The present invention relates to novel 4-Pyridinylmethyl-morpholine derivatives of general formula A

A,

processes for their preparation, pharmaceutical compositions containing them and their use in therapy, particularly in the treatment or prevention of conditions having an asso ciation with NR2B negative allosteric modulating properties.

The compounds of the invention according to general formula A show NR2B negative allosteric modulating properties.

Extensive studies over the past twenty years have indicated that N-methyl-D-aspartate receptors (NMD A) play a relevant role in Alzheimer's disease, Parkinson's disease, dys- kinesia, stroke, motor neuron disease, psychosis, epilepsy, anxiety, schizophrenia and pain.

The non-selective NMDA receptor antagonist ketamine, (racemic as well as the S enan tiomer), a medication mainly used for starting and maintaining anaesthesia, has demon strated over the last years clinical efficacy in treating major depressive disorder (MDD) at subanaesthetic doses (Murrough et al. 2013, Am J Psychiatry. 170: 1134; Singh et al. 2016, Biol Psychiatry. 80: 424). More precisely, ketamine elicits a rapid onset of effica cy which lasts several days in MDD patients insufficiently responding to standard drug therapy (Berman et al. 2000. Biol Psychiatry 47:351, Serafini et al. 2014. Curr. Neuro- pharmaco 1.12:444). However, non-selective NMDA receptor antagonists have a range of undesirable effects which limit their application. In particular dissociative and psy chogenic side effects are prominent for the non-selective NMDA receptor antagonists such as ketamine (Krystal et al. 1994. Arch. Gen. Psychiatry 51 :199). In the early l990s, it was found that multiple NMDA receptor subtypes exist, which contain differ ent NR2(A-D) subunits (Paoletti et ah, 2013 Nat Rev. Neurosci 14:383). More recently, NR2B subtype selective NMDA receptor negative allosteric modulators (NR2B NAM) have raised interest and have shown potential in a wide range of clinical indications, such as attention, emotion, mood, and pain, as well as being involved in a number of different human disorders (Mony et. al. 2009. Br. J. Pharmacol. 157:1301; Chaffey et al, Current Anaesthesia & Critical Care 19, 183). In particular, NR2B NAM have also demonstrated antidepressant efficacy in the early stage of clinical trials (Preskom et al. 2008. J Clin Psychopharmacol 70:58). Preclinical studies using NR2B NAM as well as applying various transgenic mice strains have shown that NR2B containing NMDA- receptors are mediating the positive effect of ketamine in e.g. the Forced Swim Test (Miller et al. 2014 eLife 3:e0358l; Kiselycznyk et al. 2015, Behav Brain Res, 287:89). Furthermore, selective NR2B NAM have advantages over unselective NMDA receptor antagonists, such as ketamine, due to greatly diminished dissociative and psychotomi- metic side effects (Jimenez- Sanchez et al. 2014. Neuropsychopharmacology 39:2673).

NR2B NAM described to date have exhibited drawbacks with regard to their receptor pharmacology and/or to other drug properties which have limited potential use in hu man drug therapy (Taylor, et al., 2006, Clin Pharmacokinet.45: 989;Addy et al. 2009 J of Clinical Pharmacology 49:856)).

WO2015/130905 discloses compounds of formula (I)

that are inhibitors of Navl.6 useful in the treatment of multiple sclerosis, polyneuritis, multiple neuritis, amyotrophic lateral sclerosis, Alzheimer's disease or Parkinson's dis- ease. W02015/130905 discloses the specific examples 100, 105, 106 and 107 in which ring B corresponds to a meta-disubstituted phenyl ring. Example 100 Example 105 Example 106 Example 107

W02015/130905 reports specific examples 100, 105, 106 and 107 to be weak Navl.6 inhibitors (Nav 1.6 blockage of examples 100, 105 and 107 at 1-5 mM, and Nav 1.6 blockage of example 106 at >5 mM).

Compounds of the present invention are generically encompassed by formula (I) of WO2015/130905. The compounds of the present invention differ structurally from the examples 100, 105, 106 and 107 explicitly disclosed in W02015/130905 in that they contain a para-disubstituted pyridyl substructure in place of the meta-disubstituted phe- nyl ring.

The structural differences unexpectedly result in potent NR2B negative allosteric modu- lators (see Table 1), whereas the specific examples 100, 105, 106 and 107 of

W02015/130905 do not show any activity on the NR1-NR2B ion channel (see Table 2). Furthermore, compounds of the present invention do not inhibit Nav 1.6 at concentra tions at which specific examples 100 and 105 of W02015/130905 inhibit Nav 1.6 (5 mM; see Tables 3 and 4).

Further, the compounds of the present invention show good membrane permeability and no in vitro efflux (see Table 5 for MDCK assay MDR1 (P-gp)). Therefore, compounds of the present invention are expected to show a favorable brain penetration which is re- quired for efficacious CNS medicaments.

The MDCK assays provide information on the potential of a compound to pass the blood brain barrier. Permeability measurements across polarized, confluent MDCK- MDR1 cell monolayers grown on permeable filter supports are used as an in vitro ab- sorption model: apparent permeability coefficients (PE) of the compounds across the MDCK-MDR1 cell monolayers are measured (pH 7.4, 37°C) in apical-to-basal (AB) and basal-to-apical (BA) transport direction. The AB permeability (PEAB) represents drug absorption from the blood into the brain and the BA permeability (PEBA) drug efflux from the brain back into the blood via both, passive permeability as well as active transport mechanisms mediated by efflux and uptake transporters that are expressed on the MDCK-MDR1 cells, predominantly by the overexpressed human MDR1. Identical or similar permeabilities in both transport directions indicate passive permeation (PE- BA/PEAB <l), vectorial permeability points to additional active transport mechanisms. Higher PEBA than PEAB (PEBA/PEAB >5) indicates the involvement of active efflux mediated by MDR1 , which might compromise the goal to achieve sufficient brain expo- sure. Therefore, this assay provides valuable support for selection of compounds appli cable for further in vivo testing. High permeability not limited by efflux at the blood brain barrier is a favorable characteristic for compounds that are to be used for drugs acting primarily in the CNS.

Further, the compounds of the present invention are metabolically stable in human liver microsomes (see Table 6, metabolic stability). Therefore, compounds of the present in vention are expected to have a favorable in vivo clearance and thus the desired duration of action in humans.

Stability in human liver microsomes refers to the susceptibility of compounds to bio transformation in the context of selecting and/or designing drugs with favorable phar macokinetic properties. The primary site of metabolism for many drugs is the liver. Human liver microsomes contain the cytochrome P450s (CYPs), and thus represent a model system for studying drug metabolism in vitro. Enhanced stability in human liver microsomes is associated with several advantages, including increased bioavailability and adequate half-life, which can enable lower and less frequent dosing of patients. Thus, enhanced stability in human liver microsomes is a favorable characteristic for compounds that are to be used for drugs. Consequently, compounds of the present invention must be more viable for human use.

The objective technical problem is thus to provide potent and selective NR2B negative allosteric modulators. The present invention provides novel 4-Pyridinylmethyl-morpholine derivatives of for mula A

A

in which

Xi is N and X ₂ is CH, or

Xi is CH and X ₂ is N, R ¹ represents methyl, ethyl, propyl, /.so- propyl, cyclopropyl, H ₃ C-CH ₂ -CH ₂ -CH ₂ -, cyclobutyl;

R ² represents phenyl which is optionally substituted with 1 , 2 or 3 substituents se- lected from the group consisting of fluoro, chloro, methyl, ethyl, cyclopropyl; or a salt thereof, particularly a pharmaceutically acceptable salt thereof

According to another embodiment, the present invention comprises compounds of the general formula A1 or formula A2

A1 A2,

in which R ¹ and R ² have the same meaning as defined in any of the preceding embodi- ments. In another embodiment, in the general formula A, Al, A2, Xi, X ₂ , R ² have the same meaning as defined in any of the preceding embodiments, and

R ¹ represents methyl. In another embodiment, in the general formula A, Al, A2, Xi, X ₂ , R ¹ have the same meaning as defined in any of the preceding embodiments, and

R ² represents

The present invention provides novel 4-Pyridinylmethyl-morpholine derivatives of gen eral formula A that unexpectedly are potent and selective negative allosteric modulators ofNR2B.

Another aspect of the invention refers to compounds according to formula A as potent and selective NR2B negative allosteric modulators having high membrane permeability and no in vitro efflux.

Another aspect of the invention refers to compounds according to formula A as potent and selective NR2B negative allosteric modulators having high metabolic stability in human liver microsomes. Another aspect of the invention refers to compounds according to formula A as potent and selective NR2B negative allosteric modulators having high membrane permeability, no in vitro efflux, and high metabolic stability in human liver microsomes. Another aspect of the invention refers to pharmaceutical compositions, containing at least one compound according to formula A optionally together with one or more inert carriers and/or diluents.

A further aspect of the present invention refers to compounds according to formula A, for the use in the prevention and/or treatment of disorders associated with NR2B nega tive allosteric modulators.

Another aspect of the invention refers to processes of manufacture of the compounds of the present invention.

Preparation

The following schemes shall illustrate generally how to manufacture the compounds according to general formula A and the corresponding intermediate compounds by way of example. The abbreviated substituents may be as defined above if not defined other- wise within the context of the schemes.

Scheme 1

Scheme 1 illustrates the synthesis of pyridine derivatives of general formula A2.The first step is a nucleophilic substitution of a substituted phenol derivative R2-OH and 6- chloro-pyridine-3-carbaldehyde; the last step is represented by a reductive amination involving the aldehyde and a slight excess of an amide derivative of the (S)- Morpholine-2-carboxylic acid obtained by reacting (S)-Morpholine-2-carboxylic acid methyl ester with the corresponding amine Rl-NH ₂ .

The described synthetic approach can be used also for gram scale synthesis applying different purification techniques such as crystallization or column chromatography. Scheme 2

Scheme 2 illustrates the synthesis of pyridine derivatives of general formula Al.The first step is a nucleophilic substitution of a substituted phenol derivative R2-OH and 5- Fluoro-pyridine-2-carbaldehyde; the last step is represented by a reductive amination involving the aldehyde and a slight excess of an amide derivative of the (S)- Morpholine-2-carboxylic acid obtained by reacting (S)-Morpholine-2-carboxylic acid methyl ester with the corresponding amine RI-NH2.

The described synthetic approach can be used also for gram scale synthesis applying different purification techniques such as crystallization or column chromatography.

GENERAL DEFINITIONS

Terms not specifically defined herein should be given the meanings that would be given to them by one skilled in the art in light of the disclosure and the context. NR2B ion channel should be understood as NMDA receptor containing the NR2B pro- tein.

In case a compound of the present invention is depicted in form of a chemical name as well as a formula, the formula shall prevail in case of any discrepancy.

An asterisk may be used in sub-formulas to indicate the bond which is connected to the core molecule or to the substituent to which it is bound as defined.

The term "substituted" as used herein means that any one or more hydrogens on the des- ignated atom is replaced with a selection from the indicated group, provided that the designated atom's viable valence number is not exceeded, and that the substitution re- sults in a stable compound.

Stereochemistry:

Unless specifically indicated, throughout the specification and the appended claims, a given chemical formula or name shall encompass rotamers, tautomers and all stereo, optical and geometrical isomers (e.g. enantiomers, diastereoisomers, E/Z isomers etc.) and racemates thereof, as well as mixtures in different proportions of the separate enan tiomers, mixtures of diastereoisomers, or mixtures of any of the foregoing forms where such isomers and enantiomers exist. Salts:

The phrase "pharmaceutically acceptable" is employed herein to refer to those com pounds, materials, compositions, and/or dosage forms which are, within the scope of sound medical judgment, suitable for use in contact with the tissues of human beings without excessive toxicity, irritation, allergic response, or other problem or complica- tion, and commensurate with a reasonable benefit/risk ratio.

As used herein, "pharmaceutically acceptable salts" refer to derivatives of the disclosed compounds wherein the parent compound forms a salt or a complex with an acid or a base.

Examples for acids forming a pharmaceutically acceptable salt with a parent compound containing a basic moiety include mineral or organic acids such as benzenesulfonic ac id, benzoic acid, citric acid, ethanesulfonic acid, fumaric acid, gentisic acid, hydrobro- mic acid, hydrochloric acid, maleic acid, malic acid, malonic acid, mandelic acid, me- thanesulfonic acid, 4-methyl-benzenesulfonic acid, phosphoric acid, salicylic acid, suc cinic acid, sulfuric acid or tartaric acid. Examples for cations and bases forming a pharmaceutically acceptable salt with a parent compound containing an acidic moiety include Na ⁺ , K ⁺ , Ca ²⁺ , Mg ²⁺ , NH ₄ ⁺ , L-arginine, 2,2’-iminobisethanol, L-lysine, N-methyl-D-glucamine or tris(hydroxymethyl)- aminomethane.

The pharmaceutically acceptable salts of the present invention can be synthesized from the parent compound which contains a basic or acidic moiety by conventional chemical methods. Generally, such salts can be prepared by reacting the free acid or base forms of these compounds with a sufficient amount of the appropriate base or acid in water or in an organic diluent like ether, ethyl acetate, ethanol, isopropanol, or acetonitrile, or a mixture thereof Salts of other acids than those mentioned above which for example are useful for purifying or isolating the compounds of the present invention (e.g. trifluoro- acetate salts) also comprise a part of the invention.

BIOLOGICAL ASSAYS AND DATA

List of abbreviations

DMEM Dulbecco's Modified Eagle's Medium

FBS fetal Bovine Serum

FLIPR fluorometric imaging plate reader

HEK293 cell line derived from human embryonic kidney cells

HEPES hydroxyethyl-piperazineethane-sulfonic acid buffer

IC50 half maximal inhibitory concentration

MDCK Madin-Darby canine kidney

MDR1 Multi drug resistance protein 1

P-gp p-Glycoprotein

SEM standard error mean

EGTA (ethylene glycol-bis(P-aminoethyl ether)-N,N,N’,N’-tetraacetic acid), also known as egtazic acid

In-vitro effect:

Determination of in vitro Pharmacological Activity

The activity of the compounds of the invention may be demonstrated using the follow- ing in vitro NMD A NR1/NR2B cell assays: Method:

A human HEK293 cell line with tetracyclin-inducible expression of NMD A NR1/NR2B receptor was used as a test system for compound efficacy and potency. The cell line was purchased from ChanTest, Catalog #CT6l2l. Compound activity was determined by measuring the effect of compounds on intracellular calcium concentration induced by glycine/glutamate agonism in a FLIPRtetra system (Molecular Devices).

Cell culture:

The cells were obtained as frozen cells in cryo-vials and stored until use at -l50°C. Cells were grown in culture medium (DMEM/F12, 10% FBS, 5pg/mF Blasticidin, 150 Lig/mL Zeozin, 500pg/mF Geneticin). It is important that density does not exceed 80% confluence. For sub-culturing the cells were detached from flasks by Versene. For the assay, cells were detached, washed twice with induction medium (DMEM/F12 without glutamine, 10% FBS, 2pg/mF Tetracycline, 2mM Ketamine) and seeded to 384 well pure coat amine plates (Becton Dickinson, 50000 cells per well in 50 mΐ) 48 h prior to assay in induction medium.

Compound preparation

The test compounds were dissolved in 100% DMSO at a concentration of 10 mM and in a first step diluted in DMSO to a concentration of 5 mM, followed by serial dilution steps in 100% DMSO. Dilution factor and number of dilution steps may vary according to needs. Typically 8 different concentrations by 1 :5 dilutions were prepared in dupli- cate, further intermediate dilutions (1:37.5) of the substances were carried out with aqueous assay buffer (l37mM NaCl, 4mM KC1, l.8mM CaCl ₂ , lOmM HEPES, lOmM Glucose, pH 7.4) resulting in a compound concentration 3 times above the final test concentration and DMSO at 2.7% resulting in 0.9% final DMSO concentration in the assay.

FLIPR assay:

At the assay day cells were washed 3x with assay buffer (as described above), 10 mE buffer remained in the wells after washing. 10 mE Ca kit loading buffer (AAT Bioquest; prepared from the kit containing the following components: Component A: Fluo-8 NW dissolved in 200mE DMSO and 20 mΐ of this solution are mixed with 10 ml buffer pre- pared out of component B and C , Component B: 10X Pluronic® F127 Plus diluted 1 : 10 in component C, Component C: HHBS (Hanks with 20 mM Hepes) was added to the cells and the plates were incubated with lid for 60 minutes at room temperature.

20 mΐ assay buffer containing 60 mM glycine (20mM final) and 3 mM glutamate (1 mM final) was added to column 1-23, column 24 got assay buffer without glycine/glutamate to serve as negative unstimulated control. Fluorescence (indicating the calcium influx as a result of the NR1/NR2B ion channel activation) was read on the FLIPRtetra device for 60 seconds to monitor the glutamate induced effects. After 2 minutes 20 pL of com pound dilution prepared as described above or controls (row 1-22) in assay buffer were carefully added to the wells. Fluorescence was read on the FLIPR tetra device for addi- tional 6 minutes to monitor the compound induced effects after activation by agonists. The average of 2 measurements at 5 minutes and 5 min 10 seconds after compound ad dition is calculated and further used for IC50 calculations. Each assay microtiter com pound dilution plate contained wells (in column 23 or 24) with DMSO controls instead of compound as controls for glycine/glutamate induced fluorescence (high controls) and wells with 1 mM of a reference NR2B NAM as low controls (Compound 22; reference: Layton, Mark E et al, ACS Chemical Neuroscience 2011, 2(7), 352-362).

Data evaluation and calculation:

The output file of the reader contains the well number and measured average fluores- cence units. For data evaluation and calculation, the measurement of the low control was set as 0% control and the measurement of the high control was set as 100% control. The IC50 values were calculated using the standard 4 parameter logistic regression for mula. Calculation: [y=(a-d)/(l+(x/c) ^A b)+d], a = low value, d = high value; x = cone M; c=IC50 M; b = slope.

NR2B negative allosteric modulators covered by general structure A and exhibiting a low IC5 ₀ value are preferred.

Table 1 In vitro NR2B affinity of the compounds of the present invention as obtained in the FLIPR assay

Table 2 In vitro NR2B affinity of the closest prior art compounds (examples 100, 105, 106 and 107 in W02015/130905) as obtained in the same FLIPR assay as compounds in Table 1

Determination of Nav 1.6.Inhibition

Equipment:

IonWorks Quattro electrophysio logical platform Compound Plate Preparation

The compounds were prepared in DMSO at 300x the final assay concentrations of 1 and 5mM.

The 300x DMSO stock solutions were transferred into assay plates where 2m1 per well of each 300x stock solution were placed. All assay plates were stored at -80°C until the day of assay.

On the day of the assay, the appropriate assay plate was thawed at room temperature, centrifuged, and 198m1 of external recording solution was added and mixed thoroughly. This provided a 1 : 100 dilution. A further 1 :3 dilution occurred upon addition to the cells in the IonWorks Quattro electrophysio logical platform, giving a 1 :300 dilution in total. On each assay plate, at least 8 wells were reserved for vehicle control (0.3% DMSO) and at least 8 wells for each positive control specific to the cell line tested. The positive controls were tested at a maximal blocking and an approximate IC50 concentration. As positive control Lidocaine at concentrations of 30 and 1000 mM was used.

Electrophysiological Recording Solutions

The solutions for recording Navi.6 currents were as follows:

External Recording Solution

NaCl l37mM

KC1 4mM

MgCl ₂ lmM

CaCl ₂ l.8mM

HEPES lOmM

Glucose lOmM

pH 7.3 (titrated with 10M NaOH)

Internal Recording Solution

CsF 90mM

CsCl 45mM

HEPES lOmM

EGTA lOmM

pH 7.3 (titrated with 1M CsOH) Amphotericin B was used to obtain electrical access to the cell interior at a final concen tration of 200pg/ml in internal recording solution.

Experimental Protocols & Data Analysis

Navi.6 Experimental Protocol

State-dependent inhibition: Sodium channels when held at depolarized potential or long test pulse, the channels open and inactivate and then stay inactivated until the membrane potential is stepped back to hyperpolarized potentials, when the inactivated channels recover from inactivation into closed state. An example is Tetracaine inhibition, which is much stronger at depolarized potentials than at hyperpolarized potential.

Command Voltage

Time (msec)

Navl.6 Data Analysis

Cells were held at -l20mV. In order to completely inactivate the sodium channels (pulse 1), the cells were pulsed to +0mV for 2500ms and stepped back to -l20mV for lOms (to completely recover from inactivation, however channels that had drugs bound to them will not recover from inactivation) before stepping to +0mV for 20ms (pulse 2).

IonChannel Profiler Data Filters

Assay Control Results

Both the positive and vehicle control data associated with each cell line assayed are shown below as an example. The mean is shown for each positive and negative control as solid symbol with the total number of individual well replicates given next to the sol- id symbol. In addition, the individual data of each well are shown on the graph as open symbols so that the variation about the mean value can be readily assessed. These data are provided to aid in determining whether a compound has activities on the ion channel relative to the control data and provides an indication of assay variability and according- ly is used to judge the effect size of a compound-specific effect that can be detected.

Shown below are the assay controls for the Navl.6 IonWorks Quattro assay. Lidocaine, a Navl.6 reference compound, inhibited evoked currents in a concentration and use de- pendent manner as predicted.

Pl - pulse 1; P25 - pulse 25.

A Post/Pre value of 1.0 corresponds to 0% inhibition, a Post/Pre value of 0.0 corresponds to 100% inhibition. To illustrate the variation of the assay, both example 106 of W02015/130905 showing 14% inhibition of Nav 1.6 at 5 mM (normalized, see Table 3) and example 19 of the present invention show- ing -6.3% inhibition of Nav 1.6 at 5 mM (normalized, see Table 4), respective- ly, are within the variation of the assay when compared to assay control data, and are therefore not showing any significant inhibition of the Nav 1.6 channel at 5 mM.

Tables 3 and 4 show the normalized percentage inhibition of Navl.6 channel. The nor malized data show the compound data normalized to vehicle control (0% inhibition) and maximal inhibition control (100% inhibition); maximum inhibition at Pl by 1000 mM lidocaine (not normalized) was ranging from 46.4% to 47.2% across the experiments. (see also the figure Assay Control Results above).

Table 3 Normalized in vitro Nav 1.6 inhibition of the closest prior art compounds (ex amples 100, 105, 106 and 107 in W02015/130905) as obtained in the same electrophysiology assay as compounds in Table 4 (concentrations: 1 mM and 5 mM).

Table 4 Normalized in vitro Nav 1.6 inhibition of the compounds of the present inven tion as obtained in the same electrophysiology assay as prior art compounds in Table 3 (concentrations: 1 mM and 5 mM).

NR2B negative allosteric modulators covered by general structure A which are not showing any significant Navl.6 inhibition are preferred.

The compounds of the present invention do not show any significant inhibition of the Nav 1.6 channel at 1 and 5 mM, respectively (see Table 4 and Assay Control Results), whereas examples 100 and 105 of WO2015/130905 show 37.8% and 68% inhibition of Nav 1.6 at 5mM (see Table 3). Examples_106 and 107 of W02015/130905 do not show any significant inhibition of the Nav 1.6 channel at 1 and 5 mM, respectively (i.e. inhibi- tion is within assay variability, see Table 3 and Assay Control Results).

MDCK assay P-gp

Apparent permeability coefficients (Papp) of the compounds across the MDCK-MDR1 monolayers (MDCKII cells transfected with human MDR1 cDNA expression plasmid) are measured in apical-to-basal (AB) and basal-to-apical (BA) direction.

MDCK-MDR1 cells (6 x 10 ⁵ cells/cm ² ) are seeded on filter inserts (Coming, Transwell, polycarbonate, 0.4 pm pore size) and cultured for 9 to 10 days. Compounds dissolved in DMSO stock solution (1 - 20 mM) are diluted with HTP-4 aqueous buffer (128.13 mM NaCl, 5.36 mM KC1, 1 mM MgS0 ₄ , 1.8 mM CaCl ₂ , 4.17 mM NaHCOs, 1.19 mM Na ₂ HP0 ₄ , 0.41 mM NaH ₂ P0 ₄ , 15 mM HEPES, 20 mM glucose, pH 7.4) supplemented with 0.25% BSA to prepare the transport solutions (final concentration: 1 or 10 mM, fi nal DMSO <= 0.5 %). The transport solution is applied to the apical or baso lateral do- nor side for measuring A-B or B-A permeability, respectively. The receiver side con tains HTP-4 buffer supplemented with 0.25% BSA. Samples are collected at the start and end of experiment from the donor and at various time intervals for up to 2 hours also from the receiver side for concentration measurement by HPLC-MS/MS (Rapid- Fire High-throughput MS System (Agilent) coupled to QTrap 6500 (AB Sciex) or TSQ Vantage (Thermo Scientific)). Sampled receiver volumes are replaced with fresh re- ceiver solution. Efflux ratio is calculated dividing the Papp (b-a) values by the Papp (a- b) values. Results are shown in Table 5.

Table 5

The experimental results above show that compounds of the present invention are po- tent NR2B NAMs having high membrane permeability and no in vitro efflux anticipat- ing excellent capability to cross the blood brain barrier.

Metabolic stability

The metabolic degradation of the test compound was assayed at 37 °C with pooled hu- man liver microsomes. The final incubation volume of 60 mΐ per time point contains TRIS buffer pH 7.6 at room temperature (0.1 M), magnesium chloride (5 mM aqueous solution), microsomal protein (1 mg/mL for human) and the test compound at a final concentration of 1 mM. Following a short preincubation period at 37°C, the reactions were initiated by addition of betanicotinamide adenine dinucleotide phosphate, reduced form (NADPH, 1 mM), and terminated by transferring an aliquot into acetonitril after different time points. After centrifugation (10000 g, 5 min), an aliquot of the superna tant was assayed by HPLC-MS/MS as described above for the MDCK assay P-gp for the amount of parent compound. The half-life was determined by the slope of the semi- logarithmic plot of the concentration-time profile. Results are shown in Table 6.

Table 6

The experimental results above show that compounds of the present invention are po tent NR2B NAMs having high stability in human liver microsomes.

The present invention provides compounds according to formula A that unexpectedly result in a favorable combination of the following key parameters:

1) potent and selective negative allosteric modulation of NR2B,

2) high stability in human liver microsomes, and

3) high permeability and no in vitro efflux at MDCK-MDR1 cell transporters. Pharmaceutical Composition

Suitable preparations for administering the compounds of the present invention will be apparent to those with ordinary skill in the art and include for example tablets, pills, capsules, suppositories, lozenges, troches, solutions, syrups, elixirs, sachets, injectables, inhalatives, powders, etc.. The content of the pharmaceutically active compound(s) may vary in the range from 0.1 to 95 wt.-%, preferably 5.0 to 90 wt.-% of the composition as a whole.

Suitable tablets may be obtained, for example, by mixing a compound of the present invention with known excipients, for example inert diluents, carriers, disintegrants, ad- juvants, surfactants, binders and/or lubricants and pressing the resulting mixture to form tablets.

Use in treatment/method of use

Human therapeutic applications of NR2B NAM have been summarized in reviews by Traynelis et al. (Traynelis et ah, Pharmacology Reviews, 2010, 62:405), Beinat et al. (Beinat et al., Current Medicinal Chemistry, 2010, 17:4166) and Mony et al. (Mony et al, British J. Pharmacology, 2009, 157:1301).

The present invention relates to compounds which are useful in the treatment of psychi atric disorders, diseases and conditions wherein negative allosteric modulation of NR2B is of therapeutic benefit, including: (1) mood disorders and mood affective disorders;

(2) schizophrenia spectrum disorders; (3) neurotic, stress-related and somatoform disor ders including anxiety disorders; (4) disorders of psychological development; (5) behav ioral syndromes associated with physiological disturbances and physical factors; (6) substance-related and addictive disorders; (7) disease associated with symptoms of neg- ative and positive valence; (8) pain; (9) cerebrovascular diseases; (10) episodic and par oxysmal disorders; (11) neurodegenerative diseases.

In view of their pharmacological effect, compounds of the present invention are suitable for use in the treatment of a disorder, disease or condition selected from the list consist ing of

(1) treatment of mood disorders and mood affective disorders including bipolar disorder

I depressed, hypomanic, manic and mixed form; bipolar disorder II; depressive disor ders, such as single depressive episode or recurrent major depressive disorder, minor depressive disorder, depressive disorder with postpartum onset, depressive disorders with psychotic symptoms; major depressive disorder with or without concomitant anx- ious distress, mixed features, melancholic features, atypical features, mood-congruent psychotic features, mood-incongruent psychotic features, catatonia.

(2) treatment of mood disorders belonging to the schizophrenia spectrum and other psy- chotic disorders including schizophrenia and schizoaffective disorder with associated negative and cognitive symptoms.

(3) treatment of disorders belonging to the neurotic, stress-related and somatoform dis- orders including anxiety disorders, general anxiety disorder, panic disorder with or without agoraphobia, specific phobia, social phobia, chronic anxiety disorders; obses- sive compulsive disorder; reaction to sever stress and adjustment disorders, such as post-traumatic stress disorder; other neurotic disorders such as depersonalisation- derealisation syndrome.

(4) treatment of disorders of psychological development including pervasive develop mental disorders, including Asperger's syndrome and Ret's syndrome, autistic disor ders, childhood autism and overactive disorder associated with mental retardation and stereotyped movements, specific developmental disorder of motor function, specific de velopmental disorders of scholastic skills, atention deficit/hyperactivity disorder.

(5) treatment of behavioral syndromes associated with physiological disturbances and physical factors including mental and behavioural disorders associated with the puerper- ium, including postnatal and postpartum depression; eating disorders, including anorex- ia nervosa and bulimia nervosa and other impulse control disorders.

(6) treatment of disorders of substance-related and addicitive disorders, which are sub stance use disorders induced by alcohol, cannabis, hallucinogen, stimulant, hypnotic, tobacco.

(7) treatment of disease associated with symptoms of negative and positive valence in- eluding anhedonia, sustained threat and loss, suicidal ideation.

(8) treatment of acute and chronic pain which is related to neuropathy, e.g. diabetic neu ropathy or polyneuropathy, physiological processes and physical disorders including e.g. low back pain, pain in the joints, disease of the musculoskeletal system and connec tive tissue, e.g. rheumatism, myalgia, nerve, nerve root and plexus disorders, e.g. phan- tom limb syndrome with pain, carpal tunnel syndrome.

(9) treatment of cerebrovascular diseases, e.g. intracerebral or subararchnoid haemor rhage, cerbral infarction, stroke, occlusion and stenosis, cerebral atherosclerosis, cere bral amyloid angiopathy.

(10) treatment of episodic and paroxymal disorders, e.g. epilepsy. (11) treatment of diseases which include forms of neurodegeneration, e.g. stroke, Alz heimer’s disease and Huntingon’s disease.

As used herein, unless otherwise noted, the terms“treating”,“treatment” shall include the management and care of a human subject or human patient for the purpose of com- bating a disease, condition, or disorder and includes the administration of a compound of the present invention to prevent the onset of the symptoms or complications, alleviate the symptoms or complications, or eliminate the disease, condition, or disorder.

As used herein, unless otherwise noted, the term“prevention” shall include (a) reduc- tion in the frequency of one or more symptoms; (b) reduction in the severity of one or more symptoms; (c) the delay or avoidance of the development of additional symptoms; and/or (d) delay or avoidance of the development of the disorder or condition.

According to another aspect, the present invention provides a compound of formula A or a pharmaceutically acceptable salt thereof for use in the treatment and/or prevention of the above mentioned conditions.

According to another aspect, the present invention provides a compound of formula A according to any one of the preceding aspects characterized in that the compound of formula A is used in addition to behavioural therapy, TMS (transcranial magnetic stimulation), ECT (electroconvulsive therapy) and other therapies. Combination Therapy

Compounds according to the present invention can be combined with other treatment options known to be used in the art in connection with a treatment of any of the indica tions the treatment of which is in the focus of the present invention.

According to another aspect, the present invention provides a compound of formula A according to any one of the preceding aspects characterized in that the compound of formula A is administered in addition to treatment with one or more antidepressant se lected from the list consisting of duloxetine, escitalopram, bupropion, venlafaxine, desvenlafaxine, sertraline, paroxetine, fluoxetine, vortioxetine, mirtazapine, citalopram, vilazodone, trazodone, amitriptyline, clomipramine, agomelatine, levomilnacipran, lith- ium, doxepin, nortriptyline. The term“antidepressant” shall mean any pharmaceutical agent or drug which can be used to treat depression or diseases assocaited with depres sive symptoms.

According to another aspect, the present invention provides a compound of formula A according to any one of the preceding aspects characterized in that the compound of formula A is administered in addition to treatment with one or more antipsychotic se- lected from the list consisting of aripiprazole, paliperidone palmitate, lurasidone, queti- apine, risperidone, olanzapine, paliperidone, brexpiprazole, clozapine, asenapine, chlor- promazine, haloperidol, cariprazine, ziprasidone, amisulpride, iloperidone, fluphena- zine, blonanserin, aripiprazole lauroxil. The term“antipsychotic” shall mean any phar maceutical agent or drug which can be used to treat diseases associated with psychotic or depressive symptoms.

According to another aspect, the present invention provides a compound of formula A according to any one of the preceding aspects characterized in that the compound of formula A is administered in addition to treatment with one or more psychostimulant selected from the list consisting of lisdexamfetamine, methylphenidate, amfetamine, dexamfetamine, dexmethylphenidate, armodafinil, modafinil. The term“psychostimu- lant” shall mean any pharmaceutical agent or drug which can be used to treat diseases like mood disorders, or impulse control disorders.

According to another aspect, the present invention provides a compound of formula A according to any one of the preceding aspects characterized in that the compound of formula A is administered in addition to treatment with nootropics selected from the list consisting of oxiracetam, piracetam, or the natural product St John's-wort.

According to another aspect, the present invention provides a compound of formula A which is administered in addition to treatment with one or more antidepressant, antipsy- chotic, psychostimulant, nootropics or natural product according to any one of the pre- ceding aspects characterized in that the combination of compound of formula A and one or more antidepressant, antipsychotic, psychostimulant, nootropics or natural product is used in addition to behavioural therapy, TMS (transcranial magnetic stimulation), ECT (electroconvulsive therapy) and other therapies.

EXPERIMENTAL SECTION

Abbreviations:

ACN acetonitrile

APCI Atmospheric pressure chemical ionization

Boc tert-butylo xy carbonyl

CDI 1 , 1’-carbonyldiimidazole

C0 ₂ Carbon Dioxide

D day DA Diode Array

DCM dichloromethane

DIPE diisopropylether

DIPEA diisopropylethylamine

DMF dimethylformamide

e.e. enantiomeric excess

ESI electrospray ionization (in MS)

EtOAc ethylacetate

EtOH ethanol

Ex. example

h hour(s)

HATU 0-(7-azabenzotriazo 1- 1 -yl)-N,N,N’ ,N’ -tetramethyluronium- hexafluorophosphate

HPLC high performance liquid chromatography

HPLC-MS coupled high performance liquid chromatography-mass spectrometry M molar (mo EL)

MeOH methanol

min minute(s)

MS mass spectrometry

MW molecular weight

NH3 ammonia

PSI Pound per square inch

rt room temperature

R _t retention time

scC02 supercritical C0 ₂

solv solvent

TBTU 0-(benzotriazol- 1 -yl)-N,N,N',N'-tctramcthyluronium tetrafluoroborate

TEA triethylamine

TFA trifluoroacetic acid

THF tetrahydrofuran

TLC thin-layer chromatography

SFC Supercritical fluid chromatography

Abbreviations within spectral data:

1H- NMR Proton nuclear magnetic resonance br broad

d chemical shift

d doublet

dd doublet of doublets

dt doublet of triplets

DMSO-de hexa-deutero-dimethylsulfoxide

H proton

Hz Hertz (=1 /second)

J coupling constant

m multiplet

ppm parts per million

q quartet

s singlet

t triplet

td triplet of doublets

General Analytics.

All reactions were carried out using commercial grade reagents and solvents. NMR spectra were recorded on a Bruker AVANCE III HD 400 MHz instrument using Top- Spin 3.2 pl6 software. Chemical shifts are given in parts per million (ppm) downfield from internal reference trimethylsilane in d units. Selected data are reported in the fol- lowing manner: chemical shift, multiplicity, coupling constants (, J ), integration. Analyt ical thin-layer chromatography (TLC) was carried out using Merck silica gel 60 F254 plates. All compounds were visualized as single spots using short wave UV light. Low resolution mass spectra were obtained using a liquid chromatography mass spectrometer (LCMS) that consisted of an Agilent 1100 series LC coupled to a Agilent 6130 quadru- pole mass spectrometer (electrospray positive ionization). Methods:

HPLC-MS methods: Method 1

Method 2

Method 3

Chiral SFC analytical methods: Method 4: G IG IPA NH ₃ 001

Method s: G IG MeOH NH ₃ 001

Method 6: G C4 MeOH NH ₃ 001

Method 7: 1 SA 20 MEOH NH ₃ 001

Method 8: 1 IC 30 IPA NH ₃ 001

Microwave equipment: Biotage Initiator ⁺

Preparative HPLC method for purification:

Instrument: (Agilent 1100). Eluents: Water - NH ₄ OH 5% solution in Water - CEbCN; Flow: 50 ml/min; Temperature 60°C; Column: XBridge C18. Preparation of Intermediates:

Example la

(S)-Morpholine-2-carboxylic acid methyl ester hydrochloride (35.0 g; 193 mmol) was mixed together with 400 ml of a 8M solution of Methylamine in EtOH. The reaction mixture was stirred at room temperature over 60 hours. The solvent was removed under reduced pressure, THF (500 ml) and TEA (50 ml) were added and the reaction mixture stirred at room temperature during 12 hours. A precipitate was formed; the suspension was filtered via a glass filter and the filtrate solution was evaporated under reduced pressure. Obtained 23.5 g of the desired product as solid.

Example 5 a

6-Chloro-pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and 2,4-difluoro-phenol (1.22 ml; 12.7 mmol) are dissolved in DMF (10 ml) in a microwave vial; K2CO3 (2.20 g; 15.9 mmol) is added and the reaction mixture is stirred at 110 °C during 30 minutes. The re- action mixture is then partitioned between Ethyl Acetate (150 ml) and Water (80 ml); the organic phase is separated and washed with a solution of K2CO3 (10 % in water) and the dried over Na ₂ S0 ₄ . The crude product obtained after evaporation of the solvent is purified by flash-chromatography (Eluent: Petrol Ether / Ethyl Acetate 4/1). Obtained

2.3 g of the desired compound (content 70%) used as such in the next step. Example 5b

Example 5b was synthesised in analogy to Example 5a. Starting materials: 6-Chloro- pyridine-3 -carbaldehyde (1.50 g; 10.6 mmol) and 2-fluoro-4-methylphenol (1.38 ml; 12.7 mmol).

The crude obtained after work up was passed through a silica pad (Eluent: Petrol Ether /

Ethyl Acetate 4/1). Obtained 1.60 g of the desired compound (content 50%) used as such in the next step.

Example 5 c

Example 5c was synthesised in analogy to Example 5a. Starting materials: 6-Chloro- pyridine-3 -carbaldehyde (1.50 g; 10.6 mmol) and 2,-4-dimethylphenol (1.51 ml; 12.7 mmol).

The crude obtained after work up was passed through a silica pad (Eluent: Petrol Ether / Ethyl Acetate 4/1). Obtained 2.30 g of the desired compound (content 50%) used as such in the next step. Example 5d

Example 5d was synthesised in analogy to Example 5a. Starting materials: 6-Chloro- pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and 4-fluoro-phenol (1.43 g; 12.7 mmol). Obtained 1.40 g of the desired compound used as such in the next step.

Example 5e

Example 5e was synthesised in analogy to Example 5a. Starting materials: 6-Chloro- pyridine-3 -carbaldehyde (1.50 g; 10.6 mmol) and 2-fluoro-4-chloro-phenol (1.35 ml; 12.7 mmol).

Obtained 2.20 g of the desired compound (content 80-90%) used as such in the next step.

Example 5f

Example 5f was synthesised in analogy to Example 5a. Starting materials: 6-Chloro- pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and 4-chloro-phenol (1.63 g; 12.7 mmol). Obtained 2.40 g of the desired compound used as such in the next step.

Example 5

Example 5g was synthesised in analogy to Example 5a. Starting materials: 6-Chloro- pyridine-3 -carbaldehyde (1.50 g; 10.6 mmol) and 2-chloro-phenol (1.29 ml; 12.7 mmol).

Obtained 2.40 g of the desired compound used as such in the next step.

Example 5h

Example 5h was synthesised in analogy to Example 5a. Starting materials: 6-Chloro- pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and 2-fluoro-phenol (1.13 ml; 12.7 mmol).

Obtained 2.00 g of the desired compound used as such in the next step.

Example 5i

Example 5i was synthesised in analogy to Example 5a. Starting materials: 6-bromo- pyridine-3-carbaldehyde (1.89 g; 10.2 mmol) and 4-methyl-phenol (1.10 g; 10.2 mmol). Obtained 2.40 g of the desired compound (content 70 %) used as such in the next step.

Example 5i

4-Fluoro-phenol (1.34 g; 12.0 mmol) was dissolved in DMSO (30 ml); potassium tert- butoxide (1.48 g; 13.2 mmol) was added at room temperature and the mixture was stirred for 1 h at room temperature. 5-Fluoro-2-formyl pyridine (1.50 g; 12.0 mmol) was then added and the reaction mixture was stirred at room temperature during 16 hours. 200 ml of a 1/1 mixture Dietyl ether/Ethyl Acetate was added followed by 70 ml of wa ter. The phases were separated and the organic phase washed once more with water (20 ml). The organic phase was then dried over Na ₂ S0 ₄ ; the residue obtained after evapora- tion of solvents was purified by flash-chromatography employing as eluent Petrol Ether/Ethyl Acetate (ratio: 7/3). Obtained 1.80 g.

Example 5k

5-Fluoro-2-formyl pyridine (0.25 g; 2.00 mmol) and CS2CO3 (0.98g; 3.00 mmol) were suspended in DMF (10 ml); 2,4-difluoro-phenol (0.31 g; 2.40 mmol) was added and the reaction mixture was stirred at 80°C during 3 hours. Acetonitrile (20 ml) was added and the mixture was filtered before being purified via preparative HPLC. Obtained 0.25 g of the desired compound. Example 51

Example 51 was synthesised in analogy to example 5k. Starting materials: 5-Fluoro-2- formyl pyridine (0.25 g; 2.00 mmol) and 4-chloro-2-fluoro-phenol (0.26 ml; 2.40 mmol). Obtained: 0.35 g of the desired product.

Example 5m

Example 5m was synthesised in analogy to example 5k. Starting materials: 5-Fluoro-2- formyl pyridine (0.25 g; 2.00 mmol) and 2-fluoro-phenol (0.21 ml; 2.40 mmol).

Obtained: 0.23 g of the desired product.

Example 5n

Example 5n was synthesised in analogy to example 5k. Starting materials: 5-Fluoro-2- formyl pyridine (0.25 g; 2.00 mmol) and 2-fluoro-4-methyl-phenol (0.30 g; 2.40 mmol). Obtained: 0.34 g of the desired product.

Example 5o

5-Fluoro-2-formylpyridine (0.50 g; 4.00 mmol) and Phenol (0.45 g; 4.80 mmol) were dissolved in DMF (8 ml); CS2CO3 (1.43 g; 4.40 mmol) was added and the reaction mix ture was stirred at 80°C during 16 hours. The reaction mixture was then partitioned be- tween ethyl acetate (80 ml) and water (40 ml); the organic phase was separated and dried over Na ₂ S0 ₄ . The crude product obtained after evaporation of the solvent was di- luted with MeOH/H20 (10 mL), filtered and purified by preparative HPLC. Obtained 216 mg of the desired compound. Example 5p

6-Chloro-pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and Phenol (1.20 g; 12.7 mmol) were dissolved in DMF (10 ml) in a microwave vial; K2CO3 (2.20 g; 15.9 mmol) was added and the reaction mixture was stirred at 110 °C during 30 minutes. The reaction mixture was diluted with water (50 ml) and the obtained precipitate was filtered off, washed with water and dried in the air. Obtained 1.38 g of the desired compound.

Example 5q

6-Chloro-pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and 2,6-difluoro-phenol (1.65 g; 12.7 mmol) were dissolved in DMF (10 ml) in a microwave vial; K2CO3 (2.20 g; 15.9 mmol) was added and the reaction mixture was stirred at 110 °C during 30 minutes. The reaction mixture was then diluted with water (50 ml) and extracted with diethylether (70 ml). The organic phase was separated and dried over Na ₂ S0 ₄ . The crude product ob- tained after evaporation was used as such in the next step. Obtained 2.30 g of the de- sired compound. Example 5r

Example 5r was synthesised in analogy to example 5q. Starting materials: 6-Chloro- pyridine-3-carbaldehyde (0.40 g; 2.83 mmol) and 2-fluoro-6-methyl-phenol (0.39 g; 3.11 mmol). Obtained: 0.43 g of the desired product (content 85%).

Example 5 s

5-Fluoro-2-formylpyridine (0.50 g; 4.00 mmol) and 2,6-Difluorophenol (0.62 g; 4.80 mmol) were dissolved in DMF (8 ml) in a microwave vial; CS2CO3 (1.56 g; 4.80 mmol) was added and the reaction mixture was stirred at 80°C during 16 hours. The reaction mixture was diluted with water (40 ml) and the obtained precipitate was filtered off, washed with water and dried in the air. Obtained 0.73 g of the desired compound (con tent 85%). Example 5t

6-Chloro-pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and 2,5-difluoro-phenol (1.65 g; 12.7 mmol) were dissolved in DMF (10 ml) in a microwave vial; K2CO3 (2.20 g; 15.9 mmol) is added and the reaction mixture is stirred at 110 °C during 30 minutes. Water ( 50 ml) was added and the reaction mixture stirred over 30 min. The precipitate obtained after filtration was washed a second time with water (20 ml), dried and used as such in the next step. Obtained 2.32 g of the desired compound. Example 5u

Example 5u was synthesised in analogy to Example 5t. Starting materials: 6-Chloro- pyridine-3-carbaldehyde (1.50 g; 10.6 mmol) and 2-chloro-5-difluoro-phenol (1.32 ml; 12.7 mmol). Obtained 2.4 g of the desired cpd.

EXEMPLARY EMBODIMENTS

Example 11

Example la (150 mg; content 70%; 0.45 mmol) and Example 5a (77.2 mg, 0.54 mmol) were dissolved in DMF; Acetic acid (0.08 ml; 1.34 mmol) and DIPEA (0.11 ml; 0.63 mmol) were added and the reaction mixture was stirred 30 min. at 50°C; NaBH(OAc) ₃ (0.14 g; 0.67 mmol) was then added and the mixture was the stirred 22 hours at room temperature. The reaction mixture was then diluted with MeOH, filtered via a syringe filter and the obtained solution purified via preparative HPLC. Obtained 120 mg of the desired compound.

Example 12

Example 12 was synthesised in analogy to example 11.

Starting materials: Example 5b (150 mg; content 50%; 0.32 mmol) + Example la (56.1 mg; 0.39 mmol).

The crude was purified by preparative HPLC. Obtained 105 mg of the desired com pound.

Example 13

Example 13 was synthesised in analogy to example 11.

Starting materials: Example 5c (200 mg; content 50%; 0.44 mmol) + Example la (76.1 mg; 0.53 mmol).

The crude was purified by preparative HPLC. Obtained 119 mg of the desired com pound.

Example 14

Example 14 was synthesised in analogy to example 11.

Starting materials: Example 5d (150 mg; 0.69 mmol) + Example la (119 mg; 0.83 mmol). The crude was purified by preparative HPLC.

Obtained 149 mg of the desired compound.

Example 15

Example 15 was synthesised in analogy to example 11.

Starting materials: Example 5e (150 mg; content 85%; 0.51 mmol) + Example la (87.7 mg; 0.61 mmol). The crude was purified via preparative HPLC. Obtained 132 mg of the desired compound.

Example 16

Example 16 was synthesised in analogy to example 11.

Starting materials: Example 5f (150 mg; 0.64 mmol) + Example la (111 mg; 0.77 mmol).

The crude was purified by preparative HPLC. Obtained 85 mg of the desired compound.

Example 17

Example 17 was synthesised in analogy to example 11.

Starting materials: Example 5g (150 mg; content 90%; 0.58 mmol) + Example la (100 mg; 0.69 mmol).

The crude was purified by preparative HPLC. Obtained 191 mg of the desired com pound.

Example 19

Example 19 was synthesised in analogy to example 11.

Starting materials: Example 5h (150 mg; 0.69 mmol) + Example la (119 mg; 0.83 mmol). The crude was purified by preparative HPLC. Obtained 147 mg of the desired compound.

Example 29

Example 29 was synthesised in analogy to example 11.

Starting materials: Example 5i (250 mg; 60% content; 0.70 mmol) and Example la (127 mg; content 80%; 0.70 mmol). The crude was purified via preparative HPLC.

Obtained 174 mg of the desired product.

Example 30

Example 30 was synthesised in analogy to Example 11.

Starting materials: Example 5j (150 mg; 0.69 mmol) and Example la (124.5 mg; con tent 80%; 0.69 mmol). The crude was purified by preparative HPLC.

Obtained 157 mg of the desired compound.

Example 31

Example la (67.4 mg; 0.47 mmol) and example 5k (100 mg; 0.43 mmol) were dissolved in THF (3 ml); DIPEA (0.11 ml; 0.64 mmol) was added and the reaction mixture stirred 30 min before the addition of NaBH(OAc)3 (126 mg; 0.60 mmol). The mixture was stirred over 3 hours at room temperature, diluted with MeOH, filtered through a syringe filter and purified by preparative HPLC.

Obtained 53 mg of the desired compound.

Example 32

Example 32 was synthesised in analogy to example 31.

Starting materials: Example 51 (100 mg; 0.40 mmol) and Example la (63.0 mg; 0.44 mmol).

The crude was purified by preparative HPLC. Obtained 21 mg of the desired compound.

Example 33

Example 33 was synthesised in analogy to example 31.

Starting materials: Example 5m (100 mg; 0.46 mmol) and Example la (73.0 mg; 0.51 mmol). The crude was purified by preparative HPLC. Obtained 42 mg of the desired compound.

Example 34

Example 34 was synthesised in analogy to example 31.

Starting materials: Example 5n (100 mg; 0.43 mmol) and Example la (74.8 mg; 0.52 mmol). The crude was purified by preparative HPLC.

Obtained 62 mg of the desired compound.

Example 35

Example 35 was synthesised in analogy to example 31. Starting materials: Example 5o (100 mg; 0.50 mmol) and Example la (79.6 mg; 0.55 mmol). The mixture was stirred at room temperature overnight. The crude was purified by preparative HPLC. Obtained 95.0 mg of the desired compound.

Example 36

Example 36 was synthesised in analogy to example 31.

Starting materials: Example 5p (120 mg; 0.60 mmol) and Example la (95.5 mg; 0.66 mmol). The mixture was stirred at room temperature during 18 hours. The crude was purified by preparative HPLC. Obtained 140 mg of the desired compound.

Example 37

Example la (76.9 mg; 0.53 mmol) and example 5q (120 mg; content 95%; 0.49 mmol) were dissolved in THF (3 ml); DIPEA (0.12 ml; 0.68 mmol) was added and the reaction mixture stirred 30 min before the addition of NaBH(OAc) ₃ (126 mg; 0.60 mmol). The mixture was stirred over 18 hours at room temperature, diluted with MeOH, filtered through a syringe filter and purified by preparative HPLC. The product was diluted with water (5 ml) and the obtained precipitate is filtered off, washed with water and dried in the air. Obtained 106 mg of the desired compound.

Example 38

Example la (75.8 mg; 0.53 mmol) and example 5r (130 mg; content 85%; 0.48 mmol) were dissolved in THF (3 ml); DIPEA (0.12 ml; 0.67 mmol) was added and the reaction mixture stirred 30 min before the addition of NaBH(OAc) ₃ (152 mg; 0.72 mmol). The mixture was stirred over 18 hours at room temperature, diluted with MeOH (3 ml), fil tered through a syringe filter and purified by preparative HPLC.

Obtained 129 mg of the desired compound.

Example 39

Example 39 was synthesised in analogy to example 38.

Starting materials: Example 5s (130 mg; content 85%; 0.47 mmol) and Example la (74.5 mg; 0.52 mmol). The mixture was stirred at room temperature during 18 hours.

The crude was purified by preparative HPLC. Obtained 75.0 mg of the desired com pound.

Example 40

Example 40 was synthesised in analogy to example 38.

Starting materials: Example 5t (100 mg; 0.43 mmol) and Example la (67.43 mg; 0.47 mmol).

The crude was purified by preparative HPLC. Obtained 130 mg of the desired com- pound.

Example 41

Example 41 was synthesised in analogy to example 38.

Starting materials: Example 5u (100 mg; 0.4 mmol) and Example la (63 mg; 0.44 mmol). Obtained 135 mg of the desired compound.