Immunotherapy for tularemia.

Francisella tularensis is a gram-negative bacterium that causes the zoonotic disease tularemia. Francisella is highly infectious via the respiratory route (~10 CFUs) and pulmonary infections due to type A strains of F. tularensis are highly lethal in untreated patients (> 30%). In addition, no vaccines are licensed to prevent tularemia in humans. Due to the high infectivity and mortality of pulmonary tularemia, F. tularensis has been weaponized, including via the introduction of antibiotic resistance, by several countries. Because of the lack of efficacious vaccines, and concerns about F. tularensis acquiring resistance to antibiotics via natural or illicit means, augmentation of host immunity, and humoral immunotherapy have been investigated as countermeasures against tularemia. This manuscript will review advances made and challenges in the field of immunotherapy against tularemia.

Tularemia

Francisella tularensis is a highly infectious, gram-negative facultative intracellular bacterium that causes the zoonotic disease tularemia. In 1911, tularemia was first described as a plague-like disease of rodents and soon after the potential of tularemia as a severe and fatal human illness was recognized.F. tularensis infections can occur via insect or tick bites, cutaneous contact with infected animal carcasses, ingestion of contaminated food and water, or inhalation of viable organisms.F. tularensis has long been known as a potential hazard to laboratory workers, and has been one of the most commonly reported laboratory-acquired infections in the United States. In nature, F. tularensis mainly exists in regions of the United States, Canada, Mexico, Japan, Europe, and the former Soviet Union. Several animals, including rabbits, muskrats, and beavers can serve as reservoirs of infection. Tularemia is also carried by ticks, deerflies, and mosquitoes. The type and severity of tularemia depends on the strain, dose, and route of infection.F. tularensis subspecies tularensis (type A) and holarctica (type B) cause the majority of human cases, with subspecies tularensis being more virulent. Type A F. tularensis is found predominately in North America, while type B strains are found in Europe and Asia. All forms of tularemia generally present with sudden onset of fever, headaches, chills, sore throat, coryza, and generalized body aches 3–5 d after exposure. With appropriate antibiotic therapy, the overall mortality rate of reported tularemia cases in the United States is less than 2%.,

Cutaneous or ulceroglandular tularemia is the most common form of human disease (75–85% of patients), but is rarely fatal., A cutaneous papule appears at the site of infection around the time of generalized symptoms in ulceroglandular tularemia. The papule becomes a painful pustule and ulcerates within a few days of its first appearance. Regional lymph nodes also may become enlarged and tender within days of papule appearance. Even with appropriate antibiotic therapy, affected lymph nodes may rupture and become fluctuant and the ulcer and lymphadenopathy may persist for months.,

Pulmonary tularemia is the most severe form of disease and untreated pulmonary infections with type A F. tularensis infection have mortality rates >30%. Inhalation of F. tularensis results in respiratory or pneumonic tularemia and is most common in people in endemic areas who perform tasks that predispose them to infectious aerosols. Pulmonary tularemia can present from a mild pneumonia to an acute infection with high fever, malaise, chills, cough, delirium, and pulse-temperature dissociation., Hilar lymphadenopathy, pleural effusions, and bronchopneumonia are common radiographic findings; however, early radiologic evidence of pneumonia was found in only 25–50% of human volunteers who had developed systemic symptoms of acute illness following aerosol exposure to type A F. tularensis.,,

F. tularensis as a Biological Weapon

The World Health Organization (WHO) estimated in 1970 that an aerosol dispersal of 50 kg of virulent F. tularensis over a metropolitan area of 5 million residents would result in 250 000 incapacitating casualties including 19 000 deaths. Disease was expected to persist for several weeks and relapses of illness would occur during the following weeks and months. In 1997, the CDC estimated that the total societal base costs of a F. tularensis aerosol attack would be $5.4 billion for every 100 000 exposed persons. While a live vaccine strain (LVS) derived from F. tularensis subspecies holarctica was created over 50 years ago, questions remain regarding its efficacy and possible reversion to virulence, and it is not licensed for human use. Due to the high infectivity (~10 microorganisms) and lethality of untreated pulmonary tularemia and the lack of available vaccines, F. tularensis has long been studied as a biological weapon by several nations. F. tularensis was tested on human subjects in occupied Manchuria as part of a Japanese germ warfare program from 1932 to 1945. Tularemia outbreaks that affected tens of thousands of German and Soviet soldiers in Eastern Europe in World War II were also suggested to be the result of an intentional Soviet release of F. tularensis; however, this hypothesis has been disputed. Following World War II, the United States military studied the pathophysiology of tularemia and researched vaccine development and antibiotic prophylaxis, including work investigating antibiotic therapy in human subjects exposed to virulent F. tularensis in aerosol chambers., The United States also developed weapons that would disseminate F. tularensis aerosols and F. tularensis was one of several biological weapons stockpiled by the United States in the 1960s until the inventories were destroyed in the early 1970s. Of particular concern would be the release of F. tularensis that had been weaponized via the introduction of antibiotic resistance. Indeed the United States developed streptomycin-resistant strains of F. tularensis before shuttering its offensive biological weapons program, and the Soviet Union was purported to develop antibiotic-resistant strains of Francisella perhaps until the 1990s. Due to these concerns, F. tularensis has been determined to be a Category A biological warfare agent by CDC, and the two major spikes in tularemia research publications have come shortly after World War II and the 2001 anthrax bioterrorist attacks in the United States (Fig. 1).

Figure 1. The number of articles published per year found in PubMed using the search phrase “Francisella or tularemia or tularense or tularaemia or tularensis”.

Precautions When Investigating Immunotherapy of Tularemia

The route of Francisella challenge affects induced immune responses, and rodents are generally much more susceptible to intraperitoneal (i.p.) or pulmonary challenge then to a subcutaneous (s.c.) or intradermal challenge (i.d.). The host species used for tularemia immunity and immunotherapy studies is also of importance due to varying susceptibilities. While mice are extremely susceptible to tularemia, rats, rabbits, and non-human primates are relatively more resistant to infection. Perhaps most importantly, emerging evidence indicates that immunity against virulent strains of F. tularensis that cause disease in humans differs from protective immune responses elicited by model strains of Francisella.- Virulent strains of F. tularensis also employ mechanisms of immune suppression not found in model strains.- In addition, vaccination and immunotherapeutic strategies that confer robust protection against attenuated strains of F. tularensis have been shown to have little to no efficacy against strains of Francisella that cause disease in humans.- Therefore, the challenge strain of F. tularensis must be considered when considering the protective efficacy of immunotherapeutics. For reference, the relative virulence of common challenge strains of Francisella used in immunotherapy studies covered here is shown in Table 1 from information in reviews by Cowley and Elkins, and Wu and Lyons., In some early studies reviewed here, the challenge strain was called “virulent” but no strain designation was given. In these instances we will refer to these strains as “virulent F. tularensis”. Our review of the literature on Francisella immunotherapeutics generally follows a chronologic order under each heading or within a paragraph. However, Tables 2A, 2B, 3A, and 3B have been subdivided to clarify which immunotherapeutics are effective against virulent strains of Francisella such as SchuS4, vs. those that have only shown efficacy against model strains such as LVS or F. novicida. Also, immunotherapy strategies that confer survival of treated animals are listed before immunotherapeutics that extend the mean time to death or reduce bacterial burdens within the subdivisions of the tables. Immunity to Francisella has been recently reviewed by others,, therefore in this review we will only discuss immunity in the context of protective immunotherapy. In addition, we will have a particular emphasis on immune agonists that induce protection against tularemia.

Table 1. Virulence in mammals of Francisella challenge strains in this reviewa

Strain	Challenge strains in this review	Human infection	Mouse infection	Rat infection
Subspecies tularensis type A	Schu, SchuS4, SchuS5, Vavenby	Highly infectious and can be fatal	LD50 < 10, all routes tested	LD50 = 5 × 102 IT
Subspecies holarctica type B	FSC 171	Induces illness but rarely fatal	LD50 < 10, all routes tested	Unknown
Subspecies holarctica LVS	LVS	Attenuated Type B strain, skin or pulmonary infection induces mild side symptoms, induces protective immunity	LD50 = 106 ID, 103 IN, < 10 IP or IV	Unknown
F. novicida	U112	Infections rare, sublethal, and associated with immunodeficiencies	LD50 = 103 ID, < 10 IN, IP, or IV	LD50 = 5 × 106 IT

a Table adapted from Cowley and Elkins

Table 2A. Immune agonists that confer protection against virulent Francisella infection

Agonist	Cellular receptor	Challenge strain, route, animal	Protective effect	Requirements for protection
Acai PS	TLR4? Carbohydrate Receptors?	Mice infected via aerosol with SchuS4	i.n. pre- or post-treatment increased survival rates	IFN-γ
CLDC+MPF	TLR9+DAI	Mice infected i.n. with SchuS4	i.v. pre-treatment increased survival rate	RNS/ROS
MPL	TLR4	Mice infected i.n. with LVS or SchuS4	i.p. pre-treatment increased survival rates in animals challenged with either strain.	ND
Yeast glucans	Carbohydrate receptors?	Rats infected i.p. with SchuS4	i.v. pre-treatment increased survival rate	ND
Poly I:C	TLR3	Mice infected i.n. with LVS or SchuS4	i.n. pre- or post-treatment extended mean time to death in LVS- and SchuS4- challenged animals	ND
CLDC	TLR9+DAI	Mice infected i.n. with LVS or SchuS4	i.n. pre-treatment increased survival rates in LVS-challenged mice and extended mean time to death in SchuS4-challenged mice	IFN-γ, NK cells (LVS-challenged mice)

See text for references. ?, cellular receptor unknown or unclear; ND, not determined; astrain used for challenge unclear.

.

Immune agonists that confer protection against model strains of Francisella, but have unknown, or no protective effects against virulent F. tularensis

Agonist	Cellular receptor	Challenge strain, route, animal	Protective effect	Requirements for protection
Endotoxin	TLR4	Mice infected i.p. with F. tularensisa	i.p. pre-treatment increased survival rate	ND
AGP	TLR4	Mice infected i.n. with F. novicida	i.n. pre- and post-treatment increased survival rate	IFN-γ
LVS LPS	?	Mice infected i.p. with LVS or i.n. with SchuS4	i.p. pre-treatment increased survival rates in LVS challenged animalsNo protective effect observed in mice challenged with SchuS4	TLR2, IRAK4, B cells, antibody
CpG	TLR9	Mice infected i.p. with LVS or i.n. with SchuS4	i.p. pre-treatment increased survival rate in LVS challenged animalsi.n. or i.p. pre-treatment had no protective effect in mice challenged i.n. with SchuS4	B cells, IFN-γ TLR9
Poly I:C	TLR3	Mice infected i.p. with F. tularensisa	i.p. pre-treatment extended mean time to death	ND
Tilorone	?	Mice infected i.p. with F. tularensisa	i.p. pre-treatment extended mean time to death	ND
L1S	TLR4?	Mice infected i.p. with LVS	i.p. pretreatment lowered tissue burdens	ND

See text for references. ?, cellular receptor unknown or unclear; ND, not determined; astrain used for challenge unclear.

Table 3A. Effective serum immunotherapy against virulent F. tularensis infection

Immunogen	Serum donor	Challenge animal, route, strain	Protective effect	Requirements for protection
Formalin-killed F. tularensis Schu	Horse	Rats infected s.c. with Schu	i.p. pre-treatment increased survival rate	ND
Live F. tularensis Schu	Goat	Rats infected s.c. with Schu	i.p. pre-treatment increased survival rate	ND
Formalin-killed virulent F. tularensis	Rabbit	Rats infected i.p. with virulent F. tularensis.	Mixture of serum with inoculum before i.p. challenge increased survival rate, i.p. post-treatment delayed mean time to death	ND
Live F. tularensis	Recovered or Convalescent Human Patient	Rats infected i.p. with virulent F. tularensis	Mixture of serum with inoculum before i.p. challenge increased survival rate	ND
Formalin-killed F. tularensis	Human	Rats infected i.p. with virulent F. tularensis	Mixture of serum with inoculum before i.p. challenge increased survival rate	ND
Formalin-killed F. tularensis	Goat	Rats infected i.p. with virulent F. tularensis	Mixture of serum with inoculum before i.p. challenge increased survival rate	ND
Live F. tularensis SchuS4	Micea	Mice infected i.n. with SchuS4	i.p. pre- or post- treatment increased survival rates	ND
Live F. tularensis LVS	Rat	Rats infected i.t. with SchuS4	i.p. pre-treatment increased survival rate	IgG, CD8+ T cells
F. tularensis LVS MPF	Mice	Mice infected i.n. with SchuS4	i.p. post-treatment increased survival rate when given in conjunction with suboptimal gentamicin	ND
?	Horse	Mice infected i.p. with virulent F. tularensis	Mixture of hyperimmune serum with inoculum or i.p. treatment with serum immediately after challenge extended mean time to death	ND
Live virulent F. tularensis	Sheep	Mice infected i.p. with virulent F. tularensis	Mixture of serum with inoculum before i.p. challenge extended mean time to death	ND
Formalin-killed virulent F. tularensis	Rabbit	Mice infected i.p. or s.c. with virulent F. tularensis	Mixture of serum with inoculum before i.p. challenge extended mean time to deathi.p. pre-treatment before s.c. challenge extended mean time to death	ND
?	Horse	Guinea pigs infected s.c. with Vavenby	Intracardial pre-treatment with hyperimmune horse serum extended mean time to death	ND
Acetone-killed F. tularensis SchuS5	Mice	Mice infected i.p. or s.c. with SchuS5	i.p. pre-treatment extended mean time to death	ND
?	Mice, guinea pig, or rabbit	Mice infected i.p. with virulent F. tularensis 9K 161t	i.p. pre- and post-treatment extended mean time to death	ND
Live F. tularensis LVS	Mice	Mice infected i.d. with FSC 71	i.p. pre-treatment reduced bacterial burdens and morbidity	ND
Live and sonicated F. tularensis LVS	Mice	Mice infected i.d. with LVS or SchuS4	i.p. pre- or post-treatment with mAb reactive with LPS increased survival rate of LVS-challenged animalsi.p. pre-treatment extended time to death of SchuS4-challenged animals	ND

See text for references. ?, immunogen not stated in manuscript; ND, not determined; amice were treated with levofloxacin to survive infection; broute of antibody transfer not stated.

Table 3B. Effective serum immunotherapy strategies against model strains of Francisella that have unknown, or no protective effects against virulent F. tularensis

Immunogen	Serum donor	Challenge animal, route, strain	Protective effect	Requirements for protection
Live F. tularensis LVS	Human	Mice infected i.p. with LVS	i.p. pre-treatment increased survival rate	ND
Live F. tularensis LVS	Mice	Mice infected i.p. with LVS	i.p. pre-treatment increased survival rate	IgG, T cells, IFN-γ
Live F. tularensis LVS	Mice	Wild-type or B cell-deficient mice infected i.d. with LVS	i.p. pre-treatment increased survival rates in B cell-deficient mice, and decreased bacterial burdens in both B cell-deficient and wild-type mice	ND
LPS from F. tularensis LVS	Mice	Mice infected i.p. with LVS	i.p. pre-treatment increased survival rate	ND
Live F. novicida ∆iglC	Mice	B cell-deficient mice infected i.n. with F. novicida	i.p. pre-treatment increased survival rate	ND
Live F. tularensis LVS	Mice	Mice infected i.n. with LVS	i.p. pre- or post-treatment increased survival rates	FCγR, IFN-γ, neutrophils, macrophages
Live F. tularensis LVS	Mice	Mice infected i.n. with LVS	i.p. or i.n. post-treatment with a mAb reactive with LVS LPS increased survival rates	ND
Heat-killed F. tularensis LVS	Mice	Mice infected i.p. with LVS	i.p. pre-treatment increased survival rate	ND
Live and sonicated F. tularensis LVS	Mice	Mice infected i.d. with LVS or SchuS4	Pre- or post-treatment with FopA -reactive mAb increased survival rates in LVS-challenged animals, no effect in SchuS4-challenged animalsb	ND
Live and sonicated F. tularensis LVS	Mice	Mice infected i.d. with LVS	Post-treatment with LpnA-reactive mAb increased survival rateb	ND
F. tularensis FopA	Mice	Mice infected i.d. with LVS	Pre- and post-treatment increased survival rateb	ND
Live or heat-killed F. tularensis LVS	Mice	Irradiated mice infected i.d. with LVS	i.p. pre-treatment increased survival rate	ND

See text for references. ?, immunogen not stated in manuscript; ND, not determined; amice were treated with levofloxacin to survive infection; broute of antibody transfer not stated.

Effector Mechanisms of Immunotherapeutics against Francisella

The success of Francisella as a pathogen is correlated with its ability to replicate in phagocytic cells. Therefore, activation of phagocytic cells, such as macrophages, has been investigated as immunotherapy for tularemia. IFN-γ and TNF-α can activate macrophages in vitro to restrict the replication of F. tularensis, while deficiencies in these cytokines render mice more susceptible to LVS and/or SchuS4 infection.- TNF-α and IFN-γ induce nitric oxide production, which in turn can restrict the intramacrophagic growth of LVS. The effect of TNF-α on SchuS4 replication in macrophages is unknown; however it has been shown that IFN-γ activation of macrophages for clearance of SchuS4 is independent of reactive oxygen and nitrogen species (ROS/RNS). IL-12 and Toll-Like receptor (TLR) signaling are also involved in IFN-γ and TNF-α production and are required for protection against Francisella in some models which has made them targets for immunotherapy.,- The role of type I IFNs in experimental models of Francisella infection is strain-specific. Endogenous type I IFNs are protective against LVS, deleterious against F. novicida, but do not appear to play a role in protective immunity against SchuS4. Addition of rIFN-β to human dendritic cells does not restrict intracellular replication of SchuS4; however addition of rIFN-β to murine macrophages or human dendritic cells infected with LVS is protective., While the role of type I IFNs in Francisella varies depending on the model, type I IFNs and agonists that induce them have shown efficacy against experimental tularemia.

The protective mechanisms of serum against Francisella have not been completely characterized; however antibody treatment of experimental tularemia has been shown to have efficacy. While Francisella is generally thought of as an intracellular pathogen, recent studies have shown that Francisella has a significant extracellular phase where it would likely be recognized by antibodies. Several actions of immune serum may contribute to its protective capability against tularemia. Serum from LVS-vaccinees enhances phagocytosis and killing of LVS by human neutrophils and facilitates the development of a respiratory burst.- Stenmark et al. showed that transfer of specific antibodies increased the expression of the cytokines TNF-α and IL-12, to the site of a cutaneous F. tularensis LVS infection. Neutrophil recruitment was also enhanced; however while neutrophils play a protective role when animals are challenged i.p with LVS, they appear to play a negligible role in immunity to pulmonary infection with LVS or type A F. tularensis., Control of LVS infections in IFN-γ treated alveolar macrophages was enhanced when LVS was opsonized with antibody prior to uptake, and the FCγ receptor was required for protection, indicating a role for opsonophagocytosis. Opsonization of virulent type A F. tularensis SchuS4 with antibody also increases pro-inflammatory cytokine production by macrophages. Interestingly, SchuS4, but not LVS binds plasmin, a host serine protease that degrades opsonizing antibodies, and may explain why LVS infections are more conducive to antibody immunotherapy than SchuS4 infections.

Generation of Protective Immunity against Model Strains of Francisella by Heterologous Infection or Cytokine Therapy

Some of the earliest studies of active immunotherapy against tularemia investigated the protective effects of heterologous infection. Mice that were previously infected i.p. with Rickettsia typhi were shown to be protected against i.p. challenge with attenuated strains of F. tularensis; however no effect was obtained when the virulent Schu strain was employed. Infection with the Mycobacterium bovis BCG vaccine conferred potent protection against F. novicida when mice were challenged i.d. Three weeks after intravenous (i.v.) BCG infection, however, no effect was achieved against SchuS4. Later studies showed that i.p. pre-infection with BCG could confer 100% survival against a lethal i.p. LVS challenge in mice. Macrophages from BCG-infected animals were shown to have enhanced clearance of LVS in vitro, and BCG-mediated protection against LVS both in vitro and in vivo was dependent on IFN-γ, TNF-α, and reactive nitrogen oxides. Macrophage activation by nitric oxide was also presumed to be the mechanism by which co-infection with F. novicida reduced the organ burdens of LVS in rats challenged i.p. with both LVS and F. novicida.

Cytokine administration has also shown efficacy against Francisella challenge in animal models. While the challenge strain was unclear (presumably LVS based on other studies by the authors), murine L-cell interferon (IFN-β) extended the time to death of mice infected i.p with Francisella when administered i.p. prior to challenge. Intranasal (i.n.) rIL-12 reduced tissue burdens and extended the time to death of mice infected i.n. with F. novicida when given 24 and 4 h prior to the time of challenge. rIL-12 conferred up to 100% survival when given i.n. in conjunction with gentamicin 8 and 24 h after F. novicida U112 challenge; however, this effect waned when treatment was delayed. rIFN-γ also enhanced the survival rates of U112-challenged mice treated with gentamicin when given 8 and 24 h post-challenge. Duckett et al. obtained similar results when testing rIL-12 as immunotherapy against F. tularensis LVS. Intranasal rIL-12 given 24 h before i.n. LVS infection reduced bacterial loads in the tissues and enhanced survival rates. This effect was dependent on IFN-γ and CD8+ T cells, but was not affected by the beige mutation in NK cells. Collectively, generation of protective immunity against Francisella by heterologous infection or cytokine administration may have potential, but efficacy against virulent challenge strains has yet to be demonstrated.

Induction of Rapid Protective Immunity against LVS with Francisella-derived LPS

In contrast to traditional lipopolysaccharide (LPS) from bacteria such as Salmonella or E. coli, Francisella LPS is not known to induce potent immune responses via TLR signaling. However, several groups have shown that Francisella LPS can generate rapid protective immunity against challenge with LVS. When given i.p., LVS LPS was shown to confer 100% protection against a lethal i.p. LVS challenge 2–3 d later while LPS from E. coli or Salmonella had no effect. While LPS was protective, it did not enhance proliferation or immunoglobulin secretion by murine B cells nor enhance the production of IL-4, IL-6, or IL-12 by murine splenocytes. Protection was shown to require B cells and IFN-γ, but not TLR4. Subsequent studies showed that i.p. LVS LPS or U112 LPS both could confer protection against i.p. LVS challenge, but no protection was generated against a F. novicida U112 challenge. Further mechanistic studies on LVS LPS showed that i.p. LVS LPS treatment given 2 or 7 d before i.p. LVS challenge could reduce tissue burdens and inflammatory gene expression in the liver despite the absence of detectable antibody against F. tularensis. However, later studies showed that LVS LPS-mediated protection against LVS required B cells and antibody produced by antigen-specific B-1a cells, but was independent of TLR4. It was also demonstrated that LVS LPS, but not LVS lipid A, was protective indicating a critical role for LPS carbohydrate in the induction of protection. TLR2 was required for LVS LPS-mediated protection against LVS challenge, although protection could be rescued in TLR2−/− mice when a TLR agonist such as synthetic E. coli MPL (TLR4) or flagellin (TLR5) was co-administered with LVS LPS. However, while LVS LPS is quite potent at protecting against LVS, no protective efficacy was obtained against an i.n. SchuS4 challenge.

Targeting Cellular Receptors to Induce Immunity against Francisella

Perhaps the largest focus of active immunotherapy studies against Francisella is the targeting of cellular receptors such as TLRs to induce protective innate immune responses. Giron et al. investigated the effect of several inducers of innate immunity against Francisella. The strain used for challenge is unclear (presumably i.p. LVS); however, endotoxin pre-treatment (TLR4) decreased the mortality rate of tularemia while pre-treatment with Poly (I:C) (TLR3) or Tilorone (an activator of NK cells) extended the mean time to death of mice. Poly I:C was further investigated as immunotherapy by Pyles et al. Poly (I:C) enhanced early pulmonary cytokine expression and neutrophil recruitment while decreasing bacterial loads in the lung when administered i.n. 1 h prior to or after i.n. LVS challenge. LVS-challenged mice also displayed increased survival time when treated i.n. with Poly (I:C) 1 h prior to infection. In addition, Poly (I:C) conferred partial protection against SchuS4. Intranasal Poly (I:C) administered 1 h before or simultaneously with i.n. SchuS4 challenge extended the mean time to death by 2 and 15 d respectively. Treating mice i.n. with Poly (I:C) 1 h after SchuS4 challenge also extended the treatment window for animals to be rescued by antibiotic therapy with levofloxacin.

Bacterial DNA containing CpG motifs that signal through TLR9 were shown to be effective at inducing protective innate immunity against F. tularensis LVS when given i.p. 1–14 d before infection by Elkins et al. CpG-treated mice displayed lower bacterial loads and protection was dependent on B cells and IFN-γ. Subsequent studies showed that lymphocytes from the spleens of mice treated with CpG could control the intramacrophagic growth of LVS in bone marrow-derived macrophages, an effect dependent on IFN-γ TNF-α, and IL-12, but not IL-4 or perforin. In the same study, it was also shown that TLR9 was required for CpG-mediated protection in vivo. Klinman et al. showed that repeated CpG administration could prolong this enhanced immunity to F. tularensis LVS. However, later studies showed that CpG was not protective against aerosol infection with SchuS4. Cationic liposome-DNA complexes (CLDC) which signal through TLR9 and other receptors such as cytosolic DAI (DNA-dependent activator of IRFs) also provide protection against tularemia. CLDC reduced organ burdens and conferred 100% survival when administered i.n. 1 d prior to i.n. LVS challenge. Protection against LVS required NK cells and IFN-γ, but not type I IFNs. Intranasal administration of CLDC at times prior to, or after 24 h pre-infection, or administration of CLDC via s.c., i.v., or i.p. routes diminished efficacy. However, while CLDC conferred 100% survival against LVS, only a moderate increase in time to death was obtained when testing CLDC immunotherapy against a pulmonary SchuS4 challenge. Ireland et al. improved upon the efficacy of CLDC by combining it with a crude F. tularensis membrane protein fraction (MPF). When given i.v. 3 d prior to an i.n. infection with SchuS4, 60% of the animals that received CLDC + MPF survived a lethal challenge. CLDC + MPF was found to induce reactive nitrogen (RNS) and oxygen (ROS) species genes in vitro, and in vivo protection was shown to be dependent on RNS/ROS as nos2/gp91−/− mice were not protected against SchuS4 by CLDC + MPF.

Lembo et al. showed that i.n. administration of the synthetic TLR4 agonist AGP 48 h prior to and 24 h after aerosol F. novicida infection augmented cytokine production in the lung and reduced bacterial burdens in the tissues. This treatment regimen also enhanced the survival rate of mice by up to 50%, an effect dependent on IFN-γ; however, treatment with AGP post-infection did not affect survival. Another synthetic TLR4 agonist, MPL, conferred 43% and 20% survival when given i.p. 2 d before, or at the time of i.n. SchuS4 challenge respectively. However co-administration of LVS LPS, which confers potent protection against LVS infection, did not augment MPL-mediated protection against SchuS4. The L1S fragment of p60, a secreted protein from Listeria monocytogenes that also may signal through TLR4, also displayed efficacy against LVS. L1S enhanced activation of naïve murine NK cells in vivo and decreased tissue burdens while increasing IFN-γ levels in LVS-infected mice when L1S was administered i.p. 24 h prior to i.p. challenge.

Innate immune agonists that signal through receptors other than TLRs have also shown protection against virulent F. tularensis infection. Yeast glucans, which can induce innate immunity through various carbohydrate receptors, were shown to be efficacious against tularemia in rats by Reynolds et al. Intravenous pre-treatment of glucans for several days prior to i.p. infection with SchuS4 increased the survival rate of rats by 68%. Glucans also enhanced the survival of rats when given i.v. before aerosol challenge. In our own recent work, we have investigated the immunodulatory activity of polysaccharides derived from the pulp of the Acai berry (“Acai PS”). When given i.n. 1 d prior to aerosol infection with SchuS4, Acai PS conferred 80% survival against an otherwise lethal challenge. Acai PS was also effective when given after aerosol SchuS4 infection. Intranasal treatment of mice with Acai PS immediately after, 24 h after, or 48 h after aerosol challenge with SchuS4 resulted in respective survival rates of 73%, 60%, and 33%, making Acai PS the most potent active immunotherapeutic in the literature to treat pulmonary type A F. tularensis infection. We found that Acai PS enhanced IFN-γ expression by human NK cells in vitro, and murine NK cells in vivo, during F. tularensis infection, while neutralization of IFN-γ abrogated the protective effect of Acai PS. Further investigation of the immune responses induced by, and the cellular receptors that recognize Acai PS is ongoing, but Acai PS appears to require both TLR4/TRIF along with carbohydrate receptors (Holderness et al., manuscript in preparation) to mediate its effects. As both TLR4 and carbohydrate receptor agonists have shown efficacy against tularemia,, it is possible that activation of both of these immune receptor types by Acai PS may lead to synergetic potentiation of protective immunity. Therefore, future studies of the receptors required for Acai PS-mediated signaling and immune responses induced by Acai PS could reveal receptors and pathways of immunity to be targeted for immunotherapy against F. tularensis.

Early Studies of Immune Sera as Therapy for Tularemia

Interest in antibody therapy for tularemia was piqued by human trials in the 1940s in which Foshay purported that human tularemia patients treated with immune serum from goats or horses immunized with formaldehyde-killed Francisella before the end of the second week of disease resulted in significant reductions in mortality and all aspects of morbidity., However, studies in the 1940s also showed the difficulty of demonstrating protective efficacy against lethality induced by virulent F. tularensis challenge by serum therapy in rodent models. Francis and Felton found that treatment of mice with hyper-immune serum from sheep (infected s.c. with virulent F. tularensis), horses (immunogen unclear), or rabbits (injected i.v. with formalin-killed virulent F. tularensis) extended the mean time to death, but did not confer survival when serum was mixed with inoculum prior to i.p. challenge of mice with virulent F. tularensis. Similar results were found in guinea pigs by Bell and Kahn who showed that hyperimmune horse serum extended the mean time to death of guinea pigs when given intracardially prior to s.c. challenge with the virulent Vavenby strain of F. tularensis. Studies using immune sera raised in mice against acetone-killed F. tularensis SchuS5 (a streptomycin resistant virulent type A strain) only slightly increased the mean time to death when transferred to mice 3 d prior to i.p. or s.c. SchuS5 challenge. Comparable findings were obtained by Thorpe and Marcus who showed that sera from immunized mice, guinea pigs, or rabbits (immunogen unclear) could slightly extend the mean survival time of mice when transferred concomitantly and 24 h after i.p. challenge with the virulent F. tularensis strain, 9K 161t.

As early studies showed that transfer of immune sera into mice or guinea pigs was not able to confer survival against virulent F. tularensis challenge, Foshay et al. used the more resistant rat as the recipient of immune sera. Intraperitoneal transfer of hyperimmune serum from goats (immunized with F. tularensis Schu) or horses (immunized with formalin-killed F. tularensis Schu) at the time of s.c. challenge with the Schu strain of F. tularensis could confer survival rates as high as 87.5% as compared with 3.3–6.6% survival of rats treated with normal serum. Larson also showed that transfer of immune sera into rats could confer survival against virulent F. tularensis infection. Immune serum from goats or rabbits immunized with formalin-killed virulent Francisella conferred up to 70% survival when mixed with inoculum prior to i.p. challenge of rats with virulent F. tularensis; however, studies with rabbit serum showed that the protective effect waned when serum therapy was delayed until 24 h after challenge. Perhaps most importantly, the protective efficacy of human immune serum was also demonstrated in this study. When serum from human patients that had recovered from tularemia was mixed with virulent F. tularensis prior to i.p. infection of rats, up to 100% of rats survived an otherwise completely lethal challenge. Serum from a convalescent human tularemia patient or a human that had been immunized with formalin-killed F. tularensis also slightly increased the survival rate (up to 30%) and extended the mean time to death of rats infected i.p. with virulent F. tularensis. Convalescent and vaccine-induced serum had a significantly lower agglutination titer than serum from patients that had recovered from disease, which may explain the reduced protective efficacy of convalescent and vaccine-induced serum.

Immunotherapy Using Serum from Animals Infected with Live Francisella

After a lull in research on antibody-mediated protection against Francisella, studies in the 1990s again began to investigate humoral immunotherapy of tularemia by transferring serum from animals previously infected with Francisella. Drabick et al. demonstrated the protective efficacy of sera from human recipients of LVS vaccination. The authors found that i.p. transfer of pooled immune sera 2 h before i.p. infection with LVS fully protected mice against a 10 000 LD50 challenge. The human sera were found to react mostly with LVS lipopolysaccharide. This sera was also found to be cross-reactive with the polysaccharide from the virulent SchuS4 strain of F. tularensis; however the efficacy of challenge against virulent F. tularensis was not investigated.

Using mice as donors of serum, i.d. vaccination with LVS was shown to produce protective antibodies by several groups. Rhinehart-Jones et al. showed that transfer of immune serum from mice vaccinated i.d. with LVS at the time of i.p. LVS challenge could confer 100% survival against infection. This effect was found to be predominately dependent on IgG, and not IgM. Immune serum reduced colonization of the spleen by LVS; however serum transfer did not confer protection against LVS infection in nude mice or mice lacking IFN-γ. Immune serum generated by a sublethal i.d. LVS infection could also confer 100% survival and reduced bacterial loads in tissue when administered i.p. 1 d prior to a lethal i.d. LVS infection in B cell-deficient mice. Importantly, transfer of this immune serum also dramatically reduced bacterial burdens and morbidity in wild-type mice challenged i.d. with a virulent type B strain of F. tularensis, FSC 171. Passive transfer of antibody from animals vaccinated i.d. with LVS could also confer protection in immunodeficient irradiated mice. Kubelkova et al. showed that serum from mice given a sublethal i.d. LVS infection (or from mice that received heat-killed LVS i.d.) could provide 100% protection against a lethal i.d. LVS challenge in irradiated mice when given 2 h prior to LVS infection.

Serum immunotherapy has also proved protective in animal models of pulmonary tularemia. Antibodies obtained from mice infected i.n. with ∆iglC F. novicida conferred 80% survival when transferred i.p. into B cell-deficient mice 8 h before i.n. challenge with wild-type F. novicida. The first demonstration of therapeutic protection by antibodies against pulmonary tularemia was performed by Kirimanjeswara et al. Serum obtained from mice intranasally (i.n.) infected with a sub-lethal dose of LVS provided 100% protection and reduced tissue burdens and organ damage following a lethal i.n. LVS challenge when serum was transferred i.p. One day prior to infection. FCγR, IFN-γ, neutrophils, and macrophages, but not complement, were required for protection. Transfer of serum could also confer survival against lethal i.n. LVS infection when administered i.p. as late as 48 h post-infection. The most potent serum to treat virulent F. tularensis infection in mice was obtained from mice that were i.n. infected with F. tularensis SchuS4 and then treated with the antibiotic levofloxacin daily for 13 d beginning on day 3 post-infection. Serum from these antibiotic-treated mice was able to confer up to 100% survival when transferred i.p. 4 h before or 24 h after i.n. infection with SchuS4. Transfer of immune serum can also be effective against pulmonary tularemia due to virulent F. tularensis infection in rats. Antibodies from rats vaccinated s.c. with LVS provided protection against morbidity and provided 100% survival against intratracheal (i.t.) challenge with SchuS4 when transferred i.p. to rats 1 d before challenge. This effect was shown to be dependent on IgG, and CD8+ T cells but not by IgM. Transfer of immune serum also reduced bacterial organ burdens and inflammation.

Immunotherapy Using Serum from Animals Immunized with Inactivated Francisella or Francisella Antigens

While the majority of humoral immunotherapy studies for tularemia have utilized serum from animals infected with live Francisella, serum from animals immunized with inactivated Francisella or Francisella antigens has also proven protective. Studies by Fulop et al. showed that i.p. transfer of sera from mice immunized with LVS LPS 2 h prior to i.p. LVS challenge conferred 100% survival in mice, an effect that was independent of CD4+ or CD8+ T cells. Anti-LPS antibodies did not confer survival against i.p. challenge with virulent SchuS4, although a slight increase in time to death was observed. Lavine et al. demonstrated that serum from mice immunized with heat-killed LVS could confer 100% survival when given i.p. 8 h before a lethal i.p. LVS infection. Antibodies against LVS LPS were not required for this protection. F. tularensis outer membrane protein A (FopA) was proven to be a target of protective antibodies by Hickey et al. Serum from mice immunized with FopA could confer 100% protection against a lethal i.d. LVS infection when given i.p. before and after challenge. As mentioned earlier, serum therapy of F. tularensis has shown limited efficacy against virulent type A F. tularensis challenge in mice. Therefore, Sutherland et al. developed a model in which mice were treated i.p. with a suboptimal dose of gentamicin beginning 1 d after i.n. infection with virulent F. tularensis SchuS4 in order to extend the time to death from ~4 to ~7 d postinfection. They found that i.p. transfer of murine antibodies elicited against a Francisella membrane protein fraction (MPF) 1 d after i.n. SchuS4 challenge could reduce organ burdens and provide 100% survival when used in conjunction with suboptimal gentamicin in this model. Treatment of mice i.p. with MPF 1 d after SchuS4 challenge also conferred 100% protection when used in combination with suboptimal gentamicin.

Monoclonal Antibody Immunotherapy for Tularemia

The investigation of immunotherapy using monoclonal antibodies (MAbs) for the treatment of experimental tularemia has been limited; however, protective efficacy has been demonstrated. Using a proteome microarray Lu et al. identified several monoclonal antibodies (MAbs) from LVS-infected mice. The authors found that an IgG2a mAb reactive with LVS LPS conferred 100% survival when given i.p. or i.n. within an hour after a lethal LVS i.n. challenge. The relative protective efficacy of anti-LPS IgG antibodies in this study was determined to be IgG2a > IgG1 > IgG3. mAb studies performed by Savitt et al. showed that MAbs against LVS components could confer 100% survival and reduce organ burdens when given prior to, and after lethal i.d. challenge with LVS. When given before and after a lethal i.d. LVS challenge, anti-LVS FopA MAbs conferred partial survival from infection. Therapeutic treatment of mice with MAbs against LVS LPS, FopA and LpnA 1, 3, and 5 d after a lethal i.d. LVS infection also provided partial protection against mortality. The efficacy of mAb therapy was greatly diminished when a virulent challenge strain was used in this study; however, anti-LPS MAbs given before and after infection did modestly extend the time to death of mice challenged i.d. with type A F. tularensis SchuS4.

Perspectives and Challenges for the Study of Tularemia Immunotherapy

Immunotherapy of tularemia has received increased attention in recent years, and numerous immunotherapeutics have demonstrated protection in animal models of tularemia. However, many, if not most of these studies have utilized challenge strains that do not cause disease in humans. Virulent strains of F. tularensis possess mechanisms of immune suppression not found in attenuated strains that may interfere with immunotherapy. Also, many immunotherapy strategies reviewed here have shown impressive protective effects against F. novicida or LVS infections, but these same approaches have generally failed to provide meaningful protection against virulent strains of Francisella. These findings question the utility of F. novicida and LVS infections as models to develop immunotherapeutics against virulent F. tularensis infections. Therefore, care must be taken when translating the potential of immunotherapeutics that confer protection against attenuated strains of Francisella in animal models to their potential efficacy against Francisella strains that are pathogenic for humans. Also, it has been proposed that systemic, rather than pulmonary infection is the likely cause of death in mice following challenge with virulent F. tularensis, regardless of the route of infection., In addition, human tularemia due to inhalation of virulent Francisella often presents with systemic symptoms of illness without prominent pulmonary signs of disease. Therefore, while immunotherapies that target the lung have proven effective against experimental pulmonary tularemia, it is likely that immunotherapeutics will also need to reduce or block systemic colonization by Francisella in order to provide meaningful protection against tularemia.

The focus of antibody-mediated immunity against Francisella has been primarily related to the generation of prophylactic vaccines. However, the transfer of immune serum to human tularemia patients was purported to be protective in the 1940s, indicating a potential for humoral immunotherapy of tularemia. In animal models, numerous studies have shown that the transfer of immune serum prior to or shortly after infection could increase resistance to challenge. To enhance the potential clinical relevance of post-exposure treatment, future studies will need to investigate humoral immunotherapy at later timepoints post-infection. Also, due to the (as yet) limited ability of transferred immune serum to protect against mortality induced by virulent strains of F. tularensis in mice, it might be beneficial to perform these studies in conjunction with antibiotic therapy or in a more resistant host such as the rat.

The induction of protection against tularemia with innate immune agonists is exciting, particularly as several of these agonists, including Acai PS, CLDC, CLDC + MPF, CPG, MPL, Poly I:C, and yeast glucans have shown protection in animal models against bacterial and viral pathogens other than Francisella.,,,, Stimulation of innate immunity with these agonists may be particularly useful in an event where the etiologic agent of disease is unknown, such as a bioterror attack, as the immune responses induced by these agonists have the capability to protect against multiple pathogens. However, several mitigating factors must be considered when examining the potential of innate immune agonists. While treatment of mice with several TLR agonists prior to or at the time of infection has proven protective against tularemia in animal models, infection of mice with F. tularensis SchuS4 has been shown to suppress subsequent TLR-induced immune responses., Therefore, the targeting of TLRs for immunotherapy may have a limited window of efficacy against tularemia. Another factor that may limit the efficacy window for innate immune agonists is the hypothesis that a late upregulation of proinflammatory cytokines during pulmonary tularemia may be too late to decrease bacterial colonization, and may actually be harmful to the host. Therefore, enhancement of immunity may actually be detrimental to the host when agonists are given at later points after infection. To address this concern, immune agonists should be tested at later times post-infection and in conjunction with antibiotic therapy to determine their protective window of efficacy, and also to ensure that they do not exacerbate disease when endogenous host responses are also activated.

In conclusion, immunotherapy for tularemia has shown strong promise in animal models and will presumably continue to be a focus for future studies, particularly due to the potential threat of weaponized antibiotic-resistant Francisella. The elucidation of protective mechanisms of immunity elicited by tularemia immunotherapeutics may also reveal novel correlates of protection that will increase our understanding of immunity to Francisella and intracellular pathogens as a whole.