AU775578B2 - Nucleosides analgoues, such as antivirals including inhibitors of retroviral reverse transcriptase and the DNA polymerase of hepatitis B virus (HBV) - Google Patents

Description

AUSTRALIA

Patents Act COMPLETE SPECIFICATION

(ORIGINAL)

Class Int. Class Application Number: Lodged: Complete Specification Lodged: Accepted: Published: Priority Related Art: Name of Applicant: Medivir AB Actual Inventor(s): Xiao-Xiong Zhou, Nils-Gunnar Johansson, Horst Wahling Address for Service: PHILLIPS ORMONDE FITZPATRICK Patent and Trade Mark Attorneys 367 Collins Street Melbourne 3000 AUSTRALIA Invention Title: NUCLEOSIDES ANALOGUES, SUCH AS ANTIVIRALS INCLUDING INHIBITORS OF RETROVIRAL REVERSE TRANSCRIPTASE AND THE DNA POLYMERASE OF HEPATITIS B VIRUS (HBV) Our Ref 641247 POF Code: 226529/226529 The following statement is a full description of this invention, including the best method of performing it known to applicant(s): -1- NUCLEOSIDES ANALOGUES, SUCH AS ANTIVIRALS INCLUDING INHIBITORS OF RETROVIRAL REVERSE TRANSCRIPTASE AND THE DNA POLYMERASE OF HEPATITIS B VIRUS (HBV) This application is a Divisional of parent application 87548/98, the entire disclosure of which is incorporated herein by reference.

Technical Field This invention relates to the field of nucleoside analogues, such as antivirals including inhibitors of retroviral reverse transcriptase and the DNA polymerase of Hepatitis B Virus (HBV). The invention provides novel compounds with favourable pharmaceutical parameters, methods for their preparation, pharmaceutical 10 compositions comprising these compounds and methods employing then for the inhibition of viral and neoplastic diseases including HBV and HIV.

Background to the invention International patent application no.WO 88/00050 describes the antiretroviral and anti-HBV activity of a series of 3'-fluorinated nucleosides, including the compounds 2',3'-dideoxy, 3'-fluoroguanosine (FLG) and 3'-fluorothymidine (FLT). The latter compound underwent clinical evaluation as an anti-HIV agent and although its antiviral activity and pharmacokinetics were good, it showed unexpected toxicity (Flexner et al, J Inf Dis 170(6) 1394-403 (1994)). The former compound FLG is very active in vitro however the present inventors have detected that its bioavailability is so poor around 4% that the in vivo utility of the compound has thus far been limited to intraperitoneally or subcutaneously administered animal models.

US patent 4,963,662 discloses generically a series of 3'-fluorinated nucleosides and corresponding triphosphates and specifically describes the preparation of the palmitoyl derivative of FLT, without reporting any improvement in bioavailability.

International patent application WO 93 13778 describes FLG derivatives modified at the 6-position of the base, in particular with n-propoxy, cyclobutoxy, cyclopropanylamino, piperidino or pyrrolidino. International patent application no.

93 14103 describes FLG derivatives where the oxygen at the guanine 6-position is replaced with amino, ether, halo or sulphonate.

1B The above discussion of documents, acts, materials, devices, articles and the like is included in this specification solely for the purpose of providing a context for the present invention. It is not suggested or represented that any or all of these matters formed part of the prior art base or were common general knowledge in the field relevant to the present invention as it existed in Australia before the priority date of each claim of this application.

Throughout the description and claims of this specification, the word "comprise" and variations of the word, such as "comprising" and "comprises", is not intended to exclude other additives, integers or process steps.

W:1AoNOC)OELETEDJT.SPECAM748-u.doc 18. 2044 16:03 PHILLIPS ORMONDE 96141867 NO. 5567 P. 4 WO 99/09031 PCT/SE98/01467 ]Brief dsrpino h neto In 'accordance with one aspect of the invention there are provided compounds of the formula 1: wherein~: Ri is selected from hydroxy, amino or carboxy; optionally having esterified/arnide bonded there on a C 4 -C22 saturated or unsaturated, optionally substituted fatty acid or alcohol, or an aliphatic L-amnino acid;

R

2 is (he residue of an aliphatic L-arino acid;

L

1 is a trifunctional linker group;

L

2 is absent or a difunctional linker group; and Phirzaceutically. acceptable salts thereof..

a *..aaa COMS ID No: SBMI-00793881 Received by IP Australia: rime 16:22 Date 2004-06-17 '18. 2044 16:03 PHILLIPS ORMONDE 96141867 NO. 5567 P. In accordance with a further aspect of the invention there are provided compounds of formula I 0 R N NH

L

1 L2O N N NH 2 R2 0

F

wherein: Lt is glycerol;

L

2 is dicarboxylic acid selected from oxalyl, malonyl, succinyl, glutaryl, adipyl, or succinyl; RI is an aliphatic L-amino acid esterified to an hydroxy function of the glycerol;

R

2 is an aliphatic L-amino acid esterified to a second hydroxy function of the glycerol; wherein the third hydroxy function on Li is esterified to a first carboxy function of the dicarboxylic acid; wherein the second carboxy function of the dicarboxylic acid is esterified to the function of the nucleoside; and pharmaceutically acceptable salts thereof.

The invention further provides pharmaceutical compositions comprising the compounds and salts of formula I and pharmaceutically acceptable carriers or diluents therefor. Additional aspects of the invention, provide methods for the inhibition of HBV and retroviruses such as HIV, comprising bringing a compound or salt of the formula I into contact with a retrovirus or HBV, for example by administering an effective amount of the compound or salt to an individual afflicted with a retrovirus or HBV. The invention also extends to the use of the compounds or salts of formula I in therapy, for example in the preparation of a medicament for the treatment of retroviral or HBV infections.

In treating conditions caused by retrovimses such as HIV, or HBV, the compounds or salts of formula I are preferably administered in an amount of 50 to 1 500 mg W.Gotamad.sm.l6,,u,.==. 2A COMS ID No: SBMI-00793881 Received by IP Australia: Time 16:22 Date 2004-06-17 WO 99/09031 PCT/SE98/01467 3 once, twice or three times per day, especially 100 to 700 mg twice or thrice daily. It is desirable to achieve serum levels of the active melabolite of 0.01 to 100 pg/ml, especially 0.1 to 5 pg/ml.

Where R 1 is a fatty acid residue, it preferably has in total an even number of carbon atoms, advantageously decanoyl (Clo), lauryl (C 1 myristoyl (C 1 4 palmitoyl (C 16 stearoyl (C 8 eicosanoyl (C 20 or behenoyl (C 2 The fatty acid preferably has in total 10 to 22, and more preferably 16 to 20 carbon atoms, especially 18. The fatty acid may be unsaturated and have one to three double bonds, especially one double bond. Unsaturated fatty acids preferably belong to the n-3 or n-6 series. Convenient unsaturated R, groups include those derived from the monounsaturated acids myristoleic, myristelaidic, palmitoleic, palmitelaidic, n6-octadecenoic, oleic, elaidic, gandoic, erucic, brassidic acids or multiply unsaturated fatty acids such as linoleic, ylinolenic, arachidonic acid and a-linolenic acid. Preferably, however, RI as a fatty acid is saturated as these compounds tend to have superior stability and shelf life.

R as fatty alcohol residue preferably corresponds to one of the above described fatty acids. Alternatively the fatty alcohol may comprise residues of shorter alcohols, such as methanol, ethanol or propanol.

R as a saturated or unsaturated fatty acid or alcohol may optionally be substituted with up to five similar or different substituents independently selected from the group consisting of hydroxy, C 1

-C

6 alkyl, CI-C 6 alkoxy, CI-C 6 alkoxy CI-C 6 alkyl, CI-C 6 alkanoyl, amino, halo, cyano, azido, oxo, mercapto and nitro, and the like.

Suitable aliphatic amino acids for R 2 and, if present Ri, include L-alanine, L-leucine, L-isoleucine and most preferably L-valine. For ease of synthesis it is preferred that both R 2 and R, are residues of aliphatic amino acids, preferably the same residue.

The expression trifunctional in the context of the first linker group LI means that the linker has at least three functional groups, including at least two functional groups derived from respective hydroxy, amine or carboxyl groups, the amine and hydroxy WO 99/09031 S94 PCT/SE98/0 14 6 7 function(s) being available for esterification/amide bonding with the carboxy functions of RI and

R

2 whereas a carboxy function(s) on the linker is available for amide bonding w\ith the free a-amine function of R 2 or RI as the case may be, or esterification witil RI as a fatty alcohol. Where R, itself defines an hydroxy, amine or carboxy group, the hydroxy group being presently favoured of the three, one of said functions on the trifunctional linker simply comprises this hydroxy, amine or carboxy group.

The trifunctional linker further comprises a third functional group for linkage with either the optional second linker group L, illustrated in more detail below, or the hydroxy group at the 5' position of the mother nucleoside, such as 2 3 '-dideoxy.-3' Sfluoroguanosine. Appropriate third functional groups will depend on the nature of the cooperating function on optional linker group L, if present, and may include amino hydoxy, carbonyl, sulfonyl, phosphoryl, phosphonyl, carbamoyl and the like. If L 2 is absent, this third functional group on first linker L, will typically comprise a carboxyl function which can esterify with the 5'-O group of the nucleoside analogue.

Preferably the functional groups on the trifunctional linker which cooperate with R 1 and R 2 are hydroxyl functions and the linkage is an ester linkage with the carboxy 20 f ofan a ,ifp ,an ester linkage with the carboxyl 20 functions of an RI fatty acid, if present, and R 2 A further preferred embodiment comprises a free hydroxy group as R, and an hydroxyl function on the linker esterified to the carboxy function of R 2 An alternative embodiment comprises an (optionally protected) carboxyl group as RI and an hydroxyl funcion on the linker esterifed to a carboxy function on R 2 Useful trifunctional L, group, especially for esterifying directly to the nucleoside include linkers of the formula IIa or fTb: )n

RXA

Alk T-- SA' ()m WO 99/09031 PCT/SE98/01467 where A and A' define a respective ester linkage between an hydroxy on the linker and the carboxy on R 1 or R 2 or an ester linkage between a carboxy on the linker and the hydroxy on RI as a fatty alcohol, or an amide linkage between an amine on the linker and a carboxy on R, or R 2 or an amide linkage between a carboxy on the linker and an amine on R, or R 2 or one of A and A' is as defined and the other is hydroxy, amino or carboxy in the event that R 1 itself is a free hydroxy, amino or carboxy group.

Rx is H or CI-C 3 alkyl, T is a bond, or -NH-; Alk is absent, C|-C 4 alkyl or C 2

C

4 alkenyl, optionally substituted as described above; and m and n are independently 0, 1 or 2.

In a preferred embodiment of this aspect of the invention, the RI or R 2 groups are each esterified to a respective one of the leftmost functional hydroxy groups (viz A and of Formula IIa, while the carbonyl moiety to the right is esterified, optionally via a second linker group L 2 to the 5'-O-group of the nucleoside.

Alternatively the L, group may comprise a linker of the formula IIb: 0 Ar -Alk-T lib where Ar is a saturated or unsaturated, preferably monocyclic carbo- or heterocycle with 5 or 6 ring atoms; and A, T, Alk, m and n are as defined above.

1 WO 99/09031 6 PCT/SE98/0146 7 In Formula ib, Ar is preferably an aromatic group such as pyridine or especiaily phenyl, such as aromatic moieties wherein the arms bearing the R, and R 2 groups are respectively para and ortho, meta and ortho, both ortho, or preferably para and meta, both para or both meta to the remainder of the linker.

In formulae Ha and IIb, the following combinations of m, n and Alk are presently favoured: m n Alk 1 0 methylene 1 0 ethylene 1 absent I* methylene I ethylene :1 1 propylene 15 1 2 absent 2 methylene I ethenylene i 1 propenylene As RI and R, may have different structures, it will be apparent that many L, groups, particularly those of formula Ia, will define chiral structures and the invention includes all enantiomers thereof, as racemates or as preparations of 80%, preferably 95% enantiomerically pure compound.

A particularly preferred group of trifunctional linkers comprise glycerol derivatives of the formula IIc

A-O-

-A 0- D-

A'-O-

IIc where A is hydrogen, the acyl residue of an aliphatic L-amino acid ester or the acyl residue of a fatty acid ester, A' is the acyl residue of an aliphatic amino acid residue WO 99/09031 7 PCT/SE98/01467 and D is a C 2

-C

6 saturated or unsaturated dicarboxylic acid residue. Trifunctional linkers of the formula ic are hydrolysed or otherwise break down in vivo to release the nature identical compounds glycerol, the L-amino acid, the fatty acid (if present) and the dicarboxylic acid, each of which are generally safely metabolised and/or excreted by the body. Preferably A and A' are both residues of an aliphatic amino acid, most preferably the same residue, particularly residues of L-valine or Lisoleucine.

In the event that the dicarboxylic acid moiety in the derivative of formula IIc is esterified directly to the 5' hydroxy function (or equivalent) on the nucleoside, an alternative analysis would be to define the glycerol moiety as trifunctional linker L, and the dicarboxylic acid moiety as difunctional linker L 2 SParticularly preferred dicarboxylic acid residues include those derived from 15 oxalic, malonic, tartronic, succinic, maleic, fumaric, malic, tartaric, glutaric, glutaconic, citraconic, itaconic, ethidine-malonic, mesaconic, adipic, allylmalonic, •propylidenemalonic, hydromuconic, pyrocinchonic and muconic acids and the like.

The dicarboxylic acid residue may be optionally substituted, for example with the substituents listed above in respect of R, as a fatty acid. Hydroxy substituents can in turn be esterified with a further L-amino acid or fatty acid residue.

**e Several of the abovementioned dicarboxylic acids can themselves define a 9 S trifunctional linker. For instance hydroxy-substituted dicarboxylic acids such as tartaric acid or malic acid offer a number of configurations within the scope of the invention. Taking tartaric acid as an example a carboxyl function is available for esterification with the 5'-hydroxyl function of a nucleoside (optionally via difunctional linker L 2 The hydroxy functions are available for esterification with the respective carboxyl functions of R 2 and an RI fatty acid or amino acid while the remaining carboxy group can be free, or optionally protected, for instance with a conventional pharmaceutically acceptable ester such as the methyl or ethyl ester.

Alternatively the optional protection of the free carboxy function can itself comprise WO 99/09031 8 PCT/SE98/01 4 6 7 an ester with an R, fatty alcohol, with one or both hydroxyl functions being esterified to R 2 R1 R 2 RO O HO O O-nuc O-nuc Favoured linkers of the tartaric acid series above can be generically depicted as Formula IHe:

R

i RYO--- P -L-0q_ 0r IO I 0 0

II

R2 lie S and isomers where R, and R 2 are reversed, where RI and R 2 are as shown above, p, q and r are each independently 0 to 5, preferably 0 or I and Ry is the free acid, an RI ester or a conventional pharmaceutically acceptable carboxy protecting group, such as the methyl,benzyl or especially the ethyl ester.

Favoured linkers of the malic series have the formula Hf: R2 O

O

IIf where Ry, p,q and R 2 are as defined above, preferably those where p and q are zero.

Preferred compounds of this aspect of the invention thus include: WO 99/09031 PCT/SE98/01 467 9 -O-[3-methoxycarbonyl-2-valyloxy-propionyl]-2' ,3 '-dideoxy-3' -fluoroguanosine, -O-[3-benzyloxycarbonyl-2-valyloxy-propionyl]-2' ,3 '-dideoxy-3 '-fluoroguanosine, -O-[3-methoxycarbonyl-2-isoleucoxy-propionyl]-2' ,3 '-dideoxy-3' fluoroguanosine, 5' -O-[3-benzyloxycarbonyl-2-isoleucyloxy-propionyl]-2' ,3'-dideoxy-3 fluoroguanosine, -O-[4-methoxycarbonyl-2,3-bis-valyloxy-butyryl]-2' ,3 '-dideoxy-3' fi uoroguanosine, -O-[4-benzyloxycarbonyl-2,3-bis-valyloxy-butyryl]-2' ,3 '-dideoxy-3' fluoroguanosine, -O-[4-methoxycarbonyl-2,3-bis-isoleucyloxy-butyryl]-2' ,3 '-dideoxy-3 fluoroguanosine, 5' -O-[4-benzyloxycarbonyl-2,3-bis-isoleucyloxy-butyryl]-2' -dideoxy-3' :fluoroguanosine; particularly those derived from L-malic acid and L-tartaric acid; and corresponding derivatives employing conventional pharmnaceutically acceptable esters on the termninal carboxy function.

Particularly favoured compounds include: 5 '-O-[3-ethoxycarbonyl-2-valyloxy-propionyl]-2' ,3 '-dideoxy-3' -fluoroguanosine, -O-[3-ethoxycarbonyl-2-isoleucyloxy-propionyl]-2' ,3 '-dideoxy-3' fluoroguanosine, S '-O-[4-ethoxycarbonyl-2,3-bis-valyloxy-butyryl]-2' -dideoxy-3 '-fluoroguanosine, -O-[4-ethoxycarbonyl-2,3-bis-isoleucyloxy-butyryl]-2' ,3 -dideoxy-3 fluoroguanosine, expecially the isomers derived from L-malic and L-tartaric acid.

In a related alternative aspect of the invention one of R, and R 2 is omitted.

Representative compounds of this aspect of the invention include those of the formual la: WO 9/003110 PCT/SE98/014 6 7 0 0 N R Al N: N j'NH 2 F la where Alk is optionally substituted

C

1

-C

4 alkyl or C, C 4 alkenyl and Rz is the ester residue of an aliphatic L-amino acid or a fatty acid as defined for R, and R, above.

Linkers of this aspect of the invention are conveniently prepared from ct-hydroxy wcarboxylic acids such as carbonic acid, glycollic acid, hydroxypropanoic acid, hydoxbutri acdhydroxyvaleric aiorhydroxycaproicacd :Representative compounds of Formula ]a include: 2' ,3 '-dideoxy-3 '-fluoro-5 5 -(L-valyloxy)-pentanoylhJ gu anosine, -dideoxy-3 '-fluoro-5 6 -(L-valyloxy)-hexanoyl] guanosine, 2' ,3'-ie 'y3-fluoro-5.0-[3(L-isoleuc lyoxy)-propionyl] guanosine 2' ,3'-dideoxy- 3'-fl uoro-5 [5-(L-isol eucylIox y)pe ntan oy I] guanosine, 2',37-uiueoxy-3'- uoro5 O46(Lisolel)-heaol guanosine, and pharmaceutically acceptable salts thereof.

Particularly favoured compounds of formula la include: 2' ,3'-dideoxy-3 '-fluoro-5 '-O-[4-(L-valyloxy)-butyryl] gu anosine; and 2' ,3'-dideoxy-3 '-fluoro-5

'O

4 4 -(L-isoleucyloxy).butyryi] guanosi ne and pharmaceutically acceptable salts thereof. In these compounds hydrolysis and removal of the R 2 group in vivo leaves a reactive terminal radical which will tend to cyclize and prompt the effective release of the mother nucleoside.

In a related alternative aspect of the invention, R, as a fatty acid residue is itself used as the linker, with the aliphatic L-amino acid residue of R 2 being esterified/amide bonded to an amino, hydroxy or carboxy function on the fatty acid alkyl chain, for PCT/SE98101467 WOl 99/09031PCIE8O16 example on the P-carbon. In this embodiment the fatty acid of R, is esterified directly on the 5'-hydroxy (or equivalent) function of the nucleoside, generally with the R 2 group already esterified/amide bonded thereon. Alternatively, the functionalised fatty acid (the carboxy/hydroxy/amino function being appropriately protected) can be first esterified to the nucleoside and deprotected prior to coupling with R 2 Linkers in accordance with a preferred embodiment of this aspect have the formula fld: 0 0 H 3 0- 0P-N lid where R 2 is the residue of an aliphatic L-amino acid and, p is 0, 1 or 2-20 (optionally including a double bond) and q is 0-5, preferably 0. Representative compounds include: 2' ,3'-dideoxy-3'-fluoro-5-O-[2-(L-valyloxy)-butyryl] guanosine, 2' ,3 '-dideoxy-3 '-fluoro-5-O-[2-(L-valyloxy)-hexanoyl] guanosine, 2' ,3'-dideoxy-3 '-fluoro-5-O-[2-(L-valy loxy)-octanoyl] guanosine, 2' ,3 '-dideoxy-3 '-fluoro-5-O-[2-(L-valyloxy)-decanoyl] guanosine, -dideoxy-3 '-fluoro-5-O-[2-(L-valyloxy)-dodecanoyl] guanosine, 2' ,3'-dideoxy-3 '-fluoro-5-O-[2-(L-valyloxy)-myristoyl] guanosine, 2' ,3'-dideoxy-3 '-fluoro-5 alylIo xy)-pal mi toy I] guanosine, 2',3'-dideoxy-3'-fluoro-5-0-[2-(L-valyloxy)-stearoyl] guanosine, 2' ,3 '-dideoxy-3 '-fluoro-5-0-[2-(L-valyloxy)-docosanoyl] guanosine, 3' -dideoxy-3'-fluoro-5-O-[2-(L-valyloxy)-eicosanoyl] guanosine 2' ,3 '-dideoxy-3 '-fluoro-5-0-[2-(L-isoleucyloxy)-butyryl] guanosine, 2' ,3 '-dideoxy-3 '-fluoro-5-04[2-(L-isoleucyloxy)-hexanoyl] guanosine, 3' -dideoxy-3'-fluoro-5-O-1j2-(L-isoleucyloxy)-octanoyl) guanosine, 2' ,3 '-dideoxy-3 '-fluoro-5-O-[2-(L-isoleucyloxy)-decanoy]] guanosine, 3' -dideoxy-3' -fluoro-5-O-f12-(L-isoleucyloxy)-dodecanoyl] guanosine, 2' ,3'-dideoxy-3 '-fluoro-5-O-[2-(L-isoleucyloxy)-myristoyl] guanosine, 2' ,3'-di deoxy -3 '-fluoro-5-O- (L-is ol eucy Ioxy)-p al mitoy]) guanosine, WO 99/09031 12 PCT/SE98/0146 7 2',3'-dideoxy-3'-fluoro-5-0-[2-(L-isoleucyoxy)-stearoyl] guanosine, 2',3'-dideoxy-3'-fluoro-5-O-[2-(L-isoleucyloxy)docosanoyl] guanosine, 2',3'-dideoxy-3'-fluoro-5-0-[2-(L-isoleucyloxy)-eicosanoyl] guanosine, and the corresponding n-3 and n-6 monounsaturated analogues, such as 6 or 9 octadecenoyl derivatives.

In formula IId, p and q are preferably 0, thus defining lactic acid derivatives, preferably L-lactic acid derivatives, such as 2',3'-dideoxy-3'-fluoro-5-O-[2-(L-valyloxy)-propionyl] guanosine; and 2',3'-dideoxy-3'-fluoro-5-O-[2-(L-isoleucyloxy)-propionyl] guanosine and pharmaceutically acceptable salts thereof, as the breakdown products, lactic acid and i the amino aicd are both well accepted physiologically.

The expression bifunctional in the context of second linker group L 2 means that the the linker has two functions enabling it to act a spacer or bridge between the first linker group L 1 and the 5'-O group of the nucleoside. For instance the optional group

L

2 may comprise a linker of the formula IIIa: 4 O 0 -0

O-P-

R

4

H

Illa where R 4 and R 4 are hydrogen or CI-C 4 alkyl. In formula ma, R 4 is preferably hydrogen, methyl, ethyl or isopropyl and 4' is hydrogen. Linkers of formula lIIa are convenient as many nucleosides such as the FLG mother compound must first be phosphorylated by cellular enzymes before it can inhibit the viral polymerase. An initial or sequential hydrolysis of compounds of the invention can release a monophosphorylated nucleoside in vivo which is available for immediate conversion to the di- and triphosphate.

Alternatively the optional bifunctional linker group

L

2 may comprise a structure of the formula MIIb: WO 99/09031 PCT/SE98/01467 WO 99/09031 PCT/SE98/01467 13

R

4 0 -0--0o O0- R4 Illb where R 4 and R 4 'are independently H or C 1

-C

4 alkyl.

A still further group of bifunctional linkers have the formula mIc: R4 Illc As described above, a preferred group of bifunctional linkers comprises a,toto dicarboxylic C 2

-C

6 alkyl derivatives, such as succinic acid, which are optionally substituted (for instance with the substituents defined above for R, as a fatty acid) and/or optionally mono or polyunsaturated, such as n-3 or n-6 monounsaturated.

Preferred moieties within this class are listed above.

Although the disclosure above has concentrated on glycerol LI groups in conjunction with dicarboxylic L 2 groups, it will be appreciated that a wide variety of trifunctional linkers are appropriate with dicarboxylic L 2 groups, for instance structures of the formula IIa and IIb above lacking the rightmost carbonyl.

The invention further includes double prodrugs comprising Ri(R 2 LiL 2 -derivatives of conventional FLG prodrugs, which conventional prodrugs release FLG in vivo, such as prodrug derivatives at the 2 and 6 positions of the FLG guanine base.

Examples of such conventional FLG-prodrugs include compounds of the formula

IV:

WO 99/09031 S99/0903114 PCT/SE98/0146 7

R

3 R N R3

R

1 L1L2-0O N

N

R

2 F

IV

where RI, R 2

L

1 and L 2 are as defined above; and

R

3 is H, N 3

NH

2 or OH or a pharmaceutically acceptable ether or ester thereof; and

R

3 is an aromatic bond or hydrogen; Potential pharmaceutically acceptable esters for R 3 include the fatty acids described .i in relation to R, above, such as stearolyl, oleoyl etc or shorter esters such as acetyl or butyryl. Other potential esters include the amino acid derivatives of R 2 or esters of phosphoric acid, such as monophosphate. Alternative esters include the corresponding fatty acid or alkylaryl carbonate, carbamate or sulphonic esters.

Suitable pharmaceutically acceptable ethers for R 3 include

CI-C

6 alkyl, cycloalkyl,

C

6 -Cl2 alkaryl such as benzyl or methylpyridyl, any of which may be optionally substituted as for R, above. Convenient ethers include those described in the abovementioned WO 93 13778 such as n-propoxy, cyclobutoxy, cyclopropanylamino, piperidino or pyrrolidino and the like.

The invention has thus far been described with reference to the monohydroxylated nucleoside FLG, however it will be apparent that corresponding derivatives can be prepared of other monohydroxylated nucleoside analogues, particularly those where the monohydroxy group corresponds to the 5' hydroxy function of a nucleoside. Thus an additional aspect of the invention provides compounds of the formula Ic: wn Q9Q/9031 PCT/SE98/0167 Rl\

L

1

L

2 -O-nuc

R

2 Ic where R 1

R

2 Li and L 2 are as defined above and O-nuc is the residue of a monohydroxyl bearing D- or L-nucleoside analogue. Representative nucleosides in accordance with this aspect of the invention include acyclic nucleoside analogues such as acyclovir and cyclic nucleoside analogues such as ddl (didanosine), ddC (zalcitabine), d4T (stavudine), FTC, lamivudine (3TC), 1592U89 (4-[2-amino-6- (cyclopropylamino)-9H-purin-9-yl]-2-cyclopentene-l-methanol), AZT (zidovudine), DAPD (D-2,6-diaminopurine dioxolane), F-ddA and the like, each of which are well 10 known in the nucleoside art. A number of monohydric L-nucleosides are under development and the invention will also find utility on this compounds. Compounds within this aspect of the invention will find utility in the corresponding indications to the mother compounds, for instance herpesvirus infections for acyclovir derivatives, HIV for ddl, stavudine, ddC, lamivudine, AZT 1592U89, HBV for lamivudine, FTC etc.

A favoured subgroup within Formula Ic comprises derivatives of monohydric nucleosides of the formula Ic': A-O- 0 0 0 I Alk IO-nuc

A'-O-

Ic' where A, Alk and O-nuc are as defined above. Formula Ic' above depicts compounds wherein A and A' depend from the 1 and 3 positions of the glycereol moiety and L 2 depends from the glycerol 2 position. In alternative isomers A and A' depend 1 and 2 or 2 and 3 and L 2 from 3 or 2 respectively.

Representative compounds within this aspect of the invention include: 4'-O-[3-((2,3-bis-L-valyloxy)- -propyloxycarbonyl)propionyl] acyclovir, WO 99/090 31 PTS9/16 16 PTS9/16 4' -O-[3-((2-hydroxy-3-.Lvalyloxy) l-propyloxycarbonyl)propionyl] acyclovir, 4' 3 2 3 -bis-b..-isoleucyloxy)-. -propyloxycarbonyl)propionyl] acyclovir, 4' 3 -((2-hydroxy3-Lisoleucyloxy) I -propyloxycarbony])propionyl] acyclovir, 4' 3 -bis-L-valyloxy)-2..propyI oxycarbony])propionyl] acyclovir, 4' -yrxy3Lvlyoy--poyoycroy)prpon acyclovir, 4'

I,

3 -bis-L-isoleucyloxy-2-propyloxycarbon1)poionl] acyclovir, 4' I-hydroxy-3Lisoeucyoxy)2propyloxycarbony)poinj acyclovir, -O-[3-((2,3-bis-Lvalyloxy)-I-propyioxycarbonyl)propionyl] lamivudine, 3 -((2-hydroxy-3-L-valyloxy) -propyloxycarbonyl)propionyj] lamivucline, 5'-O-[3-((2,3-bis-L-isoleucyloxy)-propyloxycarbonyl)propionyl] lamivudine, 3 -((2-hydroxy-3-Lisoleucyloxy)- -propyloxycarbonyl)propionyl] lamivudine,

I,

3 -bis-Lvayloxy)2propy]oyaroylpoonyl] lamivudine, ~'JO-[3Ihydroxy---ay3LII)-2-poyoyabnlpoin lamivudine, 3 -bis-L-iso eucv-2prpoxn r1n.,l~p.,\....lmiud 5' I-hdoy3Lioeclx)2poyoyabnlpoin lamivudine, 5'--[3((,3-is--vlylxy)l-r'-pJAlJAYaruuoy)popionyJJDAD b-hydroxy3-LvLy so euc-royloxy)roylobi). ami udne 3 -((2,3-bis-Lvasleyloxy-l-propyloxycarbonyl)propionyl]

DAPD,

3 -((2-hydroxy-3..L.valyloxy)-I-propyloxycarbony])propionyl]

DAPD,

3 3 -bis-L-isoeucyoxy)propyoxycabonlpoin

DAPD,

3 2 -hydroxy-3-L-isoleucyloxy)-I-propyloxycarbonyl)propi oryl] DAPD, 5'-O-[3-((1-yrx--Lvllx) I -poyoyabnlpoio]-2, -O-[3-((23bsLioeclx) I DAPDxcrbnl~rponl-2,' I2-ydos-Lisoeucyoxy)- propyloxycrbony1)propoDAPD2,3 -idO-[3-((siDAPD 3 1 3-bis-L-valyloxy)-2 -propyloxycarbonyl)propionyl]-2' ,3 '-dideoxyinosine, WO 99/09031 17PCT/SE98/01 467 I -hydroxy-3-L-valyloxy)-2-propyloxycarbonyl)propionyll-2' dideoxyinosine, -O-[3-((l1,3-bis-L -isoleucyloxy)-2-propyloxycarbonyl)propionyl]-2' ,3 dideoxyinosine, 5' 1-hydroxy-3-L-isoleucyloxy)-2-propyloxycarbonyl)propiony ,3 dideoxyinosine, -bi s-L-v al yloxy)- I -propylIoxycarbonylI)propi onyl ]stavu dine, [3 -((2-hydroxy-3 -L-val yloxy)- I -propyl oxycarbonylI)propi onyl] stavu dine, -O-[3-((2,3-bis-L-isoleucyloxy)-1I-propyloxycarbonyl)propionyl] stavudine, 5' -O-[3-((2-hydroxy-3-L-isoleucyloxy)- 1-propyloxycarbonyl)propionyl] stavudine, 1,3-bis-L-valyloxy)-2-propyloxycarbonyl)propionyl] stavudine, *0 5' 1-hydroxy-3-L-valyloxy)-2-propyloxycarbonyl)propionylj stavudine, 1 -i -s l u y o y -r p l x c r o y r p o y] s a u i e I -biso--L-isoleucyloxy)-2-propyloxycarbonyl)propionyl stavudine, the corresponding derivatives of 4-[2-amino-6(cyclopropyl amino)-9H-purin-9-yl] -2cyclopentene-1 -methanol, and pharmaceutically acceptable salts thereof.

An alternative subset of compounds within this aspect of the invention comprise those of the formula Id: *000 0 Rz Ak-"--nuc Id where Rz and Alk are as defined for formula la and 0-nuc is as defined above.

Representative compounds of formula Id include 4'-O-[4-(L-valyloxy)-propionyl] acyclovir, [5-(L-valyloxy)-pen tan oyl acyclovir, 4'-O-[6-(L-valyloxy)-hexanoyl) acyclovir, 4'-O-[4-(L-isoleucyloxy)-propionyl] acyclovir, WO 99/09031 18 PCT/SE98/01 467 4' -O-[5-(L-isoleucylOxy)-pentanoyij acyclovir, 4' 6 -(L-isoleuoyloxy)-hexanOyI] acyclovir, 4 -(L-valyloxy)-propionyl] ddI, '-O-[5-(L-valyloxy)-pentanoyl] ddl, 6 -(L-valyloxy)-hexanoyl] ddl, 4 -(L-isoleucyloxy)-propionyl] ddl, ddJ, 6 -(L-isoleucyloxy)-hexanoylj ddl, 4 -(L-valyloxy).propionyl] stavudine, 5'-O-IIS-(L-valyloxy)-pentanoyil stavudine, 6 -(L-valyloxy)-hexanoyJ] stavudine, 4 -(L-isoleucyloxy)-propionyij stavudine, 5'-O-[5-(L-isoleucyloxy)-pentanoy]] stavudine, 6 -(L-isoleuc yloxy)..hexanoyl] stavudine, 15 4 -(L-valyloxy).propionyl]

DAPD,

5'-O-[5-(L-valyloxy)-pentanoyl

DAPD,

6 -(L-valyloxy)-hex anoyl]

DAPD,

4 -(L-isoleucyloxy)-.propionyI]

DAPD,

oxy) -pen tanoyl]

DAPD,

20 6 -(L-isoleucyloxy)-hexanoyl]

DAPD,

4 -(L-valyloxy)-propionyl] lamivudine, lmvdne, 6 -(L-valyloxy)-hexanoyl] lamidvudine, 4 -(L-isoleucyloxy)-propionyl] lamivudine, 5'-O-[5-(L-isoleucyloxy)-pentanoyl] lami vudine, 6 -(L-isoleucyloxy)-hexanoyl] lami vudine, and the corresponding derivatives of 4 2 -amino-6(cyclopropyl amino)-9H-purin-9yl 2 -cycl open tene- I -methanol.

Particularly preferred compounds within Formula Id include: WO 99/09031 19PCT/SE98/01 467 4'-O[4-(-valloxy-butryl~cyclv 19 4' -O-[4-(L-valeyloxy)-butyryl]acyclovir, 4' -O-[3-(L-isoleyloxy)-butyryl]acyloir -O-[4-(L-vaoleyloxy)-butyryl] ddl, 5'-O-[3-(L-ioleyloxy)-butyryll avddl, 55'-O-[4-(L-valeyloxy)-butyryl] stavudine, -O-[3-(L-soleyloxy)-butyryl] staudne 5'-O-[4-(L-valeyloxy)-butyryl] DAPD, 5'-O-[3-(L-isoleyloxy)-butyryl] DAPivDi, io 5' -O-[4-(L-valeyloxy)-butyrylllamivudine, and the corresponding derivatives of 4- [2-amino-6(cycl opropylamino)-9H-purin-9yl]-2-cyclopentene- 1-methanol; and pharmaceutic ally acceptable salts thereof, :In these compounds hydrolysis and removal of the R 2 group in vivo leaves a reactive terminal radical which will tend to cyclize and prompt the effective release of the mother nucleoside.

Similarly the invention extends to compounds of the formula If: 0 0 R-0 7 I Or Y 0 P0 R2 If where Ri, R 2 RY, p, q, r and o-nuc are as defined above.

Favoured compounds of this aspect of the invention include: -0-[3-ethoxycarbonyl-2-valyloxy-propionyl]-ddI, -O-[3-ethoxycarbonyl-2-isoleucyloxy-propionyl]-ddI -O-[4-ethoxycarbonyl-2,3-bis-valyloxy-butyryl)-ddl, 5' -O-[4-ethoxycarbonyl-2,3-bis-isoleucyloxy-butyryl]-ddI, 4' -O-[3-ethoxycarbonyl-2-valyloxy-propionyl]-acyclovir, 4' -0-[3-ethoxycarbony]-2-isoleucyloxy-propionyl]-acyclovir WO 99/09031 20 PCT/SE98/0146 7 4' 4 -ethoxycalrbonyl23bisvalJ oxyb uyy]ail v 4' 4 ethoxycarb ony .23bisoleuoybuyy]ailvr

-O[

3 ethoxycarbon2-ylaoxyproiIDD, 3 -ethoxycarbon isoleucy j. prponl-DAPD 4 -ethoxycarbonyl23bis-vallxbutrl-AD 4 -ethoxycarbonyl23bissluyoybtr 1 -AD 3 -ethoxycarbonyl2va yl oxyproi nlj sa ie 3 -ethoxycarbonyl2isoleuloyppinlstvde 4 -ethoxycarbonyl23bisvallybuyy]sadie i 3 -ethoxycarbonyl-2valyloxy-prop*ioy]- aivui 5*O[-toyabnl2-sluyoypoinl -1 ami vu dine 4 ethoxycarbony2,3bisvayoxy-butylmidi 4 -ethoxycarbonyb-2,3bis-isoleucyloxybutyryI]-laiune and the corrresponding malic and tartric derivatives of 4 2 -amino- 6 (cyclopropyl aino)9Hpuri n 9y] 2 cIoe ee I -methanol and pharpamceutically acceptable salts thereof; in each case the isomers derived from Ltartrate and L-malate derivatives being preferred.

The invention also extends to compounds of the formula Ig 0 12 0 0 Ig where

R

2 p, q and 0-nuc are as defined above.

Preferred compounds of formula Ig include: 4 2 -(L-valyloxy)-propionyl] acyclovir, 4 2 -(L-isoleucyloxy)-propionyl] acyclovir 2 -(L-valyloxy)-propiony] ddl, 2 -(L-isoleucyloxy).propionyl] ddl, 2 -(L-valyloxy)-propionyl] stavudine, WO 99/09031 21WO 99/09031 PCT/SE98/01467 2 -(L-isoleucyloxy)-propionyl] stavudine 2 -(L-valyloxy)-propionyl] lamivudine, 2 -(L-isoleucyloxy)-propionyl] lamivudine, 2 -(L-valyloxy)-propionyl]

DAPD,

5 2 -(L-isoleucyloxy)-propionyl

DAPD

and the corresponding derivatives of 4 2 -amino-6(cyclopropylamino)-9H-purin-9yl]- 2 -cyclopentene- I-methanol;and pharmaceutically acceptable salts thereof.

The breakdown products of such compounds, actic acid and the amino acid, are both well accepted physiologically.

The compounds of the invention can form salts which form an additional aspect of the invention. Appropriate pharmaceutically acceptable salts of the compounds of Formula I include salts of organic acids, especially carboxylic acids, including but not limited to acetate, trifluoroacetate, lactate, gluconate, citrate, tartrate, maleate, malate, pantothenate, isethionate, adipate, alginate, aspartate, benzoate, butyrate, digluconate, cyclopentanate, glucoheptanate, glycerophosphate, oxalate, heptanoate, hexanoate, fumarate, nicotinate, palmoate, pectinate, 3 -phenylpropionate, picrate, *pivalate, proprionate, tartrate, lactobionate, pivolate, camphorate, undecanoate and succinate, organic sulphonic acids such as methanesulphonate, ethanesulphonate, 2 -hydroxyethane sulphonate, camphorsulphonate 2 -napthalenesulphonate, :Ibenzenesulphonate p-chlorobenzenesulphonate and p-toluenesulphonate; and inorganic acids such as hydrochloride, hydrobromide, hydroiodide, sulphate, bisulphate, hemisulphate, thiocyanate, persulphate, phosphoric and sulphonic acids.

The compounds of Formula I may in some cases be isolated as the hydrate.

The term "N-protecting group" or "N-protected" as used herein refers to those groups intended to protect the N-terminus of an amino acid or peptide or to protect an amino group against undesirable reactions during synthetic procedures. Commonly used Nprotecting groups are disclosed in Greene, "Protective Groups in Organic Synthesis" (John Wiley Sons, New York, 1981), which is hereby incorporated by reference.

N-protecting groups include acyl groups such as formyl, acetyl, propionyl, pivaloyl, tbutylacetyl, 2 -chloroacetyl, 2 -bromoacetyl, trifluoracetyl, trichloroacetyl, phthalyl, o- WO 99/09031 PTS9/16 22PC/E8'16 nitrophenoxyacetyl, cx-chlorobutyryl, benzoyl, 4 -chlorobenzoy], 4 -bromobenzoy], 4nitrobenzoyl, and the like; sulfonyl groups such as benzenesulfonyl, ptoluenesulfonyl, and the like, carbamnate forming groups such as benzyloxycarbonyl, p-chlorobenzyloxycarbonyl, p-methoxybenzy loxycarbonyl, p-nitrobenzyloxycarbonyl, 2 -nitrobenzyloxycarbonyl, P-bromobenzyloxycarbonyl, 3 4 -dimethoxybenzyloxycarbonyl, 4 -methoxybenzyloxycarbonyl, 2 -nitro- 4 5 -dimethoxybenzyloxycarbonyl, 3 ,4,5-tri methoxybenzyboxycarbonyl, I -(p-biphenylyl)- I-methylethoxycarbonyl, di methoxybenzyloxycarbonyl, benzhydryl oxycarbony I, t-butoxycarbonyl, diisopropylmethoxycarbony1, isopropyloxycarbonyl, eth oxycarbonyl, methoxycarbonyl, allyloxycarbonyl, 2,2,2-trich loroethoxycarbonyl, phenoxycarbonyl, 4 -nitrophenoxycarbonylfurn-9mtoyabnl y petlxcroy, adamantyloxycarbony], cyclohexyloxycarbonyl, phenyithiocarbonyl, and the like; alkyl gropus scasbenzyl, triphenylmethyl, benzyloxymethyl adtelk;and silyl groups such as trimethylsilyl and the like. Favoured N-protecting groups include formyl, acetyl, allyl, F-moc, benzoyl, pi val oyl, t-butylacetyl, phenylsulfonyl, benzyl, t-butoxycarbonyl (B DC) and benzyloxycarbonyl (Cbz).

Hydroxy and/or carboxy protecting groups are also extensively reviewed in Greene ibid and include ethers such as methyl, substituted methyl ethers such as methoxymethyl, methylthiomethyl, benzyloxymethyl, t-butoxymethyl, 2methoxyethoxymethyl and the like, silyl ethers such as trimethylsilyl (TMS), tbutyldimethylsilyl (TBDMS) tribenzylsilyl, triphenylsiiyl, t-butyldiphenylsi]l triisopropyl silyl and the like, substituted ethyl ethers such as Il-ethoxymethyl, I methyl- I -methoxyethyl, t-butyl, ally], benzyl, p-methoxybenzyl, dipehenylmethyl, triphenylmethyl and the like, aralkyl groups such as trityl, and pixy] 9 -hydroxy.9phenylxanthene derivatives, especially the chloride). Ester hydroxy protecting groups include esters such as formnate, benzylformate, chloroacetate, methoxyacetate, phenoxyacetate, pivaloate, adamantoate, mesitoate, benzoate and the like. Carbonate hydroxy protecting groups include methyl vinyl, allyl, cinnamyl, benzyl and the like.

WO 99/09031 PCT/SE98/01467 23 In keeping with the usual practice with retroviral and HBV inhibitors it is advantageous to co-administer one to three or more additional antivirals, such as AZT, ddl, ddC, d4T, 3TC, H2G, foscarnet, ritonavir, indinavir, saquinavir, nevirapine, delaviridine, Vertex VX 478 or Agouron AG1343 and the like in the case of HIV or lamivudine, interferon, famciclovir etc in the case of HBV. Such additional antivirals will normally be administered at dosages relative to each other which broadly reflect their respective therapeutic values. Molar ratios of 100:1 to 1:100, especially 25:1 to 1:25, relative to the compound or salt of formula I will often be convenient. Administration of additional antivirals is generally less common with 10 those antiviral nucleosides intended for treating herpes infections.

While it is possible for the active agent to be administered alone, it is preferable to present it as part of a pharmaceutical formulation. Such a formulation will comprise the above defined active agent together with one or more acceptable carriers/excipients and optionally other therapeutic ingredients. The carrier(s) must be acceptable in the sense of being compatible with the other ingredients of the formulation and not deleterious to the recipient.

The formulations include those suitable for rectal, nasal, topical (including buccal and sublingual), vaginal or parenteral (including subcutaneous, intramuscular, intravenous and intradermal) administration, but preferably the formulation is an orally administered formulation. The formulations may conveniently be presented in unit dosage form, e.g. tablets and sustained release capsules, and may be prepared by any methods well known in the art of pharmacy.

Such methods include the step of bringing into association the above defined active agent with the carrier. In general, the formulations are prepared by uniformly and intimately bringing into association the active agent with liquid carriers or finely WO 99/09031 24 PCT/SE98/01467 divided solid carriers or both, and then if necessary shaping the product. The invention extends to methods for preparing a pharmaceutical composition comprising bringing a compound of Formula I or its pharmaceutically acceptable salt in conjunction or association with a pharmaceutically acceptable carrier or vehicle. If the manufacture of pharmaceutical formulations involves intimate mixing of pharmaceutical excipients and the active ingredient in salt form, then it is often preferred to use excipients which are non-basic in nature, i.e. either acidic or neutral.

Formulations for oral administration in the present invention may be presented as 10 discrete units such as capsules, cachets or tablets each containing a predetermined amount of the active agent; as a powder or granules; as a solution or a suspension of the active agent in an aqueous liquid or a non-aqueous liquid; or as an oil-in-water liquid emulsion or a water in oil liquid emulsion and as a bolus etc.

With regard to compositions for oral administration tablets and capsules), the term suitable carrier includes vehicles such as common excipients e.g. binding agents, for example syrup, acacia, gelatin, sorbitol,:tragacanth, polyvinylpyrrolidone (Povidone), methylcellulose, ethylcellulose, sodium carboxymethylcellulose, hydroxypropylmethylcellulose, sucrose and starch; fillers and carriers, for example corn starch, gelatin, lactose, sucrose, microcrystalline cellulose, kaolin, mannitol, dicalcium phosphate, sodium chloride and alginic acid; and lubricants such as magnesium stearate, sodium stearate and other metallic stearates, glycerol stearate stearic acid, silicone fluid, talc waxes, oils and colloidal silica. Flavouring agents such as peppermint, oil of wintergreen, cherry flavouring or the like can also be used.

It may be desirable to add a colouring agent to make the dosage form readily identifiable. Tablets may also be coated by methods well known in the art.

WO o/lnn31 PCT/SE98/01467 A tablet may be made by compression or moulding, optionally with one or more accessory ingredients. Compressed tablets may be prepared by compressing in a suitable machine the active agent in a free flowing form such as a powder or granules, optionally mixed with a binder, lubricant, inert diluent, preservative, surface-active or dispersing agent. Moulded tablets may be made by moulding in a suitable machine a mixture of the powdered compound moistened with an inert liquid diluent. The tablets may be optionally be coated or scored and may be formulated so as to provide slow or controlled release of the active agent.

44** 10 Other formulations suitable for oral administration include lozenges comprising the active agent in a flavoured base, usually sucrose and acacia or tragacanth; pastilles comprising the active agent in an inert base such as gelatin and glycerin, or sucrose and acacia; and mouthwashes comprising the active agent in a suitable liquid carrier.

compound of Formula I or Ic comprising the acylation of the nucleoside, represented *e here by FLG, Formula V, typically at the 5' hydroxy group: 3 R 3

SR

3 X 3 HO N N NH 2 RO NNH *0 F V F IV in which RI(R2)LIX represents an activated acid, such as the carboxylic derivatives of Formula HIa or IIb, where RI, R2, and L, are as defined above or protected derivatives thereof. Alternatively the activated acid may comprise a compound of the formula RI(R2)glycerol-D-X, where Ri, R2 and D are as defined in formula IIc or an activated Rz-O-Alk-C(=O)X derivative in the case of compounds of formula la. In the latter cases the linkers may be built up sequentially by first esterifying a suitably the latter cases the linkers may be built up sequentially by first esterifying a suitably WO 99/09031 26 PCT/SE98/0146 7 protected D or o-hydroxy carboxylic acid to the nucleoside, deprotecting the terminal carboxy or hydroxy function and esterifying the suitably protected glycerol or Rz moiety thereon.

The activated derivative used in the acylation may comprise e.g, the acid halide, acid anhydride, activated acid ester or the acid in the presence of coupling reagent, for example dicyclohexylcarbodiimide. Representative activated acid derivatives include the acid chloride, anhydrides derived from alkoxycarbonyl halides such as isobutyloxycarbonylchloride and the like, N-hydroxysuccinamide derived esters, N-hydroxyphthalimide derived esters, N-hydroxy-5-norbomene- 2 3 -dicarboxamide derived esters, 2 ,4,5-trichlorophenol derived esters and the like. Further activated acids include those where X in the formula RX represents an OR'moiety where R is R2 as defined herein, and R' is, for example COCH3,

COCH

2

CH

3 or COCF 3 or where X is benzotriazole.

Corresponding methodology will be applicable when the invention is applied to other monohydroxylated nucleosides, that is the activated derivative is correspondingly esterified to the free 5' hydroxy (or equivalent) of monohydric nucleosides such as acyclovir, ddl, FTC, lamivudine,. 1592U89, DAPD, F-ddA and the like.

The intermediates used in the above methods themselves define novel compounds, especially those of the formula: IIc' O 0 Al---X

A'-O

11c' where A, A' and Alk are as defined above (A and A' being optionally protected with conventional protecting groups) and X represents the free acid or an activated acid as illustrated above.

WO 99/09031 PCT/.qVQR/nIAr-Y 27 Representative coipounds of the formula Ic' include: malonic acid 2 ,3-bis-(L-valyloxy)-propyl ester, malonic acid 2 ,3-bis-(N-CBZ-L-valyloxy)-propyI ester, malonic acid 2,3 -bis-(N-Fmoc-L-valyloxy)-propyI ester, malonic acid 2 3 -bis-(N-Boc-L-valyloxy)-propyl ester, malonic acid 2 ,3-bis-(L-isoleucyloxy)-propyl ester, malonic acid 2,3-bis-(N-CBZ-L-isoleucyloxy)-propyI ester, malonic acid 2 3 -bis-(N-Fmoc-L-isoleucyloxy)-propyI ester, malonic acid 2,3-bis-(N-Boc-L-isoleucyloxy)-propyl ester, succinic acid 2,3-bis-(L-valyloxy)-propyl ester, :succinic acid 2,3-bis-(N-CBZ- L-valyloxy)-propyl ester, :succinic acid 2,3 -bis-(N-Fmoc-L-valyloxy)-propyl ester, succinic acid 2 3 -bis-(N-Boc-L-valyloxy)-propyl ester, succinic acid 2 3 -bis-(L-isoleucyloxy)-propyl ester, succinic acid 2,3-bis-(N-CBZ-L-isoleucyloxy)-propyl ester, sucii acd*3bs(-mcLioluyoy-r Ietr succinic acid 2 ,3-bis-(N-Foc-L-isoleucyoxy)-propy ester, s0guccinic acid 2,3-bis-(-Bol-ecyloxy)-propy I ester, acid 2,3-bis-(NCZL-valyloxy)-propyI ester, gltai acd23*s(-mcLvayoy-r Ietr glutaric acid 2,3-bis-(N-B-L-valyloxy)-propyI ester, glutaric acid 2,3-bis-(N-Foecayloxy)-propyl ester, glutaric acid 2,3-bis-(N-BZ-L-vaoeyloxy)-propy ester, glutaric acid 2 ,3-bis-(N-cL-isoleucyloxy)-propy ester, glutaric acid 2 3 -bis-(N-B-L-isoleucylo xy)-propyl ester, and the corresponding acid halides, in particular the chloride, acid anhydrides and diesters of each of the above, for instance succinic acid 2 3 -bis-(N-CBZ-L-valyloxy)-propyI ester,4-methoxybenzyl ester succinic acid 2 3 -bis-(N-CBZ-L-valyloxy)-propyI ester, 1, 1 -di methylethyl ester, etc.

WO 99/090 .31 PTS9/16 28 PTS9/16 A further preferred group of intermediates comprise those of the formula Ila': >)nk 0 Il a' where A]l*k, m, n and T are as described above, A and A' represent acyl residues of L'-aliphatic ami~no acids (N-protected as necessary) esterified to hydroxy functions on the linker or one of A and A' is the acyl residue and the other is a free hydroxy group, and X represents the free acid or an activated acid as illustrated above. Preferably A and A' are the same am-ino acid residue.

Other novel intermediates include the free or activated acid precursors of compounds of the formula Ia such as: 3-N-B oc-L-valyloxypropanoic acid, 3 -N-Fmoc-L-valyloxypropanoic acid, 3-N- CBZ-L-valyloxypropanoic acid, 3--o--sluyoytpni acid, 3-N- Fmoc-L-isoleucyloxypropanoic acid, 3--B--sluyoyrpni acid, 4 -N-Boc-L-valyloxybutyric acid, 3 -N-Fmoc-L-valyloxybutyric acid, 4-N-CBZ- L-valyloxybutyric acid, 4 -N-Boc-L-isoleucyl oxybutyric acid, 3-N-Fmoc-Lisoleucyloxybutyric acid, 3 N-CBZ-L-isoleucv~yvybtyicacd ndth lke and the activated derivatives, such as the acid halides Further novel intermediates include precursors of compounds of the formula He and Hf above, especially those derived from "natural" configurations such as Lmalic nd L-tartaric acid; for instance: 3 -ethoxycarbonyl-2valyloxy-propionic acid 3 -ethoxycarbony[-2-soleucyl oxy-propionic acid 4 -ethoxycarbonyl-2,3bis-valyloxy-butyric acid 4 -ethoxycarbonyI-2,3-bis-isoleucyloxy-butyric acid 3 -benzyloxycarbonyl.2-.valyloxy-propi onic acid WO 99/09031 PCT/SE98101467 29 3-benzyloxycarbonyl-2-isoleucyloxy-propionic acid 4-benzyloxycarbonyl-2,3-bis-valyloxy-butyric acid 4-benzyloxycarbonyl-2,3-bis-isoleucyloxy-butyric acid, and the like; and the corresponding activated derivatives such as the acid halides.

Still further novel intermnediates include precursors corresponding to structure fld, such as; 2-(L-valyloxy)propanoic acid, 2-(N-Boc-L-valyloxy)propanoic acid, 2-(N- Fmoc-L-valyloxy)propanoic acid, 2 -(N-CBZ-L-valyloxy)propanoic acid, 2-(Lisoleucyloxy)propanoic acid, 2 -(N-Boc-L-isoleucyloxy)propanoic acid, N- (Fmoc-L-isoleucyloxy)propanoic acid, N-(CBZ-L.-isoleucyloxy)propanoic acid, 2-(L-valyloxy)butyric acid, 2-(N-B oc-L-valyloxy)butyric acid, 2-(N-Fmoc-L- :valyloxy)butyric acid, 2-(N-CBZ-L-valyloxy)butyric acid, 2-(L- :isoleucyloxy)butyric acid, 2-(N-B ot-L-isoleucyloxy)butyric acid, N-(Fmoc-Lisoleucyloxy)butyric acid, N-(CBZ-L-isoleucyloxy)butyric acid, and the like; and activated derivatives therof, such as the acid halides.

Preparation of 3' fluoronucleosides such as those of formula V has been extensively reviewed by Herdiwijn et in Nucleosides and Nucleotides 8 (1) 65-96 (1989), which is hereby incorporated by reference. The preparation of other monohydric nucleosides such as acyclovir, ddl (didanosine), ddC (zalcitabine), d4T (stavudine), FTC, lamivudine (3TC), 1592U89 (4-[2-amino- 6 -(cyclopropylamino)- 9 H-purin-9-yl]-2-cyclopentene I1-methanol), AZT (zidovudine), DAPD (D-2,6-diaminopurine dioxolane), F-ddA and the like are well known and extensively described in the literature.

The reactive derivatives of the R 1

(R

2

)LIL

2 X group may be pre-formed or generated in situ by the use of reagents such as dicyclohexylcarbodiimide (DCC) or 1H-benzotriazol- 1-yl) N,N,N' ,N -tetramethyluronium tetrafluoroborate (T.BTU). When an acid halide, such as the acid chloride is used, a tertiary am-ine catalyst, such as triethylamine, N,N'-dimethylaniline, WO 99/09031 PCT/SE98/0146 7 pyridine or dimethylaminopyridine may be added to the reaction mixture to bind theliberated lydrohalic acid.

The reactions.are preferably carried out in an unreactive solvent such as N,Ndimethylformamide, tetrahydrofuran, dioxane, acetonitrile or a halogenatated hydrocarbon, such as dichloromethane. If desired, any of the above mentioned tertiary amine catalysts may be used as solvent, taking.care that a suitable excess is.present. The reaction temperature can typically be varied between 00 C and 600 C, but will preferably be kept between 5' and 500 C. After a period of 1 to 60 hours the reaction will usually be essentially complete. The progress of the reaction can be followed using thin layer chromatography (TLC) and appropriate solvent systems. In general, when the reaction is completed as determined by TLC, the product is extracted with an organic solvent and purified by chromatography and/or recrystallisation from an appropriate solvent 15 system.

By-products where acylation has-taken place on the nucleoside base can be separated by chromatography, but such misacylation can be minimized by controlled reaction conditions. These controlled conditions can be achieved, for example, by manipulating the reagent concentrations or rate of addition, especially of the acylating agent, by lowering the temperature or by the choice of solvent. The reaction can be followed by TLC to monitor the controlled conditions. It may be convenient to protect the 6-oxo group on the base and especially the 2 amino with conventional protecting groups to forestall misacylation.

Compounds of Formula IV in which

R

3 is hydrogen may be prepared by 6activating the correponding guanine compound of Formula I (wherein the exposed amino function of the amino acid residue of R 2 is optionally protected with conventional N-protecting groups) with an activating group such as halo.

The thus activated 6 -purine is subsequently reduced to purine, for instance with WO 99/0903131 PCT/SE98/01467 a palladium-catalyst and deprotected to the desired compound of Formula IV or Formula V.

Compounds wherein R 3 is an R, or other ester may be prepared by conventional esterification (analogous to the esterification described above) of the corresponding hydroxy compound of Formula I or Formula V, optionally after conventional N-protecting the exposed amine function of the amino acid residue of R2:and/or

R

3 Compounds wherein

R

3 is an ether-may be prepared analogously.to the process disclosed in the abovementioned WO 93 13778, again in conjunction with optional N-protection of exposed amine groups.

Compounds wherein

R

3 is an azide can be prepared as described in WO 97 09052.

Intermediates of the formula lid are conveniently prepared by acylation of a 15 carboxy-protected hydroxy alkanoic acid, typically a 2 -hydroxy-l-alkanoic acid, with the appropriate activated and N-protected

R

2 derivative, such as N- CBZ valyl or isoleucyl in conjunction with a conventional coupling reagent such as DMAP/DCC or with the amino acid halide. The carboxy protecting group is then removed, for instance by acid hydrolysis and the resulting intermediate is activated as described above or the free acid is unsed in conjunction with a coupling reagent to esterify the the nucleoside under conventional esterification conditions.

Compounds of the formula Ia are also conveniently prepared by the methodology in the immediately preceding paragraph, namely esterification of a carboxy protected a- hydroxy, co-carboxy acid, such as glycollic acid, lactic acid, hydroxybutyric acid etc with the appropriate N-protected

R

2 derivative, either as the free acid in conjunction with a coupling agent or activated, for instance to the corresponding acid halide. The carboxy protecting group is removed and the resulting intermediate esterified with the nucleoside with the methodology described above.

WO 99/09031 PCT/SE98/0167 32 Compounds.comprising a structure of the formula lie or IIfrare prepared by carboxy protecting the terminal carboxy groups of the respective dicarboxylic acid, such as L-tartaric acid or L-malic acid, with conventional carboxy protecting-groups such as benzoyl. The free hydroxy group are then esterified with conventional esterification techniques, such as DMAP DCC in DMF with the appropriate N-protected R 2 amino acid, such asN-Boc-L-valyl or N-Boc-L-isoleucyl. The benzoyl carboxy protecting groups-are removed and the resulting product is esterified to the 5'-hydroxy function of a monohydric nucleoside, using conventional conditions, such as those in the accompanying Examples. Finally, the free carboxy function is esterified with an R 1 group or, more preferbably a conventional pharmaceutically acceptable ester, such as the ethyl ester.

Compounds comprising a phosphorylated moiety m may be prepared by 15 reacting 2 3 '-dideoxy- 3 '-fluoroguanine-5-monophosphate with a compound of Formula VIa

.R

1 R 4

S

L -0 Ha :R2

R

4 Via where Ha is halo, such as chloro, iodo or bromo, in analagous conditions to those described in US 4 337 201, US 5 227 506, WO 94/13682 WO 94/13324, Starret et o" 20 al J Med Chem 37 1857-1864 (1994) and Iyer et al Tetrahedron Lett 30 7141-7144 (1989) which are incorporated herein by reference. The monophosphate can be prepared by conventional phosphorylation of FLG, as described, for instance, in Herdwyn et al ibid. Corresponding methodology will apply to the monophosphates of other monohydric nucleosides.

Alternatively this esterification to the phosphate ester could take part in two steps comprising a first reaction between FLG-monophosphate and a compound of the formula VII WO 99/09031 PCT/SE98/01467 33 0 R4 PGO 1 O--OH R4

VII

wherein R 4 and R 4 are as defined above and PG is a conventional hydroxy protecting group such asthose described above, followed by deprotection and esterification to a linker group L 1 whose third, rightmost function is an hydroxy group. Two examples of such a linker group L, are depicted in Scheme I below (the penultimate compounds in each series). In this embodiment the leftmost carbonyl of formula Va is synonomous with the carbonyl of linker group of the linker of Formula IIa.

Compounds comprising an optional linker L 2 may also be prepared by a two stage S- 10 process. In particular a compound of the formula CIC(=O)OC(R4)(R4')C1 can be a reacted with the 5'-hydroxy of FLG (optionally protected on the base with conventional protecting groups) as is known in the cephalosporin art. The resulting FLG-5'-O-C(=O)OC(R4)(R 4 ')chloride is then reacted with an R 1 and R 2 bearing trifunctional linker wherein the third function comprises a carboxyl function, such as the potassium salt.

It will be appreciated that trifunctional L, groups of formula IIa wherein and n and m are 1 and Alk is absent can be prepared from glycerol by regioselective esterification as depicted below in scheme 1 by reference to a stearoyl/L-valyl combination. In short RI and R 2 are regioselectively esterified to positions 1 and 3 of the glycerol and position 2 is then converted to the appropriate group, which is then esterified to the 5'-position of the fluoronucleoside or to a cooperating function on L 2 (not depicted). Alternatively the hydroxy at position 2 of the glycerol derivative can be esterified with an L 2 group containing a cooperating carbonyl function on its left hand end.

Li groups of formula IIa wherein m is 1, n is 0 and Alk is methylene can also be prepared from glycerol by regioselectively esterifying R 1 and R 2 to positions 1 and 2 WO 9909031PCT/SE98/01467 of the glycerol,4s: also depicted below in scheme 1, followed. conversion of the hydroxy at-position,3 to the appropriate -T-C(=O)-group. The leftmost series of reactions on Scheme I shows the situation where R, is esterified to position I of the glycerol and R 2 is esteri fled to position 2. The corresponding arrangement where R, is esterified to position 2 and R 2 to position I can be achieved by first treating the glycerol with' CBz-L-valine/DC yr)MAP/MFf and then protecting the 3 position with pixy] chloride prior to esterifying the fatty acid of R, to position 2 of the glycerol, deprotecting and converting the 3 position as necessary.

a a a SCHEME

I

OH stearoyl chloride OH pyridine/DMF CBz-L-valine DCC OMP CH2CI2/DM E0-stearoyl Iphosg ene 0 O-L-valyl-CBz Cl 1 0 0- stearoyl

EOH

0-stearoyl jpixyl chloride pyridine E0Pstearoyl SCBz-L-valine

DCC/DMAP/CH

2

CI

2 L- OPX 0- L-valyl-CBz FO-stearoyl C1 2

CH-CO

2

H

C H 2 C1 2 /pyrrole

O-

FO L-valyl-CBz 0-stea royl a.

I1 esterification with FLG V phosgene 0 EO0JL-CI E0- L-valyl-CBz 0-stearoyl WO 99/09031 PCT/SE98/01467 Although Scheme 1 has been illustrated byireference to a combination wherein R 1 is stearoyl and R 2 is L-valyl, it will be appreciated that this basic scheme will also be applicable to other amino acids, where present other fatty acids, or using conventional protection groups, to combinations of R 2 as an amino acid derivative and RI as hydroxy. Linkers where T comprises an -NH- group can be prepared by analogous regioselective esterification followed:by conversion of the free hydroxyl to amine, reduction to azide and reaction with.phosgene to form the corresponding chlorocarbamate.

A variation of scheme I allowing the preparation of linkers of the formula Ilc. In this variation, the phosgene step shown above is replaced by reaction with an activated dicarboxylic acid, such as succinic anhydride. This results in a glycerol triester (comprising the (optionally protected) R, ester, the protected R 2 ester and the ester of S" 15 the dicarboxylic acid) and the free carboxy on the dicarboxylic acid is then activated and esterified to the nucleoside in a conventional fashion. Alternatively linkers of formula Tic can be built up in situ on the nucleoside. In this variant, the dicarboxylic acid is esterified to a suitably protected glycerol derivative. This succinyl monoester is then esterified to the 5'-hydroxy function of the nucleoside in a conventional 20 manner. Finally one or both of the protecting groups on the glycerol moiety is replaced with the L-amino acid ester, and, if present, the remaining protecting group is replaced with a fatty acid ester or removed to leave a free hydroxy group This is depicted in Scheme IA which illustrates an example wherein the nucleoside in acyclovir (FLG shown in shadow), the dicarboxylic acid is succinyl and R, and R 2 are both CBZ-protected valyl, but will, of course be applicable to other variations of Formula Ic. In each case coupling conditions means standard esterification conditions such as coupling reagents DMAP, DCC etc or alternatively conversion of the relevant carboxy function to an activated derivative such as the acid chloride or the activated succinic moiety can also comprise the anhydride.

WO 99/09031 -PCT/SE98/01467 36 SCHEME IA 0 0 0 Ra-OH

OH

RaO

OH

0 nucleoside, -coupling conditions 0 RaO 0 O uanine Ra O r 1. acid hydrolysis of Ra 2. 1,3 bis-CBZ-valylglycerol, coupling conditions 3. deprotection 1,3 protected glycerol, coupling conditions -Oy.t/AoRRa R4-O0- J I

R

0 deprotection Rb, Rc 2. N-CBZ-valine, coupling conditions N-CBZ- 3. hydrolysis of Ra valyl -O 0 N-CBZ-

O

valyl -0 0 1. nucleoside, coupling conditions 2. deprotection 0valyl In a variation of Scheme IA, the succinic anhydride is reacted directly with the nucleoside, thus avoiding the first protection and deprotection steps. A further alternative is to regioselectively esterify the glycerol moiety with the N-protected amino acid moiety(ies), generally in conjunction with protection of the hydroxy function intended for coupling to the nucleoside, followed by deprotection of that hydroxy and coupling to the nucleoside.

WO 99/09031PC/E8047 PCT/SE98/01467 37 SCHEME II 0 0 LiAIH 4

;;;HD

DMAP DCC BOO Val z DMAP DCC 0H 2 C1 2 N-tritylVal CBzVal -0

HO::

Sstearoyll OBzVal -0 stearoyl- 0D StearoylCl

CH

2

CI

2 /pyridine TrVaI -O stearoyl- 0 KMnO 4 /QBr 0s0 4 /pyridine +lNaO 4 0 CBzVa- 0 stearoyl-D-

H

TrVal-0 0O stearoyl- 0 BOOMe-triphenyt 4phosphonium Br 0 TrVal -0 stearoyl 0D deprotection DBn esterification with FLG 4, Pd black 0 TrVal -0 stearoy- 0D-/ Linkers where m and n are 1, Alk is alkylene or alkenylene and T is a bond can be prepared as shown in Scheme II above. Other permutations of mn, n, Alk and the WO 99/09031 PCT/S/01 A67 38 various functions in the trifunctional linker group LI of formula Ha can be prepared analagously to the above with the corresponding starter materials, such as 1,2,4trihydroxybutane (CA registry number 3968-00-6), 3,4-dihydroxybutanoic acid (1518-61-2 22329-74-4), 3 4 -dihydroxybutanoic acid (51267-44-8), (R)-3,4-dihydroxybutanoic acid (158800-76-1), 1, 2 (51064-73-4 14697-46-2), (S)-1,2,5-pentanetriol (13942-73-9), pentanetriol (171335-70-9), 4 ,5-dihydroxypentanoic acid (66679-29-6 129725- 14-0), 1,3,5-pentanetriol (4328-94-3) and 3-(2-hydroxyethyl)- (53378-75-9). The preparation of each of these starting materials is described in the references to the respective registry number. Ohsawa et al in Chem Pharm Bull 41 (11) 1906-1909 (1993) and Terao et al Chem. Pharm. Bull. 39(3) 823-825 (1991) i" describe the control of the sterochemistry of trifunctional linker groups with lipase P.

P

The amino acid derivative of R 2 and, if present, RI can alternatively be esterified to the linker group with the 2 -oxa- 4 -aza-cycloalkane-1,3-dione methodology described in international patent application no. WO 94/29311, the contents of which are hereby incorporated by reference.

Linking of the carboxy function of R, and/or R 2 to an amine group on the linker derivative proceeds by conventional peptide chemistry, generally in conjunction with protection of the a-amine with conventional N-protecting groups. Formation of an amide bond between a carboxyl function on the linker and the a-amine group of R 2 also proceeds by conventional peptide chemistry, generally in conjunction with protection of the a-carboxy function. Esterification of R, as a fatty alcohol to a carboxy function on the linker proceeds analogously, but conversely, to the above esterifiation of RI as a fatty acid.

WO 99/09031 PCT/SE98/01467 39 Brief Description of the Drawings Various aspects of the invention will now be described by way of example only with reference to the following Examples and the accompanying drawings in which; Figure 1 depicts serum viral-DNA levels in treated and untreated, DHBV-infected ducks as afunction of time, as described in Biological Example 3; Figure 2 depicts weight gain in treated, DHBV-infected ducks as a function of time, as described in Biological Example 3.

EXAMPLE 1 2-(stearovloxvmethvl)-2-(N-(fluorenylmethoxycarbonyl)-L-valyloxvmethyl)propionic acid S: To a solution of 2,2-bis(hydroxymethyl) propionic acid (28.16 g, 210 mmole in water (50 ml), was added potassium hydroxide (11.78 g, 210 mmole). After 5 min, Sthe solution was evaporated in vacuo and the residue was coevaporated with dry DMF for three times. The residue was then dissolved in DMF (500 ml), and to the solution was added benzyl bromide (3.57 ml, 30 ml). After stirring for 30 min, the reaction mixture was filtered through the Celite, poured into sodium hydrogen 20 carbonate aqueous solution and extracted with dichloromethane. The organic phase was collected and then washed with sodium hydrogen carbonated aqueous solution. It was then evaporated in vacuo to give benzyl 2,2-bis(hydroxymethyl) propionate (4.37 g).

'H-NMR (CDC13): 7.35 5H), 5.20 2H), 3.91-3.71 4H), 1.10 3H).

To a solution of benzyl 2,2-bis(hydroxymethyl) propionate (4.37 g, 19.5 mmole) in pyridine (58 ml) was added dropwise stearoyl chloride (4.13 g, 13.6 mmole) in dichloromethane over 40 min. The reaction was then kept for 16 hr and then poured into sodium hydrogen carbonate aqueous solution and extracted with dichloromethane. The organic phase was collected and evaporated in vacuo. The W9900140 PCT/SE98/01467 product benzyl-2-(hydroxymethyl)..2. (stearoyloxymethyl) propionate was isolated by silica gel column chromatography (1.97 g) 'H-NMR

(CDCI

3 7.34 5H), 5.17 2H), 4.28 (dd, 2H-) 3.69 (dd, 211), 2.24 2H), 1 .57 (in, 2H, 1.25 28H, 1.22 0.87 3H).

Benzyl- 2 -(hydroxymethyl-2-(stearoyloxymethyl) propionate (1.86 g, 3.8 inmole) was dissolved in pyridine (30 ml). To the solution were added toluenesulfonic acid (73 mg, 0.39 inmole), N-fluorenylmethoxycarbonyl-L-valine (3.94 g, 11.6 inmole), and DCC (3.58 g, 17.4 mmole). The reaction was kept at 4 'C for 16 hr and then filtered through Celite. The filtrate was poured into sodium hydrogen carbonate :aqueous solution and extracted with dichioromethane. The organic phase was collected and-evaporated in vacuo. The product, benzyl -2-(N-fl uorenylmehxcabn*)Lv* oyehy)2(seryoxymethyl)propionate, was isolated *15 by silica gel column chromatography. Yield: 2.38 g.

'H-NMR (CDC1 3 7.78-7.25 (in, 13H), 5.29 (in, I 5.15 2H), 4.38 -4.23 (mn, 7H), 2.19 (t,211), 2. 10 (in, IH), 1.55 Cm, 2H), 1.24 (mn, 3 11H), 0.94 -0.83 (in, 9H).

To the solution of benzyl 2-N(loe e xcroyI--a lxmty (stearoyloxyinethyl) propionate (1.86 g, 3.8 inmole) in a mixed solvent of THF/methanol (16m1/8m1) were added ammonium formnate (376 mg, 6 minole); formic acid (1.87 ml), and palladium black (40 mg). The reaction was kept at room temperature for 16 hr, and then filtered through Celite. After evaporation, the product was isolated by silica gel column chromatography. Yield: 1.05 g.

EXAMPLE 2 I -O-stearoyl-'-O-(N-CBz.L-valyl)-' 2cerol a) Preparation of I -O-stearoylglycerol To a mixture of glycerol (30 g, 326 minol) and pyridine (25 mlJ) dissolved in DMF (300 ml) was added dropwise stearoyl chloride Cl0 g, 33 minol) dissolved in DMF WO 99/09031 PCT/SE98/01467 41 100 m19. The mixture was cooled on an ice bath until addition was complete, whereupon the reaction was maintained under an N 2 atmosphere overnight. After hours CH 2

CL

2 (300 ml) and saturated NaHCO3 (aq) was added. The phases were separated and the organic phase washed with water (50 ml) and dried with Na 2

SO

4 The solvent and any pyridine were evaporated under vacuum. The crude product was chromatographed on a silica column (CH 2 CIL -MeOH, 20:1) and recrystallised

(CH

2 C1 2 ether) to yield around 7 grams.

b) Preparation of pixyl chloride Acetyl chloride (150 ml, 2.1 mol) is added to a magnetically stirred suspension of 9hydroxy-9-phenylxanthene (20 g 72 mmol) in benzene (100 ml). An homogenous deep red solution is obtained. The solution is stirred for 30 min. at 20 The volatiles are removed under reduced pressure. Excess AcCI is neutralised by careful addition to ethanol. The residue is coevaporated with toluene (2 x 30 ml) and with cyclohexane (2 x 30 ml) to obtain a crystalline residue which is stored airtight.Pixyl chloride is alternatively available from Aldrich.

c) Preparation of 1-O-stearoyl, 3-O-pixylglycerol The product from a) above (2.28 g) and pyridine (25 ml) were mixed and heated until 20 dissolved. After cooling in an icebath pixyl chloride (1.92 g) from step b) was added.

The mixture was maintained under agitation and an argon atmoshere in an icebath for half an hour and then at room temperature for 1.5 h. The pyridine was evaporated under vacuum, the residue dissolved in CH 2

CI

2 (70 ml) and washed with 0.5 M citricacid to remove remaining pyridine. The residue was dried with Na 2

SO

4 evaporated and chromatographed (ether- hexane 1:3) to give 1.25 g pure product with a TLC Rr around 0.2.

d) Preparation of 1-O-stearoyl, 2-O-(N-CBz-L-valyl), 3 -O-pixylglycerol The product of step c) (237 mg, 0.39 mmol), CBz-L-valine (116 mg, 0.46 mmol), DCC (96 mg, 0.46 mmol) and DMAP (4.7 mg, 0.04 mmol) were dissolved in CH 2 C1 2 (4 ml). The mixture was maintained under agitation in a nitrogen atmosphere overnight. After 18 hours the mixture was filtered through a glass filter and WO 99/09031 PCT/SE98/01467 42 chromatographed on a silica gel column (ether hexane 1:4) to yield 230 mg with a TLC Rf of 0.2 e) Preparation of 1-O-stearoyl-2-O-(N-CBz-L-valyl)glycerol The pixyl group in the product of step d) was removed by selective deprotection by the method described in Example 3, step d to yield the title compound.

'H-NMR (CDC13): 5 7.35 5H), 5.3-4.9 4H), 4.35-4.25 3H), 3.8-3.6 (m, 2H), 2.31-2.25 2H), 2.20-2.10 IH), 1.60 2H), 1.02-0.86 9H).

EXAMPLE 3 0. I -O-(N-CBz-L-valyl)-2-O-stearovI glycerol a) Preparation of 1-O-(N-CBz-L-valyl)glycerol CBz-L-valine (4.35 g, 17.3 mmol) was added to a fivefold excess of glycerol (8 ml, 86.9 mmol) togehter with dicyclohexylcarbodiimide (4.29 g 20.8 mmol) and 4- *e dimethylaminopyridine (0.212 g) at room temperature. After stirring overnight the suspension was filtered and DMF removed in vacuo from the filtrate. The residue was redissolved in CH 2

C

2 washed successively with saturated NaHCO 3 brine, and water and then dried. The crude material was chromatographed on silica gel with 4/1 EtOAc hexane as eluent to yield 2.465 g. Rf (4/1 EtOAc hexane) 0.17, (20/1

CH

2 C1 2 methanol) 0.12.

b) Preparation of 1-O-(N-CBz-L-valyl)-3-O-pixylglyerol The product of step a) (0.672 g, 20.1 mmol) was dissolved in dry pyridine (3.5 ml) under nitrogen. 9 -Chloro-9-phenylxanthene (pixyl chloride, 0.65 g, 22.0 mmol, 1.1 eq prepared as above) was added and the mixture stirred at room temperature for h. MeOH (1.5 ml) was added and the mixture partitioned between 10 ml and 10 ml saturated NaHCO 3 The aqueous layer was extracted with more ether. The organic layers were combined, dried and concentrated several times with toluene to give a white solid. The crude material was chromatographed on silica gel with 3/1 hexane EtOAc as eluent to give 0.681 g.

WO 99/09031 PCT/SE98/01467 43 Alternatively a pi4yl group can be put on by the procedure described by Gaffney et al, Tetrahedron Lett 1997, 38, 2539-2542 using PxOH and acetic acid.

c) Preparation of 1-O-(N-CBz-L-valyl)-2-O-stearoyl-3-O-pixyl glycerol Stearoyl chloride (496 ml, 1.3 eq) in 1.5 ml CH 2 C12 was added dropwise to a solution of the product of step b) (0.658 g, 1.13 mmol) in 11 ml pyridine with stirring under

N

2 in an ice bath. After 15 minutes the mixture was stirred at room temperature overnight. The mixture was diluted with 20 ml Et20 and washed with 10 ml saturated NaHCO 3 The aquesous layer was extracted with more Et 2 O. The organic layers were combined, washed with brine (20 ml), dried over Na 2

SO

4 and concentrated several times with toluene. The crude material (1.37 g) was chromatographed on 130 g silica gel with 6/1 hexane EtOAc. An initial fraction of 500 ml was taken followed by 100 0 ml fractions. The desired material eluted in fractions 2 5 yielding 0.748 g.

d) Preparation of 1-O-(N-CBz-L-valyl)-2-O-stearoylglycerol To a solution of the product of step c) (0.748 g, .872 mmol) dissolved in 35 ml

CH

2

CI

2 to make 0.025 M) was added pyrrole (16.5 mol eq) and dichloroacetic acid (5.5 mol eq) at room temperature. TLC after 5 minutes showed complete reaction.

The mixture was diluted with 300 ml CH 2

C

2 and washed with 30 ml saturated NaHCO 3 The aqueous layer was extracted with more CH 2

CI

2 The organic phases were combined, washed with brine (30 ml), dried over Na 2

SO

4 and concentrated.

Crude material was chromatographed on silica gel with 2/1 hexane EtOAc (with 0.3% acetic acid) as eluent to yield 0.363 g with Rf (2/1 hexane EtOAc) 0.21.

'H NMR (CDCI 3 6 ppm 0.86-0.99 9H), 1.25 28H), 1.61 2H), 2.16 (m, 1H), 2.32 2H), 3.74 (br s, 2H), 4.28-4.44 3H), 5.09 1H), 5.11 2H), 5.22 IH), 7.36 WO 99/09031 PCT/SE98/01467 EXAMPLE 4 l-O-stearovl-3-O-(NCBz-L-valyl)lycerol The product of Example 2, part a) (2.86 g, 7.99 mmol), DCC (0.9g, 4.36 mmol) 4- (N,N-dimethyl)aminopyridine (DMAP) (0.048 mg, 0.39 mmol) and N-CBz-L-valine (Ig, 3.98 mmol) were dissolved in CH 2 Ci 2 (60 ml) and DMF (6 ml). The reaction was left at ambient temperature for 18 hours and then filtrated. The solvent was evaporated under reduced pressure. The residue was dissolved in CH 2 Cl2 (100 ml) and filtrated. The crude title compound was purified by chromatography [SiO2, ether/hexane to yield 1.3 g of the desired product. Unreacted 1stearoylglycerol may be recovered by eluting with CH 2 Cl2/MeOH (20:1).

H-NMR (CDCI 3 8 5.25 1H), 5.11 2H), 4.30-4.05 6H), 2.65 1H), 2.35 2H), 2.06 1H), 1.62 2H), 1.26 28H), 1.00-0.84 9H).

EXAMPLE CBz-valyl-- 0 0 L- Cl stearoyl -0 To an ice cooled solution of 1-chloroethyl chloroformate (1.89 g, 13.2 mmol) in dry 20 CH 2

CI

2 (5 ml), was added the compound of Example 4 in CH 2 C2 (20 ml) followed by dry pyridine (1.2 ml, 29.6 mmol). The reaction mixture was stirred with cooling under argon atmosphere until TLC (ether/hexane, 1:2) indicated consumption of the starting material. After 1.5 h, the mixture was washed with water (3 x 5 ml), sat.

NaHCO 3 (5 ml) and dried (Na 2

SO

4 Purification by chromatography [SiO 2 (etherhexane yielded the title compound (4.0 g).

'H-NMR

(CDCI

3 5 7.36-7.32 5H), 6.40 1H), 5.24 1H), 5.11 2H), 4.30 6H), 2.32 2H), 2.15 IH), 1.82 3H), 1.60 2H), 1.25 (br s, 28H), 0.97 3H), 0.86 6H).

II

WO 99/09031 PCT/SE98/01 467 EXAMPLE 6 CBz-valyl--O 0 o~ l Ho I stearoyl -0 To a solution of the compound of Example 5 (3.4 g, 4,87 mmol) in dry acetonitrile (47 ml), was added sodium iodide (3.65 g, 24.3 mmol). The solution obtained was refluxed under argon atmosphere until NMR indicated consumption of the starting material. After 4.5 h, ether (50 ml) was added and the mixture was filtrated. The solvent was removed by evaporation and the crude product dissolved in ether 10 ml). The ether solution was washed with water (2 x 10 ml) and dried (NaISO4) and evaporated under reduced pressure. Purification by chromatography [SiO 2 etherhexane yielded the title compound (2.15 g).

'H-NMR (CDCI 3 57.37 5H), 6.75 1H), 5.22 1H), 5.15 1H), 4.3 (m, 15 6H), 2.32 1H), 2.22 2H), 1.6 2H), 1.25 28H), 0.95 9H).

EXAMPLE 7 0 CH o 1 CI stearoyl -0 CBz-valyl-

O

A solution of the compound of Example 3 (810 mg, 1.37 mmol) in 2.2 mL dry dichloromethane was cooled in an ice bath with stirring under argon. 1-Chloroethyl chloroformate (298 pL, 2.74 mmol) was added, followed by the dropwise addition of pyridine (665 pL, 8.22 mmol) in 2.5 mL dichloromethane. After 2.5 hr, the mixture was diluted with 25 mL dichloromethane and washed successively with 10 mL water and 10 mL brine. The organic phase was dried over anhydrous sodium sulfate and concentrated several times with toluene to give a yellow oil. Purification by flash column chromatography on silica gel with 40/1 dichloromethane-diethyl ether gave the title compound as an oil (96 mg, quantitative yield).

WO 99/09031 PCT/SE98/01467 'H NMR (CDCI 3 5 ppm 0.85-0.98 9H), 1.25 28H), 1.60 2H), 1.83 3H, J= 5.8 Hz), 2.17 1H), 2.31 2H), 4.19-4.48 5H), 5.11 2H), 5.22 1H), 5.27 1H), 6.38-6.43 1H), 7.36 EXAMPLE 8 0 CH 3 stearoyl--0 CBz-valyl- A solution of the compound of Example 7 (1.896 g, 2.71 mmol) and sodium iodide 10 (1.80 g, 12.0 mmol) in acetonitrile (27 mL) was refluxed at 80 OC under nitrogen.

After 4.5 hours the reaction mixture was diluted with 100 mL 1/1 hexane-diethyl ether and washed with 25 mL water. The aqueous phase was extracted with more solvent (25 mL). The organic phases were combined, washed successively with aqueous sodium thiosulfate solution (25 mL) and brine (25 mL), dried over 15 anhydrous sodium sulfate, and concentrated in vacuo. Purification by flash column -chromatography on silica gel with 80/1 dichloromethane-methanol as eluant gave an oil (1.45 g) containing 90% of the title compound with 10% of the compound of Example 7.

tH NMR (CDCI 3 5 ppm 0.85-0.99 9H), 1.25 28H), 1.60 2H), 2.17 (m, 1H), 2.23 3H, J= 6 Hz), 2.31 2H), 4.16-4.49 5H), 5.10 2H), 5.20-5.29 2H), 6.69-6.79 1H), 7.36 WO 99/09031 PCT/SE98/01467 47 EXAMPLE 9 4-Benzyloxy-2-(N-trityl-L-valvloxvmethyl)- -stearoyloxybutane a) Synthesis of diethyl-2-(2-benzyloxyethyl) malonate To a freshly prepared solution of sodium (0.95g 41.4 mmole) in 50 ml ethanol was added a solution of diethylmalonate (6.4g 40 mmole) in 10 ml ethanol and the mixture was stirred for 15 minutes.Then a solution of 2 -benzyloxy-l-iodoethane (11.5g 41,35 mmole) was added drppwise. The mixture was refluxed for four hours and than evaporated in vacuo. 100ml of water was added and the mixture was extracted three times with 50ml portions of diethylether. The organic phase was dried with sodium sulfate and evaporated in vacuo and the product was isolated by silica Sgel column chromatography. Yield: 8.6g 'H-NMR (CDCI 3 1.26 6H) 2.26 2H) 3.54 3H) 4.16 4H) 4.57 2H) 7.32 b) Synthesis of 4 -benzyloxy-2-hydroxymethyl-butanol-1 To a stirred suspension of lithium aluminium hydride (3.0g 80 mmol) in 100 ml 20 diethylether was added dropwise a solution of diethyl-2-(2-benzyloxyethyl) malonate 28.8mmol) in 20 ml diethylether at about 15 0 C .The mixture was refluxed for two hours. About 4 ml water was dropwise added while cooling. The mixture was filtered and washed with dioxane. The filtrate was evaporated under reduced pressure and the product was isolated by silica gel column chromatography.

Yield: 3.4g 'H-NMR (CDCI 3 1.60 2H) 1.82 1H) 3.00 2H) 3.56 2H) 3.69 4H) 4.50 2H) 7.32 c) Synthesis of 4-benzyloxy-2-( N-trityl-L-valyloxymethyl)-butanol-1 To a solution of N-trityl-L-valine 4 .66g, 13 mmol) and 4-benzyloxy-2hydroxymethyl-butanol-1 (3.3g 15.6 mmole) in 50 ml dichloromethane was added DCC (3.0g 14.5mmole and DMAP 0.18g, 1.45mmole) and the mixture was WO 99/0903148 PCT/SE98/01467 stirred for three days. The mixture was cooled to 5 0 C and the urethane was filtered.

The solution was evaporated under reduced pressure and the product was isolated by silica gel column chromatography.

Yield: 'H-NMR (CDC3) 1.00 6H) 1.55 4H) 1.72 1H) 2.18 IH) 2.70 1H) 3.27 2H) 3.43 3H) 4.50 2H) 7.26 d) Synthesis of 4 -benzyloxy-2-(N-trityl-L-valyloxymethyl)-l-stearoyloxybutane.

To a solution of 4-benzyloxy-2-(N-trityl-l-valyloxymethyl)-butanol- 2 ,4g, 4.35 mmol) in 50 ml dichloromethane was added pyridine (1.72g, 21.7 mmol). The solution was cooled to 10°C and a solution of stearoyl chloride 2 .64g, 8.7 mmol) in O10ml dichloromethane was added dropwise between 10°C and 15 0 C The mixture was stirred overnight at room temperature. 100 ml of 5% sodium hydrogen carbonate solution was. added and the mixture stirred for 30 minutes. The organic phase Swas seperated and the water phase was extracted two times with dichloromethane S "The combined organic phases were dried with sodium sulfate and concentrated in vacuo The product was isolated by silica gel column chromatography Yield: 1 H-NMR (CDCI 3 0.98 9H) 1.26 28H) 1.54 2H) 1.94 1H) 2.25 2H) 3.23 2H) 3.44 2H) 3.58 1H) 3.91 2H) 4.10 1H) 4.47 2H) 7.28 EXAMPLE N-trityl-L-valyloxymethyl)-6-stearoloxhexanoic acid a) Preparation of 2-allyl 1, 3 -propanediol Diethyl allylmalonate (20 ml, 101 mmol) in anhydrous ether (100 ml) was added dropwise to a stirred solution of lithium aluminium hydride (9.6 g, 253 mmol) at 0°C. The reaction was warmed up to room temperature and kept for 5 hours. It was cooled down to 0 °C and water (12 ml) was carefully added dropwise. After stirring WO 99/09031 PCT/SE98/0167 49 for 30 min, the mixture was filtered through Celite and then washed with ethanol (2 x 500 ml). The solution was dried under vacuum giving 9.5 g product 'H-NMR (CDCI 3 5.78 m, 1H), 5.03 2H), 3.78 2H), 3.69 2H), 2.06 (t, 2H), 1.87 1H).

b) Preparation of 1-O-(N-trityl-L-valyl )-2-allyl-l,3-propandiol To a solution of N-trityl-L-valine (5.5 g, 15.2 mmole), 2 -allyl-1,3-propandiol (4.4 g, 38 mmol), N,N-dimethylamino pyridine (183 mg, 1.5 mmol) in dichloromethane (120 ml) was added DCC (3.5 g, 16.7 mmol). The reaction was kept under reflux overnight. After filtration through Celite, the organic phase was washed with sodium hydrogen carbonate aqueous solution and dried. Silica gel column chromatography gave 4.6 g intermediate 1-O-(N-trityl-L-valyl 2 -allyl-1,3-propandiol.

15 c) Preparation of 1-O-(N-trityl-L-valyl)-2-allyl-3-stearoyl-l,3-propandiol.

i'" To a solution of l-O-(N-trityl-L-valyl)-2-allyl-l,3-propandiol (1.83 g, 4 mmol) in dichloromethane (40 ml) and pyridine (3.2 ml, 40 mmol) at 0 OC was added dropwise stearoyl chloride (3.62 g, 12 mmol) in dichloromethane. The solution was warmed up to room temperature, and kept for 3 hr. It was then washed with sodium hydrogen 20 carbonate aqueous solution and dried. The product was isolated by silica gel column *..chromatography. 1.9 g 'H-NMR (CDCI 3 7.30 15 5.70 1H), 4.99 2H), 3.93 2H), 3.55 1H), 3.27 2H), 2.68 1H), 2.30 2H), 2.23 1H), 2.01 2H), 1.85 1H), 1.62 2H), 1.3 28H), 0.98 (dd, 6H), 0.91 3H).

d) Preparation of 3-(N-trityl-L-valyloxymethyl)-4-stearoyloxy-butyraldehyde 1-O-(N-trityl-L-valyl)-2-allyl-3-stearoyl-1,3-propandiol (580 mg, 0.8 mmol) was dissolved in dioxane (5 mi). To the solution were added osmium tetraoxide (20 mg, 0.08 mmole) and pyridine (0.05 ml, 0.64 mmole). A solution of sodium periodate in water (3.5 ml) was added to the reaction mixture. The reaction was kept overnight and then cooled down to 0 An aqueous solution of sodium hydrogen sulfite was added and the mixture was extracted with dichloromethane. The organic phase was dried and purified by silica gel column chromatography. Yield. 250 mg WO 99/09031 PCT/SE98/01467 'H-NMR (CDC13): 9.68 1H), 7.25 15 3.92 2H), 3.58 1H), 2.32 (m, 2H), 2.68 1H), 2.34 7 1.58 2H), 1.53 28 0.96 (dd, 6H), 0.86 3H).

f) Preparation of benzyl 3 -(N-trityl-L-valyloxymethyl)-4-stearoyloxyhexen-2-oate To the solution of N-trityl-L-valyloxymethyl)-4-stearoyloxybutyraldehyde (15.8 g, 21.8 mmole) in cichloromethanewere added (benzyloxycarbonylmethyl) triphenylphosphonium bromide (10.7 g, 21.8 mmole) and triethylamine (2.21 g, 21.8 mmole). The reaction was kept overnight at room temperature, and the mixture was evaporated. To the residue was added diethyl ether (200 ml and kept at 4 °C for two hours. It was then filtered and the filtrate was evaporated and the product was purified by silica gel column chromatography. Yield. 10 g 'H-NMR

(CDCI

3 7.30 20 6.89 IH), 5.88 1H), 5.19 2H), 3.95 2H), 3.57 1H), 3.29 2H), 2.68 1H), 2.23 5H), 1.93 1H), 1.60 2H), 1.32 28 0.95 (dd, 6H), 0.89 3 H).

g) Preparation of 3 -(N-trityl-L-valyloxymethyl)-4-stearoyloxyhexanoate To a solution of benzyl 3 -(N-trityl-L-valyloxymethyl)-4-stearoyloxyhexen-2-oate mg, 0.08 mmole) in methanaol (3 ml) and ethyl acetate (1 ml) was added sodium hydrogen carbonate (10 mg) and palladium black (20 mg). The reaction was kept under hydrogen at atmospheric pressure for 2 hr. The mixture was filtered and evaporated. The residue was dissolved in dichloromethane and washed successively with aqueous EDTA solution and cold aqueous 2 citric solution. The organic phase was evaporated to give 61 mg product 'H-NMR (CDC13): 7.30 15 3.93 2H), 3.57 1H), 3.25 2H), 2.30 (dt, 4H), 2.20 1H), 1.70 1H), 1.62 4H), 1.30 28 0.95 (dd, 6 H), 0.87 3 H).

WO 99/09031 PCT/SE98/01 467 51 EXAMPLE I I 3 -(N-benzvloxycarbonyl-L-valyloxymethyl).4-stearoyl oxy-butyr-ic acid a) Preparation of 1 -O-(N-benzyloxycarbonyl-L-vayl)2-a1ylyl-1 ,3-propandiol To a solution of 2 -allyl-1,3-propandiol (4.6 g, 40 mmole) and N-benzyloxycarbonyl valine (5.02 g, 20 mrmole) in dichioromethane was added dimethyl ami nopyri dine (244 mg, 2 mrnol), and DCC (4.5 g, 22 mmol). After two hours, the mixture was filtered through Ce] ite, evaporated and theproduct, I -O-(N-benzyl oxycarbonyl-Lvalyl)-2- allylyl- 1,3-propandiol, isolated to yield 5.01 g.

2 H-NMR (CDCI 3 7.36 (in, 5H), 5.78 (mn, 1H), 5.26 1H1), 5.11 2H), 5.06 (d, 2H), 4.22 (in, 3H), 3.59 (in, 2H), 2.13 (in, 1.98 (in, 2H), 0.94 (dd, 6 H).

Preparation of 1 -O-(N-benzyloxycarbonylLvalyl)2allyyl3-0stearoyl-1,3propandiol.

To a solution of l-O-(N-benzyloxycarbonyl-L-valyl)-2-allylyl.13-propandioI (4.46 g, 12.7 minol) in dichloroinethane (70 ml) and pyridinie (6.1 l, 76 inmole) in ice bath was added stearoyl chloride (7.8 g, 26 minole). The reaction mixture was warmed up to room temperature and kept for one hour. It was then poured into aqueous sodium hydrogen carbonate solution, the organic phase was dried and the product I ben zyl oxycarbonyl-L-v aly ])-2-allylyl -3 -o-stearoyl-1 I,3-propandiol was purified by silica gel column chromatography. 6.7 g I1H-NMR (CDCI 3 7.34 (mn, 5H), 5.77 (in, I1H), 5.30 1 5.11 (s 2H), 5.08 (d, 2H), 4.32 (in, I1H), 4. 10 (in, 4 2.29 2H), 2.13 (in, 4H), 1.62 (in, 3 1.25 (in, 28H), 0.90 (in, 9 H).

c) Preparation of 3 -(N-benzyloxycarbonyl-Lvalyoxymethy4stearoyloxy-butyric acid.

Potassium permanganate (756 ing, 4.8 iniole) was dissolved in water (7.5 The solution was kept under strong stirring for 10 min. A solution of 1-O-(Nbe yoyabnlLvll)2allI---taol 1 ,3-propandiol (1 g, 1.6 mmol) WO 99/09031 PTS9/16 52 PTS9/16 and tetrabutylammonium bromide (77 mg, 0.24 mimole) in benzene (5 ml) was added. The slurry was stirred for 1.5 hr, and dichioromethane was added. A sodium bisulfite aqueous solution was added to the slurry until the mixture discolored. The organic phase was acidified with acetic acid and washed with water. After evaporation, the product 3 -(N-benzyloxycarbonyl -L-valyloxymethyl-4-stearoyloxybutyric acid (390 mg) was isolated by silica gel column chromatography.

'H-NMR

(CDCI

3 7.33 (in, 5H), 5.38 IFH), 5.11 2H), 4.14 (in, 5 2.60 (mn, 111), 2.45 (in, 2 2.29 2 2.18 (in, I 1.58 (mn, 2 1.25 (mn, 28 0.90 9H).

EXAMPLE 12 '-dideoxyt-3 '-fluoro-5 '-O-f5-(L-valyloxymethvl 6 -stearoyloxyhexanoyl guanosine a) Preparation of 2 3 '-dideoxy-3'nfuoro-5'-O-[5-(N-trityl-L-valyloxymethyl)-6 stearoyloxyhexanoyl] guanosine To a solution of N-r y--ayoym h eryIoyeao acid (462 mg, 0.6 inmole) and 2'3-iex-'-loounsn (340 mng, 1.25 mmol) in DMF (3 ml) were added dimethylaininopyridine (7 mg, 0.06 minole), and DCC (136 mg, 0.66 minol). The reaction was kept at room temperature overnight, and then at 40'C for two hours. The reaction mixture was filtered through Celite and poured into dichioroinethane, and washed with aqueous sodium hydrogen carbonate solution.

The product 2' ,3 '-dideoxy-3 '-fluoro-5 tyl-L-valyloxymethyl)-6 stearoyloxyhexanoyl] guanosine was isolated by silica gel column chromatography.

(93 mng) 'H-NMR (DMSO 8-6 7.88 IH), 7.29 (mn, 15 6.52 Cs, 2H), 6.17 (dd, 11H), 5.45 (in, IH), 4.35 (in, IN), 4.20 2 3.82 (in, 2H), 3.50 2.60 (in, 5 2.30 (in, 4 2. 10 (in, I 1.70 (in, INH), 1.50 (in, 4 1.22 (in, 28 0. 85 (in, 9 H).

WO 99/09031 PCT/SE98/O1 467 53 b) Preparation of 2' ,3 '-dideoxy-3 '-fluoro-5 '-O-[5-(L-valyloxymethyl)-6stearoyloxyhexanoyl] guanosine The compound of step b) (90 mg, 0.088 mmole) was N-deprotected by treatment with 80 acetic acid (5 ml) at room temperature for 30 min. It was evaporated and product was purified by silica gel column chromatography to yield 72 mg of the title compound.

'H-NMR (DMSO 7.88 IlH), 6.54 6.18 (dd, I1H), 5.48 (dd, I1H), 4.27 (dt, I 4.19 (in, 2 3.98 (in, 4H1), 3.17 -2.55 (mn, 4 2.29 (in, 4 1.95 (mn, 1 1.75 (mn, 1 1.50 (in, 4H), 1.21 (in, 28 0.84 (in, 9 H).

EXAMPLE 13 2'.3 '-Dideoxy-3 '-fluoro-5 '-O-r 3 -(L-valyloxvmethyl)-4-stearovloxybutanoyll guanosine a) Preparation of 3' -dideoxy-3 '-fluoro-5 '-O-[3-(N-benzyloxycarbonyl-Lvalyloxy)-4-stearoyloxy-butanoyllguanosi ne To a solution of 2',3'-dideoxy-3'-fluoroguanosine (113 mg, 0.42 inmol) and 3-(Nbenzyloxycarbonyl-L-valyloxymethyl)-4-stea-royloxy-butyric acid (140 mng, 0.2 Immol) in DMF (2 ml) were added diinethylaininopyridine (3 mg, 0.02 minol) and DCC (52 mg, 0.25 inmol). After two days, dichloromethane (10 ml) and a few drops of acetic acid were added and the organic phase was filtered through Celite.

The filtrate was washed with aqueous sodium hydrogen carbonate solution and the product 2' ,3 '-dideoxy-3 '-fluoro-5' 3 (N-benzyloxycarbonyl-L-valyloxymethyl).

4-stearoyloxy-butanoyl)guanosine was isolated by silica gel column chromatography to yield 51 mg.

'H-NMR (CDCI 3 7.79 I1H), 7.26 (mn, 5 6.3 8 2H), 6.23 I 5.44 (in, 2H), 5.08 2H), 4.50-4.10 (in, 8H), 3.15-2.40 (in, 5 2.30 2 2.14 (in, 111), 1.58 (in, 2H), 1.24 (in, 28H), 0.87 (in, 9 H).

WO 99/09031 PCT/SE98/01467 54 b) Preparation of 2',3'-Dideoxy-3'-fluoro-5'-O-[ 3 -(L-valyloxymethyl)-4stearoyloxy-butanoyl]guanosine The product of step a) (76 mg, 0.084 mmole) was dissolved in a mixed solvent of methanol (3 ml), ethyl acetate (0.5 ml) and acetic acid (0.01 ml). To the solution was added palladium black (10 mg). After 2 hr, additional 10 mg palladium black was added. After 3 hr, the mixture was filtered and evaporated. The residue was dissolved in dichlorometahne and washed with aqueous EDTA solution. The organic phase was dried and coevaporated with toluene giving the title compound as the acetate salt.

Yield 65 mg.

'H-NMR (DMSO 5-6 D 2 7.87 1H), 5.16 (dd, 1H), 5.37 (dd, 1H), 4.24 (m, 4.01 4H), 3.10-2.60 3H), 2 .40 2H), 2.24 2 1.70 1H), 1.48 2H), 1.25 28H), 0.82 9H).

EXAMPLE 14 3-r 1-(N-CBz-L-vall)-2-stearoyl propyl chloroformate 1-(N-CBz-L-valyl)-2-stearoyl) glycerol 300 mg, 0.5 mmole was dissolved in phosgene in toluene 15 ml After 18 h, the solution was evaporated and the 20 residue was coevaporated with toluene for several time, giving title product in quantitative yield. This product forms a carbonate with the target nucleoside using :i standard methodology, for instance reacting in a 10:1 DMF/pyridine solution at 0 C for 3 to 24 hours, pouring into NaHCO 3 solution and extraction with dichloromethane. The amino acid is deprotected, for instance with palladium black in a methanol, ethyl acetate, acetic acid solution to yield the nucleoside-O-[1-( L-valyl)- 2 -stearoyl-3-propyloxy carbonyl 'H-NMR CDC1 3 7.40 m, 5H 5.28 m, 2H 5.10 s, 2H 4.35 m, 5H 2.35 m, 2H 2.17 m, 1 1.

5 6 2H 1.30 28 H 0.

9 5 9H WO 99/0903 1 PCT/SE98/01467 EXAMPLE 5-(N-FMOC-L-valyloxy)-4-stearoyloxy-1pentanoic acid a) Benzyl 4 ,5-dihydroxy-2..pentenoate.

A mixture of DL-glycerinaldehyde (4,5g 50 mmole and (benzyloxyc arbonylmethyl)-triphenyl-phosphoniumbromide 2 4 .57g, 50 mmole) in 100 ml I ,2-epoxybutane was refluxed overnight The mixture was evaporated under vacuum and the product was isolated by silica gel column chromatography Yield: 8g =71 'H NMR (CDCI 3 2.50 IlH) 2.96 s, IH 3.54 (im, I1H) 3.70 (in, I1H) 4.3 8 IH) 5.12 2H) 6.14 (m,IH) 6.90 (mn, 1H) 7.30 (mn, b) B enzyl A mixture of benzyl 4 ,5-dihydroxy-2-pentenoate (4.4g, 20 mmole), N-FMOC-Lvaline (5.8g, 17 iniole) and DMAP (0.21g, 1,7 mmole) in 100 ml dichioroinethane was cooled to about I 0 0 C. A solution of DCC (4.2g, 20 minole) in 25 ml] dichloromethane was added droppwise at the same temperature and the mixture was stirred overnight at room temperature. The mixture was cooled to 5'C and the urethane was filtered The filtrate was evaporated under reduced pressure and the product was isolated by silica gel column chromatography Yield: 6,6g 71 'H-NMR (CDCI 3 0.91 (in, 6H) 2.12 (in, 1H) 4.38 (mn, 5H) 5.14 2H) 5.24 (mn, lH) 6.20 111) 6.92 (in, IH) 7.30 (in, 13H) c) Beny -NFO--ayoy-4seryoy2pneot To a solution of be y 5-NFO--ayox)4hdoy2pneot 6 .5g, 12 mmol) and pyridine (2.0g, 25 minole) in 100 ml dichloromethane at I10 0 C was added dropwise a solution of stearoylchloride 4 .55g, 15 mmol) in 25 ml dichioroinethane.

The mixture was stirred overnight.l100 ml of 5% sodium hydrogencarbonate solution was added and the mixture was stirred for 30 minutes The organic phase was WO 99/09031 PCT/SE98/01467 WO 9/0901 PT/SE8/146756 seperated and the water phase was extracted two times with dichloromethane.The combined organic phases were dried with sodium sulfate and concentrated in vacuo.

The product was isolated by silica gel column chromatography .Yield 7 ,8g 'H-NMR (CDCI 3 0.88 (in, 9H) 1.25 (mn, 28H) 1.58 (in, 2H1) 2.14 (in, 111) 2.32 (in, 2H) 4.22 (in, 5H) 5.19 2H) 5.25 (mn, I H) 6.12 (in, I H) 6.85 (in, I H) 7.3 (i,13H).

d) N-FMOC-L-valy oxy)4s tearoy Io xy-pen tan oic acid.

A solution of benzyl 5-(N-FMOC-L-valyloxy)-4-stearoyloxy..2-pentenoate (3.8g.

4.69 minole) in 50 ml ethyl acetate was hydrogenated with 10% palladium on charcoal (0,5g) at normal pressure for five hours at room temperature. The catalyst .*was filtered and washed with ethyl acetate and I ,4-dioxane. The solution was evaporated under reduced pressure .Yield :3.3g 99% 'H-NMR (CDCI 3 0.92 (in, 9H) 1.25 (mn. 28H) 1.54 (mn, 2H) 1.98 (in, 2H) 2.18 (i,11H) 2.28 (in, 2H) 2.41 (in, 2H) 4,32 (in, 5H) 5.13 (mn, IH) 5.33 (mIH) 7.50 (i,8H) EXAMPLE 16 3 -(N-FMOC-L-valvloxy')-2-stearoyloxypropionic acid a) Benzyl 2 3 -dihydroxypropionate A mixture of D,L-glyceric acid, calcium salt dihydrate (2.9g, 10 inmole) and benzylbromide (3.8g, 22 imnole) in 25 ml DMF was stirred at 60'C overnight. The mixture was evaporated under reduced pressure and the product was isolated by silica gel chromatography. Yield: 4g 100% 'H-NMR (CDCI 3 3.26 IH) 3.90 (in, 2H) 4.32 (in, I H) 5.25 2H) 7.28 WO 99/09031 PCT/SE98/01467 57 b) Benzyl 3 -(N-FMOC-L-valyloxy)-2-hydroxypropionate A solution of benzyl-2,3-dihydroxypropionate 4,0g 20 mmole N-FMOC-Lvaline (5.4g, 16 mmole) and DMAP( 0.2g, 1.6 mmole) in 80 ml dichloromethane was cooled to about 10°C A solution of DCC (4.12g, 20 mmole) in 25 ml was added dropwise at the same temperature and the mixture was stirred overnight at room temperature. The mixture was cooled to 5 0 C and the urethane was filtered The solution was evaporated under reduced pressure and the product was isolated by silica gel chromatography. Yield 4.7g 'H-NMR (CDCI3) 0.88 6H) 2.05 (m,lH) 4.40 6H) 5.23 3H) 7.50 (m, 13H) c) Benzyl 3 -(N-FMOC-L-valyloxy)-2-stearoyloxypropionate To a stirred solution of benzyl 3 -(N-FMOC-L-valyloxy)-2-hydroxypropionate (4.6g 8.89 mmole) and pyridine (1.41g, 17.8 mmole) in 80 ml dichloromethane was o added dropwise a solution of stearoylchloride (3.64g, 12 mmole) in 20 ml dichloromethane and the mixture was stirred overnight at room temperature. 100 ml of 5% sodium hydrogencarbonate solution was added and the mixture stirred for 30 minutes. The organic phase was seperated and the water phase was extracted two times with dichloromethane. The combined organic phases were dried with sodium sulfate and concentrated in vacuo. The product was isolated by silica gel chromatography. Yield 6. Ig 87% 'H-NMR (CDC1 3 0.88 9H) 1.26 28H) 1.56 2H) 2.06 1H) 2.34 (m, 2H) 4.36 6H) 5.19 2H) 5.32 1 H) 7.50 13H) d) 3- (N-FMOC-L-valyloxy )-2-stearoyloxypropionic acid.

A solution of benzyl N-FMOC-L-valyloxy )-2-stearoyloxypropionate (0.78g, 1 mmole) in 20 ml ethyl acetate was hydrogenated with IP% palladium on charcoal (0.2g) at normal pressure for three hours at room temperature The catalyst was WO 99/09031 PCT/SE98/01467 58 filtered and washed with ethyl acetate and 1 ,4-dioxane. The solution was evaporated under reduced pressure. Yield: 0.63g 'H-NMR

(CDCI

3 0.88 (in, 9H) 1.24 (im, 28H) 1.40 (in, 2H) 2.12 (in, 3H) 4.30 (in, 5H) 5.16 (in,1IH) 5.60 (mn, IH) 7.40 (in, 8H) EXAMPLE 17 I enzvloxycarbonvl..L.va yloxmethl)2stearoyloxyethoxvcarbo nI chloride Bis(trichloromethyl) carbonate (160 mng; 0.54 mmcl) was added with stirring to a 9 solution of l-(N-benzyloxycarbonylLvalyl)-3stearoylglycerol; I benzyloxycarbonyl.Lvalyloxy)3stearoyloxy-2propanol; preparative example 4; (660 ing; 1. 12 mmcl) and triethylamine (200 mg; 2.0 minol) in dichloromethane ml]) at room temperature. After Ilh, n-hexane (10 ml) was added and the precipitated triethylainine hydrochloride was filtered off through a short column of silica gel, the product eluted with a further amount of n-hexane, and the solvent evaporated in vacuum to yield 6 50 mg of the title compound.

3 C NMR (CDC1 3 62.975 MHz): 8 172.8 (stear-COO); 171.2 (Val-COO); 155.9 154.1 (COCI); 136.0 (Ph-C I-Val); 128.1-127.7 67.2 (CHOH); 66.7 9 (Ph CHA) 63.1 (VaICOOCH 2 61.8 (stear-COOCH 2 hj 58.7 (Val-axC); 33.7 (stear- C2); 31.6 (stear-C1 3 1.0 (Val-13C); 29.3-28.8 (stear-C4-15); 24.5 (stear-C3); 18.6 and 17.1 (Val 2 CH 3 13.8 (stear-C18).

EXAMPLE 18 3-(N-CB z-L-valyloxvineth yl)..4-stearovloxvbutvlchloroformate a) 3- N-CBz-L-valyoxyinethyl 4 -stearoyloxy-butanol To a stirred solution of 4 -stearoyloxy..3-(N.CBzLvalyloxyinethylbutyraldehyde (prepared analogously to preparative example 6, step d) using CBz protected valine) g, 3.2 iniole) in 25 ml methanol at I10 0 C was added sodium borohydride WO 99/09031 PCT/SE98/01467 59 (0.6g, 16 rnmole) in small portions The mixture was stirred for 30 minutes and then acidified with acetic acid .The mixture was diluted with water and extracted three times with dichloromethane.The organic phase was dried with sodium sulfate and concentrated in vacuo .The product was isolated by silica gel column chromatography. Yield: 1,5g 'H-NMR (CDC1 3 0.88 (in, 9H) 1.25 (in, 28H) 1.52 (in, 4H) 2.24 (mn, 3H) 3.68 (in, 2H) 4.12 (in, 4H) 4.24 (mn, 1H) 5.08 (s 2H) 5.22 (in, IH) 7.36 (mn, io b) 3-(N-CB z-L-valyloxyinethyl)-4-stearoyloxybutyl chioroforinate A solution of the intermediate of step a) in 20 ml of a 20% solution of phosgene in toluene was stirred overnight The mixture was evaporated under reduced pressure to ~.yield the title compound.Yield 1.5g 97%.

'H-NMR (CDCI 3 0.88 (in, 9H) 1.28 (in, 28H) 1.58 (in, 2H) 1.72 (in, 2H) 2.15 (m, I H) 2.31 (mn, 2H 4.08 -4.42 (in, 5H) 5. 10 2H) 5.22 (in, I H) 7.3 6 (in, EXAMPLE 19 2',3 '-dideoxy-3 '-fluoro-5 I -(L-valvloxy)-2-stearoyloxv-3-propyloxy carbonll guanosine a) Synthesis of 2 '-dideoxy-3 -fluoro-5 I N-CBz-L-valyloxy )-2-stearoyloxy- 3-propyloxy carbonyl] guanosine.

To a solution of 2T,3'-dideoxy-3-fluoro-guanosine (270 mg, I minole) in DM4F ml) and pyridine (1 ml) was added 3-{1 N-CBz-L-valyl)-2-stearoyl} propyl chloroforinate (619 mg, 0.5 minole) at 0 After 3 h, the reaction mixture was poured into sodium hydrogen carbonate solution and extracted with dichioromethane.

The organic phase was dried in vacuo, and 2',3'-dideoxy-3'-fluoro-5'-O-[ N-CBz- L-valyloxy)-2-stearoyloxy-3-propyloxy carbonyl] guanosine was isolated by silica gel column chromatography (195 mng).

WO 99/09031 PCT/SizaRinIAK-7 T/omnAt' 'H-NMR

(CDCI

3 7.69 1H), 7.31 5H), 6.50 (in, 2H), 6.32 (in, I1-H), 5.3 (n 2H), 5.09 (mn, 2H), 4.35 (in, 7H), 2.60 (mn, 2.31 2H), 2.20 (mn, I 1.58 (n 2H), 1.23 (in, 28 0.92 (mn, 9H).

b) Synthesis of 2 ',3'-dideoxy-3 '-fluoro-5 I -(L-valyloxy)-2-stearoyloxy-3 propyloxy carbonyl] guanosine.

2',3 -dideoxy-3'-fluoro-5 N-CBz-L-valyl oxy)- 2 -stearoyloxy..3.propyloxy carbonyl] guanosine (190 mg), was dissolved in a mixed solvent of methanol (6 ml), ethyl acetate (2 ml) and acetic acid (I ml). To the solution was added palladiumn black (30 ing), and the reaction mixture was kept under hydrogen for 2h. It was then filtered and the filtrate was evaporated and the titled product was isolated by silica :gel column. 'H-NMR (DMSO-56): 7.86 (ds, IH), 6.51 6.17 (dd, IH), 5.48 (in, IH), 5.20 (in, 1H), 4.25 (in, 7H), 2.70 (in, 2H), 2.27 (mn, 2H), 1.72 (in, 1H), 1.47 (in, 2H), 1.22 (mn, 28 0.84 (mn, 911).

EXAMPLE 3 '-dideoxy-3' -fluoro-5 [5-(L-valylox v)- 4 -stearoyloxy-pentanoylI manosine.

To a solution of 3 1 -dideoxy-3'-fluoroguanosine (O.27g, I iniole) and FMCLv*lxy4sery oxpntno acid (0.94g, 1.3 minole) in 30 ml DMF was added DMA? (I16mg, 0. l3iniol) HOBT 176 g, 1.3 inmole and DCC (0.248g, 1.2 inmole). The mnixture was stirred for three days at room temperature.

4g silica gel were added and the mixture evaporate in vacuo. The product, 3'dideoxy-3'-fluoro-s [5(MCLvllx)4serolx-etnylunsn was separated by silica gel chromnatography. Yield :O.

4 'H-NMR (DMSO&.6) 0.88 (in, 9H) 1.20 (in, 28H) 1.45 (in, 2H) 1.78 (in, 2H) 2.18 2H) 2.36 2.62(in, 2H) 3.88 IH) 4.22 (in,6H) 4.92 (in,H)

S,

4 1H) 6.19 (in, IH) 6.52 2H) 7.26 7.88 (in, 8H-) WO 99/09031 PCT/SE98/01467 61 The protected intermediate is deprotected as shown above to yield the title compound.

EXAMPLE 2',3'-dideoxv-3'-fluoro-5'-O-[3-( N-FMOC-L-valyloxy)-2-stearovloxypropanoyl] guanosine To a stirred mixture of 3 -(N-FMOC-L-valyloxy)-2-stearoyloxypropanoic acid (0.61g, 0.88 mmol) in 5 ml dry diethlether was added one drop DMF and thionyl chloride(0.52g, 4.4 mmole). The mixture was refluxed for two hours and then Sevaporated under reduced pressure. The product was dissolved in dry dichloromethane and added dropwise to a solution of 3'-dideoxy-3'fluoroguanisine (0.215 g, 0.8 mmole) and pyridine (0.35g, 4.4 mmole) in 20 ml DMF. The solution was stirred overnight. Two grammes of silica gel were added and the mixture was evaporated in vacuo The product was isolated by silica gel chromatography. Yield: 0.19g 'H-NMR (CDCI 3 0.88 9H) 1.25 28H) 1.62 2H) 2.12(m, 1H) 2.38 (m, 2H) 2.58 2H) 4.12- 4.76 (m 6H) 5.32 2H) 6.12 1H) 6.26 1H) 6.44 1H) 7.12-7.78 8H).

EXAMPLE 21 N-CBz-L-valvl)-3-stearovl-2-propyl succinate monoester N-CBz-L-valyl)-3-stearoyl-glycerol (886 mg, 1.5 mmole) and succinic anhydride (450 mg, 4.5 mmole) were dissolved in a mixed solvent of DMF (15 ml) and pyridine (1 ml). The reaction was kept at room temperature for 3 h, and then at 60 oC for 5 h.

The reaction mixture was poured into a solution of acetic acid and water and extracted with dichloromethane. The organic phase was washed with water and evaporated, and the product was isolated by silica gel column chromatography to yield 900 mg.

WO 99/09031 PTS9/16 62 PTS9/16 'H-NMR

(CDCI

3 7.43 (in, 5H1), 5.27 I 5.09 (in, 2H), 4.21 (in, 5H), 2.54 (in, 4H), 2.29 2H), 2.13 (mn, lIH), 1.59 (in, 2H), 1.25 (mn, 28 0.90 (mn, 9H-).

EXAMPLE 22 2'.3 '-dideoxY-3 -fluoro-5,-0- f 3-Fl1 L-valvoxy)-3-stearoyloxy.2-propVloxy carbonyll-propanoyl Iguanosine To a solution of 2 ,3-dideoxy-3'-fluoro.guanosine (351 mg, 1.3 mmole) and 1-(N- CBz-L-valyl)-3-stearoyl-2propyl succinate inonoester (900 mng, 1.3 irole) in DMF ;(15 ml) were added dimethylaininopyridine (24 mg, 0.2 mi-nole), I hydroxybenzotriazole (175 mg, 1.3 inmole), DCC (321 mg, 1.56 inmole). After 48 h, the reaction mixture was filtered. The filtrate was poured into sodium hydrogen *carbonate solution. and extracted with dichioromethane. The product 2T,3-dideoxy.

3 '-fluoro-5 1-(N-CBz-L-valy1)-3-stearoyl glyceroloxy carbonyl]propanoyl) *..guanosine was isolated by silica gel column chromatography. 780 mg 'H-NMR DMSO-d6): 7.89 I 7.34 (in, 5H), 6.50 2H), 6.17 (dd, 11H), 5.46 (in, IH), 5.38 (in, IH), 5.02 2H), 4.22 (in, 7H), 3.32 4H), 2.80 (in, 211), 2.57 (mn, 211), 2.31 2H1), 2.05 (in, IH), 1.48 (in, 2H), 1.21 (in, 28 0.84 (in, 9H).

To the solution of 2',3 -dideoxy-3 -fluoro-5 1-(N-CBz-L-valyl)-3stearoyl-2 propyloxy carbonylipropanoy guanosine (460 mg, 0.5 inmole) in a mixed solvent of methanol (10 ml), ethyl acetate (3 ml) and acetic acid (2 ml) was added palladium black (50 ing). After reaction under hydrogen atmosphere for 2 h, the mixture was filtered and the filtrate was dried. The titled product was isolated by silica gel column chromatography. 360 mng.

'H-NMR (DMSO-d6): 7.89 IH), 6.51 2H1), 6.16 (dd, 111), 5.48 (in, lH), 5.17 (in, IH), 4.28 (in, 7H), 2.90 (in, 211), 2.58 (in, 411), 2.28 2H), 1.85 (in, IH), 1.49 (in, 211), 1.22 (in, 28 11), 0.85 (in, 9H1).

WO 99/09031 PCT/SE98/01467 63 EXAMELE.23 0 -0O- stearoyl

HO

O-valyl-N-CBz A solution of stearoyl chloride (12.1g, 40 mmol, 1.0 eq) in CH 2 C12 (100 ml) was slowly (Ih) added to a solution of 2,2-bis(hydroxymethyl)propionic acid (26.8 g, 200 mmol, 5.0 eq) in pyridine (400 ml) at room temperature. The reaction mixture was stirred at room temperature overnight and thereafter concentrated (100 ml) under S:vacuum. The reaction mixture was slowly treated with saturated NaHCO 3 (400 ml) and thereafter extracted with CH 2

CI

2 (3x300 ml). The organic layers were combined, 10 washed with brine, dried over Na 2

SO

4 and concentrated in vacuum. The crude material was chromatographed on silica gel (500 g) with 19/1 to 4/1 CH 2

CI

2 -MeOH as eluent, to yield the monostearoyl ester, Rf (9/1 CH 2 C12-MeOH) 0.33. 12.5 g solution of N-Cbz-L-valine (18.85 g, 75 mmol, 2.4 eq) and DMAP (855 mg, 7 15 mmol, 0.22 eq) in CH 2 C2 (800 ml) was cooled to 0° C and treated with DCC (14.4 g, 70 mmol, 2.2 eq). The reaction mixture was stirred at room temperature for 30 min and thereafter slowly h) treated with a solution of the above monostearoyl ester (12.5 g, 31.2 mmol, 1 eq) in CHCI 3 (200 ml, free of ethanol). After stirring overnight the suspention was filtered and the filtrate was washed with brine, dried with Na 2

SO

4 and concentrated in vacuum. The crude material was chromatographed on silica gel (500 g) with 19/1 to 4/1 CH 2 Cl 2 -MeOH as eluent, to yield the above depicted diester. Rf (9/1 CH 2 C12-MeOH) 0.46. 13.8 g (70 'H-NMR (250 MHz, CDCI 3 5 7.35-7.3 5H, ArH), 5.32 1H, CH), 5.10 2H,

CH

2 Ph), 4.33-4.18 4H, CH 2 2.28 2H, CH 2 2.22-2.05 1H, CH), 1.65- 1.50 2H, CH 2 1.35-1.15 31H), 1.00-0.82 9H, Me).

WO 99/0903 1 64 PCT/SE98/01467 EXAMPLE-24 -Dideoxcy-3 '-fluoro-5'-o-r5-(L-Valvloxvy.4..AstearJX Pentanoaaosn a) Synthesis of:2' ,3'-dj deoxy-3 '-fluoro-5 'O[5(NFMOC-L-valyoxy)-4.

stearoyloxy-pentanoyl] guanosine.

A mixture of2,'ddoy3-loounsn (269 mg, 1 .0 mmole), L-ayoy--taolx-etni acid 9 4 0mg, 1.3 Jflmole), DMAP (I 6mg, 0. 13 mrnole) and HOBT 17 6 mg, 1.3 mrnole) was coevaporated two times with DMF and reduced to about 30ml. DCC 2 4 8mg, 1.2 mmole) was added and the mixture was stirred overnight at room temperature. The mixture was filtered and the solution was evaortedunerreduced pesr.Ethyl aete(50 ml) wsadded and the organic phase was washed two times with 5% acetic acid, with 5% sodium hydrogen *carbonate and with water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product is isolated by silica gel column chromatography. Yield: 4 'H-NMR (DMS0 d-6) 0.88 9H-) 1.22 (in, 28H) 1.45 (mn, 2H-) 1.83 (in, 211) 2.21 (in, 2H) 2.37 11H) 3.90 I1-H) 5.3 6-5.5 8 I H) 6.18 (in, I1H) 6.50 2H) 7.28-7.91 1011) b) Synthesis of 2' ,3'-dideoxy-3 '-fluoro-5 '-O-[5-(L-valyloxy).4-stearoyloxy.

pentanoyl] guanosine.

A mixture of 3 'dideoxy-3 '-fluoro-5 [5-(N-CBZ-Lvalyloxy)-4stearyloxypentanoyl] guanosine 3 00 mg, 0.308 mmole) in 5mi N,N-di isopropyl ethyl amine and 5m1 DMF was stirred for three days at room temperature. Acetic acid (5 ml) was added and the mixture was evaporated under reduced pressure The product was isolated as the acetate salt by silica gel column chromatography. Yield: 90 mg 'H-NMR (DMSO d-6 0.88 (in, 911) 1.24 (in, 2811) L' 55 (mn, 2H)1.91 2H) 2.31 211) 2.44 1H) 2.56-3.08 (mn, 211) 3.15 111) 4.00-4.49 (in, 5H1) 5.08 (in, 111) 5.40-5.62 (in, 111) 6.24 (in, 111) 6.54 211) 7.96 I H) WO 9909031 PCT/SE98/01467 EXAMPLE-2 3'-DidegXyv-3 4 ifluoro-5'-O-[3-(L-valyloxy)-2-stearovloxy-propanoyl1 guanosine a) Synthesis of 3'-Dideoxy-3'-fluoro-5'-O- [3-(N-CBZ-L-valyloxy)-2stearoyloxy-propanoyl]guanosine.

A mixture of-2', 3'-dideoxy-3'-fluoroguanosine (404mg, 1.5:mmole), 3-(N-CBZ-Lvalyloxy)-2-stearoyloxy-propanoic acid (1.06g 1.75 mmole),:DMAP (24mg, 0.2 mmole) and HOBT (264mg, 1.82 mmole) was coevaporated two times with DMF and reduced to about 30ml. DCC (372mg, 1.8 mmole) was added and the mixture was stirred overnight at room temperature. The mixture was filtered and the solution was evaporated under reduced pressure. Ethyl acetate (50 ml) was added and the organic phase was washed twice with 5% acetic acid, with 5% sodium hydrogen carbonate and with water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography.Yield: 0.73g 'H-NMR (DMSO d-6) 0.82 (m,9H) 1.22 28H) 1.48 (min, 2H) 2.31 2H) 2.50- 3.00 2H) 3.91 1H) 4.18-4.52 5H) 5.00 2H) 5.30-5.61 (min, 2H) 6.16 (min, 1H) 6.50 2H) 7.32 5H) 7.71 1H) 7.92 IH) 10.18 1H) b) Synthesis of 3'-dideoxy-3'-fluoro-5'-0- [3-(L-valyloxy)-2-stearoyloxypropanoyl]guanosine.

A solution of 3'-dideoxy-3'-fluoro-5'-0-[3- (N-CBZ-L-valyloxy)-2-stearoyloxypropanoyl]guanosine (350mg, 0.4 mmole) in ethyl acetate (25ml), methanol and acetic acid (5m) was hydrogenated with palladium black (300mg) with normal pressure for three hours. The catalyst was filtered and washed with ethyl acetate and methanol. The solution was evaporated under reduced pressure and the product was isolated as the acetate salt by silica gel column chromatography. Yield: 120mg WO 99/09031 66 PCT/SE98/01 4 6 7 I-l-NMR;(DMiS.d-6) 0.84 (in, 9H) 1.22 (mn, 28H) l.50'(m,v2H)-232 (in, 2H-) 2.50-3.00 (Mn;-2H) 3.07 (in, 1H-) 4.21-4.59 (in, 5H) 5 3 8 2H) 6.17 (in, 1H-) 2H) 17IJ90-(s, 1H1) EXAMPLE!26 3 '-Dideo4X-3 '-fluoro-5 '-O-r3bi(vloxneh) piropioni acidi 2uanosine a) Synthesis bf 4,4-biS (N-CBZ-L-valyloxymethyI)-but- I -ene.

To a solution of 2 -allyl-l,3-propandiol 2 .32g, 20 mmole), N-CBZ-L-valine (10.06g, 40 mmole) and DMAP (0.

4 8 8g, 4 nimole) in 120m] dichioromethane was added DCC (9.08g, 44 mmole) in portions and the mixture was stirred overnight at room *temperature. The mxuewas cooled to 5'C and the urtaewasfitrdTh filtrate was evaporated and the product was isolated by silica gel column chromatography. Yield: 9.Og H-NMR

(CDCI

3 0.89 (in, 12H-) 5.11 2H) 5.73 (in, lI-I) 0% b) Synthesis of 3,3-Bis (NCZLvllxmehl-rpoi acid. To a cooled solution of 4,4-b is (N-CBZ-L-valyloxymethyl)..but. -ene (1 4 .6g, 25 iniole) and tetrabu tyl ammonium bromide (1.3g, 4 inmole) in 120m1 benzene was added 100m] water. Under strong stirring potassium permnanganate (Il5.8g, 100 mmole) was addded in portions and the mixture was stirred for 2 hours between I 5 0 C and 20*C A sodium bisulfite aqueous solution was added to the slurry until the mixture was discolored. The mixture was acidified with 2N hydrochloric acid and extracted four times with ethyl acetate. The organic phase was washed two times with water, dried with sodium sulfate and evaporated under reduced pressure The product was isolated by silica gel column chromatography. Yield: 'H-NMR (CDC1 3 0.89 (mn, 12H-) 2.05 (in, 2H) 2.46 (in, 2H) 2.62 (mn, I1H) 4.20 (im, 6H) 5.11 4H) 5.30 (in, 2H) 7.35 (in, I01OH) WO 99/09031 PCT/SE98/01467 67 c) Synthesis'of 2.;3-dideoxy-3'-fluoro-5'-0-[3,3-bis (N-CBZ4*lvalyloxymethyl)propionyl]guanosine.

A solution of 2',3'-ddeoxy-3'-fluoroguanosine (1.35g, 5 mmole),3,3-bis (N-CBZ-Lvalyloxymethyl)-propionic acid (3.6g, 6 mmole), DMAP (0.061g, 0.5 mmole) and HOBT (0.81 g, 6-mmole) was coevaporated two times with DMF and reduced to about 120ml.:DCC (1.24g, 6 mmole) was added and the mixture was stirred overnight at room temperature. The mixture was filtered and the solution was evaporated under reduced pressure. Ethyl acetate (200 ml) was-added and the organic phase washed twice with 5% acetic acid, 5% sodium hydrogen carbonate and water.

The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography. Yield: 2.7g 1'H-NMR (DMSO d-6) 0.88 12H) 2.00(m, 2H) 2.50-3.00 2H) 3.90-4.43 10H) 5.08 4H) 5.32-5.59 1H) 6.17 1H) 6.50 2H) 7.28 7.72 2H) 7.90 1H) d) Synthesis of 3'-Dideoxy-3'-fluoro-5'-0- [3,3-bis (L-valyloxymethyl)-propionic acid] guanosine.

A solution of 3'-dideoxy-3'-fluoro-5'-0-[3,3-bis (N-CBZ-L-valyloxymethyl)propionyl] guanosine (2.6g, 3.1 mmole) in 80ml ethyl acetate, 20ml methanol and 20ml acetic acid was hydrogenated with palladium black (0.3g) for two hours under normal pressure. The catalyst was filtered and washed with ethyl acetate and methanol. The solution was evaporated under reduced pressure and the product was isolated as the bisacetate salt by silica gel column chromatography. Yield: 1.2g 'H-NMR (DMSO d-6) 0.90 12H) 1.78 2H) 2.50-3.00 2H) 3.09 2H) 4.02-4.45 8H) 5.34-5.59 1H) 6.17 1H) 6.62 2H) 7.88 1H) W 9900168 PCT/SE98/0146 7 EXAMPLE-27 3 '-DideoXy-3 '-fluoro-5 3 (Lval doxvmnethyl)4steaovyoxvbutoxb guanosine a) Synthesis of 3 '-Dideoxy3y-fluoro5'-O 3 -(N-CBZ-L-valyloxymethy])- 4 stearoyloxy-butoxycarbonyl] guanosine.

To a souin f2,'ddoy3-loounsn 2 6 9mg, L.O-mmole in absolute DMF were added pyridine (l98mg, 2.5 mmole) and a solution of 3-(N-CBZ-Lvalyloxymethyl)4steroyloxybutoxycabl chloride 7 50mg, 1.1 mmole) in dichloromethane. The mixture was stirred for three days at room temperature. The solution was evaporated under reduced pressure and the product was isolated by *silica ge column chromatography. Yield: I 0m 'H-NMR (DMS0 d-6) 0.88 (m 9H-) 1.24 (in, 28H) 5.08 2H) 6.24 (in, IH) 8.00 11H) b) Synthesis of 3 '-Dideoxy-3 '-fluoro-5 '-O-[3-(L-valyl oxymethyl)-4-stearoyloxybutoxycarbonyl~guanosine.

A mixture of 3 '-dideoxy-3 '-fluoro-5-0- 3 -(N-CBZ-L-valyloxymethyl)-4.

stearoyloxy-butoxycar.bonyl]guanosine in I~ml ethyl acetate, 2n-1 methanol and 2m1 acetic acid was hydrogenated with palladium black 4 Omg) under normal pressure for two hours. The catalyst was filtered and washed with ethyl acetate and methanol.

The solution was evaporated and the product isolated as the acetate salt by silica gel column chromatography. Yield: 7 8mg 'H-NMR (DMS0 d-6) 0.87 (in, 9H)1.22 (in, 28H)1.48 (in, 2H)1.68 (in, 2H1) 2.12 (in, 1) 2.26 (mn, 2H) 2.50-3.00 (mn, 2H) 4.00-4.42 (in, 1011) 5.34-5.58 (in, IH) 6.18 (mn, I H) 6.52 2H) 7.82 I1-H) WO 99/09031 ''PCT/SE98/01467 69 EXAMPLE 28 -Dideoxv-3 'fluoro-5'-O-r2-(L-valyloxv) stearoyllguanosine a) Synthesis of benzyl 2-hydroxystearate.

To a stirred solution of DL-2-hydroxystearic acid (3.0g, 10 mmole) in 20 ml dry DMF was added potassium tert-butoxide (1.23g, 11 mmole) and the mixture was stirred for one hour at 60 0 C. Benzyl bromide (2.14g, 12.5 mmole) was added and the mixture was stirred for six hours at 80 0 C. The mixture was evaporated under reduced pressure and 100 ml ethyl acatate was added. The organic phase was separated and washed four times with water.The organic phase was dried with sodium sulfate and concentrated in vacuo The product was isolated by silica gel column chromatography. Yield: 3.3g 'H-NMR (CDC1 3 0.88 3H) 1.26 28H) 1.62 2H) 4.20 1H) 5.20 2H) 7.36 b) Synthesis of benzyl-2-(N-FMOC-L-valyloxy)stearate.

To a solution of benzyl-2-hydroxystearate (3.2g, 8.2 mmole), N-FMOC-L-valine (3.4g, 10 mmole) and DMAP (0.12g, I mmole) in 80 ml dichloromethane was added 20 a solution of DCC (2.5g, 12 mmole) and the mixture was stirred overnight at room temperature. The mixture was cooled to 5 0 C and the urethane was filtered. The filtrate was evaporated and the product was isolated by silica gel column chromatography. Yield: 'H-NMR (CDC1 3 0.90 6H) 1.26 6H) 1.82 2H) 2.16 1H) 4.21 1H) 4.36 2H) 5.10 1H) 5.18 2H) 5.28 1H) 7.20 7.80 13H) c) Synthesis of 2-(N-FMOC-L-valyloxy) stearic acid.

A solution of benzyl-2-(N-FMOC-L-valyloxy)stearate (4.4g, 6.2 mmole) in 50 ml ethyl acetate was hydrogenated with 10% palladium on'charcoal (0.5g) with normal pressure for two hours. The catalyst was filtered and washed with ethyl acetate and WO 99/09031 '"PCT/SE98/01467 1,4-dioxane. The'solution was.evaporated under reduced pressure and.the product was isolated by silica gel column chromatography.Yield: 3 .4g 'H-NMR

(CDCI

3 0.88 6H) 1.26 28H) 1.82 2H) 2.28 1H) 4.20 1H) 4.40 2H) 5.00 1H) 5.41 1H) 7.26 7.82 8H) d) Synthesis of 2',3'-Dideoxy-3'-fluoro-5'-0-[ 2 -(N-FMOC-L-valyloxy)stearoyl] guanosine.

A mixture of 2 3 '-dideoxy-3'-fluoroguanosine (404mg, 1.5mmole), 2-(N-FMOC-Lvalyloxy)stearic acid (1.24g, 2 mmole), DMAP (24mg, 0.2 mmole) and HOBT 2 64mg, 1,95 mmole) was coevaporated two times with DMF and reduced to about 30ml. DCC 3 72mg, 1.8 mmole) was added and the mixture was stirred overnight at room temperature. The mixture was filtered and the solution was evaporated under reduced pressure. Ethyl acetate (50 ml) was added and the organic phase washed twice with 5% acetic acid, with 5% sodium hydrogen carbonate and with water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure.

The product was isolated as the acetate salt by silica gel column chromatography.

Yield: 1.2g o 'H-NMR (DMSO d-6) 0.80-0.90 9H) 1.22 28H) 2.12 1H) 2.50-3.00 S: 2H) 3.98 (m,lH) 4.96 1H) 6.17 IH) 6.50 2H) 7.32-7.95 e) Synthesis of 2',3'-dideoxy-3'-fluoro-5'-O-[ 2 -(L-valyloxy)-stearoyl] guanosine.

To a solution of 2',3'-dideoxy-3'-fluoro-5'-O-[2-(N-FMOC-L-valyloxy) stearoyl] guanosine (800mg, 0.89 mmole) in 15ml DMF was added DBU (1.35g, 8.9 mmole) and the mixture was stirred for 5 minutes at room temperature. Acetic acid (2 ml) was added and the mixture was evaporated under reduced pressure. Water (20 ml) were added and the mixture was extracted three times with dichloromethane.The organic phase was dried with sodium sulfate and evaporated under reduced pressure.

The product was isolated by silica gel column chromatography. Yield: 16 WO 99/09031 PCT/SE98/01467 71 'H-NMR.(DMSO d-6) 0.87 9H) 1.22 28H).1..70 2H) 1.88 1H) 2.50-3.00 2H) 3.20 1H) 4.32 3H) 4.94:(m, 1H) 5.32-5.54 1H) 6.14 l.H) 6.49 (s 2H) 7.89 1H) EXAMPLE 29 3'-Dideoxy-3'-fluoro-5'-0-3-[1,3-bis-(L-valyloxy)-2-propyloxvcarbonyl propanoyl guanosine a) Synthesis of 1,3-dibenzyloxy-2-propyl:succinate monoester.

o1 A solution of 1,3-dibenzyloxypropan-2-ol (6.8g, 25 mmole) and succinic anhydride (7.5g, 75 mmole) and DMAP (12.2g, 100 mmole) was stirred for one hour at 60 0

C.

The mixture was evaporated under reduced pressure, acidified with 2N HCI and extracted two times with ethyl actate. The combined organic phase was washed three times with water, dried with sodium sulfate and evaporated under reduced pressure.

The product was isolated by silica gel column chromatography. Yield: 7.8g b) Synthesis of 3'-dideoxy-3'-fluoro-5'-O-[3-(1,3-dibenzyloxy-2propyloxycarbonyl)-propanoyl] guanosine.

A mixture of 3'-dideoxy-3'-fluoroguanosine (1.61g, 6 mmole), HOBT (0.972g, 7.2 mmole), DMAP (73.3mg, 0.6 mmole) and 1,3-dibenzyloxy-2-propyl succinate monoester (2.68g, 7,2 mmole) was coevaporated two times with DMF and reduced to about 150ml. DCC (1.55g, 7.5 mmole) was added and the mixture was stirred 72 hours at room temperature. The mixture was filtered and the solution was evaporated under reduced pressure. Ethyl acetate (200 ml) was added and the organic phase washed twice with 5% acetic acid, 5% sodium hydrogen carbonate and water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure.

The product was isolated by silica gel column chromatography. Yield: 3.3g c) Synthesis of 3'-dideoxy-3'-fluoro-5'-O [3-(1,3-dihydoxy-2propyloxy carbonyl)propanoyl]guanosine.

A solution of 3'-dideoxy-3'-fluoro-5'-0-[3-(1,3-dibenzyloxy-2-propyloxy carbonyl)propanoyl]guanosine (3.2g, 5.13 mmole) in 50ml ethyl acetate, WO9/9 172 PCT/SE98,'014 6 7 methanol and lOmI acetic acid was hydrogenated with palladium black (O.6g) under psi overnight. The catalyst was filtered and washed with methanol, The solution was evaporated under reduced pressure and the product was isolated by silica gel column chromathography. Yield: 1.

6 4g d) Synthesis of 2' ,3 '-dideoxy-3'-fluoro-5'-0- f 1,3-B is (N-CBZ-LvaIyloxy)-2-propyloxycarbony]3propanoyj )guanosine.

A mixture of 2',3 '-dideoxy-3'-fluro-5' 0 [3 (1 3 -dihydroxy-2-propyloxy carbonyl)propanoyl]guanosine (Il.93g, 2.93 mmole), N-CBZ-L-valine (1.76g, 7 inmole), HOET (0-95g, 7 mmole) and DMAP (85.5mg, 0.7 mmole) was coevaporated two times with DMF and reduced to about 6 0m]. DCC (1.55g, 7.5 mmole) was added and *the mixture was stirred overnight at room tem~per'ature. The mxuewas warmed for four hours at 60'C and then cooled to about I10 0 C. The mixture was filtered and the solution was reduced under reduced pressure. Ethyl acetate (150 ml) was added and the organic phase was washed twice with 5% acetic acid, 5% sodium hydrogen carbonate and water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography. Yield: 1.6g.

e) Synthesis of 3 '-dideoxy-3 '-fluoro-5'-O-{ l, 3 -bis-(L-valyloxy).2 propyloxycarbonyl]-propanoyl )guanosine.

A solution of 2' ,3 '-dideoxy-3 '-fluoro-5 l7 3 -bis-(N-CBZLvalyloxy)-2 propyloxycarbonyl)propanoyl~guan 0 5 jfle(J.6g, 1.75 mmole) in 80m] ethyl acetate, 20m1 methanol and 20 ml acetic acid was hydrogenated with palladium black (0.3g) for two hours at room temperature and normal pressure. The catalyst was filtered and washed with methanol. The solution was evaporated under reduced pressure and the product was isolated as the diacetate salt by silica gel column chromatography. Yield: 1.02g 'H-NMR (DMS0 d-6) 0.84 (in, 12H-) 1.

8 5(m, 2.59 (in, 4H) 2.60-3. 10 (mn, 2H-) 3.11 (in, 2H) 3.61-4.39 7H) 5.19 (in, IH) 5.35-5.56 (in, 1H) 6.16 (mn, 11-) 6.62 2H-) 7.8 9 IH) WO 99/09031 PCT/SE98/01467 73 3'-Dideoxy-3'-fluoro-5'-0- 3- I -(L-valyloxy)-3-hydroxv-2-propyloxy carbonyllpropanoyl guanosine a) :Synthesis of 2',3'-dideoxy-3'-fluoro-5'-0- I-(N-CBZ-L-valyloxy)- 3-hydroxy-2-propyloxy carbonyl]-propanoyl) guanosine.

A mixture of 3'-dideoxy-3'-fluoro-5'-O-[3-(1,3-dihydroxy-2-propyloxy carbonyl)-propanoyl] guanosine (1.3g, 2.93 mmole), N-CBZ-L-valine (1.OOg, 4 mmole), HOBT (0.54g, 4 mmole) and DMAP (48.8mg, 0.4 mmole) was 1o coevaporated two times with DMF and reduced to about 60m]. DCC (0.91g, 4.4mmole) was added and the mixture was stirred for 72 hours at room temperature.

The mixture was filtered and the solution evaporated under reduced pressure. Ethyl acetate (150 ml) was added and the organic phase washed twice with 5% acetic acid, 5% sodium hydrogen carbonate and water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography. Yield: 0.99g b) Synthesis of 3'-dideoxy-3'-fluoro-5'-0- 3-[1 -(L-valy]oxy)-3hydroxy-2-propyloxycarbonyl]-propanoyl} guanosine.

A solution of 3'-dideoxy-3'-fluoro-5'-0- {3-[1-(N-CBZ-L-valyloxy)-3-hydroxy-2propyloxycarbonyl)-propanoyl}guanosine (0.82g, 1.21 mmole) in 30ml ethyl acetate, methanol and 15ml acetic acid was hydrogenated with palladium black (0.15g) for two hours at room temperature and normal pressure. The catalyst was filtered and washed with methanol. The solution was evaporated under reduced pressure and the product was isolated as th acetate salt by silica gel column chromatography. Yield: 'H.NMR (DMSO d-6) 0.84 6H) 1.86 1H) 2.58 4H) 2.63-3.02 2H) 3.10-4.38 9H) 5.34-5.55 1H) 6.16 1H) 6.56 2H) 7.90 1IH) WO 99/09031 7PCT/SE98/01467 EXAMPLE 31 5'-L-valvl-2',3'-dideoxy-3'-fluoroguanosine To a solution of dideoxy-3'- fluoroguanosine (810 mg, 3 mmole) and 4dimethylaminopyridine (73 mg, 0.6 mmole), N-CBz-L-valine (1.5 g, 6 mmole) and 1-hydroxybenzotriazole (810 mg, 6 mmole) in DMF (20 ml) was added DCC (1.36 g, 6.6 mmole). After 72 h, the reaction mixture was filtered and concentrated in vacuo.

5'-(N-CBz-L-valyl)-2', 3'-dideoxy-3'-fluoroguanosine was isolated by silica gel column chromatography (1.15 g).

This intermediate (503 mg, 1 mmole) was dissolved in a mixed solvent of ethyl acetate (10 ml), methanol (20 ml) and acetic acid (2 ml). To the mixture was added S. palladium black (100 mg) and the reaction mixture was kept under hydrogen at atmospheric pressure for 3 h. After filtration and concentration, the titled product was isolated by silica gel column chromatography (370 mg).

goose: IH-NMR (DMSO 7.94 1H), 6.52 2 6.17 (dd, 1H), 5.47 (dd, 1H), 4.15 3H), 3.15 1 3.01-2.62 2H), 1.80 IH), 0.82 (dd, 6 H).

EXAMPLE 32 3 '-Dideoxy-3'-fluoro-5-0-[2-(-L-valvlox)-proionl osin a) Synthesis of 4 -methoxybenzyl-2-hydroxypropionate.

To a stirred solution of DL -2 hydroxypropionic acid (9.0g 100 mmole) in 100 ml dry DMF was added potassium tert-butoxide (1 2 .34g, 110 mmole) and the mixture was stirred for one hour at 60 0 C. 4 -methoxybenzyl chloride (1 8 .8g 120 mmole) was added and the mixture was stirred for eight hours at 60 0 C. The mixture was evaporated under reduced pressure and 250 ml ethyl acatate was added .The organic phase was washed four times with water. The organic phase was dried with sodium sulfate and concentrated in vacuo. Yield: 16.8g

I

WO 99/09031 PCT/SE98/01467 'H-NMR (CD.Cl).1.40 3H) 3.81 3H) 4.26 1H) 5.14 2H) 6.90 2H) 7,28 2H) b) Synthesis of 4-methoxybenzyl-2-(N-CBZ-L-valyloxy)propionate.

To a solution of 4-methoxybenzyl-2-hydroxypropionate (4.2g, 20 mmole), N-CBZ-Lvaline (5.02g, 20 mmole) and DMAP (0.24g, 2 mmole) in 100 ml dichloromethane was added a solution of DCC (4.54g, 22 mmole) and the mixture was stirred overnight at room temperature. The mixture was cooled to 5 0 C and the urethane was filtered. The filtrate was evoporated and the product was isolated by silica gel column io chromatography. Yield :7.9g :'H-NMR (CDCI 3 0.88 (min, 6H) 1.50 (min, 3H) 2.26 1H) 3.81 3H) 4.34 (inm, 1H) 5.04-5.30 (min, 6H) 6.88 2H) 7.26 7H) 15 c) Synthesis of 2-(N-CBZ-L-valyloxy)-propionic acid.

To a solution of 4-methoxybenzyl-2-(N-CBZ-L-valyloxy)-propionate (7.8g, 17.5 mmole) in dichloromethane (100 ml) was added trifluoroacetic acid (10 ml) and the solution was stirred for one hour at room temperature. The solution was evaporated under reduced pressure and the product was isolated by silica gel column chromatography.Yield: 'H-NMR (CDCl 3 0.94 6H) 1.56 3H) 2.30 1H) 4.42 (min, 1H) 5.12-5.30 (min, 4H) 7.28 d) Synthesis of 2',3'-dideoxy-3'-fluoro-5-O-[2-(N-CBZ-L-valyloxy)propionyl]guanosine.

A mixture of 2',3'-dideoxy-3'-fluoroguanosine (404mg, 1.Smmole), 2-(N-CBZ-Lvalyloxy)-propionic acid (0.582g, 1.8 mmole), DMAP (22mg, 0.18 mmole) and HOBT (243mg, 1.8 mmole was coevaporated two times with DMF and reduced to about 30ml. DCC (412mg, 2.0 mmole) was added and the mixture was stirred overnight at room temperature. The mixture was filtered and the solution was evaporated under reduced pressure. 100ml ethyl acetate was added and the organic WO 99/09031 PTS9/16 76 PTS9/16 phase was wa~hed.twice with 5% acetic acid, with 5% sodium hydrogen carbonate and with water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography*.Yield: O.72g 'H-NMR (DMSO d-6) 0.92 (in, 6H) 1.40 3H) 2.10 (mn, 1H) 2.50-3.06 (mn, 2H) 4.03 (mn, IH) 4.20-4.44 (mn, 3H) 5.04 2H-) 5.12 (in, IH) 5.44-5.58 IN) 6.18 IH) 6.52 2H) 7.36 (mn, 5H) 7.70 2H) 7.92 I H) t.0 e) Synthesis of 2' ,3 '-dideoxy-3 '-fluoro-5-O-[2-(L-valyloxy)-propanoy] guanosine :A solution of 2' -dideoxy-3 '-fluoro-5.O-[2(NCBZLvalyloxy)-propanoyl] guanosine (0-6g, 1.04 inmole) in 20m]l ethyl acetate, I inI methanol and IlOmi acetic .acid was hydrogenated with palladium black (0.1g) for two hours at room *is temperature and normal pressure. The catalyst was filtered and washed with methanol. The solution was evaporated under reduced pressure to yield the title compound as the acetate salt. Yield: 'H-NMR (DMSO d-6) 0.88 (in, 6H) 1.40 3H) 1.92 4H) 2.52-3.04 (mn, 2H) 3.18 (in, I H) 4.18-4.42 (mn, 3H) 5.06 (in, INH) 5.32-5.58 (in, 2H) 6.18 (in, I H) 6.52 2H) 7.90 I H) EXAMPLE 33 3'-Di deox -3 '-fluoro-5 O 3 -[21,3-bis-(L-valyloxy) -prop~vloxvcarbonyl proyanoyl uanosine.

a) Synthesis of 4 -inethoxybenzyl succinate inonoester.

To a mixture of succinic anhyride (75g, 750 inmole) and 4 -inethoxybenyl alcohol 6 9. 1g, 500 iniole) in 1,4-dioxane 30 0in]) was added pyridine 7 9 .l1g, 1000 minole) and the mixture was stirred for five hours at 80'C The mixture was evaporated under reduced pressure and 6 00in1 of ethyl acetate and 60 mld of acetic acid were added. The organic phase was washed three times with water, dried with sodium WO 99/09031 PCT/SE98/01467 77 sulfate and evaporated under reduced pressure. The product was recrystallized from toluene.Yield: 104 g.

'H-NMR (DMSO d-6) 2.48 4H) 3,72 3H) 5.00 2H) 6.90 2H) 7.28 2H) b) Synthesis of succinic acid 2,3-dihydroxy-propyl ester, 4methoxybenzyl ester.

To a solution of glycerol (23.0g, 250 mmole), 4-methoxybenzyl succinate monoester (5.96 g, 25 mmole) and DMAP (0.36g, 3 mmole) in DMF (200ml) was added DCC (6.2g 30 mmole) and the mixture was stirred overnight at room temperature. The mixture was evaporated under reduced pressure and 150ml dichloromethane was .added. The mixture was filtered and the solution washed twice with water. The water phase was extracted two times with dichloromethane and the combined organic 15 phases were dried with sodium sulfate. The solution was evaporated under reduced pressure and the product was isolated by silica gel column chromatography.

Yield: 'H-NMR (CDCI 3 2.65 4H) 3.61 2H) 3.80 3H) 3.90 1H) 4.18 20 2H) 5.05 2H) 6.89 2H) 7.26 2H) c) Synthesis of succinic acid 2,3-bis-(N-CBZ-L-Valyloxy)-propyl ester, 4methoxybenzyl ester.

To a stirred solution of succinic acid 2,3-dihydroxy-propyl ester, 4-methoxybenzyl ester (2.9g, 9.28 mmole), N-CBZ-L-valine (5.03g, 20 mmole) and DMAP (0.244g, 2 mmole) in dichloromethane (60ml) was added DCC (4.5g, 22 mmole) and the mixture was stirred overnight at room temperature. The mixture was filtered and the solution was evaporated under reduced pressure. The product was isolated by silica gel column chromatography.Yield: 'H-NMR (CDCI 3 0.90 12H) 2,16 2H) 2.62 4H) 3.80 3H) 4.32 4H) 5.05-5.52 9H) 6.89 2H) 7.30 12H) WO 99/0903178 PCT/SE98/0146 7 d) Synthesis of succinic acid 2 3 -bis-(N-CBZ-L-valyloxy)propyl ester.

To a solution of the above intermediate (2.3g, 2.95 mmole) in dichloromethane was added trifluoroacetic acid (2.5ml) and the solution was stirred for two hours at roomtemperature. The solution was evaporated under reduced pressure and the product was isolated by silica gel column chromatography. Yield: 1,8g 'H-NMR

(CDCI

3 0.92 12H) 2.12 2H) 2.64 4H) 4.32 4H) 5.10 (s, 4H) 5.22-5.50 3H) 7.34 e) Synthesis of 2'.3'-dideoxy-3'-fluoro-5'-0-{3-[2,3-bis

(N-CBZ-L-

valyloxy)- -propyloxycarbonyl]propanoyl} guanosine.

A mixture of 3 'dideoxy-3'-fluoroguanosine (0.

5 38g, 2 mmole), HOBT (0.

3 2 7g, 2.42 mmole), DMAP(29.3mg, 0.24 mmole) and succinci acid 2 3 -bis-(N-CBZ-Lvalyloxy)-l-propyl ester (1.6g, 2.42 mmole) was coevaporated two times with DMF and reduced to about 50ml. DCC (0.

5 36g. 2.6 mmole) was added and the mixture was stirred 72 hours at room temperature. The mixture was filtered and the solution was evaporated under reduced pressure. 100ml of ethyl acetate was added and the organic phase washed twice with 5% acetic acid, 5% sodium hydrogen carbonate and water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography.

Yield: 0.65g.

'H-NMR (DMSO-d6) 0.88 12H) 2.08 2H) 2.58-3.04 6H) 3.92 2H) 4.10-4.46 7H) 5.00 4H) 5.22 1H) 5.32-5.56 1H) 6.17 1H) 6.50 2H) 7.32 10 H) 7.70 2H) 7.92 1 H) f) Synthesis of 2',3'-dideoxy-3'-fluoro-5'-O-{ 3 2 3 -bis-(L-valyloxy)- propyloxycarbonyl]-propanoyl) guanosine.

A solution of the intermediate immediately above (0.57g, 0.626 mmole) in 2 0ml ethyl acetate, 10ml methanol and 10 ml acetic acid was hydrogenated with palladium WO 99/09031 PCT/SE98/01467 79 black (O.lg) for two hours at room temperature and normal pressure. The catalyst was filtered and washed with methanol. The solution was evaporated under reduced pressure and the product was isolated by silica gel column chromatography. The product was dissolved in dichloromethane and 1M hydrogen chloride in ether (1.lml) was added. The mixture was evaporated under reduced pressure and dried in vacuo to yield the title compound as the dihydrochloride salt. Yield: 0.37g 'H-NMR (DMSO d-6) 0.92 12H) 2.12 2H) 2.58-3.04 6H) 3.75 2H) 4.16-4.50 7H) 5.19-5.60 2H) 6.18 1H) 6.76 2H) 7.92 1H) EXAMPLE 34 3'-Dideoxy-3'-fluoro-5'-0- 3-1 ,3-bis-(L-valyloxy)-2-propyloxycarbonyl] *i propanoyl guanosine, dihydrochloride salt.

a) Synthesis of succinic acid 1,3-dibromo-2-propyl ester, 4methoxybenzyl ester.

To a solution of 1,3-dibromopropan-2-ol (21.8g, 100 mmole), succinic acid 4methoxybenzyl ester (28.6g, 120 mmole) and DMAP (1.22g, 10 mmole) in dichloromethane (400ml) was added DCC (24.8g, 120 mmole) in portions at about 20 10 0 C. The mixture was stirred overnight at room temperature and cooled to about C. The mixture was filtered and the solution was evaporated under reduced pressure. 600ml of ethyl acetate was added and the organic phase was washed twice with 5% acetic acid, 5% sodium hydrogen carbonate and water. The solution was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography.Yield: 34.8g.

'H-NMR (CDCl 3 2.69 4H) 3.57 4H) 3.81 3H) 5.07 2H) 5.14 1H) 6,88 2H) 7.26 2H) WO 99/09031 PCT/SE98/01467 b) Synthesis of succinic acid 1,3-bis-(N-CBZ-L-valyloxy)-2-propyl ester, 4-methoxybenzyl ester.

To a solution of N-CBZ-L-valine 58.5 g, 232.8 mmole) in dried DMF (300ml) was added potassium-tert.-butoxide (24,68 g, 220 mmole) and the mixture was stirred for one hour at room temperature. A solution of succinic acid 1, 3 -dibromo-2-propyl ester, 4-methoxybenzyl ester (34 g, 77.6 mmole) in dried DMF (50ml) was added and the mixture was stirred for eighteen hours at 60 0 C. The potassium bromide was filtered and the solution was evaporated under reduced pressure. 6 00ml of ethyl acetate was added and the organic phase washed twice with 5% sodium hydrogen 6arbonate and with water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography.Yield: 'H-NMR (CDC1 3 0.90 12H) 2.16 2H) 2.61 4H) 3.80 3H 4.12- 4.42 6H) 5.02 2H) 5.10 4H) 5.43 3H) 6.88 2H) 7.32 12H) c) Synthesis of succinic acid 1, 3 -bis-(N-CBZ-L-valyloxy)-2-propyl ester.

To a cooled solution of the intermediate immediately above (44.5 g, 57.1 mmole) in dichloromethane (500ml) was added trifluoroacetic acid (50ml) between 5°C and 10 0 C and the solution was stirred for two hours at 10°C. The solution was evaporated under reduced pressure and two times coevaporated with toluene. 400ml of ethanol was added and the mixture was stirred for 30 minutes at 40 0 C. The mixture was cooled and the biproduct filtered. The solution was evaporated under reduced pressure and the product was isolated by silica gel column chromatography.

Yield: 33g 'H-NMR (DMSO-d6) 0.88 12H) 2.04 2H) 2.46 4H) 3.94-4.40 6H) 5.02 4H) 5.18 1H) 7.32 10H) 7,74 2H)

I

PCT/SE98/01467 WO 9/n031 81 d) Synthesis of 2',3'-dideoxy-3'-fluoro-5'-- {3-[1,3-bis-(N-CBZ-Lvalyloxy)-2-propyloxycarbonyl]propanoyl} guanosine.

A mixture of 2',3'dideoxy-3'-fluoroguanosine (17.8 g, 66 mmole), HOBT (10.64 g, 78.8 mmole), succinic acid 1,3-bis-(N-CBZ-L-valyloxy)-2-propyl ester (52 g, 78.8 mmole) and DMAP (0.96 g, 7.88 mmole) was coevaporated two times with DMF and redued to about 500ml. DCC (17.3 g, 84 mmole) was added and the mixture was stirred overnight at room temperature. The mixture was warmed for six hours at and then cooled to about 10 0 C The mixture was filtered and the solution was reduced under reduced pressure. 1200 ml of ethyl acetate was added and the organic phase was washed twice with 5% acetic acid, 5% sodium hydrogen carbonate and water. The organic phase was dried with sodium sulfate and evaporated under :reduced pressure. The product was isolated by silica gel column chromatography.

Yield: 42g.

15 'H-NMR (DMSO-d6) 0.90 12H) 2.02 2H) 2.5-3.02 6H) 3.94 2H) 4.22 7H) 5.02 4H) 5.18 1H) 5.22-5.50 1H) 6.16 1H) 6.50 2H) 7.32 10H) 7.72 2H) 7.92 1H) e) Synthesis of 2',3'-dideoxy-3'-fluoro-5'-0-{ 3-[1,3-bis-(L-valyloxy)-2propyloxycarbonyl]-propanoyl}guanosine dihydrochloride salt.

A solution of 2',3'-dideoxy-3'-fluoro-5'-0-{ 3-[1,3-bis-(N-CBZ-L-valyloxy)-2propyloxy carbonyl]propanoyl} guanosine 5.9 mmole) in 75ml ethyl acetate and methanol was hydrogenated with palladium on activated carbon 10% Pd (1 g) one hour at room temperature and normal pressure. The catalyst was filtered and washed with methanol. The solution was evaporated under reduced pressure. The product was dissolved in dichloromethane and a solution of 1M hydrogen chloride in ether (6ml) was added, while cooling. The mixture was evaporated under reduced pressure.Yield: 'H-NMR (DMSO d-6) 0.94 12H) 2.18 2H) 2.5-3.04 6H) 4.20-4.54 7H) 5.24 1H) 5.34-5.64 1H) 6.22 1H) 6.92 2H) 8.30 1H) 8.62 6H)

C'

WO 99/09031 82 PCT/SE98/01467 EXAMPLE Alternative synthesis of 2 ''-dideoxy3'fluoro5'-0_ 3-l 3-bis-(L-valoxy)-2 propyloxycarbonyll propanoyl guanosine a) Synthesis of succinic acid 1, 3 -dibromo-2-propyl ester, 1,1dimethylethyl ester.

To a solution of 1, 3 -dibromopropan-2-ol (10.9 g 50 mmole), succinic acid 1,1dimethylethyl ester Org.Chem 59 (1994) 4864) (10.45g, 60 mmole) and DMAP (0.61 g, 5 mmole) in dichloromethane (1 8 0ml) was added DCC (12.4 g, 60 mmole) in portions at about 10 0 C. The mixture was stirred overnight at room temperature and cooled to about 5 0 C. The mixture was filtered and the solution was evaporated under reduced pressure. 2 5 0ml ethyl acetate was added and the organic phase was washed twice with 5% citric acid, 5% sodium hydrogen carbonate and water. The solution was dried with sodium sulfate and evaporated under reduced pressure. The product 15 was distilled in vacuo. (bp 0,5 135-140C Yield: 16.8 g i 'H-NMR (CDC1 3 1.45 9H) 2.58 4H) 3.61 4H) 5.12 1H) b) Synthesis of succinic acid 1,3-bis-(N-CBZ-L-valyloxy)-2-propyl ester, 20 1,1-dimethylethyl ester.

To a solution of N-CBZ-L-valine (18.85 g, 75 mmole) in dried DMF (100ml) was S, added potassium tert.-butoxide (7.85 g, 70 mmole) and the mixture was stirred for one hour at room temperature. A solution of succinic acid 1, 3 -dibromo-2-propyl ester, 1,1-dimethylethyl ester 9 3 5g, 25 mmole) in dried DMF 2 0ml) was added and the mixture was stirred for eighteen hours at 60 0 C. The potassium bromide was filtered and the solution evaporated under reduced pressure. 3 00mI of ethyl acetate were added and the organic phase washed twice with 5% sodium hydrogen carbonate and with water. The organic phase was dried with sodium sulfate and evaporated under reduced pressure. The product was isolated by silica gel column chromatography. Yield: 14g WO 99/09031 PCT/SE98/01467 83 'H-NMR (CDC1 3 0.90 12H) 1.42 9H) 2.14 2H) 2.52 4H) 4.32 6H) 5.10 4H) 5.32 3H) 7.26 c) Synthesis of 1,3-bis-( N-CBZ-L-valyloxy )-2-propyl succinate monoester.

To a cooled solution of succinic acid 1,3-bis-(N-CBZ-L-valyloxy)-2-propyl ester, 1,1-dimethylethyl ester (13 g, 18.18 mmole) in dichloromethane (I00ml) was added trifluoroacetic acid (20ml) and the solution-was stirred for six hours at room temperature. The solution was evaporated under reduced pressure. 200ml ethyl acetate was added and the organic phase was washed with 5% sodium hydrogen carbonate and water. The solution was evaporated under reduced pressure.

Yield: 11.7g o 'H-NMR (DMSO-d6) 0.88 12H) 2.04 2H) 2.46 4H) 3.94-4.40 6H) 15 5.02 4H) 5.18 1H) 7.32 10H) 7.74 2H) S" Synthesis of 2',3'-dideoxy-3'-fluoro-5'-O- 3-[1,3-bis-(L-valyloxy)-2propyloxycarbonyl] propanoyl guanosine The intermediate from step c) is esterified to FLG as shown in example 34 step d) 20 and the N-protecting groups on the valyl moieties removed by conventional techniques, such as shown in Example 35 step e) or Example 29 step e).

*o *o WO 99/09031 PCT/SE98/01467 BIOLOGICAL EXAMPLE 1 Pharmacokinetics Confirmation that orally administered prodrugs of the invention release FLG in vivo is obtained in a rat model which is recognized as a useful model for assessing pharmacokinetic parameters of nucleoside analogues. The oral compositions are administered in a pharmaceutical vehicle comprising propylene glycol, or in the case of the more soluble compounds such as that'of Example 26 or Example 34, in water, to duplicate fasted animals in a dosage corresponding to 0.1 mmol/kg. For comparison, a set of rats is iv dosed with 0.01 mmol/kg of the metabolite 2',3'-dideoxy-3'-fluoroguanosine. Serum levels of the metabolite are then monitored S:in serum collected at intervals from individual animals from 0.5 to up to 12 hours following administration (5 min to 6 hours for FLG).

The metabolite is analysed with HPLC with UV detection at 254 nm, in a manner analogous to StAble et al 1995, J Pharm. Biomed. Anal. 13, 369-376. An HPLC system can be based on a 0.05 M ammonium-dihydrogen-phosphate buffer, with 1.2 2 -propanol solvent, buffered to pH 4.5 or 30 mM sodium dihydrogen phosphate buffer with 2% acetonitrile solvent buffered to pH 7.0. The column may be a 100x 2.1 mm BAS C18 5 pm particle size with a7 pm C18 guard column or Zorbax SB-CN C18 150x 4 .6mm, 5pm column. Protein binding of the compounds of the invention is neglible as is that of the metabolite and ultrafiltration through Amicon or Microcon 30 filters is useful for serum samples. Advantageously the main peak is subject to further column chromatography to better aid in resolution of FLG over low weight serum components. The iv levels are multiplied by a factor of ten in order to obtain AUC values for comparison with the oral values. Absolute oral bioavailability is determined as the ratio between °-AUCiv and °-AUCo.

WO 99/09031 PCT/SE98/01467 Table 1 6h absolute 12h absolute bioavail. bioavail. FLG Example 22 39% Example 13 37% Example 12 29% Example 25 81.5 Example 28 47.5% Example 24 60.5% Example 26 67.5% Example 29 51% estimated. **literature value The compounds of the invention thus provide significantly enhanced oral bioavailability relative to the metabolite metabolite 2',3'-dideoxy-3'fluoroguanosine. Notably, the compounds are released into the blood in a relatively sustained manner, rather than in an immediate peak. This means that effective amounts of the active metabolite are available in the blood for many hours assisting once daily dosage. Additionally, a sustained release avoids the problems of acute 1o toxicity seen in compounds with a more rapid release rate.

Although the rat is well recognized as a good model for predicting human bioavailability of nuceoide analogues, species independent bioavailability of a compound of the invention (Example 34) was confirmed in =l 1.5 kg male and female beagle dogs administered orally with 0.05 mmol/kg (38 mg/kg) compound in water or iv 0.005 mmol/kg (1.35 mg/kg) metabolite in water. Plasma collection and analysis as above.

Male dog 12 hour absolute bioavailability 51% Female dog 12 hour absolute bioavailability 74% WO 99/09031 WO 99/0903186 PCT/SE98/01467 BIOLOGICAL EXAMPLE 2 Antiviral activity Retroviruses As can be demonstrated by the methodology of Biological Example 1, the compounds of the invention release, in vivo, the metabolite 2 ',3'-dideoxy, 3'fluoroguanosine. In vitro measurement of the antiviral activity of this metabolite will thus reflect the defacto activity of the compounds of the invention.

In the XTT dye uptake assay of Koshida et al Antimicrob Agents Chemother. 33 778-780, 1989) utilising MT4 cells, the metabolite measured in Biological Example I 1 above showed the following in vitro activities against retroviruses: Table 2 :HIV or retroviral strain ICso* HIV- IJIB I pg/ml HIV-1 24 4 1 AZTr I lg/m HIV-1b0 TIBOr I pg/ml HIV-1 29/9 HIV 07 pg/ml HIV-2sBL6669 2 pg/ml SIVsM I pg/ml *Concentration of metabolite inducing 50% inhibition of viral replication It will thus be apparent that administration of the compounds of the invention induce powerful antiviral activities against the retroviruses HIV-1, HIV-2 and SIV. It should also be noted from the HIV-12441 AZTr and HIV- I 11 TIBO' results that the antiviral activity of the compounds of the invention does not show cross resistance against strains of HIV which have become resistant to other HIV agents such as the nucleoside analogue AZT or or the non-nucleoside reverse transcriptase inhibitor

TIBO.

WO 99/09031 87 PCT/SE98/01467 BIOLOGICAL EXAMPLE 3 Antiviral activity HBV The activity of antivirals on duck hepatitis B virus (DHBV) in ducks is an acknowledged animal model for the validation of in vivo hepatitis B activity in humans. The activity of the in vivo metabolite measured in Biological Example 2 above has been assayed in the DHBV model described by Sherker et al (1986) Gastroenterology 91, pp 818-824. The results are depicted in Figures 1 and 2 In short, 4 control ducks were treated with phosphate buffered saline (PBS) and 4 ducks ith 5 mg/kg/day of the active metabolite. The ducks were two days old when inoculated with DHBV and 18 days old when treatment was commenced. The .metabolite and PBS (controls) were given intraperitoneally for 10 days as twice daily injections, at 8 am and 4 pm. Treatment lasted 33 days and the animals were followed 5 weeks after the end of treatment.

The efficacy of treatment was followed by dot blot-hybridisation of DHBV DNA in serum using a radioactive probe and the amount of DHBV measured as the amount of radioactivity hybridised. Figure 1 plots the amount of DHBV DNA in serum at different timepoints before, during and after treatment.

As can be seenin Figure 1, there is no decrease in the amount of DHBV in serum during treatment with PBS (control, solid line). The animals given the metabolite measured in Biological Example 2 (broken line) showed a dramatic decrease in the amount of DHBV in serum during the first 10 days of treatment, whereupon for the remainder of treatment the level of DHBV DNA was below the detection limit at this dose of 5 mg/kg/day. Repeat experiments at dosages of 30 and 3 mg/kg/day and with congenitally infected ducks (not shown) also produced similar results, that is a dramatic fall in serum DHBV DNA to under the detection threshold. Even at the very low dose of 0.3 mg/kg/day the metabolite caused a considerable inhibition of DHBV in vivo. After the finish of treatment, virus reappeared ip the serum, as shown in Fig. 1. Reappearance of HBV after short term treatment with conventional antivirals WO 99/09031 88 PCT/SE98/0 1 4 6 7 has been observed earlier in both humans and animals with chronic hepatitis

B

infection.

As can be seen in Fig 2, the weight of the ducks increased in the same way as in the control (PBS treated) animals. The weight increase from about 270 g to about 800 g which was observed during the treatement period is so large that toxic effects, had they occurred, should be easily visible as a change in growth rate. Similar growth curves were also observed for the ducks receiving the higher dosage rate of mg/kg/day. This metabolite is thus clearly non-toxic. As the compounds of the invention are hydrolysed in vivo to give this metabolite, as established in Example 2 above, and a nature identical and therefore easily metabolized fatty acid, it can therefore be inferred that no long term toxicity problem can be expected from adminstration of the compounds of the invention. The absence of acute (short term) toxicity of the compounds of the invention when administered orally is established in Biological Example 2 above.

o *FORMULATION EXAMPLE 1 Tablet formulation 20 The following ingredients are screened through a 0.15 mm seive and dry-mixed g 3'-dideoxy-3'-fluoro-5'-0-3-[ 3 -bis-(L-valyloxy)-2propyloxycarbonyl propanoyl]guanosine 4 0 g lactose 49 g crystalline cellulose 1 g magnesium stearate A tabletting machine is used to compress the mixture to tablets containing 250 mg of active ingredient.

WO 99/09031 PCT/SE98/01467 89 FORMULATION EXAMPLE 2 Enteric coated tablet The tablets of Formulation Example 1 are spray coated in a tablet coater with a solution comprising 120 g ethyl cellulose g propylene glycol sorbitan monooleate ad 1 000 ml aq. dist.

FORMULATION EXAMPLE 3 Controlled release formulation 50 g 2',3'-dideoxy-3'-fluoro-5'-O-[5-(L-valyloxymethyl)-6stearoyloxyhexanoyl] guanosine 12'g hydroxypropylmethylcellulose (Methocell g lactose are dry-mixed and granulated with an aqueous paste of povidone. Magnesium stearate (0.5 g) is added and the mixture compressed in a tabletting machine to 13 mm diameter tablets containing 500 mg active agent.

FORMULATION EXAMPLE 4 Soft capsules 250 g 2',3'-dideoxy-3'-fluoro-5'-O-[5-(L-valyloxymethyl)-6stearoyloxyhexanoyl] guanosine 100 g lecithin 100 g arachis oil The compound of the invention is dispersed in the lecithin and arachis oil and filled into soft gelatin capsules.

Claims (1)

18. 2044 16:04 PHILLIPS ORMONDE 96141867 NO. 5567 P. 6 CLAIMIS 1. A compound of formula I 0 RiN NH Li Ly- N N NH 2 0 F wherein: L 1 is glycerol, L 2 is dicarboxylic acid selected from- oxalyl, malonyl, succinyl, glutaryl, adipyl, or succinyl;, R, is an aliphatic L-amino acid esterified to an hydroxy function of the glycerol; R 2 is an aliphatic L-amino acid esterified to a second hydroxy function of the glycerol; wherein the third hydroxy function on L 1 is esterified to a first carboxy ftinction of the dicarboxylic acid; wherein the second carboxy function of the dicarboxylic acid is esterified to the function of the nucleoside; and pharmaceutically acceptable salts thereof. 2. A compound according claim 1, wherein the dicarboxylic acid derivative is succinyl. A compound according to claim I or 2, wherein Rz is L-alanyl, L-leucyl, L-isoleucyl or L-valyl. 4. A compound according to claim 3, wherein R 2 is L-valyl. A compound according to any preceding claim, wherein both R, and R 2 are derived from the same L-amirno acid. 6. A compound according to claim 1, denoted 3'.dideoxy-3'-fluoro-5'-0-3-2,3-bis-(L- 0valyloxy)-lI-propyloxycarbonyl]-propanoyl guanosine or 3 '-dideoxy-3 '-fluoro-5 COMS ID No: SBMI-00793881 Received by IP Australia: Time 16:22 Date 2004.06-17 '18.2044 16:04 PHILLIPS ORMONDE 96141857 NO. 5567 P. 7 (1,3-bis-(L-valyloxy)-2-propyloxycarbonyl]-propanoyl guanosine or a pharmaceutically acceptable salt thereof. 7. A compound according to claim 6 denoted 3'-dideoxy-3'-fluoro-5'-O-3-[1,3-bis-(L- valyloxy)-2-propyloxycarbonyl]-propanoyl guanosine hydrochloride salt. 8. A pharmaceutical composition comprising a compound as defined in any one of claims 1 to 6 and a pharmaceutically acceptable carrier or diluent therefor. 9. A compound or salt as defined in any one of claims 1 to 7 for use in the manufacture of a medicament for the treatment or prophylaxis of HBV or retroviral infections. A method of treatment or prophylaxis of HBV or retroviral infections comprising administering to a patient in need thereof, a compound according to claim 1 or a pharmaceutical composition according to claim 8. 11. A compound according to claim 1, substantially as hereinbefore described, with reference to any one of the Examples or drawings. DATED: 17 June, 2004 PHILLIPS ORMONDE FITZPATRICK Attorneys for: MEDIVIR AB 99*9 9 a. *9 9 a 9999 9 9 9 *999 9 9 99a 9* *99999 W.'&aA.undaetrlJ7 HMd6 a. COMS ID No: SBMI-00793881 Received by IP Australia: Time 16:22 Date 2004-06-17