Recent Developments in the Synthesis of HIV-1 Integrase Strand Transfer Inhibitors Incorporating Pyridine Moiety

Human immunodeficiency virus (HIV) causes one of the most dangerous diseases—acquired immunodeficiency syndrome (AIDS). An estimated about 40 million people are currently living with HIV worldwide, most of whom are already on antiretroviral therapy. This makes the development of effective drugs to combat this virus very relevant. Currently, one of the dynamically developing areas of organic and medicinal chemistry is the synthesis and identification of new compounds capable of inhibiting HIV-1 integrase—one of the HIV enzymes. A significant number of studies on this topic are published annually. Many compounds inhibiting integrase incorporate pyridine core. Therefore, this review is an analysis of the literature on the methods for the synthesis of pyridine-containing HIV-1 integrase inhibitors since 2003 to the present.


Introduction
The human immunodeficiency virus (HIV) causes one of the most fatal diseases-acquired immunodeficiency syndrome (AIDS). The high growth rate in the number of HIV-infected people makes the development of effective drugs to combat this virus very relevant. An extremely important and promising task of modern virology and medicinal chemistry is also the creation of compounds that do not cause the emergence of resistant strains of HIV-1 and/or have inhibitory activity against them. Currently, the main approach to the treatment of HIV infection is antiretroviral therapy (ARVT), which consists of the continuous intake of several antiviral drugs. ARVT can significantly improve the quality and increase the life expectancy of the patient. About 35 drugs are used to treat HIV infection-inhibitors of one of the three HIV enzymes (reverse transcriptase, protease, and integrase). One of the limitations of the use of ARVT is the formation of resistant forms of the virus during therapy, and, therefore, the field of chemistry associated with the synthesis of novel anti-HIV molecules continues to be in demand and relevant.
There are two major types of HIV (HIV-1 and HIV-2), which in turn consist of several groups and subtypes. HIV-1 is more virulent and transmissible than HIV-2, and most of the undertaken efforts have thus been targeted at developing inhibitors of HIV-1 enzymes. In particular, HIV-1 integrase strand transfer inhibitors (INIs) are being designed to block the action of integrase, an enzyme that inserts the viral genome into the DNA of the host cell-one of the most important steps in retroviral replication. To date five HIV-1 integrase inhibitors have been approved: Raltegravir (RAL, approved by the FDA in 2007), Elvitegravir (EVG, 2012), Dolutegravir (DTG, 2013), Bictegravir (BIC, 2018), and Cabotegravir (2021) (see Figure 1). It should be noted that four of them contain a pyridine moiety, thus emphasizing the importance of pyridine derivatives as INIs.
The first INI-Raltegravir was approved for use as a new agent for AIDS therapy in 2007 [1], but it was noticed that in some cases, the virus develops resistance to this new drug within 3 months [2]. The design of novel HIV-1 INIs is based generally on the modification of structure of these five well-established drugs, i.e., the central heterocyclic The first INI-Raltegravir was approved for use as a new agent for AIDS therapy in 2007 [1], but it was noticed that in some cases, the virus develops resistance to this new drug within 3 months [2]. The design of novel HIV-1 INIs is based generally on the modification of structure of these five well-established drugs, i.e., the central heterocyclic fragment usually incorporate a pyridine, pyrimidine, or quinoline system. In addition, compounds of some other classes are also being studied, such as indoles, isoindoles, acyclic 2,4-diketoacids, etc. A number of review articles devoted to the current use of INIs as well as discussion of their structural diversity have been published recently [3][4][5][6][7][8][9][10]. At the same time, lack of attention in the review literature has been paid to the chemical synthesis of pyridine-containing INIs. Some information can be found in two publications [11,12]. This review is an analysis of the literature on methods for the synthesis of HIV-1 integrase inhibitors of pyridine and the fused pyridine series covering the period from 2003 to the present. For convenience, the considered compounds of different structures are grouped into separate subsections: monocyclic pyridines, benzoannulated pyridines (quinolines and isoquinolines), and pyridines fused with heterocycles.

Monocyclic Pyridines
Most of the publications dealt with HIV-1 INIs over past 20 years are dedicated to development of more efficient syntheses of approved drugs and their structural analogs. Nevertheless, some monocyclic pyridine derivatives have been designed and tested as well. Thus, a new series of pyridoxine hydroxamic acids were synthesized and their antiviral properties were evaluated [13]. The authors studied a large set of pyridines with various spacers X-Y and aryl groups in position 5, Scheme 1. The structural diversity was achieved by common functional group interconversion reactions of 5-hydroxymethyl derivative 1, such as oxidation to aldehyde or carboxylic acid, conversion of the alcohol to mesylate, or halomethyl derivatives, etc. Cleavage of the acetone protection in 2 and conversion of an ester into hydroxamic acid gave target compounds 3. It was found that antiviral potency depends on the structure of spacer X-Y and substituents in the aryl group. The best results were observed in case of X − Y = NH-CH2; NH-C(O); O-CH2 and

Monocyclic Pyridines
Most of the publications dealt with HIV-1 INIs over past 20 years are dedicated to development of more efficient syntheses of approved drugs and their structural analogs. Nevertheless, some monocyclic pyridine derivatives have been designed and tested as well. Thus, a new series of pyridoxine hydroxamic acids were synthesized and their antiviral properties were evaluated [13]. The authors studied a large set of pyridines with various spacers X-Y and aryl groups in position 5, Scheme 1. The structural diversity was achieved by common functional group interconversion reactions of 5-hydroxymethyl derivative 1, such as oxidation to aldehyde or carboxylic acid, conversion of the alcohol to mesylate, or halomethyl derivatives, etc. Cleavage of the acetone protection in 2 and conversion of an ester into hydroxamic acid gave target compounds 3. It was found that antiviral potency depends on the structure of spacer X-Y and substituents in the aryl group. The best results were observed in case of X − Y = NH-CH 2 ; NH-C(O); O-CH 2 and Ar = 4-F-C 6 H 5 ; 3-Cl-4-F-C 6 H 4 ; 3,4-Cl 2 -C 6 H 4 .
Nair et al. reported on the discovery of a novel anti-HIV active INI possessing low toxicity and inhibition EC 50 value of 19-35 nM depending on the HIV subtype [14,15]. The multistep synthesis (Scheme 2) started with readily available pyridine and benzene derivatives and comprised lithiation of 5-bromo-2-methoxypyridine (4) followed by reaction with 2,6-difluorobenzaldehyde. Dehydroxylation and cleavage of methoxy protection in compound 5 afforded pyridine-2-one derivative 6 in 88% yield. Bromination and N-alkylation of a pyridine moiety gave an intermediate product 7 in 64% yield over two steps. The introduction of the acetyl group was achieved using Pd-catalyzed Stille cross-coupling with 1-ethoxyvinyl(tributyl)stannane followed by acidic work-up. Transformation of the acetyl group into diketoacid derivative 8 was performed in the usual manner via reaction with diethyl oxalate and successive acid-catalyzed hydrolysis. Finally, reaction of the acid 8 with 1-amino-2-pyrollidinone p-toluenesulfonate led to the target compound 9 with 68% yield.  [14,15]. The multistep synthesis (Scheme 2) started with readily available pyridine and benzene derivatives and comprised lithiation of 5-bromo-2-methoxypyridine (4) followed by reaction with 2,6-difluorobenzaldehyde. Dehydroxylation and cleavage of methoxy protection in compound 5 afforded pyridine-2-one derivative 6 in 88% yield. Bromination and N-alkylation of a pyridine moiety gave an intermediate product 7 in 64% yield over two steps. The introduction of the acetyl group was achieved using Pd-catalyzed Stille cross-coupling with 1-ethoxyvinyl(tributyl)stannane followed by acidic work-up. Transformation of the acetyl group into diketoacid derivative 8 was performed in the usual manner via reaction with diethyl oxalate and successive acid-catalyzed hydrolysis. Finally, reaction of the acid 8 with 1-amino-2-pyrollidinone p-toluenesulfonate led to the target compound 9 with 68% yield.  [14,15]. The multistep synthesis (Scheme 2) started with readily available pyridine and benzene derivatives and comprised lithiation of 5-bromo-2-methoxypyridine (4) followed by reaction with 2,6-difluorobenzaldehyde. Dehydroxylation and cleavage of methoxy protection in compound 5 afforded pyridine-2-one derivative 6 in 88% yield. Bromination and N-alkylation of a pyridine moiety gave an intermediate product 7 in 64% yield over two steps. The introduction of the acetyl group was achieved using Pd-catalyzed Stille cross-coupling with 1-ethoxyvinyl(tributyl)stannane followed by acidic work-up. Transformation of the acetyl group into diketoacid derivative 8 was performed in the usual manner via reaction with diethyl oxalate and successive acid-catalyzed hydrolysis. Finally, reaction of the acid 8 with 1-amino-2-pyrollidinone p-toluenesulfonate led to the target compound 9 with 68% yield. A similar synthetic scheme was applied for the preparation of β-diketo acid derivatives with 2,4-difluorobenzyl substituent in position 5 [16] and many other diversely substituted 1,5-dibenzylpyridinones [17].
2-Hydroxy-3-pyridylacrylic acid derivatives as novel HIV integrase inhibitors were synthesized on the basis of substituted 2-methylpyridines [18]. Reactions of compounds 10 with diethyl oxalate afforded 2-hydroxy-3-pyridylacrylic esters 11, which were hydrolyzed under the action of LiOH to give the corresponding acids 12 in moderate to high yields (Scheme 3). It was demonstrated that the position of substituent R in the hydrophobic domain as well as the nature of R provided useful information for the design of novel INI types.
Dual inhibitors of HIV reverse transcriptase and integrase were synthesized on the basis of pyridine-containing reverse transcriptase inhibitor Delavirdine [19]. The synthesis was accomplished starting with reactions of diversely substituted acetylindole-2-carboxylic acids 13 and 3-isopropylamino-2-(piperazyn-1-yl)-pyridine (14) in the presence of carbonyl diimidazole (CDI) to give corresponding amides 15 (Scheme 4). Further reactions with diethyl oxalate and basic hydrolysis of the esters 16 afforded target 2,4-diketoacids 17. Compounds bearing diketoacid functionality in position 5 of the indole system showed good activity against both enzymes and HIV in cell-based assays, while C-7 isomers were inactive.
2-Hydroxy-3-pyridylacrylic acid derivatives as novel HIV integrase inhibitors were synthesized on the basis of substituted 2-methylpyridines [18]. Reactions of compounds 10 with diethyl oxalate afforded 2-hydroxy-3-pyridylacrylic esters 11, which were hydrolyzed under the action of LiOH to give the corresponding acids 12 in moderate to high yields (Scheme 3). It was demonstrated that the position of substituent R in the hydrophobic domain as well as the nature of R provided useful information for the design of novel INI types. Scheme 3. Synthesis of 2-hydroxy-3-pyridylacrylic acid derivatives.
Dual inhibitors of HIV reverse transcriptase and integrase were synthesized on the basis of pyridine-containing reverse transcriptase inhibitor Delavirdine [19]. The synthesis was accomplished starting with reactions of diversely substituted acetylindole-2-carboxylic acids 13 and 3-isopropylamino-2-(piperazyn-1-yl)-pyridine (14) in the presence of carbonyl diimidazole (CDI) to give corresponding amides 15 (Scheme 4). Further reactions with diethyl oxalate and basic hydrolysis of the esters 16 afforded target 2,4-diketoacids 17. Compounds bearing diketoacid functionality in position 5 of the indole system showed good activity against both enzymes and HIV in cell-based assays, while C-7 isomers were inactive. Design, synthesis, and evaluation of novel small molecules inhibiting an interaction of HIV-1 integrase and Lens epithelium derived growth factor (LEDGF/p75) was reported by Van der Eycken et al. [20]. The substituted indoles 18 were sulfenylated with 3-mercaptobenzoic acid 19 under microwave irradiation conditions to give 3-arylthioderivatives 20 in high yields (Scheme 5). Reactions of the latter with alkoxyaminopyridines 21 in the presence of EDC hydrochloride and 1-hydroxy-7-azabenzotriazole  Dual inhibitors of HIV reverse transcriptase and integrase were synthesized on the basis of pyridine-containing reverse transcriptase inhibitor Delavirdine [19]. The synthesis was accomplished starting with reactions of diversely substituted acetylindole-2-carboxylic acids 13 and 3-isopropylamino-2-(piperazyn-1-yl)-pyridine (14) in the presence of carbonyl diimidazole (CDI) to give corresponding amides 15 (Scheme 4). Further reactions with diethyl oxalate and basic hydrolysis of the esters 16 afforded target 2,4-diketoacids 17. Compounds bearing diketoacid functionality in position 5 of the indole system showed good activity against both enzymes and HIV in cell-based assays, while C-7 isomers were inactive. Design, synthesis, and evaluation of novel small molecules inhibiting an interaction of HIV-1 integrase and Lens epithelium derived growth factor (LEDGF/p75) was reported by Van der Eycken et al. [20]. The substituted indoles 18 were sulfenylated with 3-mercaptobenzoic acid 19 under microwave irradiation conditions to give 3-arylthioderivatives 20 in high yields (Scheme 5). Reactions of the latter with alkoxyaminopyridines 21 in the presence of EDC hydrochloride and 1-hydroxy-7-azabenzotriazole Design, synthesis, and evaluation of novel small molecules inhibiting an interaction of HIV-1 integrase and Lens epithelium derived growth factor (LEDGF/p75) was reported by Van der Eycken et al. [20]. The substituted indoles 18 were sulfenylated with 3-mercaptobenzoic acid 19 under microwave irradiation conditions to give 3-arylthioderivatives 20 in high yields (Scheme 5). Reactions of the latter with alkoxyaminopyridines 21 in the presence of EDC hydrochloride and 1-hydroxy-7-azabenzotriazole (HOAt), also under microwave irradiation, afforded target amides 22 in moderate isolated yields. The inhibiting activity was found to be dependent on both R 1 and R 2 substituents: 5-chloroindoles were inactive, while 2-isopropyloxypyridine derivatives demonstrated higher activity in comparison with 2-methoxy and 2-butyloxy compounds. Novel integrase-LEDGF/p75 allosteric inhibitors based on pyridine scaffold were discovered by Sugiyama and coworkers, Scheme 6. [21]. This multistep synthesis provided a series of 5-aryl-3,6-dimethylpyridines 23-25 with various functions in position 2 on the basis of simple pyran-2-one. The authors successfully used Pd-catalyzed cross-coupling reactions to introduce aryl and amine fragments via corresponding trifluoromethanesulfonates. Substituents with intramolecular hydrogen bond at C-2, such as urea derivatives 25, are desirable for increasing antiviral activity. These compounds were obtained from 2-aminopyridines 26 by the reaction with isocyanates. Novel integrase-LEDGF/p75 allosteric inhibitors based on pyridine scaffold were discovered by Sugiyama and coworkers, Scheme 6. [21]. This multistep synthesis provided a series of 5-aryl-3,6-dimethylpyridines 23-25 with various functions in position 2 on the basis of simple pyran-2-one. The authors successfully used Pd-catalyzed cross-coupling reactions to introduce aryl and amine fragments via corresponding trifluoromethanesulfonates. Substituents with intramolecular hydrogen bond at C-2, such as urea derivatives 25, are desirable for increasing antiviral activity. These compounds were obtained from 2-aminopyridines 26 by the reaction with isocyanates. Novel integrase-LEDGF/p75 allosteric inhibitors based on pyridine scaffold were discovered by Sugiyama and coworkers, Scheme 6. [21]. This multistep synthesis provided a series of 5-aryl-3,6-dimethylpyridines 23-25 with various functions in position 2 on the basis of simple pyran-2-one. The authors successfully used Pd-catalyzed cross-coupling reactions to introduce aryl and amine fragments via corresponding trifluoromethanesulfonates. Substituents with intramolecular hydrogen bond at C-2, such as urea derivatives 25, are desirable for increasing antiviral activity. These compounds were obtained from 2-aminopyridines 26 by the reaction with isocyanates. Scheme 6. Sugiyama's approach to novel integrase-LEDGF/p75 allosteric inhibitors.
A series of pyridine-based allosteric INIs have been synthesized recently by Naidu et al. [22]. The authors proposed an elegant reaction sequence starting with 4-hydroxy-2,6-dimethylpyridine (27) (Scheme 7). It was subjected to dibromination followed by the conversion of hydroxyl to chlorine under the action of POCl3 to give intermediate 28. One of the bromine atoms was then replaced with 1,2-dicarbonyl frag-Scheme 6. Sugiyama's approach to novel integrase-LEDGF/p75 allosteric inhibitors.
A series of pyridine-based allosteric INIs have been synthesized recently by Naidu et al. [22]. The authors proposed an elegant reaction sequence starting with 4-hydroxy-2,6-dimethyl pyridine (27) (Scheme 7). It was subjected to dibromination followed by the conversion of hydroxyl to chlorine under the action of POCl 3 to give intermediate 28. One of the bromine atoms was then replaced with 1,2-dicarbonyl fragment, and 4-Cl was substituted with 4,4-dimethylpiperidine. Further asymmetric reduction of the carbonyl group in compound 29 gave the corresponding alcohols 30, which, after protection, were involved in Suzuki-Miyaura cross-coupling with various arylboronic acids and ester hydrolysis. Finally, some functional group interconversions were made to extend the raw of target compounds 31. One of the synthesized compounds (X = 4-F-C 6 H 4 CH 2 CH 2 O) was selected as the preclinical lead based on its promising antiviral potency, but multidose toxicity studies in rats revealed adverse results, which caused discontinuation of the further development.
Carbamoyl pyridone chelating scaffold was designed in 2012 [23]. It was considered as an advanced two-metal binding pharmacophore that demonstrates high activity in both enzymatic and antiviral assay formats. 4-Hydroxy-6-methylnicotinic acid (32) was brominated and converted to 4-F-benzylamide 33 using HOBT and EDC (Scheme 8). The Bromine atom was then replaced with NaOMe and the benzyloxy group was introduced through a Mitsunobu reaction with benzyl alcohol, yielding compound 34. The 2-Methyl group of 34 was converted to methoxycarbonyl via subsequent formation of pyridine-Noxide, its reaction with Ac 2 O to give 2-hydroxymethyl compound, its oxidation to aldehyde, and further to methyl ester. Thus, the key intermediate 35 was synthesized and used for the preparation of various primary and secondary amides 36 and 37. Although none of the synthesized compounds showed necessary potency against key resistant mutants, the authors positioned their study as an attractive starting point for further research. Some other 3-hydroxy-5-carbamoylpyridin-4-ones were patented as HIV-1 INIs [24]. ment, and 4-Cl was substituted with 4,4-dimethylpiperidine. Further asymmetric reduction of the carbonyl group in compound 29 gave the corresponding alcohols 30, which, after protection, were involved in Suzuki-Miyaura cross-coupling with various arylboronic acids and ester hydrolysis. Finally, some functional group interconversions were made to extend the raw of target compounds 31. One of the synthesized compounds (X = 4-F-C6H4CH2CH2O) was selected as the preclinical lead based on its promising antiviral potency, but multidose toxicity studies in rats revealed adverse results, which caused discontinuation of the further development.

Scheme 7. Synthetic route to pyridine-based allosteric INIs 31.
Carbamoyl pyridone chelating scaffold was designed in 2012 [23]. It was considered as an advanced two-metal binding pharmacophore that demonstrates high activity in both enzymatic and antiviral assay formats. 4-Hydroxy-6-methylnicotinic acid (32) was brominated and converted to 4-F-benzylamide 33 using HOBT and EDC (Scheme 8). The Bromine atom was then replaced with NaOMe and the benzyloxy group was introduced through a Mitsunobu reaction with benzyl alcohol, yielding compound 34. The 2-Methyl group of 34 was converted to methoxycarbonyl via subsequent formation of pyridine-N-oxide, its reaction with Ac2O to give 2-hydroxymethyl compound, its oxidation to aldehyde, and further to methyl ester. Thus, the key intermediate 35 was synthesized and used for the preparation of various primary and secondary amides 36 and 37. Although none of the synthesized compounds showed necessary potency against key resistant mutants, the authors positioned their study as an attractive starting point for further research. Some other 3-hydroxy-5-carbamoylpyridin-4-ones were patented as HIV-1 INIs [24]. Substituted 3-hydroxypyridine-4-ones were synthesized on the basis of kojic acid and tested as potential HIV-1 INIs, Scheme 9 [25]. The reaction of kojic acid (38) with BnBr in basic media followed by interaction with amine afforded 2-hydroxymethylpyridin-4-ones 39, which then were oxidized to the corresponding aldehydes using MnO2 and condensed with arylamines to give Shiff bases 40. On hydrogenation of the latter, the benzyl group was cleaved, accompanied by the reduction of the C=N double bond. The Shiff bases 40 exhibited higher anti-HIV activities than their hydrogenation products 41-IC50 65-100 μM and 90-1000 μM, respectively. Substituted 3-hydroxypyridine-4-ones were synthesized on the basis of kojic acid and tested as potential HIV-1 INIs, Scheme 9 [25]. The reaction of kojic acid (38) with BnBr in basic media followed by interaction with amine afforded 2-hydroxymethylpyridin-4-ones 39, which then were oxidized to the corresponding aldehydes using MnO 2 and condensed with arylamines to give Shiff bases 40. On hydrogenation of the latter, the benzyl group was cleaved, accompanied by the reduction of the C=N double bond. The Shiff bases 40 exhibited higher anti-HIV activities than their hydrogenation products 41-IC 50 65-100 µM and 90-1000 µM, respectively. Substituted 3-hydroxypyridine-4-ones were synthesized on the basis of kojic acid and tested as potential HIV-1 INIs, Scheme 9 [25]. The reaction of kojic acid (38) with BnBr in basic media followed by interaction with amine afforded 2-hydroxymethylpyridin-4-ones 39, which then were oxidized to the corresponding aldehydes using MnO2 and condensed with arylamines to give Shiff bases 40. On hydrogenation of the latter, the benzyl group was cleaved, accompanied by the reduction of the C=N double bond. The Shiff bases 40 exhibited higher anti-HIV activities than their hydrogenation products 41-IC50 65-100 μM and 90-1000 μM, respectively. Scheme 9. Approach to 3-hydroxypyridine-4-ones.
Another example of 3-hydroxypyridin-4-one synthesis was reported by Sirous et al., Scheme 10 [26]. 3-Hydroxy group of the commercially available maltol (42) was protected by the reaction with benzyl bromide and further reactions with benzyl-or phenetylamines gave 1-substituted pyridine-4-ones 43. Cleavage of the benzyl group was carried out using boron tribromide or a mixture of hydrochloric and acetic acids. The target 3-OH derivatives 44 demonstrated lower activities with respect to the correspondingly substituted pyran-4-one compounds, which represent a valuable scaffold for developing efficient INIs.

Quinolines and Isoquinolines
Elvitegravir (EVG, GS9137) is one of the famous quinoline containing drugs used in anti-HIV 1 therapy. It was developed by the Gilead Sciences, which in 2008 licensed EVG from Japan Tobacco [27]. The synthetic route for the preparation of this compound was described in patent [28] (Scheme 11). It comprised the reaction of 5-bromo-2,4-dimethoxybenzoic acid (45) with 2-chloro-3-fluorobenzaldehyde (46) followed by dehydroxylation and formation of imidazolide 47. In the next step, -ketoester functionality was introduced and reaction with DMADMF afforded the corresponding enamine 48. The quinoline skeleton was constructed in a further 3 steps: reaction with L-valinol, N,O-bis-(trimethylsilyl)acetamide, and potassium hydroxide.

Quinolines and Isoquinolines
Elvitegravir (EVG, GS9137) is one of the famous quinoline containing drugs used in anti-HIV 1 therapy. It was developed by the Gilead Sciences, which in 2008 licensed EVG from Japan Tobacco [27]. The synthetic route for the preparation of this compound was described in patent [28] (Scheme 11). It comprised the reaction of 5-bromo-2,4dimethoxybenzoic acid (45) with 2-chloro-3-fluorobenzaldehyde (46) followed by dehydroxylation and formation of imidazolide 47. In the next step, β-ketoester functionality was introduced and reaction with DMADMF afforded the corresponding enamine 48. The quinoline skeleton was constructed in a further 3 steps: reaction with L-valinol, N,O-bis-(trimethylsilyl)acetamide, and potassium hydroxide.
The invention of Elvitegravir stimulated the development of synthetic approaches, leading to structurally similar quinoline compounds and the study of their activity toward HIV-1 integrase.
A series of novel pyrazolyl-4-oxo-4H-quinoline-3-carboxylic acids bearing various substituents on the N-position of quinoline ring that are structural analogs of EVG were designed and synthesized by Hu et al. [29]. 4-Substituted 3,5-dimethylpyrazoles 49 react with p-NO 2 -benzyl bromide (50) followed by reduction of the nitro group and the introduction of methylenemalonate fragment, giving rise to the corresponding enamines 51, (Scheme 12), which on heating in diphenyl ether gave 4-quinolone compounds 52. Quinolones 52 were N-alkylated by various alkyl halides to give derivatives 53, and after basic or acidic hydrolysis, the target compounds 54 were obtained. However, shuffling of pharamacophore fragments at N(1) and R 1 did not lead to any obvious inhibitory activity.
Patil et al. reported on docking and synthesis of 6-fluoro-4-quinolone-3-carboxylic acids as potential HIV-1 INIs [30,31]. The target compounds synthesized via simple twostep procedure (Scheme 13). Reaction of 7-chloro-6-fluoroquinolone-3-carboxylates 55 with N-substituted piperazines 56 afforded chlorine-substitution products 57 in moderate yields. Hydrolysis of ester bonds with LiOH gave target compounds 58, which were evaluated for their enzymatic activity against HIV-1. Some of the synthesized compounds exhibited moderate to good anti-HIV-1 integrase inhibitory activity in comparison with the reference drugs.
Elvitegravir (EVG, GS9137) is one of the famous quinoline containing drugs used in anti-HIV 1 therapy. It was developed by the Gilead Sciences, which in 2008 licensed EVG from Japan Tobacco [27]. The synthetic route for the preparation of this compound was described in patent [28] (Scheme 11). It comprised the reaction of 5-bromo-2,4-dimethoxybenzoic acid (45) with 2-chloro-3-fluorobenzaldehyde (46) followed by dehydroxylation and formation of imidazolide 47. In the next step, -ketoester functionality was introduced and reaction with DMADMF afforded the corresponding enamine 48. The quinoline skeleton was constructed in a further 3 steps: reaction with L-valinol, N,O-bis-(trimethylsilyl)acetamide, and potassium hydroxide.
The invention of Elvitegravir stimulated the development of synthetic approaches, leading to structurally similar quinoline compounds and the study of their activity toward HIV-1 integrase.
A series of novel pyrazolyl-4-oxo-4H-quinoline-3-carboxylic acids bearing various substituents on the N-position of quinoline ring that are structural analogs of EVG were designed and synthesized by Hu et.al [29]. 4-Substituted 3,5-dimethylpyrazoles 49 react with p-NO2-benzyl bromide (50) followed by reduction of the nitro group and the introduction of methylenemalonate fragment, giving rise to the corresponding enamines 51, (Scheme 12), which on heating in diphenyl ether gave 4-quinolone compounds 52. Quinolones 52 were N-alkylated by various alkyl halides to give derivatives 53, and after basic or acidic hydrolysis, the target compounds 54 were obtained. However, shuffling of pharamacophore fragments at N(1) and R 1 did not lead to any obvious inhibitory activity. Patil et al. reported on docking and synthesis of 6-fluoro-4-quinolone-3-carboxylic acids as potential HIV-1 INIs [30,31]. The target compounds synthesized via simple two-step procedure (Scheme 13). Reaction of 7-chloro-6-fluoroquinolone-3-carboxylates 55 with N-substituted piperazines 56 afforded chlorine-substitution products 57 in moderate yields. Hydrolysis of ester bonds with LiOH gave target compounds 58, which were evaluated for their enzymatic activity against HIV-1. Some of the synthesized compounds exhibited moderate to good anti-HIV-1 integrase inhibitory activity in comparison with the reference drugs. Patil et al. reported on docking and synthesis of 6-fluoro-4-quinolone-3-carboxylic acids as potential HIV-1 INIs [30,31]. The target compounds synthesized via simple two-step procedure (Scheme 13). Reaction of 7-chloro-6-fluoroquinolone-3-carboxylates 55 with N-substituted piperazines 56 afforded chlorine-substitution products 57 in moderate yields. Hydrolysis of ester bonds with LiOH gave target compounds 58, which were evaluated for their enzymatic activity against HIV-1. Some of the synthesized compounds exhibited moderate to good anti-HIV-1 integrase inhibitory activity in comparison with the reference drugs. Chen's group reported on the synthesis of some novel 5-R-quinolone carboxylic acids-structural analogs of Elvitegravir [32,33]. The target compounds were obtained according to classical synthetic route for assembling quinoline skeleton as outlined on Scheme 14. Negishi coupling of methyl 2,6-difluoro-3-iodobenzoate (59) and 3-chloro-2-fluorobenzyl bromide (60) followed by ester hydrolysis afforded highly functionalized intermediate 61. Carboxylic acid was then converted to -ketoester 62 and reacted with DMADMF to give the enamine 63-a precursor of the quinoline ring system. The pyridine ring was annulated after reaction with aryl-or benzylamine and treatment with K2CO3. All synthesized compounds 64 showed significant inhibition activity in low Chen's group reported on the synthesis of some novel 5-R-quinolone carboxylic acids-structural analogs of Elvitegravir [32,33]. The target compounds were obtained according to classical synthetic route for assembling quinoline skeleton as outlined on Scheme 14. Negishi coupling of methyl 2,6-difluoro-3-iodobenzoate (59) and 3-chloro-2fluorobenzyl bromide (60) followed by ester hydrolysis afforded highly functionalized intermediate 61. Carboxylic acid was then converted to β-ketoester 62 and reacted with DMADMF to give the enamine 63-a precursor of the quinoline ring system. The pyridine ring was annulated after reaction with aryl-or benzylamine and treatment with K 2 CO 3 . All synthesized compounds 64 showed significant inhibition activity in low micromolar concentration range. In addition, the author revealed influence of N-substituent on inhibition (IC 50 ) and antiviral activity (EC 50 ). Some other structurally similar 6-benzylquinolone-3carboxylic acids were reported in [34]. In 2015, a method for the synthesis of new tetrahydro-1H-[1,4]oxazino [3,2-g]quinoline derivatives was patented [36]. The quite simple synthetic sequence starts from 2-amino-5nitrophenol 72 as raw material and comprises successive N-acetylation, oxazine ring closure, and the introduction of benzyl group to give intermediate 73 (Scheme 16). Reduction of the nitro group and a further Gould-Jacobs reaction with diethyl ethoxymethylenemalonate afforded quinoline 74, which on alkylation and ester hydrolysis yielded fused quinolines 75. All compounds have a certain inhibitory effect on HIV-1 integrase with IC 50 less than 500 nM. An efficient multi-kilo scale synthesis of quinoline based HIV-1 INI was accomplished by Fandrick et al. [39,40]. The molecule consists of two quinoline-based parts coupled together using Suzuki-Miyaura conditions (Scheme 18). For the synthesis of the first fragment, 4-hydroxy-2-methylquinoline 80 was used as starting compound. Its iodination with NIS and reaction with POCl3 gave iodide 81 in 63% overall yield. Acylation of 81 with methyl oxalyl chloride and asymmetric reduction of ketoester 82 provided compound 83 with excellent enantiopurity. The second structural unit was synthesized on the basis of 2-bromo-5-methoxyaniline 84. It was acylated with unsaturated anhydride 85 and cyclized under the action of sulfuric acid to compound 86. A further reaction sequence of reduction, chloro-dehydroxylation, and dechlorination afforded bromide 87, which then was converted to the corresponding boronic acid 88 in 80% yield. Assembly of the target molecule skeleton was carried out by Suzuki-Miyaura cross-coupling of compounds 83 and 88. Product 89 was O-tert-butylated and hydrolyzed to give compound 90 in 93% yield and high stereoselectivity. This protocol was patented in 2014 [41]. An efficient multi-kilo scale synthesis of quinoline based HIV-1 INI was accomplished by Fandrick et al. [39,40]. The molecule consists of two quinoline-based parts coupled together using Suzuki-Miyaura conditions (Scheme 18). For the synthesis of the first fragment, 4-hydroxy-2-methylquinoline 80 was used as starting compound. Its iodination with NIS and reaction with POCl3 gave iodide 81 in 63% overall yield. Acylation of 81 with methyl oxalyl chloride and asymmetric reduction of ketoester 82 provided compound 83 with excellent enantiopurity. The second structural unit was synthesized on the basis of 2-bromo-5-methoxyaniline 84. It was acylated with unsaturated anhydride 85 and cyclized under the action of sulfuric acid to compound 86. A further reaction sequence of reduction, chloro-dehydroxylation, and dechlorination afforded bromide 87, which then was converted to the corresponding boronic acid 88 in 80% yield. Assembly of the target molecule skeleton was carried out by Suzuki-Miyaura cross-coupling of compounds 83 and 88. Product 89 was O-tert-butylated and hydrolyzed to give compound 90 in 93% yield and high stereoselectivity. This protocol was patented in 2014 [41]. An efficient multi-kilo scale synthesis of quinoline based HIV-1 INI was accomplished by Fandrick et al. [39,40]. The molecule consists of two quinoline-based parts coupled together using Suzuki-Miyaura conditions (Scheme 18). For the synthesis of the first fragment, 4-hydroxy-2-methylquinoline 80 was used as starting compound. Its iodination with NIS and reaction with POCl 3 gave iodide 81 in 63% overall yield. Acylation of 81 with methyl oxalyl chloride and asymmetric reduction of ketoester 82 provided compound 83 with excellent enantiopurity. The second structural unit was synthesized on the basis of 2-bromo-5-methoxyaniline 84. It was acylated with unsaturated anhydride 85 and cyclized under the action of sulfuric acid to compound 86. A further reaction sequence of reduction, chloro-dehydroxylation, and dechlorination afforded bromide 87, which then was converted to the corresponding boronic acid 88 in 80% yield. Assembly of the target molecule skeleton was carried out by Suzuki-Miyaura cross-coupling of compounds 83 and 88. Product 89 was O-tert-butylated and hydrolyzed to give compound 90 in 93% yield and high stereoselectivity. This protocol was patented in 2014 [41].  [42]. The synthetic scheme is quite similar to the one mentioned above (Scheme 18), and it starts from commercially available 4-hydroxy-2-methyl-quinoline 80 that has undergone direct bromination and reaction with POCl3 to give intermediate 91 in 65% yield. It was then converted to α-hydroxyester 92 via acylation with methyl oxalyl chloride and reduction with NaBH4. Reaction of 92 with NaI followed by tert-butylation afforded 4-iodoquinoline 93, which reacted with a number of arylboronic acids to give compounds 94. Hydrolysis of esters 94 led to target carboxylic acids 95. This study has provided relevant information regarding the structure-activity relationship and defining factors for candidate INIs design. 4-Chlorophenyl and 2,3-benzo[b][1,4]dioxine derivatives showed the highest potency against HIV-1 integrase.

Scheme 19. An approach to 4-arylquinoline derivatives 95.
A six-step method for the synthesis of 2-quinolone derivatives using Morita-Baylis-Hillman methodology was developed by Sekgota et al. [43]. Substituted 2-nitrobenzaldehydes 96 reacted with methyl acrylate in the presence of DABCO to give MBH adducts 97 followed by reductive cyclization to quinolones 98 (Scheme 20). They, in turn, were converted to 3-chloromethyl compounds 99 and then to secondary amines 100. Acylation with benzoyl chloride provided amides 101.  [42]. The synthetic scheme is quite similar to the one mentioned above (Scheme 18), and it starts from commercially available 4-hydroxy-2-methyl-quinoline 80 that has undergone direct bromination and reaction with POCl3 to give intermediate 91 in 65% yield. It was then converted to α-hydroxyester 92 via acylation with methyl oxalyl chloride and reduction with NaBH4. Reaction of 92 with NaI followed by tert-butylation afforded 4-iodoquinoline 93, which reacted with a number of arylboronic acids to give compounds 94. Hydrolysis of esters 94 led to target carboxylic acids 95. This study has provided relevant information regarding the structure-activity relationship and defining factors for candidate INIs design. 4-Chlorophenyl and 2,3-benzo[b][1,4]dioxine derivatives showed the highest potency against HIV-1 integrase.

Scheme 19. An approach to 4-arylquinoline derivatives 95.
A six-step method for the synthesis of 2-quinolone derivatives using Morita-Baylis-Hillman methodology was developed by Sekgota et al. [43]. Substituted 2-nitrobenzaldehydes 96 reacted with methyl acrylate in the presence of DABCO to give MBH adducts 97 followed by reductive cyclization to quinolones 98 (Scheme 20). They, in turn, were converted to 3-chloromethyl compounds 99 and then to secondary amines 100. Acylation with benzoyl chloride provided amides 101.

Scheme 19. An approach to 4-arylquinoline derivatives 95.
A six-step method for the synthesis of 2-quinolone derivatives using Morita-Baylis-Hillman methodology was developed by Sekgota et al. [43]. Substituted 2-nitrobenzaldehydes 96 reacted with methyl acrylate in the presence of DABCO to give MBH adducts 97 followed by reductive cyclization to quinolones 98 (Scheme 20). They, in turn, were converted to 3-chloromethyl compounds 99 and then to secondary amines 100. Acylation with benzoyl chloride provided amides 101. Int Aromatic foldamers containing quinoline skeleton were proposed as HIV-1 INIs in 2018 [44]. The authors described the synthesis of several quinoline derivatives bearing phosphonate groups (Scheme 21). Phosphonate fragment was introduced into compounds 102 under Mitsunobu conditions and subsequent hydrogenation of 8-nitro-or 8-cyano derivatives 103 was accompanied with benzyl ester cleavage to give 8-amino-or 8-aminomethylquinolines 104, respectively. At the last step, Fmoc protective group was installed, affording the corresponding amides 105 in moderate yields.

Scheme 21. Synthesis of quinoline-based INIs bearing phosphonate groups.
In 2006 a microwave-assisted synthesis of fluoroquinolone ribonucleosides was described [45]. Reaction of fluoroanilines 106 with diethyl (ethoxymethylidene)malonate followed by ring closure gave fluoroquinolone derivatives 108 (Scheme 22). The target compounds 109 were obtained by coupling with 1,2,3,5-O-tetraacetyl-D-ribofuranose and deprotection of hydroxyl groups with NaOMe in MeOH. All fluoroquinolones were examined as HIV-1 INIs. Interestingly, synthesized nucleosides were found to be inactive in cell culture but demonstrated enzymatic inhibitory effect against HIV-1 integrase. Aromatic foldamers containing quinoline skeleton were proposed as HIV-1 INIs in 2018 [44]. The authors described the synthesis of several quinoline derivatives bearing phosphonate groups (Scheme 21). Phosphonate fragment was introduced into compounds 102 under Mitsunobu conditions and subsequent hydrogenation of 8-nitro-or 8-cyano derivatives 103 was accompanied with benzyl ester cleavage to give 8-amino-or 8-aminomethylquinolines 104, respectively. At the last step, Fmoc protective group was installed, affording the corresponding amides 105 in moderate yields.

Scheme 21. Synthesis of quinoline-based INIs bearing phosphonate groups.
In 2006 a microwave-assisted synthesis of fluoroquinolone ribonucleosides was described [45]. Reaction of fluoroanilines 106 with diethyl (ethoxymethylidene)malonate followed by ring closure gave fluoroquinolone derivatives 108 (Scheme 22). The target compounds 109 were obtained by coupling with 1,2,3,5-O-tetraacetyl-D-ribofuranose and deprotection of hydroxyl groups with NaOMe in MeOH. All fluoroquinolones were examined as HIV-1 INIs. Interestingly, synthesized nucleosides were found to be inactive in cell culture but demonstrated enzymatic inhibitory effect against HIV-1 integrase. In 2006 a microwave-assisted synthesis of fluoroquinolone ribonucleosides was described [45]. Reaction of fluoroanilines 106 with diethyl (ethoxymethylidene)malonate followed by ring closure gave fluoroquinolone derivatives 108 (Scheme 22). The target compounds 109 were obtained by coupling with 1,2,3,5-O-tetraacetyl-D-ribofuranose and deprotection of hydroxyl groups with NaOMe in MeOH. All fluoroquinolones were examined as HIV-1 INIs. Interestingly, synthesized nucleosides were found to be inactive in cell culture but demonstrated enzymatic inhibitory effect against HIV-1 integrase. Aromatic foldamers containing quinoline skeleton were proposed as HIV-1 INIs in 2018 [44]. The authors described the synthesis of several quinoline derivatives bearing phosphonate groups (Scheme 21). Phosphonate fragment was introduced into compounds 102 under Mitsunobu conditions and subsequent hydrogenation of 8-nitro-or 8-cyano derivatives 103 was accompanied with benzyl ester cleavage to give 8-amino-or 8-aminomethylquinolines 104, respectively. At the last step, Fmoc protective group was installed, affording the corresponding amides 105 in moderate yields. A number of simple quinaldines and their derivatives were synthesized as novel promising small molecular scaffolds-potential INIs [46,47]. Some examples are depicted on Scheme 23. Scraup reaction of 4-aminosalycilic acid 110 with crotonaldehyde gave quinoline 111, which showed IC 50 of 47 µM. Nitration of 111 afforded quinaldic acid 112 (IC 50 42 µM). Another synthetic route leads to target compounds starting from 8hydroxyquinaldine 113. This compound underwent various electrophilic functionalizations (nitration, carboxylation, or sulfonation) to give desired quinolines 114-116, which were found to be less active than 112. Int [48]. Heating of corresponding N-alkyl anilines 117 with triethyl methanetricarboxylate in Dowtherm A followed by hydrolysis led to target carboxylic acids 118 in moderate yields. These compounds were designed as diketo-bioisosteric analogs of Roquinimex that inhibited both 3′-processing and strand transfer activities. The authors assumed that derivatization of Roquinimex by changing of amide for diketo fragment would improve inhibition effect. However, all synthesized derivatives showed potency in inhibiting of HIV-1 integrase at a level of Roquinimex or less along with low cytotoxicity.

Scheme 24. Synthesis of diketo-bioisosteric analogs of Roquinimex.
Wang et al. reported design and synthesis of quinoline-pyrimidine hybrids as potential dual inhibitors of HIV-1 integrase and reverse transcriptase [49]. These compounds represent Elvitegravir analogues with formal substitution of aryl fragment with pyrimidine scaffold. Quinoline moiety was assembled using Gould-Jacobs method (Scheme 25). 4-Hydroxymethylaniline 119 reacted with ethoxymethylenemalonic ester to give corresponding enamine, and MOM protection of the hydroxyl group gave compound 120. Next, heating in Ph2O provided quinoline-4-one derivative, which on N-alkylation and protective groups interconversion gave chloromethyl derivative 121.  [48]. Heating of corresponding N-alkyl anilines 117 with triethyl methanetricarboxylate in Dowtherm A followed by hydrolysis led to target carboxylic acids 118 in moderate yields. These compounds were designed as diketo-bioisosteric analogs of Roquinimex that inhibited both 3 -processing and strand transfer activities. The authors assumed that derivatization of Roquinimex by changing of amide for diketo fragment would improve inhibition effect. However, all synthesized derivatives showed potency in inhibiting of HIV-1 integrase at a level of Roquinimex or less along with low cytotoxicity.  [48]. Heating of corresponding N-alkyl anilines 117 with triethyl methanetricarboxylate in Dowtherm A followed by hydrolysis led to target carboxylic acids 118 in moderate yields. These compounds were designed as diketo-bioisosteric analogs of Roquinimex that inhibited both 3′-processing and strand transfer activities. The authors assumed that derivatization of Roquinimex by changing of amide for diketo fragment would improve inhibition effect. However, all synthesized derivatives showed potency in inhibiting of HIV-1 integrase at a level of Roquinimex or less along with low cytotoxicity.

Scheme 24. Synthesis of diketo-bioisosteric analogs of Roquinimex.
Wang et al. reported design and synthesis of quinoline-pyrimidine hybrids as potential dual inhibitors of HIV-1 integrase and reverse transcriptase [49]. These compounds represent Elvitegravir analogues with formal substitution of aryl fragment with pyrimidine scaffold. Quinoline moiety was assembled using Gould-Jacobs method (Scheme 25). 4-Hydroxymethylaniline 119 reacted with ethoxymethylenemalonic ester to give corresponding enamine, and MOM protection of the hydroxyl group gave compound 120. Next, heating in Ph2O provided quinoline-4-one derivative, which on N-alkylation and protective groups interconversion gave chloromethyl derivative 121. Approaches to the synthesis of tricyclic pyridine derivatives as potential HIV-1 INIs were reported by Kim et al. [50][51][52]. The authors synthesized several series of 7-(4-fluorobenzyl)-6,7-dihydro-8H-pyrrolo [3,4-g]quinolin-8-one derivatives and studied their inhibitory anti-HIV-1 activity. This class has shown great potential in integrase inhibition. One of the standard synthetic sequences leading to the target compounds is depicted in Scheme 26. Heterocyclic core was assembled by esterification of starting pyridine-2,3-dicarboxylic acid 125 followed by the Dieckmann condensation with 1-(4-fluoro-benzyl)-pyrrolidine-2,5-dione 126 with the formation of tricyclic bis-phenol 127. One of the hydroxyl groups was then protected by reaction with ethyl chloroformate to give 128, and another one was converted to (diphenylmethyl)oxy group (compound 129). Reduction of one of the carbonyl groups and further conversion of OH to triflate afforded compound 130, which was, in turn, transformed into carboxylic acid 131 and finally to methylamino derivative 133. After several transformations, the desired tricyclic amides and sulfonamides 134 were obtained in moderate to high yields. Approaches to the synthesis of tricyclic pyridine derivatives as potential HIV-1 INIs were reported by Kim et al. [50][51][52]. The authors synthesized several series of 7-(4fluorobenzyl)-6,7-dihydro-8H-pyrrolo [3,4-g]quinolin-8-one derivatives and studied their inhibitory anti-HIV-1 activity. This class has shown great potential in integrase inhibition. One of the standard synthetic sequences leading to the target compounds is depicted in Scheme 26. Heterocyclic core was assembled by esterification of starting pyridine-2,3dicarboxylic acid 125 followed by the Dieckmann condensation with 1-(4-fluoro-benzyl)pyrrolidine-2,5-dione 126 with the formation of tricyclic bis-phenol 127. One of the hydroxyl groups was then protected by reaction with ethyl chloroformate to give 128, and another one was converted to (diphenylmethyl)oxy group (compound 129). Reduction of one of the carbonyl groups and further conversion of OH to triflate afforded compound 130, which was, in turn, transformed into carboxylic acid 131 and finally to methylamino derivative 133. After several transformations, the desired tricyclic amides and sulfonamides 134 were obtained in moderate to high yields.
In 2006, the first total synthesis of lamellarin α 20-sulfate as selective HIV-1 INI was reported [53]. Synthetic route started from commercially available 3,4-dimethoxyphenetylamine 135, which was alkylated with bromoacetic ester to give the corresponding iminodiacetate 136 (Scheme 27). In the next step, the Hinsberg reaction with dimethyl oxalate followed by reaction with Tf 2 O led to bistriflate derivative 137, which was successively arylated with two different boronic acids in the presence of Pd(PPh 3 ) 4 to give 3,4-diarylpyrrole 139, which was then converted to six-membered lactone 140 and then decarboxylated to compound 141. The intramolecular oxidative biaryl coupling under Kita's conditions provided 20-benzyl-13-isopropyllamellarin a 142. Finally, deprotection of the benzyl group, selective removal of the isopropyl protecting group, and deprotection of the trichloroethyl ester gave rise to target lamellarin a 20-sulfate 143. Int In 2006, the first total synthesis of lamellarin α 20-sulfate as selective HIV-1 INI was reported [53]. Synthetic route started from commercially available 3,4-dimethoxyphenetylamine 135, which was alkylated with bromoacetic ester to give the corresponding iminodiacetate 136 (Scheme 27). In the next step, the Hinsberg reaction with dimethyl oxalate followed by reaction with Tf2O led to bistriflate derivative 137, which was successively arylated with two different boronic acids in the presence of Pd(PPh3)4 to give 3,4-diarylpyrrole 139, which was then converted to six-membered lactone 140 and then decarboxylated to compound 141. The intramolecular oxidative biaryl coupling under Kita's conditions provided 20-benzyl-13-isopropyllamellarin a 142. Finally, deprotection of the benzyl group, selective removal of the isopropyl protecting group, and deprotection of the trichloroethyl ester gave rise to target lamellarin a 20-sulfate 143. Novel quinoline containing diketo acids were designed by Di Santo et al. [54]. Commercial anilines 144 reacted with ethyl orthoformate and ethyl acetoacetate in Dowtherm A to give corresponding 3-acetyl-4(1H)-quinolinones 145 (Scheme 28). Compounds 145 were then N-alkylated with 4-fluorobenzylbromide followed by condensation with diethyl oxalate affording esters 147, which were hydrolyzed in basic media to give the corresponding acids 148. 8-Fluoroquinoline (148, R 3 = F) was the most potent derivative in IN enzyme assays, 8-pyrrolidin-1-yl compound and showed the highest potency against HIV-1 in acutely infected cells. Novel quinoline containing diketo acids were designed by Di Santo et al. [54]. Commercial anilines 144 reacted with ethyl orthoformate and ethyl acetoacetate in Dowtherm A to give corresponding 3-acetyl-4(1H)-quinolinones 145 (Scheme 28). Compounds 145 were then N-alkylated with 4-fluorobenzylbromide followed by condensation with diethyl ox-alate affording esters 147, which were hydrolyzed in basic media to give the corresponding acids 148. 8-Fluoroquinoline (148, R 3 = F) was the most potent derivative in IN enzyme assays, 8-pyrrolidin-1-yl compound and showed the highest potency against HIV-1 in acutely infected cells. Scheme 27. The first total synthesis of lamellarin α 20-sulfate.
Novel quinoline containing diketo acids were designed by Di Santo et al. [54]. Commercial anilines 144 reacted with ethyl orthoformate and ethyl acetoacetate in Dowtherm A to give corresponding 3-acetyl-4(1H)-quinolinones 145 (Scheme 28). Compounds 145 were then N-alkylated with 4-fluorobenzylbromide followed by condensation with diethyl oxalate affording esters 147, which were hydrolyzed in basic media to give the corresponding acids 148. 8-Fluoroquinoline (148, R 3 = F) was the most potent derivative in IN enzyme assays, 8-pyrrolidin-1-yl compound and showed the highest potency against HIV-1 in acutely infected cells. An effort to expand of scope of potential HIV-1 inhibitors was done by Tyler et al. [56]. It was realized on the basis of the commercially available 1,3-dichloroisoquinoline 152 (Scheme 30). At the first step, the introduction of hydroxyacetic acid side chain into isoquinoline core was realized. Compound 153 was then converted into t-butyl ether 154 under the action of t-butyl acetate and HClO4. The authors found reaction conditions allowing to introduce two different aryl substituents in positions 1 and 3 of isoquinoline core. Thus, the first Suzuki-Miyaura coupling reaction with aryl boronic acid was carried out at 90 o C at more reactive position 1, while the second coupling with another boronic acid occurred under more drastic conditions to give 1,3-diarylisoquinoline esters 156. Finally, hydrolysis of esters 156 afforded desired carboxylic acids 157. An effort to expand of scope of potential HIV-1 inhibitors was done by Tyler et al. [56]. It was realized on the basis of the commercially available 1,3-dichloroisoquinoline 152 (Scheme 30). At the first step, the introduction of hydroxyacetic acid side chain into isoquinoline core was realized. Compound 153 was then converted into t-butyl ether 154 under the action of t-butyl acetate and HClO 4 . The authors found reaction conditions allowing to introduce two different aryl substituents in positions 1 and 3 of isoquinoline core. Thus, the first Suzuki-Miyaura coupling reaction with aryl boronic acid was carried out at 90 • C at more reactive position 1, while the second coupling with another boronic acid occurred under more drastic conditions to give 1,3-diarylisoquinoline esters 156. Finally, hydrolysis of esters 156 afforded desired carboxylic acids 157.
isoquinoline core was realized. Compound 153 was then converted into t-butyl ether 154 under the action of t-butyl acetate and HClO4. The authors found reaction conditions allowing to introduce two different aryl substituents in positions 1 and 3 of isoquinoline core. Thus, the first Suzuki-Miyaura coupling reaction with aryl boronic acid was carried out at 90 o C at more reactive position 1, while the second coupling with another boronic acid occurred under more drastic conditions to give 1,3-diarylisoquinoline esters 156. Finally, hydrolysis of esters 156 afforded desired carboxylic acids 157.

Scheme 30. Synthesis of 1,3-dichloroisoquinoline derivatives as potential HIV-1 inhibitors.
Satyanarayana et al. proposed a simple and efficient protocol for the synthesis of 1,2,3,4-tetrahydroisoquinoline derivatives [57]. The method is based on one-pot sequential intermolecular aza-Michael addition and Pd-catalyzed intramolecular Buchwald-Hartwig arylation of bis-benzylamines 158 (Scheme 31). Later, the same authors described chemical transformations of isoquinoline derivatives 159, such as reduction to alcohols 160 and rearranged aromatization to give isoquinolines 161 [58]. Compounds 160 and 161 possessed higher anti-HIV activity compared to 159. Compound 161a was found to be the most effective among all other synthesized analogs. It efficiently inhibits Scheme 30. Synthesis of 1,3-dichloroisoquinoline derivatives as potential HIV-1 inhibitors.
Satyanarayana et al. proposed a simple and efficient protocol for the synthesis of 1,2,3,4-tetrahydroisoquinoline derivatives [57]. The method is based on one-pot sequential intermolecular aza-Michael addition and Pd-catalyzed intramolecular Buchwald-Hartwig arylation of bis-benzylamines 158 (Scheme 31). Later, the same authors described chemical transformations of isoquinoline derivatives 159, such as reduction to alcohols 160 and rearranged aromatization to give isoquinolines 161 [58]. Compounds 160 and 161 possessed higher anti-HIV activity compared to 159. Compound 161a was found to be the most effective among all other synthesized analogs. It efficiently inhibits the interaction between LEDGF/p75 and integrase in vitro, as well as HIV-1 infection in a cell line. Therefore, this compound has been identified as a lead molecule in this study.  A series of N-hydroxyisoquinoline derivatives was designed as potential dual inhibitors of HIV-1 integrase and reverse transcriptase RNase H domain by Billamboz et. al. [59]. The method is based on the condensation of 7-substituted homophthalic acid derivatives 162 with O-benzylhydroxylamine to give the corresponding 2-benzy-loxyisoquinolines 163 followed by deprotection of the N-hydroxyl function yielding compounds 164 (Scheme 32). Most compounds inhibited RNase H and integrase at micromolar concentrations, and some of them were weakly selective for integrase. A series of N-hydroxyisoquinoline derivatives was designed as potential dual inhibitors of HIV-1 integrase and reverse transcriptase RNase H domain by Billamboz et al. [59]. The method is based on the condensation of 7-substituted homophthalic acid derivatives 162 with O-benzylhydroxylamine to give the corresponding 2-benzy-loxyisoquinolines 163 followed by deprotection of the N-hydroxyl function yielding compounds 164 (Scheme 32). Most compounds inhibited RNase H and integrase at micromolar concentrations, and some of them were weakly selective for integrase.
A series of N-hydroxyisoquinoline derivatives was designed as potential dual inhibitors of HIV-1 integrase and reverse transcriptase RNase H domain by Billamboz et. al. [59]. The method is based on the condensation of 7-substituted homophthalic acid derivatives 162 with O-benzylhydroxylamine to give the corresponding 2-benzy-loxyisoquinolines 163 followed by deprotection of the N-hydroxyl function yielding compounds 164 (Scheme 32). Most compounds inhibited RNase H and integrase at micromolar concentrations, and some of them were weakly selective for integrase. Scheme 32. Design and synthesis of N-hydroxyisoquinoline derivatives.
derivatives 162 with O-benzylhydroxylamine to give the corresponding 2-benzy-loxyisoquinolines 163 followed by deprotection of the N-hydroxyl function yielding compounds 164 (Scheme 32). Most compounds inhibited RNase H and integrase at micromolar concentrations, and some of them were weakly selective for integrase.

Synthesis
of structurally similar 4-substituted benzylideneisoquinoline-1,3(2H,4H)-dione derivatives was published by Wadhwa [60]. Isoquinoline core was synthesized by the reaction of homophthalic acid 165 and urea under microwave irradiation (Scheme 33). Then isoquinoline-1,3(2H,4H)-dione 166 reacted with various aromatic aldehydes to give desired molecules 167. Isoquinolines 167 were tested for anti-HIV-1 activity, and some of them exhibited significant percentage inhibition of HIV-1 integrase with IC50 values less than 5.96 μM. Another series of 2-hydroxyisoquinoline-1,3(2H,4H)-dione derivatives were synthesized [61]. All compounds were prepared from dimethyl homophthalate 168 in four steps (Scheme 34). Firstly, alkylation of the starting compound provided a number of monoalkyl derivatives 169, which were hydrolyzed to the corresponding acids 170. Isoquinoline ring closure was implemented via reaction with O-benzyl hydroxylamine, and deprotection under the action of boron trihalogenides gave desired N-hydroxyisoquinolines 171. Some of the synthesized compounds inhibited HIV-1 integrase at a low micromolar level, although high cytotoxicity in cell culture limited their applications as antiviral agents. Another series of 2-hydroxyisoquinoline-1,3(2H,4H)-dione derivatives were synthesized [61]. All compounds were prepared from dimethyl homophthalate 168 in four steps (Scheme 34). Firstly, alkylation of the starting compound provided a number of monoalkyl derivatives 169, which were hydrolyzed to the corresponding acids 170. Isoquinoline ring closure was implemented via reaction with O-benzyl hydroxylamine, and deprotection under the action of boron trihalogenides gave desired N-hydroxyisoquinolines 171. Some of the synthesized compounds inhibited HIV-1 integrase at a low micromolar level, although high cytotoxicity in cell culture limited their applications as antiviral agents. Scheme 34. Synthesis of 2-hydroxyisoquinoline-1,3(2H,4H)-dione derivatives.

Pyridines Fused with Heterocycles
Pyrazine-fused 3-hydroxypyridine-4-one moiety is a central part of the approved HIV-1 INIs Dolutegravir, Bictegravir, and Cabotegravir. A number of publications during the two prior decades has dealt with the design and synthesis of novel INIs of condensed piridinone series as well as of more efficient and cost-friendly procedures for known INIs [62]. For example, a process for the preparation of Dolutegravir and its sodium derivatives was reported in 2016 in the patent literature [63]. Seven-step flow synthesis of Dolutegravir was described, allowing the production of this pharmaceutical in sequential flow operations from commercially available materials [64]. The synthesis included rapid manufacturing time and the combination of multiple steps in order to avoid isolation of intermediates.

Pyridines Fused with Heterocycles
Pyrazine-fused 3-hydroxypyridine-4-one moiety is a central part of the approved HIV-1 INIs Dolutegravir, Bictegravir, and Cabotegravir. A number of publications during the two prior decades has dealt with the design and synthesis of novel INIs of condensed piridinone series as well as of more efficient and cost-friendly procedures for known INIs [62]. For example, a process for the preparation of Dolutegravir and its sodium derivatives was reported in 2016 in the patent literature [63]. Seven-step flow synthesis of Dolutegravir was described, allowing the production of this pharmaceutical in sequential flow operations from commercially available materials [64]. The synthesis included rapid manufacturing time and the combination of multiple steps in order to avoid isolation of intermediates.
Most of the published synthetic approaches to Dolutegravir follow a similar strategyconstruction of a pyridinone cycle and further annulation of saturated pyrazine and oxazine rings [65,66]. For example, synthesis of Dolutegravir, Cabotegravir, and a series of related compounds was described in 2015 [67]. Diastereoselective annulation of saturated heterocyclic rings to a pyridinone core was the main challenge of the research. For this reason, readily available chiral amino alcohols 172 and 173 reacted with previously synthesized aldehyde 174 [68] for hemiaminal ring fusion, furnishing the desired stereocenter within the tricyclic carbamoyl pyridinone scaffold (compounds 175 and 176). The target compounds were obtained after cleavage of O-benzyl protection using hydrogen and Pd/C (Scheme 35). Another approach was reported recently by Opatz et al. [69]. The authors proposed short and practical gram-scale synthesis of Dolutegravir sodium salt where assembling of the target molecule commenced with the formation of oxazine and pyrazine rings (Scheme 36). Chloroacetyl chloride as bis-electrophilic reagent first reacted with (3R)-amino-1-butanol 177 followed by reaction with (2,2-dimethoxyethyl)benzylamine. The resulting compound 178 was then cyclized and the benzylic protection cleaved to give rings B and C of Dolutegravir (compound 179). Annulation of a pyridine ring was accomplished by the condensation with diethyl-2-(ethoxymethylidene)-3-oxobutandioate 180 and finally 2,4-difluorobenzylamine fragment was introduced and sodium salt was obtained on heating with ethanolic NaOH. Another approach was reported recently by Opatz et al. [69]. The authors proposed short and practical gram-scale synthesis of Dolutegravir sodium salt where assembling of the target molecule commenced with the formation of oxazine and pyrazine rings (Scheme 36). Chloroacetyl chloride as bis-electrophilic reagent first reacted with (3R)amino-1-butanol 177 followed by reaction with (2,2-dimethoxyethyl)benzylamine. The resulting compound 178 was then cyclized and the benzylic protection cleaved to give rings B and C of Dolutegravir (compound 179). Annulation of a pyridine ring was accomplished by the condensation with diethyl-2-(ethoxymethylidene)-3-oxobutandioate 180 and finally 2,4-difluorobenzylamine fragment was introduced and sodium salt was obtained on heating with ethanolic NaOH.
Novel 2-pyridinone aminal series was designed as potential INIs [70]. The previously reported clinical candidate MK-0536 served as starting point in the optimization process (Scheme 37). Reactions of substituted 2,6-naphthyridine-2-carboxamides 181 with cyclic ketones resulted in the formation of spiro aminals 182 and 183 in low yields. Another promising spirocompounds 184 was synthesized on the basis of pivaloyl-protected ester 185 by the reaction with chiral amine 186 to give amide 187 followed by reaction with bicyclic ketone. As a result of this work, several lead molecules were discovered and their structures were optimized in order to reach the optimum ratio of the antiviral activity values and physiochemical properties. Another approach was reported recently by Opatz et al. [69]. The authors proposed short and practical gram-scale synthesis of Dolutegravir sodium salt where assembling of the target molecule commenced with the formation of oxazine and pyrazine rings (Scheme 36). Chloroacetyl chloride as bis-electrophilic reagent first reacted with (3R)-amino-1-butanol 177 followed by reaction with (2,2-dimethoxyethyl)benzylamine. The resulting compound 178 was then cyclized and the benzylic protection cleaved to give rings B and C of Dolutegravir (compound 179). Annulation of a pyridine ring was accomplished by the condensation with diethyl-2-(ethoxymethylidene)-3-oxobutandioate 180 and finally 2,4-difluorobenzylamine fragment was introduced and sodium salt was obtained on heating with ethanolic NaOH. Scheme 36. Alternative approach to Dolutegravir and its sodium salt.   The first dual HIV-1 reverse transcriptase RNase H domain and integrase inhibitors based on a 5-hydroxypyrido [2,3-b]pyrazin-6(5H)-one structure was reported in 2018 [71]. The synthetic route included the reaction of commercially available methyl 3-chloropyrazine-2-carboxylate 188 with O-benzyl hydroxyl amine leading to compound 189, further acylation with methyl 3-chloro-3-oxopropanoate, and Claisen-type condensation to yield a bicyclic intermediate 190 (Scheme 38). It was then tosylated and reacted with aromatic amines of biphenyl and naphthalene series, followed by de-benzylation to give target compounds 191. The majority of synthesized compounds inhibited both enzymes at micromolar concentrations. The best dual inhibitor possessed close IC 50 values of 1.77 µM and 1.18 µM.
3-chloropyrazine-2-carboxylate 188 with O-benzyl hydroxyl amine leading to compound 189, further acylation with methyl 3-chloro-3-oxopropanoate, and Claisen-type condensation to yield a bicyclic intermediate 190 (Scheme 38). It was then tosylated and reacted with aromatic amines of biphenyl and naphthalene series, followed by de-benzylation to give target compounds 191. The majority of synthesized compounds inhibited both enzymes at micromolar concentrations. The best dual inhibitor possessed close IC50 values of 1.77 μM and 1.18 μM.

Scheme 38. Synthesis of dual HIV-1 reverse transcriptase RNase H domain and integrase inhibitors.
An efficient and highly diastereoselective synthesis of Cabotegravir was reported by Wang et al. [72]. The method features a simple and efficient assembly of highly substituted pyridine-4-one core as well as diastereoselective construction of oxazolidine fragment. The intermediate pyridine-4-one 192 was obtained in 61% yield in a four-step one-pot operation, starting from methyl 4-methoxy-3-oxobutanoate 193, which was treated with DMA DMF and then with 2,2-dimethoxyethylamine to give the corresponding enamine 194 (Scheme 39). This enamine underwent cyclization with dimethyl oxalate, and the addition of LiOH allowed the selective hydrolyzation of one of the methoxycarbonyl groups, viz. C-5. Acetal deprotection led to in situ formation of the aldehyde 195, which reacted with l-alaninol and resulted in diastereoselective cyclization with formation of compound 196 with one more stereocenter (dr = 34:1). Finally, formation of 2,4-difluorobenzylamide and demethylation with MgBr 2 gave Cabotegravir. An efficient and highly diastereoselective synthesis of Cabotegravir was reported by Wang et al. [72]. The method features a simple and efficient assembly of highly substituted pyridine-4-one core as well as diastereoselective construction of oxazolidine fragment. The intermediate pyridine-4-one 192 was obtained in 61% yield in a four-step one-pot operation, starting from methyl 4-methoxy-3-oxobutanoate 193, which was treated with DMA DMF and then with 2,2-dimethoxyethylamine to give the corresponding enamine 194 (Scheme 39). This enamine underwent cyclization with dimethyl oxalate, and the addition of LiOH allowed the selective hydrolyzation of one of the methoxycarbonyl groups, viz. C-5. Acetal deprotection led to in situ formation of the aldehyde 195, which reacted with l-alaninol and resulted in diastereoselective cyclization with formation of compound 196 with one more stereocenter (dr = 34:1). Finally, formation of 2,4-difluorobenzylamide and demethylation with MgBr2 gave Cabotegravir.

Scheme 39. Wang's diastereoselective synthesis of Cabotegravir.
Diastereomeric ratio in the final product was increased substantially by changing the steps order (Scheme 40). Formation of the amide followed by acetal deprotection resulted in the formation of aldehyde 197, and reaction with l-alaninol in the presence of Mg(OTf)2 gave Cabotegravir with dr about 300:1. Scheme 40. Diastereoselective synthesis of Cabotegravir.
In addition to amide function, 2,4-difluorobenzyl fragment can be bound to the Diastereomeric ratio in the final product was increased substantially by changing the steps order (Scheme 40). Formation of the amide followed by acetal deprotection resulted in the formation of aldehyde 197, and reaction with l-alaninol in the presence of Mg(OTf) 2 gave Cabotegravir with dr about 300:1.
In addition to amide function, 2,4-difluorobenzyl fragment can be bound to the heterocyclic core through triple C-C-bond [73]. For this reason, the initial dimethyl acetal 192 was converted in situ to aldehyde 195 and then to tricyclic pyridinone carboxylic acid 196 (Scheme 41). Its reduction to alcohol followed by Dess-Martin oxidation gave the corresponding aldehyde 198. Alkyne moiety was introduced by the reaction with Ohira-Bestmann reagent, and then terminal alkyne 199 was coupled with 2,4-difluorobenzyl bromide in Sonogashira reaction conditions. Demethylation of 200 with BBr 3 afforded Cabotegravir 201 analog, which demonstrated significant activity (EC 50  Diastereomeric ratio in the final product was increased substantially by changing the steps order (Scheme 40). Formation of the amide followed by acetal deprotection resulted in the formation of aldehyde 197, and reaction with l-alaninol in the presence of Mg(OTf)2 gave Cabotegravir with dr about 300:1.

Scheme 40. Diastereoselective synthesis of Cabotegravir.
In addition to amide function, 2,4-difluorobenzyl fragment can be bound to the heterocyclic core through triple C-C-bond [73]. For this reason, the initial dimethyl acetal 192 was converted in situ to aldehyde 195 and then to tricyclic pyridinone carboxylic acid 196 (Scheme 41). Its reduction to alcohol followed by Dess-Martin oxidation gave the corresponding aldehyde 198. Alkyne moiety was introduced by the reaction with Ohira-Bestmann reagent, and then terminal alkyne 199 was coupled with 2,4-difluorobenzyl bromide in Sonogashira reaction conditions. Demethylation of 200 with BBr3 afforded A practical asymmetric total synthesis of partially saturated naphthyridine 202 fused with 8-membered nitrogen heterocycle was developed [74]. Earlier, compound 202 was identified as a potent HIV-1 inhibitor [75]. The elaborated reaction sequence is depicted in Scheme 42 and includes more than 10 synthetic steps proceeding generally in good yields. The key steps are the formation of the naphthyridine system and the annulation of the eight-membered cycle. Readily available D-(−)-pantolactone 203 was taken as a precursor for the corresponding chiral amino alcohol 204, which was used for the construction of the fused heterocyclic core via coupling with carboxylic acid 205. Amide 206 without isolation was converted to tricyclic derivative 208 and after removal of THP and mesylate protective groups, the target compound 202 in 14% overall yield was obtained. It should be noted that the proposed approach did not require isolation of intermediates 206 and 207 during the formation of the 8-membered ring. A practical asymmetric total synthesis of partially saturated naphthyridine 202 fused with 8-membered nitrogen heterocycle was developed [74]. Earlier, compound 202 was identified as a potent HIV-1 inhibitor [75]. The elaborated reaction sequence is depicted in Scheme 42 and includes more than 10 synthetic steps proceeding generally in good yields.
The key steps are the formation of the naphthyridine system and the annulation of the eight-membered cycle. Readily available D-(−)-pantolactone 203 was taken as a precursor for the corresponding chiral amino alcohol 204, which was used for the construction of the fused heterocyclic core via coupling with carboxylic acid 205. Amide 206 without isolation was converted to tricyclic derivative 208 and after removal of THP and mesylate protective groups, the target compound 202 in 14% overall yield was obtained. It should be noted that the proposed approach did not require isolation of intermediates 206 and 207 during the formation of the 8-membered ring.
A series of bicyclic 2-oxo-1,2-dihydro-1,8-naphthyridine-3-carboxamides, highly potent against cells harboring Raltegravir-resistant integrase mutants, were synthesized and evaluated by Burke et al. [76]. Commercially available methyl 2-fluoronicotinate 209 was treated with O-benzyl hydroxylamine and further acylated with methyl 3-chloro-3oxopropanoate to give compound 210 in 86% yield. Annulation of the second pyridine ring was achieved by Claisen-type condensation under the action of NaOMe. The resulting key A series of bicyclic 2-oxo-1,2-dihydro-1,8-naphthyridine-3-carboxamides, highly potent against cells harboring Raltegravir-resistant integrase mutants, were synthesized and evaluated by Burke et al. [76]. Commercially available methyl 2-fluoronicotinate 209 was treated with O-benzyl hydroxylamine and further acylated with methyl 3-chloro-3-oxopropanoate to give compound 210 in 86% yield. Annulation of the second pyridine ring was achieved by Claisen-type condensation under the action of NaOMe. Later, the same authors investigated the influence of substituents in position 6 and 7 of 1-hydroxy-2-oxo-1,2-dihydro-1,8-naphthyridine-3-carboxylic acid 2,4-difluorobenzylamides [77]. Basically, the synthetic scheme was quite similar to the one mentioned above, but starting compounds (nicotinic acid derivatives) bearing additional halogen atoms allowed the introduction of the necessary functions into the pyridine core. 2,6-Dichloronicotinic acid 214 was used as starting material in which both chlorine atoms were appropriately substituted to give compounds 215. Annulation of another pyridine ring was carried out as shown in Scheme 43. Removal of benzyl group gave 7-substituted naphthyridines 216 (Scheme 44). Later, the same authors investigated the influence of substituents in position 6 and 7 of 1hydroxy-2-oxo-1,2-dihydro-1,8-naphthyridine-3-carboxylic acid 2,4-difluorobenzylamides [77]. Basically, the synthetic scheme was quite similar to the one mentioned above, but starting compounds (nicotinic acid derivatives) bearing additional halogen atoms allowed the introduction of the necessary functions into the pyridine core. 2,6-Dichloronicotinic acid 214 was used as starting material in which both chlorine atoms were appropriately substituted to give compounds 215. Annulation of another pyridine ring was carried out as shown in Scheme 43. Removal of benzyl group gave 7-substituted naphthyridines 216 (Scheme 44).
Later, the same authors investigated the influence of substituents in position 6 and 7 of 1-hydroxy-2-oxo-1,2-dihydro-1,8-naphthyridine-3-carboxylic acid 2,4-difluorobenzylamides [77]. Basically, the synthetic scheme was quite similar to the one mentioned above, but starting compounds (nicotinic acid derivatives) bearing additional halogen atoms allowed the introduction of the necessary functions into the pyridine core. 2,6-Dichloronicotinic acid 214 was used as starting material in which both chlorine atoms were appropriately substituted to give compounds 215. Annulation of another pyridine ring was carried out as shown in Scheme 43. Removal of benzyl group gave 7-substituted naphthyridines 216 (Scheme 44).
give compound 232 (Scheme 48). Partial hydrolysis under basic conditions gave enol 233, which on heating in PPA underwent formation of azacoumarin 234. Reactions of 234 with aryl isocyanates or aryl isothiocyanates led to the target 4-hydroxy-5-azacoumarin-3-carbox(thio)amides 235 in low to moderate yields. Carboxamides were found to be more active inhibitors compared to thioamides-IC50 6.7-35.7 µ M and >300 µ M, respectively. Therefore, the 4-hydroxy-5-azacoumarin ring can be considered as a new scaffold in designing more potent HIV-1 INIs.
Zhao et al. reported on the synthesis of novel bicyclic pyrrolopyridine-triones, Scheme 49 [81]. The key step in synthesis is Pummerer-induced cyclization-deprotonation sequence. Acylation of (ethylthio)acetamides 236 with acyl chlorides afforded bis-acylamides 237. The latter compounds were oxidized with sodium periodate to give sulfoxides 238 in good yields. Compounds were refluxed with N-(3-chloro-4-fluorobenzyl)maleimide giving rise to corresponding cycloadducts 239, which on treatment with boron trifluoride diethyl etherate gave bicyclic pyrrolopyridines 240. All compounds showed anti-HIV-1 activity with IC50 values in the range 6.4-21.6 µ M. rial and reacted with POBr3 to give bromopyridine 242. Bromide 242 was converted to nitrile 243 under the action of Zn(CN)2, and then to esters 244. Reaction of 244 with DMADMF followed by hydrogenation led to azaindoles 245. Synthesized esters were then alkylated with a number of benzyl halides, affording N-alkylazaindoles 246. The latter compounds were transformed into hydroxamic acids 247, either by direct reaction with hydroxyl amine or via hydrolysis to acids 248, and further coupling with N,O-substituted hydroxyl amines. A series of naphthyridinone derivatives were synthesized and their structure-activity relationship as HIV-1 INIs was disclosed by Johns et al., Scheme 51 [83,84]. Cyclic anhydrides 249 were ring-opened with alcohols to afford acids 250. Curtius rearrangement of 250 under the action of DPPA in the presence of tBuOH gave N-Boc derivatives which were deprotected by TFA and underwent reactions with aldehydes and sodium triacetoxyborohydride leading to esters 251. Reactions of 251 with methyl-or ethylmalonyl chloride produced intermediates 252 which were cyclized into naphthyridinones 253. In turn, compounds 253 were converted into target carboxamides 254 by reactions with corresponding amines. The authors noted substituent effects at N-1, C-3, and 7-benzyl positions on inhibition activity.
Synthesis of azole-containing pyrido[1,2-a]pyrimidines and their utilization as an amide isostere in HIV-1 integrase inhibition was reported by Le et al. [93]. Methyl ester 287 was chosen as a key starting material for the synthesis (Scheme 57). The ester group was converted mono-hydrazide, which was further acylated with 4-fluorophenylacetyl chloride to give intermediate 288. Cyclization of this diacylhydrazide under the action of the corresponding agents and debenzylation with TMSI afforded 1,3,4-oxadiazole 289 and 1,3,4-thiadiazole 290. Triazole 291 was synthesized directly from ester 287 by treatment of aqueous ammonium hydroxide followed by reaction with Lawesson's reagent, and with MeI to give thioamide intermediate that cyclized with 4-F-phenyl acetohydrazide to form triazole ring. A similar strategy was used for synthesis of oxazole 292, thiazole 293, and imidazole 294. Ester group in 287 was hydrolyzed to produce acid 295, which underwent reaction with aminoketone affording 296. During the next steps, cyclization and deprotection produce azoles 292-294. Construction 1,2,4-oxadiazole derivative 297 was achieved via transformation of compound 287 into nitrile 298 by reaction with ammonia and dehydration with trichlorotriazine. Compound 298 was treated with hydroxylamine to give N-hydroxyamidine, which was acylated with 4-fluorophenylacetyl chloride to produce 299, which on heating in toluene led to target oxadiazole 297. Synthesis of azole-containing pyrido[1,2-a]pyrimidines and their utilization as an amide isostere in HIV-1 integrase inhibition was reported by Le et al. [93]. Methyl ester 287 was chosen as a key starting material for the synthesis (Scheme 57). The ester group was converted mono-hydrazide, which was further acylated with 4-fluorophenylacetyl chloride to give intermediate 288. Cyclization of this diacylhydrazide under the action of the corresponding agents and debenzylation with TMSI afforded 1,3,4-oxadiazole 289 and 1,3,4-thiadiazole 290. Triazole 291 was synthesized directly from ester 287 by treatment of aqueous ammonium hydroxide followed by reaction with Lawesson's reagent, and with MeI to give thioamide intermediate that cyclized with 4-F-phenyl acetohydrazide to form triazole ring. A similar strategy was used for synthesis of oxazole 292, thiazole 293, and imidazole 294. Ester group in 287 was hydrolyzed to produce acid 295, which underwent reaction with aminoketone affording 296. During the next steps, cyclization and deprotection produce azoles 292-294. Construction 1,2,4-oxadiazole derivative 297 was achieved via transformation of compound 287 into nitrile 298 by reaction with ammonia and dehydration with trichlorotriazine. Compound 298 was treated with hydroxylamine to give N-hydroxyamidine, which was acylated with 4-fluorophenylacetyl chloride to produce 299, which on heating in toluene led to target oxadiazole 297.

Conclusions
One of the goals of this review was to summarize most up-to-date approaches to the synthesis of known and new pyridine-based potential HIV-1 integrase inhibitors. An analysis of the literature over the last 20 years showed that the chemistry of monocyclic and fused pyridines is actively developing: syntheses of approved INIs are being im-Scheme 57. Synthesis of azole-containing pyrido[1,2-a]pyrimidines.

Conclusions
One of the goals of this review was to summarize most up-to-date approaches to the synthesis of known and new pyridine-based potential HIV-1 integrase inhibitors. An analysis of the literature over the last 20 years showed that the chemistry of monocyclic and fused pyridines is actively developing: syntheses of approved INIs are being improved and optimized, new syntheses are being published, and new pyridine-containing molecules are being created. Synthetic routes listed in this review are representative examples of the new developments, illustrating the importance of diverse pyridine compounds as feasible replacements or extensions of the field of anti-HIV agents.
Numerous studies confirm the importance of certain structural motifs to be included in a molecule to enhance activity, such as 4-fluoro-, 2,4-difluoro-, and 3-chloro-4-fluorobenzyl amides, 2,4-diketoacid fragment, or pyridin-4-one-3-carboxylic acid moiety in both monocyclic and condensed compounds. Since the structure of integrase is well established, including crystal and NMR studies of the individual domains, it can be predicted roughly if the designed compound would effectively block HIV replication. For this reason, molecular modeling methods, theoretical and computational, could help synthetic chemists in their routine research.
Inhibitory efficiencies are very important characteristics of the reviewed compounds. Indeed, IC 50 values of the target molecules vary widely from nM (similar to approved compounds) to 100 mM concentrations which are unacceptable for use as INIs. In addition, some of them possess high toxicity, and the others have not been tested yet. Nevertheless, high IC 50 and toxicity values do not automatically mean that the certain class of compounds should not be studied further. The main point is to find a new type of INIs that would allow to overcome resistance of the virus. Therefore, it is difficult to select the most promising compounds, and even the most promising class based solely on half maximal effective or inhibitory concentrations.
Thus, the field of chemistry associated with the synthesis of novel HIV-1 integrase inhibitors based on pyridine scaffold continues to be in demand and relevant. The results presented may serve as a basis for design and search of novel anti-HIV drugs.