The present invention generally relates to the fields of medicine and molecular biology of infectious diseases. In particular aspects, the field of the invention relates to particular compositions and methods for the treatment of diseases, such as Human Immunodeficiency Virus (HIV), Mycobacterium tuberculosis (Mtb), Gram-positive and Gram-negative bacterial infections, as well as parasitic infections.
Infectious disease is the second leading cause of death worldwide, and the third leading cause of death in the United States of America. Particularly, Tuberculosis (TB) and Human Immunodeficiency Virus (HIV) remains the top two leading cause of mortality due to an infectious disease globally. The World Health Organization (WHO) estimates that of the 34 million cases of HIV, one third is also co-infected with latent tuberculosis. A lethal synergy exists between the two pathogens, Mycobacterium tuberculosis (Mtb) and HIV, which has led to the decline in the immune function of infected individuals and a rise in morbidity and mortality rates. Due to the emergence of drug resistant TB and HIV strains, drug-to-drug interactions, and increased drug toxicity, the therapeutic management of co-infected individuals remains a challenge.
A global rise in the incidence of multidrug-resistant (MDR), extensively drug-resistant (XDR), and totally drug-resistant (TDR) strains of M. tuberculosis and co-infected individuals has made it imperative to identify potent anti-mycobacterials with novel targets. While recent studies have provided important insights to the development of novel anti-bacterial and anti-viral drugs, discovery and development of a novel class of HIV-TB co-infection inhibitors that are efficacious and selective with improved pharmacologic profiles is vital. Therefore, anti-tuberculosis agents with a novel mechanism of action that also has an anti-HIV activity may help reduction in pill burden, reduction in the cost of treatment, and possibly increase patient compliance.
The prior art is deficient in the novel compositions and methods useful for the treatment of a variety of infectious diseases by developing selective anti-infective agents that shows selectivity for various Methionine aminopeptidases over human Methionine aminopeptidases. The present invention fulfills this longstanding need and desire in the art.
The present invention is directed to a formulation. The formulation comprises a hydroxyquinoline analog having a chemical structure,
In the structure the R1 substituent may be a halogen. R2 and R3 may be independently a halogen, OH or —OC(O)CH3, or R2 and R3 together form an N-substituted 1,3-oxazinanane. The hydroxyquinoline analog may be a pharmaceutically acceptable salt. The formulation comprises the hydroxyquinoline analog, a solvent, a co-solvent or a combination thereof and a surfactant. A related formulation further comprises saline or water or a combination thereof.
The present invention also is directed to a co-solvent formulation. The formulation comprises a hydroxyquinoline analog having a chemical structure,
The hydroxyquinoline analog may be formulated as a pharmaceutically acceptable salt and may be formulated with a co-solvent and at least 2 surfactants. A related formulation further comprises saline or water or a combination thereof.
The present invention is directed further to a method for treating an infectious disease in a subject in need thereof. The method comprises administering a pharmacologically effective amount of the formulation as described herein to the subject.
The present invention is directed further still to a method for quantifying a hydroxyquinoline analog in a sample. In the method the sample is obtained and in a chromatographic process the hydroxyquinoline analog in the sample and an internal standard are eluted. In a spectrometric process a peak area of the hydroxyquinoline analog and a peak area of the internal standard eluted from the sample are measured. A ratio of the peak area of the hydroxyquinoline analog to the peak area of the internal standard is calculated and the sample peak ratio is correlated to a known concentration of the hydroxyquinoline analog on a standard curve, thereby quantifying the hydroxyquinoline analog in the sample.
Other and further aspects, features, benefits, and advantages of the present invention will be apparent from the following description of the presently preferred embodiments of the invention given for the purpose of disclosure.
For a more complete understanding of the present invention, reference is now made to the following descriptions taken in conjunction with the accompanying drawings.
Methionine aminopeptidase (MetAP), a metalloprotease that catalyzes the removal of the initiating N-terminal methionine from proteins and polypeptides, is a promising and attractive drug target. N-terminal methionine excision is required for post-translational modifications, stability, localization and maturation of a large number of proteins and is therefore an essential process. In specific embodiments in this invention, small-molecule compounds and formulations, co-solvent formulations and pharmaceutical compositions thereof are evaluated as potent inhibitors of MetAP for targeting bacterial, viral and parasitic infections. The present invention also provides simple methods of quantifying the small molecule compounds in a sample, such as, but not limited to, a solution, a biofluid or other biological sample.
In one embodiment of the present invention, there is provided a formulation comprising a hydroxyquinoline analog having a chemical structure,
where R1 is a halogen; and R2 and R3 independently are halogen, OH or —OC(O)CH3, or R2 and R3 together form an N-substituted 1,3-oxazinanane; or a pharmaceutically acceptable salt thereof; a solvent, a co-solvent or a combination thereof; and a surfactant. Further to this embodiment the formulation comprises saline or water or a combination thereof.
In both embodiments, the hydroxyquinoline analog may be contained in the formulation in a concentration of about 1 mg/mL to about 2 mg/mL. Also in both embodiments, the solvent or co-solvent may be dimethyl sulfoxide (DMSO), dimethyl acetamide (DMA), highly purified diethylene glycol monoethyl ether (TRANSCUTOL), polyethylene glycol 400, Capric Triglyceride (LABRAFAC CC), propylene glycol monocapryrate type II (CAPYROL 90), ethanol, paraffin oil, soybean oil, olive oil or a combination thereof. In a representative example, the solvent or co-solvent is contained in the formulation in a concentration from about 5% to about 100%. In addition, the surfactant is polyoxyethylene sorbitan monooleate (TWEEN 80), Polyethylene glycol sorbitan monolaurate (TWEEN 20), Caprylocaproyl polyoxyl-8 glycerides (LABRASOL), propylene glycol monocapryrate type I (PGMC) or a combination thereof. In a representative example, the surfactants may be contained in the formulation in a concentration of about 5% to about 100%.
In one aspect of both embodiments, the solvent or co-solvent are dimethylacetamide and polyethylene glycol 400 and the surfactant is polyoxyethylene sorbitan monooleate. In a respresentative example of this aspect, the dimethylacetamide is contained in the formulation in a concentration of about 5% to about 30% and the polyethylene glycol 400 and the polyoxyethylene sorbitan monooleate are contained in said formulation in a concentration from about 10% to about 90%.
In another aspect, the solvent or co-solvent may be diethylene glycol monoethyl ether and polyethylene glycol 400 and the surfactant may be polyoxyethylene sorbitan monooleate. In a representative example of this aspect, the diethylene glycol monoethyl ether may be contained in the formulation in a concentration of about 5% to about 35% and the polyethylene glycol 400 and the polyoxyethylene sorbitan monooleate are contained in said formulation in a concentration from about 5% to about 90%.
In yet another aspect the formulation may comprise the hydroxyquinoline analog having the chemical structure
dimethylacetamide or diethylene glycol monoethyl ether; and polyethylene glycol 400 and polyoxyethylene sorbitan monooleate.
In a related embodiment, there is provided a co-solvent formulation, comprising a hydroxyquinoline analog having a chemical structure
or a pharmaceutically acceptable salt thereof; a co-solvent; and at least 2 surfactants. Further to this embodiment the formulation comprises saline or water or a combination thereof.
In one aspect of this related embodiment, the co-solvent may be dimethylacetamide in a concentration of about 5% to about 30% and the surfactants may be polyethylene glycol 400 and polyoxyethylene sorbitan monooleate in a concentration of about 10% to about 90%. In another aspect, the co-solvent may be diethylene glycol monoethyl ether in a concentration from about 10% to about 35% and the surfactants may be polyethylene glycol 400 and polyoxyethylene sorbitan monooleate in a concentration of about 10% to about 90%.
In yet another embodiment of the present invention, there is provided a pharmaceutical composition comprising the formulations as described supra and a pharmaceutically acceptable carrier.
In yet another embodiment of the present invention, there is provided a method for treating an infectious disease in a subject in need thereof, comprising administering to the subject a pharmacologically effective amount of the formulation as described supra to the subject, thereby treating the infectious disease. In this embodiment, the infectious disease may be HIV, tuberculosis, enterococcal or leishmaniasis. Also in this embodiment, the formulation increases bioavailability of the hydroxyquinoline analog.
In yet another embodiment of the present invention, there is provided a method for quantifying a hydroxyquinoline analog in a sample, comprising obtaining the sample; eluting, via chromatography, the hydroxyquinoline analog in the sample and an internal standard; measuring, via spectrometry, a peak area of the hydroxyquinoline analog and a peak area of the internal standard eluted from the sample; calculating a ratio of the peak area of the hydroxyquinoline analog to the peak area of the internal standard; and correlating the sample peak area ratio to a known concentration of the hydroxyquinoline analog on a standard curve, thereby quantifying the hydroxyquinoline analog in the sample.
In one aspect of this embodiment the eluting and measuring steps may comprise running in an isocratic mobile phase the sample and the internal standard through a high-performance liquid chromatography column with an ultraviolet-visible detector. In this aspect, the hydroxyquinoline analog contained in the sample is quantifiable in a concentration of about 1 μg/mL to about 200 μg/mL.
In another aspect of this embodiment the eluting and measuring steps may comprise running in a gradient mobile phase the sample and the internal standard through a a liquid chromatography column with a tandem mass spectrometry analyzer. In this aspect, the hydroxyquinoline analog contained in the sample is quantifiable in a concentration of about 1 ng/mL to about 5000 ng/mL.
In this embodiment and all aspects thereof, the hydroxyquinoline analog may have the chemical structure
where R1 is chlorine; and R2 and R3 independently are bromine, chlorine, OH or —OC(O)CH3, or R2 and R3 together form an N-substituted 1,3-oxazinanane; or a pharmaceutically acceptable salt thereof. A representative example of the hydroxyquinoline analog has the chemical structure
Also in this embodiment and its aspects the internal standard may be clioquinol. In addition the sample may be a solution, plasma or urine.
In yet another embodiment of the present invention, there is provided a method for treating an infectious disease in a subject in need thereof, comprising administering to the subject, in a pharmaceutically acceptable medium, a therapeutically effective amount of a methionine aminopeptidase inhibitor.
In one aspect of this embodiment, the methionine aminopeptidase inhibitor may be a quinoline having the chemical structure shown in Formula I:
where R1 is a halogen; and R2 and R3 independently are halogen, OH or —OC(O)CH3, or R2 and R3 together form an N-substituted 1,3-oxazinanane; or a pharmaceutically acceptable salt or a regioisomer thereof or a combination thereof.
In another aspect of this embodiment, the methionine aminopeptidase inhibitor may be a hydrazone having the chemical structure shown in Formula II:
where R4 is
and R5 is isonicotonyl group or
or a pharmaceutically acceptable salt thereof.
In yet another aspect of this embodiment, the methionine aminopeptidase inhibitor may be a quinone having the structure shown in Formula III:
where X is a halogen such as chlorine or bromine.
In yet another aspect of this embodiment, the methionine aminopeptidase inhibitor may have the chemical structure
In this embodiment and aspects thereof, the infectious disease may be Human Immunodeficiency Virus, Mycobacterium tuberculosis, a Gram-positive bacterial infection, a Gram-negative bacterial infection, a parasitic infection or a combination thereof. For example, the subject may be co-infected with Human Immunodeficiency Virus and Mycobacterium tuberculosis. An example of a parasitic infection is Leishmaniasis. In this embodiment and aspects thereof, the Gram-positive and/or Gram-negative bacterial infection may comprise a nosocomial infection.
Preferred compounds of present invention are 5-chloro-7-iodoquinolin-8-ol; 7-bromo-5-chloroquinolin-8-ol; 5,7-dichloroquinolin-8-ol; 5,7-dichloroquinolin-8-yl acetate; 6-chloro-3-cyclohexyl-3,4-dihydro-2H-[1,3]oxazino[5,6-h]quinolin; N-benzyl-5-chloro-N,6-dimethyl-2-(pyridin-2-yl)pyrimidin-4-amine; N′-((2-hydroxynaphthalen-1-yl)methylene)isonicotinohydrazide; 2-{(E)-[2-(5,6,7,8-tetrahydro[1]benzothieno[2,3-d]pyrimidin-4-yl)hydrazinylidene]methyl}phenol; 2,3-dichloronaphthalene-1,4-dione; or 2,3-dibromonaphthalene-1,4-dione.
In a related embodiment of the present invention, there is provided a method for treating an infectious disease in a subject in need thereof, the method comprising administering to the subject, in a pharmaceutically acceptable medium, a therapeutically effective amount of a methionine aminopeptidase inhibitor having the chemical structure shown in Formula II:
where R4 is
and R5 is isonicotonyl group or
or a pharmaceutically acceptable salt or a regioisomer thereof or a combination thereof.
In this embodiment the chemical structure of methionine aminopeptidase inhibitor may be:
In this embodiment, the infectious disease may be Human Immunodeficiency Virus, Mycobacterium tuberculosis or a combination thereof or a parasitic infection. Examples of Mycobacterium tuberculosis are Wild-type M.tuberculosis, dormant M. tuberculosis or multi-drug resistant M.tuberculosis. Also, in this embodiment, a therapeutically effective amount of the compound may selectively inhibit the bacterial methionine aminopeptidase over a human methionine aminopeptidase. In this embodiment, the selectivity for Mycobacterium tuberculosis methionine aminopeptidase over human methionine aminopeptidase may be about 20 fold to about 50 fold or more depending on the inhibitor. In one aspect the Mycobacterium tuberculosis methionine aminopeptidase is MtMetAP1a or MtMetAP1c. In another aspect the human methionine aminopeptidase is HsMetAP1 or HsMetAP2. In this embodiment and aspects thereof, the parasitic infection is Leishmaniasis and the methionine aminopeptidase is L.majorMetAP1 (LmMetAP1).
In yet another embodiment of the present invention, there is provided a method for treating an infectious disease in a subject in need thereof, the method comprising administering to the subject, in a pharmaceutically acceptable medium, a therapeutically effective amount of a methionine aminopeptidase inhibitor having the chemical structure of a quinoline:
where R1 is halogen; and R2 and R3 independently are halogen, OH, or —O(O)CCH3, or R2 and R3 together form an N-substituted 1,3-oxazinanane; or a pharmaceutically acceptable salt or a regioisomer thereof or a combination thereof.
In this embodiment the chemical structure of representative quinoline compounds are:
Also in aspects of this embodiment, the subject may be infected with a Gram-positive bacterium or a Gram negative bacterium or a combination thereof. An example of a Gram-positive bacterium is Enterococcus faecalis (E. faecalis). An example of a Gram-negative bacterium is Pseudomonas areuginosa. In these aspects the Gram-positive and Gram-negative bacterial infection independently may comprise a nosocomial infection. Examples of a nosocomial infection are a bacteremia, endocarditis, pneumoniasurgical site infections or a urinary tract infection. Particularly, the bacterium is a vancomycin-resistant Enterococcus (VRE) bacterium. In another aspect of this embodiment, the cells, tissue culture or subject may be infected with Human Immunodeficiency Virus or Mycobacterium tuberculosis or a combination thereof. In this embodiment and all aspects thereof, the methionine aminopeptidase may be E. faecalis MetAP1.
In yet another embodiment of the present invention there is provided a methionine aminopeptidase inhibitor having the chemical structure shown in compounds 1-10:
In all these embodiments and aspects thereof a person having ordinary skill in this art could readily determine a useful dose of a compound of the present invention depending upon the indication to be treated or the outcome desired. The compounds of the present invention showed minimum inhibitory concentrations (MICs) in the low micro molar range. Typically, the compound is administered in a dose ranging from about 0.05 μg/mL to about 50 μg/mL, preferably from about 0.2 μg/mL to about 10 μg/mL.
As used herein the specification, “a” or “an” may mean one or more. As used herein in the claim(s), when used in conjunction with the word “comprising”, the words “a” or “an” may mean one or more than one.
As used herein “another” or “other” may mean at least a second or more of the same or different claim element or components thereof. Similarly, the word “or” is intended to include “and” unless the context clearly indicates otherwise.
As used herein “Comprise” means “include.” In specific embodiments, aspects of the invention may “consist essentially of” or “consist of” one or more sequences of the invention, for example. Some embodiments of the invention may consist of or consist essentially of one or more elements, method steps, and/or methods of the invention. It is contemplated that any method or composition described herein can be implemented with respect to any other method or composition described herein.
The term “about” refers to a numeric value, including, for example, whole numbers, fractions, and percentages, whether or not explicitly indicated. The term “about” generally refers to a range of numerical values (e.g., +/−5-10% of the recited value) that one of ordinary skill in the art would consider equivalent to the recited value (e.g., having the same function or result). In some instances, the term “about” may include numerical values that are rounded to the nearest significant figure.
As used herein, the term “subject” shall refer to a human or other animal, for example, a mammal.
The term “halogen” includes iodine, bromine, chlorine and fluorine.
The term “substituted” shall be deemed to include multiple degrees of substitution by a substituent. A substitution occurs where a valence on a chemical group or moiety is satisfied by an atom or functional group other than hydrogen. In cases of multiple substitutions, the substituted compound can be independently substituted by one or more of the disclosed or claimed substituent moieties, singly or plurally. By independently substituted, it is meant that the (two or more) substituents can be the same or different.
The term “isomers” as used herein is a form of isomerism in which molecules with the same molecular formula have bonded together in different orders and have different structural formula. Position isomers are structural isomers in which a functional group or a substituent changes position on a parent structure.
The term “effective concentration (EC50)” as used herein is defined as the concentration at which 50% of the infected treated groups are statistically significantly different from the infected (DMSO) mock-treatment group (p<0.05).
The term “lethal concentration (LC50)” as used herein is defined as the concentration at which 50% of non-infected treated groups are statistically significantly different from the non-infected (DMSO) mock-treatment group (p<0.05).
The term “minimum protective concentration (MPC)” as used herein is defined as the minimum concentration required to obtain at least 25% survival of the nematodes.
The term “pharmaceutically acceptable salt” refers herein to a salt of a compound that possesses the desired pharmacological activity of the parent compound. Such salts include: 1) acid addition salts, formed with inorganic acids such as hydrochloric acid, hydrobromic acid, sulfuric acid, nitric acid, phosphoric acid, and the like; or formed with organic acids such as acetic acid, propionic acid, hexanoic acid, cyclopentanepropionic acid, glycolic acid, pyruvic acid, lactic acid, malonic acid, succinic acid, malic acid, maleic acid, fumaric acid, tartaric acid, citric acid, benzoic acid, 3-(4-hydroxybenzoyl)benzoic acid, cinnamic acid, mandelic acid, methanesulfonic acid, ethanesulfonic acid, 1,2-ethane-disulfonic acid, 2-hydroxyethanesulfonic acid, benzenesulfonic acid, 4-chlorobenzenesulfonic acid, 2-napthalenesulfonic acid, 4-toluenesulfonic acid, camphorsulfonic acid, 4-methylbicyclo[2.2.2]-oct-2-ene-1-carboxylic acid, glucoheptonic acid, 3-phenylpropionic acid, trimethylacetic acid, tertiary butylacetic acid, lauryl sulfuric acid, gluconic acid, glutamic acid, hydroxynapthoic acid, salicylic acid, stearic acid, muconic acid, and the like; or 2) salts formed when an acidic proton present in the parent compound either is replaced by a metal ion, e.g., an alkali metal ion, an alkaline earth ion, or an aluminum ion; or coordinates with an organic base such as ethanolamine, diethanolamine, triethanolamine, tromethamine, N-methylglucamine, and the like.
As used herein, “formulation” or “co-solvent formulation” refers to a solvent system or co-solvent system generally comprising one of the small molecule compounds provided herein, one or more solvents or co-solvents and at least one, preferably at least two, surfactants. The formulations and co-solvent formulations provided herein increase solubility and bioavailability of the small molecule compound.
The present invention also includes protected derivatives and analogs of compounds disclosed herein. For example, when compounds of the present invention contain groups such as hydroxyl, amine or carbonyl, these groups can be protected with a suitable protecting group. A list of suitable protective groups can be found in T. W. Greene, Protective Groups in Organic Synthesis, John Wiley & Sons, Inc. 1981, the disclosure of which is incorporated herein by reference in its entirety. The protected derivatives of compounds of the present invention can be prepared by methods well known in the art.
Pharmaceutical compositions of the present invention comprise an effective amount of one or more compositions of the invention (and additional agent, where appropriate) dissolved or dispersed in a pharmaceutically acceptable carrier. The phrases “pharmaceutical or pharmacologically acceptable” refers to molecular entities and compositions that do not produce an adverse, allergic or other untoward reaction when administered to a human or animal, as appropriate. The preparation of a pharmaceutical composition that contains at least one MetAP inhibitor or additional active ingredient will be known to those of skill in the art in light of the present disclosure, as exemplified by Remington's Pharmaceutical Sciences, 18th Ed. Mack Printing Company, 1990. Moreover, for animal (e.g., human) administration, it will be understood that preparations should meet sterility, pyrogenicity, general safety and purity standards as required by FDA Office of Biological Standards. As used herein, “pharmaceutically acceptable carrier” includes any and all solvents, dispersion media, coatings, surfactants, antioxidants, preservatives (e.g., antibacterial agents, antifungal agents), isotonic agents, absorption delaying agents, salts, preservatives, drugs, drug stabilizers, gels, binders, excipients, disintegration agents, lubricants, sweetening agents, flavoring agents, dyes, such like materials and combinations thereof, as would be known to one of ordinary skill in the art (see, for example, Remington's Pharmaceutical Sciences, 18th Ed. Mack Printing Company, 1990, pp. 1289-1329). Except insofar as any conventional carrier is incompatible with the active ingredient, its use in the pharmaceutical compositions is contemplated.
The MetAP inhibitors may be formulated into a composition in a free base, neutral or salt form. Pharmaceutically acceptable salts, include the acid addition salts, e.g., those formed with the free amino groups of a proteinaceous composition, or which are formed with inorganic acids such as for example, hydrochloric or phosphoric acids, or such organic acids as acetic, oxalic, tartaric or mandelic acid. Salts formed with the free carboxyl groups can also be derived from inorganic bases such as for example, sodium, potassium, ammonium, calcium or ferric hydroxides; or such organic bases as isopropylamine, trimethylamine, histidine or procaine. Upon formulation, solutions will be administered in a manner compatible with the dosage formulation and in such amount as is therapeutically effective. The formulations are easily administered in a variety of dosage forms such as formulated for parenteral administrations such as injectable solutions, or aerosols for delivery to the lungs, or formulated for alimentary administrations such as drug release capsules and the like.
Further in accordance with the present invention, the composition of the present invention suitable for administration is provided in a pharmaceutically acceptable carrier with or without an inert diluent. The carrier should be assimilable and includes liquid, semi-solid, i.e., pastes, or solid carriers. Except insofar as any conventional media, agent, diluent or carrier is detrimental to the recipient or to the therapeutic effectiveness of a the composition contained therein, its use in administrable composition for use in practicing the methods of the present invention is appropriate. Examples of carriers or diluents include fats, oils, water, saline solutions, lipids, liposomes, resins, binders, fillers and the like, or combinations thereof. The composition may also comprise various antioxidants to retard oxidation of one or more component. Additionally, the prevention of the action of microorganisms can be brought about by preservatives such as various antibacterial and antifungal agents, including but not limited to parabens, e.g., methylparabens, and propylparabens, chlorobutanol, phenol, sorbic acid, thimerosal or combinations thereof. In accordance with the present invention, the composition is combined with the carrier in any convenient and practical manner, i.e., by solution, suspension, emulsification, admixture, encapsulation, absorption and the like. Such procedures are routine for those skilled in the art.
In a specific embodiment of the present invention, the composition is combined or mixed thoroughly with a semi-solid or solid carrier. The mixing can be carried out in any convenient manner such as grinding. Stabilizing agents can be also added in the mixing process in order to protect the composition from loss of therapeutic activity, i.e., denaturation in the stomach. Examples of stabilizers for use in an composition include buffers, amino acids such as glycine and lysine, carbohydrates such as dextrose, mannose, galactose, fructose, lactose, sucrose, maltose, sorbitol, mannitol, etc.
In further embodiments, the present invention may concern the use of a pharmaceutical lipid vehicle compositions that include MetAP inhibitors, one or more lipids, and an aqueous solvent. As used herein, the term “lipid” will be defined to include any of a broad range of substances that is characteristically insoluble in water and extractable with an organic solvent. This broad class of compounds are well known to those of skill in the art, and as the term “lipid” is used herein, it is not limited to any particular structure. Examples include compounds which contain long-chain aliphatic hydrocarbons and their derivatives. A lipid may be naturally occurring or synthetic (i.e., designed or produced by man). However, a lipid is usually a biological substance. Biological lipids are well known in the art, and include for example, neutral fats, phospholipids, phosphoglycerides, steroids, terpenes, lysolipids, glycosphingolipids, glycolipids, sulphatides, lipids with ether and ester-linked fatty acids and polymerizable lipids, and combinations thereof.
One of ordinary skill in the art would be familiar with the range of techniques that can be employed for dispersing a composition in a lipid vehicle. For example, the MetAP inhibitor or derivative thereof may be dispersed in a solution containing a lipid, dissolved with a lipid, emulsified with a lipid, mixed with a lipid, combined with a lipid, covalently bonded to a lipid, contained as a suspension in a lipid, contained or complexed with a micelle or liposome, or otherwise associated with a lipid or lipid structure by any means known to those of ordinary skill in the art. The dispersion may or may not result in the formation of liposomes.
Any of the compositions described herein may be comprised in a kit. In a non-limiting example, the kit comprises a composition suitable for treatment and/or prevention of one or more infectious diseases. In other embodiments of the invention, the kit comprises one or more apparatuses to obtain a sample from an individual. Such an apparatus may be one or more of a swab, such as a cotton swab, toothpick, scalpel, spatula, syringe, and so forth, for example. In another embodiment, an additional compound is provided in the kit, such as an additional compound for treatment and/or prevention of a infectious disease. Any compositions that are provided in the kits may be packaged either in aqueous media or in lyophilized form, for example. The container means of the kits will generally include at least one vial, test tube, flask, bottle, syringe or other container means, into which a component may be placed, and preferably, suitably aliquoted. Where there are more than one component in the kit, the kit also will generally contain a second, third or other additional container into which the additional components may be separately placed.
The following examples are included to demonstrate preferred embodiments of the invention. It should be appreciated by those of skill in the art that the techniques disclosed in the examples which follow represent techniques discovered by the inventor to function well in the practice of the invention, and thus can be considered to constitute preferred modes for its practice. However, those of skill in the art should, in light of the present disclosure, appreciate that many changes can be made in the specific embodiments which are disclosed and still obtain a like or similar result without departing from the spirit and scope of the invention.
A primary high throughput screen was conducted using MAP-C2 microplate processor (Titertek Instruments, Inc., Huntsville, Ala. USA). A library of 175,000 compounds at 30 μM were assayed in a 384 well plates using a dipeptide chromogenic substrate, methionine-proline coupled to p-Nitroaniline (Met-Pro-pNA). Each compound was dissolved in DMSO and stored at −20° C. until use. The total reaction volume was 50 μL, and each reaction contained 40 mM HEPES buffer (pH 7.5), 100 mM NaCl, 100 mg/mL BSA, 0.1 U/mL ProAP, 1.5 mM CoCl2, 600 mM substrate (Met-Pro-pNA), and 252 nM MtMetAP1c. The enzyme was pre-incubated with compounds for 20 minutes at room temperature followed by addition of 600 mM substrate. The reaction was then incubated at room temperature for 30 min and monitored at 405 nm on a spectrophotometer. Compounds that showed greater than 30-40% inhibition were chosen as “hits”.
The concentration needed for 50% enzyme inhibition (IC50) was determined in 96-well plates at final concentrations ranging from 100 μM to 300 nM for MetAP inhibitors. The enzyme was pre-incubated with compounds for 20 minutes at room temperature followed by addition of substrate. The reaction was incubated at room temperature for 30 min and monitored at 405 nm on a spectrophotometer. The background hydrolysis was subtracted and the data was fitted to a four-parameter logistic (variable slope) equation using GraphPad Prism software.
The HIV isolate used in this study was a dual tropic (R5 and X4) strain (HIV-1 89.6), received gratis from Dr. Monique Ferguson (UTMB Galveston). A Mycobacterium bovis (M. bovis) BCG strain expressing a red fluorescent protein (tdtomato, with a spectrum similar to Texas Red) was received from Dr. Jeffrey Cirillo (Texas A&M Health Sciences Center). M. bovis BCG working stock used for the studies were cultured using standard BCG growth media which was made from DIFCO 7H9 Broth (Becton Dickinson, San Diego, Calif.). Briefly, cultures were grown in a shaker at 100 rpm, 37° C. for 10-14 days and kanamycin (50 ng/ml) was added to the stock once in 5 days to maintain the plasmid expressing tdtomato. When the OD value of the growing stock reached 0.8-1.0, the stocks were frozen in the storage medium (long term storage) or PBS (for infections) at −80° C.
Peripheral blood was obtained from healthy donors as approved by the UTMB Institutional Review Board. Peripheral blood mononuclear cells (PBMC) were isolated from heparinized peripheral blood using Accuprep (Accurate chemicals, New York, N.Y.) and density centrifugation. An RBC Lysis buffer (Sigma, St. Louis, Mo.) was used to remove any remaining red blood cells according to the manufacturer recommendation. Cell viability of the isolated PBMC population was determined by using trypan blue exclusion and by flow cytometry using the live/dead aqua cell viability assay (Invitrogen, New York, N.Y.). Cells were cultured in cRPMI at 106 cells/ml of media in 5% CO2 at 37 C (Hogg et al. J Leukoc Biol, 86:1191, 2009). In some experiments, peripheral blood monocytes were isolated by magnetic bead-conjugated antibody separation using AutoMacs (Gonzales et al. Infect Immun, 80:234, 2012) and used to derive macrophages following 5-6 days of culture with 50 ng/ml of recombinant human M-CSF.
The mAbs against FITC-conjugated HIV p24 was purchased from Beckman Coulter (Indianapolis, Ind.). Following infection and treatment, PBMC or monocyte-derived macrophages were harvested at appropriate time points for flow cytometric analysis. After harvest, cells were incubated with CD16/CD32 Fc Block (BD Biosciences, San Jose, Calif.) to reduce non-specific binding of antibodies. Cells were permeabilized using the BD Cytofix/Cytoperm kit (BD Pharmingen, Calif.), then labeled with a FITC-conjugated antibody specific to HIV-1 (KC-67, Beckman-Coulter) as previously described (Hogg, et al. 2009). Samples were finally incubated for 48 hours in 4% formaldehyde (Polysciences Inc, Warrington, Pa.) and diluted in PBS prior to acquisition. A total of 50,000 gated events, based on expected leukocyte side scatter/forward scatter characteristics, were collected using a BD LSR II (Fortessa) flow cytometer (BD Biosciences). Analysis of data was performed by FCS Express 4 (De Novo, Los Angeles, Calif.) software. To control for background and to establish thresholds for gating positive cells, an isotype-matched FITC-labeled antibody was used.
The levels of secreted HIV p24 in culture supernatants of purified CD14+ or PBMC was measured at day 7 using an ELISA kit purchased from Zeptometrix (Buffalo, N.Y.). Secreted protein was converted to pg/ml based on the standard curve generated from known p24 standards included in the kit as recommended by the manufacturer
Cells were disrupted with 0.067% SDS and lysates used to determine bacterial growth following culture with control or standard compounds. The bacterial load was measured by colony forming unit (CFU) enumeration by limiting dilutions and determining growth on selective agar (7H11).
Peripheral blood mononuclear cells (PBMC) were isolated from healthy human volunteers and cultured in cRPMI. The PBMC cells were stimulated with PHA-P for 1-3 days. The cells were plated in a 24 well plate and infected with HIV-1 (89.6 strain) for 24 hours at 30° C. and 5% CO2. The cells were washed with antibiotic free cRPMI media to remove extracellular HIV p24 antigen. MetAP inhibitor (Compounds 1 to 8) was added to the 24 well plate at final concentrations ranging from 30 μM to 300 nM to give a total assay volume of 1 mL. The cells were incubated at 30° C. and 5% CO2 for 7 days. The cells were harvested and the supernatant was analyzed for the amount of p24 antigen using the RetroTek HIV-1 p24 ELISA kit (Zeptometrix, Buffalo, N.Y.). Azidothymidine (AZT, 10 μM), DMSO, and a blank (drug free) were used as controls in this experiment.
Determination of Minimum Inhibitory Concentration in Replicating M. tuberculosis
Compounds were serial diluted in DMSO and added to 7H9 broth, 2% Glycerol, 0.05% Tween 80, and 10% albumin/dextrose complex (ADC) at final concentrations ranging from 50 μg/mL-0.05 μg/mL. A culture of M. tuberculosis CDC 1551 was grown till O.D.=1.0 and a 1/100 dilution is done. The tubes containing the test agent with 0.1 mL of bacterial culture was inoculated yielding a total assay volume of 5 mL. DMSO (negative control), Isoniazid (positive control), and drug free media (blank) were used as controls to determine minimum inhibitory concentration of the compounds.
Activity Against Dormant M. tuberculosis
The activity of the compounds in aged non-growing M. tuberculosis was achieved using a perister model at concentrations 0.5 to 100 mM and monitored for three weeks. Briefly, 2 month old M. tuberculosis H37Ra culture was grown in 7H9 medium (Difco) with 10% albumin dextrose catalase (ADC) and 0.05% Tween 80. The bacterial culture is then resuspended in 7H9 medium (pH 5.5) without ADC and an innocula was used for determining the activity of the compounds (e.g. 2-hydroxy-1-naphthylaldehyde isonicotinoyl hydrazone) for persister bacilli. The compound was diluted from a 10 mM (in DMSO) to 10 μM (final concentration) and incubated with the bacilli in 200 mL 7H9 medium (pH 5.5) without ADC in a 96-well plate for three days without shanking under 1% oxygen in a hypoxic chamber. This assay was performed in duplicates with Rifampin (5 mg/mL). Following a 3 day drug exposure, bacilli viability was determined by adding 20 mL of 1 mg/mL of XTT (2,3-bis-(2-methoxy-4-nitro-5-sulfophenyl)-2H-tetrazolium-5-carboxanilide) and incubated at 37° C. for up to 7 days. The 96 well plates were then read at OD 485 nm.
2-hydroxy-1-naphthylaldehyde isonicotinoyl hydrazone (1) is known to inhibit HIV-1 transcription with IC50=2 μM by inhibiting proteins necessary for the cell cycle progression (Debebe et. al. 2007). Serendipitously 2-hydroxy-1-naphthylaldehyde isonicotinoyl hydrazone was identified in the M. tuberculosis screen and found that it also inhibited the production of HIV-1 p24 antigen in a dose response manner (
Inhibitory effects of compounds 2, 3, 5, 6, and 7 on HIV-1 infectivity was investigated by quantifying the level of p24 antigen produced using the ELISA (
Selectivity of 2-hydroxy-1-naphthylaldehyde Isonicotinoyl (1) Hydrazone for MtMetAP Enzymes over HsMetAPs
2-hydroxy-1-naphthylaldehyde isonicotinoyl (1) hydrazone inhibited MtMetAP1a and MtMetAP1c having IC50 values in the lower micro molar concentrations (Table 2). Further, compound 1 showed greater selectivity for MtMetAPs in comparison to HsMetAP1 and HsMetAP2. Compound 1 has at least 50 fold selectivity for MtMetAPs than HsMetAP1 and at least 20 fold selectivity for MtMetAPs than HsMetAP2. The selectivity for the MtMetAPs over HsMetAPs emphasizes the potential of compound 1 to selectively target the pathogen without leading to toxic effects for the host. It has been established in recent years that HIV-1 uses host molecular machinery for the N-terminal modification of several viral proteins. One such modification is the N-myristoylation of Nef, a HIV-1 accessory protein. Myristic acid is added to the protein by human N-myristoyltransferase-1 (NMT1). However, for NMT1 to carry out this process, MetAP must catalyze the removal the initiation methionine. Without the myristoylation of Nef by NMT, optimized viral replication and AIDS progression can be hindered. Therefore, finding one drug that targets MetAP can be effective in the suppression of HIV and TB leading to developing novel anti-infectives for the therapeutic management of co-infected individuals.
Minimum Inhibitory Concentration of MetAP Inhibitors on Replicating M. tuberculosis
The effect of the compound 1 in replicating M.tuberculosis culture was determined. The Minimum Inhibitory Concentration (MIC) was found to be less than 10.0 μg/mL (Table 1). The potency of compound 1 was agreeable to the relative activity against MtMetAP1a and MtMetAP1c in culture. Similarly, the potent effects of compound 2 in replicating M.tuberculosis culture and the Minimum Inhibitory Concentration (MIC) was determined to be less than 10.0 μg/mL. (Table 2). The potent effects of compound 3 in replicating M.tuberculosis culture and the Minimum Inhibitory Concentration (MIC) was determined to be less than 5.0 μg/ml.
Effects of 2-hydroxy-1-naphthylaldehyde Isonicotinoyl Hydrazone Against Dormant M. tuberculosis and Multi-Drug Resistant Tuberculosis
Minimum Inhibitory Concentration (MIC) of compound 1 and compound 2 on aged non-growing M. tuberculosis was determined (Table 2). At concentration of 1.82 μg/mL, compound 1 perturbed the growth of aged non-growing Mtb bacilli and inhibited the color development of redox dye XTT. Inhibitory effects of compounds 1-6, 9 and 10 on drug resistant strain M. tuberculosis HN 3409 in vivo were conducted for 29 days and the first preliminary results are outlined in Table 3 (these set of experiments are currently being repeated). The standards used for comparison where Linezolid and Kanamycin both at 5 μg/mL.
M. tuberculosis Strain H37Ra
An in vitro co-infection model for application to discovery of novel compounds for treatment of TB was developed. As outlined in
As shown in
Intracellular infection with M. bovis BCG in PBMC cultures exposed to live mycobacterium was further studied (
In order to perform high throughput analysis of various compounds by using the model developed herein, the screening assays were optimized using commercially available cell viability reagent (Invitrogen, fixable aqua live/dead viability marker) as shown in
In samples from 2 donors, cellular viability using the standard tyrpan blue exclusion test was additionally determined. M. bovis BCG infection promotes greater cell death in cultures and co-infection with HIV exacerbates this effect in some donors. The toxicity of various compounds in addition to pathogen cytotoxicity can be further determined as demonstrated with standard TB and HIV drug. These toxicity and drug interactions issues are high priority considerations in TB/HIV endemic areas (McIIIeron, et al. 2007).
The live/dead marker shown in
As shown in
Cloning of LmMetAP1 in p1RIHYG Expression Vector
The LmMetAP1 gene was amplified from L. major genomic DNA using the oligonucleotides LmMetAP1-XbaI sense (5′-TCTAGAGGATCCATGCCCTGCGA AGGCTGCGGC-3′; SEQ ID NO: 1) and LmMetAP1-XbaI antisense (5′-TCTAGAGAATTCTCAGATTTTGATTTCGCTGGGGTCTTCGG-3′; SEQ ID NO: 2) primers. Polymerase chain reaction (PCR) was performed using PCR master mix (Promega, Madison, Wis.), 420 ng of L. major genomic DNA and LmMetAP1-sense and -antisense primers under denaturation of 5 minutes at 95° C., followed by 40 cycles of 60 seconds at 95° C., 60 seconds at 68° C., and 90 seconds at 72° C.; a final 5 minute elongation period at 72° C. was performed. The PCR product was ran in a 0.8% agarose gel and purified using Wizard SV Gel and PCR Clean-Up System (Promega, Madison, Wis.). The amplified LmMetAp1 gene was then cloned into p1RIHYG expression vector by first digesting p1RIHYG expression vector with Xba I restriction enzyme and then ligating the amplified LmMetAp1 gene and transformed into DH5α E. coli. Colonies were grown in 5 mL of Terrific Broth (TB) liquid media for 18 hours and plasmid DNA from bacterial pellets was collected using QlAprep Spin Miniprep Kit (Qiagen, Valenica, Calif.). The clones were sequenced (by the DNA Analysis Core Facility, Border Biomedical Research Center, El Paso, Tex.) and confirmed using Basic Local Alignment Search Tool (BLAST) and Multiple Sequence Alignment by CLUSTALW.
Promastigote forms of L. major strain Friedlin clone V1 expressing firefly luciferase were grown in M199 medium supplemented with hemin and 10% fetal bovine serum (FBS) inactivated at 56° C. for 30 minutes and treated with 50 ng/mL streptothricin neosulfate for maintenance of LUC gene.
Leishmania major Luciferase Assay
Compounds were screened against L. major strain friedlin clone V1 promastigotes expressing firefly luciferase at concentrations ranging from 100 μM-780 nM in a 96 well plate. These experiments were done in triplicates using L. major media and 106 parasites per well. The plates were incubated for 24, 48, 72 and 96 hours at 28° C. Amphotericin B (AB) was used as a positive control at 5 μM as a comparison to the leishmanicidal activity of the inhibitors. The inhibitory effects of the compounds were assessed by monitoring parasite survival through luciferase activity. The substrate 5′-fluoroluciferin (ONE-Glo Luciferase Assay System, Promega, Madison, Wis.) was added according to the manufacturer's protocol after each time point. The plates were read using a luminometer (Luminoskan, Thermo Scientific, Rockford, Ill.). Data was analyzed using GraphPad Prism Software (GraphPad Software, Inc., La Jolla, Calif.). The compounds that showed >90% inhibition were chosen as “hits.”
Inhibitors that produced effective antiparasitic activity in L. major were further tested in the mammalian cell lines RAW 264.7 murine macrophages, U205 human osteoblasts as well as in intraperitoneal mouse macrophages. For the cell lines, cells were plated as 105 cells per well in a 96 well plate where previously diluted compounds ranging in concentrations from low nM up to 20 μM were transferred. The cells were incubated for 96 hours at 37° C. Intraperitoneal mouse macrophages were plated at a density of 106 cells per well in a 96 well plate and were incubated for 8 hours at 37° C. Compounds were diluted in a separate 96 well plate in triplicate and then transferred to the plate containing the murine intraperitoneal macrophages. Together, the compounds and cells were incubated for 24 hours.
Mammalian cell cytotoxicity of the compounds was analyzed by monitoring the reduction of the growth medium serving as an indicator of metabolic activity. After each time point, AlamarBlue reagent (Invitrogen, Carlsbad, Calif.) was added according to the manufacturer's protocol. The plates were read using a fluorometer (Flouroskan, Thermo Scientific, Rockford, Ill.). Data was analyzed using GraphPad Prism Software (GraphPad Software, Inc., La Jolla, Calif.).
A chemical genetic approach was used to elucidate the function and relevance of methionine aminopeptidase 1 in Leishmania major. The study was begun using a whole cell based approach and three pharmacophores were identified as methionine aminopeptidase inhibitors (
In order to confirm that the inhibitors were targeting LmMetAP1, a genetic approach was investigated. Overexpression of LmMetAP1 in vivo would cause resistance to the inhibitors if indeed the target was methionine aminopeptidase 1 (
L. major
L. major
Sub-Cloning MetAP from E. faecalis
N-terminal poly-His-tag EtMAP1 was amplified by PCR from E. faecalis genomic DNA using Taq polymerase. The primers used were 5′-GCGGGATCCATTACATTAAAATCACCAC-3′ (SEQ ID NO: 3) and 5′-GCGCTCGAGTTAATAAGTCAATTCTC-3′ (SEQ ID NO: 4) for forward and reverse direction respectively. The PCR product was cloned into pET28a, using the BamH I and Xho I restriction sites respectively. The EfMetAP1 clone was verified by sequencing.
Over-Expression and Purification of Recombinant MetAP1 from E. faecalis
E. coli cells (BL21) containing the expression plasmid were cultured at 37° C. in 1 Liter of Listeria Broth (LB) containing 30 mg kanamycin until OD600 reached about 0.6-0.7. Thereafter, expression was induced by addition of isopropyl β-D-galactoside (IPTG) to a final concentration of 1 mM vibrating at 37° C., and 275 rpm for 4 hrs. The cells were harvested and washed with 1× PBS (137 mM NaCl, 2.7 mM KCl, 4.3 Na2HPO4.7H2O, 1.4 mM KH2PO4). The cells were sonicated 4 times for 12 s in 1×PBS with 0.2% Triton −X-100 and EDTA-free Protease Inhibitor tablets. The resulting mixture was centrifuged at 8000 g for 10 mins. The supernatant was loaded unto pre-equilibrated (1×PBS) Talon beads. After binding for 30 min the beads were washed three times with basic buffer (10 mM Hepes pH 8.0, 100 mM KCl, 1.5 mM MgCl2, 10% glycerol). The enzyme was eluted with 75 mM Imidazole in Basic buffer. The protein was quantified using the Bradford assay. The average yield for EfMetAP1 was 38.63 mg/L of culture respectively (
Biochemical Characterization of MetAP from E. faecalis
The kinetic constants of recombinant EfMetAP1 was determined using a coupled methionine-proline aminopeptidase assay (Zhou et al., Anal Biochem. 280(1):159-65, 2000). The substrate used in this assay is a dipeptide, Methione-Proline coupled to p-Nitroaniline. The kinetic constants were obtained by varying substrate concentrations from 0 μM to 800 μM measuring the resulting enzyme activity. The reactions were carried out in 96-well plates at room temperature and monitored at 405 nm on a spectrophotometer. The total reaction volume was 50 μL and each reaction contained 40 mM Hepes buffer (pH 7.5), 100 mM NaCl, 10 μM CoCl2, 100 μg/mL BSA, 0.1 U/mL ProAP, 0-800 μM substrate (Met-Pro-pNA), and 2.4 μM EfMetAP1 respectively. The background hydrolysis was corrected and the data was fitted against the Michealis-Menten equation: V=Vmax x [S]/(Km+[S]) using the Graphpad prism software for one-site binding hyperbola (
EfMetAP1 activity was determined at different temperatures from 4° C. to 65° C. (
The reactions were carried out in 96-well plates at room temperature by measuring the activities of recombinant EfMetAP1 using different buffers. The total reaction volume was 50 μL and each reaction contained buffer (50 mM sodium acetate pH 4.0-5.5, 50 mM MES pH 5.5-7.0, 50 mM HEPES pH 7.0-8.5, 50 mM Tricine pH 8.0-9.0 and 50 mM Ethanolamine pH 8.5-10.0), 10 mM NaCl, 1 μM CoCl2, 100 μg/mL BSA, 0.1 U/mL ProAP, 600 μM substrate (Met-Pro-pNA), and 2.38 μM EfMetAP1 (
After purification, recombinant EfMetAP1 was dialyzed into buffer C (50 mM Hepes buffer pH 7.0, 10 mM NaCl and 5 mM EDTA) at 4° C. overnight and the buffer was exchanged to buffer D (50 mM Hepes buffer (pH 7.0), and 10 mM NaCl) at 4° C. The metal dependence of EfMetAP1 was determined by measuring enzymatic activity in the presence of 1 μM-10 mM CoCl2 (
175,000 compounds were screened against EfMetAP1, using the coupled methionine-proline aminopeptidase spectrophotometric assay (
The effect of EfMetAP inhibitors against Enterococcus faecalis, Enteroccocuss faecium, Bacillus anthracis, Staphylococcus aureus, Listeria monocytogenes and Streptococcus pyogenes was determined. The primary screen was conducted with 102 compounds at 32 μg/mL. The compounds were dissolved to give a final concentration of 32 μg/mL in 17 mL molten agar, 2 mL compound solution (320 μL of 2 mg/mL compound in 1.68 mL water) and 1 mL sheep blood. The plates were poured at 45° C. and left overnight. The plates were inoculated with each bacterial strain in triplicates and allowed to dry at room temperature for 1 hr then incubated for 24 hr and scored respectively on the next day.
Assay of E. faecalis Inhibition
To determine the Minimum Inhibitory Concentration (MIC) of E. faecalis, bacterial culture strains OG1Rf, V583 and PMV 158 were grown in Brain Heart Infusion (BHI) culture by incubating overnight at 37° C. Initial Optical density (OD) reading was taken and culture was normalized to 1×106 cells; A600=0.6. Serial dilutions of the respective compounds were performed and 5 μl of each concentration was plated on to 96-well plates (Fisher brand, Becton Dickson Microtest tissue culture plate #353072) with 45 μl of BHI containing 5 μl of E. faecalis (three wells per condition). Initial reading is taken at OD600 using a SpectraMax Gemini XPS plate reader (Molecular Devices, Sunnyvale, Calif.). The plate was incubated for 24 hr at 37° C. after which the final reading was taken at OD600. Kaplan-Meier log rank analysis was used to compare survival curves pairwise. P values of <0.05 were considered to be statistically significant. The software GraphPad Prism (version 5.0) was used for the analyses.
Liquid-Based Assay Using C. elegans as an Animal Model of Infection
In order to determine the Minimum Protective Concentration (MPC), synchronized glp-4;sek-1 worms were obtained from gravid adults by incubating eggs overnight in M9 buffer at 25° C. The L1-stage nematodes were hatched and plated on lawns of Nematode Growth (NG) agar media containing E. coli. Nematodes were further incubated to grow to sterile L4 larvae which are washed and then transferred onto lawn of E. faecalis grown on BHI agar plates, containing 50 μg/mL gentamycin, incubated for 5 hr at 25° C. and re-suspended in M9 buffer. Control and infected worms were transferred without agitation to 6-well plates containing 80% M9 buffer and 20% BHI plus 20 μl of compound to give a total volume of 2 mL per well (30 worms per condition). The plates were incubated at 25° C. and worms were scored daily for survival by shaking the plate and observing under a surgical microscope for motion. Dead worms did not move and exhibited rigid muscle tone. Based on this experiment it was determined if the compounds were also toxic to the worms as well as the efficacy. Kaplan-Meier log rank analysis was used to compare survival curves pairwise. P values of <0.05 were considered to be statistically significant. The software GraphPad Prism (version 5.0) was used for the analyses.
Assessment of Bacterial Viability after Treatment in Vivo
Young Adult nematodes sequentially preinfected with E. faecalis for 5 h. The nematodes were washed three times with sterile M9W and collected by centrifugation between each wash and then transferred into tubes. The wash was repeated twice using 25 mM Tetramisole hydrochloride and the supernatant was removed leaving about 50 μl. 500 μl of 25 mM tetramisole hydrochloride, 1 mg/mL of ampicillin and kanamycin are added to the tube and nematodes were incubated for 1 h to kill off excess bacteria. The nematodes were washed twice in 25 mM Tetramisole and transferred to 6 well plates containing 20% BHI and the inhibitors to recover for 48 h and 72 h. After recovery time elapsed, nematodes were then transferred into an eppendorf tube containing 200 μl of M9 and ground using motorized pestle for 1 min and tube was briefly vortexed. Ground worms were diluted and plated on BHI agar containing 10 μg/mL of Gentamycin and incubated at 37° C. for 24 h after which CFUs were counted.
Characterization experiments using the enzyme assay conditions were carried out to determine the kinetic constant, metal dependence and the effects of temperature and pH on the enzyme. The kinetic constant for EfMetAP1 was determined by measuring enzyme activity at different substrate concentrations ranging from 0 to 800 mM (
The metal dependence of EfMetAP1 using Co2+ and Mn2+ as the cofactors was investigated. The metal screen was performed by varying the metal concentration used from 0 to 10,000 μM. EfMetAP1 showed a broad range of activity, from 10 to 100 μM, in Mn2+ with a slight decrease in relative activity at higher concentrations (
E. faecalis using a dipeptide substrate (Met-Pro-pNA)
Small molecule library of 175,000 compounds against EfMetAP1 at a final concentration of 30 μM in 384-well plates using a coupled enzymatic assay was screened and 7-bromo-5 chloroquinolin-8-ol 5 was identified as an inhibitor of EfMetAP1. In order to investigate the structure-activity relationships, other structural analogs are acquired (Table 6). It was discovered that substitutions to the ortho-bromine of compound 5 for 3-cyclohexyl-1,3-oxazinan-3-ium increased enzyme activity whereas substitution of the ortho-bromine position for iodine reduced the IC50. A reduction in IC50 was also observed when the hydroxyl group of compound 5 was substituted for an acetoxy group and the ortho-bromine substituted for chlorine. Among all inhibitors tested, compound 8 was found to be most potent against EfMetAP1 enzyme with IC50 value of 5.24 μM (Table 6).
Inhibition of E. faecalis Growth in Vitro by EfMetAP1 Inhibitors
Five inhibitors were tested for their effects on E. faecalis growth in culture to obtain the minimum inhibitory concentrations (MICs). Compounds 5 and 6 were more potent against the clinical OG1RF strain of E. faecalis, achieving MIC30 between the ranges of 2.5-5.0 μg/mL, while the other three analogues had MIC30 values between the ranges of 5.0-10.0 μg/mL. Compound 5, compound 6 and compound 7 achieved MIC30 between the ranges of 0.25-0.5 μg/mL against the V583 strain, while compound 4 and compound 8 achieved MIC30 between the ranges of 0.5-1.5 μg/mL. All inhibitors were between six to ten times more potent against the V583 than the OG1 RF strain (Table 7).
Assessment of Cytotoxicity and Efficacy of EfMetAP1 Inhibitors in a C. elegans Animal Model
Toxicity and efficacy of EfMetAP1 inhibitors was assessed using C. elegans animal model. The toxicity of the inhibitors was first determined by exposing non-infected animals to different concentrations. Controls included the addition of 10 μg/mL of tetracycline, an antibiotic approved for human use at a concentration that is non-toxic and protective against infection in the worm model as a positive control and DMSO, the vehicle used to dissolve and deliver the EfMetAP1 inhibitors as a negative control. The controls did not decrease survival of the non-infected animals compared to no addition as shown in
To test if non-toxic concentrations of the EfMetAP1 inhibitors were capable of protecting C. elegans from infection, animals infected with E. faecalis OG1RF are exposed to concentrations of inhibitors ranging from 4×10−12 μg/mL to 32 μg/mL. Surprisingly, for compound 5 concentrations ranging from 4×10−5 μg/mL to 4×10−4 μg/mL the animals survived just as well, or better, than animals treated with tetracycline (
The effect of compound 5 and its analogues on animals infected with V583 was also examined. As shown in
It is proposed that Compound 5 and its analogues are conferring protection at such low concentrations due to one or a combination of the following reasons: First, they may confer protection by activating stress response pathway that releases cytoprotective proteins. Studies have shown that C. elegans responds to oxidative stresses caused by xenobiotics and metal toxicants by activating the Antioxidant Response Element (ARE) via the Nrf2 pathway. The Nrf2 orthologue in C. elegans SKN-1 has been shown to induce expression of ARE by structural relative of the inhibitors; Napthoquinolones which resulted lifespan extension in C. elegans (Hunt=[59]). Interestingly CQ has been shown to be a zinc ionophore (Ding=[60]) and that sub cytotoxic levels of zinc are able to induce expression of HO-1 (Xue=[61]). HO-1 is a cyto protective enzyme that responds by decreasing oxidative stress, weakened inflammatory response and lower apoptosis rate (loboda=[62]).
Secondly by acting as an ionophore, the inhibitors are increasing the metal concentrations in the cell causing the activation of Metal Response Elements (MRE). Activation of MRE's by increases cellular levels of zinc has been shown to induce the expression of metalloprotease called Metallothionein which is important role in detoxification, homeostasis and protection from oxidative stress inflammatory responses and other stressors (Z-Ghandour, Vallee, Klassen=[63-65]). Schmeisser et al established that Mtl-2 is essential for lifespan extension in C. elegans that were exposed to low dose arsenite; a known toxicant (Schemiesser et al=[66]). Metallothioneins also plays a role in immune response to metal toxins, xenobiotics, oxidative stress caused by infections, inflammation, and physical stress as studies have demonstrated that MTs are responsible for lymphocyte, macrophage proliferation plus enhances the cells ability to kill phagocytized organisms(Lynes and Youn=[67-68]). White et al showed that in the presence of zinc, CQ increased efflux of zinc, which led to the up regulation of metalloproteinase activity (White=[69]) that could possibly be happening in or C. elegans assay.
Thirdly, low doses of the compounds may be transiently inducing the expression of ROS which also leads to activation of the SKN-1 signaling cascade (Hoeven and Garsin 2011=[70]) leading to the activation of the MRE and ARE protective responses. Schmeisser et al showed that low dose arsenite transiently induces a ROS and p38MAPK signaling pathway that leads to lifespan extension on C. elegans. Due to the promiscuous nature of the inhibitors it is believed that they can have multiple targets in vivo. The increase in potency of the inhibitors in the C. elegans is attributed to the possibility that the inhibitors are binding to other receptors that activate the immune system as well as triggers the expression of genes that regulate other defensive mechanisms in the nematode that help clear the E. faecalis infection.
Specifically it is hypothesized that the inhibitors are increasing the expression metallothioneins (especially CeMT2) in the nematodes gut; which has known protective effects on the nematodes. Metallothioneins (MTs) are a family of small, highly conserved small cysteine rich metalloproteases. They are important in metal detoxification, homeostasis and protection from oxidative stress. Studies have shown that extracellular MT causes a burst in superoxide in peritoneal macrophages and this increase in metabolic activity leads to increase in the cells ability to kill phagocytized yeast. Intracellular MT contributes to increase in monocytes activation by while reduction of MT may limit efficacy. MTs promotes murine Lymphocyte proliferation. In C. elegans they scavenge and protect against reactive oxygen species and oxidative stress with CeMT-2 being more effective than CeMT-1. mtl-2 as well as a mitochondrial transporter tin-9 are both essential for lifespan extension of nematodes exposed to low doses of Arsenite. Therefore the protections seen in the nematode are likely due to the combination of the many advantageous effect of metallothioneine.
4 × 10−12
The ability of the compound 5 to reduce colonization of the intestinal tract was examined. As shown in
An assessment of the efficacy of the inhibitors on other clinically relevant pathogens that are responsible for nosocomial infections, as well as to predict the efficacy of the compounds in treatment of polymicrobial infections was performed. Last CDC estimates report that 16.4% of HAI were polymicrobial and one of the leading causes of gram-negative infections is Pseudomonas areuginosa. P. areuginosa is a gram-negative bacteria that causes infections in healthcare settings the most serious of which include: bacteremia, pneumonia, urosepsis and wound infections including secondary infection of burns. P. areuginosa was ranked 5th among the causative pathogens of HAI in the US with 7.5% of infections. Most importantly, infection rates are reported to be rising both in the US and globally as well as resistance to antibiotics. P. areuginosa is resistant to many antibiotics such as quinolones, carbapenems and Aminoglycosides. It has been dubbed an “ESKAPE” pathogen due to high incidence in HAI's and its ability to evade the activity of antibacterial drugs. These factors make P. areuginosa an important pathogen for which development of new therapeutics is imperative.
Screening of Select EfMetAP1 Inhibitors Against P. aeruginosa
P. aeruginosa bacterial culture strain PA14 was grown in LB media and SK media by incubating overnight at 37° C. (Rahme et al. 1995). Initial Optical density (OD) reading was taken and culture was normalized to 1×106 cells; A600=0.6. Serial dilutions of compounds 4 and 5 were performed to obtain final concentrations of 40 μg/ml to 2.5 μg/mL after 5 μl of each concentration was plated onto 96-well plates (Fisher brand, Becton Dickson Microtest tissue culture plate) with 45 μl of the respective media containing 5 μl of E. faecalis (three wells per condition). Initial reading is taken at OD600 using a MultiSkan MCC Plate reader plate reader (Fisher Scientific, Pittsburgh, Pa., USA). The plate was incubated for 24 hours at 37° C. after which the final reading was taken at OD600.
The preliminary screening of compounds 4 and 5 against P. aeruginosa infected C. elegans was performed according to standardized assay developed by Rahme et al. 1995 with modifications. The result showed that in LB media the inhibitors were able to achieve approximately 80% inhibition at a concentration of 2.5 μg/mL (
The ability of the inhibitors to not only inhibit growth of gram-positive E. faecalis but also be efficacious against gram-negative P. aeruginosa shows that this pharmacological class of compounds have a broad spectrum of activity. This is of clinical relevance as many nosocomial infections are polymicrobial. Therefore the use of a broad spectrum antibiotic that is potent would reduce the pill burden on patients, prevent drug-drug interactions and their associated cytotoxic effects and ultimately improve treatment outcomes.
A simple, sensitive and reliable analytical method employing high-performance liquid chromatography using a UV-Vis absorbance detector (HPLC-UV) has been developed for the quantification of compound 5 in solution. This validated method is suitable for the determination of compound 5 in preformation studies. Chromatographic analysis was performed using a Waters 2487 Dual A Absorbance Detector (Waters, Milford, Mass.) with the wavelength of detection set at 254 nm. Chromatographic separation was achieved by a Hypersil BDS C18 column (3.0 μm, 4.6×100 mm, Thermo Fisher Scientific, Waltham, Mass.) using Waters HPLC system comprising of a 717 Plus Auto-sampler and 600 Pump. An isocratic solvent system comprising of 60% acetonitrile in water with 0.1% trifluoroacetic acid was used at 1 mL/min. Clioquinol, a congener of compound 5 was used as internal standard (IS). The retention times for compound 5 and IS were 3.43 and 4.69 mins respectively (
Working stock solutions of compound 5 and IS were prepared by dissolving in HPLC grade acetonitrile at concentrations of 1 mg/mL respectively, and stored at −80° C. until use. Standard samples of compound 5 were prepared in mobile phase (60% acetonitrile in water containing 0.1% trifluoroacetic acid) at different concentrations ranging from 1-100 μg/mL. Quality control (QC) samples were prepared in mobile phase at low (5 μg/mL), medium (20 μg/mL) and high (80 μg/mL) compound 5 concentrations. 20 μL was injected into the column for chromatographic analysis; the assay run time was 6 mins.
Linear calibration curves in solution was generated by plotting the peak area ratio of compound 5 to IS against known standard concentrations of compound 5 (
The intra-day accuracy and precision was determined by analyzing three replicates of quality control (QC) samples at low, medium and high concentrations of compound 5 using a calibration curve constructed on the same day. The inter-day accuracy and precision were determined by analyzing three replicates of QC samples using calibration curves constructed on three different days. The accuracy of the assay was established by calculating the relative error from the theoretical compound 5 concentrations, while the precision was reflected by the coefficient of variation.
The data obtained, as represented in Table 9, shows that the accuracy and precision were well within the 15% acceptance range set by the U.S Food and Drug Administration (FDA). Our HPLC-UV analytical method was validated as accurate and precise for the quantification of solution of compound 5 ranging from 1-100 μg/mL.
A simple, specific, sensitive and reliable LC-MS/MS analytical method has been developed for the quantification of compound 5 in solution, plasma and urine. This validated method is suitable for the determination of compound 5 in preclinical studies: pre-formulation, formulation and pharmacokinetic studies as well as clinical studies. Analyst® Software 1.6 (AB Sciex, Foster City, Calif.) was used to control the LC-MS/MS system and analyze data. Chromatographic analysis was performed using 4000 QTRAP® LC-MS/MS system (AB Sciex, Foster City, Calif.), a hybrid triple quadrupole LIT (linear ion trap) mass spectrometer equipped with a Turbo V™ ion source. Pure nitrogen (curtain gas), source and exhaust gases were generated by a Peak Scientific GENIUS ABN2ZA Tri Gas Generator. The IonSpray heater was maintained at 550° C. with both the nebulizer gas and heater gas set to 55.0 and 50.0 psi respectively. The IonSpray voltage was set to 5500 V; the curtain gas set to 25.0 psi and the collision “CAD” gas set to high. Multiple reaction monitoring (MRM) method in the positive mode was used to detect the transition ions from a specific precursor ion to the product ion for OJT1 ([M]+ m/z 257.919→m/z 151.0) and the internal standard ([M]+ m/z 305.783→m/z 178.90). The collision energy was set at 53.00 eV and 39.00 eV for compound 5 and internal standard, respectively. Clioquinol, a congener of compound 5 was used as internal standard (IS). Table 10 list the electronic parameters for MS/MS acquisition of compound 5 and IS.
Chromatographic separation was achieved by a Waters XTerra® MS C18 column (3.5 μm, 4.6×50 mm, Milford, Mass.) using a Shimadzu Nexera X2 UHPLC System (Columbia, Md.). A binary solvent system was used: Solvent A was LC-MS grade water containing 0.2% formic acid and Solvent B was LC-MS grade acetonitrile containing 0.2% formic acid. All samples were analyzed using gradient elution: initial 20% B, 70% B at 0.80 min, 95% from 2.80-3.80 min, and 40% B from 4.00-5.50 min at a flow rate of 0.5 mL/min (
Working stock solutions of compound 5 and IS were prepared by dissolving in LC-MS grade acetonitrile at concentrations of 1 mg/mL respectively, and stored at −80° C. until use. Standard samples of compound 5 were prepared in mobile phase (50% acetonitrile in water containing 0.1% formic acid) and rat plasma and urine at different concentrations: 1-1000 ng/mL. Quality control (QC) samples of compound 5 were prepared in mobile phase and rat plasma and urine at low (20 ng/mL in solution, 40 ng/mL in plasma and urine), medium (400 ng/mL) and high (800 ng/mL) concentrations. The plasma and urine samples were prepared by protein precipitation method. Briefly, a 50 μL aliquot of plasma and urine samples were extracted with 200 μL of acetonitrile containing 150 ng/mL of internal standard followed by vortex mixing for 1 minute. This was then centrifuged at 14,000 rpm for 10 min, the supernatant transferred to the auto-sampler vial, and 10 μL injected into the column for LC/MS/MS analysis.
Linear calibration curves in solution, plasma and urine were generated by plotting the peak area ratio of compound 5 to IS against known standard concentrations of compound 5. The slope, intercept and correlation coefficient of linear regression equation were estimated using least square regression analysis. The calibration curves of compound 5 in solution, plasma and urine were linear in the concentration range of 1-1000 ng/mL with correlation coefficient greater than 0.998. The lower limit of quantification (LLOQ) was determined based on a signal-to-noise ratio of at least 5:1.
The assay validation described was carried out using the FDA “Guidance for Industry—Bioanalytical Method Validation” as a guide (1).
Analysis of six replicates of quality control (QC) samples of three different concentrations (low, medium and high) were performed using a calibration curve constructed on the same day to determine the intra-day accuracy and precision. The inter-day accuracy and precision were determined by analyzing six replicates of QC samples of three different concentrations using calibration curves constructed on three different days. The accuracy of the assay was obtained by calculating the relative error from the theoretical compound 5 concentrations, while the assay precision was reflected by the coefficient of variation.
The data obtained, represented in Table 11, shows that the accuracy and precision were well within the 15% acceptance range set by the FDA. The LC-MS/MS method for the analysis of compound 5 was validated to be accurate and precise for the measurement of solution, plasma and urine with compound 5 concentration ranging from 1-1000 ng/mL.
The extraction recovery and matrix effect were determined by analyzing compound 5 samples of three different concentrations: 40, 400 and 800 ng/mL. The extraction recovery of compound 5 was calculated as follows:
Extraction Recovery (%)=Responseextracted sample−Responsepost-extracted spiked sample×100%
where Responseextracted sample is the average area count for compound 5 sample, which has been through the extraction process, and Responsepost-extracted spiked sample the average area count for compound 5 sample spiked into extracted matrix after the extraction procedure. Table 12 shows the average extraction recovery obtained by measuring triplicates of QC samples at low, medium and high concentration levels of compound 5 in rat plasma and urine. The data suggest that compound 5 can be easily extracted from plasma and urine samples.
The effect of the biological matrix on compound 5 concentration was calculated as follows:
Matrix effect (%)=Responsepost-extraction spike sample−Responseneat sample×100
where Responsepost-extraction spike sample is the average peak area count for a sample into which compound 5 was spiked into extracted matrix after the extraction procedure, and Responseneat sample is the average peak area count for the same concentration of compound 5 prepared in a neat solution (acetonitrile). A positive value indicates the enhancement of the sample signal, while a negative value indicates suppression of the sample signal (2). Table 12 shows the average matrix effects obtained for low, medium and high QC plasma and urine samples respectively. The data suggest that there was no measurable matrix effect interfering with the determination compound 5 in rat plasma and urine using this LC-MS/MS method.
The short-term (bench-top) stability of compound 5 in plasma and urine samples was evaluated by analyzing three sets each of freshly prepared plasma and urine samples containing compound 5 and placed them on the bench-top for 2, 4, and 6 h, respectively or at −80° C. for 14 days. All the samples were compared with freshly prepared samples of the same concentration. Table 13 shows average recoveries of compound 5 from plasma and urine samples after 2, 4, and 6 h respectively and after storage at −80° C. for 14 days. This data indicates that compound 5 is stable in plasma and urine samples placed on the bench-top for up to 6 hours and at −80° C. for 14 days (3).
The stability of compound 5 in processed samples (on-instrument or auto-sampler stability) was also evaluated by comparing freshly prepared plasma and urine QC samples to similar samples placed on the auto-sampler for 2, 4, and 6 h respectively. One set of the plasma and urine QC samples was extracted with acetonitrile containing IS, and the other set with pure acetonitrile without IS. Table 13 shows the average recoveries of the plasma and urine samples extracted with acetonitrile containing IS and without IS respectively. This data indicates that compound 5 is stable in processed plasma and urine samples placed on the instrument for up to 6 hours, and the stability is independent on the presence of internal standard (4).
Assessment of the solubility of compound 5 in various solvents is important in developing suitable formulations for preclinical and clinical studies. The solubility of compound 5 in water, ethanol, poly ethylene glycol 400, propylene glycol monocapryrate type I (PGMC), propylene glycol monocapryrate type II (CAPYROL 90), dimethyl sulfoxide (DMSO), dimethyl acetamide (DMA), TWEEN 80, TWEEN 20, paraffin oil, soybean oil, and olive oil were determined by the shaker method. Briefly, excess amount of compound 5 was added to each of the selected solvents in a scintillation vial and placed on a reciprocating shaker to shake at room temperature for 72 h. The samples were centrifuged at 14,000 rpm for 10 min and subsequently filtered through a 0.22 μm filtration unit; the resulting filtrate was analyzed by HPLC-UV to determine the amount of compound 5 dissolved in the solvents. The experiment was conducted in triplicate. The result, summarized in Table 14, revealed that compound 5 is practically insoluble in water (0.07 mg/mL), but freely soluble in DMA (>80 mg/mL).
The octanol—water partition co-efficient (log P) of compound 5, which measures its hydrophilicity (“water-loving” property) or hydrophobicity (“water-repelling” property), was evaluated using the shaker method. Compound 5 has an estimated octanol/water partition co-efficient (x log P) value of 3.20 (Pubchem), and an experimental, M log P of 3.03±0.04. This indicate potential water solubility challenges especially for oral administration.
The water solubility of compound 5 can be improved by incorporating it in a water miscible solvent in which it has a good solubility. This method, often called a co-solvent system, is a suitable means for formulating non-water-soluble drugs for intravenous administration. A co-solvent system suitable for intravenous administration must resist precipitation of the drug upon dilution with intravenous fluids or blood. Different co-solvent systems with varying compositions and ratio of solvents were prepared with the concentration of compound 5 ranging from 5-10 mg/mL. Each system was diluted with normal saline (0.9% sodium chloride) at ratios of 1:2, 1:5, 1:10, 1:20 (v/v), to evaluate if compound 5 will precipitate within 4 hours.
The diluted formulations were observed for at least 4 hours for the presence or absence of precipitation which indicated the capability of the formulation to keep compound 5 dissolved in an aqueous environment. It also indicated that following an intravenous dose of this formulation, compound 5 will most likely not precipitate at the site of administration. The optimal formulation was selected based on (1) solubility of compound 5, (2) precipitation of compound 5 upon dilution, (3) toxicity of the solvent, and (4) stability of the formulation. The various co-solvent systems formulated and their behaviors upon dilution with normal saline are summarized in Table 15-17.
Based on the factors listed above, the co-solvent systems APT1 (consisting of 5% DMA, 35% PEG 400 and 60% TWEEN 80), and PTT6 (consisting of 10% TRANSCUTOL HP, 20% PEG 400, and 70% TWEEN 80) were selected as optimal co-solvent formulations for IV and oral/subcutaneous administration respectively. These formulations, containing 5 mg/mL and 7.5 mg/mL respectively, can be diluted with normal saline to the desired concentration of compound 5 before IV or oral administration in pre-clinical and clinical settings.
The stability of the optimal co-solvent formulations was investigated at various storage temperatures. Briefly, aliquots of the optimal co-solvent formulations were stored at different temperatures (−20° C., 4° C. and 25° C.) and analyzed using LC/MS/MS on Day 3, 7, 14 and 30 to determine the amount of compound 5 remaining. The experiment was conducted in triplicates. The stability data suggests that the compound 5 is stable in the co-solvent formulations for up to one month when stored at −20° C., 4° C. and 25° C. The optimal co-solvent formulations were applied to the pharmacokinetic study of compound 5 in rats (Table 18). The stability of compound 5 in DPT and PTT formulation is shown in
Pharmacokinetic evaluation elucidates the fate of compound 5 in living systems. The pharmacokinetic study of compound 5 was also a means to verify the applicability of the LC-MS/MS assay method and the formulations. An adult male Sprague Dawley rat model was the preferred biological system for this experiment based on the similarity to humans in metabolism and minimal interference of hormones with metabolism. Briefly, male Sprague Dawley rats (n=4 for IV group, n=3 for subcutaneous and oral groups each, body weight: 300-350 g) were cannulated through the jugular vein under anesthesia (using a cocktail of ketamine: acepromazine: xylazine at a ratio of 50: 3.3: 3.3 mg/kg). On the following day, the optimal IV co-solvent formulation was diluted five times with normal saline to 1 mg/mL. The formulation for subcutaneous and oral administration was diluted with equal amount of normal saline to 3.75 mg/mL. Each rat was administered a 2 mg/kg IV bolus dose, 10 mg/kg subcutaneous dose or 20 mg/kg oral dose of compound 5. Heparinized blood samples were withdrawn from each rat at 5, 10, 15, 30 mins, 1, 2, 4, 6, 8, 12, 24, 48, 72, 96, 144 h after injection. The blood samples were centrifuged at 14,000 rpm for 6 min and the supernatant plasma obtained and stored at −80° C. until LC-MS/MS analysis for the concentration of compound 5. Urine samples were also collected at 0, 4, 8, 12, and 24 h. The plasma and urine samples were analyzed (within 7 days) using the developed LC/MS/MS method to determine the concentration of compound 5.
The pharmacokinetic parameters for each rat were determined with Phoenix WinNonlin 6.3 software (Pharsight Corporation, Mountain View, Calif., USA) a non-compartmental analysis and a two compartment, which best described the fit for the IV bolus administration of compound 5, based on the observed and predicted fits of the plasma concentration versus time plot, the reduction in the sums of squares, and the Akaike's information criterion (AIC) for comparing compartmental models (5).
The two-compartment model is described by the equation:
C
t
=A.e
−αt
+B.e
−βt
where A and B are the coefficients, α and β are alpha and beta phase rate constants respectively, and Ct is the plasma concentration of compound 5 at time,t.
The weighting scheme of concentration−2 (Y−2) was used to determine the model that best fits the individual profiles. Table 19 & 20 shows the mean pharmacokinetic parameters and Table 20 show the plasma protein binding in rat plasma. The plasma concentration -time profiling following 20 mg/Kg oral and 10 mg/kg subcutaneous doses of compound 5 is shown in
aStatistically significant difference between oral and IV administration
bStatistically significant difference between oral and SC administration
cStatistically significant difference between SC and IV administration
In summary, following the administration of 2 mg/kg IV bolus, an average maximum plasma concentration of compound 5 (Cmax) of 2.60±0.56 mg/L was reached, rapidly declining within two hours, and steadily tailing off in the terminal elimination phase. The distribution phase half-life (T1/2α) was observed to be 0.19±0.02, and the β-phase elimination half-life (T1/2β) was 109±19.4 hr. This implies that compound 5 is rapidly distributed to the tissues of the body after administration but is slowly eliminated from the body. The mean parameters from the subcutaneous route of administration was significantly different from that obtained the IV route. The estimated relative bioavailability of compound 5 via the subcutaneous and oral route were 15.7%, and 4.6% respectively and compound 5 seems to have a long plasma half-life when administered via IV and subcutaneous route of administration.
The following references are cited herein:
1. Administration, U.S.F.D.A,. Available from: www.fda.gov/cder/guidance.
2. Matuszewski B. K. et al. Analyt. Chem. 2003; 75:3019-3030.
3. Liang, S., et al. Biomed Chromatogr. 2013; 27: 58-66.
4. Liang, S., et al. Am J Mod Chromatogr. 2014; 1:1-11.
5. Yamaoka K. et al. J Pharmaco Biopharm. 1978; 6:165-175.
This application is a continuation-in-part under 35 U.S.C. §120 of pending non-provisional application U.S. Ser. No. 14/536,024, filed Nov. 7, 2014, which claims benefit of priority under 35 U.S.C. §119(e) of provisional application U.S. Ser. No. 61/906,658, filed Nov. 20, 2013, now abandoned, the entirety of all of which is hereby incorporated by reference.
Number | Date | Country | |
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61906658 | Nov 2013 | US |
Number | Date | Country | |
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Parent | 14536024 | Nov 2014 | US |
Child | 15637245 | US |