Patent Description:
The circadian clock (circadian rhythm) has evolved as an adaptation to a <NUM>-hour solar day, and although its mechanism varies from organism to organism, it is one of the universal characteristics of life. Clock makes it possible to anticipate and prepare for regularly changing external conditions. However, it can also function in aperiodic conditions with its own genetically determined circadian period. Clock is entrainable (i.e. has ability to be synchronized) by the external cues (e.g. light, temperature, social interaction) and controls metabolic, physiological and behavioral rhythms. In mammals, circadian rhythms are controlled by a central pacemaker located in the suprachiasmatic nucleus of the hypothalamus (SCN), which is directly synchronized by light and regulates the local clock in other brain and peripheral tissues such as in the cerebral cortex, hippocampus, retina, liver, kidney, intestine, or pancreas. The main oscillator in the SCN, as well as the peripheral oscillators, are composed of interconnected transcriptional and (post) translational feedback loops (TTFLs) formed by families of clock genes such as Per, Bmal, Clock, Rev-Erb, Ror and Cry. Clock genes then rhythmically regulate a large group of predominantly tissue-specific clock-controlled genes with various functions, including regulation of metabolism, behavior, or cell division.

Interestingly, clock genes play a role in a number of other processes. For example, human ARNTL / BMAL1 upregulates myogenesis and downregulates adipogenesis through transcriptional control of Wnt signaling pathway genes. It also contributes to the normal function of pancreatic beta cells and regulates glucose-stimulated insulin secretion. It further regulates the mTORC1 signaling pathway by regulating MTOR and DEPTOR expression. Chemokine expression in Ly6C monocytes is also regulated by ARNTL / BMAL1. It further regulates the expression of genes involved in hair growth. It also plays an important role in adult hippocampal neurogenesis by timing the entry of neuronal stem cells into the cell cycle. Human PER2 plays a role in lipid metabolism (by suppressing the proadipogenic activity of PPARG) and in glucose metabolism (regulation of circulating insulin levels). PER2 contributes to the maintenance of cardiovascular function by regulating the production of NO and vasodilating prostaglandins in the aorta. It also regulates the absorption of glutamate in synaptic vesicles, the absorption of fatty acids in the liver and is involved in the regulation of inflammatory processes. Clock-controlled genes and proteins can make up more than <NUM>% of the total transcriptome and proteome, depending on the tissue. Many of these genes are associated with serious human diseases, including cancer (WEE1, p21, Ballesta et al. <NUM> [doi: <NUM> /pr. <NUM><NUM>]), myocardial infarction (PAI-<NUM>, SCA1, Crnko et al. <NUM> [doi: <NUM> / s41569-<NUM>-<NUM>-<NUM>], Sheer and Shea, <NUM> [doi: <NUM> / blood-<NUM>-<NUM>-<NUM>]), sleep disorders (CK1d, PER2, CLOCK, PER3, Jones et al. <NUM> [doi: <NUM> /j. <NUM>]) or depressive disorder (NFSC, SLC25A17, MEIS1, Ferguson et al. <NUM> [https://doi. org/<NUM>/j. Their rhythmic regulation allows cells, tissues and organs to perform physiological processes in a coordinated way, to anticipate and prepare for changes in the environment. Synchronization of individual oscillators in peripheral tissues by the SCN via hormonal and neuronal signals allows precise coordination and integration of various physiological functions.

Dysfunctions of the circadian rhythm in terms of changes in period, phase or amplitude at the level of cells, tissues, organs or the whole body as well as phase mismatch between oscillators in individual tissues/organs or between biological and external time lead to disruption of homeostasis, resulting in various pathologies. Examples of conditions associated with circadian rhythm dysfunction or impairment are FASPS, ASPD.

In the absence of external stimuli (for example in constant darkness), the endogenous period of circadian rhythm in humans is on average slightly longer than <NUM> hours. In completely blind subjects unable to synchronize with light, such a period often persists chronically. As a result, their sleep-wake cycle is free-running with respect to external time, which is often associated with negative metabolic, cognitive and emotional consequences.

The discrepancy of the circadian clock with the external time is also a typical feature of modern life. Air travel allows fast movement across time zones, which results in jet lag. Artificial light allows activity independent of natural light, which effectively synchronizes the central oscillator in the SCN. Personal preference for a specific sleep phase (chronotype) and social factors influence the timing of the individual activity and these factors are often in conflict, resulting in a so-called social jet lag (i.e. a chronic difference between the sleep phase on free days and on working days), which has a negative effect on health (Roenneberg and Merrow, <NUM> [doi: <NUM> / j. A particularly important factor causing circadian desynchronization is shift work due to its prevalence (more than <NUM>% of the EU workforce is night workers). The result is frequent sleep problems, fatigue and reduced manual and mental performance. Jet lag, social jet lag and shift work significantly affect physiological functions and increase the incidence of lifestyle diseases (Roennberg <NUM> [doi: <NUM> / j. <NUM>]; Roenneberg and Merrow <NUM> [doi: <NUM> /j. Frequent shift workers also have an increased risk of depression, metabolic syndrome (Costa et al. <NUM> [doi: <NUM> / <NUM>]), breast, prostate and rectal cancer (Sulli et al. <NUM> [doi:. / <NUM> / j. For this reason, in <NUM> the WHO International Agency for Research on Cancer (IARC) included circadian disruption among probable human carcinogens (Group 2A).

Circadian dysfunction can be assessed by measuring physiological (such as body temperature, heart activity, actigraphy) or biochemical parameters (melatonin, metabolites, clock gene RNA and protein levels in body fluids). In the case of an inherited disease, it can be diagnosed using DNA diagnostics based on PCR or sequencing.

Circadian rhythm modulators can also be used prophylactically to accelerate the proper resetting of the circadian system after traveling through time zones or during a planned change of activity (e.g., in preparation for shift work or other social activities).

Current approaches to the treatment of circadian rhythm disorders are dominated by various variants of bright light therapy and the use of melatonin or synthetic melatonin receptor agonists. However, these methods also have significant disadvantages. Bright light therapy is considered very inconvenient for many users because it requires exposure to very high levels of light in precise time windows every day (Zee et al. , <NUM> [doi: <NUM> / <NUM>. It cannot be used in blind patients. Melatonin is only effective in subset of patients with sleep disorders. It is unlikely to have a significant effect, for example, on patients suffering from FASPS, ASPD or jet lag after traveling westwards. It may cause unwanted drowsiness. In addition, there is great individual variability in response to melatonin. Another disadvantage of light or melatonin is that their effect on the rhythm phase is directly dependent on the instantaneous phase of the central clock in the SCN. For example, light applied during a subjective day has no effect on the SCN phase, as it is in that moment in non-responsive zone of the phase-response curve, so it is necessary to time the therapy to the early morning or late evening hours. Therefore, a direct effect on the molecular circadian mechanism could be a new effective way to adjust circadian rhythms. For example, the CK1δ inhibitor (PF670462, Pfizer) is very effective in prolonging the in vitro and in vivo period in mice. Its uses include arrhythmias caused by phase shift (jet lag, neurodegenerative diseases, disorders associated with aging or shift work) and / or shortening of the period (FASPS, ASPD). An important finding is that PF670462 can also be used to restore physiological rhythms fundamentally disrupted due to genetic disruption of VIP receptors in the SCN (which shortens the period and causes rhythm loss similar to some neurodegenerative diseases) or due to constant light (which also first affects the period and then causes a decrease in amplitude leading to complete loss of rhythms) in mice (Meng et al. , <NUM> [doi: /<NUM>/pnas. Another example of a compound that acts directly on the molecular mechanism is nobiletine (He, Nohara et al. <NUM> [doi: <NUM> / j. <NUM>]), which increases the amplitude of rhythms at the molecular level by acting on nuclear ROR receptors and has recently been used to prevent metabolic syndrome in a diabetic mouse model and restore physiological rhythms in the liver of mice fed a high-fat diet (He, Nohara et al. <NUM> [doi: <NUM> / j. <NUM>]), or to reduce cognitive defects caused by constant light and midazolam in a mouse model of delirium (Gile, Scott et al. <NUM> [doi: <NUM> / CCM. Similar therapy targeting the molecular mechanism directly will be beneficial in a number of disorders associated with various types of circadian dysfunctions requiring proper synchronization, period length adjustment, a single new phase adjustment, or increased overall rhythm integrity (see above). In addition, unlike light or melatonin therapies, therapy using agents that directly target the molecular mechanism does not require SCN, is equally effective day and night, and its timing in general is unlikely to significantly affect its effect, which can be easily modulated by dose adjustment.

<CIT> discloses kinetin i.e. N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine, or a pharmaceutically acceptable salt thereof (page <NUM>, lines <NUM>-<NUM>) per se and in the treatment of Parkinson's disease.

<CIT> and <CIT> are both documents from the broader technical field of anti-aging medicine preparations, which state that kinetin (N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine) has beside the effect of anti-ageing and other advantages also an effect of regulating sleep.

<CIT> discloses the use of melatonin or ramelteon as chronotherapeutic in combination with other such agents for use in prevention and/or treatment of circadian rhythm disorders, circadian rhythm diseases and/or circadian rhythm dysfunctions. <CIT> discloses the use of light therapy in combination with chronotherapeutic agents for use in prevention and/or treatment of circadian rhythm disorders, circadian rhythm diseases and/or circadian rhythm dysfunctions. <CIT> discloses N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine (kinetin), or a pharmaceutically acceptable salt or solvate thereof, alone or in combination with a chemotherapeutic (i.e. antineoplastic agent).

The invention relates to N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine (kinetin, N6-furfuryladenine) for use in treatment based on modulation of circadian rhythms in mammals, especially humans.

Circadian rhythm is an endogenous circadian rhythm of an organism or its cells, tissues and organs. Modulation of circadian rhythms includes modulation of the amplitude, period and/or phase of circadian cycle. All of these parameters are important for maintaining homeostasis, including the proper functioning of metabolism and sleep quality.

The invention is based on the finding that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine.

A major advantage of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine over a number of bioactive compounds, including other N6-substituted purines and their biosters, is its low toxicity. <NPL>]) have shown that human fibroblasts can be grown in the presence of high concentrations of this compound without any negative consequences. The compound, under the tradename Kinerase, is used in clinically tested cosmetics, and its formulation for oral administration is being evaluated as a treatment for hereditary sensory and autonomic neuropathy (clinical trial NCT02274051).

Modulation of the activity and concentration of the central molecular components of the mammalian cellular circadian oscillator influences many downstream molecular and physiological processes. These central components include clock genes, in particular the genes of the Per, Bmal, Clock, Rev-Erb, Ror and Cry families, and their protein products. Clock genes play a role in the pathogenesis of a number of diseases, including sleep disorders, cancer, myocardial infarction, and depressive disorders. Modulation of ARNTL / BMAL1 clock gene activity leads to modulation of myogenesis, adipogenesis, pancreatic beta-cell function, insulin secretion, mTOR pathway activity, chemokine expression, and hair growth. Modulation and activity of the PER2 clock gene can be used to regulate downstream processes, including the production of nitric oxide and vasodilating prostaglandins in the vessel wall, the regulation of fatty acid absorption in the liver, and the regulation of inflammatory processes.

Manipulation of the amplitude, period, and in the case of single-dose or short-term administration (<<NUM> days) also the phase, achievable by administration of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine, is able to remedy or correct diseases of circadian rhythms.

Circadian rhythm diseases where circadian rhythm dysfunction is present include advanced sleep phase syndrome (ASPD), including its inherited form (FASPD or FASPS), jet lag, social jet lag, circadian dysfunction associated with shift work. N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine can be administered prophylactically or therapeutically.

Modulation of abnormal circadian rhythm patterns by administration of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine can improve sleep quality. This improvement may be perceived only subjectively and may not reach a clinical stage. Sleep quality is satisfaction with the sleep experience integrating aspects of sleep initiation, sleep retention, amount of sleep, and the refreshing effect of sleep. Its reduction is the subjective feeling that some of these parameters are insufficient, or objective observation of changes in these parameters. Sleep quality can be assessed using questionnaires such as the University of Pittsburgh Sleep Quality Index (PSQI) or by measurement (actigraphy, polysomnography).

Increasing the circadian period by administration of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine has a therapeutic effect especially in diseases where the circadian cycle period is shortened and/or phase is advanced, such as in FASPS and ASPD. Long-term administration (more than <NUM> days) is preferred here.

Modulation of a period and/or phase (phase shift after a single or short-term extension of a period) by administration of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine can prevent or treat diseases and conditions caused by a person's or animal's circadian rhythm mismatch with the external environment. For prophylactic and/or therapeutic effects against jet-lag, social jet-lag, and/or shift-work disorder, it is preferable to administer N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine briefly (once or repeatedly for <NUM> to <NUM> days). The advantage of single and short-term administration is less burden on the body, including metabolic systems, with the drug.

Important symptoms of circadian misalignment that can be corrected by administration of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine include fatigue, worsened attention, increased reaction time, headache, memory impairment, mood disturbance, irritability, reduced manual dexterity, reduced motivation, decreased energy, or decreased initiative, nausea and sleep disturbance. A particularly important application is prevention and therapy of such symptoms in jet-lag, social-jet lag and shift-work disorder. The symptoms of jet lag that can be corrected through normalization of circadian rhythm misalignment by administration of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine include decreased performance on mental tasks and concentration, confusion, dizziness, anxiety, irritability, increased fatigue, headache, nausea, trouble to fall asleep or remaining asleep, problems with digestion, including indigestion, alterations in the frequency of defecation and stool consistency, and reduced interest in food and its enjoynment.

The disclosure also provides N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine for use in modulating the response of mammals, including humans, and their cells, tissues and organs (in vitro or in vivo) to stimuli affecting circadian rhythms. N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine and the appropriate stimulus may be administered simultaneously, for example in the form of a combined preparation (if the stimulus is a chemical), or sequentially.

In one embodiment, the stimulus is another chronotherapeutic. A chronotherapeutic is a compound that modulates the circadian rhythm or changes its sensitivity to entrainment.

The disclosure includes a combination of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine and a chronotherapeutic selected from the group consisting of CSNK1D inhibitors, CSNK1A inhibitors, CSNK1E inhibitors, GSKbeta inhibitors, ALK5 inhibitors, AMPK activators, activators SIRT1, CRY ligands, PPARG agonists, BMAL1 expression regulators, vasopressin receptor ligands, REV-ERB agonists, RORα /γ agonists. Preferably, the additional chronotherapeutic is selected from the group consisting of melatonin receptor agonists including melatonin, ramelteon, tasimelteon and agomelatine. These combinations usually have an additive or synergistic effect on the period and / or phase, but the addition of kinetin may also change the amplitude. In some cases, such as in combination with the chronotherapeutic harmine, the addition of kinetin shortens the period compared to the condition when harmine alone is used. Thus, kinetin can be used to precisely modulate the effect of other chronotherapeutics.

This disclosure may use preparations containing a combination of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine and at least one other chronotherapeutic in concentrations effective for prophylactic or therapeutic modulation of circadian rhythms and/or sleep of mammals including humans.

N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine and the chronotherapeutic may be used as described herein and/or present in the compositions in the form of pharmaceutically acceptable salts or solvates. Pharmaceutically acceptable salts of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine are formed by protonation of one of the nitrogens with an inorganic or organic acid. Examples of salts with inorganic acids include hydrochlorides, hydrobromides, hydroiodides, sulfates, nitrates, phosphates, hydrogen phosphates, dihydrogen phosphates, carbonates, bicarbonates, perchlorates. Examples of salts with organic acids include salts with straight or branched chain polyhydric or polybasic acids having <NUM> to <NUM> carbons, such as lactate, maleate, oxalate, fumarate, tartrate, malate, maleate, citrate, succinate, glycolate, nicotinate, benzoate, salicylate, ascorbate, pamoate; sulfonate, methanesulfonate, ethane sulfonate, <NUM>-hydroxyethanesulfonate, benzenesulfonate, p-toluenesulfonate, <NUM>-naphthalenesulfonate, <NUM>-phenylsulfonate and camphorsulfonate, aspartate or glutamate.

Combined pharmaceutical preparations for co-administration contain an effective amount of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine and other active ingredients (chronotherapeutics), or pharmaceutically acceptable salts or other forms thereof, alone or in combination. Mixtures with one or more excipients such as carriers, fillers, solvents, tablet degradants, lubricants, integrity enhancers, pigments, stabilizers, preservatives, antioxidants, solubility enhancers. The preparation may contain excipients that increase penetration through biological barriers, for example through the skin. However, in addition to co-administration, the active ingredients may be administered alone (sequentially) at intervals. In that case, each of these active ingredients is contained in a separate dosage form, usually together with one or more excipients.

In a preferred embodiment, these preparations are in the dosage form for oral administration. In another important embodiment, the dosage forms are for transdermal, inhalation or nasal administration. In other embodiments, the dosage forms are for other modes of parenteral administration, such as intravenous, intramuscular, subcutaneous, or topical administration.

Dosage forms for oral administration include coated and uncoated tablets, soft and hard gelatin capsules, matrix tablets, solutions, emulsions, suspensions, syrups, powders and granules for reconstitution, chewable and effervescent tablets. Dosage forms for parenteral administration include solutions, emulsions, suspensions and dispersions, powders and granules for reconstitution. Other contemplated dosage forms include suppositories, transdermal penetration dosage forms, implants, and insufflation and inhalation dosage forms. Topical dosage forms include creams, gels, ointments and patches.

Human osteosarcoma U2OS cells were grown in standard DMEM with <NUM>% fetal calf serum. U2OS cells were transduced with lentiviral particles containing the reporter pLV6-Bmal1-Luc (S. Brown, Addgene plasmid # <NUM>) and selected under Blasticidin. The cell line was clonally expanded and a single monoclonal cell line was used for further experiments. Cells were cultured in a <NUM>-well plate in growth medium to <NUM>+% confluence. Test compound or vehicle (DMSO) was applied to recording medium with <NUM> U / ml penicillin, <NUM> ug / ml streptomycin, 1x GlutaMAX (ThermoFisher, Waltham, MA, USA), <NUM>% fetal calf serum (Sigma) and <NUM> Luciferin-EF (Promega Madison, WI, USA). Luminescence was recorded every hour for an additional <NUM> hours in Luminoskan Ascent (ThermoFisher). Circadian rhythm analysis was performed using cosinor analysis. The results are shown in <FIG>.

This experiment demonstrates that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine extends the circadian rhythm period of human cells and can be used to manipulate the circadian rhythm phase, for example, to synchronize the endogenous circadian clock with solar time. The overall effect on circadian oscillations indirectly but unequivocally demonstrates that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine can also be used to modulate the concentration and activity of other oscillator components, including the critical components BMAL1, PER2, CRY and CLOCK over time, as these are an essential part of the mechanism for generating rhythmic expression of the used luminescent reporter. The concentration and level of other proteins, whose rhythmic expression is controlled by an oscillator in the brain and peripheral tissues (so-called clock-controlled genes), is also necessarily affected. The effect of N- (furan-<NUM>-ylmethyl) -<NUM>-purin-<NUM>-amine on the activity of oscillator components and subordinate genes also means influencing the physiological processes of the cell controlled by these genes and proteins.

Mouse embryonic fibroblasts NIH3T3 cells were grown in standard DMEM with <NUM>% fetal calf serum. NIH3T3 cells were transfected with <NUM>µg of Per2-Luc reporter (Meng, <NUM>) using GeneJuice (Novagen) and selected under hygromycin. The cell line was clonally expanded and a single monoclonal cell line was used for further experiments. Cells were cultured in a <NUM>-well plate in growth medium to <NUM>+% confluence. Test compound or vehicle (DMSO) was applied to recording medium with <NUM> U / ml penicillin, <NUM> ug / ml streptomycin, 1x GlutaMAX (ThermoFisher, Waltham, MA, USA), <NUM>% fetal calf serum (Sigma) and <NUM> Luciferin-EF (Promega Madison, WI, USA). Luminescence was recorded every hour for an additional <NUM> hours in a Luminoskan Ascent (ThermoFisher). Circadian rhythm analysis was performed using cosinor analysis. The results are shown in <FIG>.

The experiment demonstrates that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine prolongs the circadian rhythm period of mouse cells and can be used to manipulate the circadian rhythm phase, for example, to synchronize the internal circadian clock with solar time. The overall effect on circadian oscillations indirectly, but unequivocally, demonstrates that N- (furan-<NUM>-ylmethyl) -<NUM>-purin-<NUM>-amine can also be used to modulate the concentration and activity of other oscillator components, including the critical components Bmal1, Per2, Cry and Clock, as these are an essential part of the mechanism for generating the rhythmic expression of the luminescent reporter used. The concentration and level of other proteins, whose rhythmic expression is controlled by an oscillator in the brain and peripheral tissues (so-called clock-controlled genes), is also necessarily affected. The effect of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine on the activity of oscillator components and subordinate genes also means influencing the physiological processes of the cell by these genes and proteins controlled.

Male and female mPer2Luc mice (strain B6.129S6-Per2tm1Jt / J, JAX, USA) (Yoo et al. , <NUM>) were maintained in a light / dark cycle with <NUM> hours of light and <NUM> hours of darkness (LD12: <NUM>), killed between <NUM>:<NUM> and <NUM>:<NUM>, i.e. <NUM>-<NUM> hours after turning on the lights, by rapid cervical dislocation under isoflurane anesthesia, their brains were removed and <NUM> thick SCN slices in ice-cold HBSS medium were prepared using a vibratome (Leica, Wetzlar, Germany). Two explants containing SCN from each brain were prepared. Individual SCN explants were then placed on Millicell Culture Inserts (Merck, Darmstadt, Germany) inside <NUM> Petri dishes with test compound or DMSO vehicle in <NUM> air-buffered recording medium supplemented with <NUM> U / ml penicillin, <NUM> ug / ml streptomycin (Sigma-Aldrich, St. Luis, MO, USA), 1x GlutaMAX (ThermoFisher, Waltham, MA, USA), <NUM>% fetal calf serum (Sigma) and <NUM> Luciferin-EF (Promega Madison, WI, USA). The dishes were sealed with vacuum Vaseline and glass coverslips and placed inside a LumiCycle (Actimetrics) for bioluminescence recording. Rhythm analysis was performed in Lumicycle Analysis software (Actimetrics).

The example demonstrates that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine prolongs the circadian rhythm period and modulates the period in the complex tissue of the central pacemaker and can be used to manipulate the circadian rhythm phase, for example to synchronize the internal circadian clock with solar time. The overall effect on the circadian oscillator indirectly, but unequivocally, demonstrates that the compound can also be used to modulate the concentration and activity of other components of the oscillator, including the critical components Bmal, Per2, Cry and Clock over time. The concentration and level of other proteins, whose rhythmic expression is controlled by an oscillator in the brain and peripheral tissues (so-called clock-controlled genes), is also necessarily affected. The effect of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine on the activity of the oscillator components and subordinate genes also means influencing the physiological processes of the cell controlled by these genes and proteins.

Human osteosarcoma U2OS cells were grown in standard DMEM with <NUM>% fetal calf serum. U2OS cells were transduced with lentiviral particles containing the reporter pLV6-Bmal1-Luc (S. Brown, Addgene plasmid # <NUM>) and selected under Blasticidin. The cell line was clonally expanded and a single monoclonal cell line was used for further experiments. Cells were cultured in a <NUM>-well plate in growth medium to <NUM>+% confluence. Test compound or vehicle (DMSO) was applied to recording medium with <NUM> U / ml penicillin, <NUM> ug / ml streptomycin, 1x GlutaMAX (ThermoFisher, Waltham, MA, USA), <NUM>% fetal calf serum (Sigma) and <NUM> Luciferin-EF (Promega Madison, WI, USA). Luminescence was recorded every hour for additional <NUM> hours in Luminoskan Ascent (ThermoFisher). The results are shown in <FIG>.

The example demonstrates that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine affects Bmal1 gene expression in human cells. A change in the level of Bmal1 mRNA affects its protein level. Because this protein controls the expression of other circadian oscillator genes and directly activates the expression of a number of other genes containing the E-box in their regulatory DNA region and exhibiting circadian oscillations, N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine also affects their expression.

Mouse embryonic fibroblasts NIH3T3 cells were grown in standard DMEM with <NUM>% fetal calf serum. NIH3T3 cells were transfected with <NUM>µg of Per2-Luc reporter (Meng, <NUM>) using GeneJuice (Novagen) and selected under hygromycin. The cell line was clonally expanded and a single monoclonal cell line was used for further experiments. Cells were cultured in a <NUM>-well plate in growth medium to <NUM>+% confluence. Test compound or vehicle (DMSO) was applied to recording medium with <NUM> U / ml penicillin, <NUM> ug / ml streptomycin, 1x GlutaMAX (ThermoFisher, Waltham, MA, USA), <NUM>% fetal calf serum (Sigma) and <NUM> Luciferin-EF (Promega Madison, WI, USA). Luminescence was recorded every hour for additional <NUM> hours in Luminoskan Ascent (ThermoFisher). The results are shown in <FIG>.

The example demonstrates that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine regulates Per2 gene expression in mouse cells. The change in the mRNA level also affects the level of the PER2 protein. Because this protein controls the expression of other circadian oscillator genes and inhibits the expression of a number of other genes exhibiting circadian oscillations, N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine also affects their expression.

Human osteosarcoma U2OS cells were grown in standard DMEM with <NUM>% fetal calf serum. U2OS cells were transduced with lentiviral particles containing the reporter pLV6-Bmal1-Luc (S. Brown, Addgene plasmid # <NUM>) and selected under Blasticidin. The cell line was clonally expanded and a single monoclonal cell line was used for further experiments. Cells were cultured in a <NUM>-well plate in growth medium to <NUM>+% confluence. Test compounds or vehicle (DMSO) were applied to recording medium with <NUM> U / ml penicillin, <NUM> ug / ml streptomycin, 1x GlutaMAX (ThermoFisher, Waltham, MA, USA), <NUM>% fetal calf serum (Sigma) and <NUM> Luciferin-EF (Promega Madison, WI, USA). Luminescence was recorded every hour for additional <NUM> hours in Luminoskan Ascent (ThermoFisher). Circadian rhythm analysis was performed by cosinor analysis.

The example demonstrates that N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine in combination with compounds that extend the circadian period by different mechanisms of action has an additive or even synergistic effect on the length of the circadian period in human cells and can be used to enhance the effect of these compounds. Conversely, depending on the mechanism of action, some compounds (in this case, harmine) shorten the period after the addition of N-furan-<NUM>-ylmethyl) -<NUM>-purin-<NUM>-amine, so it can be used to negatively modulate the effect of this type of compound.

Resazurin is a blue weakly fluorescent compound that is irreversibly reduced into red highly fluorescent resofurin by mitochondria. It is used for viability testing of eukaryotic cells. The effect of the compounds in several concentrations (maximum concentraton of <NUM> microM and <NUM> three-fold dilutions) on viability of skin fibroblasts BJ and retinal epitelium cells ARPE-<NUM> was evaluated after <NUM> hour treatment. The cells were maintained in standard cultivation medium DMEM with <NUM>% fetal bovine serum. <NUM> cells were seeded into <NUM>-well plates <NUM> hours prior to the addition of test compound. DMSO vehicle was used as a negative control. After <NUM> hours, <NUM>-times concentrated solution of resazurin in DMSO was added to the cells zo the final concentration of <NUM>/ml. Fluorescence (ex = <NUM>, em= <NUM>) was measured after <NUM> hour (ARPE-<NUM>) or <NUM> hours (BJ) of incubation. IC50 values were calculated from dose response curves using drc library for R programming environment. Following results were obtained: Resazurin test after <NUM> day exposure - ARPE-<NUM> IC<NUM> ><NUM> and BJ IC<NUM> > <NUM> microM. N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine has a favorable toxicity profile for human non-cancer cells. This is an important advantage in comparison with many other N6-substituted purines and their biosters many of which are toxic sometimes because of the inhibition of cyclin dependent kinases (Voller et al. <NUM> [doi: <NUM>/j. <NUM>], Jorda et al. <NUM> [doi: <NUM>/<NUM>]).

Human fibroblasts BJ were maintained in standard cultivation medium DMEM with <NUM>% fetal bovine serum. The experiment was performed in <NUM>-well plates. <NUM>,<NUM> cells in DMEM medium with <NUM>% fetal bovine serum were seeded into the wells. The test compound was added to a final concentration in the range of <NUM>-<NUM> after <NUM> hours. DMSO vehicle was used as a negative control. In order to obtained better idea of test variability, <NUM> control wells were used (columns A and D). The cultivation medium containing either test compound or DMSO was replaced twice a week. The cells were trypsinized on the 12th day and counted on Coulter Z2 apparatus. The test compound in the evaluated concentration range and exposure time did not have a negative effect on cell growth. The results are shown in <FIG>.

N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine has a favorable toxicity profile in human noncancer cells. This is an important advantage in comparison with many other N6-substituted purines and their biosters many of which are toxic sometimes because of the inhibition of cyclin dependent kinases (Voller et al. <NUM> [doi: <NUM>/j. <NUM>], Jorda et al. <NUM> [doi: <NUM>/<NUM>]).

Quantification of N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine in the samples was performed using RapidFire RF300 system (Agilent Technologies) interfaced with QTRAP <NUM> mass spectrometer fitted with an electrospray ionization source (AB Sciex, Concord, Canada) and running in multiple - reaction monitoring mode.

This system is further referred to as RF-MS. Preparation of the lyophilized samples for the analysis is described in the sections dedicated to the individual methods. Lyophilized samples were dissolved in the mobile phase (<NUM>% water, <NUM>% acetonitrile, <NUM>% formic acid) with respective internal standards. The dissolved samples were aspired directly from <NUM>-well plates into a <NUM> µL sample loop and passed through a C4 cartridge (Agilent Technologies) with solvent A (<NUM>% water, <NUM>% formic acid, <NUM>% acetonitrile) at a flow rate of <NUM>/minute for <NUM> seconds. After the desalting step, the analyte retained on the cartridge was eluted with solvent B (<NUM>% acetonitrile, <NUM>% <NUM>% formic acid) to the mass spectrometer at a flow rate of <NUM>/minute for <NUM> seconds. Mass spectrometry was carried out using electrospray ionization in the positive ion mode. Daughter ion peaks were identified using a multiple - reaction monitoring protocol.

Test compound (a final concentration of <NUM>) was incubated with human plasma (Transfusion Department, University Hospital Olomouc, Olomouc, Czech Republic) for <NUM>, <NUM>, <NUM>, <NUM> and <NUM> at <NUM>. The reactions were stopped by addition of acetonitrile-methanol mixture (<NUM>:<NUM>). Samples were stored at -<NUM> overnight and centrifuged (<NUM>× g, <NUM>, <NUM>). Supernatants were lyophilized.

The reaction mixtures of test compounds (<NUM> µM), human liver microsomes (ThermoFisher Scientific, <NUM>/mL), NADPH generating system (NADP+ - <NUM>, isocitrate dehydrogenase - <NUM> U/mL, isocitric acid - <NUM>, and MgSO<NUM>- <NUM>) in <NUM> mol/L K<NUM>PO<NUM> buffer. The reactions were stopped by the addition of acetonitrile-methanol mixture (<NUM>:<NUM>) after <NUM>, <NUM>, <NUM>, and <NUM> at <NUM>. The samples were centrifuged (<NUM> × g, <NUM>, <NUM>) and the supernatants were lyophilized.

Calculations: The intrinsic clearance was calculated as CLint = V*(<NUM>/t<NUM>/<NUM>), where V is the volume of the reaction in µL related to the weight of the microsomal protein in mg per reaction. Elimination half-life was calculated using the equation t<NUM>/<NUM> = <NUM>/k, where k is the slope of linear regression of natural logarithm of percent substrate remaining plotted versus incubation time.

The parallel artificial membrane permeability assay (PAMPA) was performed using the Millipore MultiScreen filter MultiScreen-IP Durapore <NUM> µm plates and receiver plates (Merck Millipore) according to the manufacturer's protocol PC040EN00. The test compounds were dissolved in PBS (pH <NUM>) to the final concentration of <NUM> µM and added to the donor wells. The filter membrane was coated with <NUM>% lecithin (Sigma Aldrich) dissolved in dodecane and the acceptor wells were filled with PBS (pH <NUM>). The acceptor filter plate was carefully placed on the donor plate. Following <NUM>-hour incubation at the room temperature aliquots of acceptor and donor solutions were removed and lyophilized.

Calculations: The relative permeability logPe was calculated as logPe = log{C×-ln(<NUM>-drugA/drugE)}, where C = (VA × VD)/{(VD+VA) × A × T}. VD and VA are the volumes of the donor and acceptor solutions, respectively, A is the active surface area in cm<NUM> and T is time of the incubation in seconds. DrugA and drugE is the mass of the compound in the acceptor solution and in the solution in theoretical equilibrium (as if the donor and acceptor were combined), respectively.

The assay is based on the rapid equilibrium dialysis (RED). The RED plate inserts (Thermo Scientific™, Rockford, USA) consist of two chambers separated by a semipermeable membrane. For each compound, <NUM> µM in <NUM>% human plasma was transferred into the one chamber and the other was filled with PBS buffer (pH <NUM>). The equal volumes of the solutions from either compartment were transferred into microtubes after the <NUM>-hour incubation with shaking (<NUM> rpm). Either <NUM>% plasma or PBS buffer (pH <NUM>) was added so that all the samples had the same matrix. The reactions were stopped by the addition of acetonitrile-methanol mixture (<NUM>:<NUM>). The samples were centrifuged (<NUM>× g, <NUM>, <NUM>) and the supernatants were lyophilized.

Caco-<NUM> (American Tissue Type Collection) a MDR1-MCDK (Netherlands Cancer Institute) were cultured in DMEM medium with <NUM>% fetal bovine serum. In order to generate cell monolayers for transport studies, the cells were trypsinized and seeded on tissue culture polyester membrane filters (pore size <NUM> µm for Caco-<NUM> and <NUM> µm for MDR1-MCDK) in <NUM>-well Transwell® plates (Corning, NY, USA). The culture medium was added to both the donor and the acceptor compartments and the cells were allowed to differentiate and form the monolayers. The culture medium was changed every other day.

Caco-<NUM> and MDR1-MCDK differentiated monolayers were used only if they were intact, which was confirmed by Lucifer Yellow Rejection Assay. Prior to the experiment, the cells were washed twice with Hank's balanced buffer solution (HBBS) (Gibco, Waltham, USA) and pre-equilibrated with HBSS buffer at pH <NUM> for <NUM>. After removing the medium, the cells were treated with <NUM> µM test compounds in HBSS (pH <NUM>) for <NUM> and <NUM>, for MDCK and Caco-<NUM>, respectively. Thereafter, the samples were removed from both donor and acceptor compartments and lyophilized. All experiments were done in duplicate.

Calculations: The apparent permeability coefficient was calculated as Papp = (dQ/dt)/(C<NUM> × A), where dQ/dt is the rate of permeation of the drug across the cell monolayer, Co is the donor compartment concentration at time t = <NUM> and A is the area of the cell monolayer. The efflux ratio R was defined as ratio PBA/PAB where PBA and /PAB represent the apparent permeability of test compound from the basal to apical and apical to basal side of cell monolayer, respectively. The compounds with the efflux ratio of <NUM> or higher were considered as potential P-gp substrates.

N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine is highly stable in human plasm and after an exposure to human microsomal fraction. The data from the Caco-<NUM> model of gut wall predict that it will be orally available. Exceptionally high permeability in the MDR1-MDCK model of blood-brain barrier predict excellent CNS permeability probably through a transporter. CNS penetration is key for attaining the effects on the central pacemaker.

<NUM> capsules, each containing <NUM> ofN-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine and <NUM> melatonin as active ingrediences, are prepared as follows:.

Claim 1:
N-(furan-<NUM>-ylmethyl)-<NUM>-purin-<NUM>-amine, or a pharmaceutically acceptable salt or solvate thereof, for use in prevention and/or treatment of circadian rhythm disease selected from advanced sleep phase syndrome/disorder - ASPD, age related and hereditary forms of ASPD - FASPD/FASPS, jet-lag, social jet-lag, circadian dysfunction due to shift-work.