Dual-action, unnatural proline-rich peptides as antibiotic agents and methods thereof

Abstract

The present invention cationic amphiphilic polyproline helices (CAPHs) compounds having increased hydrophobicity and cellular internalization as antimicrobial agents. Antimicrobial compositions and methods of using the same are also provided.

Claims

1. A compound having the structure: ##STR00007## wherein R.sub.1 is an alkyl substituent, the alkyl substituent being straight, branched or cyclic, an aryl substituent, an acyl substituent, an acetyl substituent, a dye, a fluorophore, a conjugating agent, an intracellular directing group or an antimicrobial agent; wherein R.sub.2 and R.sub.3 are each independently, a hydrophobic alkyl or aryl moiety; and wherein n is from about 3 to about 10.

2. The compound of claim 1 wherein R.sub.1 is a fluorophore.

3. The compound of claim 1 wherein R.sub.1 is an antimicrobial agent.

4. The compound of claim 3 wherein the antimicrobial agent is kanamycin.

5. The compound of claim 1 wherein the hydrophobic alkyl moiety is linear, branched or cyclic and wherein the hydrophobic alkyl moiety comprises from at least 1 carbon atom to about 20 carbon atoms.

6. The compound of claim 1 wherein the hydrophobic aryl moiety comprises from about 5 carbon atoms to about 7 carbon atoms.

7. The compound of claim 1 wherein R.sub.2 and R.sub.3 are each independently n-pentyl, n-heptyl, cyclohexyl, phenyl, pmethoxyphenyl or p-nitrophenyl.

8. The compound of claim 1 wherein n is from about 3 to about 5.

9. An antimicrobial composition comprising: at least one compound of claim 1; and at least one buffer.

10. A compound having the structure: ##STR00008## wherein R.sub.1 is an alkyl substituent, the alkyl substituent being straight, branched or cyclic, an aryl substituent, an acyl substituent, an acetyl substituent, a dye, a fluorophore, a conjugating agent or an antimicrobial agent; wherein R.sub.2 and R.sub.3 are each independently, a hydrophobic alkyl or aryl moiety; wherein n is from about 3 to about 10; and wherein p is from about 1 to about 5.

11. The compound of claim 10 wherein R.sub.1 is a fluorophore.

12. The compound of claim 10 wherein R.sub.1 is an antimicrobial agent.

13. The compound of claim 3 wherein the antimicrobial agent is kanamycin.

14. The compound of claim 10 wherein the hydrophobic alkyl moiety is linear, branched or cyclic and wherein the hydrophobic alkyl moiety comprises from about 11 carbon atoms to about 20 carbon atoms.

15. The compound of claim 10 wherein the hydrophobic aryl moiety comprises from about 5 carbon atoms to about 7 carbon atoms.

16. The compound of claim 10 wherein R.sub.2 and R.sub.3 are each independently n-pentyl, n-heptyl, cyclohexyl, phenyl, pmethoxyphenyl or p-nitrophenyl.

17. The compound of claim 10 wherein n is from about 3 to about 5.

18. An antimicrobial composition comprising: at least one compound of claim 10; and at least one buffer.

Description

BRIEF DESCRIPTION OF THE DRAWINGS

(1) FIG. 1 is a schematic showing examples of compound (I) of the present invention.

DETAILED DESCRIPTION OF THE INVENTION

(2) The following detailed description is of the best currently contemplated modes of carrying out the invention. The description is not to be taken in a limiting sense, but is made merely for the purpose of illustrating the general principles of the invention, since the scope of the invention is best defined by the appended claims.

(3) The present invention provides cationic amphiphilic polyproline helices (CAPHs) that act both as cell penetrating agents and as antimicrobial agents. These properties allow the CAPHs of the present invention to penetrate a host cell, destroy the microbe invading the host cell with minimal cytotoxicity to the host cell. It is contemplated that the host cell may be mammalian or animal cell, including, but not limited to, human, dog, cat, horse and bird. It will be appreciated that the CAPH compounds of the present invention may be used in both human and veterinary applications.

(4) While CAPHs are known in the prior art, the CAPHs of the present invention have been modified to allow for increased hydrophobicity of the CAPHs. While not wishing to be bound by theory, increased hydrophobicity may increase cellular uptake. Manipulation of the hydrophobicity may also effect the method of cellular uptake and therefore, cellular localization. Previously, the proline moieties of the CAPHs were modified using an ether linkage (Scheme 1). In the present invention, an amide linkage may be used instead of the ether linkage, allowing for a wide diversity of hydrophobic substituents to be added to the CAPHs of the present invention.

(5) ##STR00003##

(6) In one embodiment of the present invention there is provided compound (I) having the structure:

(7) ##STR00004##

(8) wherein R.sub.1 may be an alkyl substituent, the alkyl substituent being straight, branched or cyclic, an aryl substituent, a dye, a fluorophore, a conjugating agent or an antimicrobial agent;

(9) R.sub.2 and R.sub.3 may each independently be, a hydrophobic alkyl or aryl moiety and

(10) n may be from about 3 to about 10.

(11) In one embodiment of the present invention n may be from about 3 to about 10 repeats. Preferably, n may be from about 3 to about 5 repeats. By increasing number of repeats (n) corresponding to the length of the CAPH, additional cationic and hydrophobic groups may be introduced into the helix. An increase of just one repeat from n=3 to n=4 may increase cellular permeation as well as effect the internalization mechanism and subcellular localization of the CAPH of the present invention. CAPHs may be internalized in a number of different ways including, but not limited to endocytosis and direct transport. When internalized of the CAPH of the present invention by endocytosis may result in endosomal entrapment of the CAPH. Direct transport, however, may allow for the CAPH to be localized in a specific, desired subcellular localization. While not wishing to be bound by theory, it has been found that increasing number of repeats or length of the CAPH allows for internalization by direct transport at lower concentrations of the CAPH.

(12) The CAPH compounds of the present invention may comprise other molecules that may allow for the monitoring of subcellular localization, may help direct subcellular localization and/or may allow for direct binding to a moiety within the host cell. In one embodiment of the present invention, R.sub.1 may be an alkyl or aryl moiety, preferable one that increases the cationic or hydrophobic propertied of the compound of the present invention. Alternatively, R.sub.1 may be a fluorophore or fluorescent molecule that allows for the tracking of the subcellular location of the compound. A non-limiting example may be fluorescein. Likewise, R.sub.1 may be any molecule that allows for tracking and detection of the molecule in the host cell. It will be appreciated that there are many compounds that may be used including dye molecules and those containing radioactive markers.

(13) Alternative, R.sub.1 may be compounds that direct subcellular localization by binding covalently or non-covalently to proteins, membranes or other subcellular organelles or moieties. Conjugating agents may be crosslinking agents, a plethora of which is known in the art. They may also be binding agents, such as but not limited to biotin. In a preferred embodiment R.sub.1 may be intracellular directing groups such as, but not limited to actin binding sequence and endoplasmic reticulum binding sequence. By way of non-limiting example, when Listeria invades a host cell, it is usually located in the macrophages where more antimicrobial agents cannot act upon it. R.sub.1 may be an actin binding sequence, allowing for the subcellular localization of the CAPH of the present invention in the macrophages and allowing it to destroy Listeria.

(14) In a further embodiment of the present invention, R.sub.1 may be a second antimicrobial agent, thereby increasing the potency of the CAPH compounds of the present invention. Antimicrobial agents are well known in the art and the skilled artisan may link these antimicrobial agents to the compounds of the present invention using methods known in the art without undue experimentation. Presented as a non-limiting example, compound (II) illustrated kanamycin bound to a CAPH through a disulfide tether.

(15) ##STR00005##

(16) In another embodiment of the present invention, R.sub.2 and R.sub.3 may be, each independent of the other, alkyl or aryl substituents. These alkyl or aryl substituents may increase the hydrophobicity of the CAPH compounds of the present invention. In one embodiment, R.sub.2 and R.sub.3 may each independently be an alkyl substituent wherein the alkyl substituent may be straight chained, branched or cyclic. The alkyl substituent may further comprise heteroatoms or, in the case of cyclic alkyl substituents, may also further comprise fused ring structures. The alkyl substituents of the present invention may comprise from about 1 carbon to about 20 carbons, from about 2 carbons to about 15 carbons or from about 5 carbons to about 10 carbons. Non-limiting examples of alkyl substituents may be n-heptyl, n-pentyl, iso-pentyl, iso-heptyl, cyclohexyl or cyclooxyl. It will be appreciated that these examples are given by way of illustration and not meant to be limiting.

(17) In an alternate embodiment, R.sub.2 and R.sub.3 may be aryl substituents. Aryl substituents may be from about 5 carbons to about 8 carbons. The aryl substituents of the present invention may be heterocyclic and/or they may comprise substituents on the aryl ring. Substituents on the ring may be, but not limited to, alkyls (both straight chained and branched), alkoxy, hydroxyl, nitro, nitrile and other substituents known in the art. In one embodiment, the substituents may be electron donating or electron withdrawing. Non-limiting example of aryl substituents may be phenyl, methoxyphenyl or nitrophenyl.

(18) The present invention further provides dimeric structures of the compounds of the present invention comprising two molecules of compound (1) and wherein R.sub.1 is a linker.

(19) The present invention also provides a dimeric CAPH having the structure of compound (III):

(20) ##STR00006##

(21) wherein R.sub.1 is an alkyl substituent, the alkyl substituent being straight, branched or cyclic, an aryl substituent, a dye, a fluorophore, a conjugating agent or an antimicrobial agent; R.sub.2 and R.sub.3 are each independently, a hydrophobic alkyl or aryl moiety; n is from about 3 to about 10 and p is from about 1 to about 5. R.sub.1, R.sub.2, R.sub.3 and n are defined as for compound (I). In one embodiment, p may be from about 1 to about 5 or from about 1 to about 3. The length of the linker may not be critical for cellular internalization of compound (III). It will be appreciated that by linking together two molecules of compound (I), the overall hydrophobicity of the compound (III) is increased and may result in more effective subcellular localization over the monomeric form, compound (I).

(22) In another embodiment of the present invention there are provided antimicrobial compositions comprising compound (I), compound (III) or both. The antimicrobial compositions of the present invention may further comprise other antimicrobial agents, a carrier or buffer or any other compound commonly used in antimicrobial compositions. The antimicrobial compositions may be a solution, a suspension or a solid.

(23) The present invention also provides methods for treating a host cell having a microbial infection comprising the steps of administering compound (I), compound (II) or a mixture of both to the host cell having the microbial infection. It will be appreciated that there may be a mixture, for example but not limited to, of different compound (I) having different substituents. It will also be appreciated from the foregoing discussion that R.sub.1 may be chosen according to the microbial infection to be treated. Methods of the present invention further provide methods for treating a patient, either mammal or animal, having a microbial infection with the compounds of the present invention. The exact compound will depend on the microbial infection of the patient. The amount of compound to be administered will depend on the infection and the type and size of the patient. The amount to be administered may be determined by the skilled artisan without undue experimentation.

Examples

(24) Modifications to CAPHs were investigated in an effort to enhance cell penetration, to probe subcellular localization, and to determine the role of the hydrophobic group on the mechanism of cell entry. An alternative method was developed to incorporate the hydrophobic moiety into CAPHs to facilitate these studies. Previously an ether linkage had been used between the proline amino acid and the hydrophobic moieties (Scheme I). This was a successful approach for the development of CAPHs, but the ether-based approach limited the ability to prepare a diverse library of CAPHs quickly, as a new amino acid was needed for the synthesis of each peptide. To remedy this deficiency, and allow for the facile preparation of focused libraries of CAPHs, the use of an amide linkage between an amino-modified proline residue (PK) and the hydrophobic group was developed (Scheme I). In this way MTT protected PK residues were incorporated into a CAPH on resin, followed by on-resin deprotection of the MTT protecting group and acylation of the resulting amine with the desired carboxylic acid. Cleavage of the peptide from the resin provided a series of alkyl- and aromatic-modified CAPHs in parallel from the starting resin bound peptide (FIG. 1).

(25) The series of alkyl-modified CAPHs were evaluated for cell uptake. The n-heptyl- and cyclohxylmodified CAPHs (FIG. 1; P11KC7RR and P11KC6CRR) were the most effective, displaying approximately a 10- and 5-fold increase in HeLa cell penetration, respectively, at 10 M as compared to CAPHs previously reported in the literature. The subcellular localization of P11KC5RR and P11KC7RR was analyzed with HeLa cells at 5-15 M. P11KC5RR was mainly localized to endosomes at 5-10 M, but some mitochondrial localization was observed at 15 M. P11 KC7RR, on the other hand localized to the mitochondria at all concentrations analyzed, with some nuclear localization detected at 10-15 M.

(26) A series of aryl-modified CAPHs with varying electron donating or withdrawing groups was also investigated (H, NO.sub.2, OCH.sub.3, FIG. 1) to probe

(27) the effect of the electronic character of the phenyl moiety. These CAPHs all displayed enhanced cellular penetration, with 3- to 6-fold increases in cellular uptake over known compounds at 10 M. The CAPH containing the most electron-rich phenyl group appended to the PK residue, P11 KFOCH3RR, was the most effective. The subcellular localization in HeLa cells treated with 5-15 M of the three CAPHs was also investigated. These CAPHs were localized to endosomes at all concentrations, with P11KFNO2RR displaying some nuclear localization at 15 M. Overall, these data demonstrate that significant increases in cell penetration may be obtained through modifications to the hydrophobic moiety, using the newly developed synthetic strategy. Differences in subcellular localization were evident with the different types of hydrophobic groups, with alkyl chains favoring mitochondrial localization through direct transport, and the phenyl-modified CAPHs localizing to endosomes and the nucleus.

(28) Antimicrobial peptides (AMPs) are a class of antibiotics that generally act by targeting microbial cell membranes resulting in cell lysis. This mechanism of action is also one of the major drawbacks associated with clinical use of AMPs due to host cell toxicity. However, a small class of non-membrane lytic AMPs have been identified. Unifying features of these non-membrane lytic AMPs are a high proline content and an overall cationic charge due to high levels of arginine. Proline-rich AMPs (P-AMPs) are less toxic than membrane-lytic AMPs, but most P-AMPs do not enter mammalian cells.

(29) The interplay of structure and function for P-AMPs with idealized, de novo designed sequences has been investigated. P11LRR and P14LRR for antibacterial activity has been evaluated and a series of peptides starting with a sequence containing four copies of the PRP triad repeat found in natural P-AMPs, FI-PRP-4, and sequences with more cationic PRR-like triad (FI-PRR-4 and FI-PP.sub.RP.sub.R-4) has been designed in an effort to improve mammalian cell uptake. This latter sequence contains all proline-based residues, including the unnatural guanidinium-containing amino acid PR, but lacks the additional hydrophobic groups of P11 LRR and P14LRR. The CD spectrum of FI-PP.sub.RP.sub.R-4, P11 LRR and P14LRR each displayed a strong peak at 225 nm, characteristic of a PPII helix. FI-PRP-4 and FI-PRR-4, however, exhibited very weak maxima at 225 nm.

(30) The antibacterial activity of the five peptides was explored with E. coli and S. aureus. Two of the most cationic peptides (P14LRR and FI-PRR-4) were the most active against both bacterial strains (Table 1). Electrostatic interactions between cationic AMPs and the negatively charged bacterial membrane are believed to be the first step in antibacterial action, thereby explaining the improved antibacterial activity when going from P11 LRR (+4 charge) to P14LRR (+8 charge). Interestingly, restricting FI-PRR-4 to a rigid PPII conformation had a detrimental effect on activity, as seen with FI-PPRPR-4. However, the addition of hydrophobic isobutyl groups to the proline backbone of (P14LRR) resulted in a dramatic improvement in activity against both bacteria (Table 1). Replacing the fluorescein moiety in P14LRR with an acetyl group led to no discernible change in activity.

(31) TABLE-US-00001 TABLE 1 Antibacterial and hemolysis activity of designed P-AMPs E. coil S. aureus Hemolysis MIC.sup.[a] [M] MIC [M] [M] Fl-PRP-4 >100 >100 >100.sup. Fl-PRR-4 40 20 >100.sup. Fl-PP.sub.RP.sub.R-4 60 >100 >100.sup. P11LRR 60 60 >100.sup. P14LRR 4 12 >100.sup. Melittin 4.6 2.1 5.sup.[b] .sup.[a]The minimum inhibitory concentration (MIC). .sup.[b]Greater than 80% hemolysis was observed at this concentration.

(32) Importantly, the designed P-AMPs caused only low levels of damage to human red blood cells (hRBCs) (<5%) after 1 h of incubation up to a concentration of 100 pM (Table 1), whereas melittin was highly hemolytic at 5 'LIM. This lack of observed hemolysis with the designed P-AMPs is a crucial feature for potential applications. P14LRR was therefore identified as the most potent, non-hemolytic antibacterial among the designed proline-rich peptides. P14LRR also has potent broad-spectrum antibacterial activity against methicillin-resistant S. aureus (MRSA) (8 pM), B. anthracis (8 pM) and the biofilm-forming clinical-isolates of P. aeruginosa and S. aureus. P14LRR was further shown to inhibit the growth of Salmonella, Listeria and Brucella, all classified as intracellular pathogens.

(33) To rescue mammalian cells infected with intracellular bacteria, antimicrobial agents need to effectively penetrate within these host cells. The cell penetrating ability of all five peptides by flow cytometry with J774A.1 macrophage cells was evaluated. Macrophages are commonly invaded by intracellular bacteria and were thus selected for uptake studies. The three peptides (FI-PRR-4, FI-PPRPR-4, P14LRR) with the highest cationic charge (+8) showed significantly higher cellular fluorescence as compared to PII LRR (+6) and FI-PRP-4 (+4). The fluorescence associated with FI-PPRPR-4 uptake, however, was mostly due to cell surface binding. Among the most cationic peptides, there was approximately a four-fold increase in uptake in going from FI-PRR-4 to P14LRR. Thus among the designed P-AMPs, P14LRR was found to be most potently internalized within J774A.1 macrophage cells, without compromising the integrity of the cellular membranes. P14LRR was also found to satisfy two vital properties for application against intracellular bacteria: minimal toxicity towards J774A.1 macrophage cells and resistance to proteolytic degradation by trypsin.

(34) With a knowledge of the separate cell penetrating and antibacterial activities of P14LRR, the ability of this P-AMP to clear intracellular bacterial pathogens, Salmonella and Brucella, within J774A.1 cells has been investigated using an in vitro bacterial protection assay. Intracellular Salmonella and Brucella were significantly reduced by 62% and 90% with the addition of P14LRR, respectively.

(35) It should be understood, of course, that the foregoing relates to exemplary embodiments of the invention and that modifications may be made without departing from the spirit and scope of the invention as set forth in the following claims.