Identification and Characterization of Novel Antimicrobial Decapeptides Generated by Combinatorial Chemistry

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Antimicrobial Agents and Chemotherapy, October 1998, p. 2534-2541, Vol. 42, No. 10
0066-4804/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Identification and Characterization of Novel Antimicrobial Decapeptides Generated by Combinatorial Chemistry

Sung Yu Hong,¹ Jong Eun Oh,¹ Mi yun Kwon,¹ Myeong Jun Choi,¹ Ji Hye Lee,² Bok Luel Lee,² Hong Mo Moon,¹ and Keun Hyeung Lee¹^,^*

Protein Chemistry Laboratory, Mogam Biotechnology Research Institute, Kyunggi-Do, 449-910,¹ and College of Pharmacy, Pusan National University, Pusan 609-735,² Korea

Received 28 January 1998/Returned for modification 8 June 1998/Accepted 15 July 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Novel combinatorial libraries consisting of simplified amino acid sequences were designed to screen for peptides active againstthe Candida albicans membrane. A novel decapeptide, KKVVFKVKFK,that had a unique primary amino acid sequence was identified inthis work. This peptide irreversibly inhibited the growth of C.albicans and showed a broad range of antibacterial activity butno hemolytic activity. Circular dichroism spectra revealed thatthe predominant secondary structure of this peptide strongly dependedon the membrane-mimetic environments; the peptide preferred toform an amphipathic $alpha$ -helical structure in the presence of 50%trifluoroethanol, while it preferred to adopt a distorted $alpha$ -helicalstructure in the presence of sodium dodecyl sulfate micelles.Experiments in which dye was released from vesicles indicatedthat this novel antimicrobial peptide killed microorganisms throughthe action on the membrane as its primary target. Replacementof amino acids in this active decapeptide on the basis of informationfrom the libraries could provide unique information about factorsaffecting its antimicrobial activity such as its secondary structure,net positive charge, and hydrophobicity.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The incidence of fungal infections has increased dramatically in the past 20 years because of the increase in the number ofpeople whose immune systems are compromised by AIDS, aging, organtransplantation, or cancer therapy (3, 11). Accordingly,the increases in the rates of morbidity and mortality becauseof fungal infections have been regarded as a major problem (46).Most of the current antifungal drugs simply reduce the level ofgrowth of fungi. Amphotericin B, called the drug of last choicefor the treatment of most systemic mycoses, is a potent fungicidalagent, but it is very toxic to the kidney and the hematopoieticand central nervous systems (2, 30). The development of resistantfungal strains in response to the widespread use of current antifungaldrugs will cause serious problems in the future (23). The recentemergence of fungal infections and resistant strains has stimulatedthe development of novel antifungal drugs (6, 24, 45).

In the past few years, membrane-active host defense molecules have been isolated from a variety of natural sources (4,7, 12, 33). Interestingly, they are small peptides or proteins,some of which have been shown to have antibacterial and antifungalactivities (4, 39, 47). Although native defense peptidesthemselves could not be used as therapeutic agents because oftheir low levels of activity and poor bioavailabilities, thesepeptides have received attention because of their low levels oftoxicity against mammalian cells and the ideal mechanism of perturbingthe membrane of the pathogen.

The development of novel antifungal agents from the peptides requires the design and synthesis of large numbers of individualpeptides for activity optimization. This process is too time-consumingand limited by the difficulty of designing peptides with the desiredstructure in the lipid membrane, by nonlinear relationships betweenactivity and structure (5, 13, 34), and by the lack ofthe detailed structural information concerning the synthesizedpeptide in the lipid membrane.

As an alternative method to overcoming these limitations, full peptide libraries have been developed (9, 10, 28, 38).However, the antimicrobial peptides identified by these librarieswere less active than the currently available antimicrobial agents.Moreover, these peptides might be too short to act on the membraneof the target pathogen.

Since the decapeptide was reported to be the peptide with the minimal length necessary for the interactions of amphipathic $alpha$ -helical peptides with phosphatidycholine liposomes (36) andsince the decapeptide derived from tenecin 1, an antimicrobialpeptide from Tenebrio molitor, killed pathogens by changing thepermeability of the lipid membrane of pathogens (32), combinatoriallibraries composed of decapeptide mixtures were required to screenfor peptides active against the membranes of pathogens. We expectedthat combinatorial libraries made up of a few amino acids insteadof 20 natural amino acids must provide enough of a peptide mixtureto screen for the activity-optimized peptide because the membraneof the pathogen must have less specificity than other biologicaltargets such as enzymes, antibodies, and hormone receptors. Accordingly,we developed combinatorial libraries with decapeptide mixturescomposed of seven amino acids (Lys, Leu, Val, Phe, Ser, Gln, andPro) to screen for the peptide active against Candida albicans.We identified a novel decapeptide which had activity against bacteriaas well as fungi but no hemolytic activity.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Synthesis of peptide libraries and individual peptides. Peptide libraries and individual peptides were synthesized on Rink amide methylbenzhydrylamine (MBHA) resin (PerSeptive BiosystemGmbH, Hamburg, Germany) by 9-fluorenylmethoxycarbonyl (Fmoc) chemistry(20, 21, 31). The amino acids used in the synthesis of peptidelibrary were Leu, Lys, Phe, Pro, Ser, Gln, and Val (Calbiochem-NovabiochemCorp., La Jolla, Calif.). Side chain protection groups were asfollows: for Lys, tert-butoxylcarbonyl; for Ser, tert-butyl; andfor Gln, trityl. In this library, lysine was fixed at the C terminus,and the other nine positions consisted of seven amino acids atequimolar concentrations. A combination step including a division,coupling, and recombination process (28) was used to synthesizethe peptide mixture. This process ensured the equimolarity ofthe peptides on the resin in the packets. Briefly, seven porouspolypropylene packets, each containing 0.1 mmol of lysine-MBHAresin, were coupled to each protected Fmoc amino acid. All couplingreactions proceeded to completion (>99.5%), as assessed by theninhydrin test of Kaiser et al. (29). The resulting resins fromeach packet were then combined and were thoroughly mixed. Thisresin mixture was separated into seven portions of equal weights,and these were placed into porous polypropylene packets, followedby removal of the Fmoc group. The resin in the packet was thenreacted with solutions of the individual activated amino acid.The division, coupling, and recombination process described abovewas repeated eight more times, yielding a final mixture of 40,353,607(7⁹) protected peptide resins. Cleavage of the peptide from the resinwas achieved by treatment with a mixture of trifluoroacetic acid(TFA)-thioaninsole-ethane-dithiol-H₂O at a ratio of 80:5:2.5:5(vol/vol) at room temperature for 12 h. After filtration of theresin and washing with TFA, a gentle stream of nitrogen was usedto remove the excess TFA. The crude peptide was triturated withdiethyl ether chilled at $-$ 20°C and was then centrifuged at 3,000× g for 10 min. An individual peptide was synthesized by the solid-phasemethod on a 431A automatic peptide synthesizer (Applied Biosystems,Foster City, Calif.). The peptide was purified by high-performanceliquid chromatography with a Waters Delta Pak C₁₈ column (25 by100 mm; Waters, Milford, Mass.). Amino acid analysis, high-performanceliquid chromatography (27), and electrospray mass spectrometryon a Platform II spectrometer (Fishons Instruments, Manchester,United Kingdom) were used to characterize the purified peptide.

Antifungal and antibacterial assays. In vitro antifungal assays were performed by the broth microdilution method by following the recommendation of the NationalCommittee for Clinical Laboratory Standards (41). Sabouraud-2%dextrose broth (pH 5.6 at 25°C; Merck, Darmstadt, Germany) wasused as the assay medium. C. albicans ATCC 36232 freshly grownon slopes of Sabouraud dextrose agar were suspended in physiologicalsaline, and the cell concentration was adjusted to 10⁴ cells per 1 ml of 2× concentrated medium for use as the inoculum.Peptide solution was added to the wells of a 96-well plate (100µl per well), and the wells were serially diluted twofold. Thefinal concentrations of the peptide mixture ranged from 0.2 to500 µg/ml. After inoculation (100 µl per well, 5 × 10³ cells per ml), the 96-well plate was incubated at 30°C for 48h, and the absorbance was measured at 620 nm by using an enzyme-linkedimmunosorbent assay reader (SLT, Salzburg, Austria) to assesscell growth. The MIC was defined as the lowest concentration ofthe peptide that completely inhibited the growth of the test organism.To measure the minimal fungicidal concentration (MFC), 100 µlof the cell suspension was taken from each well and was washedthree times with fresh Sabouraud broth. Then, each cell suspensionwas plated onto a Sabouraud dextrose agar plate and the platewas incubated at 30°C for 48 h. The MFC was determined by countingthe numbers of colonies on the Sabouraud dextrose agar plate.An in vitro antibacterial assay was performed by the aforementionedmethod used for the antifungal assay, with the exception thatthe assay medium and the incubation temperature were different.In the antibacterial assay, antibiotic medium 3 (pH 7.0 at 25°C;Difco, Detroit, Mich.) was used, and the cells were incubatedat 37°C for 24 h.

Hemolytic assay. The hemolytic assay method used in this study has been described elsewhere (15). Packed mouse erythrocytes were washed threetimes with buffer (150 mM KCl, 5 mM Tris-HCl [pH 7.4]), and thenpacked erythrocytes were suspended in 10 volumes of the same buffer(stock cell suspension). For antibiotic treatment, the cell stocksuspension was diluted 25-fold with the same buffer and was preincubatedin the water bath at 37°C for 15 min, and then the test samplewas added. After incubation for 1 h, the sample was centrifugedat 4,000 × g for 5 min and the absorbance of the supernatant wasdetermined at 540 nm. The hemolysis effected by 0.1% Triton X-100was considered 100% hemolysis.

Preparation of liposomes. Liposomes were prepared by a freezing-thawing method. Lipid mixtures (Sigma, St. Louis, Mo.) were dissolved in chloroformand were dried with a stream of nitrogen gas to form a thin lipidfilm on the wall of a glass tube. The resulting thin film washydrated in buffer (pH 7.4) that contained 12.5 mM aminonaphthalene-3,6,8-trisulfonicacid (ANTS), 45 mM N,N'-p-xylenebis(pyridinium bromide) (DPX;Molecular Probe Inc., Eugene, Oreg.), 68 mM NaCl, and 10 mM HEPES(Sigma), shaken for 30 min, and vortexed vigorously for 10 min.The resulting multilamellar vesicles were sonicated and shakenfor 1 h at room temperature. The suspension was frozen-thawedfor five cycles. The liposomes were separated from the unencapsulatedmaterial on Sephadex G-50 (Pharmacia, Upsala, Sweden) that wasequilibrated with 10 mM HEPES buffer (pH 7.4) containing 150 mMNaCl and 1 mM ethylene glycol-bis( $beta$ -aminoethyl ether)-N,N,N',N'-tetraaceticacid (Sigma).

Liposome leakage assay. The liposome leakage assay was based on the quenching of ANTS fluorescence by DPX (18, 43). The quenching of ANTS by DPXoccurs by nonradiative energy transfer and depends on the averagedistance between two molecules. When the leakage occurred, ANTSand DPX were released from the liposomes and ANTS emitted fluorescence.Therefore, the leakage was measured directly by determining therelative change in fluorescence. The liposomes initially containingboth ANTS (12.5 mM) and DPX (45 mM) emitted some fluorescence,which was set as the baseline, and the fluorescence from liposomeslysed with Triton X-100 was set as an indicator of 100% leakage.Fluorescence, excited at 360 nm and emitted at 535 nm, was measuredwith a Jasco J-777 spectrofluorometer (Jasco, Tokyo, Japan) (19).

CD measurement. Circular dichroism (CD) spectra were recorded on a Jasco J-715 spectropolarimeter (Jasco), using a quartz cell path lengthof 1 mm, at wavelengths ranging from 190 to 245 nm. A sample solutionwas prepared by mixing 50% (wt/vol) trifluoroethanol (TFE) and20 mM sodium phosphate buffer at pH 7.4 or by the addition of25 mM sodium dodecyl sulfate in 10 mM sodium phosphate bufferat pH 7.4. The peptide concentration was determined on the basisof amino acid analysis. The CD spectrum was recorded at room temperatureand was obtained with a 0.5-nm bandwidth and a scan speed of 10nm/min. Two scans were averaged to improve the signal-to-noiseratio. The CD data were analyzed for the percentage of the secondarystructure of peptides by the method of Chen et al. (14).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Design of combinatorial peptide libraries composed of simplified amino acid sequences. Seven amino acids (Lys, Leu, Val, Pro, Ser, Phe, and Gln) instead of the 20 natural amino acids were selected for use in thesynthesis of peptide mixtures by consideration of the characteristicsof amino acids (for a review, see reference 34). Lys, whichis one of the positively charged amino acids (Lys, Arg, and His),was chosen because of its high pK_a value and the easy deprotectionof its side protection group in Fmoc chemistry. Leu and Val, whichare in the class of aliphatic amino acids, were selected becauseof their secondary structure-forming propensities. Phe, whichis in the class of aromatic amino acids (Phe, Tyr, and Trp), wasselected because of the efficiency of its synthesis and deprotection.Ser was chosen for the hydroxyl amino acid, and Gln was chosenfor the hydrophilic neutral amino acid. Pro, which is known asan $alpha$ helix breaker, was also included. Cys was excluded becauseof its dimerization by disulfide bridge. Negatively charged aminoacids (Glu, Asp) were excluded because the negative charge ofthe peptides interfere with the charge-charge interactions betweenthe peptide and the negatively charged membrane. In our previouswork, replacement of the amino acids of the antimicrobial decapeptidederived from tenecin 1 indicated that the presence of positivelycharged amino acid at the N terminus or the C terminus was criticalfor antifungal activity (26). Therefore, Lys was fixed at theC terminus for the efficient synthesis of the libraries.

Screening of the active peptide against C. albicans. To identify the most active amino acid sequence against C. albicans, each peptide mixture made up of nine libraries was preparedand assayed. As shown in Fig. 1, the most active peptide sequencehad Lys at O₁ and O₂, which confirmed our previous result thata positively charged amino acid at the N or C terminus is criticalfor antifungal activity. The presence of Val at O₃ and O₄ resultedin the highest level of activity. The selectivity of the aminoacid at O₅ was not great. When Val or Phe was located at O₅, thepeptides had the same MICs; however, the 50% inhibitory concentrationwas lowest when the Phe was located at O₅ (data not shown). Thepresence of Lys at O₆ gave the highest level of antifungal activity.The MICs were the same when any aliphatic amino acid was locatedat O₇. However, Val was selected as the most active sequence atposition O₇ when the 50% inhibitory concentration of peptideswith various amino acids at O₇ were compared (data not shown).After complete screening, the most active decapeptide, KKVVFKVKFK-NH₂,named KSL, tested in this investigation was identified. The searchfor amino acid sequences similar to that of KSL by the BLAST program(http://www.ncbi.nih.gov/) showed that no similar amino acid sequencehas been registered. As shown in Fig. 2, KSL did not show theperfect amphipathic $alpha$ -helical structure in a wheel diagram andhad valine residues in the hydrophobic face.

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FIG. 1. Screening of libraries for activity that inhibits the growth of C. albicans. Each bar represents the MIC of the peptide mixture with a peptide defined at the O position with one of the seven amino acids used in the library; a, the initial position is defined (OXXXXXXXXK-NH₂); b, the second position is defined (KOXXXXXXXK-NH₂); c, the third position is defined (KKOXXXXXXK-NH₂); d, the fourth position is defined (KKVOXXXXXK-NH₂); e, the fifth position is defined (KKVVOXXXXK-NH₂); f, the sixth position is defined (KKVVFOXXXK-NH₂); g, the seventh position is defined (KKVVFKOXXK-NH₂); h, the eighth position is defined (KKVVFKVOXK-NH₂); i, the ninth position is defined (KKVVFKVKOK-NH₂).

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FIG. 2. Helical wheel diagram of KSL.

Antimicrobial and hemolytic activity of KSL. As shown in Table 1, the peptide (KSL) with the most active sequence was synthesized, and its antibacterial and antifungalactivities were measured. Although the size of KSL was much smallerthan that of magainin II (47), the MIC of KSL for C. albicanswas almost seven times lower than that of magainin II. Also, theantibacterial activity of KSL was more potent than that of magaininII against all test microorganisms, especially methicillin-resistantStaphylococcus aureus (MRSA). The MFC of KSL for C. albicans was0.78 µg/ml, which indicated that KSL irreversibly inhibited thegrowth of C. albicans at the same concentration as the MIC (0.78µg/ml). To lend credence to the activity in this assay, amphotericinB (15), fluconazole (22), and the antifungal hexapeptide identifiedby full peptide libraries (28) were assayed simultaneously andtheir activities were compared. Amphotericin B, which is knownto be the most effective antifungal agent, had the same MFC andMIC (0.2 µg/ml) in this assay system. Fluconazole as a fungistaticagent did not show a clear cutoff value up to 50 µg/ml. The antifungalhexapeptide (28) had an MFC approximately 15 times higher (MFC,12.5 µg/ml) than that of KSL (MFC, 0.78 µg/ml). To check the cytotoxicityagainst mammalian cells, KSL was added to mouse erythrocytes,and the level of hemolysis was measured. Figure 3 indicates thelevel of lysis of the mouse erythrocytes as a function of theconcentrations of KSL, melittin, and amphotericin B. AmphotericinB and melittin (16) caused 100% lysis at concentrations greaterthan 10 µg/ml, while KSL did not show hemolytic activity at concentrationsof up to 500 µg/ml. The concentration causing 50% hemolysis forKSL was approximately 600 times higher than the MIC for C. albicans(data not shown). This result indicates that KSL has a high degreeof selectivity for fungi rather than mammalian cells.

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TABLE 1. Antimicrobial activities of KSL and other antimicrobial compounds

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FIG. 3. Hemolytic activity of KSL. Erythrocytes were incubated in Tris buffer (150 mM KCl, 5 mM Tris-HCl [pH 7.4]) with various concentration of KSL for 1 h at 37°C. $open circle$ , KSL; $bullet$ , melittin; $black-down-triangle$ , amphotericin B.

Antimicrobial activities of individual peptides identified by combinatorial libraries. To confirm the results obtained with the combinatorial libraries, individual peptides were synthesized and assayed againstbacteria as well as fungi. The sequences and characteristics ofindividual peptides are summarized in Table 2. Because the positivecharge of the peptide was a critical factor for antimicrobialactivity, hydrophobic amino acids were replaced only by otherhydrophobic amino acids. All peptides had the same net positivecharge, similar hydrophobicities, and similar hydrophobic moments.As shown in Table 3, KSL1 with valine at position 5 and KSL2with phenylalanine at position 7 had the same MICs as KSL forC. albicans. The same MICs of KSL1 and KSL2 confirmed the resultsobtained with libraries in which the selectivity of hydrophobicamino acids at positions 5 and 7 for antifungal activity was notgreat. KSL3, KSL4, and KSL5, which were expected to be less potentthan KSL on the basis of the results obtained with the libraries,in fact showed low levels of antifungal activity. In particular,KSL5, which contained Pro, which is known to be an $alpha$ helix breaker,did not show activity at concentrations of up to 100 µg/ml. Theactivity of the individual peptide confirmed that KSL identifiedby the combinatorial library was the most active peptide againstC. albicans. Interestingly, KSL2 showed the same activity as KSLagainst C. albicans, while it showed activity much better thanthat of KSL against MRSA and Mycobacterium smegmatis. This resultindicated that the peptide identified by the libraries to be themost active against C. albicans could be different from that identifiedto be the most active against the other pathogens.

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TABLE 2. Sequences, $alpha$ helicities, hydrophobicities, and hydrophobic moments of KSL and its analogs^a

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TABLE 3. Antimicrobial activities of KSL and its analogs

Assay of leakage of dyes from liposomes caused by KSL. To study the mechanisms of antifungal and antibacterial activity, we prepared liposomes with the phospholipid compositionsof fungal and gram-positive bacterial membranes and measured therelease of the dye from the liposomes induced by the peptide.Amphotericin B, which is known to be a membrane-active molecule(15), and fluconazole (22) were used as positive and negativecontrols, respectively. As shown in Fig. 4A, the increase in theconcentration of KSL resulted in an increase in the level of leakageof dye from the liposomes whose compositions resembled that ofthe fungal membrane. The membrane-disrupting ability of KSL wasmuch lower than that of amphotericin B, which was consistent withthe relative potencies of the peptide and amphotericin B againstC. albicans. Fluconazole, which is known to act on the enzymein the cytoplasm as a primary target, did not cause leakage whenit was used up to a concentration comparable to that of KSL. Figure4B indicates the level of release of the dye from the liposomewhose composition mimicked that of the membrane of gram-positivebacteria as a function of the concentration of KSL. In this experiment,magainin II, which is a membrane-active peptide (47), was usedas a positive control. KSL and magainin II had similar leakagepatterns and potencies as a function of the concentration. Thus,we suggest that the antifungal and antibacterial actions of thepeptide are due to its interaction with and perturbation of thefungal and bacterial membranes. The hemolytic activities of KSLand melittin were measured by determining the level of releaseof dye from liposomes whose compositions resembled that of themembrane of human erythrocytes. As shown in Fig. 5, no significantleakage was observed that of with KSL at up to 25 µg/ml, while3 µg of melittin, which is a cytotoxic peptide (16), per mlcaused 100% leakage under the same assay conditions. From thisstudy, we confirmed that KSL was highly selective between thefungal and erythrocyte membranes, which would prove to be a greatadvantage for pharmaceutical agents.

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FIG. 4. Leakage of the dye from liposomes. (A) The phospholipid composition of the liposomes resembled that of the fungal membrane (molar ratio of phosphatidycholine:phosphatidylethanolamine:phosphatidylserine:phophatidylinositol:cerebroside:cholesterol, 30:30:10:10:5:20). Antifungal compounds were incubated with liposomes for 1 h at 37°C. $bullet$ , amphotericin B; $open circle$ , KSL; $black-down-triangle$ , fluconazole. (B) The phospholipid compositions of the liposomes resembled that of the membrane of gram-positive bacteria (molar ratio of phosphatidyglycerol:cardiolipin, 3:1). The peptides were incubated with liposomes for 1 h at 37°C. $bullet$ , magainin II; $open circle$ , KSL.

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FIG. 5. Hemolytic activities measured by the leakage of the dye from the liposome by peptide. The phospholipid compositions of the liposomes resembled that of the human erythrocyte membrane (molar ratio of phosphatidylcholine:phosphatidylethanolamine:phosphatidylserine:sphingomyelin:cholesterol, 25:22:10:18:25). The peptides were incubated with the liposomes for 1 h at 37°C. $bullet$ , melittin; $open circle$ , KSL.

CD measurements. To investigate whether the antimicrobial activities of KSL and its analogs were correlated with the secondary structure, CDspectra were measured in various environments. According to theCD spectra, all peptides formed random coil structures in thephosphate buffer; however, all peptides except KSL5 formed a well-defined $alpha$ -helical structure in the presence of TFE (Table 2). KSL5, whichhad a proline in the middle of the amino acid sequence, had arandom coil structure in the presence of 50% TFE. The helicityindicated that the activity of each peptide was not correlatedwith the $alpha$ -helical content. For example, the less active peptideKSL3 had 70% $alpha$ helicity, while the more active peptides KSL andKSL1 had 56 and 42% $alpha$ helicities, respectively.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Antimicrobial peptides act on the lipid membrane of the pathogen, which has less specificity than other biological targetssuch as enzymes, antibodies, and hormone receptors. Therefore,we have designed novel peptide libraries consisting of simplifiedamino acid sequences to identify peptides with antifungal activity.Considering the relatively low level of specificity of the lipidmembrane for the peptide, our peptide libraries can supply enoughpeptide mixtures with a variety of structures, hydrophobicities,and net charges. The results of recent studies in which the replacementof 20 natural amino acids in proteins by simplified amino acidsdid not strongly affect the structure and function support oursuggestion (25, 40, 42).

Use of our novel peptide library technique has several advantages over use of the full peptide libraries and the traditionalstructure-activity relationship design method. The novel librarydeveloped in this study can identify the active amino sequencewith less resin, labor, and cost than are required when full peptidelibraries are used. This technique also overcomes the limitationsof traditional structure-activity relationship design methods,such as the time-consuming optimization process, the nonlinearrelationship between structure and activity, and a lack of informationon the structure of the peptide in the lipid membrane. Furthermore,the results obtained in studies with these peptide libraries canprovide useful information about the structure-activity relationshipbecause the secondary structures of decapeptides can easily becharacterized by CD spectroscopy.

The characterization of KSL, a peptide whose activity was optimized, provides useful information about the factor in the membrane-activepeptide responsible antimicrobial activity. KSL has a unique aminoacid sequence; five lysine residues (net positive charge, +6)at the hydrophilic face and three valine residues at the hydrophobicface in the $alpha$ -helical wheel diagram. Also, as shown in Fig. 2,KSL did not show the perfect amphipathic structure in the $alpha$ -helicalwheel diagram, and the mean hydrophobic moment was calculatedto be 0.22. This is different from the active peptides derivedfrom structure-activity relationship studies (5, 13, 34).However, KSL showed more potent antifungal activity than the peptidesthat satisfied the perfect amphipathic structure criteria andcontained a leucine residue in the hydrophobic face in the $alpha$ -helicalwheel diagram. This result indicates the risk of using the traditionalstructure-activity relationship design method, in which more activepeptides are designed by enhancing the $alpha$ helicity only on thebasis of the $alpha$ -helical wheel diagram.

Many structure-activity studies with antibacterial peptides indicate that an amphipathic structure and a net positive chargeare fundamental factors for the activity (41-45). On the basisof the result obtained with the libraries, individual peptideswere characterized to obtain an understanding of the structure-activityrelationship. All individual peptides have a same net positivecharge; however, activity is not correlated with the $alpha$ -helicalcontent of the peptides calculated from the CD spectra measuredin the presence of 50% TFE. An inactive analog with Pro in themiddle of the amino acid sequence has a random conformation inthe presence of 50% TFE, which is consistent with the generalstructure-activity relationship. Even though KSL adopts the $alpha$ -helicalconformation in the presence of TFE, the most active peptide hasVal residues instead of Leu residues in the hydrophobic face.This is a quite surprising result because Val has a low propensityfor $alpha$ helix formation, while Leu is one of the best $alpha$ -helix-formingresidues. Also, KSL3 with Leu instead of Val in the hydrophobicface has a higher $alpha$ -helical content in the presence of TFE buthas a lower level of activity than KSL. To obtain a more detailedstructure, CD spectra of KSL and KSL3 were measured in the presenceof 25 mM sodium dodecyl sulfate. These spectra reveal that bothactive peptides adopt a distorted $alpha$ -helical conformation and thatthe less active peptide KSL3 shows a decrease in the distorted $alpha$ -helical content (data not shown). There are two possible explanationsfor this; first, the real active secondary structure of KSL mustbe the distorted $alpha$ helix because sodium dodecyl sulfate, withan anionic functional group in the end of an aliphatic lipid,rather than TFE must mimic the real biological membrane system.The other possible explanation is that there is some thresholdof the secondary structure for antimicrobial activity. If the $alpha$ helicity of the peptide is over this threshold, the structureis no longer a major factor in the activity. The former explanationseems to be more reasonable because the charge-charge interactionsbetween the positively charged peptides with the negatively chargedmembrane is important for the binding and adoption of the structureof the positively charged peptide.

Interestingly, the peptides identified to have activity against C. albicans have high levels of activity against gram-positiveand gram-negative bacteria. The different ratio and compositionof the phospholipids between bacteria and fungi can explain thisresult. Bacterial membranes consisting of phosphatidylglyceroland cardiolipin have a more negative charge than fungal membranes,so positively charged peptides interact with the more negativelycharged membranes of bacteria and enhance the permeability ofthe lipid membrane. This result supports the fact that regardlessof the species of pathogens, the charge-charge interaction betweenpositively charged antimicrobial peptides and negatively chargedmembranes is the common factor fundamental for the activitiesof the peptides. However, KSL and KSL2, which had the same activitiesagainst C. albicans, had different activities against MRSA andM. smegmatis, which strongly suggests that the lipid membraneof each microorganism has a sufficient specificity for differentiatingthe peptides consisting of simplified amino acid sequences. Thisfact indicates that our libraries can be applied to the screeningof the membrane-active peptide against special pathogens suchas MRSA.

The low level of hemolytic activity of the host defense peptides has been explained by several factors such as size, structure,and hydrophobicity. Magainin, cecropin, and other host defensepeptides containing one or more amino acids known as $alpha$ -helix breakershave the potential to adopt a less perfect $alpha$ -helical structure.This imperfect amphipathic structure is regarded as a key factorfor the differentiation of host cells from pathogenic cells (8).However, the low level of hemolytic activity of KSL without an $alpha$ -helix breaker supports the fact that the low level of hemolyticactivity of this peptide must be due to its small size or itslow level of hydrophobicity. The low level of hydrophobicity seemsto be a key factor for the differentiation of mammalian cellsfrom fungal cells because high-level hydrophobic interactionswere reported to be necessary for the lysis of the erythrocytemembrane (35). Also, a very hydrophobic peptide, indolicidin,consisting of 13 amino acid residues, was reported to have hemolyticactivity as well as antimicrobial activity (44).

Even though many host defense peptides have been isolated and their functions have been studied (10-13), most of them showantibacterial activity rather than antifungal activity. Some shorthost defense peptides such as indolicidin (1) and tachyplesinII (37) show antifungal activity as well as antibacterial activity.However, it is difficult to develop these native peptides intoantifungal agents because of their cytotoxicity for the erythrocyte(13). The activity-optimized peptide identified in this studyirreversibly inhibits the growth of C. albicans through its actionon the lipid membrane and has a very potent and a broad rangeof activity against microorganisms but has no hemolytic activity.Considering the recent emergence of bacterial and fungal infectionsand resistant strains, it is possible that this peptide can bedeveloped as a novel antimicrobial agent. Also, the characterizationof KSL and its analogs will provide unique information about theirstructure-activity relationships.

	ACKNOWLEDGMENTS

This work was supported in part by grant from the Korean Ministry of Science and Technology.

We thank Soo-Il Chung for reading and critiquing the manuscript, and we also thank Jae-Wook Huh of KGCC for help with theCD measurements.

	FOOTNOTES

^* Corresponding author. Mailing address: Protein Chemistry Laboratory, Mogam Biotechnology Research Institute, 341 Pojung-Ri,Koosung-Myun, Yongin City, Kyonggi-Do, 449-910, Korea. Phone:82-331-262-3851. Fax: 82-331-262-6622. E-mail: lkh{at}kgcc.co.kr.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Abel, R. J., Y. Q. Tang, V. S. Rao, C. H. Dobbs, D. Tran, G. Barany, and M. E. Selsted. 1995. Synthesis and characterization of indolicidin, a tryptophan-rich antimicrobial peptide from bovine neutrophils. Int. J. Peptide Protein Res. 45:401-409[Medline].

2. Andreoli, T. E. 1974. The structure and function of amphotericin B-cholesterol pores in lipid bilayer membranes. Ann. N. Y. Acad. Sci. 235:448-468[Medline].

3. Andriole, V. T. 1993. Infections with Aspergillus species. Clin. Infect. Dis. 17(Suppl.):S481-S486.

4. Barra, D., and M. Simmanco. 1995. Amphibian skin: a promising resource for antimicrobial peptides. Trends Biotechnol. 13:205-209[Medline].

5. Barrow, C. J., K. Nakanishi, and K. Tachibana. 1992. Structure activity studies of pardaxin and analogues using model membranes of phosphatidylcholine. Biochim. Biophys. Acta 1112:235-240[Medline].

6. Bergstrom, J. D., C. Dufresne, G. F. Bills, M. Nallin-Omstead, and K. Byrne. 1995. Discovery, biosynthesis, and mechanism of action of the zaragozic acids: potent inhibitors of squalene synthase. Annu. Rev. Microbiol. 49:607-639[Medline].

7. Berkowitz, B. A., C. L. Bevins, and M. A. Zasloff. 1990. Magainins: a new family of membrane-active host defense peptides. Biochem. Pharmacol. 39:625-629[Medline].

8. Blondelle, S. E., and R. A. Houghten. 1992. Design of model amphipathic peptides having potent antimicrobial activities. Biochemistry 31:12688-12694[Medline].

9. Blondelle, S. E., and R. A. Houghten. 1996. Novel antimicrobial compounds identified using synthetic combinatorial library technology. Trends Biotechnol. 14:60-65[Medline].

10. Blondelle, S. E., E. Takahashi, P. A. Weber, and R. A. Houghten. 1994. Identification of antimicrobial peptides by using combinatorial libraries made up of unnatural amino acids. Antimicrob. Agents Chemother. 38:2280-2286[Abstract/Free Full Text].

11. Bodey, G., B. Bueltmann, W. Duguid, D. Gibbs, H. Hanak, M. Hotchi, G. Mall, P. Martino, F. Meunier, and S. Milliken. 1992. Fungal infections in cancer patients: an international autopsy survey. Eur. J. Clin. Microbiol. Infect. Dis. 11:99-109[Medline].

12. Boman, H. G., and D. Hultmark. 1987. Cell-free immunity in insects. Annu. Rev. Microbiol. 41:103-126[Medline].

13. Buttner, K., and R. A. H oughten. 1991. In E. Giralt, and D. Andreu (ed.), Proceedings of the Twenty-first European Peptide Symposium, p. 478-480. Escom, Leiden, The Netherlands.

14. Chen, Y. H., J. T. Yang, and H. M. Martinez. 1972. Determination of the secondary structures of proteins by circular dichroism and optical rotatory dispersion. Biochemistry 11:4120-4131[Medline].

15. Cheron, M., B. Cybulska, J. Mazerski, J. Grzybowska, A. Czerwinski, and E. Borowski. 1988. Quantitative structure-activity relationships in amphotericin B derivatives. Biochem. Pharmacol. 37:827-836[Medline].

16. Eisenberg, D., E. Schwarz, M. Komaronmy, and R. Wall. 1984. Analysis of membrane and surface protein sequences with the hydrophobic moment plot. J. Mol. Biol. 179:125-142[Medline].

17. Eisenberg, D., R. M. Weiss, and T. C. Terwilliger. 1982. The helical hydrophobic moment: a measure of the amphiphilicity of a helix. Nature 299:371-374[Medline].

18. Ellens, H., J. Benntz, and F. C. Szoka. 1984. pH-induced destabilization of phosphatidylethanolamine-containing liposomes: role of bilayer contact. Biochemistry 23:1532-1538[Medline].

19. Ellens, H., J. Benntz, and F. C. Szoka. 1985. H⁺- and Ca²⁺-induced fusion and destabilization of liposomes. Biochemistry 24:3099-3106[Medline].

20. Fields, G. B., Z. Tian, and G. Barany. 1992. Synthetic peptide: a user's guide, p. 77-183. W. H. Freeman & Co., New York, N.Y.

21. Furka, A., F. Sebestyen, M. Asgedom, and G. Dibo. 1991. General method for rapid synthesis of multicomponent peptide mixtures. Int. J. Peptide Protein Res. 37:487-493[Medline].

22. Galgiani, J. N. 1990. Susceptibility of Candida albicans and other yeasts to fluconazole: relation between in vitro and in vivo studies. Rev. Infect. Dis. 12:5272-5275.

23. Georgopapadakou, N. H., and T. J. Walsh. 1994. Human mycoses: drugs and targets for emerging pathogens. Science 264:371-373[Free Full Text].

24. Hata, K., J. Kimura, H. Miki, T. Toyosawa, T. Nakamura, and K. Katsu. 1996. In vitro and in vivo antifungal activities of ER-30346, a novel oral triazole with a broad antifungal spectrum. Antimicrob. Agents Chemother. 40:2237-2242[Abstract].

25. Heinz, D. W., W. A. Baase, and B. W. Matthews. 1992. Folding and function of T4 lysozyme containing 10 consecutive alanines illustrate the redundancy of information in an amino acid sequence. Proc. Natl. Acad. Sci. USA 89:3751-3755[Abstract/Free Full Text].

26. Hong, S. Y., J. E. Oh, M. Y. Kwon, J. H. Lee, B. L. Lee, and K. H. Lee. Unpublished data.

27. Houghten, R. A., and S. T. DeGraw. 1987. Effect of positional environmental domains of the variation of high-performance liquid chromatographic peptide retention coefficients. J. Chromatogr. 386:223-228[Medline].

28. Houghten, R. A., C. Pinilla, S. E. Blondelle, J. R. Appel, C. T. Dooley, and J. H. Cuervo. 1991. Generation and use of synthetic peptide combinatorial libraries for basic research and drug discovery. Nature (London) 354:84-86[Medline].

29. Kaiser, E. T., R. L. Colescott, C. D. Bossinger, and P. I. Cook. 1970. Color test for detection of free terminal amino groups in the solid-phase synthesis of peptides. Anal. Biochem. 34:595-598[Medline].

30. Kinsky, S. C. 1970. Antibiotic interaction with model membranes. Annu. Rev. Pharmacol. 10:119-142[Medline].

31. Lam, K. S., S. E. Salmon, E. M. Hersh, V. J. Hruby, W. M. Kazmierski, and R. J. Knapp. 1991. A new type of synthetic peptide library for identifying ligand-binding activity. Nature (London) 354:82-84[Medline].

32. Lee, K. H., S. Y. Hong, J. H. Yoon, J. E. Oh, M. Y. Kwon, J. H. Lee, B. L. Lee, and H. M. Moon. 1998. Identification and characterization of the novel antimicrobial peptide corresponding to C-terminal $beta$ sheet domain of tenecin 1, an antibacterial protein of larvae of Tenebrio molitor. Biochem. J. 334:99-105.

33. Mak, P., K. Wojcik, I. B. Thogersen, and A. Dubin. 1996. Isolation, antimicrobial activities, and primary structures of hamster neutrophil defensins. Infect. Immun. 64:4444-4449[Abstract].

34. Maloy, W. L., and U. P. Kari. 1995. Structure-activity studies on magainins and other host defense peptides. Biopolymers 37:105-122[Medline].

35. Matsuzaki, K., K. Sugishita, N. Fuhii, and K. Miyahima. 1995. Molecular basis for membrane selectivity of an antimicrobial peptide, magainin 2. Biochemistry 34:3423-3429[Medline].

36. McLean, L. R., K. A. Hagaman, T. J. Owen, and J. L. Krstenansky. 1991. Minimal peptide length for interaction of amphipathic $alpha$ -helical peptides with phosphatidylcholine liposomes. Biochemistry 30:31-37[Medline].

37. Miyata, T., F. Tokunaga, T. Yoneya, K. Yoshikawa, S. Iwanaga, M. Niwa, T. Takao, and Y. Shimonishi. 1989. Antimicrobial peptides, isolated from horseshoe crab hemocytes, tachyplesin II, and polyphemusins I and II: chemical structures and biological activity. J. Biochem. (Tokyo) 106:663-668[Abstract/Free Full Text].

38. Ostresh, J. H., G. M. Husar, S. E. Blondelle, B. Dorner, P. A. Wever, and R. A. Houghten. 1994. "Libraries from libraries": chemical transformation of combinatorial libraries to extend the range and repertoire of chemical diversity. Proc. Natl. Acad. Sci. USA 91:11138-11142[Abstract/Free Full Text].

39. Qu, X. D., S. S. Harwig, W. M. Shafer, and R. I. Lehrer. 1997. Protegrin structure and activity against Neisseria gonorrhoeae. Infect. Immun. 65:636-639[Abstract].

40. Riddle, D. S., J. V. Santiago, S. T. Bray-Hall, N. Doshi, V. P. Grantcharova, Q. Yi, and D. Baker. 1997. Functional rapidly folding proteins from simplified amino acid sequence. Nat. Struct. Biol. 4:805-809[Medline].

41. Rodriguez-Tudela, J. L., J. Berenguer, J. V. Martinez-Sugarez, and R. Sanchez. 1996. Comparison of a spectrophotometric microdilution method with RPMI-2% glucose with the National Committee for Clinical Laboratory Standards reference macrodilution method M27-P for in vitro susceptibility testing of amphotericin B, flucytosine, and fluconazole against Candida albicans. Antimicrob. Agents Chemother. 40:1998-2003[Abstract].

42. Shang, Z., V. E. Isaac, H. Li, L. Patel, K. M. Catron, T. Curran, G. T. Montelione, and C. Abate. 1994. Design of a "minimal" homeodomain: the N-terminal arm modulates DNA binding affinity and stabilizes homeodomain structure. Proc. Natl. Acad. Sci. USA 91:3751-3755.

43. Smolarsky, M., D. Teitelbaum, M. Sela, and C. Gitler. 1977. A simple fluorescent method to determine complement-mediated liposome immune lysis. J. Immunol. Methods 15:255-265[Medline].

44. Subbalakshmi, C., V. Krishnakumari, R. Nagaraj, and N. Sitaram. 1996. Requirements for antibacterial and hemolytic activities in the bovine neutrophil derived 13-residue peptide indolicidin. FEBS Lett. 395:48-52[Medline].

45. Sugawara, T., M. Shibazaki, H. Nakahara, and K. Suzuki. 1996. YM-47522, a novel antifungal antibiotic produced by Bacillus sp. II. Structure and relative stereochemistry. J. Antibiot. (Tokyo) 49:345-348[Medline].

46. Young, L. S. 1981. Nosocomial infections in the immunocompromised adult. J. Med. 70:398-404.

47. Zasloff, M. 1987. Magainins, a class of antimicrobial peptides from Xenopus skin: isolation, characterization of two active forms, and partial cDNA sequence of a precursor. Proc. Natl. Acad. Sci. USA 84:5449[Abstract/Free Full Text].

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1.	Abel, R. J., Y. Q. Tang, V. S. Rao, C. H. Dobbs, D. Tran, G. Barany, and M. E. Selsted. 1995. Synthesis and characterization of indolicidin, a tryptophan-rich antimicrobial peptide from bovine neutrophils. Int. J. Peptide Protein Res. 45:401-409[Medline].
2.	Andreoli, T. E. 1974. The structure and function of amphotericin B-cholesterol pores in lipid bilayer membranes. Ann. N. Y. Acad. Sci. 235:448-468[Medline].
3.	Andriole, V. T. 1993. Infections with Aspergillus species. Clin. Infect. Dis. 17(Suppl.):S481-S486.
4.	Barra, D., and M. Simmanco. 1995. Amphibian skin: a promising resource for antimicrobial peptides. Trends Biotechnol. 13:205-209[Medline].
5.	Barrow, C. J., K. Nakanishi, and K. Tachibana. 1992. Structure activity studies of pardaxin and analogues using model membranes of phosphatidylcholine. Biochim. Biophys. Acta 1112:235-240[Medline].
6.	Bergstrom, J. D., C. Dufresne, G. F. Bills, M. Nallin-Omstead, and K. Byrne. 1995. Discovery, biosynthesis, and mechanism of action of the zaragozic acids: potent inhibitors of squalene synthase. Annu. Rev. Microbiol. 49:607-639[Medline].
7.	Berkowitz, B. A., C. L. Bevins, and M. A. Zasloff. 1990. Magainins: a new family of membrane-active host defense peptides. Biochem. Pharmacol. 39:625-629[Medline].
8.	Blondelle, S. E., and R. A. Houghten. 1992. Design of model amphipathic peptides having potent antimicrobial activities. Biochemistry 31:12688-12694[Medline].
9.	Blondelle, S. E., and R. A. Houghten. 1996. Novel antimicrobial compounds identified using synthetic combinatorial library technology. Trends Biotechnol. 14:60-65[Medline].
10.	Blondelle, S. E., E. Takahashi, P. A. Weber, and R. A. Houghten. 1994. Identification of antimicrobial peptides by using combinatorial libraries made up of unnatural amino acids. Antimicrob. Agents Chemother. 38:2280-2286[Abstract/Free Full Text].
11.	Bodey, G., B. Bueltmann, W. Duguid, D. Gibbs, H. Hanak, M. Hotchi, G. Mall, P. Martino, F. Meunier, and S. Milliken. 1992. Fungal infections in cancer patients: an international autopsy survey. Eur. J. Clin. Microbiol. Infect. Dis. 11:99-109[Medline].
12.	Boman, H. G., and D. Hultmark. 1987. Cell-free immunity in insects. Annu. Rev. Microbiol. 41:103-126[Medline].
13.	Buttner, K., and R. A. H oughten. 1991. In E. Giralt, and D. Andreu (ed.), Proceedings of the Twenty-first European Peptide Symposium, p. 478-480. Escom, Leiden, The Netherlands.
14.	Chen, Y. H., J. T. Yang, and H. M. Martinez. 1972. Determination of the secondary structures of proteins by circular dichroism and optical rotatory dispersion. Biochemistry 11:4120-4131[Medline].
15.	Cheron, M., B. Cybulska, J. Mazerski, J. Grzybowska, A. Czerwinski, and E. Borowski. 1988. Quantitative structure-activity relationships in amphotericin B derivatives. Biochem. Pharmacol. 37:827-836[Medline].
16.	Eisenberg, D., E. Schwarz, M. Komaronmy, and R. Wall. 1984. Analysis of membrane and surface protein sequences with the hydrophobic moment plot. J. Mol. Biol. 179:125-142[Medline].
17.	Eisenberg, D., R. M. Weiss, and T. C. Terwilliger. 1982. The helical hydrophobic moment: a measure of the amphiphilicity of a helix. Nature 299:371-374[Medline].
18.	Ellens, H., J. Benntz, and F. C. Szoka. 1984. pH-induced destabilization of phosphatidylethanolamine-containing liposomes: role of bilayer contact. Biochemistry 23:1532-1538[Medline].
19.	Ellens, H., J. Benntz, and F. C. Szoka. 1985. H⁺- and Ca²⁺-induced fusion and destabilization of liposomes. Biochemistry 24:3099-3106[Medline].
20.	Fields, G. B., Z. Tian, and G. Barany. 1992. Synthetic peptide: a user's guide, p. 77-183. W. H. Freeman & Co., New York, N.Y.
21.	Furka, A., F. Sebestyen, M. Asgedom, and G. Dibo. 1991. General method for rapid synthesis of multicomponent peptide mixtures. Int. J. Peptide Protein Res. 37:487-493[Medline].
22.	Galgiani, J. N. 1990. Susceptibility of Candida albicans and other yeasts to fluconazole: relation between in vitro and in vivo studies. Rev. Infect. Dis. 12:5272-5275.
23.	Georgopapadakou, N. H., and T. J. Walsh. 1994. Human mycoses: drugs and targets for emerging pathogens. Science 264:371-373[Free Full Text].
24.	Hata, K., J. Kimura, H. Miki, T. Toyosawa, T. Nakamura, and K. Katsu. 1996. In vitro and in vivo antifungal activities of ER-30346, a novel oral triazole with a broad antifungal spectrum. Antimicrob. Agents Chemother. 40:2237-2242[Abstract].
25.	Heinz, D. W., W. A. Baase, and B. W. Matthews. 1992. Folding and function of T4 lysozyme containing 10 consecutive alanines illustrate the redundancy of information in an amino acid sequence. Proc. Natl. Acad. Sci. USA 89:3751-3755[Abstract/Free Full Text].
26.	Hong, S. Y., J. E. Oh, M. Y. Kwon, J. H. Lee, B. L. Lee, and K. H. Lee. Unpublished data.
27.	Houghten, R. A., and S. T. DeGraw. 1987. Effect of positional environmental domains of the variation of high-performance liquid chromatographic peptide retention coefficients. J. Chromatogr. 386:223-228[Medline].
28.	Houghten, R. A., C. Pinilla, S. E. Blondelle, J. R. Appel, C. T. Dooley, and J. H. Cuervo. 1991. Generation and use of synthetic peptide combinatorial libraries for basic research and drug discovery. Nature (London) 354:84-86[Medline].
29.	Kaiser, E. T., R. L. Colescott, C. D. Bossinger, and P. I. Cook. 1970. Color test for detection of free terminal amino groups in the solid-phase synthesis of peptides. Anal. Biochem. 34:595-598[Medline].
30.	Kinsky, S. C. 1970. Antibiotic interaction with model membranes. Annu. Rev. Pharmacol. 10:119-142[Medline].
31.	Lam, K. S., S. E. Salmon, E. M. Hersh, V. J. Hruby, W. M. Kazmierski, and R. J. Knapp. 1991. A new type of synthetic peptide library for identifying ligand-binding activity. Nature (London) 354:82-84[Medline].
32.	Lee, K. H., S. Y. Hong, J. H. Yoon, J. E. Oh, M. Y. Kwon, J. H. Lee, B. L. Lee, and H. M. Moon. 1998. Identification and characterization of the novel antimicrobial peptide corresponding to C-terminal $beta$ sheet domain of tenecin 1, an antibacterial protein of larvae of Tenebrio molitor. Biochem. J. 334:99-105.
33.	Mak, P., K. Wojcik, I. B. Thogersen, and A. Dubin. 1996. Isolation, antimicrobial activities, and primary structures of hamster neutrophil defensins. Infect. Immun. 64:4444-4449[Abstract].
34.	Maloy, W. L., and U. P. Kari. 1995. Structure-activity studies on magainins and other host defense peptides. Biopolymers 37:105-122[Medline].
35.	Matsuzaki, K., K. Sugishita, N. Fuhii, and K. Miyahima. 1995. Molecular basis for membrane selectivity of an antimicrobial peptide, magainin 2. Biochemistry 34:3423-3429[Medline].
36.	McLean, L. R., K. A. Hagaman, T. J. Owen, and J. L. Krstenansky. 1991. Minimal peptide length for interaction of amphipathic $alpha$ -helical peptides with phosphatidylcholine liposomes. Biochemistry 30:31-37[Medline].
37.	Miyata, T., F. Tokunaga, T. Yoneya, K. Yoshikawa, S. Iwanaga, M. Niwa, T. Takao, and Y. Shimonishi. 1989. Antimicrobial peptides, isolated from horseshoe crab hemocytes, tachyplesin II, and polyphemusins I and II: chemical structures and biological activity. J. Biochem. (Tokyo) 106:663-668[Abstract/Free Full Text].
38.	Ostresh, J. H., G. M. Husar, S. E. Blondelle, B. Dorner, P. A. Wever, and R. A. Houghten. 1994. "Libraries from libraries": chemical transformation of combinatorial libraries to extend the range and repertoire of chemical diversity. Proc. Natl. Acad. Sci. USA 91:11138-11142[Abstract/Free Full Text].
39.	Qu, X. D., S. S. Harwig, W. M. Shafer, and R. I. Lehrer. 1997. Protegrin structure and activity against Neisseria gonorrhoeae. Infect. Immun. 65:636-639[Abstract].
40.	Riddle, D. S., J. V. Santiago, S. T. Bray-Hall, N. Doshi, V. P. Grantcharova, Q. Yi, and D. Baker. 1997. Functional rapidly folding proteins from simplified amino acid sequence. Nat. Struct. Biol. 4:805-809[Medline].
41.	Rodriguez-Tudela, J. L., J. Berenguer, J. V. Martinez-Sugarez, and R. Sanchez. 1996. Comparison of a spectrophotometric microdilution method with RPMI-2% glucose with the National Committee for Clinical Laboratory Standards reference macrodilution method M27-P for in vitro susceptibility testing of amphotericin B, flucytosine, and fluconazole against Candida albicans. Antimicrob. Agents Chemother. 40:1998-2003[Abstract].
42.	Shang, Z., V. E. Isaac, H. Li, L. Patel, K. M. Catron, T. Curran, G. T. Montelione, and C. Abate. 1994. Design of a "minimal" homeodomain: the N-terminal arm modulates DNA binding affinity and stabilizes homeodomain structure. Proc. Natl. Acad. Sci. USA 91:3751-3755.
43.	Smolarsky, M., D. Teitelbaum, M. Sela, and C. Gitler. 1977. A simple fluorescent method to determine complement-mediated liposome immune lysis. J. Immunol. Methods 15:255-265[Medline].
44.	Subbalakshmi, C., V. Krishnakumari, R. Nagaraj, and N. Sitaram. 1996. Requirements for antibacterial and hemolytic activities in the bovine neutrophil derived 13-residue peptide indolicidin. FEBS Lett. 395:48-52[Medline].
45.	Sugawara, T., M. Shibazaki, H. Nakahara, and K. Suzuki. 1996. YM-47522, a novel antifungal antibiotic produced by Bacillus sp. II. Structure and relative stereochemistry. J. Antibiot. (Tokyo) 49:345-348[Medline].
46.	Young, L. S. 1981. Nosocomial infections in the immunocompromised adult. J. Med. 70:398-404.
47.	Zasloff, M. 1987. Magainins, a class of antimicrobial peptides from Xenopus skin: isolation, characterization of two active forms, and partial cDNA sequence of a precursor. Proc. Natl. Acad. Sci. USA 84:5449[Abstract/Free Full Text].