C4-carbonothioate-substituted tryptamine derivatives and methods of using
11707447 · 2023-07-25
Assignee
Inventors
Cpc classification
C07D209/20
CHEMISTRY; METALLURGY
A61K31/4045
HUMAN NECESSITIES
International classification
A61K31/4045
HUMAN NECESSITIES
Abstract
Disclosed are novel C.sub.4-carbonothioate-substituted tryptamine derivative compounds and pharmaceutical and recreational drug formulations containing the same. The pharmaceutical formulations may be used to treat brain neurological disorders.
Claims
1. A chemical compound having chemical formula (I): ##STR00054## wherein R.sub.4 is a carbonothioate moiety or a derivative thereof; wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group; and wherein the carbonothioate moiety or derivative thereof has the chemical formula (III): ##STR00055## wherein R.sub.4b is an optionally substituted alkyl group.
2. A chemical compound according to claim 1, wherein R.sub.4b is a C.sub.1-C.sub.6 alkyl substituted with an aryl group.
3. A chemical compound according to claim 1, wherein R.sub.4b is C.sub.1-C.sub.3 alkyl substituted with an aryl group.
4. A chemical compound according to claim 1, wherein R.sub.4b is a methylene (—CH.sub.2—) substituted with an aryl group.
5. A chemical compound according to claim 3, wherein the aryl group is a phenyl group.
6. A chemical compound according to claim 4, wherein the aryl group is a phenyl group.
7. A chemical compound according to claim 1, wherein R.sub.3a and R.sub.3b are independently a C.sub.1-C.sub.6 alkyl group.
8. A chemical compound according to claim 1, wherein R.sub.3a and R.sub.3b are independently a C.sub.1-C.sub.3 alkyl group.
9. A chemical compound according to claim 1, wherein R.sub.3a and R.sub.3b are a methyl group.
10. A chemical compound according to claim 1, wherein one of R.sub.3a and R.sub.3b is a C.sub.1-C.sub.6 alkyl group, and the other of R.sub.3a and R.sub.3b is a hydrogen atom.
11. A chemical compound according to claim 1, wherein R.sub.4 is a carbonothioate moiety or derivative thereof, and wherein the compound is E(VI): ##STR00056##
12. A pharmaceutical drug formulation comprising an effective amount of a chemical according to claim 1, together with a pharmaceutically acceptable excipient, diluent, or carrier.
13. A pharmaceutical formulation according to claim 12, wherein the pharmaceutical formulation is a pro-drug pharmaceutical formulation, wherein the compound having formula (I) is in vivo hydrolyzed to form a compound having chemical formula (VI): ##STR00057## wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
(1) The disclosure is in the hereinafter provided paragraphs described, by way of example, in relation to the attached figures. The figures provided herein are provided for a better understanding of the example embodiments and to show more clearly how the various embodiments may be carried into effect. The figures are not intended to limit the present disclosure.
(2)
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(6) The figures together with the following detailed description make apparent to those skilled in the art how the disclosure may be implemented in practice.
DETAILED DESCRIPTION
(7) Various compositions, systems or processes will be described below to provide an example of an embodiment of each claimed subject matter. No embodiment described below limits any claimed subject matter and any claimed subject matter may cover processes, compositions or systems that differ from those described below. The claimed subject matter is not limited to compositions, processes or systems having all of the features of any one composition, system or process described below or to features common to multiple or all of the compositions, systems or processes described below. It is possible that a composition, system, or process described below is not an embodiment of any claimed subject matter. Any subject matter disclosed in a composition, system or process described below that is not claimed in this document may be the subject matter of another protective instrument, for example, a continuing patent application, and the applicant(s), inventor(s) or owner(s) do not intend to abandon, disclaim or dedicate to the public any such subject matter by its disclosure in this document.
(8) As used herein and in the claims, the singular forms, such “a”, “an” and “the” include the plural reference and vice versa unless the context clearly indicates otherwise. Throughout this specification, unless otherwise indicated, “comprise,” “comprises” and “comprising” are used inclusively rather than exclusively, so that a stated integer or group of integers may include one or more other non-stated integers or groups of integers.
(9) Various compositions, systems or processes will be described below to provide an example of an embodiment of each claimed subject matter. No embodiment described below limits any claimed subject matter and any claimed subject matter may cover processes, compositions or systems that differ from those described below. The claimed subject matter is not limited to compositions, processes or systems having all of the features of any one composition, system or process described below or to features common to multiple or all of the compositions, systems or processes described below. It is possible that a composition, system, or process described below is not an embodiment of any claimed subject matter. Any subject matter disclosed in a composition, system or process described below that is not claimed in this document may be the subject matter of another protective instrument, for example, a continuing patent application, and the applicant(s), inventor(s) or owner(s) do not intend to abandon, disclaim or dedicate to the public any such subject matter by its disclosure in this document.
(10) When ranges are used herein for physical properties, such as molecular weight, or chemical properties, such as chemical formulae, all combinations and sub-combinations of ranges and specific embodiments therein are intended to be included. Other than in the operating examples, or where otherwise indicated, all numbers expressing quantities of ingredients or reaction conditions used herein should be understood as modified in all instances by the term “about.” The term “about” when referring to a number or a numerical range means that the number or numerical range referred to is an approximation within experimental variability (or within statistical experimental error), and thus the number or numerical range may vary between 1% and 15% of the stated number or numerical range, as will be readily recognized by context. Furthermore, any range of values described herein is intended to specifically include the limiting values of the range, and any intermediate value or sub-range within the given range, and all such intermediate values and sub-ranges are individually and specifically disclosed (e.g., a range of 1 to 5 includes 1, 1.5, 2, 2.75, 3, 3.90, 4, and 5). Similarly, other terms of degree such as “substantially” and “approximately” as used herein mean a reasonable amount of deviation of the modified term such that the end result is not significantly changed. These terms of degree should be construed as including a deviation of the modified term if this deviation would not negate the meaning of the term it modifies.
(11) Unless otherwise defined, scientific and technical terms used in connection with the formulations described herein shall have the meanings that are commonly understood by those of ordinary skill in the art. The terminology used herein is for the purpose of describing particular embodiments only, and is not intended to limit the scope of the present invention, which is defined solely by the claims.
(12) All publications, patents and patent applications are herein incorporated by reference in their entirety to the same extent as if each individual publication, patent, or patent application was specifically and individually indicated to be incorporated by reference in its entirety.
Terms and Definitions
(13) The term “tryptamine” refers to a chemical compound having the structure set forth in
(14) The term “indole prototype structure” refers to the chemical structure shown in
(15) The term “tryptamine derivative”, as used herein, refers to compounds that can be derivatized from tryptamine, wherein such compounds include an indole prototype structure and a C.sub.3 ethylamine or ethylamine derivative group having the formula (VII):
(16) ##STR00017##
wherein R.sub.4, is a substituent (any atom or group other than a hydrogen atom) comprising a carbonothioate moiety or derivative thereto, and wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group. Thus, tryptamine derivative compounds include compounds containing a substituent at C.sub.4, as defined. Additional other atoms, such as N.sub.1, may also be substituted. Moreover, in this respect, tryptamine derivatives containing a substituent atom or group at e.g., C.sub.4 may be referred to as C.sub.4-substituted tryptamine derivatives. In chemical formula (VII), R.sub.4, can, for example, be a carbonothioate moiety or derivative thereof, and the tryptamine derivative may be referred to as a C.sub.4-carbonothioate-substituted tryptamine derivative.
(17) The term “carbonothioate moiety or derivative thereof”, as used herein, refers to a derivative including a group having chemical formula (XII).sub.a or (XII).sub.b:
(18) ##STR00018##
(19) Wherein R.sub.4′ is a hydrocarbon group, for example, an alkyl group, cyclo-alkyl group, or an aryl group. It is noted that the partially bonded oxygen atom of the group having formula (XII).sub.a and (XII).sub.b can be bonded to another entity, including, for example, to the C.sub.4 atom of tryptamine. It is further noted that R.sub.4′ can herein additionally include numerical subscripts, such as .sub.4a, 4b, 4c, 4d etc., and be represented, for example, as R.sub.4a, R.sub.4b, R.sub.4c or R.sub.4d, respectively. Where such numerical values are included, they reference a chemical entity extending from the carboxyl group extending in turn from the thus numbered C atom of the prototype indole structure. Thus, for example, R.sub.4c is a chemical entity extending from a carbonothioate group attached to the C.sub.4 atom of the indole ring structure.
(20) The terms “halogen”, “halogenated” and “halo-”, as used herein, refer to the class of chemical elements consisting of fluorine (F), chlorine (Cl), bromine (Br), and iodine (I). Accordingly, halogenated compounds can refer to “fluorinated”, “chlorinated”, “brominated”, or “iodinated” compounds.
(21) The terms “hydroxy group”, and “hydroxy”, as used herein refers to a molecule containing one atom of oxygen bonded to one atom of hydrogen and having the formula —OH. A hydroxy group through its oxygen atom may be chemically bonded to another entity.
(22) The term “alkyl group”, as used herein, refers to a straight and/or branched chain, saturated alkyl radical containing from one to “p” carbon atoms (“C.sub.1-C.sub.p-alkyl”; for example, p can be an integer between 2 and 20, for example, 3, 6, 10 or 20) and includes, depending on the identity of “p”, methyl, ethyl, propyl, isopropyl, n-butyl, s-butyl, isobutyl, t-butyl, 2,2-dimethylbutyl, n-pentyl, 2-methylpentyl, 3-methylpentyl, 4-methylpentyl, n-hexyl, and the like, where the variable p is an integer representing the largest number of carbon atoms in the alkyl radical. Alkyl groups further include hydrocarbon groups arranged in a chain having the chemical formula —C.sub.nH.sub.2n+1, including, without limitation, methyl groups (—CH.sub.3), ethyl groups (—C.sub.2H.sub.5), propyl groups (—C.sub.3H.sub.7), and butyl groups (—C.sub.4H.sub.9).
(23) The term “alkylene” refers to a divalent group derived from an alkane by removal of two hydrogen atoms from the same carbon atom. Examples of alkylenes include, without limitation, ethylene (—C.sub.2H.sub.4)—), propylene (—C.sub.3H.sub.6)—), and butylene (—C.sub.4H.sub.8)—). For the purposes of the present application further understood to be an alkylene is methylene (—CH.sub.2—).
(24) The term “cyclo-alkyl” refers to cyclo-alkyl groups, including (C.sub.3-C.sub.20), (C.sub.3-C.sub.10), and (C.sub.3-C.sub.6) cyclo-alkyl groups, and includes saturated and partially saturated cyclo-alkyl groups, further including cyclo-propane, cyclo-butane, cyclo-pentane, cyclo-hexane, cyclo-heptane, cyclopentene and cyclohexene.
(25) The term “O-alkyl group”, as used herein, refers to a hydrocarbon group arranged in a chain having the chemical formula —O—C.sub.nH.sub.2n+1. O-alkyl groups include, without limitation, O-methyl groups (—O—CH.sub.3), O-ethyl groups (—O—C.sub.2H.sub.5), O-propyl groups (—O—C.sub.3H.sub.7) and O-butyl groups (—O—C.sub.4H.sub.9).
(26) The term “aryl group”, as used herein, refers to a hydrocarbon group arranged in an aromatic ring and can, for example, be a C.sub.6-C.sub.14-aryl, a C.sub.6-C.sub.10-aryl. Aryl groups further include phenyl, naphthyl, tetrahydronaphthyl, phenanthrenyl, biphenylenyl, indanyl, tolyl, xylyl, or indenyl groups, and the like.
(27) The term “alcohol group” or “hydroxylalkyl”, as used herein, refers to a hydrocarbon group arranged in a chain having the chemical formula C.sub.nH.sub.n+1OH. Depending on the carbon chain, length specific alcohol groups may be termed a methanol group (n=1) or hydroxymethyl, an ethanol group (n=2) or hydroxyethyl, a propanol group (n=3) or hydroxypropyl, a butanol group (n=4) or hydroxybutyl etc.
(28) The term “receptor”, as used herein, refers to a protein present on the surface of a cell, or in a cell not associated with a cellular surface (e.g., a soluble receptor) capable of mediating signaling to and/or from the cell, or within the cell and thereby affect cellular physiology. Example receptors include, 5-HT.sub.1A receptors, 5-HT.sub.1B receptors, 5-HT.sub.2A receptors, and “5-HT.sub.2B receptors”, and so on. In this respect, “signaling” refers to a response in the form of a series of chemical reactions which can occur when a molecule, including, for example, the C.sub.4-substituted tryptamine derivatives disclosed herein, interacts with a receptor. Signaling generally proceeds across a cellular membrane and/or within a cell, to reach a target molecule or chemical reaction, and results in a modulation in cellular physiology. Thus, signaling can be thought of as a transduction process by which a molecule interacting with a receptor can modulate cellular physiology, and, furthermore, signaling can be a process by which molecules inside a cell can be modulated by molecules outside a cell. Signaling and interactions between molecules and receptors, including for example, affinity, binding efficiency, and kinetics, can be evaluated through a variety of assays, including, for example, assays known as receptor binding assays (for example, radioligand binding assays, such as e.g., [.sup.3H]ketanserin assays may be used to evaluate receptor 5-HT.sub.2A receptor activity), competition assays, and saturation binding assays, and the like.
(29) The term “5-HT.sub.1A receptor”, as used herein, refers to a subclass of a family of receptors for the neurotransmitter and peripheral signal mediator serotonin. 5-HT.sub.1A receptors can mediate a plurality of central and peripheral physiologic functions of serotonin. Ligand activity at 5-HT.sub.1A is generally not associated with hallucination, although many hallucinogenic compounds are known to modulate 5-HT.sub.1A receptors to impart complex physiological responses (Inserra et al., 2020, Pharmacol. Rev 73: 202). 5-HT.sub.1A receptors are implicated in various brain neurological disorders, including depression and anxiety, schizophrenia, and Parkinson's disease (Behav. Pharm. 2015, 26:45-58).
(30) The term “5-HT.sub.1B receptor”, as used herein, refers to a subclass of a family of receptors for the neurotransmitter and peripheral signal mediator serotonin. 5-HT.sub.1B receptors can mediate a plurality of central and peripheral physiologic functions of serotonin. Ligand activity at 5-HT.sub.1B is generally not associated with hallucination, although many hallucinogenic compounds are known to modulate 5-HT.sub.1A receptors to impart complex physiological responses (Inserra et al., 2020, Pharmacol. Rev. 73: 202). 5-HT.sub.1B receptors are implicated in various brain neurological disorders, including depression (Curr. Pharm. Des. 2018, 24:2541-2548).
(31) The term “5-HT.sub.2A receptor”, as used herein, refers to a subclass of a family of receptors for the neurotransmitter and peripheral signal mediator serotonin. 5-HT.sub.2A receptors can mediate a plurality of central and peripheral physiologic functions of serotonin. Central nervous system effects can include mediation of hallucinogenic effects of hallucinogenic compounds. 5-HT.sub.2A receptors are implicated in various brain neurological disorders (Nat. Rev. Drug Discov. 2022, 21:463-473; Science 2022, 375:403-411).
(32) The term “5-HT.sub.2B receptor”, as used herein, refers to a subclass of a family of receptors for the neurotransmitter and peripheral signal mediator serotonin. 5-HT.sub.2B receptors can mediate a plurality of central and peripheral physiologic functions of serotonin. Central nervous system effects can include mediation of hallucinogenic effects of hallucinogenic compounds. 5-HT.sub.bA receptors are implicated in various brain neurological disorders, including schizophrenia (Pharmacol. Ther. 2018, 181:143-155) and migraine (Cephalalgia 2017, 37:365-371).
(33) The term “5-HT.sub.3A receptor”, as used herein, refers to a subclass of a family of receptors for the neurotransmitter and peripheral signal mediator serotonin. 5-HT.sub.3A receptors can mediate a plurality of central and peripheral physiologic functions of serotonin. 5-HT.sub.3A receptors are implicated in various brain neurological disorders, including depression (Expert Rev. Neurother. 2016, 16:483-95).
(34) The term “ADRA1A receptor”, as used herein, refers to a subclass of a family of receptors, also known as α1-adrenergic receptors, which can be modulated by selective serotonin reuptake inhibitors (SSRIs) and tricyclic antidepressant (TCA) (Int. J. Mol Sci. 2021, 22: 4817; Brain Res. 1285 2009, 148-157). ADRA1A receptors are implicated in various brain neurological disorders, including depression.
(35) The term “ADRA2A receptor”, as used herein, refers to a subclass of a family of receptors, also known as α2-adrenergic receptors. ADRA2A receptors are implicated in various brain neurological disorders, including Attention Deficit Hyperactivity Disorder (ADHD) (J. Am. Acad. Child. Adolesc. Psychiatry 2014, 53:153-73), mania, bipolar disorder, and schizophrenia.
(36) The term “CHRM1 receptor”, as used herein, refers to a subclass of receptors also known as “cholinergic receptor muscarinic 1”, which can be modulated by selective serotonin reuptake inhibitors (SSRIs) (e.g., paroxetine) and tricyclic antidepressant (TCA). The class of CHRM receptors are implicated in various brain neurological disorders, including depression, major depression disorder (MDD), and bipolar disorder (Mol. Psychiatry 2019, 24: 694-709).
(37) The term “CHRM2 receptor”, as used herein, refers to a subclass of receptors also known as “cholinergic receptor muscarinic 2”, which can be modulated by tricyclic antidepressant (TCA). The class of CHRM receptors are implicated in various brain neurological disorders, including depression, major depression disorder (MDD), and bipolar disorder (Mol. Psychiatry 2019, 24: 694-709).
(38) The term “CNR1 receptor”, as used herein, refers to a subclass of receptors also known as “cannabinoid receptor CB.sub.1”, which can be modulated by cannabinoid compounds. CNR receptors are implicated in various brain neurological disorders, including depression and schizophrenia (Pharmacol. Res. 2021, 170: 105729).
(39) The term “DRD1 receptor”, as used herein, refers to a subclass of receptors also known as “dopamine receptor D.sub.1”, which can be modulated by dopamine. Dopamine receptors are implicated in various brain neurological disorders, including schizophrenia, psychosis, and depression (Neurosci. Lett. 2019, 691:26-34).
(40) The term “DRD2S receptor”, as used herein, refers to a subclass of receptors also known as “dopamine receptor D.sub.2S”, which can be modulated by dopamine. Dopamine receptors are implicated in various brain neurological disorders, including schizophrenia, psychosis, and depression (Neurosci. Lett. 2019, 691:26-34).
(41) The term “OPRD1 receptor”, as used herein, refers to a subclass of receptors also known as “opioid receptor D.sub.1”, which can be modulated by opioid compounds. OPRD1 receptors are implicated in various brain neurological disorders, including psychopathy, and substance abused disorder (Mol. Psychiatry 2020, 25:3432-3441).
(42) The term “GABAA receptor”, as used herein, refers to a subclass of receptors also known as “γ-aminobutyric acid (GABA) receptor A”, which can be modulated by γ-aminobutyric acid. GABAA receptors are implicated in various brain neurological disorders, including anxiety, major depressive disorder, and post-partem depression (Trends Pharmacol. Sci. 2018, 39:710-732).
(43) The term “NMDAR receptor”, as used herein, refers to a subclass of receptors also known as “N-methyl-D-aspartate receptor”. NMDAR receptors are glutamatergic receptors that are implicated in various brain neurological disorders, including epilepsy, autism spectrum disorder, and schizophrenia (Transl. Psychiatry 2022, 12:243).
(44) The term “DAT”, as used herein, refers to a transmembrane transport protein also known as “dopamine active transporter”, which is involved of transporting dopamine into the cytosol. DAT is implicated in various brain neurological disorders, notably dopamine related disorders such as attention deficit hyperactivity disorder (ADHD), bipolar disorder, and clinical depression, anxiety (Am. J. Med. Genet. B Neuropsychiatr. Genet. 2018, 177:211-231).
(45) The term “NET”, as used herein, refers to a transmembrane transport protein also known as “norepinephrine transporter” or “noradrenaline transporter” or “NAT” which is involved in Na.sup.+/Cl.sup.− dependent re-uptake of extracellular norepinephrine or noradrenaline. NET is implicated in various brain neurological disorders, including attention deficit hyperactivity disorder (ADHD) and clinical depression (Neurosci. Biobehav. Rev, 2013, 37:1786-800).
(46) The term “SERT”, as used herein, refers to a transmembrane transport protein also known as “serotonin transporter” which is involved in neuronal serotonin transport, notably from the synaptic cleft back to the presynaptic neuron, thereby terminating the action of serotonin. SERT is implicated in various brain neurological disorders, including anxiety and depression (Pharmacol. Rep. 2018, 70:37-46).
(47) The term “modulating receptors”, as used herein, refers to the ability of a compound disclosed herein to alter the function of receptors. A receptor modulator may activate the activity of a receptor, or inhibit the activity of a receptor depending on the concentration of the compound exposed to the receptor. Such activation or inhibition may be contingent on the occurrence of a specific event, such as activation of a signal transduction pathway, and/or maybe manifest only in particular cell types. The term “modulating receptors,” also refers to altering the function of a receptor by increasing or decreasing the probability that a complex forms between a receptor and a natural binding partner to form a multimer. A receptor modulator may increase the probability that such a complex forms between the receptor and the natural binding partner, may increase or decrease the probability that a complex forms between the receptor and the natural binding partner depending on the concentration of the compound exposed to the receptor, and or may decrease the probability that a complex forms between the receptor and the natural binding partner. It is further noted that the C.sub.4-carbonothioate-substituted tryptamine derivatives of the present disclosure may alter the function of a receptor by acting as an agonist or antagonist of the receptor, and that C.sub.4-carbonothioate-substituted tryptamine derivatives according to the present disclosure may alter the function of a receptor by directly interacting therewith or binding thereto, or by indirectly interacting therewith through one or more other molecular entities. In general, the receptor may be any receptor, including any receptor set forth herein, such as any of a 5-HT.sub.1A, 5-HT.sub.1B, 5-HT.sub.2A, and a 5-HT.sub.2B receptor, for example. Accordingly, it will be clear, that in order to refer modulating specific receptors, terms such as “modulating 5-HT.sub.1A receptors”, “modulating 5-HT.sub.1B receptors”, “modulating 5-HT.sub.2A receptors”, “modulating 5-HT.sub.2B receptors”, and so forth, may be used herein.
(48) The term “receptor-mediated disorder”, as used herein, refers to a disorder that is characterized by abnormal receptor activity. A receptor-mediated disorder may be completely or partially mediated by modulating a receptor. In particular, a receptor-mediated disorder is one in which modulation of the receptor results in some effect on an underlying disorder e.g., administration of a receptor modulator results in some improvement in at least some of the subjects being treated. In general, the receptor may be any receptor, including any receptor set forth herein, such as any of a 5-HT.sub.1A, 5-HT.sub.1B, 5-HT.sub.2A, and a 5-HT.sub.2B receptor, for example. Accordingly, it will be clear, that in order to refer specific receptor-mediated disorders, terms such as “5-HT.sub.1A receptor-mediated disorder”, “5-HT.sub.1B receptor-mediated disorder”, “5-HT.sub.2A receptor-mediated disorder”, “5-HT.sub.2B receptor-mediated disorder”, and so forth, may be used.
(49) The term “pharmaceutical formulation”, as used herein, refers to a preparation in a form which allows an active ingredient, including a psychoactive ingredient, contained therein to provide effective treatment, and which does not contain any other ingredients which cause excessive toxicity, an allergic response, irritation, or other adverse response commensurate with a reasonable risk/benefit ratio. The pharmaceutical formulation may contain other pharmaceutical ingredients such as excipients, carriers, diluents, or auxiliary agents.
(50) The term “recreational drug formulation”, as used herein, refers to a preparation in a form which allows a psychoactive ingredient contained therein to be effective for administration as a recreational drug, and which does not contain any other ingredients which cause excessive toxicity, an allergic response, irritation, or other adverse response commensurate with a reasonable risk/benefit ratio. The recreational drug formulation may contain other ingredients such as excipients, carriers, diluents, or auxiliary agents.
(51) The term “effective for administration as a recreational drug”, as used herein, refers to a preparation in a form which allows a subject to voluntarily induce a psychoactive effect for non-medical purposes upon administration, generally in the form of self-administration. The effect may include an altered state of consciousness, satisfaction, pleasure, euphoria, perceptual distortion, or hallucination.
(52) The term “effective amount”, as used herein, refers to an amount of an active agent, pharmaceutical formulation, or recreational drug formulation, sufficient to induce a desired biological or therapeutic effect, including a prophylactic effect, and further including a psychoactive effect. Such effect can include an effect with respect to the signs, symptoms or causes of a disorder, or disease or any other desired alteration of a biological system. The effective amount can vary depending, for example, on the health condition, injury stage, disorder stage, or disease stage, weight, or sex of a subject being treated, timing of the administration, manner of the administration, age of the subject, and the like, all of which can be determined by those of skill in the art.
(53) The terms “treating” and “treatment”, and the like, as used herein, are intended to mean obtaining a desirable physiological, pharmacological, or biological effect, and includes prophylactic and therapeutic treatment. The effect may result in the inhibition, attenuation, amelioration, or reversal of a sign, symptom or cause of a disorder, or disease, attributable to the disorder, or disease, which includes mental and psychiatric diseases and disorders. Clinical evidence of the prevention or treatment may vary with the disorder, or disease, the subject, and the selected treatment.
(54) The term “pharmaceutically acceptable”, as used herein, refers to materials, including excipients, carriers, diluents, or auxiliary agents, that are compatible with other materials in a pharmaceutical or recreational drug formulation and within the scope of reasonable medical judgement suitable for use in contact with a subject without excessive toxicity, allergic response, irritation, or other adverse response commensurate with a reasonable risk/benefit ratio.
(55) The terms “substantially pure” and “isolated”, as may be used interchangeably herein describe a compound, e.g., a C.sub.4-carbonothioate-substituted tryptamine derivative, which has been separated from components that naturally or synthetically accompany it. Typically, a compound is substantially pure when at least 60%, more preferably at least 75%, more preferably at least 90%, 95%, 96%, 97%, or 98%, and most preferably at least 99% of the total material (by volume, by wet or dry weight, or by mole percent or mole fraction) in a sample is the compound of interest. Purity can be measured by any appropriate method, e.g., by chromatography, gel electrophoresis or HPLC analysis.
(56) General Implementation
(57) As hereinbefore mentioned, the present disclosure relates to tryptamine derivatives. in particular, the present disclosure provides novel c.sub.4-substituted tryptamine derivatives, and in particular to C.sub.4-carbonothioate substituted tryptamine derivatives. In general, the herein provided compositions exhibit functional properties which deviate from the functional properties o tryptamine. thus, for example, the C.sub.4-carbonothioate-substituted tryptamine derivatives can exhibit pharmacological properties which deviate from tryptamine. Furthermore, the C.sub.4-carbonothioate-substituted tryptamine derivatives may exhibit physico-chemical properties which differ from tryptamine. Thus, for example, C.sub.4-carbonothioate-substituted tryptamine derivatives may exhibit superior solubility in a solvent, for example, an aqueous solvent. Furthermore, the C.sub.4-carbonothioate-substituted tryptamine derivatives may exhibit pharmacokinetics or pharmacodynamics which are different from a non-substituted compound. The C.sub.4-carbonothioate-substituted tryptamine derivatives in this respect are useful in the formulation of pharmaceutical and recreational drug formulations.
(58) In what follows selected embodiments are described with reference to the drawings.
(59) Accordingly, in one aspect, the present disclosure provides derivatives of a compound known as tryptamine of which the chemical structure is shown in
(60) Thus, in one aspect, the present disclosure provides, in accordance with the teachings herein, in at least one embodiment, a compound having chemical formula (I):
(61) ##STR00019##
wherein R.sub.4 is a carbonothioate moiety or derivative thereof; and
wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group.
(62) Thus, referring to the chemical compound having the formula (i), in an aspect hereof, R.sub.4 can be a carbonothioate moiety or derivative thereof, i.e., a carbonothioate moiety or derivative which is bonded via its oxygen atom to the C.sub.4 atom of the tryptamine compound.
(63) In some embodiments, in an aspect, the carbonothioate moiety or derivative thereof can have the chemical formula (III):
(64) ##STR00020##
wherein R.sub.4b is an alkyl group, a cyclo-alkyl group, or an aryl group, each of which are optionally substituted.
(65) In some embodiments, the carbonothioate moiety or derivative thereof can have the chemical formula (IV):
(66) ##STR00021##
wherein R.sub.4c is an alkyl group, a cyclo-alkyl group, or an aryl group, each of which are optionally substituted.
(67) In some embodiments, in the compound having chemical formula (III), R.sub.4b can be C.sub.1-C.sub.6 alkyl optionally substituted with a halogen atom (chloro, fluoro, bromo iodo), alkyl group (for example, C.sub.1-C.sub.10 alkyl or C.sub.1-C.sub.6 alkyl or C.sub.1-C.sub.3 alkyl), cycloalkyl group (for example, C.sub.3-C.sub.10 cycloalkyl or C.sub.3-C.sub.6 cycloalkyl), or an aryl group, a phenyl group, for example.
(68) In some embodiments, in the compound having chemical formula (III), R.sub.4b can be C.sub.1-C.sub.3 alkyl (i.e., a C.sub.1-C.sub.3 alkylene (e.g., methylene, ethylene, propylene), optionally substituted with a halogen atom (chloro, fluoro, bromo, iodo), alkyl group, cycloalkyl group, or an aryl group, a phenyl group, for example.
(69) In some embodiments, in the compound having chemical formula (III) R.sub.4b can be methyl, ethyl, isopropyl, butyl, —CH.sub.2-cyclopropyl, —CH(CH.sub.3)-cyclopropyl, —C(CH.sub.3).sub.2-cyclopropyl or —CH.sub.2-phenyl.
(70) In some embodiments, R.sub.4b can be an aryl group, a phenyl group, for example.
(71) In some embodiments, in the compound having chemical formula (III), R.sub.4b can be C.sub.1-C.sub.6 alkyl optionally substituted with a halogen atom (chloro, fluoro, bromo, iodo), alkyl group, cycloalkyl group, or aryl group, and wherein one or more of the carbon atoms in the C.sub.1-C.sub.6 alkyl group are replaced with oxygen (O) atoms.
(72) In some embodiments, in the compound having chemical formula (IV), R.sub.4c can be C.sub.1-C.sub.6 alkyl optionally substituted with a halogen atom (chloro, fluoro, bromo, iodo), alkyl group (for example, C.sub.1-C.sub.10 alkyl or C.sub.1-C.sub.6 alkyl or C.sub.1-C.sub.3 alkyl), cycloalkyl group (for example, C.sub.3-C.sub.10 cycloalkyl or C.sub.3-C.sub.6 cycloalkyl), or aryl group, a phenyl group for example.
(73) In some embodiments, in the compound having chemical formula (IV) R.sub.4c can be methyl, ethyl, isopropyl, butyl, —CH.sub.2-cyclopropyl, —CH(CH.sub.3)-cyclopropyl, —C(CH.sub.3).sub.2-cyclopropyl or —CH.sub.2-phenyl.
(74) In some embodiments, in the compound having chemical formula (IV) R.sub.4c can be an aryl group, a phenyl group for example.
(75) In some embodiments, in the compound having chemical formula (IV, R.sub.4c can be C.sub.1-C.sub.6 alkyl optionally substituted with a halogen atom (chloro, fluoro, bromo, iodo), alkyl group, cycloalkyl group, or aryl group, and wherein one or more of the carbon atoms in the C.sub.1-C.sub.6 alkyl group are replaced with oxygen (O) atoms.
(76) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(I):
(77) ##STR00022##
(78) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(II):
(79) ##STR00023##
(80) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(III):
(81) ##STR00024##
(82) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(IV):
(83) ##STR00025##
(84) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(V):
(85) ##STR00026##
(86) In some embodiments, in an aspect, in the compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(VI):
(87) ##STR00027##
(88) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(VII):
(89) ##STR00028##
(90) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(VIII):
(91) ##STR00029##
(92) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(IX):
(93) ##STR00030##
(94) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(X):
(95) ##STR00031##
(96) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XI):
(97) ##STR00032##
(98) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XII):
(99) ##STR00033##
(100) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XIII):
(101) ##STR00034##
(102) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XIV):
(103) ##STR00035##
(104) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XV):
(105) ##STR00036##
(106) In some embodiments, in an aspect, in the compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XVI):
(107) ##STR00037##
(108) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XVII):
(109) ##STR00038##
(110) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XVIII):
(111) ##STR00039##
(112) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XIX):
(113) ##STR00040##
(114) In an aspect, the present disclosure provides a compound having chemical formula (I) wherein R.sub.4 is a carbonothioate moiety or derivative thereof, the compound having the chemical formula E(XX):
(115) ##STR00041##
(116) Referring further to the compound having chemical formula (I), R.sub.3a and R.sub.3b can be independently a hydrogen atom or a (C.sub.1-C.sub.20)-alkyl group or an aryl group, for example a phenyl group. In another embodiment, R.sub.3a and R.sub.3b are independently a hydrogen atom or a (C.sub.1-C.sub.10)-alkyl group or an aryl group, for example a phenyl group. In another embodiment, R.sub.3a and R.sub.3b are independently a hydrogen atom or a (C.sub.1-C.sub.6)-alkyl group or an aryl group, for example a phenyl group. In another embodiment, R.sub.3a and R.sub.3b are independently a hydrogen atom, a methyl group, an ethyl group, or a propyl group, or an aryl group, for example a phenyl group.
(117) Thus, to briefly recap, the present disclosure provides C.sub.4-carbonothioate-substituted tryptamine derivatives. The disclosure provides, in particular, a chemical compound having a formula (I):
(118) ##STR00042##
wherein R.sub.4 is a carbonothioate moiety or derivative thereof; and
wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group.
(119) The foregoing provides C.sub.4-carbonothioate-substituted tryptamine including a C.sub.4-carbonothioate-substituted tryptamine wherein the carbonothioate moiety or derivative thereof can have the chemical formula (III):
(120) ##STR00043##
wherein R.sub.4b is an alkyl group, a cyclo-alkyl group, or an aryl group, each of which are optionally substituted; and further including a C.sub.4-carbonothioate-substituted tryptamine wherein the carbonothioate moiety or derivative thereof can have the chemical formula (IV):
(121) ##STR00044##
wherein R.sub.4c is an alkyl group, a cyclo-alkyl group, or an aryl group, each of which are optionally substituted.
(122) In another embodiment, R.sub.3a and R.sub.3b are independently a hydrogen atom or a (C.sub.1-C.sub.20)-alkyl group or an aryl group, for example a phenyl group. In another embodiment, R.sub.3a and R.sub.3b are independently a hydrogen atom or a (C.sub.1-C.sub.10)-alkyl group or an aryl group, for example a phenyl group. In another embodiment, R.sub.3a and R.sub.3b are independently a hydrogen atom or a (C.sub.1-C.sub.6)-alkyl group or an aryl group, for example, a phenyl group. In another embodiment, R.sub.3a and R.sub.3b are independently a hydrogen atom, a methyl group, an ethyl group, or a propyl group, or an aryl group, for example a phenyl group.
(123) The C.sub.4-carbonothioate-substituted tryptamine derivatives of the present disclosure may be used to prepare a pharmaceutical or recreational drug formulation. thus, in one embodiment, the present disclosure further provides in another aspect, pharmaceutical and recreational drug formulations comprising C.sub.4-carbonothioate-substituted tryptamine derivatives. accordingly, in one aspect, the present disclosure provides in a further embodiment a pharmaceutical or recreational drug formulation comprising a chemical compound having a formula (i):
(124) ##STR00045##
wherein R.sub.4 is a carbonothioate moiety or derivative thereof; and
wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group.
(125) The pharmaceutical or recreational drug formulations may be prepared as liquids, tablets, capsules, microcapsules, nanocapsules, trans-dermal patches, gels, foams, oils, aerosols, nanoparticulates, powders, creams, emulsions, micellar systems, films, sprays, ovules, infusions, teas, decoctions, suppositories, etc. and include a pharmaceutically acceptable salt or solvate of the C.sub.4-substituted tryptamine derivative compound together with an excipient. The term “excipient” as used herein means any ingredient other than the chemical compound of the disclosure. In order to prepare a pharmaceutical drug formulation in accordance herewith, the C.sub.4-carbonothioate-substituted tryptamine derivative compounds are generally initially prepared and obtained in a substantially pure form, most preferably, at least in a 98%, 99% or 99.9% pure form, and thereafter formulated with a pharmaceutically acceptable excipient. As will readily be appreciated by those of skill in art, the selection of excipient may depend on factors such as the particular mode of administration, the effect of the excipient on solubility of the chemical compounds of the present disclosure and methods for their preparation will be readily apparent to those skilled in the art. Such compositions and methods for their preparation may be found, for example, in “Remington's Pharmaceutical Sciences”, 22.sup.nd Edition (Pharmaceutical Press and Philadelphia College of Pharmacy at the University of the Sciences, 2012).
(126) The dose when using the compounds of the present disclosure can vary within wide limits, and as is customary and is known to those of skill in the art, the dose can be tailored to the individual conditions in each individual case. The dose depends, for example, on the nature and severity of the illness to be treated, on the condition of the patient, on the compound employed or on whether an acute or chronic disease state is treated, or prophylaxis is conducted, on the mode of delivery of the compound, or on whether further active compounds are administered in addition to the compounds of the present disclosure. Representative doses of the present invention include, but are not limited to, about 0.001 mg to about 5000 mg, about 0.001 mg to about 2500 mg, about 0.001 mg to about 1000 mg, about 0.001 mg to about 500 mg, about 0.001 mg to about 250 mg, about 0.001 mg to about 100 mg, about 0.001 mg to about 50 mg, and about 0.001 mg to about 25 mg. Representative doses of the present disclosure include, but are not limited to, about 0.0001 to about 1,000 mg, about 10 to about 160 mg, about 10 mg, about 20 mg, about 40 mg, about 80 mg or about 160 mg. Multiple doses may be administered during the day, especially when relatively large amounts are deemed to be needed, for example 2, 3 or 4, doses. Depending on the subject and as deemed appropriate from the patient's physician or care giver it may be necessary to deviate upward or downward from the doses described herein.
(127) The pharmaceutical and drug formulations comprising the C.sub.4-carbonothioate-substituted tryptamine derivative compounds of the present disclosure may be administered orally. Oral administration may involve swallowing, so that the compound enters the gastrointestinal tract, or buccal or sublingual administration may be employed by which the compound enters the blood stream directly from the mouth. Formulations suitable for oral administration include both solid and liquid formulations.
(128) Solid formulations include tablets, capsules (containing particulates, liquids, microcapsules, or powders), lozenges (including liquid-filled lozenges), chews, multi- and nano-particulates, gels, solid solutions, liposomal preparations, microencapsulated preparations, creams, films, ovules, suppositories, and sprays.
(129) Liquid formulations include suspensions, solutions, syrups, and elixirs. Such formulations may be employed as fillers in soft or hard capsules and typically comprise a carrier, for example, water, ethanol, polyethylene glycol, propylene glycol, methylcellulose, or a suitable oil, and one or more emulsifying agents and/or suspending agents. Liquid formulations may also be prepared by the reconstitution of a solid, for example, from a sachet.
(130) Binders are generally used to impart cohesive qualities to a tablet formulation. Suitable binders include microcrystalline cellulose, gelatin, sugars, polyethylene glycol, natural and synthetic gums, polyvinylpyrrolidone, pregelatinized starch, hydroxypropyl cellulose and hydroxypropyl methylcellulose.
(131) Tablets may also contain diluents, such as lactose (monohydrate, spray-dried monohydrate, anhydrous and the like), mannitol, xylitol, dextrose, sucrose, sorbitol, microcrystalline cellulose, starch, and dibasic calcium phosphate dihydrate.
(132) Tablets may also optionally comprise surface active agents, such as sodium lauryl sulfate and polysorbate 80. When present, surface active agents may comprise from 0.2% (w/w) to 5% (w/w) of the tablet.
(133) Tablets may further contain lubricants such as magnesium stearate, calcium stearate, zinc stearate, sodium stearyl fumarate, and mixtures of magnesium stearate with sodium lauryl sulphate. Lubricants generally comprise from 0.25% (w/w) to 10% (w/w), from 0.5% (w/w) to 3% (w/w) of the tablet.
(134) in addition to the C.sub.4-carbonothioate-substituted tryptamine derivative compounds, tablets may contain a disintegrant. Examples of disintegrants include sodium starch glycolate, sodium carboxymethyl cellulose, calcium carboxymethyl cellulose, croscarmellose sodium, crospovidone, polyvinylpyrrolidone, methyl cellulose, microcrystalline cellulose, lower alkyl-substituted hydroxypropyl cellulose, starch, pregelatinized starch and sodium alginate. Generally, the disintegrant will comprise from 1% (w/w) to 25% (w/w) or from 5% (w/w) to 20% (w/w) of the dosage form.
(135) Other possible auxiliary ingredients include anti-oxidants, colourants, flavouring agents, preservatives, and taste-masking agents.
(136) For tablet dosage forms, depending on the desired effective amount of the chemical compound, the chemical compound of the present disclosure may make up from 1% (w/w) to 80% (w/w) of the dosage form, more typically from 5% (w/w) to 60% (w/w) of the dosage form.
(137) Exemplary tablets contain up to about 80% (w/w) of the chemical compound, from about 10% (w/w) to about 90% (w/w) binder, from about 0% (w/w) to about 85% (w/w) diluent, from about 2% (w/w) to about 10% (w/w) disintegrant, and from about 0.25% (w/w) to about 10% (w/w) lubricant.
(138) The formulation of tablets is discussed in “Pharmaceutical Dosage Forms: Tablets”, Vol. 1-Vol. 3, by CRC Press (2008).
(139) The pharmaceutical and recreational drug formulations comprising the C.sub.4-carbonothioate-substituted tryptamine derivative compound of the present disclosure may also be administered directly into the blood stream, into muscle, or into an internal organ. Thus, the pharmaceutical and recreational drug formulations can be administered parenterally (for example, by subcutaneous, intravenous, intraarterial, intrathecal, intraventricular, intracranial, intramuscular, or intraperitoneal injection). Parenteral formulations are typically aqueous solutions which may contain excipients such as salts, carbohydrates, and buffering agents (in one embodiment, to a pH of from 3 to 9), but, for some applications, they may be more suitably formulated as a sterile non-aqueous solution or as a dried form to be used in conjunction with a suitable vehicle such as sterile water.
(140) Formulations comprising the C.sub.4-carbonothioate-substituted tryptamine derivative compound of the present disclosure for parenteral administration may be formulated to be immediate and/or modified release. Modified release formulations include delayed-, sustained-, pulsed-, controlled-, targeted and programmed release. Thus, the chemical compounds of the disclosure may be formulated as a solid, semi-solid, or thixotropic liquid for administration as an implanted depot providing modified release of the active compound. Examples of such formulations include drug-coated stents and poly(dl-lactic-coglycolic)acid (PGLA) microspheres.
(141) The pharmaceutical or recreational drug formulations of the present disclosure also may be administered topically to the skin or mucosa, i.e., dermally or transdermally. Example pharmaceutical and recreational drug formulations for this purpose include gels, hydrogels, lotions, solutions, creams, ointments, dusting powders, cosmetics, oils, eye drops, dressings, foams, films, skin patches, wafers, implants, sponges, fibres, bandages and microemulsions. Liposomes may also be used. Example carriers include alcohol, water, mineral oil, liquid petrolatum, white petrolatum, glycerin, polyethylene glycol and propylene glycol. Penetration enhancers may be incorporate (see: for example, Finnin, B. and Morgan, T. M., 1999 J. Pharm. Sci, 88 (10), 955-958).
(142) Other means of topical administration include delivery by electroporation, iontophoresis, phonophoresis, sonophoresis and microneedle or needle-free (e.g., Powderject™, Bioject™, etc.) injection.
(143) Pharmaceutical and recreational drug formulations for inhalation or insufflation include solutions and suspensions in pharmaceutically acceptable, aqueous, or organic solvents, or mixtures thereof, and powders. The liquid or solid pharmaceutical compositions can contain suitable pharmaceutically acceptable excipients. In some embodiments, the pharmaceutical compositions are administered by the oral or nasal respiratory route for local or systemic effect. Pharmaceutical compositions in pharmaceutically acceptable solvents can be nebulized by use of inert gases. Nebulized solutions can be inhaled directly from the nebulizing device, or the nebulizing device can be attached to a face mask tent, or intermittent positive pressure breathing machine. Solution, suspension, or powder pharmaceutical compositions can be administered, e.g., orally, or nasally, from devices that deliver the formulation in an appropriate manner.
(144) It is noted that in some embodiments, the chemical compounds in the pharmaceutical formulation may act as pro-drugs. Pro-drugs represent a modality to control drug bioavailability, control timing of drug release, and/or reduce negative side-effects. Similarly, formulation and delivery considerations can achieve these outcomes. Thus, optimization of all three variables together (prodrug moiety, formulation, delivery system) can be an effective strategy in drug development. Examples of ‘targeting systems’ designed to specifically reach cells within the brain, obtained by simultaneously leveraging pro-drug, nanoparticle. And nasal administration strategies are described, for example by Botti et al., 2021 Pharmaceutics 13:1114).
(145) In further embodiments, in which the C.sub.4-carbonothioate-substituted tryptamine derivative compounds of present disclosure are used as a recreational drug, the compounds may be included in compositions such as a food or food product, a beverage, a food seasoning, a personal care product, such as a cosmetic, perfume or bath oil, or oils (both for topical administration as massage oil, or to be burned or aerosolized). The chemical compounds of the present disclosure may also be included in a “vape” product, which may also include other drugs, such as nicotine, and flavorings.
(146) Thus, it will be clear that the C.sub.4-carbonothioate-substituted tryptamine derivative compounds may be used as a pharmaceutical or recreational drug. Accordingly, in another aspect the present disclosure provides, in at least one embodiment, a use of a chemical compound having a formula (I):
(147) ##STR00046##
wherein R.sub.4 is a carbonothioate moiety or derivative thereof; and wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group, as a pharmaceutical or recreational drug
(148) The pharmaceutical formulations comprising the chemical compounds of the present disclosure may be used to treat a subject, and to treat a brain neurological disorder in a subject. Accordingly, the present disclosure includes in a further embodiment, a method for treating a brain neurological disorder, the method comprising administering to a subject in need thereof a pharmaceutical formulation comprising a chemical compound having a formula (I):
(149) ##STR00047##
wherein R.sub.4 is a carbonothioate moiety or derivative thereof; and wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group, wherein the pharmaceutical formulation is administered in an effective amount to treat the brain neurological disorder.
(150) Brain neurological disorders include psychiatric disorders that may be treated include, for example, neurodevelopmental disorders such as intellectual disability, global development delay, communication disorders, autism spectrum disorder, and attention-deficit hyperactivity disorder (ADHD); bipolar and related disorders, such as mania, and depressive episodes; anxiety disorder, such as generalized anxiety disorder (GAD), agoraphobia, social anxiety disorder, specific phobias (natural events, medical, animal, situational, for example), panic disorder, and separation anxiety disorder; stress disorders, such as acute stress disorder, adjustment disorders, post-traumatic stress disorder (PTSD), and reactive attachment disorder; dissociative disorders, such as dissociative amnesia, dissociative identity disorder, and depersonalization/derealization disorder; somatoform disorders, such as somatic symptom disorders, illness anxiety disorder, conversion disorder, and factitious disorder; eating disorders, such as anorexia nervosa, bulimia nervosa, rumination disorder, pica, and binge-eating disorder; sleep disorders, such as narcolepsy, insomnia disorder, hypersomnolence, breathing-related sleep disorders, parasomnias, and restless legs syndrome; disruptive disorders, such as kleptomania, pyromania, intermittent explosive disorder, conduct disorder, and oppositional defiant disorder; depressive disorders, such as disruptive mood dysregulation disorder, major depressive disorder (MDD), persistent depressive disorder (dysthymia), premenstrual dysphoric disorder, substance/medication-induced depressive disorder, postpartum depression, and depressive disorder caused by another medical condition, for example, psychiatric and existential distress within life-threatening cancer situations (ACS Pharmacol. Transl. Sci. 4: 553-562; J. Psychiatr. Res 137: 273-282); substance-related disorders, such as alcohol-related disorders, cannabis related disorders, inhalant-use related disorders, stimulant use disorders, and tobacco use disorders; neurocognitive disorders, such as delirium; schizophrenia; compulsive disorders, such as obsessive compulsive disorders (OCD), body dysmorphic disorder, hoarding disorder, trichotillomania disorder, excoriation disorder, substance/medication induced obsessive-compulsive disorder, and obsessive-compulsive disorder related to another medical condition; and personality disorders, such as antisocial personality disorder, avoidant personality disorder, borderline personality disorder, dependent personality disorder, histrionic personality disorder, narcissistic personality disorder, obsessive-compulsive personality disorder, paranoid personality disorder, schizoid personality disorder, and schizotypal personality disorder. Brain neurological disorders further include headache disorders, including migraines, including, for example, aural migraine, non-aural migraine, menstrual migraine, chronic migraine, vestibular migraine, abdominal migraine, hemiplegic migraine, and other headache disorders.
(151) In an aspect, the compounds of the present disclosure may be used to be contacted with a receptor to thereby modulate the receptor. Such contacting includes bringing a compound of the present disclosure and receptor together under in vitro conditions, for example, by introducing the compounds in a sample containing a receptor, for example, a sample containing purified receptors, or a sample containing cells comprising receptors. In vitro conditions further include the conditions described in Example 1 hereof. Contacting further includes bringing a compound of the present disclosure and receptor together under in vivo conditions. Such in vivo conditions include the administration to an animal or human subject, for example, of a pharmaceutically effective amount of the compound of the present disclosure, when the compound is formulated together with a pharmaceutically active carrier, diluent, or excipient, as hereinbefore described, to thereby treat the subject. Upon having contacted the 5 receptor, the compound may activate the receptor or inhibit the receptor.
(152) In an aspect receptors with which the compounds of the present disclosure may be contacted include, for example, the 5-HT.sub.1A receptor, the 5-HT.sub.2A receptor, the 5-HT.sub.1B receptor, the 5-HT.sub.2B receptor, the 5-HT.sub.3A receptor, the ADRA1A receptor, the ADRA2A receptor, the CHRM1 receptor, the CHRM2 receptor, the CNR1 receptor, the DRD1 receptor, the DRD2S receptor, the OPRD1 receptor, the GABAA receptor, or the NMDAR receptor.
(153) Thus, in a further aspect, the condition that may be treated in accordance herewith can be any receptor mediated disorder, including, for example, a 5-HT.sub.1A receptor-mediated disorder, a 5-HT.sub.2A receptor-mediated disorder, a 5-HT.sub.1B receptor-mediated disorder, a 5-HT.sub.2B receptor-mediated disorder, a 5-HT.sub.3A receptor-mediated disorder, a ADRA2A receptor-mediated disorder, a AVPR1A receptor-mediated disorder, a CHRM1 receptor-mediated disorder, a CHRM2 receptor-mediated disorder, a CNR1 receptor-mediated disorder, a DRD1 receptor-mediated disorder, a DRD2S receptor-mediated disorder, a OPRD1 receptor-mediated disorder, a GABAA receptor-mediated disorder, or a NMDAR receptor-mediated disorder. Such disorders include, but are not limited to schizophrenia, psychotic disorder, attention deficit hyperactivity disorder, autism, and bipolar disorder.
(154) In some embodiments, upon having contacted a receptor and a receptor, the compound may modulate the receptor. However at the same time other receptors may not be modulated. e.g., a compound may activate or inhibit a first receptor, e.g., a 5-HT.sub.1A receptor, however the compound may at the same time not modulate a second receptor, e.g., a 5-HT.sub.2A receptor, or upon having contacted a first 5-HT.sub.2A receptor and a second 5-HT.sub.1A receptor, the compound may modulate the first 5-HT.sub.2A receptor, e.g., activate or inhibit the 5-HT.sub.2A receptor, however the compound may at the same time not modulate the second 5-HT.sub.1A receptor.
(155) In one embodiment, in an aspect, upon administration the compounds of the present disclosure can interact with a transmembrane transport protein in the subject to thereby modulate the transmembrane transport protein and exert a pharmacological effect. Such contacting includes bringing a compound of the present disclosure and transmembrane protein together under in vitro conditions, for example, by introducing the compounds in a sample containing a transmembrane transport protein, for example, a sample containing a purified transmembrane transport protein, or a sample containing cells comprising a transmembrane transport protein. Contacting further includes bringing a compound of the present disclosure and a transmembrane transport protein together under in vivo conditions. Such in vivo conditions include the administration to an animal or human subject, for example, of a pharmaceutically effective amount of the compound of the present disclosure, when the compound is formulated together with a pharmaceutically active carrier, diluent, or excipient, as hereinbefore described, to thereby treat the subject.
(156) In one embodiment, in an aspect, the transmembrane transport protein can be a dopamine active transporter (DAT), a norephedrine transporter (NET) or a serotonin transporter (SERT) transmembrane transport protein.
(157) It is noted that in one embodiment, in an aspect, upon administration the compound having formula (I) may be in vivo hydrolyzed to form a compound having chemical formula (VI):
(158) ##STR00048##
wherein R.sub.3a and R.sub.3b are each independently a hydrogen atom, an alkyl group, or an aryl group,
and wherein the compound having chemical formula (VI) interacts with a receptor to thereby modulate the receptor in the subject and exert a pharmacological effect. In this respect, the compounds of the present disclosure may be formulated as a pro-drug pharmaceutical formulation, i.e., a formulation wherein it is not the formulated compound itself that mediates a pharmacological effect, but rather a compound that is obtained following in vivo hydrolyzation of the formulated compound by the subject. Hydrolyzation may occur, for example, in the gastro-intestinal tract of a person upon oral delivery of a pro-drug pharmaceutical formulation.
(159) Turning now to methods of making the C.sub.4-carbonothioate-substituted tryptamine derivative compounds of the present disclosure, it is initially noted, by way of general comment that the C.sub.4-carbonothioate-substituted tryptamine derivative compounds of the present disclosure may be prepared in any suitable manner, including by any organic chemical synthesis methods, biosynthetic methods, or a combination thereof.
(160) Examples of suitable chemical reactions that may be performed in accordance herewith are depicted in
(161) In general, as is known to those of skill in the art, in order to perform chemical synthetic reactions selected reactants are reacted under reaction conditions suitable for the reactants to chemically react with each other and form a product, i.e., the C.sub.4-carbonothioate-substituted tryptamine derivative compounds of the present disclosure. Such suitable reactions conditions may be selected, adjusted, and optimized as known by those of skill in the art. The reactions may be conducted in any suitable reaction vessel (e.g., a tube, bottle). Suitable solvents that may be used are polar solvents such as, for example, dichloromethane, dimethylformamide, dichloroethane, toluene, and so called participating solvents such as acetonitrile and diethyl ether. Suitable temperatures may range from, for example, e.g., from about −78° C. to about 60° C. Furthermore, catalysts, also known as promoters, may be included in the reaction such as iodonium dicollidine perchlorate (IDCP), any silver or mercury salts, trimethylsilyl trifluoromethanesulfonate (TMS-triflate, TMSOTf), or trifluoronmethanesulfonic acid (triflic acid, TfOH), N-iodosuccinimide, methyl triflate. Furthermore, reaction times may be varied. As will readily be appreciated by those of skill in the art, the reaction conditions may be optimized, for example, by preparing several reactant preparations and reacting these in separate reaction vessels under different reaction conditions, for example, different temperatures, using different solvents etc., evaluating the obtained C.sub.4-carboxylic acid-substituted tryptamine derivative compounds product, adjusting reaction conditions, and selecting a desired reaction condition.
(162) Referring to
(163) ##STR00049##
and the method of making the compound having formula E(VI) can involve the performance of chemical reaction (h):
(164) ##STR00050##
wherein the chemical reaction is performed under conditions suitable to convert compound 8 and form E(VI).
(165) Suitable and sufficient reaction conditions for the performance of chemical reaction (h) include conducting reaction (h) in the presence of from about 0.1 M-1.5 M tetrabutylammonium fluoride (TBAF), including for example, about 0.75, 0.9 M, 1 M, 1.1 m or 1.25 M TBAF in tetrahydrofuran (THF). Thus, for example, TBAF, may be added dropwise at 0° C., and after 30 min, water can be added, and the aqueous layer can be separated and extracted with dichloromethane DCM to obtain E(VI).
(166) Referring to
(167) Thus, in one example embodiment, preceding reaction (h), chemical reaction (g) can be performed (in the indicated consecutive (i.e., alphabetical) order).
(168) In one example embodiment, preceding reaction (h), chemical reactions (f) and (g) can be sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(169) In one example embodiment, preceding reaction (h), chemical reactions (e), (f), and (g) can be sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(170) In one example embodiment, preceding reaction (h), chemical reactions (d), (e), (f), and (g) are sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(171) In one example embodiment, preceding reaction (h), chemical reactions (c), (d), (e), (f), and (g) can be sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(172) In one example embodiment, preceding reaction (h), chemical reactions (b), (c), (d), (e), (f), and (g) can be sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(173) In one example embodiment, in preceding reaction (h), chemical reactions (a), (b), (c), (d), (e), (f), and (g) can be sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(174) Referring next to
(175) ##STR00051##
and the method of making the compound having formula E(VI) can involve the performance of chemical reaction (I):
(176) ##STR00052##
wherein the chemical reaction is performed under conditions suitable to convert compound 15 and form E(VI).
(177) Suitable and sufficient reaction conditions for the performance of chemical reaction (I) include conducting reaction (I) by adding to solution of compound 15 and potassium carbonate in dimethyl formamide (DMF), a solution of benzylchlorothioformate in DMF, and reacting reactants 15 and benzylchlorothioformate, for example, at room temperature, for example for a period of at least 6 hours, e.g., for about 6 hours, 9 hours, 12 hours, 15, hours, 18, hours or 24 hours, to form E(VI).
(178) Referring to
(179) Thus, in one example embodiment, preceding reaction (I), chemical reaction (k) is performed (in alphabetical order).
(180) In one example embodiment, preceding reaction (I), chemical reactions (j) and (k) can be sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(181) In one example embodiment, preceding reaction (I), chemical reactions (i), (j), and (k) can be sequentially performed (in the indicated consecutive (i.e., alphabetical) order).
(182) In one example embodiment, optionally preceding chemical reaction (I), reaction (m) can be performed.
(183) In some embodiments, the chemical compounds referred to herein, including, without limitation, the C.sub.4-carbonothioate-substituted tryptamine derivatives having chemical formulas E(I), E(II), E(III), E(IV), E(V), E(VI), E(VII), E(VIII), E(IX), E(X), E(XI), E(XII), E(XIII), E(XIV), E(XV), E(XVI), E(XVII), E(XVIII), E(XIX), or E(XX), may be isolated in pure or substantially pure form. Thus the compounds referred to herein may be, for example, at least 90%, 95%, 96%, 97%, or 98%, or at least 99% pure.
(184) It will now be clear from the foregoing that novel C.sub.4-carbonothioate-substituted tryptamine derivatives are disclosed herein. the C.sub.4-carbonothioate-substituted tryptamine derivatives may be formulated for use as a pharmaceutical drug or recreational drug. Example embodiments and implementations of the present disclosure are further illustrated by the following examples.
EXAMPLES
Example 1—Synthesis and Analysis of a First C.SUB.4.-Carbonothioate-Substituted Tryptamine Derivative
(185) This Example 1 initially discusses example methods for the synthesis of an example compound disclosed herein, in particular, synthesis of an example C.sub.4-carbonothioate substituted tryptamine having chemical formula E(VI) with reference to
(186) Thus, referring initially to
(187) Lithium aluminum hydride (LiAlH.sub.4) (60.2 mL, 120 mmol) (2M in THF) was added to a dry 3-neck flask under argon. The flask was fitted with a reflux condenser and an addition funnel. Dry 1,4-dioxane (100 mL) was added, and the mixture was heated to 60° C. in an oil bath. In a separate flask, compound 3 (7.46 g, 23.1 mmol) was dissolved in a mixture of THF (60 mL) and 1,4-dioxane (120 mL). With rapid stirring, this solution was added dropwise to the reaction flask over 1 h using an addition funnel. The oil bath temperature was held at 70° C. for 4 h, followed by vigorous reflux overnight (16 h) in an oil bath temperature of 95° C. The reaction was placed in an ice bath, and a solution of distilled H.sub.2O (25 mL) in THF (65 mL) was added dropwise to quench LiAlH.sub.4, resulting in a gray flocculent precipitate. Et.sub.2O (160 mL) was added to assist breakup of the complex and improve filtration. This slurry was stirred for 1 h and the mixture was then filtered using a Buchner funnel. The filter cake was washed on the filter with warm Et.sub.2O (2×200 mL) and was broken up, transferred back into the reaction flask, and vigorously stirred with additional warm Et.sub.2O (300 mL). This slurry was filtered, and the cake was washed on the filter with Et.sub.2O (120 mL) and hexane (2×120 mL). All the organic filtrates were combined and dried (MgSO.sub.4). After the drying agent was removed by filtration, the filtrate was concentrated under vacuum and dried under high vacuum. The crude residue was triturated with EtOAc/hexanes (1:9, 25 mL) to afford the crude product (4) which was used in the next step without further purification (see: reaction ©).
(188) To a solution of 4 (5.00 g, 17.0 mmol) in dry THF (100 mL) cooled to −78° C. under argon was added dropwise a 1 M solution of potassium bis(trimethylsilyl)amide (KHMDS) (18.7 mL, 18.7 mmol) in THF. After stirring at −78° C. for 1 h, a solution of triisopropylsilyl chloride (TIPSCl) (3.82 mL, 17.8 mmol) in THF (19.0 mL) was added dropwise over 15 minutes, and the reaction mixture was allowed to warm up to RT. After stirring at RT for 1 h, the reaction was quenched with H.sub.2O (40 mL), THF was evaporated under reduced pressure, and the aqueous solution was further diluted with H.sub.2O (75 mL) and extracted with DCM (3×100 mL). The organic layers were combined and washed with brine, dried over Na.sub.2SO.sub.4, filtered, and concentrated under reduced pressure. The crude product was purified by flash column chromatography (MeOH/DCM 5:95 to 10:90) to afford the pure product as a light brown oil (6.99 g, 91%). Product (5) was confirmed as follows: .sup.1H NMR (400 MHz, CDCl.sub.3) δ 7.58-7.51 (m, 2H), 7.44-7.39 (m, 2H), 7.38-7.33 (m, 1H), 7.12 (dd, J=8.4, 0.8 Hz, 1H), 7.08-6.99 (m, 1H), 6.94 (s, 1H), 6.60 (dd, J=7.7, 0.7 Hz, 1H), 5.20 (s, 2H), 3.12-3.04 (m, 2H), 2.67-2.58 (m, 2H), 2.16 (s, 6H), 1.69 (h, J=7.5 Hz, 3H), 1.16 (d, J=7.5 Hz, 18H) (see: reaction (d)).
(189) To a stirring solution of 5 (6.99 g, 15.5 mmol) dissolved in EtOH, 95% (310 mL), was added 10% palladium on carbon (1.65 g, 1.55 mmol). This mixture was put under vacuum for five minutes, then alternately purged with H.sub.2 gas until pressurized hydrogen atmosphere was established, then allowed to stir for 75 minutes at room temperature. The palladium on carbon was removed by filtration through celite, the filtrate dried with anhydrous magnesium sulphate, and concentrated under reduced pressure to yield 6 (4.67 g, 84%) as an off-white solid. Data confirming 6 are as follows: MS-ESI: calculated: 361.2670; observed: 361. 2668 m/z [M+H].sup.+. .sup.1H NMR (400 MHz, MeOD) δ 6.98 (d, J=8.6 Hz, 2H), 6.91 (dd, J=8.4, 7.5 Hz, 1H), 6.42 (dd, J=7.5, 0.8 Hz, 1H), 3.06 (t, J=6.9 Hz, 2H), 2.77 (t, J=6.9 Hz, 2H), 2.39 (s, 6H), 1.72 (p, J=7.5 Hz, 3H), 1.16 (d, J=7.5 Hz, 18H). Notably, the organosilyl substituent on N1 of compound 6 can be abbreviated as TIPS (triisopropyl silyl). Thus, compound 6 may be referred to as TIPS-psilocin (see: reaction (e)).
(190) Referring next to
(191) Compound 9 (formula E(VI)) can also be synthesized using an alternative route without production of a psilocin intermediate according to example synthesis methods depicted in
(192) It is noted that there are several ways to introduce a thiocarbonate moiety on a molecule, including: (1) formation of an activated p-nitrophenyl carbonate, followed by displacement of the p-nitrophenol with the desired thiol (see: reactions (f) and (g) in
(193) ##STR00053##
(194) Due to the presence of competing nucleophilic sites on psilocin (4-OH and indolic nitrogen), the above thiocarbonylating reagents show different reactivities towards this molecule. To obtain an optimized synthesis route for installing a thiocarbonate moiety, synthesis reactions using various reagents (e.g., compounds 11, 16) and reactions (e.g., reactions ((f), (g)), or (l)) may be conducted and compared in different synthesis routes, for example, with respect to yield, ease of operation, and a preferred reagent and reaction may be selected.
(195) It is noted that a difference between the synthesis pathway shown in
(196) Assessment of Cell Viability Upon Treatment of a Psilocin Derivative.
(197) To establish suitable ligand concentrations for competitive binding assays, PrestoBlue assays were first performed. The PrestoBlue assay measures cell viable activity based on the metabolic reduction of the redox indicator resazurin, and is a preferred method for routine cell viability assays (Terrasso et al., 2017, J. Pharmacol. Toxicol. Methods 83: 72). Results of these assays were conducted using both control ligands (e.g., psilocybin, psilocin, DMT) and novel derivatives, in part as a pre-screen for any remarkable toxic effects on cell cultures up to concentrations of 1 mM. A known cellular toxin (Triton X-100, Pyrgiotakis G. et al., 2009, Ann. Biomed. Eng. 37: 1464-1473) was included as a general marker of toxicity. Drug-induced changes in cell health within simple in vitro systems such as the HepG2 cell line are commonly adopted as first-line screening approaches in the pharmaceutical industry (Weaver et al., 2017, Expert Opin. Drug Metab. Toxicol. 13: 767). HepG2 is a human hepatoma that is most commonly used in drug metabolism and hepatotoxicity studies (Donato et al., 2015, Methods Mol Biol 1250: 77). Herein, HepG2 cells were cultured using standard procedures using the manufacture's protocols (ATCC, HB-8065). Briefly, cells were cultured in Eagle's minimum essential medium supplemented with 10% fetal bovine serum and grown at 37° C. in the presence of 5% CO.sub.2. To test the various compounds with the cell line, cells were seeded in a clear 96-well culture plate at 20,000 cells per well. After allowing cells to attach and grow for 24 hours, compounds were added at 1 mM, 10 mM, 100 mM, and 1 mM. Methanol was used as vehicle, at concentrations 0.001, 0.01, 0.1, and 1%. As a positive control for toxicity, TritonX concentrations used were 0.0001, 0.001, 0.01 and 0.1%. Cells were incubated with compounds for 48 hours before assessing cell viability with the PrestoBlue assay following the manufacture's protocol (ThermoFisher Scientific, P50200). PrestoBlue reagent was added to cells and allowed to incubate for 1 hour before reading. Absorbance readings were performed at 570 nm with the reference at 600 nm on a SpectraMax iD3 plate reader. Non-treated cells were assigned 100% viability. Bar graphs show the mean+/−SD, n=3. Significance was determined by 2-way ANOVA followed by Dunnett's multiple comparison test and is indicated by *** (P<0.0001), **(P<0.001), *(P<0.005). Data acquired for the derivative having chemical formula E(VI) is displayed as “E(VI)” on the x-axis in
(198) Radioligand Receptor Binding Assays.
(199) Activity at 5-HT.sub.2A receptor was assessed as described as follows. Evaluation of drug binding is an essential step to characterization of all drug-target interactions (Fang 2012, Exp. Opin. Drug Discov. 7:969). The binding affinity of a drug to a target is traditionally viewed as an acceptable surrogate of its in vivo efficacy (Núñez et al., 2012, Drug Disc. Today 17: 10). Competition assays, also called displacement or modulation binding assays, are a common approach to measure activity of a ligand at a target receptor (Flanagan 2016, Methods Cell Biol 132: 191). In these assays, standard radioligands acting either as agonists or antagonists are ascribed to specific receptors. In the case of G protein-coupled receptor 5-HT.sub.2A, [.sup.3H]ketanserin is a well-established antagonist used routinely in competition assays to evaluate competitive activity of novel drug candidates at the 5-HT.sub.2A receptor (Maguire et al., 2012, Methods Mol Biol 897: 31). Thus, to evaluate activity of novel C.sub.4-carbonothioate-substituted tryptamine derivatives at the 5-HT.sub.2A receptor, competition assays using [.sup.3H]ketanserin were employed as follows. SPA beads (RPNQ0010), [.sup.3H]ketanserin (NET1233025UC), membranes containing 5-HT.sub.2A (ES-313-M400UA), and isoplate-96 microplate (6005040) were all purchased from PerkinElmer. Radioactive binding assays were carried out using Scintillation Proximity Assay (SPA). For saturation binding assays, mixtures of 10 ug of membrane containing 5-HT.sub.2A receptor was pre-coupled to 1 mg of SPA beads at room temperature in a tube rotator for 1 hour in binding buffer (50 mM Tris-HCl pH7.4, 4 mM CaCl.sub.2, 1 mM ascorbic acid, 10 mM pargyline HCl). After pre-coupling, the beads and membrane were aliquoted in an isoplate-96 microplate with increasing amounts of [.sup.3H]ketanserin (0.1525 nM to 5 nM) and incubated for two hours at room temperature in the dark with shaking. After incubation, the samples were read on a MicroBeta 2 Microplate Counter (Perkin Elmer). Determination of non-specific binding was carried out in the presence of 20 mM of spiperone (S7395-250MG, Sigma). Equilibrium binding constants for ketanserin (K.sub.d) were determined from saturation binding curves using the ‘one-site saturation binding analysis’ method of GraphPad PRISM software (Version 9.2.0). Competition binding assays were performed using fixed (1 nM) [.sup.3H]ketanserin and different concentrations of tryptophan (3 nM to 1 mM), psilocin (30 pM to 10 mM) or unlabeled test compound (3 nM to 1 mM) similar to the saturation binding assay. K.sub.i values were calculated from the competition displacement data using the competitive binding analysis from GraphPad PRISM software. Tryptophan was included as a negative control as it has no activity at the 5-HT.sub.2A receptor. In contrast, psilocin was used as a positive control since it has established binding activity at the 5-HT.sub.2A receptor (Kim et al., 2020, Cell 182: 1574).
(200) Cell Lines and Control Ligands Used to Assess Activity at 5-HT.sub.1A.
(201) CHO-K1/Ga.sub.15 (GenScript, M00257) (−5-HT.sub.1A) and CHO-K1/5-HT.sub.1A/Ga.sub.15 (GenScript, M00330) (+5-HT.sub.1A) cells lines were used. Briefly, CHO-K1/Ga.sub.15 is a control cell line that constitutively expresses Ga.sub.15 which is a promiscuous G.sub.q protein. This control cell line lacks any transgene encoding 5-HT.sub.1A receptors, but still responds to forskolin; thus, cAMP response to forskolin should be the same regardless of whether or not 5-HT.sub.1A agonists are present. Conversely, CHO-K1/5-HT.sub.1A/Ga.sub.15 cells stably express 5-HT.sub.1A receptor in the CHO-K1 host background. Notably, Ga.sub.15 is a promiscuous G protein known to induce calcium flux response, present in both control and 5-HT.sub.1A cell lines. In +5-HT.sub.1A cells, Ga.sub.15 may be recruited in place of G.sub.ai/o, which could theoretically dampen cAMP response (Rojas and Fiedler 2016, Front Cell Neurosci. 10: 272). Thus, we included two known 5-HT.sub.1A agonists, psilocin (Cameron and Olson 2018, ACS Chem Neurosci. 9: 2344) and serotonin (Rojas and Fiedler 2016, Front Cell Neurosci. 10: 272) as positive controls to ensure sufficient cAMP response was observed, thereby indicating measurable recruitment of G.sub.ai/o protein to activated 5-HT.sub.1A receptors. In contrast, tryptophan is not known to activate 5-HT.sub.1A receptors, and was thus used as a negative control. Cells were maintained in complete growth media as recommended by supplier (GenScript) which is constituted as follows: Ham's F12 Nutrient mix (HAM's F12, GIBCO #11765-047) with 10% fetal bovine serum (FBS) (Thermo Scientific #12483020), 200 mg/ml zeocin (Thermo Scientific #R25005) and/or 100 mg/ml hygromycin (Thermo Scientific #10687010). The cells were cultured in a humidified incubator with 37° C. and 5% CO.sub.2. Cells maintenance was carried out as recommended by the cell supplier. Briefly, vials with cells were removed from the liquid nitrogen and thawed quickly in 37° C. water bath. Just before the cells were completely thawed the vial's outside was decontaminated by 70% ethanol spray. The cell suspension was then retrieved from the vial and added to warm (37° C.) complete growth media, and centrifuged at 1,000 rpm for 5 minutes. The supernatant was discarded, and the cell pellet was then resuspended in another 10 ml of complete growth media, and added to the 10 cm cell culture dish (Greiner Bio-One #664160). The media was changed every third day until the cells were about 90% confluent. The ˜90% confluent cells were then split 10:1 for maintenance or used for experiment.
(202) Evaluation of 5-HT.sub.1A Receptor Modulation.
(203) As 5-HT.sub.1A activation inhibits cAMP formation, the agonist activity of test molecules on 5-HT.sub.1A was measured via the reduction in the levels of cAMP produced due to application of 4 mM forskolin. The change in intracellular cAMP levels due to the treatment of novel molecules was measured using cAMP-Glo Assay kit (Promega # V1501). Briefly, +5-HT.sub.1A cells were seeded on 1-6 columns and base −5-HT.sub.1A cells were seeded on columns 7-12 of the white walled clear bottom 96-well plate (Corning, #3903). Both cells were seeded at the density of 30,000 cells/well in 100 ml complete growth media and cultured 24 hrs in humidified incubator at 37° C. and 5% CO.sub.2. On the experiment day, the media of cells was replaced with serum/antibiotic free culture media. Then the cells were treated for 20 minutes with test molecules dissolved in induction medium (serum/antibiotic free culture media containing 4 mM forskolin, 500 mM IBMX (isobutyl-1-methylxanthine, Sigma-Aldrich, Cat. #17018) and 100 mM (RO 20-1724, Sigma-Aldrich, Cat. #B8279)). Forskolin induced cAMP formation whereas IBMX and RO 20-1724 inhibited the degradation of cAMP. The level of luminescence in cells incubated with induction medium (containing 4 mM forskolin) without test molecules was normalized to represent 100% cAMP in this assay. PKA was added to the lysate, mixed, and subsequently the substrate of the PKA was added. PKA was activated by cAMP, and the amount of ATP consumed due to PKA phosphorylation directly corresponded to cAMP levels in the lysate. Reduced ATP caused reduced conversion of luciferin to oxyluciferin, conferring diminished luminescence as the result of 5-HT.sub.1A activation.
(204) In Vitro Metabolic Stability Assays Using Intestinal Fractions, Liver Fractions, Serum Fractions, Alkaline Phosphatase Buffer, Esterase Buffer, and Control Buffer.
(205) A fundamental evaluation in drug development is the assessment of absorption, distribution, metabolism, excretion, and pharmacokinetics (ADME/PK) (Eddershaw et al., 2000, Drug Discovery Today 5(9): 409-414). The first ADME screen that a novel chemical entity is subjected to is an in vitro metabolic stability screen (Ackley et al., 2004, Methods in Pharmacology and Toxicology Optimization in Drug Discovery (in vitro methods), Yan Z, Caldwell G. W. Eds; Humana Press Inc, New Jersey, pp. 151-164). Drug stability upon exposure to human liver microsomes and liver S9 cellular fractions is a common in vitro assay to approximate in vivo, liver-based drug metabolism (Richardson et al., 2016 Drug Metabolism Letters 10:83-90). First-pass metabolism is also often approximated in vitro using intestinal microsome and cellular S9 fractions (Hatley et al., 2017, Biopharmaceuticals & Drug Disposition, 38(2):155-160). Further, it is well known that human serum, and particularly circulating serum esterases can contribute to systemic drug metabolism (Williams, F M 1987, Pharmacology and Therapeutics, 34:99-109). Many pharmacological agents are classified as prodrugs, as they undergo metabolic transformation in vivo upon administration to release the active drug compound into the systemic compartment (Zawilska J B, et al. 2013, Pharmacological Reports, 65:1-14). Psilocybin, a serotonergic psychedelic agent, is well known prodrug that is metabolized into the psychoactive product, psilocin (Dinis-Oliveira, R J 2017, Drug Metabolism Reviews, 49(1):84-91). To evaluate the capacity of test molecules to similarly serve as prodrugs of psilocin, time-dependent, metabolic stability assays using human AB serum, human intestinal microsomes (HIM), human intestinal S9 fractions (HIS9), human liver microsomes (HLM), human liver S9 fractions (HLS9), human alkaline phosphatase, and porcine esterase were performed. Assays in enzyme-free buffer were also performed for control purposes, and for general assessment of compound stability. Liquid chromatography coupled mass spectrometry (LC-MS) was employed to track the conversion of the test molecules into psilocin. All intestinal and liver fractions and NADPH RapidStart reagent was purchased from Sekisui/XenoTech. Human AB serum was purchased from Sigma. For intestine and liver metabolism assays, 2.5 μM candidate compounds were incubated in 400 μg/ml of each cellular fraction (HLM, HLS9, HIM, or HIS9) in 50 mM potassium phosphate buffer (pH 7.4) containing 3 mM MgCl.sub.2 and 1 mM EDTA supplemented with NADPH RapidStart at 37° C. Samples were taken at the start of the assay, and at every 20 minutes for 2 hours. Time-point samples were precipitated with 1:1 volume of acetonitrile to quench the reaction before centrifugation at 4000×g for 20 minutes. Supernatants were analyzed for the presence of candidate prodrugs (parent molecule) and psilocin (the predicted metabolite) using Orbitrap LC-MS (Thermo Scientific) using previously described methods (Menéndez-Perdomo et al., 2021, J. Mass Spectrom., 56: e4683). The serum assays were carried out in 10% human AB serum in 50 mM potassium phosphate buffer (pH 7.4) containing 3 mM MgCl.sub.2 and 1 mM EDTA. Bovine alkaline phosphatase assays were carried out using one unit of purified enzyme in 50 mM potassium phosphate buffer (pH 7.4) containing 3 mM MgCl.sub.2 and 1 mM EDTA. Porcine esterase assays were carried out using one unit of purified enzyme in 50 mM potassium phosphate buffer (pH 7.4) containing 3 mM MgCl.sub.2 and 1 mM EDTA. Assay concentrations (μM) of both parent ‘prodrug’ molecule and psilocin metabolite, as quantified through LC-MS using routine standard curve procedures, were plotted as functions of assay time (minutes). The metabolism rate (T.sub.1/2) was determined from the metabolism curve plot using the one phase decay feature of GraphPad PRISM software (Version 9.2.0). The quantity of parent prodrug at time zero was set as 100%.
(206) Positive controls were first tested to ensure that assays were functioning properly. Psilocybin is known to be metabolized to psilocin in the intestine and through alkaline phosphatase (Dinis-Oliveira, 2017 Drug Metab. Rev. 49: 84-91) and thus served as a positive control for HIM, HIS9 and alkaline phosphatase assays. Procaine is known to be metabolized to 4-amino benzoic acid in serum, liver, and through esterase (Henrikus and Kampffmeyer, 1992, Xenobiotica 22: 1357-1366) and thus served as a positive control for AB serum, HLM and esterase assays. Verapamil is known to be metabolized into a variety of metabolites in liver (Hanada et al., 2008, Drug Metab. Dispos. 36: 2037-2042) (catabolites not examined in this study) and thus served as an additional control for HLS9 and HLM assays.
(207)
(208) In Vivo Evaluation of 5-HT.sub.2A Receptor Agonism in Mice.
(209) Drug-induced Head Twitch Response (HTR), a rapid, involuntary movement of the mouse's head with little or no involvement of the trunk, is an established in vivo model behavior used to measure neuronal 5-HT.sub.2A receptor (5-HT2AR) activation by established and novel hallucinogenic compounds (Canal and Morgan 2012, Drug Testing Analysis, 4:556-576). Indeed, HTR is widely utilized as a behavioral proxy in mice and rats to predict human hallucinogenic potential and can reliably differentiate between hallucinogenic and non-hallucinogenic 5-HT2AR agonists (Halberstadt and Geyer 2013, Psychopharmacology 227: 727-739; Gonzalez-Maeso et al., 2007, Neuron 53:439-452). To evaluate 5-HT2AR agonisms in vivo, HTR was measured in mice treated with a control and test compounds over a fixed window of time post-administration. All experiments were approved by the University of Calgary Animal Care and Use Committee in accordance with Canadian Council on Animal Care guidelines. Briefly, 8-week old C57BL/6-Elite male and female mice were obtained from Charles River. Prior to compound administration, all mice were group-housed, then single-housed on a 12:12 h light/dark schedule (lights on at 07:00 hours) with ad libitum access to food and water. Before any behavioral screening, mice were handled and exposed to the testing chamber for at least 5 min each day for three successive days and habituated to the experimental room 1 h before testing. The testing chamber was cleaned with a 70% ethanol solution between experiments. Control and test compounds, which were prepared at stock concentrations of 100 mM in DMSO, were diluted in sterile saline solution (0.9% NaCl). Prior to drug administration, mice were video monitored for 30 minutes in a plexiglass testing chamber (25.5×12.5×12.5 cm [L×W×H]) to allow for acclimation to the testing environment and to examine pre-drug spontaneous HTRs. After 30 minutes, compounds were administered via intraperitoneal (i.p.) injection at 1 mg/kg and mice were video monitored for 30 minutes then returned to their home cage. HTR analysis was conducted by an individual blinded to the subject treatment group using Behavioral Observation Research Interactive Software (BORIS, version 7, DOI: 10.1111/2041-210X.12584). Pre-drug behavior was examined during the 15-to-30-minute window prior to drug administration. Post-drug behavior was analyzed during the 15-to-30-minute window following drug administration. HTR associated with i.p. administration of psilocybin was included as a positive control measure. HTR associated with i.p. administration of vehicle (0.9% NaCl) was included as a negative control measure. Elevated incidences of HTR within the defined period of monitoring was observed in (1) psilocybin-treated mice, and (2) those treated with compound E(VI), relative to control mice treated with i.p. injected vehicle (0.9% NaCl). These results are illustrated in
(210) Mouse Pharmacokinetic (PK) Evaluation of Drug Metabolism to Psilocin.
(211) Prodrugs are molecules with little or no pharmacological activity in their own right but have a built in structural lability, whether by chance or by design, that permits bioconversion in vivo. Psilocybin was recognized as a natural prodrug of the active agent psilocin shortly after the identification and chemical synthesis of the former compound in 1957 (Coppola et al., 2022 J Xenobiot. 12: 41-52).
(212) To further explore the potential of novel C4-carboxylic acid-substituted tryptamine derivatives for use as psilocin prodrugs, a mouse PK study was performed. The aim of this study was to evaluate the time-dependent, in vivo conversion of novel derivative (“parent molecule”) to active psilocin metabolite. Specifically, the study was conducted using both PO (per os, by mouth) and IV (intravenous) dosing. Briefly, the procedure was as follows. For every compound (i.e., parent molecule), N=12 male C57Bl/6 mice were administered a single IV does (1 mg/kg) or a single oral dose (1, 3, or 10 mg/kg), with N=3 mice per dose group. Serial blood sampling via tail snip was performed at 8 time points up to 24 hours post-dosing. Samples were collected in K.sub.2EDTA tubes, plasma was separated, and all samples were frozen until bioanalysis for parent compound and psilocin metabolite. Psilocybin was also assessed as a parent compound using this same protocol to establish a control benchmark PK profile. LC-MS/MS methodology was developed for (1) each parent compound, and (2) psilocin metabolite, using a 6-8 point calibration curve in singlet (75% of standards within +/−25% accuracy (+/−25% LLOQ)). Sample processing and analysis included 96 plasma and 4 dosing solutions per compound, with two calibration curves bracketing the sample batch. Nominal analyte concentrations were calculated for dosing solutions based on the quantity of weighed analyte dissolved in exact volume of dosing solution. However, to account for any analyte instability or other confounding factors, dosing solutions were sampled by LC-MS immediately prior to animal administration to obtain “measured” analyte quantity. Measured dose was considered the same as nominal dose when the formulation concentration was within 20% of nominal concentration. However, if the measured dose was outside this window, this new “measured” dose was used in all calculations. Each mouse was designated its own number (e.g., M01, M02 . . . ). Calculated values were as follows: T.sub.max is the time at which maximum analyte concentration was observed; C.sub.max is the maximum observed concentration; Apparent t.sub.1/2 is the apparent terminal half-life; AUC.sub.0-tlast is the area under the “concentration versus time curve” from time zero to the time of the last measurable concentration; AUC.sub.0-int is the area under the “concentration versus time curve” from time zero to infinity; MRT.sub.0-inf is the mean residence time from time zero to infinity; V.sub.ss is the steady-state volume of distribution; F(%) is bioavailability=(Dose.sup.iv*AUC.sup.po)/(Dose.sup.po*AUC.sup.iv)*100. SD signifies significant deviation with N=3 unless indicated otherwise. A further detailed description of the methodology that was used to perform the foregoing mouse PK study can be found at: https://intervivo.com/pk-safety-studies/#pk-bridge; accessed Jul. 19, 2022.
(213) Results for psilocybin PK following psilocybin administration are found in Tables 1A-1B, and
(214) TABLE-US-00001 TABLE 1A Plasma concentrations of psilocybin following 1 mg/kg i.v. administration of psilocybin. ‘No Peak’ denotes no detectable compound by LC-MS; n/a denotes not applicable. Bolded value was considered an outlier and not included in calculations. Experimental Plasma concentration (ng/mL) time (h) M01 M02 M03 Mean ± SD 0.0833 19.7 76.8 334 144 ± 167 0.25 3.32 8.95 27.2 13.2 ± 12.5 0.5 No Peak 2.35 6.21 4.28 (n = 2) 1 No Peak No Peak 1.21 1.21 (n = 1) 2 No Peak No Peak No Peak n/a 4 No Peak No Peak No Peak n/a 6 No Peak No Peak No Peak n/a 8 No Peak No Peak 2.54 n/a
(215) TABLE-US-00002 TABLE 1B Summary of plasma PK parameters for psilocybin following 1 mg/kg i.v. administration of psilocybin Parameter estimate for each animal Parameter M01 M02 M03 Mean ± SD t.sub.max (h) 0.0833 0.0833 0.0833 0.0833 ± 0.00 C.sub.max (ng/mL) 19.7 76.8 334 144 ± 167
(216) TABLE-US-00003 TABLE 2A Plasma concentrations of psilocin following 1 mg/kg i.v. administration of psilocybin. Experimental Plasma concentration (ng/mL) time (h) M01 M02 M03 Mean ± SD 0.0833 76.5 106 124 102 ± 24.0 0.25 84.5 61.3 73.5 73.1 ± 11.6 0.5 43.6 43.5 62.4 49.8 ± 10.9 1 36.7 25.5 20.5 27.6 ± 8.30 2 5.16 26.9 3.16 11.7 ± 13.2 4 1.98 5.36 1.70 3.01 ± 2.04 6 4.33 2.01 0.810 2.38 ± 1.79 8 0.439 0.250 1.32 0.670 ± 0.571
(217) TABLE-US-00004 TABLE 2B Summary of plasma PK parameters for psilocin, following 1 mg/kg i.v. administration of psilocybin.sup.a. Parameter estimate for each animal Parameter M01 M02 M03 Mean ± SD t.sub.max (h) 0.250 0.0833 0.0833 0.139 ± 0.0962 C.sub.max (ng/mL) 84.5 106 124 105 ± 19.8 C.sub.max/Dose.sup.a 84.5 106 124 105 ± 19.8 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) nc.sup.b 0.905 nc 0.905 (n = 1) AUC.sub.0-tlast 84.5 109 75.5 89.8 ± 17.5 (h * ng/mL) AUC.sub.0-tlast/Dose.sup.a 84.5 109 75.5 89.8 ± 17.5 (h * kg * ng/mL/mg) AUC.sub.0-inf n/a.sup.c 110 n/a 110 (n = 1) (h * ng/mL) MRT.sub.0-inf (h) n/a.sup. 1.64 n/a 1.64 (n = 1) .sup.aPsilocybin dose was used. .sup.bnc denotes not calculable as the terminal phase is not well defined. .sup.cn/a denotes not applicable.
(218) TABLE-US-00005 TABLE 3A Plasma concentrations of psilocin following 1.56 mg/kg oral administration of psilocybin Experimental Plasma concentration (ng/mL) time (h) M04 M05 M06 Mean ± SD 0.25 50.2 53.8 29.6 44.5 ± 13.1 0.5 40.5 52.5 57.2 50.1 ± 8.61 1 26.8 31.2 37.9 32.0 ± 5.59 2 11.3 7.04 7.50 8.61 ± 2.34 4 1.64 1.86 1.25 1.58 ± 0.309 6 0.445 1.05 0.611 0.702 ± 0.313 8 1.24 0.511 0.738 0.830 ± 0.373 24 BLQ BLQ BLQ n/a BLQ denotes below the ower limit of quantitation (0.2 ng/mL). n/a denotes not applicable.
(219) TABLE-US-00006 TABLE 3B Summary of plasma PK parameters for psilocin, following 1.56 mg/kg oral administration of psilocybin.sup.a. Parameter estimate for each animal Parameter M04 M05 M06 Mean ± SD t.sub.max (h) 0.250 0.250 0.500 0.333 ± 0.144 C.sub.max (ng/mL) 50.2 53.8 57.2 53.7 ± 3.50 C.sub.max/Dose.sup.a 32.2 34.5 36.7 34.4 ± 2.24 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) nc.sup.b 2.15.sup.c nc 2.15 (n = 1) AUC.sub.0-tlast (h * ng/mL) 65.6 68.8 66.9 67.1 ± 1.61 AUC.sub.0-tlast/Dose.sup.a 42.1 44.1 42.9 43.0 ± 1.03 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/mL) n/a.sup.d 70.4 n/a 70.4 (n = 1) MRT.sub.0-inf (h) n/a 1.53 n/a 1.53 (n = 1) .sup.aAdministered dose of psilocybin (1.56 mg/kg) was used. .sup.bnc denotes not calculable as the terminal phase is not well defined. .sup.cApparent t.sub.1/2 estimate may not be accurate; sampling interval during the terminal phase <2 × t.sub.1/2. .sup.dn/a denotes not applicable.
(220) TABLE-US-00007 TABLE 4A Plasma concentrations of psilocin following 3 mg/kg oral administration of psilocybin. Experimental Plasma concentration (ng/mL) time (h) M07 M08 M09 Mean ± SD 0.25 52.6 53.0 41.5 49.0 ± 6.53 0.5 55.3 62.0 35.0 50.8 ± 14.1 1 23.2 35.5 36.2 31.6 ± 7.31 2 13.1 10.5 23.2 15.6 ± 6.71 4 2.28 1.93 3.16 2.46 ± 0.634 6 1.43 1.04 1.79 1.42 ± 0.375 8 0.734 0.368 0.493 0.532 ± 0.186 24 BLQ 0.111 0.402 0.257 (n = 2) BLQ denotes below the lower limit of quantitation (0.2 ng/mL). Value in italics is below the lower limit of quantitation (BLQ, 0.2 ng/mL) but was included in calculations.
(221) TABLE-US-00008 TABLE 4B Summary of plasma PK parameters for psilocin, following 3 mg/kg oral administration of psilocybin.sup.a. Parameter estimate for each animal Parameter M07 M08 M09 Mean ± SD t.sub.max (h) 0.500 0.500 0.250 0.417 ± 0.144 C.sub.max (ng/mL) 55.3 62.0 41.5 52.9 ± 10.5 C.sub.max/Dose.sup.a 18.4 20.7 13.8 17.6 ± 3.48 (kg * ng/mL/mg) Apparent t.sub.1/2 (h).sup.b 2.45 6.58 nc.sup.c 4.51 (n = 2) AUC.sub.0-tlast (h * ng/mL) 74.3 83.0 95.8 84.4 ± 10.8 AUC.sub.0-tlast/Dose.sup.a 24.8 27.7 31.9 28.1 ± 3.61 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/mL) 76.9 84.1 n/a.sup.d 80.5 (n = 2) MRT.sub.0-inf (h) 1.84 2.24 n/a.sup. 2.04 (n = 2) .sup.aPsilocybin dose was used. .sup.bFor M07, apparent t.sub.1/2 estimate may not be accurate; sampling interval during the terminal phase <2 × t.sub.1/2. .sup.c nc denotes not calculable as the terminal phase is not well defined. .sup.dn/a denotes not applicable.
(222) TABLE-US-00009 TABLE 5A Plasma concentrations of psilocin following 10 mg/kg oral administration of psilocybin. Experimental Plasma concentration (ng/mL) time (h) M10 M11 M12 Mean ± SD 0.25 238 234 202 225 ± 19.7 0.5 202 289 156 216 ± 67.5 1 145 156 166 156 ± 10.5 2 53.9 54.7 66.6 58.4 ± 7.11 4 8.32 23.5 10.2 14.0 ± 8.28 6 3.51 16.8 10.3 10.2 ± 6.65 8 3.13 5.18 7.06 5.12 ± 1.97 24 0.258 0.201 0.186 0.215 ± 0.0380 BLQ denotes below the lower limit of quantitation (0.2 ng/ml). Value in italics is below the lower limit of quantitation (BLQ, 0.2 ng/mL) but was included in calculations.
(223) TABLE-US-00010 TABLE 5B Summary of plasma PK parameters for psilocin following 10 mg/kg oral administration of psilocybin.sup.a. Parameter estimate for each animal Parameter M10 M11 M12 Mean ± SD t.sub.max (h) 0.250 0.500 0.250 0.333 ± 0.144 C.sub.max (ng/mL) 238 289 202 243 ± 43.7 C.sub.max/Dose.sup.a 23.8 28.9 20.2 24.3 ± 4.37 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) 4.64 3.02 3.09 3.58 ± 0.920 AUC.sub.0-tlast (h * ng/mL) 348 457 387 397 ± 55.5 AUC.sub.0-tlast/Dose.sup.a 34.8 45.7 38.7 39.7 ± 5.55 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/ml) 349 458 388 398 ± 55.1 MRT.sub.0-inf (h) 2.14 2.44 2.60 2.39 ± 0.236 .sup.aPsilocybin dose was used.
(224) TABLE-US-00011 TABLE 6 Summary of mean plasma exposure of psilocin as a function of psilocybin dose. Psilocybin dose 1 mg/kg 1.56 mg/kg 3 mg/kg 10 mg/kg Parameter i.v. p.o. p.o. p.o. C.sub.max/Dose.sup.a 105 ± 19.8 34.4 ± 2.24 17.6 ± 3.48 24.3 ± 4.37 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) 0.905 (n = 1) 2.15 (n = 1) 4.51 (n = 2) 3.58 ± 0.920 AUC.sub.0-tlast/Dose.sup.a 89.8 ± 17.5 43.0 ± 1.03 28.1 ± 3.61 39.7 ± 5.55 (h * kg * ng/mL/mg)
(225) Results for compound E(VI) PK following E(VI) administration are found in Tables 7A and 7B. Notably, only plasma from animals intravenously administered E(VI) revealed detectable levels of E(VI). Conversely, plasma from animals orally administered E(VI) did not yield any detectable levels of E(VI). As seen in Tables 7A and 7B, mean E(VI) plasma concentrations were associated with relatively high standard deviations (SD), perhaps resulting from difficulties in quantitation (see Table 7A notes).
(226) TABLE-US-00012 TABLE 7A Plasma concentrations of E(VI) following 1 mg/kg i.v. administration of E(VI). Experimental Plasma concentration (ng/mL).sup.a time (h) M13 M14 M15 Mean ± SD 0.0833 3.20 59.0 11.1 24.4 ± 30.2 0.25 72.1 110 7.79 63.3 ± 51.7 0.5 13.1 9.29 1.03 7.81 ± 6.17 1 3.14 5.84 No Peak 4.49 (n = 2) 2 0.776 0.594 No Peak 0.685 (n = 2) 4 BLQ BLQ No Peak n/a 6 No Peak BLQ No Peak n/a 8 No Peak No Peak No Peak n/a .sup.afreshly spiked calibration curve was used for quantification as E(VI) is not stable in plasma; concentrations are not considered accurate. Values in italics are below the lower limit of quantitation (BLQ, 1 ng/mL) but were included in calculations. BLQ denotes below the lower limit of quantitation (1 ng/mL). n/a denotes not applicable.
(227) TABLE-US-00013 TABLE 7B Summary of plasma PK parameters for E(VI) following 1 mg/kg i.v. administration of E(VI). Parameter estimate for each animal Parameter M13 M14 M15 Mean ± SD C.sub.0 (ng/mL) 3.20 59.0 13.2 25.1 ± 29.7 Apparent t.sub.1/2 (h) 0.382 0.365 nc.sup.a 0.374 ± 0.0118 AUC.sub.0-tlast (h * ng/mL) 20.4 35.2 3.40 19.7 ± 15.9 AUC.sub.0-tlast/Dose 20.4 35.2 3.40 19.7 ± 15.9 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/mL) 20.8 35.5 .sup. n/a.sup.b 28.2 (n = 2) CL (mL/h/kg) 48084 28159 n/a 38100 (n = 2) MRT.sub.0-inf (h) 0.497 0.360 n/a 0.429 (n = 2) V.sub.ss (mL/kg) 23899 10146 n/a 17000 (n = 2) .sup.an/c denotes not calculable as terminal phase is not well defined. .sup.bn/a denotes not applicable.
Results for psilocin PK following E(VI) administration are found in Tables 8A-8B (1 mg/kg IV dose), Tables 9A-9B (1 mg/kg oral dose), Tables 10A-10B (3 mg/kg oral dose), Tables 11A-11B (10 mg/kg oral dose), Table 12 (comparative summary for IV data), Table 13 (comparative summary for oral data), Table 14 (psilocin exposure) and
(228) TABLE-US-00014 TABLE 8A Plasma concentrations of psilocin following 1 mg/kg i.v. administration of E(VI) Experimental time (h) M13 M14 M15 Mean ± SD 0.0833 732 882 47.4 554 ± 445 0.25 408 363 41.0 271 ± 200 0.5 82.6 91.7 25.8 66.7 ± 35.7 1 31.4 36.3 6.56 24.8 ± 15.9 2 8.50 5.03 1.31 4.95 ± 3.60 4 4.07 1.53 0.313 1.97 ± 1.92 6 0.712 1.38 0.132 0.741 ± 0.625 8 0.160 3.32 0.136 1.21 ± 1.83 Values in italics are below the lower limit of quantitation (BLQ, 0.2 ng/mL) but were included in calculations.
(229) TABLE-US-00015 TABLE 8B Summary of plasma PK parameters for Psilocin following 1 mg/kg i.v. administration of MM590 (Group 5). Parameter estimate for each animal Parameter M13 M14 M15 Mean ± SD t.sub.max (h) 0.0833 0.0833 0.0833 0.0833 ± 0.00 C.sub.max (ng/mL) 732 882 47.4 554 ± 445 C.sub.max/Dose.sup.a 732 882 47.4 554 ± 445 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) 0.857 nc.sup.b 1.81 1.33 (n = 2) AUC.sub.0-tlast (h * ng/mL) 234 243 29.9 169 ± 121 AUC.sub.0-tlast/Dose.sup.a 234 243 29.9 169 ± 121 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/mL) 235 n/a.sup.b 30.3 132 (n = 2) MRT.sub.0-inf (h) 0.586 n/a.sup. 0.835 0.711 (n = 2) .sup.aMM590 dose was used. .sup.bn/c denotes not calculable as terminal phase is not well defined. .sup.cn/a denotes not applicable.
(230) TABLE-US-00016 TABLE 9A Plasma concentrations of psilocin following 1 mg/kg oral administration of E(VI). Experimental Plasma concentration (ng/mL) time (h) M16 M17 M18 Mean ± SD 0.25 8.32 5.06 6.75 6.71 ± 1.63 0.5 4.64 5.14 5.91 5.23 ± 0.640 1 3.64 3.66 2.60 3.30 ± 0.606 2 1.56 2.52 1.75 1.94 ± 0.508 4 0.752 0.466 0.608 0.609 ± 0.143 6 0.348 0.183 0.767 0.433 ± 0.301 8 0.149 BLQ 0.227 0.188 (n = 2) 24 No Peak No Peak No Peak n/a BLQ denotes below the lower limit of quantitation (0.2 ng/mL). Values in italics are below the lower limit of quantitation (BLQ, 0.2 ng/mL) but were included in calculations. n/a denotes not applicable.
(231) TABLE-US-00017 TABLE 9B Summary of plasma PK parameters for psilocin following 1 mg/kg oral administration of E(VI). Parameter estimate for each animal Parameter M16 M17 M18 Mean ± SD t.sub.max (h) 0.250 0.500 0.250 0.333 ± 0.144 C.sub.max (ng/mL) 8.32 5.14 6.75 6.74 ± 1.59 C.sub.max/Dose.sup.a 8.32 5.14 6.75 6.74 ± 1.59 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) 1.71 1.06 2.21 1.66 ± 0.577 AUC.sub.0-tlast (h * ng/mL) 10.9 10.2 11.0 10.7 ± 0.442 AUC.sub.0-tlast/Dose.sup.a 10.9 10.2 11.0 10.7 ± 0.442 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/mL) 11.2 10.5 11.7 11.1 ± 0.641 MRT.sub.0-inf (h) 2.18 1.76 2.78 2.24 ± 0.515 aMM590 dose was used.
(232) TABLE-US-00018 TABLE 10A Plasma concentrations of psilocin following 3 mg/kg oral administration of E(VI). Experimental Plasma concentration (ng/mL) time (h) M19 M20 M21 Mean ± SD 0.25 25.7 13.5 23.3 20.8 ± 6.46 0.5 30.5 22.6 18.0 23.7 ± 6.32 1 13.2 11.0 8.57 10.9 ± 2.32 2 3.39 5.39 3.60 4.13 ± 1.10 4 1.02 1.21 1.70 1.31 ± 0.351 6 0.233 0.763 1.16 0.719 ± 0.465 8 0.152 0.512 0.844 0.503 ± 0.346 24 No Peak BLQ No Peak n/a BLQ denotes below the lower limit of quantitation (0.2 ng/mL). Value in italics is below the lower limit of quantitation (BLQ, 0.2 ng/mL) but was included in calculations. n/a denotes not applicable.
(233) TABLE-US-00019 TABLE 10B Summary of plasma PK parameters for psilocin following 3 mg/kg oral administration of E(VI). Parameter estimate for each animal Parameter M19 M20 M21 Mean ± SD t.sub.max (h) 0.500 0.500 0.250 0.417 ± 0.144 C.sub.max (ng/mL) 30.5 22.6 23.3 25.5 ± 4.37 C.sub.max/Dose.sup.a 10.2 7.53 7.77 8.49 ± 1.46 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) 1.28 1.84 2.93 2.02 ± 0.836 AUC.sub.0-tlast (h * ng/mL) 33.2 30.9 30.0 31.4 ± 1.63 AUC.sub.0-tlast/Dose.sup.a 11.1 10.3 10.0 10.5 ± 0.544 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/mL) 33.5 33.3 34.8 33.9 ± 0.835 MRT.sub.0-inf (h) 1.27 2.09 3.02 2.13 ± 0.874 .sup.aMM590 dose was used. .sup.bFor M20 and M21, apparent t.sub.1/2 estimate may not be accurate; sampling interval during the terminal phase <2 × t.sub.1/2
(234) TABLE-US-00020 TABLE 11A Plasma concentrations of psilocin following 10 mg/kg oral administration of E(VI). Experimental Plasma concentration (ng/mL) time (h) M22 M23 M24 Mean ± SD 0.25 53.8 34.9 78.6 55.8 ± 21.9 0.5 66.2 61.1 113 80.1 ± 28.6 1 41.7 43.6 45.2 43.5 ± 1.75 2 32.0 23.6 15.1 23.6 ± 8.45 4 5.58 4.19 2.62 4.13 ± 1.48 6 1.24 8.11 3.34 4.23 ± 3.52 8 0.764 4.19 4.24 3.06 ± 1.99 24 BLQ BLQ BLQ n/a BLQ denotes below the lower limit of quantitation (0.2 ng/mL). n/a denotes not applicable.
(235) TABLE-US-00021 TABLE 11B Summary of plasma PK parameters for psilocin following 10 mg/kg oral administration of E(VI). Parameter estimate for each animal Parameter M22 M23 M24 Mean ± SD t.sub.max (h) 0.500 0.500 0.500 0.500 ± 0.00 C.sub.max (ng/mL) 66.2 61.1 113 80.1 ± 28.6 C.sub.max/Dose.sup.a 6.62 6.11 11.3 8.01 ± 2.86 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) 1.39 nc.sup.b nc 1.39 (n = 1) AUC.sub.0-tlast (h * ng/mL) 123 122 126 123 ± 2.31 AUC.sub.0-tlast/Dose.sup.a 12.3 12.2 12.6 12.3 ± 0.231 (h * kg * ng/mL/mg) AUC.sub.0-inf (h * ng/mL) 124 n/a.sup.c n/a 124 (n = 1) MRT.sub.0-inf (h) 1.77 n/a.sup. n/a 1.77 (n = 1) .sup.aMM590 dose was used. .sup.bn/c denotes not calculable as terminal phase is not well defined. .sup.cn/a denotes not applicable.
(236) TABLE-US-00022 TABLE 12 Summary of mean plasma exposure of psilocin as a function of E(VI). MM590 dose 1 mg/kg 1 mg/kg 3 mg/kg 10 mg/kg Parameter i.v. p.o. p.o. p.o. C.sub.max/Dose.sup.a 554 ± 445 6.74 ± 1.59 8.49 ± 1.46 8.01 ± 2.86 (kg * ng/ml/mg) Apparent t.sub.1/2 (h) 1.33 (n = 2) 1.66 ± 0.577 2.88 ± 1.29 1.39 (n = 1) AUC.sub.0-tlast/Dose.sup.a 169 ± 121 10.7 ± 0.442 10.5 ± 0.544 12.3 ± 0.231 (h * kg * ng/mL/mg) .sup.aMM590 dose.
In Vitro Survey of Pharmacological Interaction Profiles at Receptors, Transporters and Enzymes Linked to Targeted Health Conditions.
(237) To expand pharmacological profiling to include a broader range of targets with known involvement in, or connection to, brain neurological disorders, compound E(VI) was evaluated with respect to receptor interaction (https://www.eurofinsdiscoveryservices.com/). Specifically, the cell-based screening assay panel known as “SAFETYscan E/IC150 ELECT” was used to generate data regarding interaction of derivative molecules with 20 different proteins, including 12 GPCR receptors (ADRA1A, ADRA2A, AVPR1A, CHRM1, CHRM2, CNR1, DRD1, DRD2S, HTR1A (5-HT.sub.1A), HTR1B (5-HTR.sub.1B), HTR2B (5-HT.sub.2B), OPRD1), 3 ion channels (GABAA, HTR3A (5-HT.sub.3A), NMDAR), one enzyme (MAO-A), and 3 transporters (DAT, NET, SERT).
(238) i. EFC-Based cAMP Secondary Messenger Assay.
(239) Of the 12 GPCR proteins, 8 were assayed via a cAMP secondary messenger assay: ADRA2A, CHRM2, CNR1, DRD1, DRD2S, HTR1A, HTR1B, OPRD1. Briefly, employed a panel of cell lines stably expressing non-tagged GPCR proteins that endogenously signal through cAMP. These assays monitored the activation of a GPCR through G.sub.i or G.sub.s secondary messenger signaling in a homogenous, non-imaging assay format using a technology termed Enzyme Fragment Complementation (EFC). EFC uses β-galactosidase (β-gal) as the functional endpoint. The β-gal enzyme is split into two complementary portions: Enzyme Acceptor (EA) and Enzyme Donor (ED). In the assay, exogenously introduced ED fused to cAMP (ED-cAMP) competes with endogenously generated cAMP for binding to an anti-cAMP-specific antibody. Active β-gal is formed by complementation of exogenous EA to any unbound ED-cAMP. Active enzyme can then convert a chemiluminescent substrate, generating an output signal detectable on a standard microplate reader.
(240) These 8 cAMP-based assays were conducted in both agonist and antagonist modes, either in G.sub.s format (no forskolin) or in G.sub.i format (in the presence of EC.sub.80 forskolin). For G.sub.s and G.sub.i agonist assays: cell media was aspirated from GPCR-containing cultures and replaced with 15 μl 2:1HBSS/1-mM HEPES:cAMP XS+Ab reagent. Five microlitres of derivative compound, prepared as a stock solution (also containing EC.sub.80 forskolin in the case of G.sub.i format) were added to the cells at final target concentrations and pre-incubated for 30 minutes. Final assay vehicle concentration was 1%. After pre-incubation, assay signal was generated through the addition of (1) 20 μL cAMP XS+ED/CL lysis cocktail, and (2) 20 μL cAMP XS+EA reagent, allowing incubation periods of one and three hours, respectively. Antagonist assays were performed in the same manner as agonist assays, except pre-incubation entailed exposure to the test derivative (30 minutes) followed by exposure to an established agonist at EC.sub.80 (“agonist challenge”, 30 minutes). In the case of antagonist assays of G.sub.i-coupled GPCRs, EC.sub.80 forskolin was included in assay buffers.
(241) In all 8 cAMP assays (agonist or antagonist mode), the resulting chemiluminescent signal was measured using a PerkinElmer Envision™ instrument. Compound activity was analyzed using CBIS data analysis suite (ChemInnovation, CA). Percent activity (%) was calculated according to standard procedures. For example: in G.sub.s agonist mode assays, percentage activity was calculated using the following formula: % activity=100%×[mean RLU of test derivative−mean RLU of vehicle control]/[mean RLU of control ligand−mean RLU of vehicle control]. For G.sub.s antagonist mode assays, percentage inhibition was calculated using the following formula: % inhibition=100%×[1−[mean RLU of test derivative−mean RLU of vehicle control]/[mean RLU of EC.sub.80 control ligand−mean RLU of vehicle control]]. For G.sub.i agonist mode assays, percentage activity was calculated using the following formula: % activity=100%×[1−[mean RLU of test derivative−mean RLU of control ligand]/[mean RLU of vehicle control−mean RLU of control ligand]]. For G.sub.i antagonist or negative allosteric mode assays, percentage inhibition was calculated using the following formula: % inhibition=100%×[mean RLU of test compound−mean RLU of EC.sub.80 control ligand]/[mean RLU of forskolin positive control−mean RLU of EC.sub.80 control]. For primary screens, percent response was capped at 0% or 100% where calculated percent response returned a negative value or a value greater than 100, respectively. To assess assay performance and establish positive control benchmarks, ligands listed in Table 13 were evaluated alongside test derivatives. Results for EFC-based cAMP secondary messenger assays on GPCRs using compound E(VI) ligand or positive controls are shown in Table 14.
(242) ii. Calcium Secondary Messenger Assay.
(243) Of the 12 GPCR proteins, 4 were assayed via a calcium secondary messenger assay: ADRA1A, AVPR1A, CHRM1, HTR2B. Briefly, the Calcium No WashPLUS assay monitors GPCR activity via G.sub.q secondary messenger signaling in a live cell, non-imaging assay format. Eurofins DiscoverX employed proprietary cell lines stably expressing G.sub.q-coupled GPCR proteins. Calcium mobilization was monitored using a calcium-sensitive dye loaded into cells. GPCR activation by a test or control compound resulted in the release of calcium from intracellular stores and an increase in dye fluorescence that is measured in real-time.
(244) The four GPCR proteins assayed via calcium secondary messenger assay were surveyed in both agonist and antagonist modes. Cell lines were expanded from freezer stocks according to standard procedures, seeded into microplates and incubated at 37° C. prior to testing. Assays were performed in 1× dye loading buffer consisting of 1× dye (DiscoverX, Calcium No WashPLUS kit, Catalog No. 90-0091), 1× Additive A and 2.5 mM probenecid in HBSS/20 mM Hepes. Cells were loaded with dye prior to testing. Media was aspirated from cells and replaced with 25 μL dye loading buffer, incubated for 45 minutes at 37° C. and then 20 minutes at room temperature. For agonist determination, cells were incubated with sample compound to induce response. After dye loading, cells were removed from the incubator and 25 μL of 2× compound in HBSS/20 mM Hepes was added using a FLIPR Tetra (MDS). Compound agonist activity was measured on a FLIPR Tetra. Calcium mobilization was monitored for 2 minutes with a 5 second baseline read. For antagonist determination, cells were pre-incubated with sample compound followed by agonist challenge at the EC.sub.80 concentration. After dye loading, cells were removed from the incubator and 25 μL 2× sample compound was added. Cells were incubated for 30 minutes at room temperature in the dark to equilibrate plate temperature. After incubation, antagonist determination was initiated with addition of 25 μL 1× derivative compound with 3× EC.sub.80 agonist using FLIPR. Compound antagonist activity was measured on a FLIPR Tetra (MDS). Calcium mobilization was monitored for 2 minutes with a 5 second baseline read. In both agonist and antagonist modes, data analysis was initiated using FLIPR, where area under the curve was calculated for the entire two minute read. Compound activity was analyzed using CBIS data analysis suite (ChemInnovation, CA). For agonist mode assays, percentage activity was calculated using the following formula: % activity=100%×[mean RFU of test compound−mean RFU of vehicle control]/[mean RFU control ligand−mean RFU of vehicle control]. For antagonist mode assays, percentage inhibition was calculated using the following formula: % inhibition=100%×[1−[mean RFU of test compound−mean RFU of vehicle control]/[mean RFU of EC.sub.80 control−mean RFU of vehicle control]]. For primary screens, percent response was capped at 0% or 100%, where calculated percent response returned a negative value or a value greater than 100, respectively. To assess assay performance and establish positive control benchmarks, ligands listed in Table 13 were evaluated alongside test derivatives. Results for EFC-based cAMP secondary messenger assays on GPCRs using compound E(VI) ligand or positive controls are shown in Table 14.
(245) iii. Ion Channel Assays.
(246) Both ‘blocker’ and ‘opener’ activities of putative ligands on three distinct ion channels (GABAA, HTR3A, NMDAR) were surveyed. Briefly, Eurofins DiscoverX was employed in conjunction with the FLIPR Membrane Potential Assay Kit (Molecular Devices) which utilizes a proprietary fluorescent indicator dye in combination with a quencher to reflect real-time membrane potential changes associated with ionchannel activation and ion transporter proteins. Unlike traditional dyes such as DiBAC, the FLIPR Membrane Potential Assay Kit detects bidirectional ion fluxes so both variable and control conditions can be monitored within a single experiment. Cell lines were expanded from freezer stocks according to standard procedures, seeded onto microplates, and incubated at 37° C. Assays were performed in 1× Dye Loading Buffer consisting of 1× Dye and 2.5 mM probenecid when applicable. Cells were loaded with dye prior to testing and incubated for 30-60 minutes at 37° C. For agonist (‘Opener’) assays, cells were incubated with sample (i.e., containing derivative or control compound; Table 13) to induce response as follows. Dilution of sample stocks was performed to generate 2-5× sample (i.e., containing derivative or control compound) in assay buffer. Next, 10-25 μL of 2-5× sample was added to cells and incubated at 37° C. or room temperature for 30 minutes. Antagonist (‘Blocker’) assays were performed using the same procedure except that after dye loading, cells were removed from the incubator and 10-25 μL 2-5× sample (i.e., containing derivative or control compound) was added to cells in the presence of EC.sub.80 agonist. Cells were incubated for 30 minutes at room temperature in the dark to equilibrate plate temperature. Compound activity was measured on a FLIPR Tetra (Molecular Devices). Compound activity was analyzed using CBIS data analysis suite (ChemInnovation, CA). For agonist mode assays, percentage activity was calculated using the following formula: % activity=100%×[mean RLU of test derivative−mean RLU of vehicle control]/[mean control ligand−mean RLU of vehicle control]. For antagonist mode, percentage inhibition was calculated using the following formula: % inhibition=100%×[1−[mean RLU of test derivative−mean RLU of vehicle control]/[mean RLU of EC.sub.80 control−mean RLU of vehicle control]]. For primary screens, percent response was capped at 0% or 100% where calculated percent response returned a negative value or a value greater than 100, respectively. To assess assay performance and establish positive control benchmarks, ligands listed in Table 13 were evaluated alongside test derivatives. Results for EFC-based cAMP secondary messenger assays on GPCRs using compound E(VI) ligand or positive controls are shown in Table 14.
(247) iv. Neurotransmitter Transporter Uptake Assays.
(248) The Neurotransmitter Transporter Uptake Assay Kit from Molecular Devices was used to examine impact of test compounds on 3 distinct transporters (DAT, NET, SERT). This kit provided a homogeneous fluorescence-based assay for the detection of dopamine, norepinephrine or serotonin transporter activity in cells expressing these transporters. The kit employed a fluorescent substrate that mimics the biogenic amine neurotransmitters that are taken into the cell through the specific transporters, resulting in increased intracellular fluorescence intensity. Cell lines were expanded from freezer stocks according to standard procedures, seeded into microplates and incubated at 37° C. prior to testing. Assays were performed in 1× Dye Loading Buffer consisting of 1× Dye, and 2.5 mM probenecid as applicable. Next, cells were loaded with dye and incubated for 30-60 minutes at 37° C. “Blocker” or antagonist format assays were performed, where cells were pre-incubated with sample (i.e., containing sample derivative or positive control compound) as follows. Dilution of sample stocks (i.e., containing sample derivative or positive control compound; Table 13) was conducted to generate 2-5× sample in assay buffer. After dye loading, cells were removed from the incubator and 10-25 μL 2-5× sample (i.e., containing sample derivative or positive control compound) was added to cells in the presence of EC.sub.80 agonist as appropriate. Cells were incubated for 30 minutes at room temperature in the dark to equilibrate plate temperature. Compound activity was measured on a FLIPR Tetra (Molecular Devices), and activity was analyzed using CBIS data analysis suite (ChemInnovation, CA). For antagonist (‘Blocker’) mode, percentage inhibition was calculated using the following formula: % inhibition=100%×[1−[mean RLU of test sample−mean RLU of vehicle control]/[mean RLU of EC.sub.80 control−mean RLU of vehicle control]]. For primary screens, percent response was capped at 0% or 100% where calculated percent response returned a negative value or a value greater than 100, respectively. To assess assay performance and establish positive control benchmarks, ligands listed in Table 13 were evaluated alongside test derivative. Results for EFC-based cAMP secondary messenger assays on GPCRs using compound E(VI) ligand or positive controls are shown in Table 14.
(249) v. MAO-A Enzyme Assay.
(250) For the MAO-A assay, all chemicals and enzyme preparations were sourced from Sigma. Briefly, enzyme and test compound (i.e., derivative or control compound; see Table 13) were preincubated for 15 minutes at 37° C. before substrate addition. The reaction was initiated by addition of kynuramine and incubated at 37° C. for 30 minutes. The reaction was terminated by addition of NaOH. The amount of 4-hydroquioline formed was determined through spectrofluorimetric readout with the emission detection at 380 nm and excitation wavelength 310 nm. For each assay, microplates were transferred to a PerkinElmer Envision™ instrument for readouts as per standard procedures. Compound activity was analyzed using CBIS data analysis suite (ChemInnovation, CA). Percentage inhibition was calculated using the following formula: % inhibition=100%×[1−[mean RLU of test sample−mean RLU of vehicle control]/[mean RLU of positive control−mean RLU of vehicle control]]. For primary screens, percent response was capped at 0% or 100% where calculated percent response returned a negative value or a value greater than 100, respectively. To assess assay performance and establish positive control benchmarks, ligands listed in Table 13 were evaluated alongside test derivative. Results for EFC-based cAMP secondary messenger assays on GPCRs using compound E(VI) ligand or positive controls are shown in Table 14.
(251) TABLE-US-00023 TABLE 13 Control ligands used for target assays (GPCR, G-protein coupled receptor; IC, ion channel; EN, enzyme; TR, transporter). Target Assay Type Control ligand/modulator ADRA1A Agonist GPCR A 61603 Hydrobromide ADRA1A Antagonist GPCR Tamsulosin ADRA2A Agonist GPCR UK 14304 ADRA2A Antagonist GPCR Yohimbine AVPR1A Agonist GPCR [Arg8]-Vasopressin AVPR1A Antagonist GPCR SR 49059 CHRM1 Agonist GPCR Acetylcholine chloride CHRM1 Antagonist GPCR Atropine CHRM2 Agonist GPCR Acetylcholine chloride CHRM2 Antagonist GPCR Atropine CNR1 Agonist GPCR CP 55940 CNR1 Antagonist GPCR AM 251 DRD1 Agonist GPCR Dopamine DRD1 Antagonist GPCR SCH 39166 DRD2S Agonist GPCR Dopamine DRD2S Antagonist GPCR Risperidone HTR1A Agonist GPCR Serotonin hydrochloride HTR1A Antagonist GPCR Spiperone HTR1B Agonist GPCR Serotonin hydrochloride HTR1B Antagonist GPCR SB 224289 HTR2B Agonist GPCR Serotonin hydrochloride HTR2B Antagonist GPCR LY 272015 OPRD1 Agonist GPCR DADLE OPRD1 Antagonist GPCR Naltriben GABAA Opener IC GABA GABAA Blocker IC Picrotoxin HTR3A Opener IC Serotonin hydrochloride HTR3A Blocker IC Bemesetron MAO-A Inhibitor EN Clorgyline DAT Blocker TR GBR 12909 NET Blocker TR Desipramine SERT Blocker TR Clomipramine NMDAR Blocker IC (+)-MK801 NMDAR Opener IC L-Glutamic acid
(252) TABLE-US-00024 TABLE 14 Data summary table of target assays for compound E(VI) and control (C) ligands. Target Target Assay EC.sub.50 IC.sub.50 EC.sub.50 IC.sub.50 name type type C C E(VI) E(VI) ADRA1A GPCR AGN 5.00E−05 — >100 — ADRA1A GPCR ANT — 9.60E−04 — 1.09 ADRA2A GPCR AGN 4.00E−05 — >100 — ADRA2A GPCR ANT — 3.10E−03 — 19.78 AVPR1A GPCR AGN 4.20E−04 — >100 — AVPR1A GPCR ANT — 1.60E−03 — >100 CHRM1 GPCR AGN 9.70E−03 — >100 — CHRM1 GPCR ANT — 6.10E−03 — 15.1 CHRM2 GPCR AGN 2.70E−02 — >100 — CHRM2 GPCR ANT — 3.20E−03 — 51.24 CNR1 GPCR AGN 1.00E−05 — >100 — CNR1 GPCR ANT — 6.20E−04 — 96.99 DRD1 GPCR AGN 9.10E−02 — >100 — DRD1 GPCR ANT — 7.10E−04 — 7.11 DRD2S GPCR AGN 5.10E−04 — >100 — DRD2S GPCR ANT — 9.60E−04 — 13.28 HTR1A GPCR AGN 1.70E−03 — 11.36 — HTR1A GPCR ANT — 4.60E−02 — >100 HTR1B GPCR AGN 9.00E−05 — 2.36E−01 — HTR1B GPCR ANT — 5.80E−03 — >100 HTR2B GPCR AGN 6.30E−04 — >100 — HTR2B GPCR ANT — 4.00E−04 — 8.57E−02 OPRD1 GPCR AGN 5.00E−05 — 28.52 — OPRD1 GPCR ANT — 5.80E−04 — >100 GABAA Ion OP 6.2 — >100 — channel GABAA Ion BL — 4.6 — 32.17 channel HTR3A Ion OP 3.00E−01 — >100 — channel HTR3A Ion BL — 1.90E−03 — 1.87 channel MAO-A Enzyme IN — 2.90E−03 — >100 DAT trans- BL — 1.40E−03 — 1 porter NET trans- BL — 6.70E−03 — 9.25 porter SERT trans- BL — 1.80E−03 — 9.06 porter NMDAR Ion BL — 8.00E−02 — 15 channel NMDAR Ion OP 4.40E−01 — >100 — channel Potency (EC.sub.50 or IC.sub.50) is provided in units of μM. AGN, agonist; ANT, antagonist; OP, opener; BL, blocker; IN, inhibitor.
Example 2—Comparative Evaluation of a C.SUB.4.-Carbonothioate-Substituted Tryptamine Derivative and a C.SUB.4.-Carbonic Ester-Substituted Tryptamine Derivative
(253) Referring to
(254) It is noted that benzylcarbonate moieties (see: Portion C, compound 6) (as possessed by B(II)) are routinely and extensively used as a protecting group for alcohols and amines in organic synthetic reactions. However, by contrast, there exists a paucity of equivalent reports using benzylthiocarbonate moieties (see: Portion C, compound 7) (as possessed by E(VI)) for this purpose.
(255) Furthermore, once installed, a benzylcarbonate (see: Portion C, compound 6) (as possessed by B(II)) can be robustly deprotected using hydrogen gas under reductive conditions to reveal the unprotected alcohol, while a benzylthiocarbonate (see: Portion C, compound 7) (as possessed by E(VI)) may be cleaved under oxidative conditions (e.g., H.sub.2O.sub.2) or using nucleophilic fluoride (Greene's Protective Groups in Organic Synthesis, 5.sup.th Edition, P. G. M. Wuts, Wiley, 2014).
(256) Furthermore, referring to Portion B in
(257) Furthermore, with respect to chemical stability, the carbonothioate 7 and carbonic ester 6 functional groups are known to display substantially different rates of hydrolysis (Pharmaceutical Research, 1993, 10, 639-648).
(258) Furthermore, functional pharmacological attributes of B(II) and E(VI) were evaluated and will hereinafter be described.
(259) To further compare B(II) and E(VI), B(II) was subjected to the same pharmacological assays as E(VI). The first series of assays, namely (1) cell viability assays, (2) radioligand receptor binding assays, and (3) evaluation of 5-HT.sub.1A receptor modulation revealed very little difference between B(II) and E(VI). Briefly, the results were as follows. First, cell viability was assessed as described for Example 1, except B(II) was evaluated in place E(VI). It was determined that cytotoxicity was relatively similar for these two compounds, with a result of CD.sub.50=65.9 μM for B(II) and CD.sub.50=74.5 μM for E(VI) (
(260) However, unexpected differences between B(II) and E(VI) were observed upon conducting in vitro metabolic stability assays. Evaluations of metabolic stability and capacity of novel molecules to release psilocin under various in vitro conditions were performed as described in Example 1, except that compound B(II) was used in place of compound E(VI).
(261) Further potentially meaningful differences between B(II) and E(VI) were observed during in vivo evaluation of 5-HT.sub.2A receptor agonism in mice. Evaluation of in vivo HTR was conducted as described in Example 1, except that compound B(II) was used in place of compound E(VI). For ease of comparison, B(II) and E(VI) data are summarized side-by-side in
(262) In support of the in vitro metabolic conversion data, in vivo mouse pharmacokinetic (PK) evaluation of drug metabolism to psilocin revealed key differences between B(II) and E(VI). Pharmacokinetic (PK) evaluations were performed in the same manner as described in Example 1, except compound B(II) was used in place of compound E(VI). Congruent with in vitro data (
(263) The PK profile of psilocin was also different in mice dosed with B(II) compared with E(VI). Data in Tables 16 and 17 show higher psilocin levels in B(II)-treated mice, leading to overall greater psilocin exposure in these animals during the sampling period. That B(II) displays greater stability than E(VI) under a variety of in vitro and in vivo conditions, yet mice treated with B(II) appear to harbour greater psilocin levels, can be reconciled in a number of possible ways. First, it's possible that E(VI) instability in plasma (
(264) Yet further differences between B(II) and E(VI) were observed upon an in vitro survey of pharmacological interaction profiles. All assays were performed as described using “SAFETYscan E/IC150 ELECT” (https://www.eurofinsdiscovervservices.com/) except compound B(II) was used in place of E(VI). For ease of comparison, Table 18 summarizes data for both B(II) and E(VI), respectively. Several assays revealed differences between B(II) and E(VI) behavior. For example, B(II) failed to elicit a response (EC.sub.50>100 μM, or IC.sub.50>100 μM; Table 18) in CHRM2 (antagonist mode) and OPRD1 (agonist mode) assays, whereas E(VI) elicited a response in both cases (IC.sub.50=51.24 μM and EC.sub.50=28.52 μM, respectively). Furthermore, E(VI) failed to elicit a response (IC.sub.50>100 μM; Table 18) in AVPR1A (antagonist mode) and MAO-A (inhibitor mode) assays, whereas B(II) elicited a response in both cases (IC.sub.50=42.64 μM and IC.sub.50=21.86 μM, respectively).
(265) Thus, in summary, this Example 2 documents substantive differences in chemical as well as pharmacological attributes when compounds E(VI) and B(II) are compared. Notably, when E(VI) and B(II) are evaluated in various pharmacological assays, the two compounds exhibit unexpectedly substantially different pharmacological attributes. These differences in pharmacological attributes are deemed particularly surprising in light of the structural similarities between E(VI) and B (II).
(266) TABLE-US-00025 TABLE 15 Mean plasma concentrations of B(II) or E(VI) derivative (ng/mL) following oral administration of B(II) or E(VI) derivative. Fields marked (nd) indicate compound was either not detected or fell below acceptable limits of detection. Mean values ± SD were derived from n = 3 mice unless otherwise indicated. Time 3 mg/kg 10 mg/kg (h) B(II) E(VI) B(II) E(VI) 0.25 0.162 (n = 2) nd 0.994 ± 0.145 nd 0.5 0.162 (n = 1) nd 0.584 ± 0.186 nd 1 nd nd 0.272 ± 0.123 nd 2 nd nd 0.141 (n = 2) nd 4 nd nd 0.164 (n = 1) nd 6 nd nd nd nd 8 nd nd nd nd 24 nd nd nd nd
(267) TABLE-US-00026 TABLE 16 Mean plasma concentrations of psilocin (ng/mL) following oral administration of B(II) or E(VI) derivative. Time 1 mg/kg 3 mg/kg 10 mg/kg (h) B(II) E(VI) B(II) E(VI) B(II) E(VI) 0.25 19.7 ± 5.50 6.71 ± 1.63 55.6 ± 8.67 20.8 ± 6.46 306 ± 34.6 55.8 ± 21.9 0.5 11.9 ± 2.03 5.23 ± 0.640 32.3 ± 4.98 23.7 ± 6.32 125 ± 16.3 80.1 ± 28.6 1 4.63 ± 0.788 3.30 ± 0.606 9.29 ± 3.05 10.9 ± 2.32 49.6 ± 10.5 43.5 ± 1.75 2 2.20 ± 0.850 1.94 ± 0.508 7.67 ± 0.921 4.13 ± 1.10 20.7 ± 1.42 23.6 ± 8.45 4 2.05 ± 0.359 0.609 ± 0.143 6.76 ± 2.13 1.31 ± 0.351 31.4 ± 6.34 4.13 ± 1.48 6 0.739 ± 0.288 0.433 ± 0.301 2.41 ± 0.845 0.719 ± 0.465 11.5 ± 1.43 4.23 ± 3.52 8 0.453 ± 0.0460 0.188 0.722 ± 0.368 0.503 ± 0.346 6.38 ± 2.98 3.06 ± 1.99 (n = 2) 24 nd nd nd nd 0.104 nd (n = 1) Fields marked (nd) indicate psilocin was either not detected or fell below acceptable limits of detection. Mean ± SD were derived from n = 3 mice unless otherwise indicated.
(268) TABLE-US-00027 TABLE 17 Summary of mean plasma exposure of psilocin as a function of B(II) or E(VI) dose. Mean ± SD were derived from n = 3 mice unless otherwise indicated. 1 mg/kg 3 mg/kg 10 mg/kg B(II) E(VI) B(II) E(VI) B(II) E(VI) C.sub.max/Dose 19.7 ± 5.50 6.74 ± 1.59 18.5 ± 2.89 8.49 ± 1.46 30.6 ± 3.46 8.01 ± 2.86 (kg * ng/mL/mg) Apparent t.sub.1/2 (h) 1.69 ± 0.107 1.66 ± 0.577 1.23 ± 0.202 2.88 ± 1.29 1.84 ± 0.538 1.39 (n = 1) AUC.sub.0-tlast/Dose.sup.a 21.0 ± 1.55 10.7 ± 0.442 20.3 ± 2.78 10.5 ± 0.544 28.2 ± 4.12 12.3 ± 0.231 (h * kg * ng/mL/mg)
(269) TABLE-US-00028 TABLE 18 Data summary table of target assays for compounds B(II), E(VI) and control (C) ligands. Target Target Assay EC.sub.50 IC.sub.50 EC.sub.50 IC.sub.50 EC.sub.50 IC.sub.50 name type type C C B(II) B(ll) E(VI) E(VI) ADRA1A GPCR AGN 5.00E−05 — >100 — >100 — ADRA1A GPCR ANT — 9.60E−04 — 3.66 — 1.09 ADRA2A GPCR AGN 4.00E−05 — >100 — >100 — ADRA2A GPCR ANT — 3.10E−03 — 9.08 — 19.78 AVPR1A GPCR AGN 4.20E−04 — >100 — >100 — AVPR1A GPCR ANT — 1.60E−03 — 42.64 — >100 CHRM1 GPCR AGN 9.70E−03 — >100 — >100 — CHRM1 GPCR ANT — 6.10E−03 — 24.54 — 15.1 CHRM2 GPCR AGN 2.70E−02 — >100 — >100 — CHRM2 GPCR ANT — 3.20E−03 — >100 — 51.24 CNR1 GPCR AGN 1.00E−05 — >100 — >100 — CNR1 GPCR ANT — 6.20E−04 — 68.63 — 96.99 DRD1 GPCR AGN 9.10E−02 — >100 — >100 — DRD1 GPCR ANT — 7.10E−04 — 5.39 — 7.11 DRD2S GPCR AGN 5.10E−04 — >100 — >100 — DRD2S GPCR ANT — 9.60E−04 — 12.39 — 13.28 HTR1A GPCR AGN 1.70E−03 — 13.6 — 11.36 — HTR1A GPCR ANT — 4.60E−02 — >100 — >100 HTR1B GPCR AGN 9.00E−05 — 4.46E−01 — 2.36E−01 — HTR1B GPCR ANT — 5.80E−03 — >100 — >100 HTR2B GPCR AGN 6.30E−04 — >100 — >100 — HTR2B GPCR ANT — 4.00E−04 — 2.81E−01 — 8.57E−02 OPRD1 GPCR AGN 5.00E−05 — >100 — 28.52 — OPRD1 GPCR ANT — 5.80E−04 — >100 — >100 GABAA Ion OP 6.2 — >100 — >100 — channel GABAA Ion BL — 4.6 — 21 — 32.17 channel HTR3A Ion OP 3.00E−01 — >100 — >100 — channel HTR3A Ion BL — 1.90E−03 — 2.34 — 1.87 channel MAO-A Enzyme IN — 2.90E−03 — 21.86 — >100 DAT trans- BL — 1.40E−03 — 4.69 — 1 porter NET trans- BL — 6.70E−03 — 26.53 — 9.25 porter SERT trans- BL — 1.80E−03 — 10.36 — 9.06 porter NMDAR Ion BL — 8.00E−02 — 16.02 — 15 channel NMDAR Ion OP 4.40E−01 — >100 — >100 — channel Potency (EC.sub.50 or IC.sub.50) is provided in units of μM. AGN, agonist; ANT, antagonist; OP, opener; BL, blocker; IN, inhibitor. Note that ‘C’ refers to control compounds listed in Table 13.