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    • The nitrophenols b d were prepared as

    2020-03-11

    The nitrophenols 34b–d were prepared as described in Scheme 3b. Nitration of phenols 39b–d with 1equiv of sodium nitrate in the presence of hydrochloric A 804598 mg gave an inseparable mixture of 34b–d and 40b–d (1:1). This synthetic problem was successfully avoided as described below. Nitration of 39b–d with 2equiv of sodium nitrate afforded a separable mixture of 34b–d and 41b–d (1:1) because preferential nitration of the byproducts 40b–d gave dinitro compounds 41b–d. Synthesis of 11 is described in Scheme 4. O-Protection of 2-aminonaphthol 42 as TBS ether provided a TBS ether 43. N-Sulfonylation of 43 with 5-methylfuran-2-sulfonyl chloride afforded a sulfonamide 44, N-alkylation of which with isobutanol under Mitsunobu reaction conditions provided 45. Deprotection of TBS ether afforded 46. O-Alkylation of 46 with methyl 4-(bromomethyl)benzoate gave 47, alkaline hydrolysis of which resulted in 11.
    Results and discussion Further optimization of the A 804598 mg carboxylic acid analogs was carried out because of their less potent P450 enzyme inhibition. Table 3 shows the effect of substituting the benzoic acid moiety on activity profiles. 2-Chlorobenzoic acid, 3-chlorobenzoic acid, 3-methylbenzoic acid, and 3,5-dimethylbenzoic acid analogs 3, 4, 5, and 6 were tested for their receptor affinities and were found to be less potent than 1. They were also tested for their antagonist activities. Predictably, compound 3 had nearly 15-fold less potent activity than 1, because of the presumed masking effect of hydrophilic carboxylic acid function by the hydrophobic 2-chloro substituent, whereas 3- and/or 5-substituted benzoic acid analogs 4–6 without such a masking effect had equipotent antagonist activity with 1 regardless of their reduced receptor affinities. As reported in our previous paper, the aminophenoxy moiety showed a tendency to prefer more hydrophobic substituents. Based on the information, 5-methyl analog 7 and 4,5-disubstituted analogs 8–13 were synthesized and evaluated. Table 4 shows the effect of substituting the aminophenoxy moiety on activity profiles. Replacement of the trifluoromethyl residue of 1 with a methyl residue afforded 7, which had a 3.5-fold less potent receptor affinity and a 3-fold less potent antagonist activity. Introduction of another methyl residue into position 4 of the 2-aminophenoxy moiety of7 produced 8, which had a slightly more potent receptor affinity and a nearly 8-fold more potent antagonist activity. Indane analog 9 had nearly 3-fold less potent receptor affinity relative to 8, but it had equipotent antagonist activity. Tetrahydronaphthalene analog 10 had slightly less potent activity relative to 9 with respect to both receptor affinity and antagonist activity. Naphthalene analog 11 had an increased receptor affinity relative to 10, although it had a reduced antagonist activity. Introduction of another methyl residue into position 3 of the benzoic acid residue of 8 afforded 12, which had a reduced receptor affinity but a similar antagonist activity. Introduction of another methyl residue into position 3 of the benzoic acid moiety of9 produced13, which had a reduced receptor affinity but a nearly equipotent antagonist activity. Table 5 shows the structure–activity relationships (SAR) of N-thiazole-2-sulfonyl analogs 14–18, because N-thiazole-2-sulfonyl residue is one of the optimized heteroaryl sulfonyl residues as reported previously.N-Thiazole-2-sulfonyl analogs 14–18 had equipotent to slightly more potent antagonist activity compared with their corresponding N-5-methylfuran-2-sulfonyl analogs 1, 8–9, and 12–13, respectively, whereas their EP1 receptor affinities were not always consistent with the potency of their functional activities. In particular, N-thiazole-2-sulfonyl analogs 16–18 did not show increased functional activities in tandem with their increases in EP1 receptor affinities relative to their corresponding N-5-methylfuran-2-sulfonyl analogs 9 and 12 and 13.