An Isochroman Analog of CD3254 and Allyl-, Isochroman-Analogs of NEt-TMN Prove to Be More Potent Retinoid-X-Receptor (RXR) Selective Agonists Than Bexarotene

Bexarotene is an FDA-approved drug for the treatment of cutaneous T-cell lymphoma (CTCL); however, its use provokes or disrupts other retinoid-X-receptor (RXR)-dependent nuclear receptor pathways and thereby incites side effects including hypothyroidism and raised triglycerides. Two novel bexarotene analogs, as well as three unique CD3254 analogs and thirteen novel NEt-TMN analogs, were synthesized and characterized for their ability to induce RXR agonism in comparison to bexarotene (1). Several analogs in all three groups possessed an isochroman ring substitution for the bexarotene aliphatic group. Analogs were modeled for RXR binding affinity, and EC50 as well as IC50 values were established for all analogs in a KMT2A-MLLT3 leukemia cell line. All analogs were assessed for liver-X-receptor (LXR) activity in an LXRE system to gauge the potential for the compounds to provoke raised triglycerides by increasing LXR activity, as well as to drive LXRE-mediated transcription of brain ApoE expression as a marker for potential therapeutic use in neurodegenerative disorders. Preliminary results suggest these compounds display a broad spectrum of off-target activities. However, many of the novel compounds were observed to be more potent than 1. While some RXR agonists cross-signal the retinoic acid receptor (RAR), many of the rexinoids in this work displayed reduced RAR activity. The isochroman group did not appear to substantially reduce RXR activity on its own. The results of this study reveal that modifying potent, selective rexinoids like bexarotene, CD3254, and NEt-TMN can provide rexinoids with increased RXR selectivity, decreased potential for cross-signaling, and improved anti-proliferative characteristics in leukemia models compared to 1.


Introduction
Nuclear receptors (NRs) are ligand-dependent transcription factors that bind DNA sequence-specific motifs in enhancers and promoters to transactivate their target genes [1]. The retinoid X receptors (RXRs) are ligand-activated NRs that have pleiotropic effects including the control of hematopoietic stem cell self-renewal and differentiation. There noid shown to be more selective and potent for RXR than its enantiomer. The 9cUAB30 (4) [44] is another rexinoid in clinical trials for breast cancer [45][46][47], and studies of its methylated analogs [48,49] have helped elucidate the reasons that 4 does not provoke hyperlipidemia via LXR-RXR agonism. Boehm's group reported unbranched trienes terminating in carboxylic acids [50], along with analogs incorporating one [51] or fused aryl ring-systems [52]-in the case of the latter, compound 5 [52] is an example. When our group first entered the field, we reported a fluorinated bexarotene analog (6) [53] followed by other halogenated, and even a difluorinated bexarotene analog (7) [54]. The pyridine bexarotene analog (8) [55] and the pyrimidine bexarotene analog (9) [56], as well as LGD100268 (10) [55] and the LGD100268 pyrimidine analog (11) [56] all showed enhanced RXR activity compared to 1 and superior therapeutic effects in mouse models of cancer [28,57]. Installing an unsaturation in bexarotene's aliphatic ring results in compound 12 [58,59], and the unsaturated-fluorinated bexarotene (13) [56] also activates LXR [60]. CD3254 (14) [61] and CD2915 (15) [62] are two synthetic rexinoids with activity comparable to 1. Our group utilized 14 and 15 to design analogous rexinoids 16-19 [56]. Kakuta and colleagues reported compound 20 (NEt-TMN) [63][64][65][66] as well as its analogous compounds 21 [67][68][69] and 22 [67,68]-all of which showed high potency and selectivity for RXR alongside many other NEt-TMN derivatives that our group reported [70]. Even replacing the ethyl group with a methyl group on the linking nitrogen atom of NEt-TMN leads to potent rexinoids such as 23 [71], 24 [71], and 25 [71] (Figure 1). profiles. One well-known rexinoid that is in phase II clinical trials for prostate cancer [42] and pre-clinical trials for PD, AD, and multiple sclerosis is IRX-4204 (3) [43], a chiral rexinoid shown to be more selective and potent for RXR than its enantiomer. The 9cUAB30 (4) [44] is another rexinoid in clinical trials for breast cancer [45][46][47], and studies of its methylated analogs [48,49] have helped elucidate the reasons that 4 does not provoke hyperlipidemia via LXR-RXR agonism. Boehm's group reported unbranched trienes terminating in carboxylic acids [50], along with analogs incorporating one [51] or fused aryl ring-systems [52]-in the case of the latter, compound 5 [52] is an example. When our group first entered the field, we reported a fluorinated bexarotene analog (6) [53] followed by other halogenated, and even a difluorinated bexarotene analog (7) [54]. The pyridine bexarotene analog (8) [55] and the pyrimidine bexarotene analog (9) [56], as well as LGD100268 (10) [55] and the LGD100268 pyrimidine analog (11) [56] all showed enhanced RXR activity compared to 1 and superior therapeutic effects in mouse models of cancer [28,57]. Installing an unsaturation in bexarotene's aliphatic ring results in compound 12 [58,59], and the unsaturated-fluorinated bexarotene (13) [56] also activates LXR [60]. CD3254 (14) [61] and CD2915 (15) [62] are two synthetic rexinoids with activity comparable to 1. Our group utilized 14 and 15 to design analogous rexinoids 16-19 [56]. Kakuta and colleagues reported compound 20 (NEt-TMN) [63][64][65][66] as well as its analogous compounds 21 [67][68][69] and 22 [67,68]-all of which showed high potency and selectivity for RXR alongside many other NEt-TMN derivatives that our group reported [70]. Even replacing the ethyl group with a methyl group on the linking nitrogen atom of NEt-TMN leads to potent rexinoids such as 23 [71], 24 [71], and 25 [71] (Figure 1).  The current study uses many of the above compounds cited above as starting points to investigate how introducing new modifications result in changes to the compounds' activities. For example, we were interested in substituting an isochroman group for the aliphatic ring system in bexarotene and some of the CD3254 analogs that have been reported, as well as a multiple fused aryl-ring system, and hence we targeted the synthesis of rexinoids 26-30. We were also interested in exploring a pyridine aromatic ring substitution from reported analogs 23-25, so we targeted the synthesis of 31. Due to the potency of NEt-TMN (20) and its analogs, we were curious about the impacts that substituting an allyl group, varying aromatic rings, and adding a methyl group would have on RXR activity for the new rexinoids, so we targeted the synthesis of 32-35. Finally, we were interested in substituting the isochroman group for the aliphatic ring system of NEt-TMN and then varying the N-alkyl chains-including methy, ethyl and allyl-along with different aromatic acid ring systems, and so we targeted 36-44 for synthesis ( Figure 2). Interestingly, compound 34 [67] was previously made and disclosed by Kagechika and co-workers, so we were eager to synthesize several possible analogs of it (32,33,35,40,41, and 44) and compare their activities.
activities. For example, we were interested in substituting an isochroman group for the aliphatic ring system in bexarotene and some of the CD3254 analogs that have been reported, as well as a multiple fused aryl-ring system, and hence we targeted the synthesis of rexinoids 26-30. We were also interested in exploring a pyridine aromatic ring substitution from reported analogs 23-25, so we targeted the synthesis of 31. Due to the potency of NEt-TMN (20) and its analogs, we were curious about the impacts that substituting an allyl group, varying aromatic rings, and adding a methyl group would have on RXR activity for the new rexinoids, so we targeted the synthesis of 32-35. Finally, we were interested in substituting the isochroman group for the aliphatic ring system of NEt-TMN and then varying the N-alkyl chains-including methy, ethyl and allyl-along with different aromatic acid ring systems, and so we targeted 36-44 for synthesis ( Figure 2). Interestingly, compound 34 [67] was previously made and disclosed by Kagechika and co-workers, so we were eager to synthesize several possible analogs of it (32, 33, 35, 40, 41, and 44) and compare their activities. While the isochroman group places a fairly polar, hydrogen-bonding oxygen atom in the nonpolar aliphatic ring system for the known parent rexinoids, we hypothesized that it would not disrupt the largely non-polar binding interaction in the RXR LBD. Further, we hypothesized that the isochroman group would make the rexinoids possessing it more resistant to metabolic oxidation. If the isochroman rexinoids were as potent and selective as their non-isochroman counterparts, we also hypothesized that they would possess similar in vitro activities as their parent compounds. Importantly, we wanted to assess these specific hypotheses about the incorporation of an isochroman group across multiple parent compound structures that include bexarotene (1), CD3254 (14), and various NEt-TMN (20) analogs coupled with other potential modifications to assess similarities or differences in the activities of the resulting analogs and their predecessors. Hence, we proceeded with the synthesis and testing of these compounds. While the isochroman group places a fairly polar, hydrogen-bonding oxygen atom in the nonpolar aliphatic ring system for the known parent rexinoids, we hypothesized that it would not disrupt the largely non-polar binding interaction in the RXR LBD. Further, we hypothesized that the isochroman group would make the rexinoids possessing it more resistant to metabolic oxidation. If the isochroman rexinoids were as potent and selective as their non-isochroman counterparts, we also hypothesized that they would possess similar in vitro activities as their parent compounds. Importantly, we wanted to assess these specific hypotheses about the incorporation of an isochroman group across multiple parent compound structures that include bexarotene (1), CD3254 (14), and various NEt-TMN (20) analogs coupled with other potential modifications to assess similarities or differences in the activities of the resulting analogs and their predecessors. Hence, we proceeded with the synthesis and testing of these compounds.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydro-gen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.

Results: Molecular Modeling
The binding affinity, predicted using AutoDock Vina [72], of human-RXR for each ligand is output as an energy unit (in kcal/mol, Table 1). These predicted ligand-bound RXR complexes were then visually inspected using PyMol (version 2.3, Shrodinger, LLC) ( Figure 3). To further analyze and illustrate the interactions between RXR protein residue sidechains with the ligands, PoseView (BioSolvIT [73,74]) was used to generate the detailed two-dimensional depictions ( Figure 3B,C). In these two-dimensional depictions, hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.  The AutoDock Vina docking results showed that the standard compound bexaroten (1), with a score of −12.7 kcal/mol, was the most potent among all compounds. Compound 26 has a comparable score of −12.4 kcal/mol. Additionally, similar interactions with RXR residue sidechains were observed between 1 and 26 such as direct interactions between Phe313 and the aromatic cores of either ligand, as well as hydrophobic residues Ile268 Ile345, and Ala272 bearing common interactions ( Figure 3B,C). Several other compound have similar but slightly lower scores of −11.9 kcal/mol (30), −11.7 kcal/mol (28), −11.6 kcal/mol (34), and −11.5 kcal/mol (23, 29, 31, 32, 42, 43, and 44) (Table 1). Therefore, we can The AutoDock Vina docking results showed that the standard compound bexarotene (1), with a score of −12.7 kcal/mol, was the most potent among all compounds. Compound 26 has a comparable score of −12.4 kcal/mol. Additionally, similar interactions with RXR residue sidechains were observed between 1 and 26 such as direct interactions between Phe313 and the aromatic cores of either ligand, as well as hydrophobic residues Ile268, Ile345, and Ala272 bearing common interactions ( Figure 3B,C). Several other compounds have similar but slightly lower scores of −11.9 kcal/mol (30), −11.7 kcal/mol (28), −11.6 kcal/mol (34), and −11.5 kcal/mol (23, 29, 31, 32, 42, 43, and 44) (Table 1). Therefore, we can conclude that RXR compounds with a docking score within 10% that of bexarotene could potentially possess comparable, or better, EC 50 and IC 50 profiles for further study.
the interactions between protein residue sidechains with bexarotene (B) and compound 26 (C) using PoseView (BioSolvIT [73,74]). In both (B) and (C), hydrogen bonds are presented as dashed lines between interaction partners, and hydrophobic interactions are depicted as smooth contour lines.
The AutoDock Vina docking results showed that the standard compound bexarotene (1), with a score of −12.7 kcal/mol, was the most potent among all compounds. Compound 26 has a comparable score of −12.4 kcal/mol. Additionally, similar interactions with RXR residue sidechains were observed between 1 and 26 such as direct interactions between Phe313 and the aromatic cores of either ligand, as well as hydrophobic residues Ile268, Ile345, and Ala272 bearing common interactions ( Figure 3B,C). Several other compounds have similar but slightly lower scores of −11.9 kcal/mol (30), −11.7 kcal/mol (28), −11.6 kcal/mol (34), and −11.5 kcal/mol (23, 29, 31, 32, 42, 43, and 44) (Table 1). Therefore, we can conclude that RXR compounds with a docking score within 10% that of bexarotene could potentially possess comparable, or better, EC50 and IC50 profiles for further study.

Results: Chemistry
The synthesis of compound 26 begins with the bromination of commercially available 1,1,4,4,7-pentamethylisochroman (45) with bromine in dichloromethane and aluminum chloride catalyst to give 6-bromo-1,1,4,4,7-pentamethylisochroman (46) in 96% yield (Scheme 1) [75]. Compound 46 was lithiated by treatment with n-butyllithium, and the resulting aryl lithium reagent (47) was transferred to a solution of the reported amide 48 [59] in THF to provide ketone (49) in 56% purified yield whose nitrile group is then hydrolyzed to a carboxylic acid (50) in quantitative yield. Compound 50, when treated with more than two equivalents of methylmagnesium chloride is converted to alcohol 51 that is then dehydrated to compound 26 in 58.3% over two steps (Scheme 2). Compound 46 was lithiated by treatment with n-butyllithium, and the resulting aryl lithium reagent (47) was transferred to a solution of the reported amide 48 [59] in THF to provide ketone (49) in 56% purified yield whose nitrile group is then hydrolyzed to a carboxylic acid (50) in quantitative yield. Compound 50, when treated with more than two equivalents of methylmagnesium chloride is converted to alcohol 51 that is then dehydrated to compound 26 in 58.3% over two steps (Scheme 2).

Scheme 2.
Conversion of 46 to lithium-isochroman 47, its reaction with amide-nitrile 48 to give ketone-nitrile 49 that was subsequently hydrolyzed to ketone-acid 50 which was converted to alcohol-acid 51 that was finally dehydrated to isochroman acid 26.
Acid 26 formed single, transparent crystals, so an X-ray diffraction study was conducted to confirm the structure of 26 (Figure 4).

Scheme 2.
Conversion of 46 to lithium-isochroman 47, its reaction with amide-nitrile 48 to give ketone-nitrile 49 that was subsequently hydrolyzed to ketone-acid 50 which was converted to alcoholacid 51 that was finally dehydrated to isochroman acid 26.
Acid 26 formed single, transparent crystals, so an X-ray diffraction study was conducted to confirm the structure of 26 (Figure 4). Compound 46 was lithiated by treatment with n-butyllithium, and the resulting aryl lithium reagent (47) was transferred to a solution of the reported amide 48 [59] in THF to provide ketone (49) in 56% purified yield whose nitrile group is then hydrolyzed to a carboxylic acid (50) in quantitative yield. Compound 50, when treated with more than two equivalents of methylmagnesium chloride is converted to alcohol 51 that is then dehydrated to compound 26 in 58.3% over two steps (Scheme 2).

Scheme 2.
Conversion of 46 to lithium-isochroman 47, its reaction with amide-nitrile 48 to give ketone-nitrile 49 that was subsequently hydrolyzed to ketone-acid 50 which was converted to alcohol-acid 51 that was finally dehydrated to isochroman acid 26.
Acid 26 formed single, transparent crystals, so an X-ray diffraction study was conducted to confirm the structure of 26 (Figure 4).  To synthesize compound 27, compound 46 was treated with n-butyllithium and then triisopropylborate to give 52 in 73% yield (Scheme 3). To synthesize compound 27, compound 46 was treated with n-butyllithium and then triisopropylborate to give 52 in 73% yield (Scheme 3). The known ethyl ester 53 [56] was combined with boronic acid 53 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 54 in 64% yield, and ethyl ester 54 was saponified with KOH in methanol to give 27 in 81.8% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 4).
Int. J. Mol. Sci. 2022, 23, 16213 10 of 23 The known ethyl ester 53 [56] was combined with boronic acid 53 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 54 in 64% yield, and ethyl ester 54 was saponified with KOH in methanol to give 27 in 81.8% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 4).

Scheme 4. Synthesis of biphenyl 54 and its saponification to give acid 27.
A similar procedure was used to make compounds 28, 29, and 30. For compound 28, the known ethyl ester 55 [56] was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 56 in 67% yield, and ethyl ester 56 was saponified with KOH in methanol to give 28 in 71.9% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 5).

Scheme 5. Synthesis of biphenyl 56 and its saponification to give acid 28.
For compound 5, the known ethyl ester 57 [56] was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 58 in 41.7% yield, and ethyl ester 58 was saponified with KOH in methanol to give 29 in 75% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 6). Scheme 6. Synthesis of biphenyl 58 and its saponification to give acid 29.

Scheme 4. Synthesis of biphenyl 54 and its saponification to give acid 27.
A similar procedure was used to make compounds 28, 29, and 30. For compound 28, the known ethyl ester 55 [56] was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 56 in 67% yield, and ethyl ester 56 was saponified with KOH in methanol to give 28 in 71.9% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 5).
Int. J. Mol. Sci. 2022, 23, 16213 10 of 23 The known ethyl ester 53 [56] was combined with boronic acid 53 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 54 in 64% yield, and ethyl ester 54 was saponified with KOH in methanol to give 27 in 81.8% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 4).

Scheme 4. Synthesis of biphenyl 54 and its saponification to give acid 27.
A similar procedure was used to make compounds 28, 29, and 30. For compound 28, the known ethyl ester 55 [56] was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 56 in 67% yield, and ethyl ester 56 was saponified with KOH in methanol to give 28 in 71.9% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 5).

Scheme 5. Synthesis of biphenyl 56 and its saponification to give acid 28.
For compound 5, the known ethyl ester 57 [56] was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 58 in 41.7% yield, and ethyl ester 58 was saponified with KOH in methanol to give 29 in 75% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 6). Scheme 6. Synthesis of biphenyl 58 and its saponification to give acid 29. For compound 5, the known ethyl ester 57 [56] was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 58 in 41.7% yield, and ethyl ester 58 was saponified with KOH in methanol to give 29 in 75% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 6).
For compound 30, the commercially available methyl ester 59 was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 60 in 48% yield, and methyl ester 60 was saponified with KOH in methanol to give 30 in 83% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 7). Scheme 5. Synthesis of biphenyl 56 and its saponification to give acid 28.
For compound 5, the known ethyl ester 57 [56] was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 58 in 41.7% yield, and ethyl ester 58 was saponified with KOH in methanol to give 29 in 75% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 6). Scheme 6. Synthesis of biphenyl 58 and its saponification to give acid 29.
For compound 30, the commercially available methyl ester 59 was combined with boronic acid 52 along with Pd(II) diacetate, TBAB, and sodium carbonate in water and heated to boiling for 5 min to give 60 in 48% yield, and methyl ester 60 was saponified with KOH in methanol to give 30 in 83% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 7).

Scheme 7.
Synthesis of methyl ester 60 and its saponification to give acid 30.
The synthesis of known compounds 23, 24, 25, and novel compound 31 begins with the conversion of known compounds 61-64 [70] to compounds 65-68 by treatment with sodium hydride followed by methyl iodide in DMF with stirring at room temperature in good yields. The methyl esters 65-68 were saponified by treatment with KOH in methanol followed by acidification and purification to give compounds 23-25 and 31, respectively, in moderate to good yields (Scheme 8). The synthesis of compounds 32-35 begins with the conversion of known compounds [70] 64, 62, 61, and 63 to compounds 69-72 by treatment with sodium hydride followed by allyl bromide in DMF with stirring at room temperature in good yields. The methyl esters 69-72 were saponified by treatment with KOH in methanol followed by acidification and purification to give compounds 32-35 in moderate to good yields (Scheme 9). The synthesis of compounds 36-41 begins with the palladium-catalyzed reaction of the known aryl bromide 46 with methyl 6-aminonicotinate (73) or methyl 2-aminopyrimidine-5-carboxylate (74) to give diaryl amines 75 or 76 in moderate yields of 55% and 40%, respectively. The diaryl amines 75 and 76 were treated with sodium hydride followed by methyl iodide, ethyl iodide, or allyl bromide to give methyl esters 77-82 in moderate to good yields which were then saponified by treatment with KOH in methanol followed by acidification and purification to give compounds 36-41 in moderate to good yields (Scheme 10).  with KOH in methanol to give 30 in 83% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 7).

Scheme 7.
Synthesis of methyl ester 60 and its saponification to give acid 30.
The synthesis of known compounds 23, 24, 25, and novel compound 31 begins with the conversion of known compounds 61-64 [70] to compounds 65-68 by treatment with sodium hydride followed by methyl iodide in DMF with stirring at room temperature in good yields. The methyl esters 65-68 were saponified by treatment with KOH in methanol followed by acidification and purification to give compounds 23-25 and 31, respectively, in moderate to good yields (Scheme 8). The synthesis of compounds 32-35 begins with the conversion of known compounds [70] 64, 62, 61, and 63 to compounds 69-72 by treatment with sodium hydride followed by allyl bromide in DMF with stirring at room temperature in good yields. The methyl esters 69-72 were saponified by treatment with KOH in methanol followed by acidification and purification to give compounds 32-35 in moderate to good yields (Scheme 9). 13 11 of 23 with KOH in methanol to give 30 in 83% yield after acidification with 1N HCl, filtration, and purification by column chromatography (Scheme 7).

Scheme 7.
Synthesis of methyl ester 60 and its saponification to give acid 30.
The synthesis of known compounds 23, 24, 25, and novel compound 31 begins with the conversion of known compounds 61-64 [70] to compounds 65-68 by treatment with sodium hydride followed by methyl iodide in DMF with stirring at room temperature in good yields. The methyl esters 65-68 were saponified by treatment with KOH in methanol followed by acidification and purification to give compounds 23-25 and 31, respectively, in moderate to good yields (Scheme 8). The synthesis of compounds 36-41 begins with the palladium-catalyzed reaction of the known aryl bromide 46 with methyl 6-aminonicotinate (73) or methyl 2-aminopyrimidine-5-carboxylate (74) to give diaryl amines 75 or 76 in moderate yields of 55% and 40%, respectively. The diaryl amines 75 and 76 were treated with sodium hydride followed by methyl iodide, ethyl iodide, or allyl bromide to give methyl esters 77-82 in moderate to good yields which were then saponified by treatment with KOH in methanol followed by The synthesis of compounds 36-41 begins with the palladium-catalyzed reaction of the known aryl bromide 46 with methyl 6-aminonicotinate (73) or methyl 2-aminopyrimidine-5-carboxylate (74) to give diaryl amines 75 or 76 in moderate yields of 55% and 40%, respectively. The diaryl amines 75 and 76 were treated with sodium hydride followed by methyl iodide, ethyl iodide, or allyl bromide to give methyl esters 77-82 in moderate to good yields which were then saponified by treatment with KOH in methanol followed by acidification and purification to give compounds 36-41 in moderate to good yields (Scheme 10). Acid 41 formed single, transparent crystals from d6-DMSO, so an X-ray diffraction study was undertaken to confirm the structure for 41 ( Figure 5). Finally, the synthesis of novel rexinoids 42-44 begins with the nitration of isochroman (45) to give 83 in 98% yield, followed by the hydrogenation of 83 to give aryl amine 84 in quantitative yield. Aryl amine 84 is then combined with 4-iodomethylbenzoate (85) in a palladium-catalyzed reaction to give 86 in 24% yield. Diaryl amine 86 is then treated with sodium hydride followed by methyl iodide, ethyl iodide, or allyl bromide to give methyl esters 87-89 in moderate to good yields and the methyl esters are saponified with potassium hydroxide in methanol followed by acid work-up to give rexinoids 42-44 in good yields after purification (Scheme 11). Acid 41 formed single, transparent crystals from d6-DMSO, so an X-ray diffraction study was undertaken to confirm the structure for 41 ( Figure 5). Acid 41 formed single, transparent crystals from d6-DMSO, so an X-ray diffraction study was undertaken to confirm the structure for 41 ( Figure 5). Finally, the synthesis of novel rexinoids 42-44 begins with the nitration of isochroman (45) to give 83 in 98% yield, followed by the hydrogenation of 83 to give aryl amine 84 in quantitative yield. Aryl amine 84 is then combined with 4-iodomethylbenzoate (85) in a palladium-catalyzed reaction to give 86 in 24% yield. Diaryl amine 86 is then treated with sodium hydride followed by methyl iodide, ethyl iodide, or allyl bromide to give methyl esters 87-89 in moderate to good yields and the methyl esters are saponified with potassium hydroxide in methanol followed by acid work-up to give rexinoids 42-44 in good yields after purification (Scheme 11). Finally, the synthesis of novel rexinoids 42-44 begins with the nitration of isochroman (45) to give 83 in 98% yield, followed by the hydrogenation of 83 to give aryl amine 84 in quantitative yield. Aryl amine 84 is then combined with 4-iodomethylbenzoate (85) in a palladium-catalyzed reaction to give 86 in 24% yield. Diaryl amine 86 is then treated with sodium hydride followed by methyl iodide, ethyl iodide, or allyl bromide to give methyl esters 87-89 in moderate to good yields and the methyl esters are saponified with potassium hydroxide in methanol followed by acid work-up to give rexinoids 42-44 in good yields after purification (Scheme 11). Scheme 11. Synthesis of nitro-isochroman 83, its reduction to aniline 84 and subsequent coupling with 85 to provide 86 and its subsequent alkylation to give methyl esters 87-89 and their saponification to yield acids 42-44.

Results and Discussion: Biological Assays
Bexarotene (1) and the isochroman and other analogs of bexarotene, CD3254, and NEt-TMN 26-44 were tested in a KMT2A-MLLT3 cell line to determine RXRα activation EC50 values by both a Luc-and GFP-assay, and then IC50 values for a 96 h cell viability assay were determined both in the presence and absence of 100 nM ATRA and the resulting data is tabulated in Table 1. Compounds 1 and 26-44 were examined for cytotoxicity and mutagenicity in Saccharomyces cerevisiae [76]. None of the compounds were mutagenic or cytotoxic.
We also evaluated the analogs for their capacity to bind and activate the liver-X-receptor (LXR) using a liver-X-receptor responsive element (LXRE)-based assay, and assessed the effects in the presence vs. absence of an authentic LXR compound (TO901317), as well as with bexarotene alone. LXR is known to regulate inflammatory responses and lipid metabolism in multiple tissues, including the central nervous system, and there is sufficient evidence that strong cholesterol and lipid metabolism in the brain, along with enhanced ApoE expression, is paramount to reducing the risk of human dementias. The "activity assessment" of our novel RXR agonists for their ability to enhance gene expression using a DNA responsive element sequence (LXRE) that is found to occur in the natural human promoter of LXR-RXR controlled genes (such as ApoE) was carried out in U87 glial cells with bexarotene (1) as a comparative control. Using the above assay system, the activation from this natural LXRE was probed with either 100 nM RXR analogs (or bexarotene) alone or in combination with 100 nM of both the RXR agonist and an LXR ligand T0901317 (TO). The employment of both LXR and RXR agonists collectively was anticipated to demonstrate a more vigorous response in LXRE transactivation due to cumulative and/or synergistic effects of dual ligand activation of the RXR-LXR heterodimer. The results demonstrated that in comparison to the parent bexarotene (1) compound alone, separate dosing of the cells with analogs 26, 27, 28, 29, and 30 displayed more LXR/LXRE activity ( Figure 6A, p < 0.05). Scheme 11. Synthesis of nitro-isochroman 83, its reduction to aniline 84 and subsequent coupling with 85 to provide 86 and its subsequent alkylation to give methyl esters 87-89 and their saponification to yield acids 42-44.

Results and Discussion: Biological Assays
Bexarotene (1) and the isochroman and other analogs of bexarotene, CD3254, and NEt-TMN 26-44 were tested in a KMT2A-MLLT3 cell line to determine RXRα activation EC50 values by both a Luc-and GFP-assay, and then IC50 values for a 96 h cell viability assay were determined both in the presence and absence of 100 nM ATRA and the resulting data is tabulated in Table 1. Compounds 1 and 26-44 were examined for cytotoxicity and mutagenicity in Saccharomyces cerevisiae [76]. None of the compounds were mutagenic or cytotoxic.
We also evaluated the analogs for their capacity to bind and activate the liver-X-receptor (LXR) using a liver-X-receptor responsive element (LXRE)-based assay, and assessed the effects in the presence vs. absence of an authentic LXR compound (TO901317), as well as with bexarotene alone. LXR is known to regulate inflammatory responses and lipid metabolism in multiple tissues, including the central nervous system, and there is sufficient evidence that strong cholesterol and lipid metabolism in the brain, along with enhanced ApoE expression, is paramount to reducing the risk of human dementias. The "activity assessment" of our novel RXR agonists for their ability to enhance gene expression using a DNA responsive element sequence (LXRE) that is found to occur in the natural human promoter of LXR-RXR controlled genes (such as ApoE) was carried out in U87 glial cells with bexarotene (1) as a comparative control. Using the above assay system, the activation from this natural LXRE was probed with either 100 nM RXR analogs (or bexarotene) alone or in combination with 100 nM of both the RXR agonist and an LXR ligand T0901317 (TO). The employment of both LXR and RXR agonists collectively was anticipated to demonstrate a more vigorous response in LXRE transactivation due to cumulative and/or synergistic effects of dual ligand activation of the RXR-LXR heterodimer. The results demonstrated that in comparison to the parent bexarotene (1) compound alone, separate dosing of the cells with analogs 26, 27, 28, 29, and 30 displayed more LXR/LXRE activity ( Figure 6A, p < 0.05).
Specifically, the analogs displayed activities ranging from 52% to 254% of the bexarotene control (set to 100%; Table 1). Furthermore, when the LXR synthetic ligand (TO) was used in combination with bexarotene (1) or analogs, similar results were observed ( Figure 6A, Figure 7A, and Figure 8A, stippled bars). Although some of the analogs exhibit lower LXR activation when compared to bexarotene (1), it is imperative to evaluate this activity in the background of the RXR-RXR homodimer activity of each analog, and to thus "normalize" the LXR/LXRE heterodimer activation results. The LXRE Heterodimer Specificity (LHS) score ( Figure 6B, Figure 7B, and Figure 8B) is thus calculated based on both the RXR homodimer activity, as well as the LXR heterodimer activation. The results of this LHS analysis (Table 1) reveal that many of our novel compounds (e.g., 26, 27, 29, 30, 31, and 37, p < 0.05) display enhanced LXR/LXRE activity via increased heterodimer specificity compared to the parent bexarotene (1).
Finally, even though compound 1 is selective for binding to RXR, it does include some "residual" RAR activity. We assessed the potential of our analogs to induce transcription via the retinoic acid response element (RARE) and retinoic acid receptor. For these studies, we employed human embryonic cells (HEK293) that were transfected with human RARα and dosed with 10 nM of either all-trans retinoic acid (ATRA), the endogenous ligand for RARα, compound 1, or our panel of analogs. The results of the assay revealed that compound 1 displayed an average of 37% of the activity of the ATRA control (set to 100%, Table 1). Analog 32 exhibited the greatest RARE activation at 62% of ATRA, while analog 37 showed the lowest RARE activity at 4%, which is indistinguishable from the ethanol control (Table 1). Importantly, most of our novel analogs (14 out of 18) possess attenuated "cross-over" onto RAR-RARE signaling compared to bexarotene (1). Specifically, the analogs displayed activities ranging from 52% to 254% of the bexarotene control (set to 100%; Table 1). Furthermore, when the LXR synthetic ligand (TO) was used in combination with bexarotene (1) or analogs, similar results were observed (Figures 6A, 7A, and 8A, stippled bars). Although some of the analogs exhibit lower LXR activation when compared to bexarotene (1), it is imperative to evaluate this activity in the background of the RXR-RXR homodimer activity of each analog, and to thus "normalize" the LXR/LXRE heterodimer activation results. The LXRE Heterodimer Specificity (LHS) score ( Figures 6B, 7B, and 8B) is thus calculated based on both the RXR homodimer activity, as well as the LXR heterodimer activation. The results of this LHS analysis (Table 1) reveal that many of our novel compounds (e.g., 26, 27, 29, 30, 31, and 37, p < 0.05) display enhanced LXR/LXRE activity via increased heterodimer specificity compared to the parent bexarotene (1).  ApoE gene, and a Renilla control plasmid. Cells were transfected for 24 h utilizing a liposome-mediated transfection protocol and then treated with ethanol vehicle, or 100 nM of the indicated compound alone or in combination with 100 nM TO901317 (TO). LXRE-directed activity was compared to compound 1 (Bexarotene), set to 100%. (B) The "Heterodimer Specificity Score" was determined by the LXRE:RXRE ratio with compound 1 set to 1.0. All error bars represent standard deviations; the data are representative of at least three independent experiments with six replicates in each treatment group. * p < 0.05 versus control compound 1. Finally, even though compound 1 is selective for binding to RXR, it does include some "residual" RAR activity. We assessed the potential of our analogs to induce transcription via the retinoic acid response element (RARE) and retinoic acid receptor. For these studies, we employed human embryonic cells (HEK293) that were transfected with human RARα and dosed with 10 nM of either all-trans retinoic acid (ATRA), the endogenous ligand for RARα, compound 1, or our panel of analogs. The results of the assay revealed that compound 1 displayed an average of 37% of the activity of the ATRA control (set to 100%, Table 1). Analog 32 exhibited the greatest RARE activation at 62% of ATRA, while analog 37 showed the lowest RARE activity at 4%, which is indistinguishable from

Conclusions
While the substitution of the saturated, pentamethyl-tetrahydronaphthyl ring system of bexarotene, CD3254, or Net-TMN-analog parent compound frameworks with a pentamethyl-isochroman ring system tended to decrease both modeled binding scores as well as RXR EC50 values, there were nevertheless some examples of very potent compounds possessing the pentamethyl-isochroman ring system. Several reported and novel compounds displayed lower or equivalent EC50 values than bexarotene (e.g., reported compounds 23-25 and novel compounds 29, 31-33, 35, and 40), and several reported and novel compounds exhibited lower IC50 values along with 100 nM ATRA (e.g., reported compounds 23 and 24, and novel compounds 29 and 31-35) than bexarotene. It should be noted that compound 29 is an isochroman analog of CD3254 and compound 40 is an isochroman analog of NEt-TMN, so while the isochroman substituted analog tends to reduce potency compared to the parent compounds, rexinoids possessing the isochroman group can still be synthesized that exhibit greater potency than bexarotene. Notably, some of the compounds possessing the greatest RARE activity at 10 nM vs. ATRA also exhibited lower IC50 values along with 100 nM ATRA (e.g., 29 and 31-33). Additionally, the range of LXRE activity vs. bexarotene demonstrated that several compounds exhibit increased LXR activity and specificity vs. bexarotene. In particular, compounds 29 and 31-35 appear to be good candidates for further investigation, and this study suggests that modification of known, potent rexinoids results in novel compounds with unique and promising therapeutic potential meriting further examination. We are actively pursuing additional studies towards these ends.

Materials and Methods
Molecular Modeling. The three-dimensional structures of the compounds reported herein were generated using ChemDraw 3D (PerkinElmer Informatics, Waltham, MA, USA), energy minimized, and exported in the Protein Data Bank (PDB) format. The human RXR alpha ligand binding domain structure model was obtained from the PDB (PDB code: 1FBY [77]). The crystallized ligand, 9-cis retinoic acid, was removed from the protein model prior to docking simulations. Further, 9-cis retinoic acid was also used as a positive control in the docking studies presented here. Both the protein and ligand models were prepared using MGLTools (version 1.5.7) [78] and screened virtually using AutoDock Vina [72] overnight and transduced with MSCV-KMT2A-MLLT3 retrovirus by spinfection with 10 µg/mL polybrene and 10 mM HEPES at 2400 rpm, 30 • C for 90 min in an Eppendorf 5810R centrifuge. Cells were transplanted into sublethally irradiated mice and subsequent leukemia harvested 4 to 6 months later. KMT2A-MLLT3 leukemia cells were cultured in vitro using similar media, but without Flt3L or thrombopoietin.
UAS/Gal4 assay. Bone marrow cells from UAS-GFP mice [79] were transduced with retroviruses MSCV-Gal4 (DNA binding domain, DBD)-RXRα (ligand binding domain, LBD)-IRES-mCherry. Gal4 is a yeast transcription factor and the UAS sequence is not recognized by mammalian transcription factors. Cells were treated, and after 48 h, GFP was measured by flow cytometry.
Luciferase detection. HEK293T cells were transfected using Lipofectamine 2000 (Invitrogen) [80]. Six hours after transfection, the cells were collected and plated into a 48-well plate in 1% BSA media in biological triplicates and treated with compounds. After 40 h incubation, the cells were harvested and assayed for luciferase (Luc Assay System with Reporter Lysis Buffer, Promega) in a Beckman Coulter LD400 plate reader. LXRE assay. Human glioblastoma cells (U87) were purchased from American Type Culture Collection (ATCC, Manassas, VA, USA) and used to perform the LXRE-mediated assays. Authentication and validation of these master stocks included both testing for mycoplasma contamination (via Universal Mycoplasma Detection Kit; ATCC, Cat. #30-1012K), as well as short tandem repeat (STR) analysis to confirm cell line identity. For LXRE experiments, cells were seeded at a density of 80,000 cells/well in a 24-well plate and maintained in DMEM (Hyclone) supplemented with 10% fetal bovine serum, 100 µg/mL streptomycin, 100 U/mL penicillin (Invitrogen, Carlsbad, CA, USA) at 37 degrees Celsius, 5% CO2 for 24 h. The cells were transiently transfected in individual wells using Polyethylenimine (PEI) (Polysciences, Inc., Warrington, PA, USA) according to the manufacturer's protocol. The cells in each well received 250 ng of an LXRE-luciferase reporter gene, 50 ng of CMX-h-LXRα (an expression vector for human LXRα), 50 ng of pSG5-human RXRα (an expression vector for human RXRα), and 20 ng of Renilla control plasmid was used along with 1.25 µL of PEI reagent. After 22-24 h of transfection, the cells were treated with either vehicle control ethanol, reference compound bexarotene (100 nM) alone, or in combination with 100 nM T0901317 (an LXR ligand), or 100 nM of the indicated bexarotene analog either alone or in combination with T0901317, as indicated. All compounds were solubilized in ethanol. After 24 h of treatment, the cells were lysed in 1X passive lysis buffer (Promega, Madison, WI USA) and the amount of reporter gene product (luciferase) was quantified using the Dual-Luciferase Reporter Assay System based on the manufacturer's protocol (Promega) in a Sirius FB12 luminometer (Berthold Detection Systems, Pforzheim, Germany). Luminescence resulting from the inducible firefly luciferase was divided by luminescence from the constitutively expressed Renilla luciferase in order to normalize for transfection efficacy, cell death, and cellular toxicity from ligand exposure. The data are a compilation of between six to eight independent assays with each treatment group dosed in triplicate for each independent assay. The LXRE-directed transcriptional activation of the reporter gene was measured in comparison to the reference compound bexarotene (1) set to 100%. Error bars on all graphs indicate the standard deviation of the replicate experiments. RARE assay. Human embryonic kidney cells (HEK293) were plated at 60,000 cells per well in a 24-well plate and maintained as described above. After 22-24 h, the cells were transiently transfected with 250 ng pTK-DR5(X2)-Luc, 25 ng pSG5-human RXRα, and 20 ng of Renilla control plasmid using 1.25 µL polyethylenimine (PEI) per well for 24 h. The sequence of the double DR5 RARE is: 5'-AAAGGTCACCGAAAGGTCACCATCCCGGG AGGTCACCGAAAGGTCACC-3' (DR5 responsive elements underlined). After 22-24 h of transfection, the cells were treated with ethanol vehicle (0.1%), all-trans-retinoic acid (ATRA, the endogenous ligand for RAR), or the indicated rexinoid analog at a final concentration of 10 nM. After 24 h of treatment, the cells were lysed and the retinoid activity was measured as described above (dual luciferase assay). The activity of compound 1 (or analog) divided by the activity of ATRA (expressed as a percentage) represents the RARE activity. The data (Table 1) are a compilation of between three to four independent assays with each treatment group dosed in triplicate for each independent experiment. The value for the positive control ATRA was set to 100%.
Data analysis. Statistical analysis was performed using Microsoft Excel (Microsoft, Redmond, WA, USA) software. t-tests were performed, as appropriate. All error bars represent the standard deviation. For Figures 6-8, data are expressed as means ± SD. Statistical differences between two groups (generally the bexarotene (1) control group versus bexarotene analog group) were determined by a two-sided Student's t-test. A p-value of less than or equal to 0.05 was considered significant.
Mutagenicity and Toxicity Assay. Mutagenicity and toxicity were assessed in a eukaryotic Saccharomyces cerevisiae model as described previously [76]. Each compound was solubilized in DMSO at increasing concentrations. D7 S. cerevisiae indicator cells were incubated with the compounds for 3 h before plating on selective media or YPD. Growth on plates was used to determine mutagenicity and cytotoxicity. Growth of colonies on the full nutrient YPD plate for each treatment was compared to the DMSO only control. Eleven micrograms per microliter was the highest concentration tested.
X-ray Data Collection, Structure Solution and Refinement. A colorless crystal of indicated dimensions was mounted on a glass fiber and transferred to a Bruker SMART APEX II diffractometer system. The APEX2 (APEX2 Version 2014.11-0, Bruker AXS, Inc.; Madison, WI 2014 USA) program package was used to determine the unit-cell parameters and for data collection (60 sec/frame scan time). The raw frame data were processed using SAINT (SAINT Version 8.34a, Bruker AXS, Inc.; Madison, WI 2013) and SADABS (Sheldrick, G.M. SADABS, Version 2014/5, Bruker AXS, Inc.; Madison, WI 2014 USA) to yield the reflection data file. Subsequent calculations were carried out using the SHELXTL (Sheldrick, G.M. SHELXTL, Version 2014/7, Bruker AXS, Inc.; Madison, WI 2014 USA) program package. For compound 26, the diffraction symmetry was 2/m and the systematic absences were consistent with the monoclinic space group P2 1 /n that was later determined to be correct. The structure for 26 was solved by direct methods and refined on F 2 by full-matrix least-squares techniques, and the analytical scattering factors [81] for neutral atoms were used throughout the analysis. Hydrogen atoms in 26, except those associated with C(14), were located from a difference-Fourier map and refined (x,y,z and U iso ), and H(14A), H(14B), and H(14C) were included using a riding model. Least-squares analysis for 26 yielded wR2 = 0.1064 and Goof = 1.025 for 328 variables refined against 3880 data (0.80 Å), R1 = 0.0426 for those 3293 data with I > 2.0σ(I). For compound 41, the diffraction symmetry was 2/m and the systematic absences were consistent with the monoclinic space groups Cc and C2/c, and it was later determined that space group Cc was correct. The structure for 41 was solved by direct methods and refined on F 2 by full-matrix least-squares techniques, and again, the analytical scattering factors for neutral atoms were used throughout the analysis. Hydrogen atoms in 41 were located from a difference-Fourier map and refined (x,y,z and U iso ), and there was one water solvent molecule present. Least-squares analysis for 41 yielded wR2 = 0.0792 and Goof = 1.022 for 378 variables refined against 5116 data (0.73 Å), R1 = 0.0322 for those 4861 data with I > 2.0σ(I), and the absolute structure could not be assigned by refinement of the Flack parameter [82].