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Antimicrobial Agents and Chemotherapy, July 2005, p. 2921-2927, Vol. 49, No. 7
0066-4804/05/$08.00+0     doi:10.1128/AAC.49.7.2921-2927.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

Antimicrobial Peptide Therapeutics for Cystic Fibrosis

Helix Biomedix Inc., 22122 20th Avenue SE, Bothell, Washington 98021,¹ Department of Microbiology and Infectious Diseases, University of Calgary Health Sciences Centre, Calgary, Alberta, Canada,² Department of Microbiology and Immunology, University of British Columbia, 2259 Lower Mall Research Station, Vancouver, Canada³

Received 30 November 2004/ Returned for modification 25 February 2005/ Accepted 11 April 2005

	ABSTRACT

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Greater than 90% of lung infections in cystic fibrosis (CF) patients are caused by Pseudomonas aeruginosa, and the majority of these patients subsequently die from lung damage. Current therapies are either targeted at reducing obstruction, reducing inflammation, or reducing infection. To identify potential therapeutic agents for the CF lung, 150 antimicrobial peptides consisting of three distinct structural classes were screened against mucoid and multidrug-resistant clinical isolates of P. aeruginosa, Stenotrophomonas maltophilia, Achromobacter xylosoxidans, and Staphylococcus aureus. Five peptides that retained potent antimicrobial activities in physiological salt and divalent cation environment were further characterized in vivo using a rat chronic lung infection model. All animals were inoculated intratracheally with 10⁴ P. aeruginosa mucoid PAO1 cells in agar beads. Three days following inoculation treatment was initiated. Animals were treated daily for 3 days with 100 µl of peptide solution (1 mg/ml) in 10 mM sodium citrate, which was deposited via either intratracheal instillation or aerosolization. Control animals received daily exposure to vehicle alone. At the end of the treatment the lungs of the animals were removed for quantitative culture. Four peptides, HBCM2, HBCM3, HBCP-2, and HB71, demonstrated significant reduction in Pseudomonas bioburden in the lung of rats. Further in vivo studies provided direct evidence that anti-inflammatory activity was associated with three of these peptides. Therefore, small bioactive peptides have the potential to attack two of the components responsible for the progression of lung damage in the CF disease: infection and inflammation.

	INTRODUCTION

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Cystic fibrosis (CF) is an autosomal-recessive genetic disease due to a defect in the CF transmembrane conductance regulator (CFTR) gene of chromosome 7 encoding the CFTR chloride channel protein (30). It is the most common life-shortening genetic disease among caucasians and affects approximately 60,000 people worldwide. The major morbidity and mortality in CF are caused by the progressive loss of pulmonary function that results from a cycle of inflammation and infection. Patients with cystic fibrosis typically harbor multiple morphologically distinct microorganisms. By 18 years of age, 80% of patients become chronically infected with Pseudomonas aeruginosa (1, 25). P. aeruginosa is a difficult organism to treat in most human infections due to its high intrinsic antibiotic resistance, due primarily to low outer membrane permeability bolstered by effective multidrug efflux and an inducible class C ß-lactamase. In the setting of the CF lung this issue appears to be exacerbated, and further development of cross-resistance to ciprofloxacin and ofloxacin is regularly seen while resistance to aminoglycosides is also a problem in CF patients with chronic P. aeruginosa infections (12, 22). Other well-characterized CF pathogens include Staphylococcus aureus and nontypeable Haemophilus influenzae, which are of significance primarily during the first decade of life (26). In the past two decades, intrinsically antibiotic-resistant, gram-negative organisms such as Burkholderia cepacia, Stenotrophomonas maltophilia, and Achromobacter xylosoxidans are newly emerging microorganisms isolated with increased frequencies from CF lungs (9, 23, 26). The inadequacy and deficiency of effective antibiotics for CF has led medical professionals to reconsider the value of conventional antibiotics, even when they do not have strong anti-pseudomonal activity. For example, the macrolide antibiotic azithromycin has been evaluated in patients with chronic Pseudomonas lung infection (14). However, this approach has also failed to demonstrate success and furthermore put patients under selective pressure promoting the carriage of macrolide-resistant bacteria. Chronic inflammation complicates therapy in the CF airways leading, for example, to high concentrations of DNA and neutrophil elastase (10). As a consequence of inflammation, the immune response in the CF lungs appears to be dysfunctional. Therefore, there is a vital need to develop new effective anti-pseudomonal as well as anti-inflammatory therapeutics.

Antimicrobial cationic peptides are ubiquitous in nature. They are a key component of the innate immune system acting as the first line of defense against infectious agents. The properties of these peptides make them extremely attractive candidates for development as therapeutics for CF. Not only are they fast acting, bactericidal, and active against multidrug-resistant bacteria, but certain peptides exhibit anti-inflammatory, immunomodulatory, and wound healing activities in addition to antimicrobial activity (11, 13, 18, 21, 34). Although lung epithelial cells secrete cationic antimicrobial peptides and proteins, most endogenous peptides such as ß-defensins and LL-37 are in very low concentrations in the lung and are salt sensitive in vitro and thus are presumably ineffective in the high-salt environment created on the apical side of CF epithelial cells (3, 15). A promising therapeutic approach would be to exogenously apply antimicrobial cationic peptides with combined antimicrobial and anti-inflammatory activity to the lung against P. aeruginosa infections and inflammation via aerosol formulation (18). The rationale for use of such peptides in CF therapy is further supported by work demonstrating that the overexpression of LL-37 by viral gene transfer results in the augmentation of innate host defenses against P. aeruginosa in a bronchial xenograft model of cystic fibrosis (4).

In this study, we took the approach of screening for peptides with activity against CF pathogens in the presence of factors that mimic the physiological environment of the CF lung. Peptides with good anti-inflammatory as well as antimicrobial activity were then tested in animal models for in vivo efficacy. Our data suggest that the lead peptides significantly reduced the numbers of viable bacteria in the infected lungs of rats as well as demonstrating good anti-inflammatory activity in mice.

	MATERIALS AND METHODS

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Peptide synthesis. All peptides were synthesized using standard Fmoc chemistry on an Advanced ChemTech (Louisville, KY) Apex 396 Multiple Peptide Synthesizer. Primary sequence confirmation and preparative purification to >95% purity was accomplished using a liquid chromatography-tandem mass spectrometry system (ABI API2000).

Bacterial strains and culture conditions. Bacterial strains included in this study are listed in Table 1. P. aeruginosa, S. aureus, and Candida species were grown in Mueller Hinton (MH; Difco, BD Biosciences, MD) agar plates and broth at 37°C unless otherwise indicated. Bacteria from frozen stock were subcultured onto freshly made MH agar plates prior to susceptibility testing. P. aeruginosa clinical isolates, multidrug-resistant isolates, and methicillin-resistant S. aureus (MRSA) were all from laboratory stocks at the University of British Columbia, Vancouver, Canada. Tobramycin, rifampin, chloramphenicol, calf thymus DNA, and mucin were purchased from Sigma Chemical Company (St. Louis, MO).

To test peptide activity in the presence of DNA or mucin, approximately 2 x 10⁵ CFU/ml of bacteria was added to 1.2% hog gastric mucin or 0.8 mg/ml of calf thymus DNA in saline and dispensed (80 µl) into each well of a 96-well plate, containing 10 µl of 2-fold serial diluted peptides. After incubation at 37°C for 2 h, the cell viability was determined by spotting 10 µl of the reaction mix onto fresh MH agar plates and subsequent incubation at 37°C overnight. The MIC was taken as the lowest concentration at which no colonies were observed.

Activity of peptides in sputum. Individual sputum samples from CF patients were pooled and diluted 10-fold with 10 mM phosphate buffer (pH 7.0). The suspensions were thoroughly mixed and then centrifuged at 1,000 rpm for 10 min (Mini Centrifuge C1200; National Labnet Co., Woodbridge, NJ). Supernatants were saved and used in killing and stability tests. For killing assays, about 5 x 10⁷ CFU/ml of P. aeruginosa were added to a 10% diluted sputum supernatant, and peptide was added to a final concentration of 100 µg/ml. The mixture was incubated at 37°C for 1 h and then diluted and plated on freshly made MH agar plates.

For stability tests, individual peptides were added to the 10% diluted sputum supernatant to a final concentration of 100 µg/ml, and the mixture was incubated at 37°C for various time intervals, after which the reaction was stopped by the addition of 10 µl of 10% HCl. Residual peptide concentrations were determined with a reversed-phase high-performance liquid chromatography system.

Rat CF lung model. The chronic rat lung model of agar bead coated P. aeruginosa infection was used to assess the effects of peptides on the bioburden in the lungs (16). Rats (5 animals in each group) were inoculated intratracheally with approximately 10⁴ CFU of P. aeruginosa strain PAO1 in agar beads. Treatment was conducted by either intratracheal instillation or nebulization. For intratracheal instillation of peptides, treatment was initiated 3 days after inoculation and deposited intratracheally. Peptides (100 µg in 100 µl sodium citrate buffer) were administered intratracheally to anesthetized animals using a laryngoscope introduced into the oral cavity while the incisors were suspended over a holding bar of an instrument that permitted observation of the entrance to the trachea. A 22-gauge gavage needle was then introduced into the oral cavity between the visible vocal folds, allowing the solution to be introduced into the left lung. Control animals (group 1) received daily exposure to saline, and treatment groups received daily exposure to one of five different formulations of peptides (groups 2 to 6). Animals were sacrificed on day 3, and the lungs of animals removed for quantitative culture.

For nebulization studies, rats were exposed to aerosol preparations using an Aero-tech II nebulizer (CIS-US, Bedford, MA) operated at 45 lb/in², with a flow rate of 10 liters/min and containing 10 ml of the preparation to be aerosolized. The 10-ml volume was dispensed in 25 to 30 min, during which rats were inhaling the drug aerosol. Animals (5 in each group) were treated once daily for 3 days; control animals received daily exposure to 10 ml of 10 mM sodium citrate (pH 7.0); one treatment group received daily exposure to 10 ml of 10 mM sodium citrate (pH 7.0) containing 5 mg/ml of HBCM3; one treatment group received daily exposure to 10 ml of 10 mM sodium citrate (pH 7.0) containing 5 mg/ml of HBCP2. Animals were sacrificed on day 3, and the lungs removed for quantitative culture. The amount of compound delivered to the lung in this model was estimated to be approximately 10 to 15 µg per treatment based on analogous studies with similar doses of the polycationic aminoglycoside antibiotic amikacin (D. E. Woods, unpublished data).

In vivo anti-inflammation assay using an ear edema model in mice. Inflammation assays were perform in mice by CEREP (Paris, France) using the technology described by Chang et al. (8). Twenty-five CD-1 male mice weighing 21 to 25 g were used. Thirty minutes after topical application of the test peptide (20 µg/ear), an irritant, phorbyl myristoyl acetate (PMA; 5 µg in 20 µl of ethanol) was topically applied to the inner and outer surface of the right ear. Thirty minutes later a second dose of the test peptide was topically applied on the ear. Ear weight was measured 6 h after PMA application. The mean ear weight, expressed in milligrams, was calculated as the difference between the right and left ear weight. Bethamethasone was used as a positive control at 0.3 mg/ear.

Resistance. The MIC of peptides for P. aeruginosa was assessed as described above. The cells treated with the concentration of peptide equivalent to one half the MIC were diluted in saline and used as an inoculum in the next round of MIC assessment. These procedures were repeated 30 times. Chloramphenicol and rifampin were used as antibiotic controls. Cross-resistance was tested after 30 passages for a panel of peptides.

	RESULTS

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Antimicrobial activity of peptides. A total of 155 peptides were tested for their antimicrobial activity against bacteria and yeast. Table 2 shows some representative peptides with distinctive activities. A group of peptides represented by HBCM2, HBCM3, HBCP2, (formerly termed CM2, CM3 and CP2, respectively [28]), HB12, HB71, and HB46 exhibited selective activity against gram-negative bacteria, although HB71 and HB46 also showed moderate antifungal activity against Candida albicans (Table 2). Certain peptides were more antibacterial than antifungal, e.g., HB25, HB300, and HB301. In contrast, both HB77 and HB401 were yeast selective and ineffective against bacteria (Table 2). Most peptides, represented by HB35, HB43, HB55, HB146, HB153, and HBPM4, formerly termed PV-7 (34), displayed a broad spectrum activity with MICs ranging from 1 to 16 µg/ml against both bacteria and yeast (Table 2).

Table 2 also shows the results for the same peptides against clinical isolates of CF pathogens. The mean MIC of peptides against two mucoid clinical isolates of P. aeruginosa ranged from 2 to 32 µg/ml, which was comparable to the MIC of the same peptides against their nonmucoid isogenic counterparts. The two efflux pump overexpressing mutants, that were resistant to 5,000 µg/ml nalidixic acid, retained susceptibility to antimicrobial peptides with MICs of 2 to 8 µg/ml. Similarly, strains resistant to 16 to 32 µg/ml of tobramycin generally also showed similar susceptibility to antimicrobial peptides with MICs ranging from 8 to 16 µg/ml. Among the multidrug-resistant clinical isolates of P. aeruginosa that were resistant to ß-lactams aminoglycosides and imipenem, represented by M76, M917, M1251, M1426, and R70, all peptides were highly effective, although elevated MICs were observed for M917.

All tested peptides were highly active against other Pseudomonas species isolated from sputum, including P. stutzeri, P. fluorescens, and P. pickettii, with MICs of 2 to 16 µg/ml. They also were demonstrated potent activity against S. maltophilia. Some peptides, including HBCM2, HB71, HB35, HB146, and HB301, were more active than others against Achromobacter xylosoxidans, which possesses intrinsic resistance to macrolide antibiotics as well as resistance to 128 µg/ml tobramycin.

Activity of peptides in the presence of salt, DNA, and mucin. It has been speculated that the NaCl concentration may be elevated in CF airway surface liquid, resulting in ineffective defense of some endogenous antimicrobial peptides such as defensins and LL37 against bacteria (4, 16), although it is still disputed as to whether the ionic composition of the airway surface fluid is different between CF and healthy individuals (33, 35). It has been reported that the epithelial environment of CF lung has an NaCl concentration of 120 to 150 mM (33, 35) and a divalent cation concentration around 1 to 2 mM (2, 17). Another important factor in the CF lung is dead neutrophils present at concentrations around 1,000-fold higher than those observed for healthy individuals (10). Indeed, it has been proposed that the release of long, viscous DNA strands and glycoproteins from such dead cells are a principal cause of airway clogging and damage. Such polyanionic polymers which are found in CF sputum would also be anticipated to antagonize the activity of polycationic antibiotics due to electrostatic binding.

We therefore tested the effects of salts, DNA, and mucin on the activity of several peptides. Most peptides retained activity in salt, divalent cations, and DNA, with moderate two- to fourfold increases in MIC. In contrast, none of the peptides tested here were effective in the presence of 1% gastric mucin (Table 3). Tobramycin, however, was less antagonized by DNA or mucin than physiological salt concentrations (Table 3).

In vivo efficacy of antimicrobial peptides in a chronically infected rat lung model. Intratracheal instillation of peptide allows for the use of significantly lower concentrations of antibiotic and is thus particularly useful in preliminary efficacy studies prior to aerosolization studies (24). Using such a delivery procedure, quantitative bacterial counts indicated that animals that received treatments of 100 µg of either HBCM2 or HB71 once daily for 3 days demonstrated, respectively, 74% (P < 0.05) and 91% (P < 0.01) reductions in total P. aeruginosa counts from 4.9 x 10⁴ to 1.3 x 10⁴ and 4.5 x 10³, respectively, compared to the control group that received saline only during the same period of time (Fig. 1A). This compares favorably with the results of Omri et al. (24) who, using the same model, delivered, by intratracheal installation, a 500-µg dose of polymyxin B to the lungs of rats, leading to a therapeutic (87%) reduction in P. aeruginosa bioburden. In contrast, rats receiving HB50 and HBPM4 showed no significant reduction in cell counts in the lung (Fig. 2A).

View larger version (23K): [in this window] [in a new window]   FIG. 1. In vivo efficacy assessment in rat chronic lung infection model. A. P. aeruginosa bioburden in the lungs of rats after three consecutive daily treatments via intratracheal instillation of peptide. Shown is the percentage of the number of CFU per milliliter of bronchoalveolar lavage recovered from the lungs treated daily with 100 µg of the named peptide relative to that for control animals treated with saline alone. B. P. aeruginosa bioburden in the lungs of rats after three consecutive daily treatments via nebulization of peptide.

View larger version (27K): [in this window] [in a new window]   FIG. 2. Effect of topical application of peptides in chronic phobol-ester-induced ear edema in mice. Anti-inflammatory activity is shown as reduction in milligram of ear edema weight in mice treated with peptides in comparison to a vehicle group. Bethamethasone (Beta), as a positive control, was applied at 0.3 mg/ear; peptides were applied at 20 µg/ear.

Anti-inflammatory activity in an ear edema mouse model. A major factor in CF lung disease is inflammation which appears to be responsible for a considerable amount of lung damage. It was previously demonstrated that a variety of peptides, including HBCM2, HBCM3, HBCP2, and HBPM4 (28, 34), demonstrated activity in neutralizing endotoxin, which causes a clinical syndrome analogous to extreme inflammation. Therefore, we examined here if peptides have anti-inflammatory activity. Three peptides were selected for the mouse ear edema model. HBCM2 was chosen because previous work suggested that cecropin:melittin hybrid peptides have anti-endotoxic activity and can modulate innate immune responses (6, 28). HB146 was an alternative antimicrobial -helical peptide, while HB107 was a nonantimicrobial -helical peptide. As shown in Fig. 2, HBCM2 at 2 µg per ear significantly reduced phorbol-ester-induced edema. To a lesser extent, HB107 and HB147 appeared to marginally reduce inflammation.

Resistance induction in vitro. P. aeruginosa was serially transferred daily in the presence of sub-MIC concentrations of HB50, HB153, HBPM4, and HB71. After 30 passages (Table 4), mean MICs were increased to a panel of 8 peptides by no more than fourfold. However, such resistance appeared to be transient, since a single passage of each resistant strain in the absence of peptide lead to reversion to near susceptible levels with less than twofold alterations in MIC compared to the original parent strain (data not shown). In contrast, serial transfers on chloramphenicol or rifampin had little effect on susceptibility to peptides while increasing resistance to the utilized drug by 8- to 16-fold.

	DISCUSSION

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Our animal model studies on selected peptides revealed the greater effectiveness, in accelerating bacterial clearance from the airways during chronic P. aeruginosa lung infection in rats, of certain gram-negative selective peptides, including HBCM2, HB71 (by intratracheal therapy), HBCM3, and HBCP2 (by nebulization therapy), when compared to a broad-spectrum peptides such as HBPM4 (Fig. 2), despite similar MICs for P. aeruginosa. The extent of decrease in colony counts for the successful peptides compares favorably to the levels of protection afforded by the nonliposomally encapsulated polycationic antibiotics polymyxin B (24) and aminoglycosides (5 and D. E. Woods, unpublished data). The animal model employed is one of the most utilized animal models developed to study the pathogenesis of chronic P. aeruginosa infections and has been used to test the efficacy of a number of anti-pseudomonal antibiotics prior to clinical trials (5, 7, 24, 32). It involves the incorporation of P. aeruginosa into agar beads followed by intratracheal deposition into the lungs of rats to ensure a chronic infection, and animals have been studied up to 1 year following inoculation and remain chronically infected (32). For cationic peptides it represents a particularly stringent model as the anionic polysaccharide that makes up agar would be anticipated to antagonize the activity of the peptides. Indeed, it is well known that most peptides have no activity on solid medium-based MIC assays unless agarose is substituted for agar. The successful reduction of bioburden observed in this model indicates that either the biological half-life of peptides at the lung surface is sufficient to accelerate bacterial clearance despite the prospective susceptibility of peptides in general to degradation by high levels of active neutrophil elastase and other proteases present in the rat lungs, or that the peptides work in some other way, such as via immune enhancement (6). Indeed, with respect to the alternative mechanisms, other animal model data demonstrated that the peptides had anti-inflammatory activities. Thus, given that CF is complicated by a destructive inflammatory response that is associated with chronic infection by P. aeruginosa, the anti-inflammatory activity represents a major asset of such peptides.

The main method of combating lung infections in CF patients is antibiotic treatment (19). With the increasing life expectancy of such patients due to improved care, more courses of antibiotics are used for longer terms and at higher doses, with the adverse consequence of increasing antimicrobial resistance. The observation of lack of potential resistance and/or cross-resistance makes antimicrobial peptides extremely interesting candidates for use in CF therapy. After 30 passages in the presence of sub-MIC concentrations, changes in mean MICs of selected peptides against P. aeruginosa were only two- to fourfold greater than the initial MICs for most peptides. Also, no cross-resistance was observed to different peptides. This was inconsistent with the finding that resistance to the cationic lipopeptide colistin (a mixture of peptides polymyxins E1 and E2) is seldom seen, despite daily selective pressure in patients receiving colistin by inhalation (20, 31).

Our own data with P113D, a D-isomer of histatin 5, disagreed with an earlier study (27) that had suggested that while it did not possess activity in broth against P. aeruginosa, it was highly effective in sputum against this bacterium. In our hands, P113D, like HB71 and HB71D, when added at final concentration of 1 mg/ml to a pooled of undiluted sputum containing 10⁷ CFU/ml of P. aeruginosa, was unable to effectively reduce bacterial counts. Reducing the sputum concentration to 10% and the peptide concentration to 100 µg/ml led to modest killing by HB71 and HB71D, but again P113D was completely ineffective. Our results were perhaps not surprising, since sputum contains as much as 12% mucin, and we observed that most peptides were ineffective in vitro in 1% of gastric mucin (Table 3). However, the lack of in vitro activity of peptides in sputum raises an interesting question as to whether this assay is clinically relevant, since we were able to demonstrate here that four such peptides were efficacious in vivo.

	ACKNOWLEDGMENTS

 
R.E.W.H. and D.E.W. were financially supported by the SPARx program of the Canadian Cystic Fibrosis Foundation and the Canadian Bacterial Diseases Network, and each are the recipients of a Canada Research Chair.

	FOOTNOTES

 
* Corresponding author. Mailing address: 22122 20th Ave. SE, Bothell, WA 98021. Phone: (425) 402-8400. Fax: (425) 806-2999. E-mail: lzhang{at}helixbiomedix.com.

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