IL99172A

IL99172A - Antisense oligonucleotides complementary to a herpes simplex virus type 1 beta gene which are active as antiviral agents and their uses

Info

Publication number: IL99172A
Application number: IL9917291A
Authority: IL
Original assignee: Genta Inc
Priority date: 1990-08-15
Filing date: 1991-08-13
Publication date: 1999-03-12
Also published as: EP0547149A1; NZ239372A; AU3776395A; AU8617691A; TW226408B; CA2089476A1; IL99172A0; KR930701105A; IE912883A1; WO1992003051A1; EP0547149A4; JPH06500469A

Description

99172/2 Antisense oligonucleotides complementary to a herpes simplex virus type 1 β gene which are active as antiviral agents and their uses Genta Incorporated C.84239 99172/3 BACKGROUND OF THE INVENTION The present invention is directed to antisense oligomers which are complementary to a vital region of a viral genome which are active as antiviral agents.

The present invention is also directed to methods of interfering with replication of a virus after infection of host cells by the virus and to antisense oligomers which are useful in interfering with viral replication.

In viral replication, viral genes are typically activated and expressed in phases. In the replication of a virus such as a virus of the Herpes family, genes are expressed in three phases. Phase I involves the expression of about five genes. These genes are mostly regulatory in nature and are termed "alpha genes." The second set of genes expressed are called "beta genes;" their function is to make proteins that affect nucleic acid metabolism and synthesis or replication of viral DNA. The third set! of genes, the gamma genes, comprise about 30 to 40 genes that control the synthesis of structural proteins of the virus. The gamma genes are induced after the onset of viral DNA synthesis. In the usual course of viral infection and replication, the infected cell is "killed", _it may be killed outright, but alternatively; may be constructively "killed" by being unable to divide or express its own genes. In order to prevent production of viral progeny and/or minimize the number of viral progeny produced, the viral replication process should be interrupted at a stage prior to where viral progeny are produced. At a time soon after infection, viral components reprogram the infected cell's metabolism for the production of 99172/2 The use of antisense oligonucleotides that are complementary to and bind to specific target nucleic sequences, particularly specific messenger RNA's, has been suggested as a means to deactivate specific genes. (See Weintraub, "Antisense RNA and DNA, Scientific American, pages 40 to 46 (January 1990)).

The use of antisense oligomers which are complementary ' to certain splice junction mRNA' s of herpes simplex virus type 1 C'HSV-l") to specifically inhibit virus replication has been reported (See Kulka et al., Proc. Nat. Acad. Sci. (USA) 8£:6868-6872 (September, 1989)).

SUMMARY OF THE INVENTION According to the present invention, an/oligomer as described in the examples is provided, which is complementary to a target sequence of a mRNA transcript of an essential HSV-1 β gene selected from UL5, UL8, UL9, UL1½, UL29, UL30, UL42 and UL52 and which comprises a nucleic acid sequence which is necessary for viral replication such that if the sequence is deleted or, rendered nonfunctional, the virus is incapable of replication, or a mRNA transcript thereof which when hybridized to said target-" sequence inhibits or interferes with viral DNA synthesis or replication. Suitable target sequences include sequences at o proximate to a · 5'-terminal translational start or a 3'-terminal polyadenylation signal of the gene.

The present invention is also directed to the use of such an oligomer for the preparation of a pharmaceutical composition useful in methods of interfering with replication of 99172/2 oligomer which is complementary to a target sequence which comprises a vital region of the viral genome or mRNA transcript thereof. Optionally, two or more oligomers may be used wherein each oligomer is complementary to a different target sequence. Target sequences may be portions of the same gene or of different genes . ' ■ In one aspect, the present application is directed to a use for the preparation of a pharmaceutical composition useful in a method of interfering with replication of a virus after infection of host cells by the virus wherein the cells or their growth environment is contacted with an amount of an oligomer which is complementary to and which hybridizes with a messenger RNA sequence for a gene essential for viral DNA synthesis and/or replication, that is effective to interfere with/expression or function of said gene.

In one preferred aspect of the present invention, the methods of the use of the present invention are especially useful in interfering with viral replication ( in infections resulting from viruses of the family Herpesviridae, particularly human herpes viruses, especially Herpes . Simplex viruses. Thus, the present invention is also directed to uses for the preparation of a pharmaceutical composition useful in methods of inhibiting or interfering with replication of a human herpes virus, especially-a Herpes simplex virus, by contacting the virus viral DNA or ^ cells infected therewith with an oligomer complementary to a nucleic acid target sequence essential for viral DNA synthesis or replication and wherein the oligomer can selectively hybridize with said target sequenced. For Herpes Simplex viruses, preferably the target sequence comprises a mRNA transcript of an essential ?-gene. Suitable β genes include UL5, UL8, UL9, UL15, UL29, UL30, UL42 and UL52. Suitable regions of these genes for 99172/2 Among other factors, in one preferred aspect, the present invention is based on our finding that oligomers complementary to mRNA transcripts of genes that code for the β group of polypeptides that are essential for viral replication are especially effective in decreasing and/or inhibiting viral replication "in Herpes Simplex viruses.

According to an additional aspect of the present invention, uses for the preparation of a pharmaceutical composition useful in methods of treating an organism infected with a Herpes-viradae virus are provided.

Definitions As used herein, the following terms have the following meanings, unless expressly stated to the contrary: The term "nucleoside" Includes a nucleosidyl unit and is used interchangeably therewith. ^ ^ The term "nucleotide" refers to a subunit of a nucleic acid consisting of a phosphate group, a 5 carbon sugar and a nitrogen containing base. In RNA the 5 carbon sugar is ri os^; In DNA, it is a 2-deoxyribose. The term also includes analogs of l l such subunits. -· - The term "nucleotide multimer" refers to a chain of nucleotides linked by phosphodiester bonds, or analogs thereof.

An "oligonucleotide" is a nucleotide multimer generally about 3 to about 100 nucleotides in length, but which may be greater than 100 nucleotides in length. They are usually considered to be synthesized from nucleotide monomers.

A "deoxyribooligonucleotide" is an oligonucleotide consisting of deoxyribonucleotide monomers.

PATENT 191/177 A "nucleotide multimer probe" is a nucleotide multimer having a nucleotide sequence complementary with a target nucleotide sequence contained within a second nucleotide multimer, usually a polynucleotide. Usually the probe is selected to be perfectly complementary to the corresponding base in the target sequence. However, in some cases it may be adequate or even desirable that one or more nucleotides in the probe not be complementary to the corresponding base in the target sequence.

A "non-nucleotide monomeric unit" refers to a monomeric unit which does not significantly participate in hybridization of an oligomer. Such monomeric units must not, for example, participate in any significant hydrogen bonding with a nucleotide, and optionally include groupings capable of interacting after hybridization of oligomer to the target sequence, such as crosslinking alkylation, intercalating and chelating agents.

A nucleotide/non-nucleotide polymer" refers to a polymer comprised of nucleotide and non-nucleotide monomeric units.

An "oligonucleotide/non-nucleotide multimer" is a multimer generally of synthetic origin having less than 100 nucleotides, but which may contain in excess of 200 nucleotides and which contains one or more non-nucleotide monomeric units.

A "monomeric unit" refers to a unit of either a nucleotide reagent or a non-nucleotide reagent of the present invention, which the reagent contributes to a polymer.

A "hybrid" is the complex formed between two nucleotide multimers by Watson-Crick base pairing s between the PATENT 191/177 phosphorothioate analogs of oligonucleotides, phosphoamidate analogs of oligonucleotides, neutral phosphate ester oligonucleotide analogs, such as phosphotriesters and other oligonucleotide analogs and modified oligonucleotides, and also includes nucleotide/non-nucleotide polymers. The term also includes nucleotide/non-nucleotide polymers wherein one or more of the phosphorous group linkages between monomeric units has been replaced by a non-phosphorous linkage such as a formacetal linkage or a carbamate linkage.

The term "alkyl- or aryl-phosphonate oligomer" refers to nucleotide oligomers (or nucleotide/non-nucleotide polymers) having internucleoside (or intermonomer) phosphorus group linkages wherein at least one alkyl- or aryl- phosphonate linkage replaces a phosphodiester linkage.

The term "methylphosphonate oligomer" (or "MP-oligo er") refers to nucleotide oligomers (or nucleotide/non-nucleotide polymer) having internucleoside (or intermonomer) phosphorus group linkages wherein at least one methylphosphonate internucleoside linkage replaces a phosphodiester internucleoside linkage.

In some of the various oligomer sequences listed herein "p" in, e.g., as in ApA represents a phosphate diester linkage, and "E" in, e.g., as in CfiG represents a methylphosphonate linkage. Certain other sequences are depicted without the use of p or E to indicate the type of phosphorus diester linkage. In such occurrences, A as in ATC indicates a phosphate diester linkage between the 3 '-carbon of A and the 5· carbon of T, whereas A, as in ATC or ATC indicates a methylphosphonate linkage between the 3· -carbon of A and the 5 '-carbon of T or T. duplex is comprised of two complementary DNA strands, one termed the "sense" strand and one termed the "antisense" strand.

Messenger RNA transcripts are synthesized using the antisense DNA strand as a template and hence are homologous (with the replacement of T with A) to the sense strand.

The term "vital region" of a viral genome or viral DNA refers to a nucleic acid sequence which is necessary for viral replication such that if the sequence is deleted or rendered nonfunctional, the virus is incapable of replication.

The term "deblocking conditions" describes the conditions used to remove the blocking (or protecting) group from the 5* -OH group on a ribose or deoxyribose group.

The term "deprotecting conditions" describes the conditions used to remove the protecting groups from the nucleoside bases.

The term "tandem oligonucleotide" or "tandem oligomer" 1 ■ '' refers to an oligonucleotide or oligomer which is complementary to a sequence 5' or 3 ' to a target nucleic acid sequence and which is co-hybridized with the oligomer complementary to the/ target sequence. Tandem oligomers may improve hybridization of I these oligomers to the target by helping to make the target sequence more accessible to such oligomers, such as by decreasing the secondary structure of the target nucleic acid sequence.

The melting temperature or "Tm" of a duplex (such as 'a double stranded nucleic acid DNA: DNA or RNA:DNA) is defined a the temperature at which half the helical structure is lost.

Passages of the description which are not within the scope of the claims do not constitute part of the invention.

DETAILED DESCRIPTION OF THE INVENTION The present invention is directed to antisense oligomers useful as antiviral agents and to methods of interfering with viral replication in a host cell after its PATENT 191/177 are complementary to (and which hybridize with) a target nucleic acid sequence of a gene essential for viral replication or a viral messenger RNA transcript of said gene.

Preferred Target Sequences In general, preferred are target nucleic acid sequences which comprise a vital region of the viral genome. These target sequences may comprise portions of an essential gene for viral DNA replication or a mRNA transcript thereof which are "available", i.e. are in a state where the complementary oligomer is able to hybridize with the target sequence. Thus, these target sequences are preferably single stranded and relatively free of secondary structure and bound protein.

Preferred target sequences include mRNA transcripts of genes which are "essential" for DNA replication. Moreover, mRNA transcripts which are present in low numbers comprise particularly advantageous target sequences for this antisense therapy. With fewer mRNA transcripts, a lower concentration of oligomer can hybridize with and interfere with the function of a larger percentage of the mRNA from a particular gene.

Certain genes which code for mRNA's which are present in large amounts comprise less preferred target sequences, since if the function of these mRNA's is only partially blocked, the unhybridized mRNA's may proceed with the normal replicative cycle of the virus. Moreover, a proportionally larger amount of oligomer would be required to block an equivalent fraction of the mRNA.

Preferred are essential genes which are expressed during the earlier stages of DNA replication, but after the cell PATENT 191/177 ϊ been "committed" to death it will die whether or not functional virus particles are made and after death, will be dealt with by the host organism's immune system. These cells include cells which, due to the viral infection, are unable to divide and/or express their own genes. If viral DNA replication is blocked before the cell has been committed to death, the viral DNA in the cell will not be destroyed and viral DNA replication may recommence later on.

Suitable target sequences include sequences which are at or proximate to a 51 -terminal translational start or a 3 '-terminal polyadenylation signal.

Preferred target sequences include those which have a relatively high local G-C base content. Sequences having a relatively high local G-C content are preferred in part because they tend to hybridize more tightly to the complementary oligomer and exhibit a correspondingly higher Tm. Especially preferred target sequences have a high G-C base content on both ends of the target sequence that is complementary to and hybridizes with the complementary oligomer, which enables the ends of the oligomer to hybridize more tightly to the target sequence.

Preferred Oligomers These oligomers may comprise either ribonucleoside or deoxyribonucleoside monomeric units; however, deoxyribonucleoside mono eric units are preferred.

Preferred are oligomers which comprise from about 6 to about 40 nucleotides, more preferably from about 12 to about 20 nucleotides. Although oligomers which comprise more than about 20 nucleotides may be used, where complementarity to a longer PATENT 191/177 i structure of the target nucleic acid, such as a mRNA.

Alternatively, it may be advantageous to use more than one oligomer, each oligomer complementary to a distinct target sequence which may be part of the same gene or a different gene.

Although nucleotide oligomers (i.e., having the phosphodiester internucleoside linkages present in natural nucleotide oligomers, as well as other oligonucleotide analogs) may be used according to the present invention, preferred oligomers comprise oligonucleoside alkyl and aryl-phosphonate analogs, phosphorothioate oligonucleoside analogs, phosphoro- amidate analogs and phosphotriester oligonucleotide analogs.

However, especially preferred are oligonucleoside alkyl- and aryl-analogs which contain phosphonate linkages replacing the phosphodiester linkages which connect two nucleosides. The preparation of such oligonucleoside alkyl and aryl-phosphonate analogs and their use to inhibit expression of preselected nucleic acid sequences is disclosed in U.S. Patent Nos. 4,469,863; 4,511,713; 4,757,055; 4,507,433; and 4,591,614, the disclosures of which are incorporated herein by reference. A particularly preferred class of those phosphonate analogs are methylphosphonate oligomers.

Such alkyl- and aryl-phosphonate oligomers advantageously have a nonionic phosphorus backbone which allows better uptake of oligomers by cells. Also, the alkyl- and aryl-phosphonate intermonomeric linkages of such alkyl- and aryl-phosphonate oligomers are advantageously resistant to nucleases.

Where the oligomers comprise alkyl- or aryl-phosphonate oligomers, it may be advantageous to incorporate nucleoside monomeric units having modified ribosyl moieties. The use of PATENT 191/177 i oligomers may advantageously improve hybridization of the oligomer to its complementary target nucleic acid sequence.

Synthetic methods for preparing methylphosphate oligomers ("MP-oligomers") are described in Lee, BL. ejt al. , Biochemistry 27:3197-3203 (1988) and Miller, P.W., et ai. , Biochemistry 25:5092-5097 (1986), the disclosure of which are incorporated herein by reference.

Preferred are oligonucleoside alkyl- and aryl-phosphonate analogs wherein at least one of the phosphodiester internucleoside linkages is replaced by a 31 - 5' linked internucleoside methylphosphonyl (MP) group (or "methyl-phosphonate") . The methylphosphonate linkage is isosteric with respect to the phosphate groups of oligonucleotides. Thus, these methylphosphonate oligomers ("MP-oligomers") should present minimal steric restrictions to interaction with complementary polynucleotides or single-stranded regions of nucleic acid molecules. These MP-oligomers should be more resistant to hydrolysis by various nuclease and esterase activities, since the methylphosphonyl group is not found in naturally occurring nucleic acid molecules. It has been found that certain MP-oligomers are more resistant to nuclease hydrolysis, are taken up in intact form by mammalian cells in culture and can exert specific inhibitory effects on cellular DNA and protein synthesis (See, e.g., U.S. Patent No. 4,469,863).

If desired, labeling groups such as psoralen, chemiluminescent groups, cross-linking agents, intercalating agents such as acridine, alkylating agents or groups capable of cleaving the targeted portion of the viral nucleic acid such as molecular scissors like o-phenanthroline-copper or EDTA-iron may PATENT 191/177 binding to the desired nucleic acid sequence. More preferred are MP-oligomers having from about 6 to about 40 nucleosides, especially preferred are those having from about 10 to about 25 nucleosides. Due to a combination of ease of preparation, with specificity for a selected sequence and minimization of intra- oligomer-internucleoside interactions such as folding and coiling, particularly preferred are MP-oligomers of from about 12 to 20 nucleosides.

One group of preferred MP-oligomers includes MP- oligomers where the 5 · -internucleoside linkage is a phosphodiester linkage and the remainder of the internucleoside linkages are methylphosphonyl (or methylphosphonate) linkages. Having a phosphodiester linkage on the 5' -end of the MP-oligomer permits kinase labelling and electrophoresis of the oligomer.

Preferred Embodiment of the Invention Infections due to viruses of the family Herpesvirdae comprise particularly suitable targets for therapy using the antisense oligomers and methods of the present invention. Herpes viruses vary greatly in their biological properties. Some have a wide host cell range, multiply efficiently and rapidly destroy the cells which they infect (HSV-1, HSV-2) . Others have a narrow host cell range. A ubiquitous property of these herpes viruses is their capacity to remain latent in the host in which they multiply. The mechanism by which the virus perpetuates itself appears to reflect a function of dedicated viral genes as well as association with appropriate cells. In general, infections caused by herpes viruses have been found to be persistent.

Herpes viruses for which therapy using these antisense oligomers PATENT 191/177 i Varicella-Zoster virus, Epstein-Barr virus, Cytomegalovirus and human herpes viruses 6 and 7.

In one preferred embodiment, the present invention is directed to antisense oligomers which are useful as antiviral agents against herpes simplex virus ("HSV") , particularly type 1 ("HSV-l"), and to methods of controlling HSV-1 infections by inhibiting and/or interfering with replication of HSV-1.

According to the present invention, antisense oligomers are provided that are complementary to "essential" genes.

In Herpes viruses, as much as about one half of viral genes are non essential; that is, they may be deleted or at least reduced in expression or treated with antisense oligomers and not effect viral replication.

Preferred target sequences for these antisense oligomers comprise essential genes, that is genes which when deleted or their function is compromised, significantly affect viral replication, particularly the synthesis and/or replication of DNA. Also, as noted, preferred target sequences include mRNA transcripts of such essential genes, wherein copies are present only in low numbers. For this reason, we have found that essential β genes of HSV-1 to comprise particularly suitable target seguences for these antisense oligomers.

HSV-1 has about 15 β genes, of which at least about 8 have been reported to be essential. These essential β genes include the genes termed UL5, UL8, UL9, UL15, UL29, UL30, UL42 and UL52. These genes have been reported to code for proteins which are necessary for viral DNA synthesis and/or replication. Seven of these genes have been reported to be required for viral-origin-dependent DNA synthesis and to map in the L component of PATENT 191/177 protein designated as ICP8 (UL29) with an apparent molecular weight of 124,000; a protein binding to the origin of viral DNA synthesis (UL9) with a translated molecular weight of 94,000; a protein that binds to double-stranded DNA (UL42) with a molecular weight of 62,000; and three additional proteins (UL5, predicted molecular weight of 99,000; UL8, predicted molecular weight of 80,000; and UL52, predicted molecular weight of 114,000). These three proteins form a complex in which each protein is present in equimolar ratios and which functions as a primase and helicase. The protein specified by UL5 has independently been shown to act as a DNA dependent ATPase.

The above noted seven proteins appear to be all that is necessary for ori8-dependent amplification of DNA transfected into cells. For this reason, oligomers which are complementary to the mRNA of one of these seven genes are particularly preferred and comprise especially suitable antiviral agents against HSV-1.

Of the above noted seven essential genes, preferred are the genes denoted UL5, UL8 and UL52. It is believed that the mRNA transcripts of these genes comprise target sequences which are particularly susceptible to inhibition using these antisense oligomers.

Portions of these essential genes which may be relatively more available to these antisense oligomers comprise especially suitable target sequences. It is believed that sequences that are proximate to the 5' -terminal translational start of these mRNA transcripts or to the 3 ' -terminal polyadenylation signal comprise especially suitable target sequences in view of their demonstrated susceptibility to PATENT 191/177 :l the mRNA does not interfere with its ability to hybridize to a complementary oligomer.

Antisense oligomers complementary to selected regions of mRNA transcripts of these seven genes have been assayed for antiviral activity using a Virus Titer Reduction Assay (see Example A) and a Direct Plaque Assay (Example B) and have been found to demonstrate antiviral activity (see Tables II, III and IV) .

To assist in understanding the present invention, the following examples are included which described the results of a series of experiments. The following examples relating to this invention should not, of course, be construed in specifically limiting the invention and such variations of the invention, now known or later developed, which would be within the purview of one skilled in the art are considered to fall within the scope of the present invention as hereinafter claimed.

EXAMPLE 1 PREPARATION OF PHOSPHATE DIESTER OLIGOMERS Phosphate diester oligomers are prepared using a Biosearch model 8750 DNA synthesizer using standard phosphoro-amidite chemistry (M.H. Caruthers, et ai. , Methods of Enzymol. 154:287-313 (1985)) according to the manufacturers recommendations. The 51 -dimethoxytrityl protecting group is left on at the end of the synthesis to permit purification on a Sep- TM · · · Pak C18 cartridge (Millipore/Waters, Bedford, MA) as described by K.M. Lo et al. (Proc. Natl. Acad. Sci. (USA) 11:2285-2289 (1984)). During this procedure, the dimethoxytrityl protecting group was removed.

PATENT 191/177 i EXAMPLE 2 PREPARATION OF METHYLPHOSPHONATE OLIGOMERS Methylphosphonate oligomers are synthesized using methylphosphonamidite monomers, according to the chemical methods described by P.S. Miller et al. (Nucleic Acids Res. 11: 6225-6242 (1983) ), A. Jager and J. Engels (Tetrahedron Letters 2J5: 1437-1440 (1984) ) and M.A. Dorman et al. (Tetrahedron Letters 40:95-102 (1984)). Solid phase synthesis is performed on a Biosearch Model 8750 DNA synthesizer according to the manufacturer's recommendations with the following modifications: "G" and "C" monomers are dissolved in 1:1 acetonitrile/dichloromethane at a concentration of 100 mM. "A" and "T" monomers are dissolved in acetonitrile at a concentration of 100 mM. DEBLOCK reagent -2.5% dichloroacetic acid in dichloromethane. OXIDIZER reagent = 25 g/L iodine in 2.5% water, 25% 2 , 6-lutidine, 72.5% tetrohydrofuran. CAP A= 10% acetic anhydride in acetonitrile. CAP B = 0.625% Ν,Ν-dimethylaminopyridine in pyridine. The 5'-dimethoxytrityl protecting group is left on at the end of the synthesis to facilitate purification of the oligomers, as described below.

The crude, protected methylphosphonate oligomers are removed from the solid support by mixing with concentrated ammonium hydroxide for two hours at room temperature. The solution is drained from the support using an Econo-Column™ (Bio-Rad, Richmond, CA) and the support is washed five times with 1:1 acetonitrile/water. The eluted oligomer is evaporated to dryness under vacuum at room temperature. Next, the protecting groups are removed from the bases with a solution of ethylenediamine/ethanol/acetonitrile/water (50:23.5:23.5:2.5) for PATENT 191/177 'ί The 51 -dimethoxytrityl ("trityl") containing oligomers are purified from non-tritylated failure sequences using a Sep- Pak™ C18 cartridge (Millipore/Waters Bedford, MA) as follows: The cartridge is washed with acetonitrile, 50% acetonitrile in 100 mM, triethylammonium bicarbonate (TEAB, pH 7.5) and 25 mM TEAB. Next," the crude methylphosphonate oligomer is dissolved in a small volume of 1:1 acetonitrile/water and then diluted with 25 mM TEAB to a final concentration of 5% acetonitrile. This solution is then passed through the cartridge. Next, the cartridge is washed with 15-20% acetonitrile in 25 mM TEAB to elute failure sequences from the cartridge. The trityl-on oligomer remaining bound to the cartridge is then detritylated by washing with 25 mM TEAB, 2% trifluoroacetic acid, and 25 mM TEAB, in that order. Finally, the trityl-selected oligomer is eluted from the cartridge with 50% acetonitrile/water and evaporated to dryness under vacuum at room temperature.

The methylphosphonate oligomers are further purified by reverse-phase HPLC chromatography as follows: A Beckman System Gold HPLC is used with a Hamilton P P-1 column (Reno, NV, 10 μ, 7 mm i.d. x 305 mm long). Buffer A = 50 mM triethylammonium acetate (pH 7) ; Buffer B = 50% acetonitrile in 50 mM triethylammonium acetate (pH 7) . The sample, dissolved in a small volume of 10-50% acetonitrile/water, is loaded onto the column while flowing at 2.5-3 ml/minute with 100% Buffer A.

Next, a linear gradient of 0-70% Buffer B is run over about 30-50 minutes at a flow rate of about 2.5-30 ml/minute.

Fractions containing full length methylphosphonate oligomer are collected, evaporated under vacuum and resuspended in 50% acetonitrile/water.

PATENT 191/177 ;l EXAMPLE 3 INHIBITION OF HERPES SIMPLEX VIRUS-1 REPLICATION Oligomers complementary to designated sequences of certain genes of herpes simplex virus-1 ("HSV-1") were prepared.

Sequences are reported in Tables I and IV.

These oligomers were assayed for their ability to inhibit HSV-1 replication according to the Virus Titer Reduction Assay (Example A) and/or The Direct Plaque Assay (Example B) .

Results are reported in Tables II, III, IV and V.

EXAMPLE A VIRUS TITER REDUCTION The Virus Titer Reduction assay measures the ability of an oligomer to inhibit the total yield of virus produced by a group of cells. This test consists of two parts. First, a plate of cells is infected with virus; second, oligomer in media or media alone is added; and third, the cells are incubated for one to several replications of virus. The cells are then harvested from the well and various dilutions of this harvest are used to infect fresh monolayers of cells. The amount of virus found, measured by plaque formation, is the total amount of virus produced by the initial cells. A comparison of the total virus produced by treated and untreated cells is a measure of the inhibition of virus by the test drug. Results are reported in Tables II, III, IV (under "VTR" ) , and V.

EXAMPLE B DIRECT PLAQUE ASSAY The Direct Plaque Assay measures the ability of an PATENT 191/177 1 overlay limits all spread of virus from cell to cell through the extracellular fluid, but not by direct contact or extension. The resultant plaques can then be counted and observed for size. A comparison of plaque number and size in treated and untreated cells provides the information desired. Results are reported in Table IV under "PLAQUE.11 PATENT 191/177 TABLE I A . COMPLEMENTARY TO AREA AROUND TRANSLATIONAL START OLIGOMER NO. GENE LOCATION SEOUENCE 0015 UL5 -15 — +3 5 -CAT-GAC-CGC-ACC-ACG-CTC-31 0013 UL8 -5 -→ +13 5 -CTG-CQG-TGT-CCA-TCG-CAC-31 0021 UL8 +1 -→ +18 5 -GAT-ATC-TGC-GGT-GTC-CAT-3 ' 0028 UL8 +19 -→ +35 5 -CTC-TCC-TCC-ACC-CAC-AC-3 » 0046 UL8 5 -CCT-CCA-CCC-ACA-GCG-TAT-3 ' 0047 UL8 5 -GGC-CCC-TAA-GGA-TCA-CGG-3 ' 0007 UL9 -5 -→ +13 5 -CCA-CGA-AAG-GCA-TGA-CCG-31 0056 UL15 -6 — +12 5 -CTG-ACC-AAA-CAT-CGC-GCA-31 0054 UL29 -5 -→ +13 5 -GCT-TTG-TCT-CCA-TGT-CCT-3 ' 0039 UL30 -3 -→ +15 5 -GCC-ACC-GGA-AAA-CAT-CGC-3 » 0016 UL 2 -7 -→ +11 5 -GAA-TCC-GTC-ATC-CCA-ACG-3 ' 0052 UL52 -21 -→ -4 5 -GTC-CGC-GCG-CCC-AAG-GGC-3 ' 0019 UL52 -3 -→ +15 51 -GTC-TTC-CTG-CCC-CAT-TGC-31 0053 UL52 +16 -→ +33 5' -CCT-CTC-CCC-GCG-GTT-CCC-31 A, C, G or T = Phosphate diester linkage A, C, G or T = Methylphosphonate linkage PATENT 191/177 B. COMPLEMENTARY TO POLY A SIGNAL OLIGOMER NO. GENE LOCATION SEOUENCE 0005 UL5 -3 +15 5 -TTT-GTT-GTC-TTT-AAT-GGA-3 0006 UL5 +5 —* +22 5 -CTG-GTT-GTT-TGT-TGT-CTT-3 0020 UL5 +12 —» +29 5 -AAT-TTG-GCT-GGT-TGT-TTG-3 0008 UL5 +23 —→ +40 5 -AAT-AAC-ACA-TAA-ATT-TGG-3 0023 UL5 +41 —► +58 5 -GCG-TGT-TTG-ATC-TTA-ATA-3 0059 UL5 +59 —-► +76 5 -ACC-CTG-ATC-GCC-CGT-CGC-3 0051 UL8 -15 -→ +3 5 -AAC-AGA-AAC-GAC-ATC-TTG-3 0024 UL8 +4 «■- +21 5 -ATT-GGT-CAA-ACT-GAG-GCA-3 0014 UL8 +22 —→ +39 5 -TCT-CAG-GGC-AAT-GTT-TTT-3 0022 UL8 +40 —→ +57 5 -CAC-GGG-GGA-GCG-CTC-TTG-3 0057 UL15 -13 -→ +5 5 -TTA-TTQ-GQC-GCT-CAC-QAG-3 0055 UL29 +4 — +21 , 5 -ATG-TCG-TAG-CAA-TAA-TTT-3 0040 UL30 +3 —+ +20 5 -GTC-GGC-CGC-AGA-CAT-TTA-3 0025 UL42 -6 ——> +12 5 -ACC-AAG-TTT-ATT-TAC-ATT-3 0017 UL42 +4 —→ +21 5 -TTG-GGC-AAT-ACC-AAG-TTT-3 0018 UL 2 +22 —→ +39 5' -GCG-ACA-CGC-GGG-AAA-GTG-3 0026 UL 2 +40 +58 5 -CAC-ACA-CAT-GAA-CCA-CAC-3 0151 UL42 +59 —♦ +76 5 -GAG-GGT-GGG-GGC-GCC-AGG-3 0027 UL52 +3 +20 5' -GTA-CGT-GGC-ATG-TAT-T A-3 0038 UL52 +21 —+ +38 5' -ACC-AAT-CAG-ACA-CCA-TAA-3 0035 UL52 +39 +56 5' -CCT-CCG-GCA-CAG-ACA-AGG-3 A, C, G or T = Phosphate diester linkage A, C, G or T = Methylphosphonate linkage PATENT 191/177 TABLE II -HERPES SIMPLEX VIRUS TYPE 1 ACTIVITY (TRANSLATIONAL START) OLIGOMER NO. GENE LOCATION ¾ INHIBITION (Gene Product) (ATG START +1) (MAXIMUM) +1 UL5 0015 DNA DNP. ATPase -15--- -+3 63% UL8 HELICASE/PRIMASE 0013 5- -+13 78% 0021 +1- +18 45% 0028 -+35 62% UL9 ORIGIN BINDING PROTEIN 0007 -+13 49% UL15 SPLICE JUNCTION 0056 -6- -+12 7% UL29 BINDING PROTEIN 0054 -5- -+13 68% UL30 DNA POLYMERASE 0039 -3· -+15 50% UL42 DNA SYNTHESIS PROTEIN 0016 26% UL52 HELICASE/PRIMASE 0052 -21 4 63% 0019 -3- -+15 79% 0053 +16- -+33 74% PATENT 191/177 TABLE III ANTI-HERPES SIMPLEX VIRUS TYPE 1 ACTIVITY (POLY A SIGNAL) OLIGOMER NO. GENE LOCATION % INHIBITION (Gene Product) +1 (MAXIMUM) A (A) TAAA UL5 DNA DNP. ATPase 0005 -3 +15 73% 0006 +5 +22 69% 0020 +12 +29 18% 0008 +23 +40 17% 0023 +41 +58 96% 0059 +59 : +76 18% UL8 HELICASE/PRIMASE 0051 -15 +3 86% 0024 +4 +21 71% 0014 +22 +39 10% 0022 +40 +57 58% UL15 SPLICE JUNCTION 0057 -13 +5 32% UL29 DNA BINDING PROTEIN 0055 +4 +21 10% UL30 DNA POLYMERASE 0040 +3 +20 55% UL42 DNA SYNTHESIS PROTEIN 0025 -6 +12 17% 0017 +4 +21 33% 0018 +22 +39 54% 0026 +40 +58 93% 0151 +59 +76 44% UL52 HELICASE/PRIMASE 0027 +3 +20 87% 0038 +21 +38 98% 0035 +39 +56 66% PATENT 191/177 TABLE IV % REDUCTION OLIGOMER OF HSV-1 NO. GENE SEOUENCE CONC. VTR PLAOUE 0002 UL8 51 -CTG-CGG-TGT-CCA-TCG-CAC-31 ΙΟΟμΜ 35% 0002 UL8 5 ' -CTG-CGG-TGT-CCA-TCG-CAC-3 · 200μΜ 63% 0002 UL8 5 · -CTG-CGG-TGT-CCA-TCG-CAC-3 · ΙΟΟμΜ 49% 0002 UL8 51 -CTG-CGG-TGT-CCA-TCG-CAC-3 · 200μΜ 76% 0002 UL8 51 -CTG-CGG-TGT-CCA-TCG-CAC-31 200μΜ 29% 0002 UL8 51 -CTG-CGG-TGT-CCA-TCG-CAC-31 200μΜ 23% 0004 UL8 5 ' -GAT-ATC-TGC-GGT-GTC-CAT-3 · 200μΜ 32% A, C, G or Τ = Phosphate diester linkage , C, G or T = Methylphosphonate linkage TABLE V A. MULTIPLE OLIGOMERS COMPLEMENTARY TO ONE GENE Oligomer No. Gene Alone Together (1) 0021 UL8 (32%) 82% 0028 UL8 (62%) (2) 0013 UL8 0046 UL8 99% 0047 UL8 B. TWO OLIGOMERS COMPLEMENTARY TO TWO GENES Oligomer No. Gene Together 0013 UL8 67%

Claims

1. 25 99172/4 WE CLAIM: 1. An oligomer as hereinbefore described, which is complementary to a target sequence of a mRNA transcript of an essential HSV-1 β gene selected from UL5, UL8, UL9, UL15, UL29, UL30, UL42 and UL52, which comprises a nucleic acid sequence which is necessary for viral replication such that if the sequence is deleted or rendered nonfunctional, the virus is incapable of replication, or a mRNA transcript thereof which when hybridized to said target sequence inhibits or interferes with viral DNA synthesis or replication. 2. · An oligomer according to claim 1 which comprises an alkyl- or aryl-phosphonate oligomer. 3. An oligomer according to claim 2 which comprises a methylphosphonate oligomer. 4. An oligomer according to claim 3 wherein said target sequence comprises a portion of a mRNA transcript of a gene essential for viral DNA synthesis or replication as hereinbefore described. 1 5. An oligomer according to claim 4 wherein said target sequence is at or proximate to a 5' -terminal translational start or a 3' -terminal polyadenylation signal of said gene. 6. An oligomer according to claim 1 wherein said target sequence is at or proximate to a 5' -terminal translational start or a 3 ' -terminal polyadenylation signal of said gene. 7. An oligomer according to claim 1 wherein said oligomer comprises a methylphosphonate oligomer. 26 99172/4 8. The use of an oligomer according to Claim 1 for the preparation of a pharmaceutical composition useful in a method of interfering with replication of a virus after infection of host cells by said virus, said method comprising contacting said cells or their growth environment with an amount of said oligomer which is complementary to and which hybridizes with a messenger RNA sequence for a gene essential for viral DNA replication as hereinbefore described effective to interfere with expression or function of said gene, substantially as described in the specification. 9. · . Λ use according to claim 8 wherein said virus is a Herpesviridae virus. 10. Λ use according to claim 9 wherein said virus is selected from Herpes Simplex Virus Type 1, Herpes Simplex Virus Type 2, Varicella-Zoster virus, Epstein-Barr Virus, Cytomegalovirus, human herpes virus 6 and human herpes virus 7. 11. , Λ use according to claim 10 wherein ■ said virus comprises a Herpes Simplex Virus. ί / 12. Λ use according to' claim 11 wherein said gene comprises an essential beta gene as hereinbefore described. 13. , A use according to claim 12 wherein said gene is selected from UL5 , UL8 , .UL15 , UL9 , UL29, UL30, UL42 and UL52. 14.. A - use according to' claim 13wherein said oligomer is complementary to a sequence at or proximate to the 5' -terminal translational start or the 3' -terminal polyadenylation signal of said gene. 15. A use according to claim ^ wherein said gene is selected from UL5, UL8 or UL52. 16. ·· A use according to claim 15 wherein said oligomer is complementary to a sequence at or promixate to the 5' -terminal translational start or the 3 '- erminal' polyadenylation signal of said gene. 27 99172/4 , 17. The use of an oligomer according to Claim 1 for the preparation of a pharmaceutical composition useful in a method of inhibiting or interfering with DNA synthesis or replication of a virus, said method comprising contacting said virus or viral DNA or their environment with said oligomer which is complementary to a target sequence which comprises a vital region of the viral genome as hereinbefore described or a mRNA transcript thereof, substantially as described in the specification. 18.' Λ use · according to claim 17 wherein said vital region comprises a gene essential for viral DNA synthesis or replication. . 19. Λ use according to claim 18 wherein said virus is a Herpesviridae virus. - 20. The use of an oligomer according to Claim 1 for the preparation of a pharmaceutical compositio useful in a method of inhibiting or interfering with replication of a human herpes virus, said method comprising contacting said virus, viral DNA or cells infected therewith with said oligomer complementary to a nucleic acid target sequence essential for viral DNA synthesis or repli- cation as hereinbefore described wherein said oligomer can selectively hybridize with said target sequence, substantially as described in the specification . ' 21. Λ use according to claim20 wherein said human herpes virus comprises a Herpes Simplex Virus and said target sequence qomprises a inRNA transcript of an essential pgene as hereinbefore described. 22· Λ use according to claim 21 wherein said gene is selected from UL5 , ULB , UL9, UL15, UL29, UL30, UL42 and UL52. 23. A use according to claim 22 wherein said oligomer comprises a methylphosphonate oligomer. 24. Λ use according to claim 22 wherein said target 28 99172/4 Λ use according to claim 2 wherein said gene is selected from UL5, UL8 and UL52. 26. Λ use according to claim 25 wherein said oligomer comprises a methylphosphonate oligomer. 27.·_ Λ use according to claim 25 wherein said target sequence is proximate to a 5' -terminal translational start or a 3' -terminal polyadenylation signal. 28. Λ use according to claim 27 wherein said oligomer comprises a methylphosphonate oligomer. 29. · . The use of an oligomer according to Claim 1 for the preparation of a pharmaceutical composition useful in a method of treating an organism infected with a Herpesviradae virus, said method comprising contacting said organism or cells thereof with a therapeutically effective amount of an oligomer which is complementary to a target sequence which comprises an essential gene for DNA synthesis or replication as hereinbefore described or a mRNA transcript thereof, substantially as described in the specification. j | 30. Λ use according to claim 29 wherein said virus is selected from a Herpes Simplex Virus, type 1 or 2, Epstein-Barr virus, Cytomegalovirus, Varicella-Zoster virus, humn herpes virus 6 and human herpes* /virus 7. 31, The use of an oligomer according to Claim 1 for the preparation of a pharmaceutical composition useful in a method of treating an organism or cells thereof infected with Herpes Simplex Type 1 Virus, said method comprising the administration to said organ ism or cells of a therapeutically effective amount of an oligomer which is sufficiently complementary to selectively hybridize to a target sequence which comprises a gene essential for viral DNA replication or synthesis as hereinbefore described or mRNA transcript thereof, substantially as described in the specifica 29 99172/4 32.. Λ use according to claim 31 wherein said gene is selected from UL5, ULB, UL9, UL15, UL29, UL30, UL42 and UL52. 33.. Λ use according to claim 32 wherein said oligomer comprises only methylphosphonate internucleoside ' linkages. 34. Λ use according to claim 33 wherein said oligomer comprises from about 6 to about 30 nucleosides. or , The use of an oligomer according to Claim 1 for the preparation of a pharmaceutical composition useful in a method of inhibiting or interfering DNA synthesis or replication of a virus, said method comprising contacting said virus or a viral DNA with two or more oligomers wherein each oligomer is complementary to a different specific target sequence and wherein each target sequence comprises a vital region of the viral genome or as hereinbefore described, a mRNA transcript theredf, substantially as described in the specification. 3g# Λ use according to claim 35 wherein each tax-get sequence comprises a portion of a mR]h transcript complementary to an essential gene as hereinbefore described. 37. A use according to claim 36 wherein each target sequence comprises a portion of the same essential gene. j 38. Λ use ^according to claim 37 comprising three or more oligomers. ■ 39· A use according to claim 37 wherein each target sequence comprises a portion of a different essential gene. 40. A use according to claim .39 comprising three or more oligomers. 30 99172/3 .41,· The use of an oligomer' according to Claim 1 for the preparation of a pharmaceutical composition useful in a method of treating an organism infected with a Herpesviradae virus , said method comprising contacting said organism or cell's thereof with a therapeutically effective amount of two or more oligomers, wherein each oligomer is complementary to a different target sequence which comprises a portion of an essential gene for DNA synthesis, as hereinbefore described or a mRNA transcript there- of, substantially as described in the specification. . 42, A use according to claim 41 wherein each target sequence comprises a portion of the same essential gene. 43. Λ use according to claim 42 comprising three or more oligomers. 44. A -use according to claim ,41 whe'r,ein each target seuqence comprises a portion of a different essential gene. 45. A use according to claim 44 comprising three or more oligomers.