CRYSTALLINE FORM OF LORLATINIB FREE BASE

Description

Field of the Invention

[0001] This invention relates to a new crystalline form of (10R)-7-amino-12-fluoro-2,10,16-trimethyl-15-oxo-10,15,16,17-tetrahydro-2H-8,4-(metheno)pyrazolo[4,3-h][2,5,11]benzoxadiaza-cyclotetradecine-3-carbonitrile (lorlatinib) free base (Form 7) and to Form 7 for use in the treatment of abnormal cell growth in mammals.

Background of the Invention

[0002] The compound (10R)-7-amino-12-fluoro-2,10,16-trimethyl-15-oxo-10,15,16,17-tetrahydro-2H-8,4-(metheno)pyrazolo[4,3-h][2,5,11]benzoxadiazacyclotetradecine-3-carbonitrile (PF-06463922), represented by the formula (I):

has been assigned the International Nonproprietary Name (INN) lorlatinib, as described in WHO Drug Information, Vol. 29, No. 4, page 541 (2015). Lorlatinib is a potent, macrocyclic inhibitor of both wild type and resistance mutant forms of anaplastic lymphoma kinase (ALK) and c-ros oncogene 1 (ROS1) receptor tyrosine kinase.

[0003] Preparation of the free base of lorlatinib as an amorphous solid is disclosed in International Patent Publication No. WO 2013/132376 and in United States Patent No. 8,680,111. Solvated forms of lorlatinib free base are disclosed in International Patent Publication No. WO 2014/207606.

[0004] Human cancers comprise a diverse array of diseases that collectively are one of the leading causes of death in developed countries throughout the world (American Cancer Society, Cancer Facts and Figures 2005. Atlanta: American Cancer Society; 2005). The progression of cancers is caused by a complex series of multiple genetic and molecular events including gene mutations, chromosomal translocations, and karyotypic abnormalities (Hanahan & Weinberg, The hallmarks of cancer. Cell 2000; 100: 57-70). Although the underlying genetic causes of cancer are both diverse and complex, each cancer type has been observed to exhibit common traits and acquired capabilities that facilitate its progression. These acquired capabilities include dysregulated cell growth, sustained ability to recruit blood vessels (i.e., angiogenesis), and ability of tumor cells to spread locally as well as metastasize to secondary organ sites (Hanahan & Weinberg 2000). Therefore, the ability to identify novel therapeutic agents that inhibit molecular targets that are altered during cancer progression or target multiple processes that are common to cancer progression in a variety of tumors presents a significant unmet need.

[0005] Receptor tyrosine kinases (RTKs) play fundamental roles in cellular processes, including cell proliferation, migration, metabolism, differentiation, and survival. RTK activity is tightly controlled in normal cells. The constitutively enhanced RTK activities from point mutation, amplification, and rearrangement of the corresponding genes have been implicated in the development and progression of many types of cancer. (Gschwind et al., The discovery of receptor tyrosine kinases: targets for cancer therapy. Nat. Rev. Cancer 2004; 4, 361-370; Krause & Van Etten, Tyrosine kinases as targets for cancer therapy. N. Engl. J. Med. 2005; 353: 172-187.)

[0006] Anaplastic lymphoma kinase (ALK) is a receptor tyrosine kinase, grouped together with leukocyte tyrosine kinase (LTK) to a subfamily within the insulin receptor (IR) superfamily. ALK was first discovered as a fusion protein with nucleophosmin (NPM) in anaplastic large cell lymphoma (ALCL) cell lines in 1994. (Morris et al., Fusion of a kinase gene, ALK, to a nucleolar protein gene, NPM, in non-Hodgkin's lymphoma. Science 1994; 263:1281-1284.) NPM-ALK, which results from a chromosomal translocation, is implicated in the pathogenesis of human anaplastic large cell lymphoma (ALCL) (Pulford et al., Anaplastic lymphoma kinase proteins in growth control and cancer. J. Cell Physiol., 2004; 199: 330-58). The roles of aberrant expression of constitutively active ALK chimeric proteins in the pathogenesis of ALCL have been defined (Wan et. al., Anaplastic lymphoma kinase activity is essential for the proliferation and survival of anaplastic large cell lymphoma cells. Blood, 2006; 107:1617-1623). Other chromosomal rearrangements resulting in ALK fusions have been subsequently detected in ALCL (50-60%), inflammatory myofibroblastic tumors (27%), and non-small-cell lung cancer (NSCLC) (2-7%). (Palmer et al., Anaplastic lymphoma kinase: signaling in development and disease. Biochem. J. 2009; 420:345-361.)

[0007] The EML4-ALK fusion gene, comprising portions of the echinoderm microtubule associated protein-like 4 (EML4) gene and the ALK gene, was first discovered in NSCLC archived clinical specimens and cell lines. (Soda et al., Identification of the transforming EML4-ALK fusion gene in non-small cell lung cancer. Nature 2007; 448:561-566; Rikova et al., Cell 2007; 131:1190-1203.) EML4-ALK fusion variants were demonstrated to transform NIH-3T3 fibroblasts and cause lung adenocarcinoma when expressed in transgenic mice, confirming the potent oncogenic activity of the EML4-ALK fusion kinase. (Soda et al., A mouse model for EML4-ALK-positive lung cancer. Proc. Natl. Acad. Sci. U.S.A. 2008; 105:19893-19897.) Oncogenic mutations of ALK in both familial and sporadic cases of neuroblastoma have also been reported. (Caren et al., High incidence of DNA mutations and gene amplifications of the ALK gene in advanced sporadic neuroblastoma tumors. Biochem. J. 2008; 416:153-159.)

[0008] ROS1 is a proto-oncogene receptor tyrosine kinase that belongs to the insulin receptor subfamily, and is involved in cell proliferation and differentiation processes. (Nagarajan et al. Proc Natl Acad Sci 1986; 83:6568-6572). ROS1 is expressed, in humans, in epithelial cells of a variety of different tissues. Defects in ROS1 expression and/or activation have been found in glioblastoma, as well as tumors of the central nervous system (Charest et al., Genes Chromos. Can. 2003; 37(1): 58-71). Genetic alterations involving ROS1 that result in aberrant fusion proteins of ROS1 kinase have been described, including the FIG-ROS1 deletion translocation in glioblastoma (Charest et al. (2003); Birchmeier et al. Proc Natl Acad Sci 1987; 84:9270-9274; and NSCLC (Rimkunas et al., Analysis of Receptor Tyrosine Kinase ROS1-Positive Tumors in Non-Small Cell Lung Cancer: Identification of FIG-ROS1 Fusion, Clin Cancer Res 2012; 18:4449-4457), the SLC34A2-ROS1 translocation in NSCLC (Rikova et al. Cell 2007;131:1190-1203), the CD74-ROS1 translocation in NSCLC (Rikova et al. (2007)) and cholangiocarcinoma (Gu et al. PLoS ONE 2011; 6(1): e15640), and a truncated, active form of ROS1 known to drive tumor growth in mice (Birchmeier et al. Mol. Cell. Bio. 1986; 6(9):3109-3115). Additional fusions, including TPM3-ROS1, SDC4-ROS1, EZR-ROS1 and LRIG3-ROS1, have been reported in lung cancer patient tumor samples (Takeuchi et al., RET, ROS1 and ALK fusions in lung cancer, Nature Medicine 2012; 18(3):378-381).

[0009] The ALK/ROS1/c-MET inhibitor crizotinib was approved in 2011 for the treatment of patients with locally advanced or metastatic NSCLC that is ALK-positive as detected by an FDA-approved test. Crizotinib has also shown efficacy in treatment of NSCLC with ROS1 translocations. (Shaw et al. Clinical activity of crizotinib in advanced non-small cell lung cancer (NSCLC) harboring ROS1 gene rearrangement. Presented at the Annual Meeting of the American Society of Clinical Oncology, Chicago, June 1-5, 2012.) As observed clinically for other tyrosine kinase inhibitors, mutations in ALK and ROS1 that confer resistance to ALK inhibitors have been described (Choi et al., EML4-ALK Mutations in Lung Cancer than Confer Resistance to ALK Inhibitors, N Engl J Med 2010; 363:1734-1739; Awad et al., Acquired Resistance to Crizotinib from a Mutation in CD74-ROS1, N Engl J Med 2013; 368:2395-2401).

[0010] Thus, ALK and ROS1 are attractive molecular targets for cancer therapeutic intervention. There remains a need to identify compounds having novel activity profiles against wild-type and mutant forms of ALK and ROS1.

[0011] The present invention provides a novel crystalline form of lorlatinib free base (Form 7) having desirable properties, such as high crystallinity, high purity, low hygroscopicity, and favorable dissolution and mechanical properties. In particular, Form 7 provides improved physical stability in the drug product formulation relative to the acetic acid solvate disclosed in International Patent Publication No. WO 2014/207606. Such solvated forms may present challenges for drug development, in particular with respect to physical stability. Consequently, there remains a need to identify novel forms having desirable physicochemical properties.

Summary of the Invention

[0012] In one aspect, the invention provides a novel crystalline form of lorlatinib free base (Form 7). Form 7 of lorlatinib free base is characterized by one or more of the following methods: (1) powder X-ray diffraction (PXRD) (2θ); (2) Raman spectroscopy (cm^-1); (3) ¹³C solid state NMR spectroscopy (ppm); or (4) ¹⁹F solid state NMR spectroscopy (ppm).

[0013] In a first aspect, the invention provides an anhydrous, non-solvated crystalline form of (10R)-7-amino-12-fluoro-2,10,16-trimethyl-15-oxo-10,15,16,17-tetrahydro-2H-8,4-(metheno)pyrazolo[4,3-h][2,5,11]benzoxadiaza-cyclotetradecine-3-carbonitrile (lorlatinib) free base (Form 7), which is characterized by having a ¹⁹F solid state NMR spectrum comprising resonance (ppm) values of -108.2 and -115.2 ppm ± 0.2 ppm, relative to an external standard of 50/50 volume/volume of trifluoroacetic acid and water, setting its resonances to -76.54 ppm.

[0014] The anhydrous, non-solvated crystalline form of lorlatinib free base (Form 7) is also characterized by having:

(1) a powder X-ray diffraction (PXRD) pattern (2θ) measured using copper wavelength radiation_comprising: (a) one, two, three, four, five, or more than five peaks selected from the group consisting of the peaks in Table 1 in °2θ ± 0.2 °2θ; (b) one, two, three, four, five, or more than five peaks selected from the group consisting of the characteristic peaks in Table 1 in °2θ ± 0.2 °2θ; or (c) peaks at 2θ values essentially the same as shown in Figure 1; or

(2) a Raman spectrum comprising: (a) one, two, three, four, five, or more than five wavenumber (cm^-1) values selected from the group consisting of the values in Table 2 in cm^-1 ± 2 cm^-1; (b) one, two, three, four, five, or more than five wavenumber (cm^-1) values selected from the group consisting of the characteristic values in Table 2 in cm^-1 ± 2 cm^-1; or (c) wavenumber (cm^-1) values essentially the same as shown in Figure 2; or

(3) a ¹³C solid state NMR spectrum (ppm) comprising: (a) one, two, three, four, five, or more than five resonance (ppm) values selected from the group consisting of the values in Table 3 in ppm ± 0.2 ppm; (b) one, two, three, four, five, or more than five resonance (ppm) values selected from the group consisting of the characteristic values in Table 3 in ppm ± 0.2 ppm; or (c) resonance (ppm) values essentially the same as shown in Figure 3, relative to an external standard of crystalline adamantane, setting its upfield resonance to 29.5 ppm;

or a combination of any one, two, or three of the foregoing embodiments (1)(a)-(c), (2)(a)-(c), or (3)(a)-(c), with the ¹⁹F solid state NMR spectrum as described herein, provided they are not inconsistent with each other.

[0015] In another aspect, the invention further provides a pharmaceutical composition comprising lorlatinib free base (Form 7), according to any of the embodiments described herein, and a pharmaceutically acceptable carrier or excipient.

[0016] In another aspect, the invention provides lorlatinib free base (Form 7), according to any of the embodiments described herein for use in the treatment of abnormal cell growth in a mammal, including a human.

[0017] In another aspect, the invention provides a pharmaceutical composition comprising lorlatinib free base (Form 7), according to any of the aspects or embodiments described herein, for use in the treatment of abnormal cell growth in a mammal.

[0018] In frequent embodiments, the abnormal cell growth is cancer. In one embodiment, the abnormal cell growth is cancer mediated by ALK or ROS1. In some such embodiments, the abnormal cell growth is cancer mediated by ALK. In other such embodiments, the abnormal cell growth is cancer mediated by ROS1. In further embodiments, the abnormal cell growth is cancer mediated by at least one genetically altered tyrosine kinase, such as a genetically altered ALK or a genetically altered ROS1 kinase.

[0019] In some such embodiments, the cancer is selected from lung cancer, bone cancer, pancreatic cancer, skin cancer, cancer of the head or neck, cutaneous or intraocular melanoma, uterine cancer, ovarian cancer, rectal cancer, cancer of the anal region, stomach cancer, colon cancer, breast cancer, carcinoma of the fallopian tubes, carcinoma of the endometrium, carcinoma of the cervix, carcinoma of the vagina, carcinoma of the vulva, Hodgkin's Disease, cancer of the esophagus, cancer of the small intestine, cancer of the endocrine system, cancer of the thyroid gland, cancer of the parathyroid gland, cancer of the adrenal gland, sarcoma of soft tissue, cancer of the urethra, cancer of the penis, prostate cancer, chronic or acute leukemia, lymphocytic lymphomas, cancer of the bladder, cancer of the kidney or ureter, renal cell carcinoma, carcinoma of the renal pelvis, neoplasms of the central nervous system (CNS), primary CNS lymphoma, spinal axis tumors, brain stem glioma, or pituitary adenoma, and combinations thereof.

[0020] In other such embodiments, the cancer is selected from the group consisting of non-small cell lung cancer (NSCLC), squamous cell carcinoma, hormone-refractory prostate cancer, papillary renal cell carcinoma, colorectal adenocarcinoma, neuroblastoma, anaplastic large cell lymphoma (ALCL) and gastric cancer. In specific embodiments, the cancer is non-small cell lung cancer (NSCLC). In particular embodiments, the cancer is NSCLC mediated by ALK or ROS1, and more particularly, NSCLC mediated by a genetically altered ALK or a genetically altered ROS1.

Brief Description of the Drawings

[0021] 

Figure 1. PXRD pattern of lorlatinib free base (Form 7).

Figure 2. FT-Raman spectrum of lorlatinib free base (Form 7).

Figure 3. Carbon CPMAS spectrum of lorlatinib free base (Form 7).

Figure 4. Fluorine MAS spectrum of lorlatinib free base (Form 7).

Figure 5. PXRD pattern of lactose tablet of lorlatinib free base (Form 7).

Figure 6. PXRD pattern of dibasic calcium phosphate (DCP) tablet of lorlatinib free base (Form 7).

Figure 7. FT-Raman spectrum of lactose tablet of lorlatinib free base (Form 7).

Figure 8. FT-Raman spectrum of DCP tablet of lorlatinib free base (Form 7).

Detailed Description of the Invention

[0022] The present invention may be understood more readily by reference to the following detailed description of the embodiments of the invention and the Examples included herein. It is to be understood that the terminology used herein is for the purpose of describing specific embodiments only and is not intended to be limiting. It is further to be understood that unless specifically defined herein, the terminology used herein is to be given its traditional meaning as known in the relevant art.

[0023] As used herein, the singular form "a", "an", and "the" include plural references unless indicated otherwise. For example, "a" substituent includes one or more substituents.

[0024] The term "about" means having a value falling within an accepted standard of error of the mean, when considered by one of ordinary skill in the art.

[0025] As used herein, the term "essentially the same" means that variability typical for a particular method is taken into account. For example, with reference to X-ray diffraction peak positions, the term "essentially the same" means that typical variability in peak position and intensity are taken into account. One skilled in the art will appreciate that the peak positions (2θ) will show some variability, typically as much as ± 0.2°. Further, one skilled in the art will appreciate that relative peak intensities will show inter-apparatus variability as well as variability due to degree of crystallinity, preferred orientation, prepared sample surface, and other factors known to those skilled in the art, and should be taken as qualitative measures only. Similarly, Raman spectrum wavenumber (cm^-1) values show variability, typically as much as ± 2 cm^-1, while ¹³C and ¹⁹F solid state NMR spectrum (ppm) show variability, typically as much as ± 0.2 ppm.

[0026] The term "crystalline" as used herein, means having a regularly repeating arrangement of molecules or external face planes. Crystalline forms may differ with respect to thermodynamic stability, physical parameters, x-ray structure and preparation processes.

[0027] The term "amorphous" refers to a disordered solid state.

[0028] The term "solvate" as used herein, means having on a surface, in a lattice or on a surface and in a lattice, a stoichiometric or non-stoichiometric amount of a solvent such as water, acetic acid, methanol, etc., or mixtures thereof, bound by non-covalent intermolecular forces. The term "hydrate" may be used specifically to describe a solvate comprising water.

[0029] The term "anhydrous" as used herein, means a crystalline form containing less than about 1% (w/w) of adsorbed moisture as determined by standard methods, such as a Karl Fisher analysis.

[0030] The invention described herein may be suitably practiced in the absence of any element(s) not specifically disclosed herein. Thus, for example, in each instance herein any of the terms "comprising", "consisting essentially of", and "consisting of" may be replaced with either of the other two terms.

[0031] In one aspect, the invention provides lorlatinib free base (Form 7). As disclosed herein, Form 7 is an anhydrous, non-solvated crystalline form of lorlatinib free base having physical stability, manufacturability and mechanical properties that are favorable for use in pharmaceutical formulations. The methods described herein provide lorlatinib free base (Form 7) which is substantially pure and free of alternative forms, including the solvated forms disclosed previously.

[0032] As described herein, Form 7 was characterized by PXRD, Raman spectroscopy, and ¹³C and ¹⁹F solid state NMR spectroscopy. Such crystalline forms may be further characterized by additional techniques, such as Fourier-Transform InfraRed Spectroscopy (FTIR), Differential Scanning Calorimetry (DSC), Thermogravimetric Analysis (TGA) or Differential Thermal Analysis (DTA).

[0033] In some embodiments of each of the aspects of the invention, lorlatinib free base (Form 7) is characterized by its powder X-ray diffraction (PXRD) pattern. In other embodiments of each of the aspects of the invention, lorlatinib free base (Form 7) is characterized by its Raman spectrum. In other embodiments of each of the aspects of the invention, lorlatinib free base (Form 7) is characterized by its ¹³C solid state NMR spectrum. In still other embodiments of each of the aspects of the invention, lorlatinib free base (Form 7) is characterized by its ¹⁹F solid state NMR spectrum.

[0034] In further embodiments, lorlatinib free base (Form 7) is characterized by a combination of two, three or four of these methods. Exemplary combinations including two or more of the following are provided herein: powder X-ray diffraction (PXRD) pattern (2θ); Raman spectrum wavenumber values (cm^-1); ¹³C solid state NMR spectrum (ppm); or ¹⁹F solid state NMR spectrum (ppm). It will be understood that other combinations of two, three or four techniques may be used to uniquely characterize lorlatinib free base (Form 7) disclosed herein.

[0035] In one embodiment, lorlatinib free base (Form 7) has a PXRD pattern comprising two or more peaks at 2θ values selected from the group consisting of: 9.6, 10.1, 14.3, 16.2 and 17.3 °2θ ± 0.2 °2θ. In another embodiment, lorlatinib free base (Form 7) has a PXRD pattern comprising three or more peaks at 2θ values selected from the group consisting of: 9.6, 10.1, 14.3, 16.2 and 17.3 °2θ± 0.2 °2θ.

[0036] In another embodiment, Form 7 has a PXRD pattern comprising peaks at 2θ values of: 9.6, 10.1 and 16.2 °2θ ± 0.2 °2θ. In some such embodiments, Form 7 has a PXRD pattern further comprising a peak at the 2θ value of: 17.3 °2θ ± 0.2 °2θ. In other such embodiments, Form 7 has a PXRD pattern further comprising a peak at the 2θ value of: 14.3 °2θ ± 0.2 °2θ.

[0037] In another embodiment, lorlatinib free base (Form 7) has a PXRD pattern comprising peaks at 2θ values of: 9.6, 10.1, 16.2 and 17.3 °2θ ± 0.2 °2θ. In another embodiment, lorlatinib free base (Form 7) has a PXRD pattern comprising peaks at 2θ values of: 9.6, 10.1, 14.3 and 16.2 °2θ ± 0.2 °2θ. In yet another embodiment, lorlatinib free base (Form 7) has a PXRD pattern comprising peaks at 2θ values of: 9.6, 10.1, 14.3, 16.2 and 17.3 °2θ ± 0.2 °2θ. In some such embodiments, the PXRD pattern further comprises one or more additional peaks at 2θ values selected from the group consisting of the peaks in Table 1.

[0038] In specific embodiments, lorlatinib free base (Form 7) has a PXRD pattern comprising: peaks at 2θ values essentially the same as shown in Figure 1.

[0039] In one embodiment, lorlatinib free base (Form 7) has a Raman spectrum comprising two or more wavenumber (cm^-1) values selected from the group consisting of: 774, 1553, 1619, 2229 and 2240 cm^-1 ± 2 cm^-1. In another embodiment, lorlatinib free base (Form 7) has a Raman spectrum comprising three or more wavenumber (cm^-1) values selected from the group consisting of: 774, 1553, 1619, 2229 and 2240 cm^-1 ± 2 cm^-1.

[0040] In another embodiment, lorlatinib free base (Form 7) has a Raman spectrum comprising wavenumber (cm^-1) values of: 2229 and 2240 cm^-1 ± 2 cm^-1. In some such embodiments, Form 7 has a Raman spectrum further comprising the wavenumber (cm^-1) value of: 1619 cm^-1 ± 2 cm^-1. In other such embodiments, Form 7 has a Raman spectrum further comprising the wavenumber (cm^-1) value of: 1553 cm^-1 ± 2 cm^-1. In still other such embodiments, Form 7 has a Raman spectrum further comprising the wavenumber (cm^-1) value of: 774 cm^-1 ± 2 cm^-1.

[0041] In another embodiment, Form 7 has a Raman spectrum comprising wavenumber (cm^-1) values of 1619, 2229 and 2240 cm^-1 ± 2 cm^-1. In another embodiment, Form 7 has a Raman spectrum comprising wavenumber (cm^-1) values of: 1553, 2229 and 2240 cm^-1 ± 2 cm^-1. In still another embodiment, Form 7 has a Raman spectrum comprising wavenumber (cm^-1) values of: 774, 2229 and 2240 cm^-1 ± 2 cm^-1. In a further embodiment, Form 7 has a Raman spectrum comprising wavenumber (cm^-1) values of: 774, 1619, 2229 and 2240 cm^-1 ± 2 cm^-1. In another embodiment, Form 7 has a Raman spectrum comprising wavenumber (cm^-1) values of: 774, 1553, 2229 and 2240 cm^-1 ± 2 cm^-1. In yet another embodiment, Form 7 has a Raman spectrum comprising wavenumber (cm^-1) values of: 774, 1553, 1619, 2229 and 2240 cm^-1 ± 2 cm^-1.

[0042] In specific embodiments, lorlatinib free base (Form 7) has a Raman spectrum comprising=wavenumber (cm^-1) values essentially the same as shown in Figure 2.

[0043] In one embodiment, lorlatinib free base (Form 7) has a ¹³C solid state NMR spectrum comprising two or more resonance (ppm) values selected from the group consisting of: 25.8, 39.1, 112.3, 117.7 and 142.1 ppm ± 0.2 ppm. In another embodiment, lorlatinib free base (Form 7) has a ¹³C solid state NMR spectrum comprising three or more resonance (ppm) values selected from the group consisting of: 25.8, 39.1, 112.3, 117.7 and 142.1 ppm ± 0.2 ppm.

[0044] In some embodiments, Form 7 has a ¹³C solid state NMR spectrum comprising the resonance (ppm) values of: 39.1 and 142.1 ppm ± 0.2 ppm. In some such embodiments, Form 7 has a ¹³C solid state NMR spectrum further comprising the resonance (ppm) value of: 112.3 ppm ± 0.2 ppm. In other such embodiments, Form 7 has a ¹³C solid state NMR spectrum further comprising the resonance (ppm) value of: 25.8 ppm ± 0.2 ppm. In still other such embodiments, Form 7 has a ¹³C solid state NMR spectrum further comprising the resonance (ppm) value of: 117.7 ppm ± 0.2 ppm.

[0045] In another embodiment, Form 7 has a ¹³C solid state NMR spectrum comprising the resonance (ppm) values of: 39.1, 112.3 and 142.1 ppm ± 0.2 ppm. In another embodiment, Form 7 has a ¹³C solid state NMR spectrum comprising the resonance (ppm) values of: 25.8, 39.1 and 142.1 ppm ± 0.2 ppm. In another embodiment, Form 7 has a ¹³C solid state NMR spectrum comprising the resonance (ppm) values of: 39.1, 117.7 and 142.1 ppm ± 0.2 ppm. In another embodiment, Form 7 has a ¹³C solid state NMR spectrum comprising the resonance (ppm) values of: 25.8, 39.1, 112.3, 117.7 and 142.1 ppm ± 0.2 ppm.

[0046] In specific embodiments, lorlatinib free base (Form 7) has a ¹³C solid state NMR spectrum (ppm) comprising resonance (ppm) values essentially the same as shown in Figure 3.

[0047] In one embodiment, lorlatinib free base (Form 7) has a ¹⁹F solid state NMR spectrum comprising resonance (ppm) values of: -108.2 and -115.2 ppm ± 0.2 ppm.

[0048] In another embodiment, Form 7 has a ¹⁹F solid state NMR spectrum (ppm) comprising resonance (ppm) values essentially the same as shown in Figure 4.

[0049] In further embodiments, lorlatinib free base (Form 7) is characterized by a combination of the ¹⁹F solid state NMR spectrum as described herein with one, two, or three of the other embodiments described above that are not inconsistent with each other. Exemplary embodiments that may be used to uniquely characterize Form 7 of lorlatinib free base are provided below.

[0050] In one embodiment, lorlatinib free base (Form 7) has a ¹⁹F solid state NMR spectrum comprising resonance (ppm) values of: -115.2 and -108.2 ppm ± 0.2 ppm.

[0051] In another embodiment, lorlatinib free base (Form 7) additionally has a powder X-ray diffraction pattern comprising peaks at 2θ values of: 9.6, 10.1 and 16.2 °2θ ± 0.2 °2θ.

[0052] In another embodiment, lorlatinib free base (Form 7) additionally has a powder X-ray diffraction pattern comprising peaks at 2θ values of: 9.6, 10.1, 16.2 and 17.3 °2θ ± 0.2 °2θ.

[0053] In another embodiment, lorlatinib free base (Form 7) additionally has a powder X-ray diffraction pattern comprising peaks at 2θ value of: 9.6, 10.1, 16.2 14.3 and 17.3 °2θ ± 0.2 °2θ.

[0054] In a further embodiment, lorlatinib free base (Form 7) additionally has: (a) a powder X-ray diffraction pattern comprising peaks at 2θ value of: 9.6, 10.1, 16.2 °2θ ± 0.2 °2θ; and (b) a Raman spectrum comprising wavenumber (cm^-1) values of: 2229 and 2240 cm^-1 ± 2 cm^-1.

[0055] In yet another embodiment, lorlatinib free base (Form 7) additionally has: (a) a powder X-ray diffraction pattern comprising peaks at 2θ values of: 9.6, 10.1 and 16.2 °2θ ± 0.2 °2θ; and (b) a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 39.1 and 142.1 ppm ± 0.2 ppm.

[0056] In another embodiment, lorlatinib free base (Form 7) additionally has a Raman spectrum comprising wavenumber (cm^-1) values of: 2229 and 2240 cm^-1 ± 2 cm^-1.

[0057] In another embodiment, lorlatinib free base (Form 7) additionally has a Raman spectrum comprising wavenumber (cm^-1) values of: 1619, 2229 and 2240 cm^-1 ± 2 cm^-1.

[0058] In still another embodiment, lorlatinib free base (Form 7) additionally has a Raman spectrum comprising wavenumber (cm^-1) values of: 1553, 1619, 2229 and 2240 cm^-1 ± 2 cm^-1.

[0059] In yet another embodiment, lorlatinib free base (Form 7) additionally has a Raman spectrum comprising wavenumber (cm^-1) values of: 774, 1553, 1619, 2229 and 2240 cm^-1 ± 2 cm^-1.

[0060] In another embodiment, lorlatinib free base (Form 7) additionally has: (a) a Raman spectrum comprising wavenumber (cm^-1) values of: 2229 and 2240 cm^-1 ± 2 cm^-1; and (b) a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 39.1 and 142.1 ppm ± 0.2 ppm.

[0061] In another embodiment, lorlatinib free base (Form 7) additionally has a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 39.1 and 142.1 ppm ± 0.2 ppm.

[0062] In another embodiment, lorlatinib free base (Form 7) additionally has a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 39.1, 112.3 and 142.1 ppm ± 0.2 ppm.

[0063] In yet embodiment, lorlatinib free base (Form 7) additionally has a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 25.8, 39.1, 112.3 and 142.1 ppm ± 0.2 ppm.

[0064] In still another embodiment, lorlatinib free base (Form 7) additionally has a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 25.8, 39.1, 112.3, 117.7 and 142.1 ppm ± 0.2 ppm.

[0065] In another aspect, the description provides a pharmaceutical composition comprising lorlatinib free base (Form 7) characterized according to any of the embodiments described herein, and a pharmaceutically acceptable carrier or excipient.

[0066] In another aspect, the description provides a pharmaceutical composition of the invention for the treatment of abnormal cell growth in a mammal, preferably a human.

[0067] The term "therapeutically effective amount" as used herein refers to that amount of a compound being administered which will relieve to some extent one or more of the symptoms of the disorder being treated. In reference to the treatment of cancer, a therapeutically effective amount refers to that amount which has the effect of (1) reducing the size of the tumor, (2) inhibiting (that is, slowing to some extent, preferably stopping) tumor metastasis, (3) inhibiting to some extent (that is, slowing to some extent, preferably stopping) tumor growth or tumor invasiveness, and/or (4) relieving to some extent (or, preferably, eliminating) one or more signs or symptoms associated with the cancer.

[0068] As used herein, "mammal" refers to a human or animal subject. In certain preferred embodiments, the mammal is a human.

[0069] The term "treating", as used herein, unless otherwise indicated, means reversing, alleviating, inhibiting the progress of, or preventing the disorder or condition to which such term applies, or one or more symptoms of such disorder or condition. The term "treatment", as used herein, unless otherwise indicated, refers to the act of treating as "treating" is defined immediately above. The term "treating" also includes adjuvant and neo-adjuvant treatment of a subject.

[0070] "Abnormal cell growth", as used herein, unless otherwise indicated, refers to cell growth that is independent of normal regulatory mechanisms (e.g., loss of contact inhibition). Abnormal cell growth may be benign (not cancerous), or malignant (cancerous). In frequent embodiments of the methods provided herein, the abnormal cell growth is cancer.

[0071] As used herein "cancer" refers to any malignant and/or invasive growth or tumor caused by abnormal cell growth. The term "cancer" includes but is not limited to a primary cancer that originates at a specific site in the body, a metastatic cancer that has spread from the place in which it started to other parts of the body, a recurrence from the original primary cancer after remission, and a second primary cancer that is a new primary cancer in a person with a history of previous cancer of different type from latter one.

[0072] In some embodiments, the abnormal cell growth is cancer mediated by an anaplastic lymphoma kinase (ALK). In some such embodiments, the ALK is a genetically altered ALK. In other embodiments, the abnormal cell growth is cancer mediated by ROS1 kinase. In some such embodiments, the ROS1 kinase is a genetically altered ROS1 kinase. In frequent embodiments, the abnormal cell growth is cancer, in particular NSCLC. In some such embodiments, the NSCLC is mediated by ALK or ROS1. In specific embodiments, the cancer is NSCLC is mediated by genetically altered ALK or genetically altered ROS1.

[0073] Pharmaceutical compositions of the present description may, for example, be in a form suitable for oral administration as a tablet, capsule, pill, powder, sustained release formulations, solution, suspension, for parenteral injection as a sterile solution, suspension or emulsion, for topical administration as an ointment or cream or for rectal administration as a suppository. The pharmaceutical composition may be in unit dosage forms suitable for single administration of precise dosages. The pharmaceutical composition will include a conventional pharmaceutical carrier or excipient and a compound according to the invention as an active ingredient. In addition, it may include other medicinal or pharmaceutical agents, carriers, adjuvants, etc.

[0074] Exemplary parenteral administration forms include solutions or suspensions of active compounds in sterile aqueous solutions, for example, aqueous propylene glycol or dextrose solutions. Such dosage forms can be suitably buffered, if desired.

[0075] Suitable pharmaceutical carriers include inert diluents or fillers, water and various organic solvents. The pharmaceutical compositions may, if desired, contain additional ingredients such as flavorings, binders, excipients and the like. Thus for oral administration, tablets containing various excipients, such as citric acid may be employed together with various disintegrants such as starch, alginic acid and certain complex silicates and with binding agents such as sucrose, gelatin and acacia. Additionally, lubricating agents such as magnesium stearate, sodium lauryl sulfate and talc are often useful for tableting purposes. Solid compositions of a similar type may also be employed in soft and hard filled gelatin capsules. Preferred materials include lactose or milk sugar and high molecular weight polyethylene glycols. When aqueous suspensions or elixirs are desired for oral administration the active compound therein may be combined with various sweetening or flavoring agents, coloring matters or dyes and, if desired, emulsifying agents or suspending agents, together with diluents such as water, ethanol, propylene glycol, glycerin, or combinations thereof.

[0076] Methods of preparing various pharmaceutical compositions with a specific amount of active compound are known, or will be apparent, to those skilled in this art. For examples, see Remington's Pharmaceutical Sciences, Mack Publishing Company, Easter, Pa., 15th Edition (1975).

Examples

[0077] The examples and preparations provided below further illustrate and exemplify particular aspects and embodiments of the invention.

General Method 1. Powder X-ray Diffraction (PXRD)

[0078] The PXRD data in Figure 1 were collected according to the following general protocol.

Instrument Method:

[0079] PXRD patterns were collected on a Bruker-AXS Ltd. D4 powder X-ray diffractometer fitted with an automatic sample changer, a theta-theta goniometer, automatic beam divergence slit, and a PSD Vantec-1 detector. The X-ray tube voltage and amperage were set to 40 kV and 40 mA respectively. The diffractometer was aligned and a calibration check performed using a corundum reference material on the day of data collection. Data was collected at the Cu wavelength using a step size of 0.018 degrees and scan time of 11.3 hours scanning from 2.0 to 65.0 degrees 2-theta. The sample powders were prepared by placing the powder in a slightly greased low background holder. The sample powder was pressed by a glass slide to ensure that a proper sample height was achieved and rotated during collection. Data were collected using Bruker DIFFRAC software and analysis was performed by DIFFRAC EVA software (Version 3.1).

[0080] The PXRD patterns collected were imported into Bruker DIFFRAC EVA software. The measured PXRD pattern for Form 7 of the active pharmaceutical ingredient (API) was aligned with the simulated pattern from single crystal data prior to selecting the peak positions. A peak search was performed using the Bruker software. The peak selection was carefully checked to ensure that all peaks had been captured and all peak positions had been accurately assigned.

Peak picking method:

[0081] Peak picking was achieved using the peak search algorithm in the EVA software (Version 3.1). A threshold value of 1 and a width value of 0.27 (max 0.55, minimum 0.02) were used to make preliminary peak assignments. The output of automated assignments was visually checked to ensure validity and adjustments were manually made if necessary. Peak intensities were normalized relative to highest intensity peak equaling 100%. Peaks with relative intensity of ≥ 2% were generally chosen. A typical error of ± 0.2° 2-theta in peak position applies to this data. The minor error associated with this measurement can occur as a result of a variety of factors including: (a) sample preparation (e.g., sample height), (b) instrument, (c) calibration, (d) operator (including those errors present when determining the peak locations), and (e) the nature of the material (e.g. preferred orientation and transparency errors). Therefore peaks are considered to have a typical associated error of ± 0.2° 2-theta. When two peaks, in the list, are considered to overlap (± 0.2° 2-theta) the less intense peak has been removed from the listing. Peaks existing as shoulders, on a higher intensity adjacent peak, have also been removed from the peak list.

[0082] Ideally the powder pattern should be aligned against a reference. This could either be the simulated powder pattern from the crystal structure of the same form, or an internal standard e.g. silica. The measured PXRD pattern for Form 7 of the API used to generate the peak listing in Table 1 was aligned to the simulated pattern from the single crystal structure.

General Method 2. Raman Spectroscopy

[0083] The Raman spectral data in Figure 2 were collected according to the following general protocol.

Instrument Method:

[0084] Raman spectra were collected using a RAM II FT Raman module attached to a Vertex 70 FTIR spectrometer (Bruker, UK). The instrument is equipped with a 1064 nm Nd:YAG laser and a liquid nitrogen cooled germanium detector. Prior to data acquisition, instrument performance and calibration verifications were conducted using a white light source, and polystyrene and naphthalene references.

[0085] Samples were analyzed in truncated NMR tubes (5 mm diameter) that were spun during spectral collection. The backscattered Raman signal from the sample in the rotator was optimized and spectra from each sample were acquired using the following parameters:

Laser power:	500 mW
Spectral resolution:	2 cm-1
Collection range:	4000 - 50 cm-1
Number of scans:	512
Apodization function:	Blackmann-Harris 4-term

[0086] The variability in the peak positions in this experimental configuration is within ± 2 cm^-1.

Peak picking method

[0087] Prior to peak picking the intensity scale of the Stokes scattered Raman signal was normalized to 1.00. Peaks positions were then identified using the peak picking functionality in the GRAMS/AI v.9.1 software (Thermo Fisher Scientific) with the threshold set to 0.007.

[0088] Peaks with relative intensities between 1.00 and 0.75, 0.74 and 0.30, and below 0.29 were labelled as strong, medium and weak respectively.
It is expected that, since FT-Raman and dispersive Raman are similar techniques, peak positions reported herein for FT-Raman spectra would be consistent with those which would be observed using a dispersive Raman measurement, assuming appropriate instrument calibration.

General Method 3. Solid state NMR (ssNMR) Spectroscopy:

[0089] The carbon CPMAS and fluorine MAS ssNMR data in Figures 3 and 4 were collected according to the following general protocol.

Instrument Method:

[0090] Solid state NMR (ssNMR) analysis was conducted at ambient temperature and pressure on a Bruker-BioSpin CPMAS probe positioned into a Bruker-BioSpin Avance III 500 MHz (¹H frequency) NMR spectrometer. The packed rotor was oriented at the magic angle and spun at 14.5 kHz. The carbon ssNMR spectrum was collected using a proton decoupled cross-polarization magic angle spinning experiment. A phase modulated proton decoupling field of 80-90 kHz was applied during spectral acquisition. The cross-polarization contact time was set to 2 ms and the recycle delay to 5 seconds. The number of scans was adjusted to obtain an adequate signal to noise ratio. The carbon spectrum was referenced using an external standard of crystalline adamantane, setting its upfield resonance to 29.5 ppm (as determined from neat TMS). The fluorine ssNMR spectrum was collected using a proton decoupled direct polarization magic angle spinning experiment. A phase modulated proton decoupling field of 80-90 kHz was applied during spectral acquisition. The recycle delay was set to 60 seconds. The number of scans was adjusted to obtain an adequate signal to noise ratio. The fluorine chemical shift scale was referenced using a direct polarization experiment on an external standard of 50/50 volume/volume of trifluoroacetic acid and water, setting its resonances to -76.54 ppm.

Peak picking method:

[0091] Automatic peak picking was performed using Bruker-BioSpin TopSpin version 3.2 software. Generally, a threshold value of 5% relative intensity was used to preliminary select peaks. The output of the automated peak picking was visually checked to ensure validity and adjustments were manually made if necessary.

[0092] Although specific ¹³C and ¹⁹F solid state NMR peak values are reported herein there does exist a range for these peak values due to differences in instruments, samples, and sample preparation. This is common practice in the art of solid state NMR because of the variation inherent in peak values. A typical variability for a ¹³C and ¹⁹F chemical shift x-axis value is on the order of plus or minus 0.2 ppm for a crystalline solid. The solid state NMR peak heights reported herein are relative intensities. The solid state NMR intensities can vary depending on the actual setup of the experimental parameters and the thermal history of the sample.

Example 1

Lab Scale Preparation of Form 7 of (10R)-7-amino-12-fluoro-2,10,16-trimethyl-15-oxo-10,15,16,17-tetrahydro-2H-8,4-(metheno)pyrazolo[4,3-h][2,5,11]benzoxadiazacyclotetradecine-3-carbonitrile (lorlatinib) Free Base

[0093] 

[0094] Form 7 of lorlatinib free base was prepared by de-solvation of the acetic acid solvate of lorlatinib (Form 3), prepared as described in International Patent Publication No. WO 2014/207606, via an intermediate methanol solvate hydrate form of lorlatinib (Form 2).

[0095] The acetic acid solvate of lorlatinib (Form 3) (5 g, 10.72 mmol) was slurried in methanol (10 mL/g, 1235.9 mmol) at room temperature in an Easymax flask with magnetic stirring to which triethylamine (1.2 equiv., 12.86 mmol) was added over 10 minutes. The resulting solution was heated to 60°C and water (12.5 mL/g, 3469.3 mmol) was added over 10 minutes, while maintaining a temperature of 60°C. Crystallization was initiated by scratching the inside of the glass vessel to form a rapidly precipitating suspension which was triturated to make the system mobile. The suspension was then cooled to 25°C over 1 hour, then cooled to 5°C and granulated for 4 hours. The white slurry was filtered and washed with 1 mL/g chilled water/methanol (1:1) then dried under vacuum at 50°C overnight to provide the methanol solvate hydrate Form 2 of lorlatinib.

[0096] Form 7 was then prepared via a re-slurry of the methanol solvate hydrate Form 2 of lorlatinib in heptane. 100 mg of lorlatinib Form 2 was weighed into a 4-dram vial and 3 mL of heptane was added. The mixture was slurried at room temperature on a roller mixer for 2 hours. Form conversion was confirmed by PXRD revealing complete form change to Form 7 of lorlatinib free base.

Example 2

Alternative Preparation of Form 7 of (10R)-7-amino-12-fluoro-2,10,16-trimethyl-15-oxo-10,15,16,17-tetrahydro-2H-8,4-(metheno)pyrazolo[4,3-h][2,5,11]benzoxadiazacyclotetradecine-3-carbonitrile (lorlatinib) Free Base

[0097] 

[0098] Into a 100 mL Easymax reactor equipped with an overhead stirrer, was added the bis-Boc protected macrocycle 1 (prepared as described in International Patent Publication No. WO 2014/207606 at Example 4) (7g, 10 mmol) and methanol (28 mL; 4 mL/g of PF-06668559). The slurry was heated to 60°C and treated with 6N hydrochloric acid (9 mL, 54 mmol) and held for 3 hours. Once reaction was determined complete, the mixture was cooled to 40°C and treated with 1N sodium hydroxide (39mL, 39 mmol) to partially neutralize the mixture. The mixture was treated with 2-methyltetrahydrofuran (53 mL), followed by neutralization to pH 7 with 1 N sodium hydroxide (13.5 mL, 13.5 mmol). The mixture was treated with sodium chloride (10.1 g, 173 mmol) and warmed to 60°C. The bottom aqueous layer was removed using a separatory funnel. The organic phase was washed with water (50 mL) at 60°C. The water wash was removed by separatory funnel. The organic layer was speck free filtered into a clean 125 mL reactor fitted with overhead agitator and distillation head. Additional 2-methyltetrahydrofuran (70mL) was added to the organic mixture and the mixture was concentrated by atmospheric distillation to a volume of approximately 30 mL. The solution was treated with 2-methyltetrahydrofuran (12 mL) and adjusted to 60°C.

[0099] The solution was treated with n-heptane (10.5 mL), followed by seeding with Form 7 of lorlatinib free base (45 mg, 0.11mmol). After aging the slurry for 1 hour, n heptane (73.5 mL) was added over 2 hours at 60°C. The resultant slurry was held for 1 hour at 60°C followed by cooling to 20°C over 1 hour and granulated for 16 hours. The slurry was filtered, and the product cake was washed with n heptane (12 mL). The solids were dried in the oven at 60°C for 12 hours to give Form 7 of PF-0463922 free base (8.24 mmol, 3.36 g) as a white solid in 82% yield with >98% purity.

Characterization of Lorlatinib Free Base (Form 7)

PXRD Data

[0100] Figure 1 shows PXRD data for lorlatinib free base (Form 7), collected according to General Method 1. A list of PXRD peaks at diffraction angles 2-Theta ° (°2θ) ± 0.2 °2θ and their relative intensities is provided in Table 1. Characteristic PXRD peaks distinguishing Form 7 are indicated by an asterisk (*).

Table 1: PXRD Peak List for Form 7 (2-Theta °)

Angle °2θ ± 0.2 °2θ	Intensity %
7.5	2.6
9.6*	12.9
10.1*	13.0
11.0	1.3
11.8	6.0
12.6*	19.9
14.3*	22.1
15.0	13.9
16.2*	100.0
17.3*	72.1
18.3	14.0
19.3*	31.4
19.9	20.3
20.3	7.6
21.2	60.7
22.1	3.2
22.5	13.7
23.3	25.2
24.0	17.2
24.6	9.8

FT-Raman Data

[0101] Figure 2 shows the FT-Raman spectrum of lorlatinib free base (Form 7), collected according to General Method 2. A list of FT-Raman peaks (cm^-1) and qualitative intensities is provided in Table 2 in cm^-1 ± 2 cm^-1. Characteristic FT-Raman peaks (cm^-1) peaks distinguishing Form 7 are indicated by an asterisk (*). Normalized peak intensities are indicated as follows: W= weak; M= medium; S= strong.

Table 2: FT Raman Peak List for Form 7 (cm^-1)

Wave number cm-1 ± 2 cm-1	Normalized peak intensity
3064	w
3012	w
2983	w
2937	w
2917	w
2871	w
2240*	m
2229*	m
1645	w
1619*	s
1572	w
1553*	s
1440	m
1422	m
1396	w
1367	w
1347	w
1335	w
1315	m
1301	w
1260	w
1232	w
1220	w
1203	w
1155	w
1143	w
1085	w
1068	w
1035	w
972	w
949	w
937	w
908	w
903	w
889	w
862	w
807	w
774*	w
733	w
702	w
693	w
663	w
641	w
633	w
623	w
601	w
590	w
570	w
559	w
492	w
472	w
460	w
442	w
426	w
383	w
321	w
287	w
263	w
256	w
234	w

ssNMR data

[0102] Figure 3 shows the carbon CPMAS spectrum of lorlatinib free base (Form 7), which was collected according to General Method 3. Chemical shifts are expressed in parts per million (ppm) and are referenced to external sample of solid phase adamantane at 29.5 ppm. A list of ssNMR ¹³C chemical shifts (ppm) for Form 7 is provided in Table 3 in ppm ± 0.2 ppm. Characteristic ssNMR ¹³C chemical shifts (ppm) distinguishing Form 7 are indicated by an asterisk (*).

Table 3: ssNMR ¹³C Chemical Shifts for Form 7 (ppm)

13C Chemical Shifts [ppm ± 0.2 ppm]	Intensity
21.6	88
25.8*	85
27.3	68
34.7	70
38.2	73
39.1*	77
46.7	51
48.2	50
71.3	68
73.2	68
110.9	12
112.3*	75
114.1	78
114.5	64
116.3	37
117.7*	84
120.1	51
125.5	33
127.6	76
129.8	48
131.8	60
132.1	62
134.1	42
137.2	33
139.5	62
139.9	68
142.1*	100
143.8	55
144.9	50
150.8	39
151.8	38
162.8	27
163.8	29
164.9	17
165.9	16
168.1	37
170.3	41

[0103] Figure 4 shows the fluorine MAS (ssNMR) spectrum of lorlatinib free base (Form 7), collected according to General Method 3. Chemical shifts are expressed in parts per million (ppm) referenced to an external sample of trifluoroacetic acid (50% V/V in H₂O) at - 76.54 ppm.

[0104] The ssNMR ¹⁹F chemical shift (ppm) for Form 7 is provided in Table 4 in ppm ± 0.2 ppm. The characteristic ssNMR ¹⁹F chemical shifts (ppm) distinguishing Form 7 are indicated by an asterisk (*).

Table 4: ssNMR ¹⁹F Chemical Shifts for Form 7 (ppm)

19F Chemical Shifts [ppm ± 0.2 ppm]	Intensity
-115.2*	100
-108.2*	76

Reference Example 3

Representative Drug Product Formulations of Lorlatinib Free Base (Form 7)

[0105] Immediate release (IR) tablets comprising lorlatinib free base (Form 7) may be prepared using conventional excipients commonly used in tableted formulations.

[0106] Tablets typically contain from 1-30% of lorlatinib on a w/w basis. Microcrystalline cellulose, dibasic calcium phosphate anhydrous (DCP) and lactose monohydrate may be used as tablet fillers, and sodium starch glycolate may be used as a disintegrant. Magnesium stearate may be used as a lubricant.

[0107] A typical IR tablet formulation of Form 7 containing Dibasic Calcium Phosphate Anhydrous (DCP) as a tablet filler (DCP tablet) is provided in Table 5.

Table 5. Typical Composition of IR Tablet using Dibasic Calcium Phosphate Anhydrous (DCP) as a tablet filler

		% composition
Form 7	Active Ingredient	1-30
Microcrystalline Cellulose	Filler	35-60
Dibasic Calcium Phosphate Anhydrous	Filler	10-35
Sodium Starch Glycolate	Disintegrant	2-5
Magnesium Stearate	Lubricant	0.5-1.5
Total Tablet Weight		100.0

[0108] A typical IR tablet formulation of Form 7 containing lactose as a tablet filler (lactose tablet) is provided in Table 6.

Table 6. Typical Composition of IR Tablet using lactose as a tablet filler

		% composition
Form 7	Active Ingredient	1-30
Microcrystalline Cellulose	Filler	35-60
Lactose monohydrate	Filler	10-35
Sodium Starch Glycolate	Disintegrant	2-5
Magnesium Stearate	Lubricant	0.5-1.5
Total Tablet Weight		100.0

[0109] IR tablets of lorlatinib free base (Form 7) may be manufactured using a dry granulation process prior to compression. In this process the crystalline material is blended with some proportion of the excipients falling within the ranges outline above and the blend is dry granulated using a roller compactor. The granule is milled as part of this process. The granules are blended with remainder of any of the excipients (e.g., magnesium stearate) prior to compression.

[0110] Figures 5 and 6 show the PXRD patterns of a prototype lactose tablet and DCP tablet, respectively, comprising 10% w/w of lorlatinib free base (Form 7). Figures 7 and 8 show the FT-Raman spectrum of a prototype lactose tablet and DCP tablet, respectively, comprising 10% w/w of lorlatinib free base (Form 7).

Example 4

Thermodynamic Stability of Lorlatinib Free Base (Form 7)

[0111] The thermodynamic stability of anhydrous lorlatinib free base (Form 7) was evaluated employing slurry experiments under a range of water activity and temperature conditions. Suspensions of Form 7 were equilibrated for two weeks in diverse solvent systems at three different temperatures: 5°C, room temperature and 40°C and water activities 0.25 to 1.00. After 2 weeks, the solids in equilibrium were isolated and the solid form was evaluated by PXRD.

[0112] The results summarized in Table 7 demonstrate that anhydrous Form 7 API could form solvated forms in several solvent systems and a hydrate in pure water, but does not convert to a different anhydrous solid state under the conditions explored.

Table 7. Slurry Output for anhydrous lorlatinib Form 7. Form 5, 13, 16 and 20 are solvated forms of the lorlatinib free base and Form 18 is a hydrate.

Solvent	Water activity	5°C	RT	40°C
nBuOH	0	Form 7	Form 20	Form 7
iProAc	0	Form 7	Form 7	Form 7
MiBK	0	Form 7	Form 7	Form 7
TBME	0	Form 7	Form 7	Form 7
Toluene	0	Form 7	Form 7	Form 7
IPA	0.25	Form 16	Form 7	Form 7
IPA	0.50	Form 13	Form 13	Form 5
IPA	0.70	Form 13	Form 13	Form 5
IPA	0.90	Form 13	Form 13	Form 13
Water	1.00	Form 7+Form 18	Form 18	Form 7

Example 5

Solid-state Physical Stability of anhydrous lorlatinib free base (Form 7) and Drug Product

[0113] The physical stability of anhydrous lorlatinib free base (Form 7) API was investigated at elevated relative humidities (%RH) for extended time period and at accelerated stability conditions for shorter period. Form 7 stored at ambient temperature and humidity levels of 75%RH and 90%RH for 12 months and at 70°C/75%RH and 80°C/75%RH for 1 week did not undergo any physical change. Results are shown in Table 8.

Table 8. Long term stability of Form 7 API

Conditions	Time	Solid Form
75%RH, ambient temperature	12 months	Form 7
90%RH, ambient temperature	12 months	Form 7
70°C/75%RH	1 week	Form 7
80°C/40%RH	1 week	Form 7

[0114] A representative drug product formulation of Form 7 demonstrated superior physical stability relative to the acetic acid solvate of lorlatinib free base disclosed in WO 2014/207606.

[0115] The physical stabilities of lorlatinib Form 7 and acetic acid solvate in the drug product were investigated under a variety of conditions using FT-Raman and Solid State NMR spectroscopy. Results are summarized in Table 9.

Table 9. Physical stability of Form 7 drug product vs. acetic acid solvate comparing amount of physical impurity

Conditions	Time	lorlatinib acetic acid solvate	lorlatinib free base Form 7
70°C/75%RH	1 week	impurity >50%	No change detected
50°C/75%RH	2 weeks	>10% impurity<50%	No change detected
70°C/40%RH	2 weeks	impurity >50%	No change detected
70°C/10%RH	3 weeks	impurity >50%	No change detected
25°C/60%RH	12 months	>10% impurity<50%	No change detected
30°C/65%RH	12 months	>10% impurity<50%	No change detected

Table 10. Summary of physical stability studies for Lorlatinib Free Base Form 7 for several drug product formulations

Conditions	Excipients	Time	Output Solid Form
50°C/75%RH	tablet with lactose, magnesium stearate, Polyplasdone XL	2 weeks	Form 7
50°C/75%RH	tablet with DCP, stearic acid, Explotab	2 weeks	Form 7
50°C/75%RH	tablet with mannitol, magnesium stearate, Explotab	2 weeks	Form 7
50°C/75%RH	tablet with DCP, stearic acid, Polyplasdone XL	2 weeks	Form 7
50°C/75%RH	tablet with lactose, stearic acid, Explotab	2 weeks	Form 7
50°C/75%RH	tablet with DCP, magnesium stearate, Polyplasdone XL	2 weeks	Form 7
50°C/75%RH	tablet with mannitol, stearic acid, Polyplasdone XL	2 weeks	Form 7
50°C/75%RH	tablet with DCP, magnesium stearate, Explotab	2 weeks	Form 7

Reference Example 6

Representative Tablet Formulations

[0116] Immediate release, film coated tablets were prepared in 25 mg, 50 mg and 100 mg immediate dosages using a dry granulation manufacturing process. The compositions of the tablets are provided in Table 11.

Table 11. Compositions of IR tablets of three different strengths

Component	Component Role	25 mg tablet (mg/tablet)	50 mg tablet (mg/tablet)	100 mg tablet (mg/tablet)
lorlatinib free base (Form 7)	Active ingredient	25.000	50.000	100.00
Microcrystalline Cellulose	Filler	143.325	286.650	355.540
Dibasic Calcium Phosphate Anhydrous	Filler	71.675	143.350	177.800
Sodium Starch Glycolate	Disintegrant	7.500	15.000	20.000
Magnesium Stearate	Lubricant	2.500	5.000	13.330
Tablet core weight		250.00	500.00	666.670
Opadry II Tan or Lavender	Coating agent	7.500	15.000	20.000
Sterile water for irrigation*		(42.500)	(85.000)	(113.330)
Total weight (mg)		257.500	515.000	686.670

*removed during processing. Does not appear in final product

Example 7

Chemical Stability of Representative Tablet Formulation

[0117] Chemical stability data was generated at 25°C/60%RH and 30°C/75%RH for 12 months and at 40°C/75%RH for 6 months for the 25 mg tablets prepared according to Example 6. Three main degradation products (amide, formaldehyde dimer and oxidative photodegradant) were monitored to assess the chemical stability of the test formulation. The chemical stability data for these chemical impurities is provided in Table 12.

Table 12. Summary of chemical stability data for 25 mg IR film coated tablet of lorlatinib Form 7

Impurity	12 months	12 months	6 months
	25°C/60%RH	30°C/75%RH	40°C/75%RH
amide	NMT 0.05	0.08	0.15
dimer	0.09	0.16	0.19
photodegradant	NMT 0.05	NMT 0.05	NMT 0.05

Claims

1. An anhydrous, non-solvated crystalline form of (10R)-7-amino-12-fluoro-2,10,16-trimethyl-15-oxo-10,15,16,17-tetrahydro-2H-8,4-(metheno)pyrazolo[4,3-h][2,5,11] benzoxadiazacyclotetradecine-3-carbonitrile (lorlatinib) free base, having a ¹⁹F solid state NMR spectrum comprising resonance (ppm) values of: -108.2 and -115.2 ppm ± 0.2 ppm, relative to an external standard of 50/50 volume/volume of trifluoroacetic acid and water, setting its resonances to -76.54 ppm.

2. The crystalline form of claim 1, having a powder X-ray diffraction (PXRD) pattern measured using copper wavelength radiation comprising two or more peaks at 2θ values selected from the group consisting of: 9.6, 10.1, 14.3, 16.2 and 17.3 °2θ ± 0.2 °2θ.

3. The crystalline form of claim 2, having a PXRD pattern comprising peaks at 2θ value of: 9.6, 10.1 and 16.2 °2θ ± 0.2 °2θ.

4. The crystalline form of claim 3, having a PXRD pattern further comprising a peak at the 2θ value of: 17.3 °2θ ± 0.2 °2θ.

5. The crystalline form of claim 3 or 4, having a PXRD pattern further comprising a peak at the 2θ value of: 14.3 °2θ ± 0.2 °2θ.

6. The crystalline form of any one of claims 2 to 5, having a Raman spectrum comprising wavenumber (cm^-1) values of: 2229 and 2240 cm^-1 ± 2 cm^-1.

7. The crystalline form of any one of claims 2 to 6, having a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 39.1 and 142.1 ppm ± 0.2 ppm, relative to an external standard of crystalline adamantane, setting its upfield resonance to 29.5 ppm.

8. A crystalline form of lorlatinib free base as claimed in claim 1 having a Raman spectrum comprising two or more wavenumber (cm^-1) values selected from the group consisting of: 774, 1553, 1619, 2229 and 2240 cm^-1 ± 2 cm^-1.

9. The crystalline form of claim 8, having a Raman spectrum comprising the wavenumber (cm^-1) value of: 2229 and 2240 cm^-1 ± 2 cm^-1.

10. The crystalline form of claim 9, having a Raman spectrum further comprising the wavenumber (cm^-1) value of: 1619 cm^-1 ± 2 cm^-1.

11. The crystalline form of claim 9 or 10, having a Raman spectrum further comprising the wavenumber (cm^-1) value of: 1553 cm^-1 ± 2 cm^-1.

12. The crystalline form of claim 9, 10 or 11, having a Raman spectrum further comprising the wavenumber (cm^-1) value of: 774 cm^-1 ± 2 cm^-1.

13. The crystalline form of any one of claims 8 to 12, having a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 39.1 and 142.1 ppm ± 0.2 ppm, relative to an external standard of crystalline adamantane, setting its upfield resonance to 29.5 ppm.

14. A crystalline form of lorlatinib free base as claimed in claim 1 having a ¹³C solid state NMR spectrum comprising two or more resonance (ppm) values selected from the group consisting of: 25.8, 39.1, 112.3, 117.7 and 142.1 ppm ± 0.2 ppm, relative to an external standard of crystalline adamantane, setting its upfield resonance to 29.5 ppm.

15. The crystalline form of claim 14, having a ¹³C solid state NMR spectrum comprising resonance (ppm) values of: 39.1 and 142.1 ppm ± 0.2 ppm.

16. The crystalline form of claim 15, having a ¹³C solid state NMR spectrum further comprising the resonance (ppm) value of: 112.3 ppm ± 0.2 ppm.

17. The crystalline form of claim 15 or 16, having a ¹³C solid state NMR spectrum further comprising the resonance (ppm) value of: 25.8 ppm ± 0.2 ppm.

18. The crystalline form of claim 15, 16 or 17, having a ¹³C solid state NMR spectrum further comprising the resonance (ppm) value of: 117.7 ppm ± 0.2 ppm.

19. A crystalline form of lorlatinib free base according to any one of claims 1 to 18 for use in the treatment of abnormal cell growth in a mammal.

20. The lorlatinib free base for use of claim 19, wherein the abnormal cell growth is cancer.

21. The lorlatinib free base for use of claim 20, wherein the cancer is mediated by anaplastic lymphoma kinase (ALK) or c-ros oncogene 1 receptor tyrosine kinase (ROS1).

22. The lorlatinib free base for use of claim 20 or 21, wherein the cancer is non-small cell lung cancer (NSCLC).

Ansprüche

1. Wasserfreie, nicht-solvatisierte, kristalline Form der freien Base von (10R)-7-Amino-12-fluor-2,10,16-trimethyl-15-oxo-10,15,16,17-tetrahydro-2H-8,4-(metheno)pyrazolo[4,3-h][2,5,11]benzoxadiazacyclotetradecin-3-carbonitril (Lorlatinib) mit einem ¹⁹F-Festphasen-NMR-Spektrum, umfassend Resonanzwerte (ppm): -108,2 und -115,2 ppm ± 0,2 ppm, in Bezug auf einen externen Standard von 50/50 V/V von Trifluoressigsäure und Wasser, der seine Resonanzen auf -76,54 ppm festlegt.

2. Kristalline Form gemäß Anspruch 1 mit einem Pulver-Röntgenbeugungs (PXRD)-Muster, gemessen unter Verwendung von Kupfer-Wellenlängenstrahlung mit zwei oder mehr Peaks bei 2θ-Werten, ausgewählt aus der Gruppe, bestehend aus 9,6, 10,1, 14,3, 16,2 und 17,3 °2θ ± 0,2 °2θ.

3. Kristalline Form gemäß Anspruch 2 mit einem PXRD-Muster, umfassend Peaks bei 2θ-Werten: 9,6, 10,1 und 16,2 °2θ ± 0,2 °2θ.

4. Kristalline Form gemäß Anspruch 3 mit einem PXRD-Muster, umfassend einen Peak bei dem 2θ-Wert: 17,3 °2θ ± 0,2 °2θ.

5. Kristalline Form gemäß Anspruch 3 oder 4 mit einem PXRD-Muster, umfassend einen Peak bei dem 2θ-Wert: 14,3 °2θ ± 0,2 °2θ.

6. Kristalline Form gemäß einem der Ansprüche 2 bis 5 mit einem Raman-Spektrum, umfassend Wellenzahlenwert (cm^-1) : 2229 und 2240 cm^-1 ± 2 cm^-1.

7. Kristalline Form gemäß einem der Ansprüche 2 bis 6 mit einem ¹³C-Festphasen-NMR-Spektrum, umfassend Resonanzwerte (ppm) : 39, 1 und 142,1 ppm ± 0,2 ppm, in Bezug auf einen externen Standard von kristallinem Adamantan, der die Hochfeldresonanz auf 29,5 ppm festlegt.

8. Kristalline Form der freien Base von Lorlatinib gemäß Anspruch 1 mit einem Raman-Spektrum, umfassend zwei oder mehr Wellenzahlenwerte (cm^-1), ausgewählt aus der Gruppe, bestehend aus: 774, 1553, 1619, 2229 und 2240 cm^-1 ± 2 cm^-1.

9. Kristalline Form gemäß Anspruch 8 mit einem Raman-Spektrum, umfassend die Wellenzahlenwerte (cm^-1) : 2229 und 2240 cm^-1 ± 2 cm^-1.

10. Kristalline Form gemäß Anspruch 9 mit einem Raman-Spektrum, des Weiteren umfassend den Wellenzahlenwert (cm^-1): 1619 cm^-1 ± 2 cm^-1.

11. Kristalline Form gemäß Anspruch 9 oder 10 mit einem Raman-Spektrum, des Weiteren umfassend den Wellenzahlenwert (cm^-1): 1553 cm^-1 ± 2 cm^-1.

12. Kristalline Form gemäß Anspruch 9, 10 oder 11 mit einem Raman-Spektrum, des Weiteren umfassend den Wellenzahlenwerte (cm^-1) : 774 cm^-1 ± 2 cm^-1.

13. Kristalline Form gemäß einem der Ansprüche 8 bis 12 mit einem ¹³C-Festphasen-NMR-Spektrum, umfassend Resonanzwerte (ppm) : 39, 1 und 142,1 ppm ± 0,2 ppm, in Bezug auf einen externen Standard von kristallinem Adamantan, der die Hochfeldresonanz auf 29,5 ppm festlegt.

14. Kristalline Form der freien Base von Lorlatinib gemäß Anspruch 1 mit einem ¹³C-Festphasen-NMR-Spektrum, umfassend zwei oder mehr Resonanzwerte (ppm), ausgewählt aus der Gruppe, bestehend aus: 25,8, 39,1, 112,3, 117,7 und 142,1 ppm ± 0,2 ppm, bezogen auf einen externen Standard von kristallinem Adamantan, der die Hochfeldresonanz auf 29,5 ppm festlegt.

15. Kristalline Form gemäß Anspruch 14 mit einem ¹³C-Festphasen-NMR-Spektrum, umfassend Resonanzwerte (ppm): 39,1 und 142,1 ppm ± 0,2 ppm.

16. Kristalline Form gemäß Anspruch 15 mit einem ¹³C-Festphasen-NMR-Spektrum, umfassend den Resonanzwert (ppm): 112,3 ppm ± 0,2 ppm.

17. Kristalline Form gemäß Anspruch 15 oder 16 mit einem ¹³C-Festphasen-NMR-Spektrum, umfassend den Resonanzwert (ppm): 25,8 ppm ± 0,2 ppm.

18. Kristalline Form gemäß Anspruch 15, 16 oder 17 mit einem ¹³C-Festphasen-NMR-Spektrum, umfassend den Resonanzwert (ppm): 117,7 ppm ± 0,2 ppm.

19. Kristalline Form der freien Base von Lorlatinib gemäß einem der Ansprüche 1 bis 18 zur Verwendung in der Behandlung von abnormalem Zellwachstum in einem Säuger.

20. Freie Base von Lorlatinib zur Verwendung gemäß Anspruch 19, wobei das abnormale Zellwachstum Krebserkrankung ist.

21. Freie Base von Lorlatinib zur Verwendung gemäß Anspruch 20, wobei die Krebserkrankung durch anaplastischer Lymphomkinase (ALK) oder c-ros-Onkogen-1-Rezeptortyrosinkinase (ROS1) vermittelt ist.

22. Freie Base von Lorlatinib zur Verwendung gemäß Anspruch 20 oder 21, wobei die Krebserkrankung nichtkleinzelliges Lungenkarzinom (NSCLC) ist.

Revendications

1. Forme cristalline non solvatée anhydre de base libre de (10R)-7-amino-12-fluoro-2,10,16-triméthyl-15-oxo-10,15,16,17-tétrahydro-2H-8,4-(méthéno)pyrazolo[4,3-h] [2,5,11] benzoxadiazacyclotétradécine-3-carbonitrile (lorlatinib), ayant un spectre RMN à l'état solide de ¹⁹F comprenant des valeurs de résonance (en ppm) de : -108,2 et -115,2 ppm ± 0,2 ppm, par rapport à un étalon externe de 50/50 volume/volume d'acide trifluoroacétique et d'eau, établissant ses résonances à -76,54 ppm.

2. Forme cristalline selon la revendication 1, ayant un profil de diffraction aux rayons X sur poudre (PXRD) mesuré à l'aide d'un rayonnement de longueur d'onde du cuivre comprenant deux pics ou plus à des valeurs 2θ sélectionnées dans le groupe constitué par : 9,6, 10,1, 14,3, 16,2 et 17,3 °2θ ± 0,2 °2θ.

3. Forme cristalline selon la revendication 2, ayant un profil PXRD comprenant des pics à la valeur 2θ de : 9,6, 10,1 et 16,2 °2θ ± 0,2 °2θ.

4. Forme cristalline selon la revendication 3, ayant un profil PXRD comprenant en outre un pic à la valeur 2θ de : 17,3 °2θ ± 0,2 °2θ.

5. Forme cristalline selon la revendication 3 ou 4, ayant un profil PXRD comprenant en outre un pic à la valeur 2θ de : 14,3 °2θ ± 0,2 °2θ

6. Forme cristalline selon l'une des revendications 2 à 5, ayant un spectre de Raman comprenant des valeurs de nombre d'ondes (en cm^-1) de : 2229 et 2240 cm^-1 ± 2 cm^-1

7. Forme cristalline selon l'une des revendications 2 à 6, ayant un spectre RMN à l'état solide de ¹³C comprenant des valeurs de résonance (en ppm) de : 39,1 et 142,1 ppm ± 0,2 ppm, par rapport à un étalon externe d'adamantane cristallin, établissant sa résonance avancée à 29,5 ppm.

8. Forme cristalline de base libre de lorlatinib selon la revendication 1 ayant un spectre de Raman comprenant deux valeurs de nombre d'ondes (en cm^-1) ou plus sélectionnées dans le groupe constitué par : 774, 1553, 1619, 2229 et 2240 cm^-1 ± 2 cm^-1.

9. Forme cristalline selon la revendication 8, ayant un spectre de Raman comprenant la valeur du nombre d'ondes (en cm^-1) de : 2229 et 2240 cm^-1 ± 2 cm^-1.

10. Forme cristalline selon la revendication 9, ayant un spectre de Raman comprenant en outre la valeur du nombre d'ondes (en cm^-1) de : 1619 cm^-1 ± 2 cm^-1.

11. Forme cristalline selon la revendication 9 ou 10, ayant un spectre de Raman comprenant en outre la valeur du nombre d'ondes (en cm^-1) de : 1553 cm^-1 ± 2 cm^-1.

12. Forme cristalline selon la revendication 9, 10 ou 11, ayant un spectre de Raman comprenant en outre la valeur du nombre d'ondes (en cm^-1) de : 774 cm^-1 ± 2 cm^-1.

13. Forme cristalline selon l'une des revendications 8 à 12, ayant un spectre RMN à l'état solide de ¹³C comprenant des valeurs de résonance (en ppm) de : 39,1 et 142,1 ppm ± 0,2 ppm, par rapport à un étalon externe d'adamantane cristallin, établissant sa résonance avancée à 29,5 ppm.

14. Forme cristalline de base libre de lorlatinib selon la revendication 1 ayant un spectre RMN à l'état solide de ¹³C comprenant deux valeurs de résonance (en ppm) ou plus sélectionnées dans le groupe constitué par : 25,8, 39,1, 112,3, 117,7 et 142,1 ppm ± 0,2 ppm, par rapport à un étalon externe d'adamantane cristallin, établissant sa résonance avancée à 29,5 ppm.

15. Forme cristalline selon la revendication 14, ayant un spectre RMN à l'état solide de ¹³C comprenant des valeurs de résonance (en ppm) de : 39,1 et 142,1 ppm ± 0,2 ppm.

16. Forme cristalline selon la revendication 15, ayant un spectre RMN à l'état solide de ¹³C comprenant la valeur de résonance (en ppm) de : 112,3 ppm ± 0,2 ppm.

17. Forme cristalline selon la revendication 15 ou 16, ayant un spectre RMN à l'état solide de ¹³C comprenant la valeur de résonance (en ppm) de : 25,8 ppm ± 0,2 ppm.

18. Forme cristalline selon la revendication 15, 16 ou 17 ayant un spectre RMN à l'état solide de ¹³C comprenant en outre la valeur de résonance (en ppm) de : 117,7 ppm ± 0,2 ppm.

19. Forme cristalline de base libre de lorlatinib, selon l'une des revendications 1 à 18 pour une utilisation dans le traitement d'une croissance cellulaire anormale chez un mammifère.

20. Base libre de lorlatinib pour une utilisation selon la revendication 19, dans laquelle la croissance cellulaire anormale est un cancer.

21. Base libre de lorlatinib pour une utilisation selon la revendication 20, dans laquelle le cancer est médié par la kinase du lymphome anaplasique (ALK) ou le récepteur à tyrosine kinase oncogène c-ros 1 (ROS1).

22. Base libre de lorlatinib pour une utilisation selon la revendication 20 ou 21, dans laquelle le cancer est un cancer du poumon non à petites cellules (NSCLC).

Drawing