AU697095B2

AU697095B2 - Expression of viral decoy proteins under the control of a locus control region and uses thereof

Info

Publication number: AU697095B2
Application number: AU77026/94A
Authority: AU
Inventors: David Abraham; Roger Kingdon Craig; Elaine Dzierzak; Franklin Gerardus Grosveld
Original assignee: Medical Research Council; Therexsys Ltd
Current assignee: Medical Research Council; Cobra Therapeutics Ltd
Priority date: 1993-09-24
Filing date: 1994-09-26
Publication date: 1998-09-24
Anticipated expiration: 2014-09-26
Also published as: WO1995008635A1; AU7702694A; CA2172073A1; EP0725830A1; GB9319772D0; JPH09505984A

Description

WO 95/08635 PCT/GB94/02092 EXPRESSION OF VIRAL DECOY PROTEINS UNDER THE CONTROL OF A LOCUS CONTROL REGION AND USES THEREOF The present invention relates to an agent for anti-viral therapy which possesses a protective effect when administered to healthy individuals. In particular, the agent of the invention may be a mutant HIV gene product.

Introduction Human immunodeficiency virus (HIV) has been identified as the ctiological agent in human acquired immunodeficiency syndrome (AIDS) (Barre-Sinoussi et al., 1983; Gallo et al., 1984). Conventional therapeutic strategies have concentrated on antiviral drugs such as AZT and on the development of preventive vaccines. However, the intracellular immunisation approach (Baltimore, 1988) has lead to the development of molecular strategies for the inhibition of HIV replication (Malim et al., 1989, Trono et al., 1989, Sczckiel et al., 1991, Sullenger et al., 1990).

Molecular systems for in vivo cell specific therapy have been described whereby a gene encoding a toxic product can be controlled in its expression by regulatory regions of genes active only in particular cells.

Initial studies on cell-specific ablation therapy have utilised cytotoxic agents such as diphtheria toxin A or ricin A chain genes under the control of lens (Breitman et al., 1987; Landel et al., 1988) or pituitary (Behringer et al., 1988) specific promoters. After microinjection into mouse embryos and the production of transgenic animals, these constructs resulted in the destruction of either lens or pituitary cells. However, when associated with leaky promoter elements, these toxin genes are unsuitable for somatic therapy because of the constitutive cell lethality dnd the extreme sensitivity of mammalian cells to diphtheria and ricin toxins.

W11 Oc/n8ic OPr'lI-/G /n2 9 A more versatile toxin-encoding gene for potential. use in human ablative therapy has been described (Borelli et al., 1988). The Herpes Simplex Virus type 1 thymidine kinase (tk) gene product is a conditional cell lethal and has been shown to be toxic to mammalian cells only in the presence of nucleoside analogues such as acyclovir (ACV) or gancyclovir (GCV). These analogues kill actively cycling cells because they possess high affinity for the tk gene product with little or no affinity for endogenous mammalian tk. Model systems have demonstrated in vivo lymphocyte specific lethality by anti-herpetic drug treatment of tk transgenic mice (Borelli et al., 1988, Heyman et al., 1989).

Specificity ot conditional toxicity is due to lymphoid specific transcriptional control elements and quantitative flexibility is inherent within the levels of tk transgene expression and/or administered drug dose. Upon withdrawal of the drug in these studies, mature lymphocytes are restored to normal numbers. Thus, the in vivo ablative system is regenerative, reversible and does not affect stem cells.

Even advanced ablative systems, however, have their disadvantages in antiviral therapy. In particular, the rationale of the system is flawed in that it relies on the destruction of viral2y infected cells. Although this prevents viral replication, the pathogenic effect of the virus, the destruction of T-lymphocytes in the case of HIV, is actually promoted. Therefore, ablative systems are unlikely to be app-icable to cases of established infection and must rely on reaching substantially all cells infected by the virus.

Another potential system for use in anti-HIV therapy involves the expression in cells susceptible to HIV infection of a decoy gene.

Decoy genes encode proteins which act as antagonists to natural proteins involved in the replication of the HIV I II wn o5/0s8635 PrT/nd94/092 3 virus. For example, a decoy gene may encode a detective mutant of a transactivator protein which is capable of binding to the transactivator-responsive site ol. he host or viral genome, yet is incapable of activating transcription.

Transdominant mutations have been reported in a number of viral transactivators which abolish or attenuate the ability of the wild-type protein to transactivate the target gene.

Examples include transdominant mutations of E1A (Glen et al., 1987), tax (Wachsman et al., 1987) and VM65 (Friedman et al., 1988). Similar mutations in HIV genes have been described for the Tat transactivator (Pearson et al., 1990) and the Rev transactivator (Bevac et al, 1992; Malim et al., 1992).

Expression of such mutant proteins in a HIV-infected cell line leads to competition with the natural transactivator and resultant loss of transactivating activity. See, for example, International patent application WO 9014427 (Sandoz). A potential disadvantage of the use of decoy gene approaches is that when a decoy is expressed in the absence of the infecting virus a negative biological effect may be exerted on the host. For example, a host immune response may result from the production of the decoy gene product, leading to destruction of the host cell by, for example, cytotoxic T-lymphocytes (CTL). Furthermore, it must be borne in mind that decoy proteins are derived from biologically active gene products of pathogenic organisms and may therefore exert a deleterious effect on the host.

For example, certain allelic variants of the HIV nef gene product have been shown to downregulate CD4 expression on thymocytes and to reduce the numbers of CD4 thymocytes in transgenic mice (see our copending U.K. Patent Application No. 9305759.4 and Guy et al., 1990).

In order to avoid these disadvantages it has been suggested that transcription and expression of decoy gene products should be restricted to cells actually infected by HIV, for I- -d _P

I~~

WO/N (O8/nrI PCT/GB94/02092 4 example by using a transactivatable expression system for decoy expression which is transactivated by an HIV gene product (see WO 9011359).

However, because the decoy gene product is only expressed in cells after HIV infection, a considerable excess of decoy gene product is required in order to successfully arrest viral replication, since the virus has an effective head start. The production of large amounts of decoy in infected cells is likely to give rise to the aforementioned negative biological effects against such cells, leading zo death or incapacitation of infected cells and the concomitant disadvantages of ablative systems discussed above.

An alternative approach, which has not been proposed in the prior art, would be to ensure constitutive expression of decoy proteins which do not give rise to a negative biological effect in cells susceptible to HIV infection.

Locus control regions (LCRs) are elements which confer position-independent, copy number-dependent expression of genes in gene transfer approaches. They have also been shown to permit high levels of expression of cloned genes and to possess tissue-specific properties. First discovered in globin genes (Grosveld et al, 1987) these elements are believed +t direct the creation of independent regulatory domains within the chromatin structure of cell genomes, thereby ensuring the activity of a co-transferred gene.

A number of LCRs other than those for globin genes have been described, for example in the CD2 gene in T-lymphocytes (Greaves et al., 1989) arid the lysozyme gene in macrophages (Bonifer et al., 1990) and B-cells (see European patent application 460042).

The targets of HIV infection are primarily CD4 Tlymphocytes, but also include macrophages and, dendritic cells which are related to macrophages and of importance in -I I~-PC ~Is initiating an inunune response (reviewed in McCune, 1991). These cells share very few common features except for being derived from common haematopoietic stem cells and susceptibility of HIV infection.

Haematopoietic stem cells are not infected by HIV (Molina et al., 1990; David et al. 1991).

We have now determined that by inserting a transcription unit encoding a decoy gene under the control ot the CD2 LCR into stem cells, constitutive expression of the decoy may be achieved in T-lymphocytes in transgenic mice and passed through the germ line, without disadvantageous effects on the host, by selection of decoy genes having low deleterious properties.

Throughout this specification, unless the context requires otherwise, the word "comprise", or variations such as "comprises" or "comprising", will be understood to imply the inclusion of a stated element, integer or step, or 15 group of elements, integers or steps, but not the exclusion of any other element, integer or step, or group of elements, integers or steps.

Disclosure of the Invention According to a first aspect of the invention, therefore, there is provided a recombinant nucleic acid vector for the delivery of nucleic acid to a host 20 organism comprising a transcription unit encoding a transdominant negative mutant of a viral gene product which has been selected substantially to avoid a negative biological effect under the control of a DNA sequence active in cells normally infected by a virus which is effective to confer constitutive tissue-specific, integration site independent, copy-number dependent 25 expression of the transcription unit.

By "substantially avoid a negative biological effect" it is intended to denote that the decoy used in the present invention has been selected or specifically modified to give rise to a negligible adverse effect on host cells, which may safely be disregarded in therapeutic situations, or, preferably, no adverse effect at all. The negative biological effect may be a biological impairment of cell function or the raising of a CTL response, as set out above, or both.

By "biological impairment of cell function" it is intended to denote biological effects on host cells, such as

-I

wn ()/0835 PCT/GB94/02092 6 downregulation of CD4, which may have a negative effect on the patient. In some cases the host cells may be affected by the decoy in a manner similar to the pathologic activity of the virus. In other cases, the decoy proteins may have effects not normally associated with viral infection but which are undesirable when associated with a constitutively expressed foreign protein.

For example,where the virus is HIV, the decoy is selected to avoid, inter alia, an impairment of immune function in the host.

Impairment of immune function has been demonstrated in vitro for certain allelic variants of nef (Guy et al., 1990).

These results are reinforced in vivo in our copending U.K.

Patent Application No. 9305759.4, which shows that nef expression may play a role in CD4 downregulation and in decreasing the numbers of CD4+ T-cells in transgenic mice.

CD4 downregulation and loss of CD4+ T-cells is one of the pathogenic features associated with HIV infection and AIDS.

CTL response to SIV proteins has been observed in SIVinfected macaques (Venet et al., 1992) and in human retroviral infection (Kannagi et al., 1983; Mitsuya et al., 1983; Autran et al., 1991; Nixon and McMichael, 1991). CTL responses to Nef antigens and Rev antigens are strong. CTL responses to Tat antigens are, however, rare and thought to be very weak (Lamhamedi-Cherradi et al., 1992).

We have shown that the HIV tat gene product does not impair cell function in transgenic mice. The tat gene product, therefore, appears to exert little or no impairment of cell function, while at the same time is of very low CTL-inducing activity. Preferably, therefore, the invention comprises the constitutive expression of a Tat decoy.

The invention further provides the use of other natural decoy gene products which possess the desired characteristics displayed by tat, namely the absence of

'I

substantial negative biological effects.

Alternatively, the invention provides for the use of a decoy gene product which has been specifically mutated to reduce the incidence and strength of negative biological responses thereto. This may be achieved, for example, by mutation or deletion of certain domains of a decoy gene product. For example, the cell-impairing effects of a decoy gene product n,-y be reduced or eliminated by the introduction of point mutations in the gene (see Guy et al., 1990).

For example, we have shown that, in transgenic mice, expression of the Tat gene product under the control of the CD2 LCR gives rise to a three-fold increase in the levels of mRNA encoding certain cycokines, namely TGF-3, IL4 receptor and TNF-3.

In contrast, when a mutated Tat gene product is used comprising a point mutation which abolishes its effector function, cytokine mRNA levels are not affected.

advantageously, therefore, a mutated Tat gene product is used in the present invention.

CTL response to a protein may be modified, either by the introduction of mutations at certain residues involved in binding to the presenting HLA molecules or interacting with the T-cell receptors (see choppin et al., 1992; 1991a, b; Gotch et al., 1988 Furthermore, it is possible to modify a protein to reduce its rate of degradation by the cell and thereby lower the incidence of presentation of antigens derived from the protein (McMichael et al., 1977; bachmair et al., 1986; Townsend et al., 1988; Morrison et al., 1992).

It has been shown that HIV naturally mutates to avoid CTL responses in vivo and that the sites of amino acid variation tend to be conserved, at least to a certain extent, in different patients (Phillips et al., 1991). Preferably, therefore, the decoy of the invention may be mutated in AMENDED

SHEET

WO 9-/08635 PCTIGB9410m092 8 accordance with naturally-derived HIV isolates which display a reduced CTL response.

However, it should be pointed out that CTL responses will vary between individuals due to variation in the antigenpresenting molecules present. Therefore, although some general mutations may be carried out to reduce CTL response caused by common HLA types, it remains possible that certain individuals may show a CTL response even to decoys which are believed to be of low CTL-inducing activity. In this case, the invention provides means to mutate the decoy on an individual basis in order to reduce or eliminate the CTL response in that individual.

By "transdominant negative mutant" it is intended to refer to a gene product which is rendered functionally transdominant over its viral analogue and is effective to block the activity of the viral analogue. Therefore, the term is to be interpreted functionally, and comprises mutants in the normal sense of the term, having an altered amino acid sequence, as well as mutants which are alternatively processed or spliced, and mutants which differ from the wild-.type protein in patterns of expression. For example, the Nef gene product of HIV is known to be a transdominant inhibitor when expressed in excess.

Therefore, an overproduced Nef protein is included in the term "transdominant negative mutant".

Constitutive expression confers a particular advantage of the invention, that is that the presence of the decoy in healthy cells effectively prevents the infecting virus from becoming established. If the decoy gene is only activated after infection by the virus, there is the possibility that the virus may become established before the decoy is able to exert any significant anti-viral effect The DNA sequence controlling the transcription unit of the vector of the invention is preferably a Locus Control Region a WO 95/08635 PCT/GB94/02092 9 (LCR). A number of LCRs have been described in the art and the selection of an appropriate LCR is within the capabilities of a person skilled in the art. In the case of the treatment of HIV infections, however, the use of the CD2 and the macrophage-specific lysozyme LCR is preferred. Both T-cells, in which the CD2 LCR is active, and macrophages are targets for HIV infection.

In addition to the LCR, the vector of the invention is equipped with a promoter which is constitutively active in the target tissue type. For example, if the cells to be targeted are T-cells, the CD2 promoter may be used. The promoter, however, may be active in cells other than the target tissue. In such a case, high-level expression in non-target cells is unlikely, because the LCR is inactive in these cells. Even if a certain amount of non-specific expression cells does occur, such expression will not be harmful as the gene product is selected to avoid negative biological effects. In any event, non-specific expression can be minimised by the use of efficient vector targeting techniques to deliver the vector of the invention.

The nucleic acid vector may be any vector capable of delivering nucleic acid to a cell. For example, the vector may be a plasmid, a virus or a linear DNA fragment. The vector may be naked, complexed with proteins or packaged in a delivery system such as a liposome, virosome, or receptor mediated complex.

The vector of the invention is preferably for use in the transfection of stem cells. Therefrom stems a further advantage of the invention, that is that the decoy is expressed in all cells of a particular lineage.

When the vector encodes an HIV decoy, the stem cells may be hematopoietic stem cells.

Alternatively, T-cells may be targeted directly. The targeting of T-cells is desirable, for example, in the case wn 95r)83 PrT/Grn/(?02 where HIV infection is already established but the virus has not yet spread to the peripheral T-cell population. In this instance, such cells may be affe-cively protected from viral infection.

A number of protocols for the transfection of stem cells and T-cells are known in the art. Some involve the isolation of stem cells from total cell populations, as described in, for example, European patent applications 0 455 482 and 0 451 611.

An improved process for che transfection of stem cells and T-cells is described in our copending U.K. Patent Application No. 9317380.5, the disclosure of which is incorporated herein by reference.

The host organism may be a mammal, insect, fish, plant or any other organism which it is desired to protect from viral disease. Preferably, the host organism is man.

Where the decoy is a Tat decoy, the decoy may be prepared following any of the protocols known in the art. For example, the method of Pearson et al. (1990) may be used to generate deletion mutants of Tat which lack the transactivating function but retain the ability to bind to the tat region. Such deletion mutants may be tested for decoy activity as described in Pearson et al. or according to the methods set forth in our copending U.K. Patent Applic'tion No. 9305759.4 as well as International Patent Application W090/14427.

The potential toxicity of any such mutants may be tested by the methods described hereinbelow. Should such mutants prove to give rise to a CTL response in a patient, they may be further mutated to reduce this response, in accordance methods known in the art.

I WO 95/08635 PCT/GB94/02092 11 The decoy gene may be derived from any virus which gives rise to infection in man or other organisms, including plants. Especially preferred, however, are HIV decoys such as Tat, Rev or Nef decoys.

The decoy may be derived from the same virus as it is intended to combat with the vector of the invention.

However, it is envisaged that decoys derived from viruses other than one it is intended to treat may be used. For example, it has been noted that an HTLV1 Rex decoy is active in suppressing HIV1 Rev function (Bohnlein et al., 1991).

7urthermore, it is envisaged that entirely artificial decoy genes encoding specialised decoy proteins may be designed.

For example, an artificial decoy gene may be designed which encodes the tar-binding domain only of the HIV Tat transactivator, or an analogue of the tar-binding domain which effectively competes for tar binding with wild type Tat.

The vector of the invention is preferably for use in the transfection of a patient's cells in vivo or ex vivo, for the treatment of a viral disease. According to a second aspect of the. invention, therefore, there is provided a vector according to the first aspect of the invention for use in therapy.

By "therapy", it is intended to denote both the prevention and the attenuation or elimination of viral infection. As set out hereinbefore, it is preferred that the vectors of the invention be used for the prophylaxis of viral infections because it is believed that it may be important to avoid establishment of the viral infection in the host.

However, especially in the early stages of a viral infection, it is envisaged that the vectors of the invention may have a conventional therapeutic application effective to attenuate and eventually eliminate the viral infection.

Preferably, the vector of the invention is used for the P. _-L WO 95/086i35 PCT/GB94/02092 12 treatment of stem cells or T-cells ex vivo. Accordingly, in a third aspect of the present invention there is providd a vector according to the first aspect of the invention for use in the treatment of stem cells or T-cells ex vivo.

Stem cells or T-cells may be isolated according to procedures described in the prior art, as set out hereinbefore. Alternatively, as is preferred, stem cells or T-cells may be targeted using an efficient targeted transfection technique, such as that described in our copending U.K. Patent Application No. 9317380.5. Using such a technique, it is possible to transfect stem cells or Tcells in whole blood obtained from patients with extremely high efficiency.

According to a further aspect of the invention, there is provided a method for treating or preventing a viral infection comprising the steps of: a) removing a cell from the body of a patient; b) transfecting the cell with a vector according to the first aspect of the invention; and c) returning the cell to the body of the patient.

Preferably, the cell is a stem cell. For example, the cell is a haematopoietic stem cell. Alternatively, the cell may be a T-cell.

Haematopoietic stem cells and T-cells are easily removed from the body of a patient, for example from cord blood, peripheral blood or bone marrow aspirate.

Transfection of stem cells may be accomplished by any of the protocols cited hereinbefore.

The transfected stem cells, once returned to the body of the I -B *WO 95/08635 PCT/GB94/02092 patient, will divide in the usual manner and populate the patient with cell lineages carrying the heterologous gene comprised in the vector of the invention. The cell lineages thus derived will possess the antiviral capabilities conferred by the heterologous gene.

According to a still further aspect of the invention, there is provided the use of a vector according to the invention in the manufacture of a composition for use in the treatment or prophylaxis of a viral disease.

Preferably, the composition comprises the vector of the invention in a suitable buffer for use in the transfection of cells either in vivo or ex vivo. When used in vivo, the buffer will c: sist essentially of pharmaceutically acceptable excipients, diluents or carriers. For use ex vivo, the nature of the buffer will be determined by the transfection protocol being employed. For example, if The method described in our copending U.K. Patent Application No. 9317380.5 is to be used, the buffer as described therein is used.

In a still further aspect of the invention, there is provided a cell comprising a transcription unit encoded by the vector of the invention. Preferably, the cell is a stem cell and advantageously it is a haematopoietic stem cell.

Alternatively, the cell may be a T-cell.

The invention further provides a method for the treatment or prevention of a viral infection comprising administering to a patient a pharmaceutically effective amount of a composition comprising the vector of the invention in admixture with a pharmaceutically acceptable excipient, diluent or carrier.

The invention will now be described for the purpose of illustration only in the following examples, with reference to the Figures, in which: I- OE/oI035 PCTIGB94/02092 S4 .juJ-3.. 1 .4 Figure 1 is a diagrammatic representation of the structure of the CD2-Tat transgene; Figure 2 shows the identification of the Tat DNA in transgenic mice carrying the CD2-Tat transgene.; Figures 3 A and B show the identification of Tat RNA in transgenic mice carrying the CD2-Tat transgene; Figure 4 shows a FACS analysis of thymus tissue from transgenic and non-transgenic mice; Figure 5 shows a FACS analysis of spleen ana lymph node tissues from transgenic and non-transgenic mice; Figure 6 shows the impact of the presence of tne Tat transgene on cytokine gene expression in transgenic mice; Figure 7 is a slot blot showing the generation of transgenic mice carrying a mutated Tat transgene in which Tyr 47 has been mutated to Ala; and Figure 8 is d slot blot which demonstrates that mutant Tat has no effect on the expression of the TNF-3 gene.

METHODS

CD2-Tat mice A DNA fragment comprising the Tat coding sequence (see Figure 1) was ligated into a unique EcoRl site in the first exon of the CD2 gene in the p2629 CD2 expression plasmid, which was obtained from Dr. D. Kioussis, NIMR, Mill Hill, Great Britain. A 4.5 kb fragment containing the CD2 LCR was isolated from p2694 (also obtained from Dr. Kioussis) and ligated into the unique Bam H1 Not 1 sites of p 2629.

The 12 kb Sal 1 Not 1 fragment comprising the CD2-Tat construct was then excised and microinjected into single-

I

t" cell mouse embryos as previously described (Grosveld et al., 1987). Positive founder animals were bred with CBA x C57 mice and lines maintained as heterozygotes.

DNA~ an4 Expre'sion Analysis Tail DNA (10gg) from founder animals was analysed by Southern blot anialysis after digestion with ijindIII or Asp718- DNA was run on a It agarose/Tris-;5cetnte, EDTA gel, lo blotted onto nitrocellulose and probed with a randomly primed BamHI-Sma2. Tat fragment. A 1.2 Kb Thy-l.2 fragment was used as a loading control probe.

Appropriate amounts of pCD2Tat spiked in 10 pAg genomic DNA were used as a copy number controls. Quantitation was performed on the Molecular Dynamics Phosphorlmager.

RNIA was prepared using the lithium chloride/urea method (Fraser et al., 1990). For Northern blot analysis (Sambrook et al., 1989) l0pg of RNA was run on a it formaldehyde gel, blotted onto nitrocell.ulose and probed with a 800 bp 8>amlI- SinaI neff fragment from pTG1147. For RNA slot blots (Sambrook et al., 1989) 5gg of RNA was blotted onto nitrocellulose and probed as above. RNA f rom the Nei' producing CRI? L producer cell line (Schwartz et al., 1992) was used as a positive control.

Example 2.

Expression off CD2-Tat in Transclenic Mice Exon I (encoding aa 1-72) of the HIV-l TAT gene was inserted downstream of the transcriptional start site in the first axon of the human CD2 gene (Figures I and A stop codon was constructed in the sequence of human CD2 exon 2 s5o as to eliminate the production of CD2 protein. The human CD2 LCP.

element was ligated to the 3' end of the construct. A Sall- SNoti fragment was injected into fertilized mouse eggs. At AMrNDEO SHEET least three transgenic lines .,ere created. Line C (2 on figure 3A) containas 70 copies and line E (4 on figure 3A) contains 40 copieG.

Si nucl.ease RNA protection vas performed on various tissues from a transgenic and a non-transgenic mouse using a TAT exon 1 probe. As shown in figure 3B only thymus expressed TAT highly. Spleen expressed Tat only to low levels. No expression was observed in the 3cidney or liver of: the transgenic mouse or in any of the tissues of the control non-transgen ic In order to determine whether the CD4 and CDO T cells subsets are affected by the overexpression of HINV-TAT, antibody staining and FACS analysis was performc:I on thymocytes, spleen and lymph node cells from CD2-TAT transgenic mice (Figures 4 and Single cell suspensions were prepared from the tissues of line C and line E transgenic mice (samples 3 and 4 respectively) and their non-transgenic littermates (samples 1 and PE labeled C08 and FIT lab~eled CD4 antibodies were incubated with the cells and FACS analysis performed. As shown in the contour plots, no changes in the percentage of double negative, double positive or single positive subsets were found in the thymus of transgenic mice. Furthermore, no changes in the percentages of CD4 or CD8 single positive subsets were found in spleen or lymph nodes of the transgenic mice when compared to non-transgenics. Thus, high level expression of HIV-TAT docs not affect subset distribution in vivco in the lymphoid organs.

TAT induced transcriptional upregulation of TNT-O leads to overproduction of functional T"~-ft as measured by Cytotoxicity.

Northern blot analysis of RNA from TAT transgenic lines C and E derinstrated an increase of 2.3 fold in TLNfl transcription (Figuris 6A). In order to test whether this VME.'JDED i== Is, I 1. L. I IL. 17 resulted in incr-eased TNF-# protein produaction, we perfoarred cytotoxicity assays with cell lysates of T cells from TAT tran5s4enic mice (C4-1, C+2, E+1 and 3+2) and ron-transgenic littermates and Active equivalents of TNF-0 protein in each sample was quantitated against a known TNF-0 protein standard (in units). As shown in Figure 6S, all of ifour transgenic mice produced siognif icantly higher levels of TNF-0 (2-4 fold) as compared to the non-transgenic controls.

Cytokine gene expression is affected by the pressure o~f HIV-

TAT.

Northern blot analysis was performed on RNA from CD2-TAT transgenic nice to test for quantitative differences in cytokine gene expression (Figure 6A). Total mRNA was prepared from thymocytes of line C transgenic -mice (C4-1 and C+2) and a ron-transgenic littermate and from thyinocytes of line E transgenic mice (E4-l and E+2) and a non-transgenic littermate 10 Ag of RNN was loaded per lane on a formaldehyde agarose gel. RNA was transferred onto a filter and hybridized with a O3-actin probe as an RNA quantitation control and a TAT probe for verification of transgene expression. The filter was rehybridized several times with probes tor cytoine genes TGF-0, IL-4R, TNF-3 and TNF-a. Autoradiograns of the Northern blot demonstrate an increase in expression of TGF-3, IL-4R and TN1F-f3 gene expression in the TAT transgenic mice. However, hybridization signal with the TNF-a probe suggests no change or a decrease in TWF-a gene expression in the Tat positive mice.

The results of this Northern blot were quantitarted on a Phosphorimager and fold increases or decreases were calculated. Ks shown in Table 1, when signal was normalized against the j-actin quantitation control, TGF-O, IL-4R and TGF-0 steady state riRNA was increased in the transgenic mice,, TGF-O levels increased on average 2.8 fold, IL-4R Slevels increased 3.5 fold and TNF-g Levels increased 2.3 AMENDED SHEET f old. TNF-a levels decrease by about 25%. Thus, the expression of TAT in thymooytes has an effect on cytokine gene expression.

L~,

guantitation of Cytokine RNAS in CtD2-TAT Transgenic Mice Transgenio line. Line C Line E mouse 1 2 1 '2 TGF-#3 2.20 3.26 2.74 2.88 IL-4R 3.40 2.76 4.03 2.76 TNF-e3 2.29 2.32 1.20 2.22 TNF-a 0.81 0.67 0.74 0.85 Fold RNA change as compared to non-transgenic littermates.

jXAMipIe 2 Expression of CD2-TAT (47ala) in transgenic mice.

A 12kb Sall-Notl fragment containing the CD2 promoter and LCR element and exon 1 (encoding aa 1-72) of a mutant form of the HIV'-1 TAT gene in which amino acid 47 had been converted from a tyrosine into an alanine, (47 Tyr Ala), was injected into fertilized mouse eggs. As shown in figure 7, three transgenic founders were created (Lines A6, A7 and A8) in comparison with transgene copy number controls from 0 to 50 (Lane these founders contained between 8 and copies of the transgene.

in order to determine whether thymocyte T cell subsets are affected by the expression of the mutant form of the H~IV-TAT (47ala), antibody staining and FACS analysis was performed on thymocytes from CD2-TAT (47ala) transgenic mice. Single i E',D~r SHEET cell suspensions were prepared from mouse A6 and a nontransgenic animal, A4. PE-labelled COB and FITC -labelled CD4 were incubated with the calls and FACS analysis was performed. As shown in Table 2, no changes were found in the total number of thymocytes derived from either transgeniC or non-transgenic mice. Furthermore, no difference was observed in the relative percentages of double negative (DN) double positive (DP) or single positive (SP) C04 or CDB cells in the thyinus from the transgenic compared with the non-transgenic. mouse.

Table 2 Thymic T cell Subsets in CD2-TAT (47ala) Transgenia Mice Total DN OP SP SP T-cells (CD4-CDB-) (CD4-/CDB-) (CD4-) (CDB+) X101 Non-Transgenic 2.5 4.1 80.7 11.5 3.7 Transgenic 2.2 7.4 75.9 12.6 4.2 Cytokine gene expression (Tlq-3) is not affected by the presence of the mutant HIV-TAT (47ala) RNA slot blot analysis was performed on R.NA from CD2-TAT' (47ala) transgenic niice to test for quantitatiLve differences in cytokine gene expression (Fig-ure 8) Total RNA was prepared from the thymocytes of CD2-TAT (47ala) transgenic mice A.6 and A.7, two non transgenic controls A.4 and and from two transgenic mice, ona fromn line C(c.1; and one from line ECE.l) harbouring the wild type HIV-TAT.

Duplicated l0gg RNA samples were denatured and loaded onto the filter and hybridized with a j3-actin prob. as an RNA quantitation control, and then with a probe specific for the AMENDED

SHSST

I cy'tokine -INF-j8. Autoradiographs of the 1R}R blots demonstrate that while an increase in expression of TNF-0 is seen in transgenic nice containing the wild type HIV-TAT, no increase in expression of TNF-,6 is observed in nice containing the mutant HIV-TAT (47ala).

The results of this RNA slot blot were quantitated on a phosphorlinager and the told changes in cytokine gene expression determined. As shown in Table 3, when the signals are normalized against the internal guantitation control actin, although TNF-j3 steady state mRNA was elevated in lines C and E, there was no increase in expression of this cytokine in the nutant IIIV-TAT (47ala) transgeuiic mice.

Thus, the expression of the mutant HIV-TAT (47ala) has no effect on TNF-O cytokine expression.

TABLt 3 -Quantitation of cytokine (TNP'-j) RNA in HIV-TP.T (47ala) transgenic mice Transgenic mouse A.6 A.7 C.1 E.1 TN-t0.97 0.89 1.9 2.4 Fold R~NA change as compared with non-transgenic mice.

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Claims

1. A recombinant nucleic acid vector for the delivery of nucleic acid to a host organism comprising a transcription unit encoding a transdominant negative mutant of a viral gene product which has been selected to avoid a negative biological effect in the host under the control of a DNA sequence active in cells normally infected by a virus which is effective to confer constitutive tissue-specific, integration site-independent, copy-number dependent expression of the transcription unit.

2. A recombinant nucleic acid vector according to claim 1 encoding a virrl gene product which has been selected to avoid a CTL response in the host.

3. A recombinant nucleic acid vector according to claim 1 or claim 2 encoding a viral gene product which has been selected to avoid immune impairment in the host. 15 4. A recombinant nucleic acid vector according to any one of the preceding claims wherein the DNA sequence controlling the transcription unit comprises a Locus Control Region (LCR).

5. A recombinant nucleic acid vector according to any one of the preceding claims wherein the DNA sequence controlling the transcription 20 unit comprises a constitutively active promoter.

6. A recombinant nucleic acid vector according to any one of the preceding claims which is specific for a target cell.

7. A recombinant nucleic acid vector according to claim 6 wherein the target cell is a haematopoietic stem cell.

8. A recombinant nucleic acid vector according to claim 6 wherein the target cell is a T-cell.

9. A recombinant nucleic acid vector according to claim 6 wherein the target cell is a rnacrophage. A recombinant nucleic acid vector according to any one of the preceding claims wherein the transcription unit encodes a transdominant negative mutant of an HIV gene product.

11. A recombinant nucleic acid vector according to claim 8 wherein the transcription unit encodes a transdominant negative mutant of the HIV Tat gene product.

12. A recombinant nucleic acid vector according to any one of the preceding claims wherein the transcription unit encodes a transdominant negative mutant which is further mutated to reduce any negative biological effect.

13. A recombinant nucleic acid vector according to claim 12 wherein the transcription unit encodes a transdominant negative mutant which has been modified to reduce or eliminate effects on cytokine gene expression.

14. A method for the treatment of a viral disease in a patient, comprising administering to said patient an effective amount of a nucleic acid vector according to any one of the preceding claims. A method for the treatment or prophylaxis of a stem cell, a T-cell or a macrophage in vivo in a patient, comprising adminisiering to said patient an effective amount of a nucleic acid vector according to any one of the preceding claims.

16. A method for the treatment of prophylaxis of a stem cell, a T-cell or a macrophage ex vivo in a patient, comprising administering to said patient anl effective amount of nucleic acid vector according to any one of the preceding clainms.

017. A method for treating or preventing a viral infection comprising the V steps of: removing a cell from the body of a patient; 20 transfecting the cell with a vector according to any one of claims 1 to 8; and returning the cell to the body of the patient. *8 A methc r treating or preventing a viral infection comprising administering to a patient a pharmaceutically effective dose of a composition 25 comprising the vector of any one of claims 1 to 13 in admixture with a pharmaceutically acceptable excipient, diluent or carrier.

19. The use of a vector according to any one of claims 1 to 13 in the manufacture of a composition for use in the treatment or prophylaxis of a viral disease.

20. A cell comprising the transcription unit encoded by the vector of any one of claims I to '13.

21. A cell according to claim 20 which is a stem cell.

22. A cell according to claim 20 which is a T-cell.

23. A cell according to claim 20 which is a macrophage. Dated this 6th day of August 1998 THiEREXSYS LIMITED AND MIEDICAL RESEARCH COUNCIL Patent Attorneys for the Applicant: F B RICE CO