Synthesis, characterization, and preclinical validation of a PET radiopharmaceutical for interrogating Aβ (β-amyloid) plaques in Alzheimer’s disease

For synthesis, 6-methoxy-2-methylbenzothiazole 1 was obtained using literature procedures [23, 33] and condensed with 6-(dimethyl-amino)-nicotinaldehyde in an aqueous potassium hydroxide (50%) solution dissolved in DMSO to obtain 2. Following purification, 2 was demethylated in the presence of BBr₃ to yield the phenolic derivative 3. Further, 3 was alkylated with 2-bromoethoxy-t-butyl-dimethylsilane in the presence of cesium carbonate to obtain t-butyl-dimethylsiloxy-ethoxy intermediate 4. Following treatment with TBAF, the intermediate yielded the corresponding ethanol derivative 5. Upon treatment with p-toluene sulfonylchloride, final precursor ligand 6 was obtained (Scheme 1). While the unlabeled counterpart 7A was obtained by treatment of precursor ligand 6 with TBAF, the no-carrier-added counterpart PET-tracer ¹⁸F-7B was obtained via standard nucleophilic substitution, using a well-established krytofix/¹⁸F methodology. While all intermediates 1, 2, 3, 4, 5, and 6 were characterized via routine analytical methods, the ¹⁸F-7B was characterized via co-injection with a well-characterized sample of its unlabeled counterpart 7A (Figure 1). The PET tracer ¹⁸F-7B eluted as a single chemical entity (radiochemical purity >95%), with a retention time of 9.5 min on a semi-preparative HPLC column (Phenomenex Luna® C18; 100 Å) (5 μm, 250 × 10 mm; flow rate, 3 mL/min). The appropriate fraction eluting at 9.5 min was collected, concentrated, dissolved in 10% ethanol in saline, and employed for bioassays (specific activity: 1,200 to 1,400 Ci/mmol). Although brain-imaging agents post-intravenous injection are known to show extremely facile penetration within the brain, nevertheless, permeation of competing labeled entities could complicate analysis. To assess preliminary stability in vivo, ¹⁸F-7B was incubated in human serum at 37°C up to 60 min, and radio-HPLC indicated the presence of primarily the parental compound. Of note, radio-HPLC detects the presence of mobile species thereby allowing immobile species to be retained on the column. Therefore, both radio-HPLC and radio-TLC have been used to allow detection of both polar and nonpolar radiometric metabolites. The radio-TLC demonstrated the presence of the single radiometric peak thus consistent with presence of ¹⁸F-7B under these conditions. Overall, the correlation of radio-HPLC and radio-TLC data indicated the metabolic stability of ¹⁸F-7B in the human serum under these conditions.

For assessing the ability of ¹⁸F-7B to bind Aβ plaques, preliminary binding assays with either preformed Aβ_1-42 aggregates or AD homogenates were performed in PBS. Nonspecific binding was determined in the presence of 7A (5 μM) as a competitor. Overall, the binding assay of ¹⁸F-7B with AD homogenates (Figure 2) indicates a saturable specific binding (K _d = 17.7 nM; B _max = 1,432 pmol/g wet weight; Figure 2a,b). Similarly, the binding affinity of ¹⁸F-7B with preformed fibrils (K _d = 61 nM; B _max = 6 pmol/nmol Aβ; Figure 2c,d) is nearly identical to the K _d value (59 nM) of 7A reported earlier [23]. Thus, the radiotracer binding assay technique shows a very close correlation with that of the fluorescence assay indicating identical binding properties of both the labeled and unlabeled counterparts. Furthermore, ¹⁸F-7B shows 3.4-fold higher affinity for AD homogenates compared with that of fibrils, a promising trait of translatable agents. Importantly, binding affinity of ¹⁸F-7B to AD homogenates is 2.6- and 5-fold lower than the FDA-approved radiotracers Flutemetamol [16] and Florbetapir [11], respectively. Furthermore, binding affinity of ¹⁸F-7B is fairly close to that of Florbetaben (K _d: 16 nM), the other FDA-approved radiotracer. However, it can also be argued that any advantage or disadvantage of a given imaging agent attributed only to the binding affinity is also equally dependent upon levels of occurrences of a given biomarker (that could be present either in very low or very high concentrations) in the targeted tissue [34]. One of the guiding principles for designing optimal brain-imaging agents also involves attaining a binding potential (BP) B _max/K _d ratio ≥10, although a lower value of BP could also enable PET molecular-imaging applications [22, 34, 35]. Given the high concentration of potential Aβ plaques and associated binding sites in AD brain [34], this could also mean that a radioligand with a K _d value of approximately 18 nM (BP (a combined measure of receptor density and affinity) = 1,432 nM/18 nM = 80) may be sufficient for imaging Aβ in AD. However, it is quite possible that the concentration of potential Aβ binding sites in earliest or presymptomatic AD brain is 1 order of magnitude less than 1,400 nM. Therefore, high-affinity ligands could offer better alternatives specifically when high-affinity binding sites predominate in the cortex and hippocampus of AD homogenates and are absent in the cerebellum [21]. Further analysis of BP of ¹⁸F-7B indicates that its value of 80 (in homogenates) is also 6- and 2-folds lower than that of ¹¹C-PIB (B _max: 1,407 nM; K _d: 2.5 nM; BP: 563) [28] and ¹⁸F-Florbetaben (B _max: 2,431 nM; K_d: 16 nM; BP: 152), respectively [36]. Combined results of binding affinity data suggest that PET-imaging characteristics of ¹⁸ F-7B could be slightly inferior to that of Flutemetamol and Florbetapir. Further, to evaluate the ability of ¹⁸F-7B for labeling Aβ in autopsy-confirmed human brain sections, autoradiography and immunohistochemical correlations were also performed. Following incubation of AD frontal cortex sections (12 μm) with ¹⁸F-7B (10 nM) for 60 min, the agent showed labeling of cortical Aβ plaques, and the binding was inhibited upon incubation in the presence of 7A (2.5 μM) (Figure 3a,c). These data indicate sensitivity and specificity of the ¹⁸F-7B. Additionally, immunohistochemical staining of these sections using anti-Aβ antibody indicated the presence of Aβ plaques in the cortex of these sections (Figure 3b,d), thus demonstrating excellent correlation of immunohistochemical staining data with that of autoradiography data. However, nuclear imaging of a given biomarker in vivo is a net function of signal to noise and thus also equally dependent upon pharmacokinetics of a given radiotracer in vivo.

Recently [23, 24], we have demonstrated via multiphoton imaging that 7A could traverse the BBB to label parenchymal plaques in the brain of transgenic mice. However, doses used for fluorescence were several folds higher than required for PET-imaging applications in vivo. Therefore, to assess whether or not PET counterpart ¹⁸F-7B administered at tracer concentrations relevant for nuclear imaging also displays similar kinetics in vivo, its pharmacokinetic studies in normal mice and microPET-imaging studies in transgenic mice and WT counterparts were performed. To accomplish this objective, biodistribution studies of ¹⁸F-7B were performed in normal FVB mice for preliminary assessment of signal-to-noise ratios and its clearance profiles. Uptake in brain and other critical organs was analyzed in terms of percent injected dose per gram of the tissue (%ID/g) Table 1. For in vivo imaging of Aβ plaques, the basic pharmacokinetic model in normal brains involves a high initial penetration of the agent, followed by facile clearance due to lack of a binding target. Preliminary biodistribution studies (Table 1) with HPLC-purified ¹⁸F-7B in normal mice show transient brain uptake values of 7.23 ± 0.47%ID/g and 1.55 ± 0.01%ID/g, 5- and 120-min post tail-vein injection, respectively, thus providing a 5 min/120 min clearance a ratio of 4.66. For comparison, brain uptake ratios of Florbetapir (2 min/2 h) and Florbetaben (2 min/4 h) in normal mice are 4.07 (%ID/g (brain): 2 min: 7.33 ± 1.54; 2 h: 1.80 ± 0.07; 7.33/1.80; 4.07) [11] and 5.0 (%ID/g (brain): 2 min: 4.77; 4 h: 0.95; 4.77/0.95; 5.02) [37], respectively. Therefore, the brain uptake clearance ratio of ¹⁸F-7B (5 min/120 min) is slightly superior to Florbetapir and comparable to that of Florbetaben in healthy mice. For an agent to be able to serve as an Aβ-imaging agent, literature precedents indicate that brain uptake ratio (%ID/g; the earliest time point; 2 to 5 min to that of the latest time point; typically for carbon-11; 30 to 60 min; and F-18, 2 h) of 3.5 or above could be considered as a benchmark for the ability of a given agent to cross the blood-brain barrier [38]. Additionally, brain uptake of a given imaging agent is a net function of several components, such as cerebral regional blood flow, BBB permeability, plasma radiotracer concentration, and free fractions of the radiotracer in plasma and in the brain. Additionally, the lipophilicity of a given compound reflects critical physicochemical trait for neuroimaging radiotracers due to its direct relationship to membrane permeability, solubility in water, and entropic contribution to binding. Literature precedents indicate that lipophilic drugs readily cross the BBB, although other chemical characteristics, including the number of hydrogen bonds, molecular weight, polar surface area, and molecular size, are also known to be critical to passive transport. Lipophilicity measured via LogP_OCT, the partition coefficient for nonionized molecules between octanol and water, is a good indicator of a molecule to permeate the brain, and molecules possessing Log P values of 0.9 and 3.0 have been shown to cross the BBB [39]. Conversely, radiotracers that are too lipophilic can also bind plasma proteins and undergo fast metabolism and also display high nonspecific binding. ¹⁸F-7B demonstrates a log P value of 1.3 which is identical to that of PIB (1.3) but considerably lower than that of Florbetapir (2.4) and Florbetaben (3.22). The clearance ratio of 4.66 (%ID/g; 5 min/120 min; Table 1) provides further evidence for the ability of the radiotracer to traverse the BBB in vivo and is consistent with previous data using multiphoton imaging [23]. Additionally, the agent ¹⁸F-7B showed excretion from other critical organs over 2 h and slight defluorination as a function of time indicated by bone accumulation thus consistent with pharmacokinetic profiles of other FDA-approved agents [11, 15, 16].

Transgenic mice expressing mutated forms of the gene for the human amyloid precursor protein (hAPP) show a marked elevation in Aβ-protein levels and their deposition in the cerebral cortex and hippocampus [40], which represent neuropathological hallmarks similar to those observed in human AD brains. It is also noteworthy that presenilin-1 (PS1) mutant transgenic mice show increased Aβ_1-42 peptide formation, thus augmenting amyloid deposition in Tg2576 APP mice at 6 months of age [41]. Therefore, the double-transgenic mice having co-expression of these mutated genes (APP^+/−/PS1^+/−) exhibit a strikingly accelerated accumulation of Aβ deposits compared with the single APP transgenic counterparts [42, 43]. Noticeably, several Aβ ligands [44‐46] and disease-modifying therapeutics have been investigated for their efficacy using APP^+/−/PS1^+/− transgenic models [47, 48]. Previously, we have shown via multiphoton imaging the pharmacokinetics of 7A in brains of transgenic mice at the highest resolution and its ability to penetrate the BBB to label Aβ plaques in brain parenchyma and blood vessels (CAA) [23]. Additionally, the low level of background fluorescence from residual retention of 7A in nearby brain regions suggested high signal-to-background ratios thus desirable of PET imaging in vivo. While fluorescence imaging offers high-resolution spatial localization of an imaging probe within a narrow field of view, the PET imaging provides its assessment at a relatively lower resolution within the whole organ. Therefore, it is necessary to interrogate sensitivity of the radiotracer for detecting Aβ in vivo at concentrations relevant for clinical nuclear imaging. To directly access the potential of ¹⁸F-7B to bind Aβ plaques in vivo, we performed microPET/CT imaging in age-matched APP^+/−/PS1^+/− mice (n = 3) compared to their WT counterparts, 5-min to 2-h post tail-vein injection. For any given agent to serve as an Aβ-targeted agent, a pharmacokinetic model would involve an initial high and equal influx of the tracer into the brains of transgenic and WT mice, followed by clearance of the radiotracer from brains of WT mice, thus demonstrating differential retention in regions of brains, as the agent binds to Aβ plaques in transgenic mice. Given that initial brain influx would be expected to be the same in both mouse models, and differential retention of ¹⁸F-7B in transgenic mice could result from its binding to Aβ plaques and clearance of the unbound tracer as a function of time, we therefore used dynamic PET imaging over 1 to 75 min to interrogate regional localization of ¹⁸F-7B within the brains of transgenic and WT mice. Preliminary microPET/CT imaging indicates a higher retention of ¹⁸F-7B in the frontal cortex of transgenic mice compared with their WT age-matched counterparts (Figure 4A,B) indicating its ability to traverse the BBB and label Aβ plaques in transgenic mice. Similar to ¹¹C-PIB [46, 49] and Florbetaben [45], ¹⁸F-7B shows also considerable retention in extracerebral regions, such as nasal and eye cavities. Furthermore, coupled with binding affinity and pharmacokinetic profiles of a given imaging agent, the presentation of different forms (diffuse and compact forms) of Aβ and the degree of fibrillary plaques can also impact signal-to-noise ratios (SNRs), thus influencing image quality. Additionally, Florbetaben, PiB, and Amyvid are known to preferentially bind fibrillary plaques, while 7A shows binding to both diffuse and fibrillary plaques, though with a lower affinity compared with approved tracers. Given these variations in targeting profiles and binding affinity, slightly lower SNR was observed using microPET imaging. For evaluation of kinetics, time-activity curves were obtained in the cortex and cerebellum (reference) regions of transgenic and WT mice (Figure 5). The data show a consistently higher retention of ¹⁸F-7B (40 min post-injection) in the cortex of transgenic mice compared to their age-matched WT controls (Figure 5), and these observations are in accord with other FDA-approved agents in rodents [44‐46]. For further evaluation of imaging potential of ¹⁸F-7B and analysis of SNRs in vivo, microPET imaging of transgenic mice as a function of aging profiles is under investigation. Overall, these PET data show excellent correlation with earlier studies employing its unlabeled counterpart 7A via multiphoton imaging [23].