in complement-sensitive borreliae disseminating and a novel mechanism is utilized by complement-sensitive strains.
CD59-Like Protein
Little information is available regarding the CD59-like protein of B. burgdorferi. Pausa et al. (164) demonstrated an increase in serum sensitivity and MAC formation in a serum-resistant B. burgdorferi isolate treated with anti-CD59 antibodies compared to the control treated B. burgdorferi and the serum-sensitive B. garinii isolate. In eukaryotic cells, CD59 is a surface-exposed membrane protein that prevents C9 polymerization and thus the formation of the MAC (19, 20). Still, it is not clear Borrelia possesses a protein homologous to mammalian or rodent CD59. While human anti-CD59 antibodies bound a surface-exposed integral membrane protein (29 kDa), this protein has never been identified though several known borrelial proteins can and have been ruled out based on molecular weight (e.g., BGA66, BGA71, OspA, OspB, OspC) (124). Given the demonstrated complement resistance conferred by this unknown borrelial protein, more attention should be given to identifying and clarifying the role this protein plays in complement resistance.
Complement Inhibition by Ixodes and Ornithodoros Salivary Proteins
A large number of proteins with a vast array of functions have been identified in the saliva of feeding Ixodes spp. with more being identified and characterized (165–169). While the details and mechanisms for some of these proteins remain to be elucidated, the beneficial nature of Ixodes salivary proteins to spirochete transmission and survival has been established (170–177). Ixodes saliva contains adaptive and innate immunomodulatory and anticomplement proteins (165, 178–183). A recent study demonstrated changes in the salivary protein profile over the course of a feeding, which has implications for the efficacy of the host immune response at the feeding pit and for transmitting spirochetes (168). Currently, several members of the anticomplement family of proteins have been characterized from I. scapularis, I. ricinus, and I. persulcatus including Salp15, Salp20, Isac, Irac I, Irac II, and Ixac-B1, -2, -3, -4, -5.
Salp15 is able to inhibit both adaptive and innate immune responses (184, 185). Salp15 binds OspC, which both serum-resistant and serum-sensitive B. burgdorferi s.l. produce, to inhibit deposition of the MAC and block the recognition and binding of antibodies to OspC (172, 186–188). In addition, Salp15 expression increases when ticks are infected with B. burgdorferi (172). Interestingly, mice passively immunized with anti-Salp15 antibodies were protected from infection with B. burgdorferi (189).
Salp20 inhibits the alternative complement pathway through binding properdin, which prevents stabilization of C3 convertase and propagation of the alternative pathway (183, 190, 191). In addition, Salp20 enhances the activity of FH to inhibit the alternative pathway (183). Incubating a serum-sensitive B. garinii strain with Salp20 protected the strain from complement activation and lysis (190). The mechanism(s) by which Salp20 confer(s) protection to B. garinii is unknown.
The Isac-like family of proteins include Ixodes scapularis anticomplement (Isac), I. ricinus anticomplement (Irac I), Irac II, and Ixac-B1 through -5 (I. ricinus anticomplement). Proteins in this family are similar in function to Salp20 (180, 182, 192). Inhibition of the alternative complement pathway is achieved through targeting C3 convertase via interactions with properdin, as Salp20 does, and by preventing factor B from binding C3b or displacing factor B from C3 convertase.
Ornithodoros salivary gland extracts also possess proteins that inhibit the host immune response (193). To date, however, one complement inhibitor has been identified and characterized from one Ornithodoros spp. O. moubata, found in Africa, is the vector of the relapsing fever spirochete B. duttonii (194). O. moubata complement inhibitor (OmCI) is a lipocalin that binds to and prevents cleavage of C5 (195, 196). OmCI was found to be effective at inhibiting C5 cleavage in different mammalian and rodent hosts (196). It is unknown if OmCI protects B. duttonii or if homologous proteins are found in other Ornithodoros spp.
Evasion by Borrelia of the Mammalian Humoral Immune Response by Surface Protein Variation
Evasion of complement is undoubtedly a vital mechanism to ensure spirochetes survive and establish infection. However, Borrelia will elicit an humoral immune response, and there are clear roles for this immune response in controlling and preventing Borrelia infection (113–118, 197, 198). These responses form the basis of an intense research effort for effective Lyme vaccines. Fortunately for Borrelia, they are quite adept at evading the host humoral response primarily through variation of surface-exposed proteins. Lyme disease Borrelia possess Osps and variable membrane protein-like [Vmp-like sequences (Vls)] proteins, while relapsing fever Borrelia possess Vmps (includes variable large and variable small proteins) (199–203). Some species hide antigens by inducing erythrocyte rosetting (204).
Osps and VlsE of Lyme Borrelia
The Osps, particularly OspC, are one of the most studied group of Borrelia proteins. For comprehensive reviews of Borrelia Osps, see Ref. (145, 205, 206). OspE and OspF are discussed above with FHBPs. Less is known about OspA, a protein predominantly involved in uptake and survival in ticks. OspA is immunogenic and able to block antibody binding to another surface-exposed protein, P66 (207, 208).
OspC has diverse roles, many of which are essential for transmission from Ixodes and establishing infection in mammals (209–216). These studies were key in demonstrating that ospC is upregulated during the early stages of infection, downregulated after infection has been established, and deleting or overexpressing ospC results in spirochetes that are quickly cleared from a host.
A handful of immune evasion functions have been identified for OspC. As discussed above, OspC protects Borrelia by binding Salp15. OspC also prevents phagocytosis by macrophages (216). In addition, several OspC types have been identified and correlated with a strains ability to establish infection in hosts and reservoirs (217–222). However, as each Osp is present as a single-copy locus, genetic variation is seen at the population level. That is, outside of random mutation or horizontal gene transfer events, a single spirochete cannot produce different OspC types in situ.
In contrast, the Vls system can change the expressed surface antigen in situ (Figure 2). Antigenic recombination of VlsE is important in maintaining infection in mammals and helps Lyme Borrelia evade the humoral immune response (223–236). The Vls system is composed of approximately 16 vls cassettes (the exact number varies by strain) and one expression locus, vlsE. All of the identified vls cassettes are located on the same plasmid (lp28-1) in close proximity to but in the opposite direction of vlsE. Expression at vlsE occurs through the random recombination of segments of multiple vls cassettes rather than recombination of an entire, single vls cassette. Thus, recombination events result in thousands of unique VlsE variants, all approximately 36 kDa.
Figure 2
Vmps of Relapsing Fever Borrelia
Variable membrane proteins, a system similar to Vls, are one of the best characterized immune evasion mechanisms (199, 237–240). B. hermsii has approximately 60 unique and promoterless vmp cassettes (i.e., silent cassettes) scattered throughout its genome and one promoter-driven vmp expression locus (Figure 2). A single vmp cassette is expressed when the entire cassette is moved to the expression locus.
The majority of spirochetes are cleared from the host through specific anti-Vmp IgM antibodies raised against the predominantly expressed Vmps, which results in a significant decrease in spirochete load (from approximately 105–107to <104 spirochetes/mL). The remaining spirochetes consist of a small population expressing different cassettes. Since the host has not raised a strong antibody response to these non-dominantly expressed Vmps, this minority population of spirochetes can proliferate to high concentrations until an antibody response is mounted and the majority of spirochetes are once again cleared. This cycle of vmp conversion, peaking spirochete loads, and antibody-mediated clearing repeats a minimum of two times resulting in the characteristic symptoms of a relapsing fever illness.
Mechanisms of Immune Evasion by B. miyamotoi: Where We are
Given the genetic similarity of B. miyamotoi to relapsing fever spirochetes, it is likely B. miyamotoi utilizes some homologous mechanisms to evade host immune responses. While B. miyamotoi is resistant to complement in vitro (241, 242), complement inactivation is not required for relapsing fever spirochetes to establish infection. OspE homologs have been identified in B. miyamotoi FR64b (isolated from the blood of A. argenteus); however, McDowell et al. were unable to demonstrate FH-binding (125). This suggests, as is the case for relapsing fever spirochetes, inactivation of complement may not be required to resolve spirochetemia during infection with B. miyamotoi (115, 243).
Instead, it appears B. miyamotoi utilizes a Vmp system (244), and Wagemakers et al. (100) recently demonstrated antigenic variation of Vmps in B. miyamotoi. C3H/HeN mice infected with B. miyamotoi LB-2001 produced anti-Vsp1 IgM and IgG antibodies that were effective in clearing the initial spirochetemic peak of B. miyamotoi from SCID mice. Despite this clearing, a second spirochetemic relapse occurred. Analyses of the secondary B. miyamotoi population revealed expression of vlpC2, not vsp1, as would be expected in the case of antigenic variation. They also noted vlpC2 was present in the initial B. miyamotoi population in a much lower prevalence compared to vsp1.
Mechanisms of Immune Evasion by B. miyamotoi: Where We Need to be
Even though B. miyamotoi is genetically similar to relapsing fever spirochetes, it has evolved and exists in different vectors (Ixodes not Ornithodoros) with different enzootic cycles and different co-pathogens compared to relapsing fever spirochetes. We should not assume B. miyamotoi utilizes the same set of mechanisms as other relapsing fever spirochetes. B. miyamotoi may use a combination of relapsing fever and Lyme Borrelia mechanisms as well as completely novel mechanisms.
The role of IgM in clearing B. miyamotoi has not been demonstrated. As discussed above, IgM is key in clearing relapsing fever infections. During B. hermsii infections, IgM targets FhbA and other surface proteins (113). IgM likely is important in clearing B. miyamotoi. All immunocompromised patients diagnosed with a B. miyamotoi infection developed meningoencephalitis. A shared factor with these patients has been treatment with rituximab, a monoclonal anti-CD20 antibody targeting IgM-producing CD20-positive B cells. Depletion of B cells may explain how B. miyamotoi is able to migrate to the CNS and causes meningoencephalitis in patients treated with rituximab. The presence of unknown complement inhibitors, however, could contribute to the complement resistance of B. miyamotoi and may be useful in establishing infection (241, 242).
The effects of tick saliva on B. miyamotoi survival have not yet been studied. However, being vectored by Ixodes, B. miyamotoi likely takes advantage of the protective proteins in tick saliva. In addition, understanding interactions between host, vector, and pathogen will aid in the development of Lyme and relapsing fever prevention strategies and thus requires more attention.
Concluding Remarks
Infection with B. miyamotoi in immunocompetent patients generally results in non-specific symptoms (e.g., headache, malaise), recurrent fever, and spirochetemia characteristic of relapsing fever. However, additional symptoms characteristic of relapsing fever have not been demonstrated, namely rapid symptom onset with a crisis event suggesting B. miyamotoi infection is not synonymous with relapsing fever and is rather a relapsing fever-like illness (90). This should not be surprising given the different lifestyle of B. miyamotoi compared to the vast majority of relapsing fever spirochetes.
The ability to evade the immune response is important for any successful pathogen but many of the mechanisms B. miyamotoi utilizes remain undiscovered. Hindered by the lack of a robust animal model, the relatively long-standing inability to culture in vitro, and being unaware of its pathogenicity, our understanding of B. miyamotoi is still in its infancy. However, we are making large strides forward with recent advances in culture techniques, animals models, physicians actively considering B. miyamotoi infection, as well as a growing wealth of epidemiological data that will allow us to clarify the details of infection, genetics, and physiology of this emerging pathogen.
Statements
Author contributions
All authors listed have made substantial, direct, and intellectual contribution to the work and approved it for publication.
Funding
This work was supported by NIH/NIAID grant 1R21AI26883-01 to CAB.
Conflict of interest
The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
References
1
SparaganoOGeorgeDGiangasperoAŠpitalskáE. Arthropods and associated arthropod-borne diseases transmitted by migrating birds. The case of ticks and tick-borne pathogens. Vet Parasitol (2015) 213:61–6.10.1016/j.vetpar.2015.08.028
2
Diuk-WasserMAVannierEKrausePJ. Coinfection by Ixodes tick-borne pathogens: ecological, epidemiological, and clinical consequences. Trends Parasitol (2016) 32:30–42.10.1016/j.pt.2015.09.008
3
NelderMPRussellCBSheehanNJSanderBMooreSLiYet alHuman pathogens associated with the blacklegged tick Ixodes scapularis: a systematic review. Parasit Vectors (2016) 9:265.10.1186/s13071-016-1529-y
4
RichterDSchleeDBAllgöwerRMatuschkaF-R. Relationships of a novel Lyme disease spirochete, Borrelia spielmani sp. nov., with its hosts in central Europe. Appl Environ Microbiol (2004) 70:6414–9.10.1128/AEM.70.11.6414-6419.2004
5
MargosGVollmerSACornetMGarnierMFingerleVWilskeBet alA new Borrelia species defined by multilocus sequence analysis of housekeeping genes. Appl Environ Microbiol (2009) 75:5410–6.10.1128/AEM.00116-09
6
MargosGVollmerSAOgdenNHFishD. Population genetics, taxonomy, phylogeny and evolution of Borrelia burgdorferi sensu lato. Infect Genet Evol (2011) 11:1545–63.10.1016/j.meegid.2011.07.022
7
StanekGReiterM. The expanding Lyme Borrelia complex – clinical significance of genomic species?Clin Microbiol Infect (2011) 17:487–93.10.1111/j.1469-0691.2011.03492.x
8
RudenkoNGolovchenkoMGrubhofferLOliverJHJr. Updates on Borrelia burgdorferi sensu lato complex with respect to public health. Ticks Tick Borne Dis (2011) 2:123–8.10.1016/j.ttbdis.2011.04.002
9
IvanovaLBTomovaAGonzález-AcuñaDMurúaRMorenoCXHernándezCet alBorrelia chilensis, a new member of the Borrelia burgdorferi sensu lato complex that extends the range of this genospecies in the Southern Hemisphere. Environ Microbiol (2014) 16:1069–80.10.1111/1462-2920.12310
10
MargosGPiesmanJLaneRSOgdenNHSingAStraubingerRKet alBorrelia kurtenbachii sp. nov., a widely distributed member of the Borrelia burgdorferi sensu lato species complex in North America. Int J Syst Evol Microbiol (2014) 64:128–30.10.1099/ijs.0.054593-0
11
TheilerA. Spirillosis of cattle. J Comp Pathol Ther (1904) 17:47–55.10.1016/S0368-1742(04)80003-1
12
BarbourAGMaupinGOTeltowGJCarterCJPiesmanJ. Identification of an uncultivable Borrelia species in the hard tick Amblyomma americanum: possible agent of a Lyme disease-like illness. J Infect Dis (1996) 173:403–9.10.1093/infdis/173.2.403
13
TakanoAGokaKUneYShimadaYFujitaHShiinoTet alIsolation and characterization of a novel Borrelia group of tick-borne borreliae from imported reptiles and their associated ticks. Environ Microbiol (2010) 12:134–46.10.1111/j.1462-2920.2009.02054.x
14
SteereACCoburnJGlicksteinL. The emergence of Lyme disease. J Clin Invest (2004) 113:1093–101.10.1172/JCI21681
15
StanekGWormserGPGrayJStrleF. Lyme borreliosis. Lancet (2012) 379:461–73.10.1016/S0140-6736(11)60103-7
16
FukunagaMTakahashiYTsurutaYMatsushitaORalphDMcClellandMet alGenetic and phenotypic analysis of Borrelia miyamotoi sp. nov., isolated from the ixodid tick Ixodes persulcatus, the vector for Lyme disease in Japan. Int J Syst Bacteriol (1995) 45:804–10.10.1099/00207713-45-4-804
17
ScolesGAPaperoMBeatiLFishD. A relapsing fever group spirochete transmitted by Ixodes scapularis ticks. Vector Borne Zoonotic Dis (2001) 1:21–34.10.1089/153036601750137624
18
FraenkelC-JGarpmoUBerglundJ. Determination of novel Borrelia genospecies in Swedish Ixodes ricinus ticks. J Clin Microbiol (2002) 40:3308–12.10.1128/JCM.40.9.3308-3312.2002
19
RichterDSchleeDBMatuschkaF-R. Relapsing fever-like spirochetes infecting European vector tick of Lyme disease agent. Emerg Infect Dis (2003) 9:697–701.10.3201/eid0906.020459
20
UllmannAJGabitzschESSchulzeTLZeidnerNSPiesmanJ. Three multiplex assays for detection of Borrelia burgdorferi sensu lato and Borrelia miyamotoi sensu lato in field-collected Ixodes nymphs in North America. J Med Entomol (2005) 42:1057–62.10.1093/jmedent/42.6.1057
21
MunJEisenRJEisenLLaneRS. Detection of a Borrelia miyamotoi sensu lato relapsing-fever group spirochete from Ixodes pacificus in California. J Med Entomol (2006) 43:120–3.10.1093/jmedent/43.1.120
22
RichterDMatuschkaF-R. Modulatory effect of cattle on risk for Lyme disease. Emerg Infect Dis (2006) 12:1919.10.3201/eid1212.051552
23
HulínskáDVotỳpkaJKřížBHolínkováNNovákováJHulínskỳV. Phenotypic and genotypic analysis of Borrelia spp. isolated from Ixodes ricinus ticks by using electrophoretic chips and real-time polymerase chain reaction. Folia Microbiol (Praha) (2007) 52:315–24.10.1007/BF02932085
24
BarbourAGBunikisJTravinskyBHoenAGDiuk-WasserMAFishDet alNiche partitioning of Borrelia burgdorferi and Borrelia miyamotoi in the same tick vector and mammalian reservoir species. Am J Trop Med Hyg (2009) 81:1120–31.10.4269/ajtmh.2009.09-0208
25
HoenAGRollendLGPaperoMACarrollJFDanielsTJMatherTNet alEffects of tick control by acaricide self-treatment of white-tailed deer on host-seeking tick infection prevalence and entomologic risk for Ixodes scapularis-borne pathogens. Vector Borne Zoonotic Dis (2009) 9:431–8.10.1089/vbz.2008.0155
26
WodeckaBLeonskaASkotarczakB. A comparative analysis of molecular markers for the detection and identification of Borrelia spirochaetes in Ixodes ricinus. J Med Microbiol (2010) 59:309–14.10.1099/jmm.0.013508-0
27
TokarzRJainKBennettABrieseTLipkinWI. Assessment of polymicrobial infections in ticks in New York State. Vector Borne Zoonotic Dis (2010) 10:217–21.10.1089/vbz.2009.0036
28
HamerSATsaoJIWalkerEDHicklingGJ. Invasion of the Lyme disease vector Ixodes scapularis: implications for Borrelia burgdorferi endemicity. Ecohealth (2010) 7:47–63.10.1007/s10393-010-0287-0
29
ScottMCRosenMEHamerSABakerEEdwardsHCrowderCet alHigh-prevalence Borrelia miyamotoi infection among wild turkeys (Meleagris gallopavo) in Tennessee. J Med Entomol (2010) 47:1238–42.10.1603/ME10075
30
WilhelmssonPFrylandLBorjessonSNordgrenJBergstromSErnerudhJet alPrevalence and diversity of Borrelia species in ticks that have bitten humans in Sweden. J Clin Microbiol (2010) 48:4169–76.10.1128/JCM.01061-10
31
RichterDMatuschkaF-R. Elimination of Lyme disease spirochetes from ticks feeding on domestic ruminants. Appl Environ Microbiol (2010) 76:7650–2.10.1128/AEM.01649-10
32
OgdenNHMargosGAanensenDMDrebotMAFeilEJHanincovaKet alInvestigation of genotypes of Borrelia burgdorferi in Ixodes scapularis ticks collected during surveillance in Canada. Appl Environ Microbiol (2011) 77:3244–54.10.1128/AEM.02636-10
33
PadgettKABonillaDL. Novel exposure sites for nymphal Ixodes pacificus within picnic areas. Ticks Tick Borne Dis (2011) 2:191–5.10.1016/j.ttbdis.2011.07.002
34
RichterDDebskiAHubalekZMatuschkaF-R. Absence of Lyme disease spirochetes in larval Ixodes ricinus ticks. Vector Borne Zoonotic Dis (2012) 12:21–7.10.1089/vbz.2011.0668
35
HamerSAHicklingGJKeithRSidgeJLWalkerEDTsaoJI. Associations of passerine birds, rabbits, and ticks with Borrelia miyamotoi and Borrelia andersonii in Michigan, U.S.A. Parasit Vectors (2012) 5:231.10.1186/1756-3305-5-231
36
RosenMEHamerSAGerhardtRRJonesCJMullerLIScottMCet alBorrelia burgdorferi not detected in widespread Ixodes scapularis (Acari: Ixodidae) collected from white-tailed deer in Tennessee. J Med Entomol (2012) 49:1473–80.10.1603/ME11255
37
GellerJNazarovaLKatarginaOJärvekülgLFomenkoNGolovljovaI. Detection and genetic characterization of relapsing fever spirochete Borrelia miyamotoi in Estonian ticks. PLoS One (2012) 7:e51914.10.1371/journal.pone.0051914
38
SubramanianGSekeyovaZRaoultDMediannikovO. Multiple tick-associated bacteria in Ixodes ricinus from Slovakia. Ticks Tick Borne Dis (2012) 3:406–10.10.1016/j.ttbdis.2012.10.001
39
RollendLFishDChildsJE. Transovarial transmission of Borrelia spirochetes by Ixodes scapularis: a summary of the literature and recent observations. Ticks Tick Borne Dis (2013) 4:46–51.10.1016/j.ttbdis.2012.06.008
40
TaylorKRTakanoAKonnaiSShimozuruMKawabataHTsubotaT. Borrelia miyamotoi infections among wild rodents show age and month independence and correlation with Ixodes persulcatus larval attachment in Hokkaido, Japan. Vector Borne Zoonotic Dis (2013) 13:92–7.10.1089/vbz.2012.1027
41
WodeckaBRymaszewskaASkotarczakB. Host and pathogen DNA identification in blood meals of nymphal Ixodes ricinus ticks from forest parks and rural forests of Poland. Exp Appl Acarol (2013) 62:543–55.10.1007/s10493-013-9763-x
42
SalkeldDJCinkovichSNietoNC. Tick-borne pathogens in northwestern California, USA. Emerg Infect Dis (2014) 20:493–4.10.3201/eid2003.130668
43
MicheletLDelannoySDevillersEUmhangGAspanAJuremalmMet alHigh-throughput screening of tick-borne pathogens in Europe. Front Cell Infect Microbiol (2014) 4:103.10.3389/fcimb.2014.00103
44
MaysSEHendricksBMPaulsenDJHoustonAETrout FryxellRT. Prevalence of five tick-borne bacterial genera in adult Ixodes scapularis removed from white-tailed deer in western Tennessee. Parasit Vectors (2014) 7:473.10.1186/s13071-014-0473-y
45
PadgettKBonillaDKjemtrupAVilcinsI-MYoshimizuMHHuiLet alLarge scale spatial risk and comparative prevalence of Borrelia miyamotoi and Borrelia burgdorferi sensu lato in Ixodes pacificus. PLoS One (2014) 9:e110853.10.1371/journal.pone.0110853
46
CossonJ-FMicheletLChotteJNaourELCoteMDevillersEet alGenetic characterization of the human relapsing fever spirochete Borrelia miyamotoi in vectors and animal reservoirs of Lyme disease spirochetes in France. Parasit Vectors (2014) 7:233.10.1186/1756-3305-7-233
47
FonvilleMFriesemaIHMHengeveldPDDocters van LeeuwenAJahfariSHarmsMGet alHuman exposure to tickborne relapsing fever spirochete Borrelia miyamotoi, the Netherlands. Emerg Infect Dis (2014) 20:1244–5.10.3201/eid2007.131525
48
DibernardoACoteTOgdenNHLindsayLR. The prevalence of Borrelia miyamotoi infection, and co-infections with other Borrelia spp. in Ixodes scapularis ticks collected in Canada. Parasit Vectors (2014) 7:183.10.1186/1756-3305-7-183
49
EshooMWCrowderCDCarolanHERoundsMAEckerDJHaagHet alBroad-range survey of tick-borne pathogens in Southern Germany reveals a high prevalence of Babesia microti and a diversity of other tick-borne pathogens. Vector Borne Zoonotic Dis (2014) 14:584–91.10.1089/vbz.2013.1498
50
BurriCSchumannOSchumannCGernL. Are Apodemus spp. mice and Myodes glareolus reservoirs for Borrelia miyamotoi, Candidatus Neoehrlichia mikurensis, Rickettsia helvetica, R. monacensis and Anaplasma phagocytophilum?Ticks Tick Borne Dis (2014) 5:245–51.10.1016/j.ttbdis.2013.11.007
51
MukhachevaTAKovalevSY. Borrelia spirochetes in Russia: genospecies differentiation by real-time PCR. Ticks Tick Borne Dis (2014) 5:722–6.10.1016/j.ttbdis.2014.05.016
52
TakanoAToyomaneKKonnaiSOhashiKNakaoMItoTet alTick surveillance for relapsing fever spirochete Borrelia miyamotoi in Hokkaido, Japan. PLoS ONE (2014) 9:e104532.10.1371/journal.pone.0104532
53
CrowderCDCarolanHERoundsMAHonigVMothesBHaagHet alPrevalence of Borrelia miyamotoi in Ixodes ticks in Europe and the United States. Emerg Infect Dis (2014) 20:1678–82.10.3201/eid2010.131583
54
HamerSAHicklingGJWalkerEDTsaoJI. Increased diversity of zoonotic pathogens and Borrelia burgdorferi strains in established versus incipient Ixodes scapularis populations across the Midwestern United States. Infect Genet Evol (2014) 27:531–42.10.1016/j.meegid.2014.06.003
55
KiewraDStańczakJRichterM. Ixodes ricinus ticks (Acari, Ixodidae) as a vector of Borrelia burgdorferi sensu lato and Borrelia miyamotoi in Lower Silesia, Poland – preliminary study. Ticks Tick Borne Dis (2014) 5:892–7.10.1016/j.ttbdis.2014.07.004
56
FedorovaNKleinjanJEJamesDHuiLTPeetersHLaneRS. Remarkable diversity of tick or mammalian-associated Borreliae in the metropolitan San Francisco Bay Area, California. Ticks Tick Borne Dis (2014) 5:951–61.10.1016/j.ttbdis.2014.07.015
57
LommanoEDvořákCVallottonLJenniLGernL. Tick-borne pathogens in ticks collected from breeding and migratory birds in Switzerland. Ticks Tick Borne Dis (2014) 5:871–82.10.1016/j.ttbdis.2014.07.001
58
SchreiberCKrückenJBeckSMaazDPachnickeSKriegerKet alPathogens in ticks collected from dogs in Berlin/Brandenburg, Germany. Parasit Vectors (2014) 7:535.10.1186/s13071-014-0535-1
59
MukhachevaTASalikhovaIIKovalevSY. Multilocus spacer analysis revealed highly homogeneous genetic background of Asian type of Borrelia miyamotoi. Infect Genet Evol (2015) 31:257–62.10.1016/j.meegid.2015.02.009
60
ReiterMSchöttaA-MMüllerAStockingerHStanekG. A newly established real-time PCR for detection of Borrelia miyamotoi in Ixodes ricinus ticks. Ticks Tick Borne Dis (2015) 6(3):303–8.10.1016/j.ttbdis.2015.02.002
61
HansfordKMFonvilleMJahfariSSprongHMedlockJM. Borrelia miyamotoi in host-seeking Ixodes ricinus ticks in England. Epidemiol Infect (2015) 143:1079–87.10.1017/S0950268814001691
62
CochezCHeymanPHeylenDFonvilleMHengeveldPTakkenWet alThe presence of Borrelia miyamotoi, a relapsing fever spirochaete, in questing Ixodes ricinus in Belgium and in the Netherlands. Zoonoses Public Health (2015) 62:331–3.10.1111/zph.12154
63
EshooMWCarolanHEMassireCChouDMCrowderCDRoundsMAet alSurvey of Ixodes pacificus ticks in California reveals a diversity of microorganisms and a novel and widespread Anaplasmataceae species. PLoS One (2015) 10:e0135828.10.1371/journal.pone.0135828
64
SalkeldDJNietoNCCarbajales-DalePCarbajales-DaleMCinkovichSSLambinEF. Disease risk & landscape attributes of tick-borne Borrelia pathogens in the San Francisco Bay Area, California. PLoS One (2015) 10:e0134812.10.1371/journal.pone.0134812
65
SzekeresSCoipanECRigóKMajorosGJahfariSSprongHet alEco-epidemiology of Borrelia miyamotoi and Lyme borreliosis spirochetes in a popular hunting and recreational forest area in Hungary. Parasit Vectors (2015) 8:309.10.1186/s13071-015-0922-2
66
QuarstenHSkarpaasTFajsLNoraasSKjellandV. Tick-borne bacteria in Ixodes ricinus collected in southern Norway evaluated by a commercial kit and established real-time PCR protocols. Ticks Tick Borne Dis (2015) 6:538–44.10.1016/j.ttbdis.2015.04.008
67
KjellandVRollumRKorslundLSlettanATveitnesD. Borrelia miyamotoi is widespread in Ixodes ricinus ticks in southern Norway. Ticks Tick Borne Dis (2015) 6:516–21.10.1016/j.ttbdis.2015.04.004
68
NunesMParreiraRLopesNMaiaCCarreiraTSousaCet alMolecular identification of Borrelia miyamotoi in Ixodes ricinus from Portugal. Vector Borne Zoonotic Dis (2015) 15:515–7.10.1089/vbz.2014.1765
69
CerarTKorvaMAvšič-ŽupancTRužić-SabljićE. Detection, identification and genotyping of Borrellia spp. in rodents in Slovenia by PCR and culture. BMC Vet Res (2015) 11:188.10.1186/s12917-015-0501-y
70
EdwardsMJBarbalatoLAMakkapatiAPhamKDBugbeeLM. Relatively low prevalence of Babesia microti and Anaplasma phagocytophilum in Ixodes scapularis ticks collected in the Lehigh Valley region of eastern Pennsylvania. Ticks Tick Borne Dis (2015) 6:812–9.10.1016/j.ttbdis.2015.07.009
71
SytykiewiczHKarbowiakGChorostowska-WynimkoJSzpechcińskiASupergan-MarwiczMHorbowiczMet alCoexistence of Borrelia burgdorferi s.l. genospecies within Ixodes ricinus ticks from central and eastern Poland. Acta Parasitol (2015) 60:654–61.10.1515/ap-2015-0093
72
WodeckaBSkotarczakB. Identification of host blood-meal sources and Borrelia in field-collected Ixodes ricinus ticks in north-western Poland. Ann Agric Environ Med (2016) 23:59–63.10.5604/12321966.1196853
73
SormunenJJKlemolaTVesterinenEJVuorinenIHytönenJHänninenJet alAssessing the abundance, seasonal questing activity, and Borrelia and tick-borne encephalitis virus (TBEV) prevalence of Ixodes ricinus ticks in a Lyme borreliosis endemic area in Southwest Finland. Ticks Tick Borne Dis (2016) 7:208–15.10.1016/j.ttbdis.2015.10.011
74
HanSHicklingGJTsaoJI. High prevalence of Borrelia miyamotoi among adult blacklegged ticks from white-tailed deer. Emerg Infect Dis (2016) 22:316–8.10.3201/eid2202.151218
75
TadinATokarzRMarkotićAMargaletićJTurkNHabušJet alMolecular survey of zoonotic agents in rodents and other small mammals in Croatia. Am J Trop Med Hyg (2016) 94:466–73.10.4269/ajtmh.15-0517
76
van DuijvendijkGCoipanCWagemakersAFonvilleMErsözJOeiAet alLarvae of Ixodes ricinus transmit Borrelia afzelii and B. miyamotoi to vertebrate hosts. Parasit Vectors (2016) 9:97.10.1186/s13071-016-1389-5
77
KhasnatinovMADanchinovaGATakanoAKawabataHOhashiNMasuzawaT. Prevalence of Borrelia miyamotoi in Ixodes persulcatus in Irkutsk city and its neighboring territories, Russia. Ticks Tick Borne Dis (2016) 7:394–7.10.1016/j.ttbdis.2015.12.016
78
HeylenDFonvilleMvan LeeuwenADSprongH. Co-infections and transmission dynamics in a tick-borne bacterium community exposed to songbirds. Environ Microbiol (2016) 18:988–96.10.1111/1462-2920.13164
79
KalmárZSprongHMihalcaADGhermanCMDumitracheMOCoipanECet alBorrelia miyamotoi and Candidatus Neoehrlichia mikurensis in Ixodes ricinus Ticks, Romania. Emerg Infect Dis (2016) 22:550–1.10.3201/eid2203.150140
80
SormunenJJPenttinenRKlemolaTHänninenJVuorinenILaaksonenMet alTick-borne bacterial pathogens in southwestern Finland. Parasit Vectors (2016) 9:168.10.1186/s13071-016-1449-x
81
PaulRELCoteMLe NaourEBonnetSI. Environmental factors influencing tick densities over seven years in a French suburban forest. Parasit Vectors (2016) 9:309.10.1186/s13071-016-1591-5
82
SkotarczakBWodeckaBRymaszewskaAAdamskaM. Molecular evidence for bacterial pathogens in Ixodes ricinus ticks infesting Shetland ponies. Exp Appl Acarol (2016) 69:179–89.10.1007/s10493-016-0027-4
83
WodeckaBMichalikJLaneRSNowak-ChmuraMWierzbickaA. Differential associations of Borrelia species with European badgers (Meles meles) and raccoon dogs (Nyctereutes procyonoides) in western Poland. Ticks Tick Borne Dis (2016) 7:1010–6.10.1016/j.ttbdis.2016.05.008
84
PotkonjakAKleinermanGGutiérrezRSavićSVračarVNachum-BialaYet alOccurrence of Borrelia burgdorferi sensu lato in Ixodes ricinus ticks with first identification of Borrelia miyamotoi in Vojvodina, Serbia. Vector Borne Zoonotic Dis (2016) 16(10):631–5.10.1089/vbz.2016.2008
85
PlatonovAEKaranLSKolyasnikovaNMMakhnevaNAToporkovaMGMaleevVVet alHumans Infected with relapsing fever spirochete Borrelia miyamotoi, Russia. Emerg Infect Dis (2011) 17:1816–23.10.3201/eid1710.101474
86
ChowdriHRGugliottaJLBerardiVPGoethertHKMolloyPJSterlingSLet alBorrelia miyamotoi infection presenting as human granulocytic anaplasmosis: a case report. Ann Intern Med (2013) 159:21–7.10.7326/0003-4819-159-1-201307020-00005
87
HoviusJWRde WeverBSohneMBrouwerMCCoumouJWagemakersAet alA case of meningoencephalitis by the relapsing fever spirochaete Borrelia miyamotoi in Europe. Lancet (2013) 382:658.10.1016/S0140-6736(13)61644-X
88
GugliottaJLGoethertHKBerardiVPTelfordSRIII. Meningoencephalitis from Borrelia miyamotoi in an immunocompromised patient. N Engl J Med (2013) 368:240–5.10.1056/NEJMoa1209039
89
SatoKTakanoAKonnaiSNakaoMItoTKoyamaKet alHuman infections with Borrelia miyamotoi, Japan. Emerg Infect Dis (2014) 20:1391–4.10.3201/eid2008.131761
90
TelfordSRIIIGoethertHKMolloyPJBerardiVPChowdriHRGugliottaJLet alBorrelia miyamotoi disease: neither Lyme disease nor relapsing fever. Clin Lab Med (2015) 35(4):867–82.10.1016/j.cll.2015.08.002
91
MolloyPJTelfordSRChowdriHRLeporeTJGugliottaJLWeeksKEet alBorrelia miyamotoi disease in the Northeastern United States: a case series. Ann Intern Med (2015) 163:91–8.10.7326/M15-0333
92
SudhindraPWangGSchrieferMEMcKennaDZhugeJKrausePJet alInsights into Borrelia miyamotoi infection from an untreated case demonstrating relapsing fever, monocytosis and a positive C6 Lyme serology. Diagn Microbiol Infect Dis (2016) 86:93–6.10.1016/j.diagmicrobio.2016.06.015
93
MagnarelliLAAndersonJFJohnsonRC. Cross-reactivity in serological tests for Lyme disease and other spirochetal infections. J Infect Dis (1987) 156:183–8.10.1093/infdis/156.1.183
94
LeeSVigliottiJVigliottiVJonesWShearerD. Detection of borreliae in archived sera from patients with clinically suspect Lyme disease. Int J Mol Sci (2014) 15:4284–98.10.3390/ijms15034284
95
MargolisNHoganDCieplakWSchwanTGRosaPA. Homology between Borrelia burgdorferi OspC and members of the family of Borrelia hermsii variable major proteins. Gene (1994) 143:105–10.10.1016/0378-1119(94)90613-0
96
CutlerSJMossJFukunagaMWrightDJFekadeDWarrellD. Borrelia recurrentis characterization and comparison with relapsing-fever, Lyme-associated, and other Borrelia spp. Int J Syst Bacteriol (1997) 47:958–68.10.1099/00207713-47-4-958
97
StevensonBPorcellaSFOieKLFitzpatrickCARaffelSJLubkeLet alThe relapsing fever spirochete Borrelia hermsii contains multiple, antigen-encoding circular plasmids that are homologous to the cp32 plasmids of Lyme disease spirochetes. Infect Immun (2000) 68:3900–8.10.1128/IAI.68.7.3900-3908.2000
98
DiLPaganPEPackerDMartinCLAktherSRamrattanGet alBorreliaBase: a phylogeny-centered browser of Borrelia genomes. BMC Bioinformatics (2014) 15:233.10.1186/1471-2105-15-233
99
KrausePJHendricksonJESteevesTKFishD. Blood transfusion transmission of the tick-borne relapsing fever spirochete Borrelia miyamotoi in mice. Transfusion (2015) 55:593–7.10.1111/trf.12879
100
WagemakersAKoetsveldJNarasimhanSWickelMDeponteKBleijlevensBet alVariable major proteins as targets for specific antibodies against Borrelia miyamotoi. J Immunol (2016) 196:4185–95.10.4049/jimmunol.1600014
101
BartholdSWBeckDSHansenGMTerwilligerGAMoodyKD. Lyme borreliosis in selected strains and ages of laboratory mice. J Infect Dis (1990) 162:133–8.10.1093/infdis/162.1.133
102
BartholdSWde SouzaMSJanotkaJLSmithALPersingDH. Chronic Lyme borreliosis in the laboratory mouse. Am J Pathol (1993) 143:959–71.
103
CadavidD. The mammalian host response to Borrelia infection. Wien Klin Wochenschr (2006) 118:653–8.10.1007/s00508-006-0692-0
104
KrausePJNarasimhanSWormserGPRollendLFikrigELeporeTet alHuman Borrelia miyamotoi infection in the United States. N Engl J Med (2013) 368:291–3.10.1056/NEJMc1215469
105
KrausePJNarasimhanSWormserGPBarbourAGPlatonovAEBrancatoJet alBorrelia miyamotoi sensu lato seroreactivity and seroprevalence in the Northeastern United States. Emerg Infect Dis (2014) 20:1183–90.10.3201/eid2007.131587
106
HuLTTsibrisAMBrandaJA. Case 24-2015: a 28-year-old pregnant woman with fever, chills, headache, and fatigue. N Engl J Med (2015) 373:468–75.10.1056/NEJMcpc1501763
107
SarksyanDSPlatonovAEKaranLSShipulinGASprongHHoviusJWR. Probability of spirochete Borrelia miyamotoi transmission from ticks to humans. Emerg Infect Dis (2015) 21:2273–4.10.3201/eid2112.151097
108
CerarTStrleFStupicaDRuzic-SabljicEMcHughGSteereACet alDifferences in genotype, clinical features, and inflammatory potential of Borrelia burgdorferi sensu stricto strains from Europe and the United States. Emerg Infect Dis (2016) 22:818–27.10.3201/eid2205.151806
109
BunikisJTsaoJGarpmoUBerglundJFishDBarbourAG. Typing of Borrelia relapsing fever group strains. Emerg Infect Dis (2004) 10:1661.10.3201/eid1009.040236
110
FihnSLarsonEB. Tick-borne relapsing fever in the Pacific Northwest: an underdiagnosed illness?West J Med (1980) 133:203–9.
111
BodenKLobensteinSHermannBMargosGFingerleV. Borrelia miyamotoi-associated neuroborreliosis in immunocompromised person. Emerg Infect Dis (2016) 22:1617–20.10.3201/eid2209.152034
112
MerleNSChurchSEFremeaux-BacchiVRoumeninaLT. Complement system part I – molecular mechanisms of activation and regulation. Front Immunol (2015) 6:262.10.3389/fimmu.2015.00262
113
ColomboMJAlugupalliKR. Complement factor H-binding protein, a putative virulence determinant of Borrelia hermsii, is an antigenic target for protective B1b lymphocytes. J Immunol (2008) 180:4858–64.10.4049/jimmunol.180.7.4858
114
BelperronAADaileyCMBockenstedtLK. Infection-induced marginal zone B cell production of Borrelia hermsii-specific antibody is impaired in the absence of CD1d. J Immunol (2005) 174:5681–6.10.4049/jimmunol.174.9.5681
115
ConnollySEBenachJL. Cutting edge: the spirochetemia of murine relapsing fever is cleared by complement-independent bactericidal antibodies. J Immunol (2001) 167:3029–32.10.4049/jimmunol.167.6.3029
116
AlugupalliKRLeongJMWoodlandRTMuramatsuMHonjoTGersteinRM. B1b lymphocytes confer T cell-independent long-lasting immunity. Immunity (2004) 21:379–90.10.1016/j.immuni.2004.06.019
117
AlugupalliKRGersteinRMChenJSzomolanyi-TsudaEWoodlandRTLeongJM. The resolution of relapsing fever borreliosis requires IgM and is concurrent with expansion of B1b lymphocytes. J Immunol (2003) 170:3819–27.10.4049/jimmunol.170.7.3819
118
BarbourAGBundocV. In vitro and in vivo neutralization of the relapsing fever agent Borrelia hermsii with serotype-specific immunoglobulin M antibodies. Infect Immun (2001) 69:1009–15.10.1128/IAI.69.2.1009-1015.2001
119
DickinsonGSPicconeHSunGLienEGattoLAlugupalliKR. Toll-like receptor 2 deficiency results in impaired antibody responses and septic shock during Borrelia hermsii infection. Infect Immun (2010) 78:4579–88.10.1128/IAI.00438-10
120
VuyyuruRLiuHManserTAlugupalliKR. Characteristics of Borrelia hermsii infection in human hematopoietic stem cell-engrafted mice mirror those of human relapsing fever. Proc Natl Acad Sci U S A (2011) 108:20707–12.10.1073/pnas.1108776109
121
DickinsonGSSunGBramRJAlugupalliKR. Efficient B cell responses to Borrelia hermsii infection depend on BAFF and BAFFR but not TACI. Infect Immun (2014) 82:453–9.10.1128/IAI.01147-13
122
NorisMRemuzziG. Overview of complement activation and regulation. Semin Nephrol (2013) 33:479–92.10.1016/j.semnephrol.2013.08.001
123
RicklinDReisESLambrisJD. Complement in disease: a defence system turning offensive. Nat Rev Nephrol (2016) 12:383–401.10.1038/nrneph.2016.70
124
KraiczyP. Hide and seek: how Lyme disease spirochetes overcome complement attack. Front Immunol (2016) 7:385.10.3389/fimmu.2016.00385
125
McDowellJVWolfgangJTranEMettsMSHamiltonDMarconiRT. Comprehensive analysis of the factor H binding capabilities of Borrelia species associated with Lyme disease: delineation of two distinct classes of factor H binding proteins. Infect Immun (2003) 71:3597–602.10.1128/IAI.71.6.3597-3602.2003
126
KraiczyPSkerkaCKirschfinkMZipfelPFBradeV. Immune evasion of Borrelia burgdorferi: insufficient killing of the pathogens by complement and antibody. Int J Med Microbiol (2002) 291(Suppl 33):141–6.10.1016/S1438-4221(02)80027-3
127
BradeVKleberIAckerG. Differences of two Borrelia burgdorferi strains in complement activation and serum resistance. Immunobiology (1992) 185:453–65.10.1016/S0171-2985(11)80087-2
128
Breitner-RuddockSWürznerRSchulzeJBradeV. Heterogeneity in the complement-dependent bacteriolysis within the species of Borrelia burgdorferi. Med Microbiol Immunol (1997) 185:253–60.10.1007/s004300050038
129
KraiczyPHunfeldK-PBreitner-RuddockSWürznerRAckerGBradeV. Comparison of two laboratory methods for the determination of serum resistance in Borrelia burgdorferi isolates. Immunobiology (2000) 201:406–19.10.1016/S0171-2985(00)80094-7
130
Van DamAPOeiAJasparsRFijenCWilskeBSpanjaardLet alComplement-mediated serum sensitivity among spirochetes that cause Lyme disease. Infect Immun (1997) 65:1228–36.
131
KurtenbachKDe MichelisSEttiSSchäferSMSewellH-SBradeVet alHost association of Borrelia burgdorferi sensu lato – the key role of host complement. Trends Microbiol (2002) 10:74–9.10.1016/S0966-842X(01)02298-3
132
FrieseMAHellwageJJokirantaTSMeriSPeterHHEibelHet alFHL-1/reconectin and factor H: two human complement regulators which are encoded by the same gene are differently expressed and regulated. Mol Immunol (1999) 36:809–18.10.1016/S0161-5890(99)00101-7
133
GordonDLKaufmanRMBlackmoreTKKwongJLublinDM. Identification of complement regulatory domains in human factor H. J Immunol (1995) 155:348–56.
134
KühnSSkerkaCZipfelPF. Mapping of the complement regulatory domains in the human factor H-like protein 1 and in factor H. J Immunol (1995) 155:5663–70.
135
OppermannMManuelianTJózsiMBrandtEJokirantaTSHeinenSet alThe C-terminus of complement regulator factor H mediates target recognition: evidence for a compact conformation of the native protein. Clin Exp Immunol (2006) 144:342–52.10.1111/j.1365-2249.2006.03071.x
136
PangburnMKAtkinsonMAMeriS. Localization of the heparin-binding site on complement factor H. J Biol Chem (1991) 266:16847–53.
137
BlackmoreTKHellwageJSadlonTAHiggsNZipfelPFWardHMet alIdentification of the second heparin-binding domain in human complement factor H. J Immunol (1998) 160:3342–8.
138
BlackmoreTKSadlonTAWardHMLublinDMGordonDL. Identification of a heparin binding domain in the seventh short consensus repeat of complement factor H. J Immunol (1996) 157:5422–7.
139
MeriSPangburnMK. Discrimination between activators and nonactivators of the alternative pathway of complement: regulation via a sialic acid/polyanion binding site on factor H. Proc Natl Acad Sci U S A (1990) 87:3982–6.10.1073/pnas.87.10.3982
140
MeriSPangburnMK. Regulation of alternative pathway complement activation by glycosaminoglycans: specificity of the polyanion binding site on factor H. Biochem Biophys Res Commun (1994) 198:52–9.10.1006/bbrc.1994.1008
141
KouserLAbdul-AzizMNayakAStoverCMMSimRBPKishoreUP. Properdin and factor H: opposing players on the alternative complement pathway “see-saw”. Front Immunol (2013) 4:93.10.3389/fimmu.2013.00093
142
FerreiraVPPangburnMKCortésC. Complement control protein factor H: the good, the bad, and the inadequate. Mol Immunol (2010) 47:2187–97.10.1016/j.molimm.2010.05.007
143
AlitaloAMeriTRämöLJokirantaTSHeikkiläTSeppäläIJTet alComplement evasion by Borrelia burgdorferi: serum-resistant strains promote C3b inactivation. Infect Immun (2001) 69:3685–91.10.1128/IAI.69.6.3685-3691.2001
144
KraiczyPStevensonB. Complement regulator-acquiring surface proteins of Borrelia burgdorferi: structure, function and regulation of gene expression. Ticks Tick Borne Dis (2013) 4:26–34.10.1016/j.ttbdis.2012.10.039
145
PulzovaLBhideM. Outer surface proteins of Borrelia: peerless immune evasion tools. Curr Protein Pept Sci (2014) 15:75–88.10.2174/1389203715666140221124213
146
MeriTCutlerSJBlomAMMeriSJokirantaTS. Relapsing fever spirochetes Borrelia recurrentis and B. duttonii acquire complement regulators C4b-binding protein and factor H. Infect Immun (2006) 74:4157–63.10.1128/IAI.00007-06
147
BhideMREscuderoRCamafeitaEGilHJadoIAndaP. Complement factor H binding by different Lyme disease and relapsing fever Borrelia in animals and human. BMC Res Notes (2009) 2:134.10.1186/1756-0500-2-134
148
GrosskinskySSchottMBrennerCCutlerSJSimonMMWallichR. Human complement regulators C4b-binding protein and C1 esterase inhibitor interact with a novel outer surface protein of Borrelia recurrentis. PLoS Negl Trop Dis (2010) 4:e698.10.1371/journal.pntd.0000698
149
BrennerCBomansKHabichtJSimonMMWallichR. Mapping the ligand-binding region of Borrelia hermsii fibronectin-binding protein. PLoS One (2013) 8:e63437.10.1371/journal.pone.0063437
150
SchwabJHammerschmidtCRichterDSkerkaCMatuschkaF-RWallichRet alBorrelia valaisiana resist complement-mediated killing independently of the recruitment of immune regulators and inactivation of complement components. PLoS One (2013) 8:e53659.10.1371/journal.pone.0053659
151
LewisERGMarcsisinRAMillerSACHueFPhillipsAAuCoinDPet alFibronectin-binding protein of Borrelia hermsii expressed in the blood of mice with relapsing fever. Infect Immun (2014) 82:2520–31.10.1128/IAI.01582-14
152
HovisKMMcDowellJVGriffinLMarconiRT. Identification and characterization of a linear-plasmid-encoded factor H-binding protein (FhbA) of the relapsing fever spirochete Borrelia hermsii. J Bacteriol (2004) 186:2612–8.10.1128/JB.186.9.2612-2618.2004
153
RossmannEKraiczyPHerzbergerPSkerkaCKirschfinkMSimonMMet alDual binding specificity of a Borrelia hermsii-associated complement regulator-acquiring surface protein for factor H and plasminogen discloses a putative virulence factor of relapsing fever spirochetes. J Immunol (2007) 178:7292–301.10.4049/jimmunol.178.11.7292
154
WoodmanMECooleyAEAvdiushkoRBowmanABottoMWootenRMet alRoles for phagocytic cells and complement in controlling relapsing fever infection. J Leukoc Biol (2009) 86:727–36.10.1189/jlb.0309169
155
FineLMMillerDPMalloryKLTegelsBKEarnhartCGMarconiRT. The Borrelia hermsii factor H binding protein FhbA is not required for infectivity in mice or for resistance to human complement in vitro. Infect Immun (2014) 82:3324–32.10.1128/IAI.01892-14
156
ErmertDBlomAM. C4b-binding protein: the good, the bad and the deadly. Novel functions of an old friend. Immunol Lett (2016) 169:82–92.10.1016/j.imlet.2015.11.014
157
PietikäinenJMeriTBlomAMMeriS. Binding of the complement inhibitor C4b-binding protein to Lyme disease borreliae. Mol Immunol (2010) 47:1299–305.10.1016/j.molimm.2009.11.028
158
SandholmKHenningssonAJSäveSBergströmSForsbergPJonssonNet alEarly cytokine release in response to live Borrelia burgdorferi sensu lato spirochetes is largely complement independent. PLoS One (2014) 9:e108013.10.1371/journal.pone.0108013
159
MadarMBencurovaEMlynarcikPAlmeidaAMSoaresRBhideKet alExploitation of complement regulatory proteins by Borrelia and Francisella. Mol Biosyst (2015) 11:1684–95.10.1039/C5MB00027K
160
HammerschmidtCKlevenhausYKoenigsAHallströmTFingerleVSkerkaCet alBGA66 and BGA71 facilitate complement resistance of Borrelia bavariensis by inhibiting assembly of the membrane attack complex. Mol Microbiol (2016) 99:407–24.10.1111/mmi.13239
161
van DamAPKuiperHVosKWidjojokusumoAde JonghBMSpanjaardLet alDifferent genospecies of Borrelia burgdorferi are associated with distinct clinical manifestations of Lyme borreliosis. Clin Infect Dis (1993) 17:708–17.10.1093/clinids/17.4.708
162
AlitaloAMeriTComstedtPJefferyLTornbergJStrandinTet alExpression of complement factor H binding immunoevasion proteins in Borrelia garinii isolated from patients with neuroborreliosis. Eur J Immunol (2005) 35:3043–53.10.1002/eji.200526354
163
HodzicEFengSBartholdSW. Assessment of transcriptional activity of Borrelia burgdorferi and host cytokine genes during early and late infection in a mouse model. Vector Borne Zoonotic Dis (2013) 13:694–711.10.1089/vbz.2012.1189
164
PausaMPellisVCincoMGiulianiniPGPresaniGPerticarariSet alSerum-resistant strains of Borrelia burgdorferi evade complement-mediated killing by expressing a CD59-like complement inhibitory molecule. J Immunol (2003) 170:3214–22.10.4049/jimmunol.170.6.3214
165
RibeiroJMWeisJJTelfordSR. Saliva of the tick Ixodes dammini inhibits neutrophil function. Exp Parasitol (1990) 70:382–8.10.1016/0014-4894(90)90121-R
166
RibeiroJMCAlarcon-ChaidezFBFrancischettiIMMansBJMatherTNValenzuelaJGet alAn annotated catalog of salivary gland transcripts from Ixodes scapularis ticks. Insect Biochem Mol Biol (2006) 36:111–29.10.1016/j.ibmb.2005.11.005
167
LewisLARadulovićŽMKimTKPorterLMMulengaA. Identification of 24 h Ixodes scapularis immunogenic tick saliva proteins. Ticks Tick Borne Dis (2015) 6:424–34.10.1016/j.ttbdis.2015.03.012
168
KimTKTirloniLPintoAFMMorescoJYatesJRIIIda Silva VazIJret alIxodes scapularis tick saliva proteins sequentially secreted every 24 h during blood feeding. PLoS Negl Trop Dis (2016) 10:e0004323.10.1371/journal.pntd.0004323
169
NuttallPALabudaM. Tick–host interactions: saliva-activated transmission. Parasitology (2004) 129:S177–89.10.1017/S0031182004005633
170
NarasimhanSDePonteKMarcantonioNLiangXRoyceTENelsonKFet alImmunity against Ixodes scapularis salivary proteins expressed within 24 hours of attachment thwarts tick feeding and impairs Borrelia transmission. PLoS One (2007) 2:e451.10.1371/journal.pone.0000451
171
ZeidnerNSSchneiderBSNuncioMSGernLPiesmanJ. Coinoculation of Borrelia spp. with tick salivary gland lysate enhances spirochete load in mice and is tick species-specific. J Parasitol (2002) 88:1276–8.10.1645/0022-3395(2002)088[1276:COBSWT]2.0.CO;2
172
RamamoorthiNNarasimhanSPalUBaoFYangXFFishDet alThe Lyme disease agent exploits a tick protein to infect the mammalian host. Nature (2005) 436:573–7.10.1038/nature03812
173
KuthejlováMKopeckýJStepánováGMacelaA. Tick salivary gland extract inhibits killing of Borrelia afzelii spirochetes by mouse macrophages. Infect Immun (2001) 69:575–8.10.1128/IAI.69.1.575-578.2001
174
SeverinováJSalátJKročováZŘezníčkováJDemováHHorkáHet alCo-inoculation of Borrelia afzelii with tick salivary gland extract influences distribution of immunocompetent cells in the skin and lymph nodes of mice. Folia Microbiol (Praha) (2005) 50:457–63.10.1007/BF02931430
175
GuoXBoothCJPaleyMAWangXDePonteKFikrigEet alInhibition of neutrophil function by two tick salivary proteins. Infect Immun (2009) 77:2320–9.10.1128/IAI.01507-08
176
HorkáHCerná-KýckováKSkallováAKopeckýJ. Tick saliva affects both proliferation and distribution of Borrelia burgdorferi spirochetes in mouse organs and increases transmission of spirochetes to ticks. Int J Med Microbiol (2009) 299:373–80.10.1016/j.ijmm.2008.10.009
177
MarchalCSchrammFKernALuftBJYangXSchuijtTet alAntialarmin effect of tick saliva during the transmission of Lyme disease. Infect Immun (2011) 79:774–85.10.1128/IAI.00482-10
178
LawrieCHRandolphSENuttallPA. Ixodes ticks: serum species sensitivity of anticomplement activity. Exp Parasitol (1999) 93:207–14.10.1006/expr.1999.4456
179
GillespieRDMbowMLTitusRG. The immunomodulatory factors of bloodfeeding arthropod saliva. Parasite Immunol (2000) 22:319–31.10.1046/j.1365-3024.2000.00309.x
180
ValenzuelaJGCharlabRMatherTNRibeiroJMC. Purification, cloning, and expression of a novel salivary anticomplement protein from the tick, Ixodes scapularis. J Biol Chem (2000) 275:18717–23.10.1074/jbc.M001486200
181
LawrieCHSimRBNuttallPA. Investigation of the mechanisms of anti-complement activity in Ixodes ricinus ticks. Mol Immunol (2005) 42:31–8.10.1016/j.molimm.2004.07.001
182
DaixVSchroederHPraetNGeorginJ-PChiappinoIGilletLet alIxodes ticks belonging to the Ixodes ricinus complex encode a family of anticomplement proteins. Insect Mol Biol (2007) 16:155–66.10.1111/j.1365-2583.2006.00710.x
183
HourcadeDEAkkAMMitchellLMZhouHHauhartRPhamCTN. Anti-complement activity of the Ixodes scapularis salivary protein Salp20. Mol Immunol (2016) 69:62–9.10.1016/j.molimm.2015.11.008
184
HoviusJWRde JongMAWPden DunnenJLitjensMFikrigEvan der PollTet alSalp15 binding to DC-SIGN inhibits cytokine expression by impairing both nucleosome remodeling and mRNA stabilization. PLoS Pathog (2008) 4:e31.10.1371/journal.ppat.0040031
185
AnguitaJRamamoorthiNHoviusJWRDasSThomasVPersinskiRet alSalp15, an Ixodes scapularis salivary protein, inhibits CD4+ T cell activation. Immunity (2002) 16:849–59.10.1016/S1074-7613(02)00325-4
186
HoviusJWSchuijtTJde GrootKARoelofsJJTHOeiGAMarquartJAet alPreferential protection of Borrelia burgdorferi sensu stricto by a Salp 15 homologue in Ixodes ricinus saliva. J Infect Dis (2008) 198:1189–97.10.1086/591917
187
SchuijtTJHoviusJWRvan BurgelNDRamamoorthiNFikrigEvan DamAP. The tick salivary protein Salp15 inhibits the killing of serum-sensitive Borrelia burgdorferi sensu lato isolates. Infect Immun (2008) 76:2888–94.10.1128/IAI.00232-08
188
MuraseYKonnaiSYamadaSGithakaNIsezakiMItoTet alAn investigation of binding ability of Ixodes persulcatus Schulze Salp15 with Lyme disease spirochetes. Insect Biochem Mol Biol (2015) 60:59–67.10.1016/j.ibmb.2015.01.010
189
DaiJWangPAdusumilliSBoothCJNarasimhanSAnguitaJet alAntibodies against a tick protein, Salp15, protect mice from the Lyme disease agent. Cell Host Microbe (2009) 6:482–92.10.1016/j.chom.2009.10.006
190
TysonKElkinsCPattersonHFikrigEDe SilvaA. Biochemical and functional characterization of Salp20, an Ixodes scapularis tick salivary protein that inhibits the complement pathway. Insect Mol Biol (2007) 16:469–79.10.1111/j.1365-2583.2007.00742.x
191
TysonKRElkinsCde SilvaAM. A novel mechanism of complement inhibition unmasked by a tick salivary protein that binds to properdin. J Immunol (2008) 180:3964–8.10.4049/jimmunol.180.6.3964
192
CouvreurBBeaufaysJCharonCLahayeKGensaleFDenisVet alVariability and action mechanism of a family of anticomplement proteins in Ixodes ricinus. PLoS One (2008) 3:e1400.10.1371/journal.pone.0001400
193
AstigarragaAOleaga-PérezAPérez-SánchezRBarandaJAEncinas-GrandesA. Host immune response evasion strategies in Ornithodoros erraticus and O. moubata and their relationship to the development of an antiargasid vaccine. Parasite Immunol (1997) 19:401–10.10.1046/j.1365-3024.1997.d01-236.x
194
TabuchiNKataoka-UshijimaYTalbertAMitaniHFukunagaM. Absence of transovarial transmission of Borrelia duttonii, a tick-borne relapsing fever agent, by the vector tick Ornithodoros moubata. Vector Borne Zoonotic Dis (2008) 8:607–13.10.1089/vbz.2007.0279
195
NunnMASharmaAPaesenGCAdamsonSLissinaOWillisACet alComplement inhibitor of C5 activation from the soft tick Ornithodoros moubata. J Immunol (2005) 174:2084–91.10.4049/jimmunol.174.4.2084
196
HepburnNJWilliamsASNunnMAChamberlain-BanoubJCHamerJMorganBPet alIn vivo characterization and therapeutic efficacy of a C5-specific inhibitor from the soft tick Ornithodoros moubata. J Biol Chem (2007) 282:8292–9.10.1074/jbc.M609858200
197
MaYWeisJJ. Borrelia burgdorferi outer surface lipoproteins OspA and OspB possess B-cell mitogenic and cytokine-stimulatory properties. Infect Immun (1993) 61:3843–53.
198
BolzDDSundsbakRSMaYAkiraSKirschningCJZacharyJFet alMyD88 plays a unique role in host defense but not arthritis development in Lyme disease. J Immunol (2004) 173:2003–10.10.4049/jimmunol.173.3.2003
199
MeierJTSimonMIBarbourAG. Antigenic variation is associated with DNA rearrangements in a relapsing fever Borrelia. Cell (1985) 41:403–9.10.1016/S0092-8674(85)80013-1
200
BarbourAGBurmanNCarterCJKittenTBergströmS. Variable antigen genes of the relapsing fever agent Borrelia hermsii are activated by promoter addition. Mol Microbiol (1991) 5:489–93.10.1111/j.1365-2958.1991.tb02132.x
201
MarconiRTSamuelsDSSchwanTGGaronCF. Identification of a protein in several Borrelia species which is related to OspC of the Lyme disease spirochetes. J Clin Microbiol (1993) 31:2577–83.
202
CarterCJBergströmSNorrisSJBarbourAG. A family of surface-exposed proteins of 20 kilodaltons in the genus Borrelia. Infect Immun (1994) 62:2792–9.
203
ZhangJ-RHardhamJMBarbourAGNorrisSJ. Antigenic variation in Lyme disease borreliae by promiscuous recombination of Vmp-like sequence cassettes. Cell (1997) 89:275–85.10.1016/S0092-8674(00)80206-8
204
BurmanNShamaei-TousiABergströmS. The spirochete Borrelia crocidurae causes erythrocyte rosetting during relapsing fever. Infect Immun (1998) 66:815–9.
205
BrissetteCACooleyAEBurnsLHRileySPVermaAWoodmanMEet alLyme borreliosis spirochete Erp proteins, their known host ligands, and potential roles in mammalian infection. Int J Med Microbiol (2008) 298:257–67.10.1016/j.ijmm.2007.09.004
206
KenedyMRLenhartTRAkinsDR. The role of Borrelia burgdorferi outer surface proteins. FEMS Immunol Med Microbiol (2012) 66:1–19.10.1111/j.1574-695X.2012.00980.x
207
SchutzerSECoylePKKruppLBDengZBelmanALDattwylerRet alSimultaneous expression of Borrelia OspA and OspC and IgM response in cerebrospinal fluid in early neurologic Lyme disease. J Clin Invest (1997) 100:763–7.10.1172/JCI119589
208
BunikisJBarbourAG. Access of antibody or trypsin to an integral outer membrane protein (P66) of Borrelia burgdorferi is hindered by Osp lipoproteins. Infect Immun (1999) 67:2874–83.
209
SchwanTGPiesmanJGoldeWTDolanMCRosaPA. Induction of an outer surface protein on Borrelia burgdorferi during tick feeding. Proc Natl Acad Sci U S A (1995) 92:2909–13.10.1073/pnas.92.7.2909
210
LiangFTJacobsMBBowersLCPhilippMT. An immune evasion mechanism for spirochetal persistence in Lyme borreliosis. J Exp Med (2002) 195:415–22.10.1084/jem.20011870
211
GrimmDTillyKByramRStewartPEKrumJGBueschelDMet alOuter-surface protein C of the Lyme disease spirochete: a protein induced in ticks for infection of mammals. Proc Natl Acad Sci U S A (2004) 101:3142–7.10.1073/pnas.0306845101
212
PalUYangXChenMBockenstedtLKAndersonJFFlavellRAet alOspC facilitates Borrelia burgdorferi invasion of Ixodes scapularis salivary glands. J Clin Invest (2004) 113:220–30.10.1172/JCI19894
213
LagalVPortnoïDFaureGPosticDBarantonG. Borrelia burgdorferi sensu stricto invasiveness is correlated with OspC-plasminogen affinity. Microbes Infect (2006) 8:645–52.10.1016/j.micinf.2005.08.017
214
TillyKKrumJGBestorAJewettMWGrimmDBueschelDet alBorrelia burgdorferi OspC protein required exclusively in a crucial early stage of mammalian infection. Infect Immun (2006) 74:3554–64.10.1128/IAI.01950-05
215
TillyKBestorAJewettMWRosaP. Rapid clearance of Lyme disease spirochetes lacking OspC from skin. Infect Immun (2007) 75:1517–9.10.1128/IAI.01725-06
216
CarrascoSETroxellBYangYBrandtSLLiHSanduskyGEet alOuter surface protein OspC is an antiphagocytic factor that protects Borrelia burgdorferi from phagocytosis by macrophages. Infect Immun (2015) 83:4848–60.10.1128/IAI.01215-15
217
TheisenMBorreMMathiesenMJMikkelsenBLebechA-MHansenK. Evolution of the Borrelia burgdorferi outer surface protein OspC. J Bacteriol (1995) 177:3036–44.10.1128/jb.177.11.3036-3044.1995
218
SeinostGDykhuizenDEDattwylerRJGoldeWTDunnJJWangI-Net alFour clones of Borrelia burgdorferi sensu stricto cause invasive infection in humans. Infect Immun (1999) 67:3518–24.
219
WangI-NDykhuizenDEQiuWDunnJJBoslerEMLuftBJ. Genetic diversity of ospC in a local population of Borrelia burgdorferi sensu stricto. Genetics (1999) 151:15–30.
220
BrissonDDykhuizenDE. ospC diversity in Borrelia burgdorferi different hosts are different niches. Genetics (2004) 168:713–22.10.1534/genetics.104.028738
221
EarnhartCGBucklesELDumlerJSMarconiRT. Demonstration of OspC type diversity in invasive human Lyme disease isolates and identification of previously uncharacterized epitopes that define the specificity of the OspC murine antibody response. Infect Immun (2005) 73:7869–77.10.1128/IAI.73.12.7869-7877.2005
222
WormserGPBrissonDLiverisDHanincováKSandigurskySNowakowskiJet alBorrelia burgdorferi genotype predicts the capacity for hematogenous dissemination during early Lyme disease. J Infect Dis (2008) 198:1358–64.10.1086/592279
223
LawrenzMBHardhamJMOwensRTNowakowskiJSteereACWormserGPet alHuman antibody responses to VlsE antigenic variation protein of Borrelia burgdorferi. J Clin Microbiol (1999) 37:3997–4004.
224
HudsonCRFryeJGQuinnFDGherardiniFC. Increased expression of Borrelia burgdorferi vlsE in response to human endothelial cell membranes. Mol Microbiol (2001) 41:229–39.10.1046/j.1365-2958.2001.02511.x
225
AnguitaJThomasVSamantaSPersinskiRHernanzCBartholdSWet alBorrelia burgdorferi-induced inflammation facilitates spirochete adaptation and variable major protein-like sequence locus recombination. J Immunol (2001) 167:3383–90.10.4049/jimmunol.167.6.3383
226
CrotherTRChampionCIWuX-YBlancoDRMillerJNLovettMA. Antigenic composition of Borrelia burgdorferi during infection of SCID mice. Infect Immun (2003) 71:3419–28.10.1128/IAI.71.6.3419-3428.2003
227
PiesmanJZeidnerNSSchneiderBS. Dynamic changes in Borrelia burgdorferi populations in Ixodes scapularis (Acari: Ixodidae) during transmission: studies at the mRNA level. Vector Borne Zoonotic Dis (2003) 3:125–32.10.1089/153036603768395825
228
LiangFTYanJMbowMLSviatSLGilmoreRDMamulaMet alBorrelia burgdorferi changes its surface antigenic expression in response to host immune responses. Infect Immun (2004) 72:5759–67.10.1128/IAI.72.10.5759-5767.2004
229
LawrenzMBWootenRMNorrisSJ. Effects of vlsE complementation on the infectivity of Borrelia burgdorferi lacking the linear plasmid lp28-1. Infect Immun (2004) 72:6577–85.10.1128/IAI.72.11.6577-6585.2004
230
BankheadTChaconasG. The role of VlsE antigenic variation in the Lyme disease spirochete: persistence through a mechanism that differs from other pathogens. Mol Microbiol (2007) 65:1547–58.10.1111/j.1365-2958.2007.05895.x
231
CoutteLBotkinDJGaoLNorrisSJ. Detailed analysis of sequence changes occurring during vlsE antigenic variation in the mouse model of Borrelia burgdorferi infection. PLoS Pathog (2009) 5:e1000293.10.1371/journal.ppat.1000293
232
BaumEHueFBarbourAG. Experimental infections of the reservoir species Peromyscus leucopus with diverse strains of Borrelia burgdorferi, a Lyme disease agent. MBio (2012) 3:e434–412.10.1128/mBio.00434-12
233
RogovskyyASBankheadT. Variable VlsE is critical for host reinfection by the Lyme disease spirochete. PLoS One (2013) 8:e61226.10.1371/journal.pone.0061226
234
TillyKBestorARosaPA. Lipoprotein succession in Borrelia burgdorferi: similar but distinct roles for OspC and VlsE at different stages of mammalian infection. Mol Microbiol (2013) 89:216–27.10.1111/mmi.12271
235
NorrisSJ. vls antigenic variation systems of Lyme disease Borrelia: eluding host immunity through both random, segmental gene conversion and framework heterogeneity. Microbiol Spectr (2014) (6):1–18.10.1128/microbiolspec.MDNA3-0038-2014
236
JacekETangKSKomorowskiLAjamianMProbstCStevensonBet alEpitope-specific evolution of human B cell responses to Borrelia burgdorferi VlsE protein from early to late stages of Lyme disease. J Immunol (2016) 196:1036–43.10.4049/jimmunol.1501861
237
BarbourAG. Antigenic variation of a relapsing fever Borrelia species. Annu Rev Microbiol (1990) 44:155–71.10.1146/annurev.mi.44.100190.001103
238
BarbourAGCarterCJSohaskeyCD. Surface protein variation by expression site switching in the relapsing fever agent Borrelia hermsii. Infect Immun (2000) 68:7114–21.10.1128/IAI.68.12.7114-7121.2000
239
BarbourAGDaiQRestrepoBIStoennerHGFrankSA. Pathogen escape from host immunity by a genome program for antigenic variation. Proc Natl Acad Sci U S A (2006) 103:18290–5.10.1073/pnas.0605302103
240
DaiQRestrepoBIPorcellaSFRaffelSJSchwanTGBarbourAG. Antigenic variation by Borrelia hermsii occurs through recombination between extragenic repetitive elements on linear plasmids. Mol Microbiol (2006) 60:1329–43.10.1111/j.1365-2958.2006.05177.x
241
TeeglerAHerzbergerPMargosGFingerleVKraiczyP. The relapsing fever spirochete Borrelia miyamotoi resists complement-mediated killing by human serum. Ticks Tick Borne Dis (2014) 5:898–901.10.1016/j.ttbdis.2014.07.011
242
WagemakersAOeiAFikrigMMMielletWRHoviusJW. The relapsing fever spirochete Borrelia miyamotoi is cultivable in a modified Kelly-Pettenkofer medium, and is resistant to human complement. Parasit Vectors (2014) 7:418.10.1186/1756-3305-7-418
243
NewmanKJohnsonRC. In vivo evidence that an intact lytic complement pathway is not essential for successful removal of circulating Borrelia turicatae from mouse blood. Infect Immun (1981) 31:465–9.
244
HamaseATakahashiYNohgiKFukunagaM. Homology of variable major protein genes between Borrelia hermsii and Borrelia miyamotoi. FEMS Microbiol Lett (1996) 140:131–7.10.1111/j.1574-6968.1996.tb08326.x
Summary
Keywords
Borrelia miyamotoi, spirochetes, relapsing fever, Lyme disease, complement, factor H, antigenic variation, immune response
Citation
Stone BL and Brissette CA (2017) Host Immune Evasion by Lyme and Relapsing Fever Borreliae: Findings to Lead Future Studies for Borrelia miyamotoi. Front. Immunol. 8:12. doi: 10.3389/fimmu.2017.00012
Received
21 October 2016
Accepted
05 January 2017
Published
19 January 2017
Volume
8 - 2017
Edited by
Monica E. Embers, Tulane University, USA
Reviewed by
Peter Kraiczy, Goethe University Frankfurt, Germany; Robert D. Gilmore, Centers for Disease Control and Prevention, USA
Updates
Copyright
© 2017 Stone and Brissette.
This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
*Correspondence: Catherine A. Brissette, catherine.brissette@med.und.edu
Specialty section: This article was submitted to Microbial Immunology, a section of the journal Frontiers in Immunology
Disclaimer
All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article or claim that may be made by its manufacturer is not guaranteed or endorsed by the publisher.