Patent Description:
Adenoviruses are an attractive and versatile tool in biotechnology, having well understood genetics and the ability to grow to high yields in tissue culture. The replication cycle of Adenoviruses is highly complex, involving both early and late phases. The transition from early to late is considered to occur following DNA replication and the activation of the Major Late promoter (MLP) in the virus genome. The MLP drives the expression of all virus late transcripts, and can convert up to <NUM>% of the cells' protein into virus structural proteins. Modification to the MLP in situ to provide inducible expression has not previously been demonstrated, primarily because the virus DNA polymerase coding sequence is in the opposing DNA strand.

Whilst adenoviruses are useful laboratory tools for a number of applications, the fact they are so productive represents a major problem if they are used in a manufacturing work flow, namely they generate substantial amounts of virus particles that must be removed during downstream processing. For example, when adenovirus has previously been used for protein expression purposes, or the production of other virus-like particles, or the large scale manufacture of Adeno-associated virus (AAV), the presence of intact Adenoviral particles at the end of the production process is highly undesirable.

The ability to manufacture proteins in mammalian cells is increasingly attractive, with many high value recombinant proteins now being produced in these systems, affording optimum protein processing, folding and glycosylation. This is frequently achieved using transient transfection of a plasmid encoding the required transgene under the control of a strong promoter, such as the Cytomegalovirus (CMV) immediate early promoter. However, compared to some viral systems in other organisms (such as Baculovirus in insect cells), this process is relatively inefficient, often demonstrating variable protein yields that rarely exceed <NUM>% of the total cell protein mass.

The extensive characterisation of the Adenovirus genome, coupled with the wealth of knowledge regarding its gene expression and life cycle, makes this virus an ideal candidate platform on which to significantly improve recombinant protein yields. One major benefit is demonstrated by the virus' ability to actively hijack the mammalian cell's machinery, and to inhibit the production of cellular proteins.

However, in addition to inhibiting the production of cellular proteins, considerable cellular resources are used by the virus to produce viral structural proteins. The quantity of capsid proteins produced, for example, is vast and has been calculated to be up to <NUM>% of total cell protein, and removing these proteins and the assembled virus particles after production is challenging.

Similar to recombinant proteins, the demand for adeno-associated virus particles is increasing significantly, owing to recent clinal successes in the treatment of retinal disorders and haemophilia. Traditionally, the production of AAV has been achieved through two different routes. Initially, AAV was generated using wild-type (WT) Adenovirus serotype <NUM> whilst transfecting cells with plasmids encoding the Rep and Cap genes and the AAV genome. This allowed the WT adenovirus to provide a number of factors in trans that facilitated virus replication. However, there a number of limitations to this approach: for example, each batch of AAV must be separated from the Ad5 particles to provide a pure product and ensuring that all Ad5 has been removed is challenging. Moreover, the fact that during production the cell is devoting huge resource to the production of Adenoviral particles rather than AAV is also undesirable.

More recently, the adenovirus-based systems have been replaced with plasmids encoding the sections of the Adenovirus genome required for AAV production. Whilst this has solved some of the concerns over Adenovirus particles being present in the final virus preparation, a number of issues remain. These include the requirement to pre-manufacture sufficient plasmid for transfection into the production cell line and the inherently inefficient process of transfection itself. The yields from these systems are also lower than those using Ad5 based approaches. The inventors have now discovered that transcription of the late adenoviral genes can be regulated (e.g. inhibited) by the insertion of a repressor element into the Major Late Promoter. By "switching off" expression of the Late genes, the cell's protein-manufacturing capabilities can be diverted toward the production of a desired recombinant protein. Importantly, the strategic silencing of the Major Late promoter in the adenovirus genome in accordance with the current invention allows the virus to still replicate its DNA in the cell, providing thousands of DNA copies of the virus genome that can be transcribed for a range of applications.

This invention provides a range of advantages. For example, it can be used to direct a cell's protein production capability towards the production of specific recombinant proteins at increased yields compared to comparable systems wherein the viral Late genes are still expressed. Furthermore, the ability to "switch off' the production of viral structural proteins means that no or essentially no viral particles are produced during the protein-production process. Consequently, economic savings can be made due to a reduction in the need to remove virus particles from the purified protein.

The invention also has the advantage of providing a simple, cost-effective, way to manufacture AAV particles where the Rep and Cap proteins of AAV can be encoded within the Adenovirus to provide the high expression levels which are required to make the AAV particles by maintaining the replication of the Adenoviral genome, but also preventing the production Adenovirus particles in the final AAV preparation.

Some modifications of the MPL have previously been reported. These include making a copy of the MLP and placing it either in other plasmids for expression level analysis (El-Mogy, <NUM>) or within the E1 region of the Adenovirus genome subject to the insertion of sites to regulate its expression (Molin, <NUM>). Other work has included the mutation of the MLP TATA box for both basic research (Concino et al. , <NUM>; Concino et al. , <NUM>) and in order to allow the virus to be selectively grown only in cells which have a trans-complementing factor in a cell. Importantly, the latter approach provides for a system where the activity of the major late promoter is entirely dependent on a complementing protein factor being present in a cell, and therefore in a cell where this factor is absent the MLP is not active. The invention, however, provides the converse of this, where the MLP maintains it full expression activity level in cells where a repressor not bound, providing high level virus replication with minimal disturbance to the virus life cycle.

The virus of the invention described herein is therefore fully active when not repressed but is capable of being repressed, depending on the presence or absence of a repressor. A repressor binding site has not previously successfully been inserted into the MLP in situ for the regulation of its expression in an adenovirus genome. The current inventors have further improved this system to place the repressor protein coding sequence under the control of the Major Late Promoter itself. In this approach, the Major Late Promoter self-represses itself because when the Major Late Promoter tries to transcribe the structural proteins of the virus, it will also transcribe a repressor capable of repressing its own activity, thereby allowing for a negative feedback loop that prevents MLP activity and providing tight regulation of MLP expression.

It is therefore an object of the invention to provide an adenoviral vector system which provides increased yields of recombinant proteins, and can be used to provide non-adenovirus virus and virus-like particles.

It is also an object of the invention to provide a process of producing a transgene product in isolated adenovirus-infected mammalian cells, which reduces the need to remove virus particles from the purified product which may be a protein, non-adenovirus particle or virus-like particle.

In one embodiment, the invention provides an adenoviral vector comprising a repressible Major Late Promoter (MLP) and a plurality of adenoviral late genes, wherein the MLP comprises one or more repressor elements which are capable of regulating or controlling transcription of the adenoviral late genes, wherein the one or more repressor elements are inserted between the MLP TATA box and the +<NUM> position of transcription, wherein the one or more repressor elements are ones which are capable of being bound by a repressor protein and wherein the repressor protein is the tetracycline repressor, the lactose repressor, the ecdysone repressor, rat glucocorticoid receptor or human estrogen receptor.

In another embodiment, the invention provides an adenoviral vector as claimed in claim <NUM>, additionally comprising: (a) a plurality of adenoviral early genes and (b) a transgene.

Preferably, a gene encoding a repressor protein which is capable of binding to the repressor element is encoded within the adenoviral genome.

Preferably, the transgene comprises a Tripartite Leader (TPL) in its <NUM>'-UTR.

Preferably, the presence of the repressor element does not affect production of the adenoviral E2B protein.

Preferably, the repressor protein is transcribed from the MLP.

The one or more repressor elements are inserted between the MLP TATA box and the +<NUM> position of transcription.

Adenovirus is the most commonly investigated and exploited virus in modern scientific research. It has found utility in the fields of vaccination, gene therapy, virotherapy, and also as complex tools for understanding biological systems (McConnell et al.

The adenoviridae family of viruses are double stranded DNA viruses which were first isolated from the adenoids of infected children in <NUM> (Rowe et al. The family consists of many species infecting a broad variety of hosts including humans, birds and amphibians and is divided into four genuses to reflect the wide variety of hosts they infect.

The mastadenoviridae consists of <NUM> unique adenovirus species infecting mammalian hosts. Within this genus there are currently seven distinct species of adenovirus that infect humans. They are denoted by a letter as human adenoviruses A-G. Within these species multiple serotypes have been identified that are numbered from <NUM>-<NUM> and are all recognised as independent strains by the International Committee on the Taxonomy of Viruses:.

Adenoviruses are small (approximately <NUM> in diameter) non-enveloped viruses with an icosahedral capsid with <NUM> fibres projecting from the icosahedron vertices. The virus consists of <NUM> hexon trimers, <NUM> penton pentamers, <NUM> Illa monomers, <NUM> fiber trimers, <NUM> VII hexamers, <NUM> IX trimers as well as two terminal repeat proteins and multiple core proteins. Many of the latter are essential for intracellular trafficking and proteolytic cleavage of endocytosed viral capsids.

The DNA genome of adenovirus varies in length dependent on serotype but is typically <NUM>-<NUM> kilobases in length. The adenovirus serotype five genome is usually is <NUM> base pairs with a <NUM> base pair terminal repeat at each end and a <NUM>% GC content. The genome is linear within the capsid structure and for the majority of the replication cycle but can form pan-handle circular structures within the nucleus during genome replication.

The process of cell attachment for adenoviruses varies dependent on the serotype. Adenovirus species C (including serotypes two and five) have been shown to attach to cells via their fibre domain binding to the cell surface coxsackie and adenovirus receptor (CAR) (Tomko et al. , <NUM>) which is a component of cellular tight junctions (Honda et al. This initial interaction is high affinity and is followed by a lower affinity interaction between the virus penton base and cell surface integrins (αVβ3 & αVβ5) which are abundant on epithelial cells (Wickham et al. Following absorption to the cell surface virions are endocytosed and in a poorly defined step the virus capsid escapes from the endosome into the cytosol. Within the cytosol adenoviral capsids bind to the microtubule network and are transported via a Dynein dependent mechanism to the nucleus where the DNA is delivered into the nuclear lumen following capsid interaction with the nuclear pore complex (Trotman et al. , <NUM>; Kelkar et al.

Our understanding of adenovirus genetics, transcription and translation is primarily derived from virological studies using adenovirus species C serotype five. The sequential process of gene transcription from the adenovirus genome reflects the protein requirements of the virus at each stage of the replication process. The transcription from the adenovirus genome is therefore divided into early and late events dependent on the timing of initiation of transcription from each viral promoter (<FIG>). The first proteins produced from the virus genome are the E1A proteins. The E1A transcription unit produces multiple mRNA molecules through alternative splicing which in turn produce multiple proteins ranging from <NUM>-<NUM> kDa. The E1A proteins have two major roles within an infected cell. Firstly, they induce the cell to enter the S phase of the cell cycle to allow the efficient replication of the viral genome. Secondly, they induce transcription of the other early promoters within the viral genome through transactivation. These promoters control the production of the E1B, E2, E3, E4 and E5 proteins. E1A expression is immediately followed by VA RNA and E1B and E3 protein production. These proteins and RNA molecules help to prevent the development of an anti-viral response. These early events in viral replication help to shape the intracellular environment to allow the replication of the viral genome before packaging. Later transcription events involve the production of structural proteins and proteins essential for cell lysis which are derived primarily from a single promoter (the major late promoter) which transcribes the late regions <NUM>-<NUM>. Cell lysis is dependent on the E3-<NUM> protein (also termed the adenovirus death protein) which despite its labelling as an early gene is only produced late in infection and from the major late promoter (Tollefson et al.

Adenovirus genes are divided into early (E1-<NUM>) and late (L1-<NUM>) transcripts, with multiple protein isoforms driven from a range of splicing events. The early regions are divided into E1, E2, E3 and E4. E1 is essential for transitioning the cell into a phase of the cell cycle that is conducive to virus replication and inhibiting apoptosis and promoting cell division. The E2 region is largely responsible for the replication of the DNA genome, containing the DNA binding protein (E2A), the terminal protein and the DNA polymerase (E2B). E3 contains genes involved in immune regulation of host responses and E4 contains a range of genes involved in regulating cell pathways such as non-homologous end joining (NHEJ) and complexing with E1B-<NUM> to mediate p53 degradation.

The adenovirus late genes are all transcribed from the same promoter, the Major Late Promoter and all share the same <NUM>' mRNA terminus which contains three exons that collectively form the tri-partite leader sequence. The late genes are expressed by a series of splice events that allow the expression of approximately <NUM> proteins that either form a part of the virus particle (e.g. Hexon and Fibre) or involved in its assembly (e.g. <NUM> protein).

Adenoviral vectors are vectors which are based on or derived from the genome of a virus of the family Adenoviridae. Preferably, the adenovirus is a human adenovirus from group A, B, C, D, E, F or G. More preferably, the adenovirus is a human adenovirus from group B or C or D. Even more preferably, the adenovirus is a human adenovirus from groups B or C.

The adenoviral vector may comprise a plurality of adenoviral early genes (<FIG>).

The E1A proteins are the translation products of the first gene transcription events from the adenovirus genome within the nucleus at the E1A region. This initial transcription is driven by a strong constitutively active enhancer element within the E1A promoter and allows significant quantities of E1A mRNA to be produced. They are one of two sets of proteins in the adenovirus genome which are capable of inducing transformation with E1B proteins also able to induce cell cycle progression. E1A and E1B genes are essential for virus replication.

The E2 genes are divided into two sections in the adenovirus genome: the E2A and the E2B regions, and both are required for virus replication. E2B contains the DNA polymerase gene which is fundamentally required for the amplification of the virus genomic DNA. Similarly, this region also contains the Terminal protein which is required for the initiation of virus genome replication. The terminal protein is covalently attached the end of the virus genomic DNA. The E2A region contains a DNA binding protein that is required for DNA replication. All E2 genes are fundamentally required for virus replication.

The E3 genes are primarily involved in regulating cell and host immune responses to virus infection, however, as the majority of viruses used for biotechnology applications are in vitro many, if not all, of these virus genes can be removed without reducing virus replication efficiency. The majority of the E3 genes are not essential for virus replication. However, some genes such as the Adenovirus Death Protein (ADP) are required for efficient replication and virus production.

The E4 region of the adenovirus genome is similar to the E1 region in that it is primarily involved in producing proteins that help the virus control and regulate the cell to ensure efficient virus replication and production. The region includes <NUM> open reading frames (ORFs) that are able to aid in preventing non-homologous end joining and apoptosis amongst a number of other discrete functions. The relative importance of each E4 transcript to virus replication is variable with some being essential whilst others can be deleted or modified with little to no effect of virus growth kinetics and production.

The adenoviral vector of the invention preferably comprises sufficient adenoviral early genes in order for the adenovirus to be capable of replicating the viral genome in the nucleus of a cell in which it is placed.

The adenoviral vector comprises a plurality of adenoviral late genes (<FIG>).

The virus late genes are divided into five main transcript families named L1-L5. These transcripts primarily encode proteins that are involved in virus assembly and the structural proteins of the virus. During virus replication they can represent as much as <NUM>-<NUM>% of the cells protein content (Garnier, <NUM>; Ginsberg, <NUM>).

The L1 series of transcripts encode for the <NUM>, <NUM>, and PIIIa proteins. These proteins are all involved in virus assembly and particle production. L1 genes are required for successful virus assembly but not genomic DNA replication.

The L2 series of transcripts encode for the penton base, pVII, V, pX proteins. These form structural parts of the virus capsid and are required for the particle to assemble correctly.

Penton base contains an RGD motif that is important for virus attachment to the cell surface during infection. L2 genes are required for successful virus assembly but not genomic DNA replication.

The L3 series of transcripts encode for the pVI, hexon, and protease proteins. The Hexon protein is a major component of the virus capsid and is antigenically diverse between serotypes. The protease protein is involved in cellular entry and the virus capsid maturation. L3 genes are required for successful virus assembly but not genomic DNA replication.

The L4 series of transcripts encode the <NUM>, <NUM>, <NUM>, pVII proteins. These proteins are involved in a range of functions. <NUM> protein is involved in both aiding virus hexon assembly and nuclear import but may also play a role in shifting cell mRNA translation to cap-independent translation. In one embodiment of the invention, the <NUM> protein may be provided in trans within a cell rather than from within the virus genome. The <NUM> protein is involved in virus encapsidation. L4 genes are required for successful virus assembly but not genomic DNA replication. However, the <NUM> protein may aid in shifting cellular protein translation towards those transcripts that contain a tripartite leader (TPL) sequence.

As such, in one embodiment of the invention, the expression of the <NUM> protein may not be controlled by the MLP. The <NUM> protein in one embodiment may be transferred to another position in the virus genome not under the control of the MLP. In another embodiment, the <NUM> protein may be transferred to a separate virus. In another embodiment, the <NUM> protein may be transferred to the chromosome of a cell or provide in trans by DNA transfection or electroporation.

L5 encodes the Fibre gene. Fibre is a virus structural protein involved in attachment to cell surfaces and in mediating virus cellular infection. The Fibre protein is produced in significant excess of its requirement for virus particle formation. An embodiment of the invention may silence a minimum of one of either Fibre or Hexon (L3) proteins as these are some of the most abundant proteins produced during virus replication. L5 genes are required for successful virus assembly but not genomic DNA replication.

The adenoviral vector of the invention preferably comprises sufficient adenoviral late genes in order for the adenovirus to be capable of being packaged in a cell to produce virus particles capable of infecting another mammalian cell. The virus genome will contain at least one late transcript generated from the Major Late promoter. Some proteins may be removed and provided in trans and others may be transferred into a host cell chromosome.

In the wild-type adenoviral genome, a single Major Late Promoter (MLP) is responsible for promoting the parallel transcription of the adenoviral late transcripts, L1-L5 (<FIG>). The adenoviral vector of the invention also comprises a MLP. The MLP is situated at the <NUM>'-end of these late transcripts.

Multiple mRNAs are produced from the late transcripts via differential use of <NUM>'-splice and poly(A) sites. All of these transcripts contain the tripartite leader (TPL) sequence.

<FIG> shows an annotated sequence of the major late promoter. Key features in the promoter include a number of transcription factor binding sites. This includes a CAAT box, a UPE box, a TATA box, a MAZ/SP1 binding site, a +<NUM> position of transcription, and INR element, and an enhancer region containing an R1 region, DE1 and DE2 sub-region. These features have been shown to be important to varying degrees for major late promoter activity. Key features that are known to significantly reduce promoter activity if modified or deleted are the TATA box, INR element, the R region and DE1 and DE2 regions. The TATA box is considered the single most important feature, with transcription initiation occurring at the <NUM>th base pair after the last base of the TATA sequence itself.

The nucleotide sequence of the wild-type Ad5 MLP is given below:
<IMG>.

The TATA box is underlined in the above sequence and the final base (in bold) denotes the position of transcription initiation (i.e. the +<NUM> position).

In the adenoviral vector of the invention, the MLP comprises one or more repressor elements. The repressor element(s) are capable of regulating or controlling transcription of the adenoviral late genes. Preferably, the repressor element(s) are capable of repressing transcription of the downstream adenoviral late genes.

One or more repressor elements may be present in the MLP. Preferably, there are <NUM>, <NUM>, <NUM> or <NUM> repressor elements; more preferably <NUM> or <NUM>.

One or more (preferably one) repressor elements are located downstream of the MLP's TATA box. In other embodiments, one or more (preferably one) repressor elements are additionally located upstream of the MLP's TATA box. In other embodiments, one or more (preferably one) repressor elements are located upstream of the MLP's TATA box and one or more (preferably one) repressor elements are located downstream of the MLP's TATA box.

One or more repressor elements are inserted between the MLP TATA box and the +<NUM> position of transcription. Even more preferably, the start of one or more repressor elements is placed less than <NUM> nucleotides, more preferably less than <NUM> nucleotides, and even more preferably less than <NUM> nucleotides downstream of the TATA box.

The repressor is a DNA binding protein. The repressor will either bind to DNA and directly inhibit the recruitment of transcription factors required for transcription initiation, or the repressor will sterically hinder the initiation of transcription by occupying a key footprint on the DNA that prevents transcription factors that are required for transcription initiation from binding. The repressor may be regulated by a small molecule that causes a conformational shift in the repressor protein that either enables, or prevents, its DNA binding. The repressor is not an activator.

Promoters regulated by a repressor are typically induced by the presence or absence of biotic or abiotic factors.

The proteins that may be used as repressors in the context of this invention are the tetracycline repressor, the lactose repressor, the ecdysone repressor, rat glucocorticoid receptor and human estrogen receptor.

Preferably, the repressor is the tetracycline repressor, the lactose repressor or the ecdysone repressor. Most preferably, the repressor is a Tet repressor protein (TetR).

The TetR binding site may have a wild-type sequence. Preferably, the TetR binding site has been subject to one or more improvements by incorporating minor sequence changes. A preferred version that can be used in an embodiment of the invention has the sequence:
tccctatcagtgatagaga (SEQ ID NO: <NUM>).

Alternative versions of the repressor element that bind the TetR protein or derivatives of the TetR protein may also be used in an embodiment of the invention provided that the TetR repressor protein binds to the TetR binding sequence variant used. Some repressor/binding site variants will have higher than wild-type affinity for each other; these are preferable in an embodiment of the invention.

In one embodiment of the invention, the DNA sequence of the TetR protein is:
<IMG>
or a sequence having at least <NUM>%, more preferably at least <NUM>%, <NUM>% or <NUM>% sequence identity thereto and which codes for a TetR protein.

In one embodiment of the invention, the amino acid sequence of the TetR protein is:
<IMG>
or a sequence having at least <NUM>%, more preferably at least <NUM>%, <NUM>% or <NUM>% sequence identity thereto and which encodes a TetR protein.

When TetR is bound to the repressor element (e.g. repressor binding site), tight suppression of transcription is obtained. However, in the presence of doxycycline, suppression is alleviated, thus allowing the associated promoter to regain full transcriptional activity. Doxycycline is preferable over tetracycline.

The repressor element may be introduced into the MLP by modification of the MLP sequence. The repressor element may be introduced by insertion of a repressor element into the MLP sequence; by substitution of one or more nucleotides in the MLP sequence to create a repressor element sequence; or by a combination of insertion/deletion of a new sequence.

In one embodiment of the invention, the distance between the TATA box and the +<NUM> position of DNA transcription of the MLP is maintained (+/- <NUM>%), but a repressor binding site is inserted between the two. Within this region, there is a MAX/SP1 binding site. This site is not fundamental to MLP expression and therefore, in one embodiment of the invention, it can be replaced. <FIG> shows an embodiment of the invention where the region between the TATA box and the +<NUM> position of transcription has been replaced with a binding site for the tetracycline repressor protein (TetR).

In some adenoviral vectors, the section of the DNA strand which is opposite to that of the MLP sequence encodes the early viral protein E2B (which encodes the viral DNA polymerase). In order to maintain the ability of such adenoviral vectors to replicate their genomes, it is necessary to ensure that the modifications which are made to the MLP sequence do not significantly adversely affect the production, stability or efficacy of the E2B protein.

In Adenovirus serotype <NUM>, the MLP resides in the middle of the E2B polymerase Exon <NUM>. As such, in one embodiment of the invention, the insertion of a repressor element (e.g. repressor binding site) into the MLP must maintain the coding frame of the DNA polymerase coding sequence in the opposing DNA strand or ensure that the modifications which are made to the MLP sequence do not significantly adversely affect the production, stability or efficacy of the E2B protein.

Preferably, some or all of the changes to the MLP sequence are silent changes, i.e. they do not change the E2B codons. In other embodiments, some or all of the changes to the MPL are conservative changes, i.e. one or more E2B codons are changed such that they encode an amino acid having a similar side chain.

Families of amino acid residues having similar side chains have been defined in the art. These families include amino acids with basic side chains (e.g. lysine, arginine, histidine), acidic side chains (e.g. aspartic acid, glutamic acid), uncharged polar side chains (e.g. glycine, asparagine, glutamine, serine, threonine, tyrosine, cysteine, tryptophan), nonpolar side chains (e.g. alanine, valine, leucine, isoleucine, proline, phenylalanine, methionine), beta-branched side chains (e.g. threonine, valine, isoleucine) and aromatic side chains (e.g. tyrosine, phenylalanine, tryptophan, histidine).

Thus, one or more amino acid residues within the E2B protein can be replaced with other amino acid residues from the same side chain family and the altered E2B protein can be tested for any significant loss in function or activity.

In one embodiment of the invention, a TetR binding site is positioned into the MLP between the TATA box and the +<NUM> position. <FIG> shows the coding sequence of the DNA polymerase. In the region between the MLP TATA box and the +<NUM> position, the amino acid coding sequence of the DNA polymerase is ENERAPTP (SEQ ID NO: <NUM>). <FIG> shows that the strategic placing of a TetR binding site into this region creates a sequence ESLSLIGT (SEQ ID NO: <NUM>). This sequence maintains the reading frame of the DNA polymerase but also allows for more than <NUM>% of the wild type amino acids to be exchanged for those with similar side chains. Importantly, the sequence of the TetR binding site contains stop codons in the opposing DNA strand if positioned incorrectly which would likely create a non-functional DNA polymerase.

In one embodiment of the invention, therefore, the sequence on the opposite strand of the TetR binding site is or comprises a sequence encoding ESLSLIGT (SEQ ID NO: <NUM>). Preferably, the DNA polymerase comprises a sequence of SEQ ID NO: <NUM>.

Some loss in amount of E2B mRNA or protein produced may be tolerated, as may some changes in the amino acid sequence of the E2B protein. The skilled person will readily be able to assess the effect of changes on the E2B gene sequence on the ability of the virus to replicate simply by assessing the viral titre of a modified adenoviral vector under standard conditions in comparison to the original unmodified virus. Changes which reduce the viral titre by less than <NUM>%, preferably less than <NUM>% and more preferably less than <NUM>% may be considered to be ones which do not significantly adversely affect the production, stability or efficacy of the E2B protein.

In other adenoviral vectors of the invention, the E2B gene is positioned elsewhere in the adenoviral vector such that modifications in the MLP do not affect the production of the E2B protein.

An example of a modified MLP which contains one TetR binding site between the TATA box and the +<NUM> position of transcription is given below:
<IMG>.

The TATA box is underlined and the TetR binding site is shown in bold.

An example of a modified MLP which contains one TetR binding site between the TATA box and the +<NUM> position of transcription and a second site upstream of the TATA box between the UPE element and the TATA box is shown below:
<IMG>.

The repressor which binds to the repressor element(s) may be applied exogenously (to the cells); it may be encoded within the cellular or mitochondrial genome (or a plasmid or vector within the cell); or it may be encoded within the adenoviral genome. Preferably, the repressor is encoded by a gene within the adenoviral genome.

More preferably, the repressor gene is located within one or more of the viral early expression regions or the late gene expression regions. Even more preferably, the repressor gene is located in the virus late region. Even more preferably the repressor is located in a late transcript that is transcribed from an MLP that is regulated by the repressor. The system is thereby self-repressing.

In one embodiment, the gene encoding the repressor protein is under the control of an independent promoter (i.e. a promoter which is not the adenoviral major early promoter or major late promoter). Preferably, the gene encoding the repressor protein is under the control of a strong promoter (e.g. the cytomegalovirus (CMV) promoter). Even more preferably, the repressor protein is under the control of the MLP to which it binds.

Preferably, the mRNA encoding the repressor protein comprises a Tripartite Leader (TPL) sequence in its <NUM>'-UTR. TPL is a <NUM>' untranslated sequence which is present in all of the late, but none of the early, viral mRNA. TPL facilitates mRNA transport and accumulation in the cytoplasm and is responsible for the selective translation of the late viral proteins in preference to the cellular proteins.

The Ad5 leader sequence is <NUM> bp formed by the splicing of three exons during the post-translational modifications.

The adenoviral vector of the invention may comprise at least one transgene. In such embodiments, a key function of the adenoviral vector is to facilitate production of the transgene product.

During adenoviral infection up to <NUM>% of the mRNAs can be from the viral genome and these can be preferentially translated to maximise virus output. The selective production of virus specific mRNA is down to a combination of the amplification of the virus DNA polymerase and a shift towards the production of late mRNA transcripts. The replication of the virus DNA genome allows for thousands more copies of the DNA template for transcription to occur from. This activity, coupled with the presence of the tri-partite leader at the <NUM>' end of late transcripts, allows the selective expression of late mRNA. This is because the tripartite leader, whilst highly active in normal translation processes, is also selectively translated when cap-independent translation is turned on within a cell. Multiple virus proteins are involved in this process.

Preferably, the transgene is inserted within one of the adenoviral early regions. More preferably, the transgene is inserted within the adenoviral E1 region. Even more preferably, the E1A and E1B genes are deleted from the Adenovirus genome and the transgene is inserted into this region. Preferably, the transgene comprises a TPL sequence in its <NUM>'UTR. This ensures that the transgene is expressed in a cap-independent manner.

The transgene may be any desired DNA sequence. There may be more than one transgene (e.g. <NUM>, <NUM>, <NUM>, or <NUM> transgenes). The DNA sequence of the transgene(s) may be a coding or noncoding sequence. It may be genomic DNA or cDNA. Preferably, the DNA sequence encodes a polypeptide, more preferably a therapeutic polypeptide. In some cases, the transgene will encode multiple proteins. Preferably, the transgene is operably associated with one or more transcriptional and/or translational control elements (e.g. an enhancer, promoter, terminator sequence, etc.).

A polypeptide encoded by a transgene could be a human gene or modified form thereof or encode a protein from a virus that infects human cells.

Examples of preferred therapeutic polypeptides include antibodies, CAR-T molecules, scFV, BiTEs, DARPins and T-cell receptors and antigens from human viral pathogens.

In some embodiments, the therapeutic polypeptide is a G-protein coupled receptor (GPCR), e.g. DRD1. In some embodiments, the therapeutic polypeptide is an immunotherapy target, e.g. CD19, CD40 or CD38. In some embodiments, the therapeutic polypeptide is a functioning copy of a gene involved in human vision or retinal function, e.g. RPE65 or REP. In some embodiments, the therapeutic polypeptide is a functioning copy of a gene involved in human blood production or is a blood component, e.g. Factor IX, or those involved in beta and alpha thalassemia or sickle cell anaemia. In some embodiments, the therapeutic polypeptide is a functioning copy of a gene involved in immune function such as that in severe combined immune-deficiency (SCID) or Adenosine deaminase deficiency (ADA-SCID). In some embodiments, the therapeutic polypeptide is a protein which increases/decreases proliferation of cells, e.g. a growth factor receptor. In some embodiments, the therapeutic polypeptide is an ion channel polypeptide. In some preferred embodiments, the therapeutic polypeptide is an immune checkpoint molecule. Preferably, the immune checkpoint molecule is a member of the tumour necrosis factor (TNF) receptor superfamily (e.g. CD27, CD40, OX40, GITR or CD137) or a member of the B7-CD28 superfamily (e.g. CD28, CTLA4 or ICOS). In some embodiments the polypeptide encoded is an immune checkpoint molecule is PD1, PDL1, CTLA4, Lag1 or GITR.

In some embodiments the transgene encodes a virus polypeptide or multiple thereof such as the antigenically important CMV pentamer.

In other embodiments, the transgene or transgenes will encode proteins involved in the replication or structure of viruses other than Adenovirus.

Most vaccines are composed of a collection of viral proteins: either a virus-like particle (VLP), inactivated virus particle or a live attenuated virus. VLPs have the advantage of typically being composed entirely of protein and as such have none of the potential pathogenicity of the original virus. They also have the advantage over inactivated virus particles that their structure is the same as the original virus and has not been altered by the inactivation process. A number of VLPs have been shown to be successful vaccines including HPV, Hepatitis B and the Malaria vaccine RTSS. However, production in mammalian systems is often lower than required to make the VLP a commercially-viable product. An example of this is the observation that the Hepatitis B vaccine VLP is manufactured in Yeast. A system to generate VLPs in large quantities in mammalian cells is therefore desirable to ensure proper folding and glycosylation.

In some embodiments, the transgene will encode proteins that will assemble in, or outside, of the cell to produce VLPs. These VLPs may make useful vaccine products.

In a preferable embodiment, the transgenes will encode proteins from Parvoviridae (e.g. adeno-associated virus), Retroviridae (e.g. HIV), Flaviviridae (e.g. Hepatitis C virus) and Orthomyxoviridae (e.g. Influenza virus), and/or Caliciviridae (e.g. Norovirus). In a preferred embodiment, the transgene will encode Norovirus VP1 or Hepatitis B HBsAG.

Recombinant adeno-associated viruses (rAAV) are in many ways ideal vectors for the delivery of transgenes to cells for recombinant protein production or gene therapy applications. They are able to infect a wide range of hosts, elicit a robust and sustained transgene expression profile, whilst exerting minimal toxicity to the host cell. AAV is a helper-dependent DNA parvovirus that requires helper function for completion of its natural life cycle. These helper functions may be provided by many agents that include co-infection with vaccinia viruses, herpesviruses or adenoviruses. In the absence of helper agents and functions, AAV infection enters a latent phase wherein the AAV viral genome is integrated into the host cell chromosome. Subsequently, in the presence of a helper virus, the integrated AAV provirus is rescued allowing viral replication, packaging in preformed protein capsids and production of infectious virions.

In current approaches to using AAV as a biotechnology tool for DNA delivery, AAV is engineered to replace the viral rep and cap coding sequence region with the transgene of interest for delivery into target cells. The rep and cap gene sequences required for replication, integration and expression of viral capsids are supplied in trans by DNA expression plasmids, viral vectors or cell lines which are engineered to stably express these genes from the host genome.

A traditional method of rAAV production involves co-transfection of two DNA vectors: <NUM>) a plasmid containing the rAAV sequences; and <NUM>) a plasmid containing AAV rep and cap sequences. Subsequently, helper functions can be provided in trans by infection with an adenovirus or herpes virus. The amount of rep proteins required for efficient rAAV production is unclear. While it was reported that attenuation of the translation initiation codon for Rep78/<NUM> led to high levels of rAAV production (<NPL>), others have reported the exchange of the p5 promoter responsible for transcription of AAV rep with strong viral promoters, such as the human immunodeficiency virus long terminal repeat (HIV LTR) have resulted in the production of high levels of rAAV (see <CIT>). Since the discussed methods required the co-transfection of two plasmids and co-infection with a helper virus e.g. adenovirus, to produce rAAV, reproducibility and batch variation are significantly problematic. Additionally, rAAV are required to be purified from helper agents (e.g. adenoviruses) for downstream and industrial application. The final preparation also has to be free from the helper virus proteins, particularly those that are antigens from the helper virus as this could affect the human response to such an AAV product.

A second method required for production of rAAV involves the co-transfection of three DNA plasmid vectors into producer cell lines. The cis plasmids contain: the <NUM>) rAAV ITRs and transgene; <NUM>) a trans DNA plasmid encoding the AAV rep and cap; and <NUM>) a trans DNA plasmid encoding sequences from a helper virus (e.g. adenovirus). While this method has the advantage of being free of contamination from helper virus particles, co-transfection of three DNA plasmids with significantly large sizes results in poor reproducibility and substantial drop in rAAV viral titre yield.

A third method involves the construction of rAAV packaging cell lines where the rep and cap gene sequences are integrated into host cell genome. Typically, rAAV is produced from this method by transfection of the DNA cis plasmid encoding the AAV ITRs and transgene, followed by introduction of the helper agent (e.g. infection with helper adenoviruses). Alternatively, the helper viruses carrying the cis DNA AAV ITRS and transgenes (e.g. hybrid Ad/AAV) can be introduced into producer cell lines for production of rAAV (see <CIT>).

The disadvantage of this method is that it requires complex engineering of producer cell lines wherein the AAV rep and cap are stably integrated and expressed to a sufficient amount. Additionally, use of helper viruses for delivery of the cis DNA sequence (e.g. AAV ITRS and transgenes) results in contamination from helper viruses and requires downstream purification. Furthermore, toxicity of the AAV rep protein in cell lines have been reported and constitutive expression results in anti-proliferation and cell death (<NPL>). Additionally, the Rep protein was also reported to induce a negative feedback loop for repression of its own transcription (<NPL>). Other attempts to circumvent AAV rep toxicity by modification of packaging cell lines to expressed Rep have used an inducible transcription system (see <CIT> and <NPL>). Typically, these stable systems have failed to yield the required level of AAV to make them commercially scalable systems.

A fourth method of producing rAAV involves the use of helper agents (e.g. helper adenoviruses) for delivery of the AAV rep and cap genes. In this method, the recombinant adenoviruses comprise rep and cap genes which are inserted into the genome of the helper virus (typically, in the E1 region of a recombinant adenovirus). These are subsequently used for infection into packaging cell lines that may contain the cis AAV DNA sequence (e.g. AAV ITRs and transgene) or the cis DNA plasmids can be introduced by methods of transfection (<NPL>). The significant disadvantages of this method are similar to those of the traditional method of rAAV production, where difficult and costly purification steps are required for removal of contamination from the helper virus and any proteins (particularly structural proteins) from the final product.

In one embodiment of the invention, one or more transgenes in the adenoviral vector of the invention encodes an AAV Rep-Cap polypeptide. In another embodiment of the invention, one or more of the transgenes encodes an AAV genome. Preferably, the AAV genome comprises or consists of a <NUM>' and <NUM>' ITR sequence from AAV with intervening sequences. In another embodiment of the invention, one or more of the transgenes encodes a Rep-Cap polypeptide from an AAV and an AAV genome with ITRs flanking a sequence of interest. Rep or Cap or sub-transcripts or regions thereof may be encoded individually in an embodiment of the invention.

The adenoviral vector may additionally comprise, but not limited to, one or more other elements, selected from the group consisting of reporter genes, restriction enzyme sites, promoters, polyadenylation signals, un-translated regions, enhancers and insulators.

In some embodiments, the adenoviral vector additionally comprises one or more multiple-restriction enzyme sites. These sites will most preferably be Type II and either <NUM> or <NUM> base pairs in length.

The invention also provides a composition comprising an adenovirus particle comprising an adenoviral vector of the invention, together with one or more physiologically-acceptable carriers, excipients or diluents. Examples of suitable physiologically-acceptable carriers, excipients or diluents for use with virus particles are well known in the art. Preferably, the composition comprises an adenovirus particle comprising an adenoviral vector of the invention in an aqueous buffer solution. Preferably, the aqueous buffer solution comprises MgCl<NUM> and/or glycerol.

The invention also provides a kit comprising an adenoviral vector of the invention, wherein the kit additionally comprises one or more additional components selected from the group consisting of (i) a cell line that allows the adenoviral vector to infect the cells and replicate its genome, wherein the cell line will repress the adenoviral vector's MLP and (ii) one or more DNA plasmids for aiding in the construction of the adenoviral vector.

Preferably, the kit will comprise a plasmid containing the adenoviral vector that contains sites for insertion of a transgene. More preferably there will be two plasmids: the adenoviral vector plasmid and a shuttle plasmid to allow the easy manipulation of the adenoviral vector. The shuttle plasmid will contain either regions of homology to the adenoviral vector to allow homologous recombination to create a final adenoviral vector, or restriction sites that are compatible with the adenoviral vector to allow shuttling of DNA from the shuttle plasmid to the adenoviral vector plasmid.

The kit may also contain materials for the purification of the adenoviral particles such as those involved in the density banding and purification of viral particles, e.g. one or more of centrifuge tubes, benzonase, dialysis buffers, dialysis cassettes.

In other embodiments, the invention provides an adenoviral vector or a nucleic acid molecule comprising the nucleotide sequence:
<IMG>.

The above-mentioned nucleotide sequence comprises the sequence tccctatcagtgatagaga (SEQ ID NO: <NUM>)(i.e. the repressor element is not altered).

The invention also provides an isolated mammalian cell comprising an adenoviral vector of the invention. The cells are isolated cells, e.g. they are not present in a living animal. Examples of mammalian cells include those from any organ or tissue from humans, mice, rats, hamsters, monkeys, rabbits, donkeys, horses, sheep, cows and apes. Preferably, the cells are human cells. The cells may be primary or immortalised cells. Preferred human cells include HEK293, HEK293T, HEK293A, PerC6, <NUM>, HeLa and COS cells.

HEK-<NUM> cells have been modified to contain the E1A and E1B proteins and this allows the creation of viruses that have a deletion of the E1A and E1B regions to be grown in this cell line by trans-complementation. Similarly, PerC6 and <NUM> cells contain a similar modification and can also be used. Most preferably, the human cells are HEK293, HEK293T, HEK293A, PerC6 or <NUM>. Other preferred cells include CHO and VERO cells.

Adenoviral vectors may be produced by several methods, the most common of which involves homologous recombination of adenovirus plasmids in either mammalian cells or microorganisms, including bacteria and yeast. Two plasmids, termed a shuttle plasmid and an adenoviral (also called backbone) plasmid, are recombined into a DNA molecule that incorporates sequences from both plasmids. This DNA molecule can then be transfected into mammalian packaging cell lines to generate adenovirus particles.

In an embodiment of the invention wherein the MLP is regulated by a TetR protein, the virus is recovered in the presence of doxycycline which will inhibit the repressor protein and thereby prevent it from binding to the repressor element/site in the MLP promoter. This should allow for production of the adenovirus at high titres.

For protein production or the expression of virus proteins, infecting with the virus into any cell line that can be infected by adenovirus (e.g. HEK-<NUM> cells), in the absence of doxycycline, will allow the expressed TetR repressor protein to bind to the MLP repressor element and thereby shutting down the production of virus late gene expression and preventing virus particle production.

The TetR protein can be provided within the cell line infected, either transiently or stably, or encoded within the virus itself. If under the control of the MLP then with each genome replication, activation of the MLP will provide a feedback loop, further shutting down any potential new virus late gene expression.

In a further embodiment, the invention provides a process for producing a modified mammalian cell, the process comprising the step:.

In yet a further embodiment, the invention provides a process for producing a transgene product, the process comprising the steps:.

Suitable conditions for the culturing of infected mammalian cells are well known in the art.

Transgene product expression levels may be improved by the co-expression of the 100kDa L4/elF48 protein. Furthermore, the repressor protein needs to be active as a repressor (e.g. doxycycline is not present if the repressor protein is TetR).

The processes of the invention are preferably carried out in vitro or ex vivo.

The present invention is further illustrated by the following Examples, in which parts and percentages are by weight and degrees are Celsius, unless otherwise stated. It should be understood that these Examples, while indicating preferred embodiments of the invention, are given by way of illustration only.

The methods used for cloning and production of the adenoviral vectors were as follows.

Transformation of Escherichia coli (E. coli) allowed amplification of plasmids and subsequent screening for desired final DNA clones. DNA transformation was performed by thawing E. coli cells on ice, followed by the addition of <NUM>-<NUM> ng of DNA per transformation. Cells were incubated in ice for <NUM> minutes followed by <NUM> minutes heat-shock at <NUM>. LB medium (<NUM> per sample) was added to each tube and incubated for a further <NUM> minutes at <NUM>. Samples were either poured into nutrient agar plates containing selection antibiotic or <NUM>µL of each sample was streaked out to allow individual colony isolation.

Successfully transformed clones were amplified and selected using antibiotic resistance using the appropriate antibiotic in growth media. Bacterial culture broth and plates containing either Kanamycin (<NUM>µg/mL, Kanamycin Sulfate, Invitrogen, UK) or Ampicillin (<NUM>µg/mL, Ampicillin Sodium salt, Sigma Aldrich) were prepared using Lennox LB Broth Base (<NUM>/L) and Lennox LB Agar (<NUM>/L) (Invitrogen, UK), respectively. Single bacterial colonies obtained on culture plates after transformation were picked and grown overnight in broth (<NUM> mini-prep or <NUM> maxi-prep) at <NUM> with agitation (<NUM> rpm) using a Sanyo orbital incubator (SANYO Electric Biomedical Co.

Plasmids were purified by mini-prep using the QlAprep Spin Miniprep Kit (Qiagen, UK) or maxi-prep using the Qiagen High Speed Maxi-prep kit (Qiagen, UK). Plasmid clones were selected and confirmed by diagnostic restriction digestion and DNA sequencing.

For the majority of small (<<NUM> Kb) DNA constructs, DH5u E. coli bacteria (Invitrogen) were used to amplify plasmids. For larger (><NUM> Kb) constructs, XL10 Gold Ultracompetent E. coli bacteria (Stratagene) were used to amplify DNA. These cells have been engineered in order to allow the efficient delivery of large DNA plasmids via heat-shock treatment and reduce bias towards selecting for small plasmids libraries. For growing DNA which was free of DAM and DMC methylation at key restriction sites, JM110 E. coli (Stratagene) were used. These cells are deficient in methyl transferase enzymes and allow high purity methyl deficient DNA to be amplified. For recombination of DNA molecules, BJ5183 E. coli cells were used. These cells allow the recombination between two DNA molecules due to both the mutation of Endonuclease I and the expression of a RecET homologue which allows the efficient repair of double-strand breaks at homologous regions. All strains were grown in Lennox LB media or on LB agar plates at <NUM>.

Restriction endonucleases were used to generate diagnostic digestion patterns or to produce DNA molecules with sticky (non-blunt) ends or blunt ends, allowing subsequent ligation of DNA fragments with other DNA molecules with either blunt or compatible overhangs. All digestions were performed according to conditions specified by the manufacturer (enzymes were purchased from New England Biolabs, UK or Promega, UK). Where digestions were performed for molecular engineering purposes, DNA fragments of correct sizes were visualised by gel electrophoresis and purified either from excised gel bands using the QIAEX II Gel Extraction Kit for large fragments (><NUM> Kb) (Qiagen, UK) and the MinElute Gel Extraction Kit for small fragments (Qiagen, UK), or, where it was unnecessary to resolve fragments of different sizes, purified directly from the digestion reaction (QIAquick PCR Purification Kit). HyperLadder™ I (Bioline Ltd, UK) was used as a molecular weight marker for fragments ranging from <NUM>-<NUM> Kb. For larger DNA fragments a Lambda Hind3 digest ladder was used (New England Biolabs, UK). For fragments less than <NUM> Kb a <NUM> base pair ladder was used (New England Biolabs, UK).

Donor (insert) and recipient (vector) DNA were digested with single or double (for directional cloning) restriction enzyme(s) generating compatible overhangs for complementary base-pairing. Digested insert was gel-purified or cleaned up, while the vector was de-phosphorylated by treatment with <NUM>µL of calf intestinal alkaline phosphatase (<NUM>, <NUM>) (Invitrogen, UK) to reduce background contamination resulting from vector re-ligation. Vectors were then purified using the MinElute Gel Extraction Kit (Qiagen, UK) or the QIAquick PCR Purification Kit (Qiagen, UK) using the manufacturer's protocols. All purified DNA was eluted in nuclease-free water. Ligation reactions were prepared using T4 DNA Ligase (New England Biolabs, UK) according to the manufacturer's protocol.

Heat Shock DNA competent E. coli cells were produced by inoculating a single colony of E. coli into <NUM> 2xYT broth media (<NUM>/L Bacto Tryptone, <NUM>/L Yeast Extract, <NUM>/L NaCl, pH <NUM> with <NUM> NaOH) which was shaken at <NUM> for <NUM> hours. This was transferred to <NUM> prewarmed 2xYT media. When the culture reached OD <NUM> the cells were pelleted at <NUM> rpm in a swing out centrifuge at <NUM> for <NUM> minutes. Cells were re-suspended in a total of <NUM> cold TFBI1 (<NUM> KC<NUM>H<NUM>O<NUM> (Potassium acetate), <NUM> RbCI, <NUM> CaCl<NUM>·<NUM><NUM>O, <NUM> MnCl<NUM>·<NUM><NUM>O, <NUM>% v/v glycerol, adjusted to pH <NUM> using <NUM> CH<NUM>COOH, filter sterile). Cells were spun as above and re-suspended in <NUM> of TFBI2 (<NUM> MOPS, <NUM> RbCI, <NUM> CaCl<NUM>·<NUM><NUM>O, <NUM>% v/v glycerol, adjusted to pH <NUM> using <NUM> KOH, filter sterile). <NUM>µl of cells were pipette into pre-chilled <NUM> microfuge tubes and frozen on dry ice. Tubes were then transferred to -<NUM> for long term storage.

Polymerase chain reactions (PCR) were performed using oligonucleotide primers designed according to the requirements for molecular manipulation, sequencing or screening procedures (purchased from Sigma-Genosys, UK). Primer sequences employed for vector engineering and molecular characterisation purposes are described below.

For sub-cloning of DNA fragments generated by PCR amplification from DNA templates, high fidelity AccuPrime™ Pfx proofreading DNA polymerase (Invitrogen, UK) was used. For routine screening for the presence of specific DNA sequences by PCR, PCR SuperMix (Invitrogen, UK) was used. Primers were dissolved in de-ionised, nuclease-free water at <NUM>; <NUM>-<NUM>µL of each of the forward and reverse primers were used per PCR reaction. Reactions were carried out according to recommended protocols provided by the suppliers of enzymes and reagents. Where necessary, primer concentrations were varied and a gradient of annealing temperatures was run to determine optimal reaction conditions. PCRs were performed using a PTC-<NUM> Peltier Thermal Cycler DNA Engine Tetrad (MJ Research, USA).

Size fractionation of DNA on <NUM>% (w/v) agarose (Invitrogen, UK) gels containing ethidium bromide (Sigma-Aldrich, UK) (<NUM>µg/mL) in <NUM> x TAE buffer (<NUM> Tris-base, <NUM> glacial acetic acid, <NUM> EDTA in <NUM>) enabled visualisation of DNA and size estimation, by relative comparison to commercially available molecular weight markers described above. DNA molecules from purified plasmids or fragments from PCR reactions or restriction digestions were subjected to gel electrophoresis (<NUM> volts per cm gel length, <NUM>-<NUM> minutes) in horizontal DNA electrophoresis gel tanks (Bio-Rad Laboratories Ltd, UK). DNA bands were visualised using a gel and fluorescent imaging system (Alphalmager, Alpha Innotech Corporation, USA) under ultraviolet light.

DNA was quantified using a Nanodrop (Thermo Scientific, UK) spectrophotometer. Prior to analysis equipment was blanked using distilled water and then background readings were performed using the solution in which the DNA was dissolved (TE, EB or H<NUM>O). Samples were tested in triplicate and data was interpreted using the ND-1000v <NUM>. <NUM> software according to the manufacturer's instructions. The final quantity of DNA was expressed as nanograms/microlitre.

Swal-linearised adenoviral plasmids containing either recombinant adenoviral genomic DNA or the wild-type adenovirus genome were transfected into HEK-<NUM> cells using Lipofectamine <NUM> transfection. HEK-<NUM> cells were seeded in wells of a <NUM>-well plate <NUM> prior to transfection so that they were <NUM>-<NUM>% confluent at the time of transfection. For each well, lipofectamine <NUM> suspended in 100u! Opti-MEM Reduced Serum Media (Thermo Fisher Scientific) was mixed with DNA solution (<NUM>µg in <NUM>µL Opti-MEM Reduced Serum Media) at a <NUM>:<NUM> ratio of total DNA mass to lipofectamine <NUM> and incubated at room temperature before being added dropwise to adherent HEK-<NUM> which were growing in DMEM with <NUM>% Fetal Bovine Serum (FBS) from Gibco® (Thermo Fisher Scientific UK).

The culture media containing the lipofectamine <NUM> transfection complex was removed at <NUM> post-transfection. Fresh DMEM media containing <NUM>% FCS was added to each well. Cytopathic effects (CPE) were observed in wells containing successfully transfected cells between <NUM> and <NUM> days post-transfection. Virus stocks were serially <NUM>-fold diluted into <NUM> well plates. Single clones were picked and amplified in <NUM> dishes from which infectious supernatants were collected and stored as seed stock for further amplification and virus production.

Single virus clones were amplified in HEK-<NUM> cells cultured in DMEM media containing <NUM>% FCS, using approximately <NUM>-<NUM> confluent <NUM><NUM> monolayers for each purification. HEK-<NUM> monolayers containing virus-packed cells were harvested (<NUM> hours post-infection, when CPE was observable but infected cells were not lysed) by gentle agitation and pelleted cells were re-suspended in infectious supernatant (<NUM>, volume accommodated in three banding columns), then lysed by three freeze-thaw cycles to release virus particles. The mixture containing lysed cells and free virus particles was centrifuged at <NUM> (<NUM>, <NUM>). The mixture was incubated on ice for <NUM>, followed by centrifugation at <NUM> (<NUM>, <NUM>). The pellet was discarded and the supernatant (containing virus particles) was loaded onto centrifuge tubes (Ultra-clearTM Beckman Centrifuge tubes, Beckman Coulter UK Ltd) containing a caesium chloride (CsCI) gradient. The gradients were centrifuged (<NUM>,<NUM> rpm, <NUM>, <NUM> without deceleration using a Beckman L8-<NUM> Ultracentrifuge with rotor type SW40 Tl) (Beckman Coulter, Inc, USA). Two discrete bands were obtained after centrifugation: a faint band higher in the column containing 'empty' viral particles, and a thicker, opaque lower band containing intact infectious viral particles. The virus was harvested by puncturing the tube below the level of the virus band with an <NUM>-gauge needle and extracting the desired band into a syringe.

CsCI was subsequently removed by consecutive dialyses in buffers (<NUM>, <NUM>) containing <NUM> HEPES, 1x PBS, <NUM>/L CaCl<NUM>, <NUM>/L (initial dialysis) or <NUM>/L (final dialysis) MgCl<NUM> and <NUM>% glycerol at pH <NUM>, using a <NUM>-<NUM> dialysis cassette for the initial dialysis (Pierce Slide-A-Lyzer® Dialysis Cassette, Pierce Biotechnology, Inc. , USA) after which the virus was recovered and treated with Benzonase DNA nuclease (<NUM>µL/mL, Novagen, UK) for <NUM> minutes at room temperature. The virus was subsequently re-banded by CsCI gradient centrifugation and dialysed overnight in the final dialysis buffer using a <NUM>-<NUM> cassette (Pierce Slide-A-Lyzer® Dialysis Cassette, Pierce Biotechnology, Inc. For each dialysis, the buffer was changed and replaced with fresh buffer after <NUM> hour and <NUM> hours, followed by an overnight dialysis. Virus obtained after the final dialysis was aliquoted and stored immediately at -<NUM>.

Adenoviral DNA concentrations were determined using the PicoGreen assay (Quant-iT™ PicoGreen ® dsDNA Reagent, Molecular Probes, Invitrogen). The assay contains a fluorescent nucleic acid probe for double-stranded DNA (dsDNA), allowing quantification of adenoviral genome content. Appropriate dilutions of virus stock solutions (<NUM> to <NUM>-fold) were made and were transferred (<NUM>µL) to a solution containing <NUM> x TE buffer (<NUM>µL) and <NUM> % sodium dodecyl sulphate (SDS) in <NUM> x TE (<NUM>µL). Samples were incubated at <NUM> (<NUM>) to disrupt virus particles. Six four-fold serial dilutions of known concentrations of the bacteriophage lambda DNA provided in the Quant-iT™ PicoGreen® Kit were carried out (highest concentration at <NUM>µg/mL), allowing the construction of a standard curve (last standard blank) from which the DNA content in unknown samples were calculated. The PicoGreen reagent was diluted <NUM>-fold in <NUM> x TE buffer. <NUM>µL of the diluted reagent was placed in wells of a black <NUM>-well plate (Corning, UK) for each standard or unknown sample. <NUM>µL of appropriately diluted standards and samples were added to the wells in duplicate. The plate was read in a Wallac <NUM> Victor2 multi-label counter, using the `Fluorescein <NUM>/<NUM>, <NUM> second' program for analysis. The number of viral particles present in each sample was calculated on the basis that <NUM>µg of DNA is approximately equal to <NUM> x <NUM><NUM> adenoviral particles.

The tissue culture infectious dose <NUM> (TCID50) method (Karber, <NUM>) was used to estimate the number of infectious virus particles, or plaque forming units (pfu), and is based on the development of cytopathic effects (CPE) in HEK-<NUM> cells after infection with <NUM>-fold serially diluted samples of virus preparation. This method is described in full in the manual for the AdEasy non-replicating virus platform available from QBiogene (France).

All adenoviruses were grown in HEK-<NUM> cells, purified by double banding in CsCI gradients as described above. Viral particle (vp) number was determined by measuring DNA content using a modified version of the PicoGreen assay (Invitrogen, Paisley, UK) (Mittereder et al. Infectivity was calculated using the TCID50 system with the KARBER statistical method (Karber, <NUM>) and was used to estimate the adenovirus titer (TCID50 units/mL) and corrected to determine plaque forming units/mL (pfu/mL).

HEK293 human embryonic kidney cells were obtained from the European Collection of Cell Cultures (Porton Down, UK), and maintained in DMEM media with <NUM> % FCS (PAA Laboratories, Yeovil, UK) including penicillin (<NUM> U/mL) and streptomycin (<NUM>/mL) at <NUM> in <NUM> % CO<NUM> in a humidified incubator.

The Q-PCR methodology for measurement of adenoviral particles has been previously described (Green et al. Briefly, viral DNA from infected cells or tissue samples was extracted using a mammalian genomic Genelute DNA extraction kit (Sigma). Reactions were performed using Applied Biosystems master mix following the manufacturer's protocol. The cycles were as follows: <NUM> degrees Celsius <NUM>, then <NUM> times at <NUM> ° Celsius <NUM>, <NUM> °Celsius <NUM>. Primers sequences for targeting Ad5 fiber were: Forward primer - <NUM>' TGG CTG TTA AAG GCA GTT TGG <NUM>' (SEQ ID NO: <NUM>) (Ad5 <NUM>-<NUM> nucleotides) and reverse primer - <NUM>' GCA CTC CAT TTT CGT CAA ATC TT <NUM>' (SEQ ID NO: <NUM>) (Ad5 <NUM>-<NUM> nt) and the TaqMan probe- <NUM>' TCC AAT ATC TGG AAC AGT TCA AAG TGC TCA TCT <NUM>' (SEQ ID NO: <NUM>) (Ad5 <NUM>-<NUM> nt), dual labelled at the <NUM>' end with <NUM>-carboxyfluorescein and the <NUM>' end with <NUM>-carboxytetramethylrhodamine. The results were analyzed with the Sequence Detection System software (Applied Biosystems). Standard curves for tissues and cells were prepared by spiking samples of cell lysate or tissue homogenate with serial dilutions of known concentrations of virus particles followed by extraction and analysis of each sample separately by Q-PCR as described above.

Where determination of adenoviral genome numbers was necessary, viral DNA was extracted from culture supernatants or cell lysates prepared in either lysis solution C (Sigma, UK) or lysis solution from the luciferase assay system (Promega, UK). Samples were treated with proteinase K (<NUM>/mL) and incubated at <NUM> degrees Celsius for <NUM> minutes to degrade viral capsid proteins, followed by a <NUM> minute incubation at <NUM> degrees Celsius. Total cellular DNA extraction was then performed using the Genelute mammalian DNA extraction kit (Sigma-Aldrich, UK) according to the manufacturer's instructions.

Cells were seeded in triplicate in <NUM> well plates. After <NUM> plasmid DNA (<NUM>µg) was added to <NUM>µL of HBS buffer and mixed with <NUM>µL DOTAP reagent (Roche) also in <NUM>µL sterile HBS. The complex was incubated at room temperature for <NUM>. <NUM>µL of transfection mixture was added to each well and incubated at <NUM> for <NUM>. Cells were washed with PBS and incubated with DMEM containing <NUM> % fetal calf serum (FCS) (PAA Laboratories, Yeovil, UK). <NUM> following transfection media was removed and <NUM>µL of reporter cell lysis buffer (Promega) was added to the cells. Cells were then frozen at -<NUM> for <NUM> before thawing. Luciferin (<NUM>µL) (Promega, Southampton, UK) was added to <NUM>µL aliquots of cell lysate and relative luminescence was measured by luminometry (Lumat LB9507, Berthold Technologies, Redbourn, UK).

Cells are cultured using the conditions described above, or conditions favourable for any such cell line, in which a transgene within the virus of the invention is to be expressed. Virus is added to the culture supernatant of the cells at an MOI from <NUM>-<NUM>, more preferably an MOI of <NUM>-<NUM> and more preferably still an MOI of <NUM>-<NUM>.

Transgene expression level or the level of expression of late proteins within a cell is measured via Western blot or an Enzyme-linked Immunosorbant Assay (ELISA). The method taken depends on whether the product being measured is intracellular or secreted outside of the cell. For the former, the level of protein is measured by lysing the cells to create a cell lysate followed by western blot or ELISA. For secreted material, the supernatant is analysed immediately by western blot or ELISA.

If a western blot protocol is used, the following approach is taken. <NUM>µg of protein is loaded onto a <NUM>% polyacrylamide gel after quantitation using a QuantiPro BCA assay (Sigma Aldrich, cat: QPBCA-1KT). The gel is run at <NUM> V for <NUM> and then protein is blotted onto to a nitrocellulose membrane overnight at <NUM> degrees Celsius at 30V. Nitrocellulose membrane is stained with Ponceau solution (described below) to confirm equal loading and transfer of samples and then blocked using <NUM> % milk powder (Fluka, Sigma Aldrich) for <NUM> (E1A) or overnight (Aldolase A). Membranes are then washed twice with PBS, <NUM> % Tween <NUM>, and then once with PBS. For detecting repression levels of adenovirus late proteins, an anti-Hexon western blot is used. A primary antibody recognising Hexon (AbCam, Cambridge, UK, cat number: Ab8249) is added at <NUM>:<NUM> dilution in <NUM> % milk powder in PBS for <NUM> hr. Membrane is washed as above. Secondary anti-rabbit HRP labelled antibody is added at <NUM>:<NUM> dilution in <NUM> % milk powder for <NUM>. The membranes are washed as above and then bathed in ECL western blotting detection reagent (Amersham, GE Healthcare) at <NUM>/cm<NUM> for <NUM> minute. Blot is visualised in an Alpha Innotech gel documentation system for <NUM>, <NUM> and <NUM> minutes using chemi-luminescence detection. Molecular weights are calculated against a dual colour molecular weight ladder (Bio-Rad).

To confirm successful transfer of protein from poly-acrylamide gels onto nitrocellulose membranes and to ensure equal loading and transfer, membranes are stained for <NUM> minutes with Ponceau S solution (<NUM> % w/v Ponceau S in <NUM> % v/v acetic acid made up with de-ionised distilled H<NUM>O) prior to blocking. The stain is then poured off and membranes washed briefly in PBS twice before imaging. Membranes are then washed twice with PBS <NUM> % Tween <NUM> and then once with PBS to remove all residual stain prior to blocking.

Rather than assessing protein levels by western blot, an ELISA may be used. To do this, a sample to be studied is first diluted in coating buffer (cat. <NUM> Thermofisher). Typically, samples are coated onto the plates at different concentrations such as <NUM>:<NUM>; <NUM>:<NUM>; <NUM>:<NUM> to determine optimal detection range. A standard curve is created by using a pre-made quantity of the protein to be detected and coating wells the highest standard point of 4µg/ml by dilution followed by <NUM>-fold serial dilution into adjacent wells. For example, a standard protein at <NUM>/ml requires 4µl with 196µl of non-transfected culture media and <NUM> of coating buffer. This is used to generate an <NUM>-point standard curve by performing <NUM>-fold serial dilution by adding <NUM> of reconstituted standard and <NUM> of coating buffer in <NUM> tubes. <NUM> microliters of each standard is then added in duplicate to the ELISA plate. <NUM> microlitres of each sample is added to a well of the immuno-microplate. <NUM> microlitres of coating buffer is added to one well as a no-antigen control. <NUM> microlitres of a positive control sample is included, if available. The plate is incubated at <NUM> degrees Celsius overnight. The plate is washed with PBS-T (<NUM>% Tween) three times. 200µL of blocking buffer is added (the original coating buffer with <NUM>% BSA) per well and the plate is incubated at <NUM> for 1hr. The plate is washed with PBS-T (<NUM>% tween) three times). The Primary antibody (<NUM>#) is added to the diluent solution at the required dilution and <NUM>µL is added to each well. The plate is incubated at room temperature for <NUM>-<NUM> hours. The plate is washed with PBS-T (<NUM>% tween) three times. A HRP-labelled secondary antibody is added to the diluent solution at the required dilution. <NUM> microlitres is added to each well. The plate is incubated at room temperature for <NUM> hour. The plate is washed with PBS-T (<NUM>% tween) three times. The plate is washed with PBS once. <NUM> microlitres of <NUM>,<NUM>' <NUM>,<NUM>'-Tetramethylbenzidine (TMB) is added to each well. It is then necessary to wait for the colour to develop and to record the time taken. <NUM> microlitres of the stop solution (<NUM> HCl) is added. Data acquisition is achieved by reading the plates absorbance in a plate reader at <NUM>.

The levels of VLP production from a cell Transgene expression level or the level of expression of late proteins are measured via Western blot or ELISA as described above but using antibodies recognising an epitope on the VLP surface.

Five expression constructs were created wherein the GFP reporter gene was transcribed by the wildtype Ad5 MLP (pMLPwt-GFP), repressor mutant MLPs (pMLP-TET01a-GFP; pMLP-TET01b-GFP; pMLP-TET02-GFP) or the control construct in which no internal promoter was present (pMCS-GFP) for determining low level baseline transcription. The vectors are shown in <FIG>.

Five expression constructs were created wherein the GFP reporter gene was transcribed by the wildtype Ad5 MLP (pMLPwt-GFP), repressor mutant MLPs (pMLP-TET01a-GFP; pMLP-TET01b-GFP; pMLP-TET02-GFP) or the control construct in which no internal promoter was present (pMCS-GFP) for determining low level baseline transcription. HEK293 cells were seeded in tissue culture treated <NUM>-well plates at a density of 3e4 cells/well, <NUM>-hours before transfection. HEK293 cells were transfected with the plasmids pMLPwt-GFP; pMLP-TET01a-GFP; pMLP-TET01 b-GFP; pMLP-TET02-GFP; pMCS-GFP using branched PEI (25kDA) at a <NUM>:<NUM> ratio of total DNA mass to PE!. Transfection was carried out in triplicates and cells were harvested at <NUM> hours, <NUM> hours and <NUM> hours post transfection for analysis by flow cytometry. Data is presented in <FIG> as MFI (mean fluorescent intensity) of GFP positive cells. Error bars indicate SD of triple biological replicates. Data NS p><NUM> by Student's t-test.

Five expression constructs were created wherein the GFP reporter gene was transcribed by the wildtype Ad5 MLP (pMLPwt-GFP), repressor mutant MLP (pMLP-TET01a-GFP; pMLP-TET01b-GFP; pMLP-TET02-GFP) or the control construct in which no internal promoter was present (pMCS-GFP) for determining low level baseline transcription. Wildtype Ad5 MLP (pMLPwt-GFP), repressor mutant MLP (pMLP-TET01a-GFP; pMLP-TET01b-GFP; pMLP-TET02-GFP) or the control construct expressing the GFP reporter was co-transfected with a TETR expression plasmid (pTETR), under the control of the constitutive CMV (cytomegalovirus) promoter, at a <NUM>:<NUM> ratio of total DNA mass, in HEK293 cells treated with doxycycline <NUM>. 2µg/ml or DMSO. HEK293 cells were seeded in tissue culture treated <NUM>-well plates at a density of 3e4 cells/well, <NUM>-hours before transfection. Transfection was carried out in triplicates using branched PEI (25kDA) at a <NUM>:<NUM> ratio of total DNA mass to PE! and cells were analysed by flow cytometry at <NUM>, <NUM> and <NUM> hours post transfection. Data is presented in <FIG> as percentage repression of MFI (mean fluorescent intensity) in GFP positive cells compared against the activity of the Ad5 MLP wildtype (pMLPwt-GFP) and normalised against the promoterless control construct for background expression signal. Data as mean ± SD NS p><NUM>; *p≤<NUM>; **p≤<NUM>; ***p≤ <NUM>; ****P≤<NUM>; unpaired, two tailed Student's.

Adenoviruses engineered by molecular cloning methods to incorporate the repressor sequences were recovered in HEK293 cells. Ad5 genome with the MLP repressor sequence MLP-TET01a, MLP-TET01b, TET02 or wild-type MLP were excised away from bacterial plasmid DNA by restriction digest with Swal restriction enzymes to release the <NUM>' and <NUM>' flanking Ad5 ITR sequences. HEK293 cells were seeded in <NUM>-cm tissue culture plates at a density of 1e5 cells/plate for <NUM>-hours and transfected with 10µg of DNA containing MLP repressor Ad5 or Ad5 MLPwt genomes, using lipofectamine <NUM> at a <NUM>:<NUM> ratio of total DNA mass to lipofectamine <NUM>. Viruses were harvested following observation of viral infection and cytoplasmic effect, typically, <NUM>-<NUM> days post transfection. <NUM> T-Rex Flp cells were seeded in <NUM>-well tissue culture treated plates at a density of 4e4 cells/well for <NUM>-hours and transduced with adenoviruses Ad5-MLP-TET01a, Ad5-MLP-TET01b, Ad5-MLP-TET02 or standard E1-E3 deleted Ad5 (Ad5-MLPwt) in the presence of doxycycline <NUM>. 2µg/ml or DMSO and imaged by light miscopy <NUM>-days post infection. Data shown in <FIG> is representative of triplicate biological replicates. Bar = <NUM>.

Adenoviruses engineered by molecular cloning methods to incorporate the repressor sequences MLP-TET01b were recovered in HEK293 cells. Ad5 genome with the MLP repressor sequence MLP-TET01b were excised away from bacterial plasmid DNA by restriction digest with Swal restriction enzymes to release the <NUM>' and <NUM>' flanking Ad5 ITR sequences. HEK293 cells were seeded in <NUM>-cm tissue culture plates at a density of 1e5 cells/plate for <NUM>-hours and transfected with 10ug of DNA containing MLP repressor Ad5, using lipofectamine <NUM> at a <NUM>:<NUM> ratio of total DNA mass to lipofectamine <NUM>. Viruses were harvested following observation of viral infection and cytoplasmic effect, typically, <NUM>-<NUM> days post transfection. HEK293 cells were seeded in <NUM>-cm tissue culture plates were transfected with pTETR (5µg) or stuffer DNA, using lipofectamine <NUM> at a <NUM>:<NUM> ratio of total DNA mass to lipofectamine <NUM>, prior to infection with adenoviruses Ad5-MLP-TET01b. The results are shown in <FIG>. Data imaged by light microscopy <NUM>, <NUM>, <NUM> and <NUM> hours post-infection.

Adenoviruses engineered by molecular cloning methods to incorporate the repressor sequences were recovered in HEK293 cells. Ad5 genome with the MLP repressor sequence MLP-TET01a, MLP-TET01b, TET02 or wildtype MLP were excised away from bacterial plasmid DNA by restriction digest with Swal restriction enzymes to release the <NUM>' and <NUM>' flanking Ad5 ITR sequences. <NUM> T-Rex Flp cells were seeded in <NUM>-cm tissue culture plates at a density of 1e5 cells/plate for <NUM>-hours and transfected with 10µg of DNA containing MLP repressor Ad5 or Ad5 MLPwt genomes, using lipofectamine <NUM> at a <NUM>:<NUM> ratio of total DNA mass to lipofectamine <NUM>. Viruses were harvested following observation of viral infection and cytoplasmic effect, typically <NUM>-<NUM> days post transfection. <NUM> T-Rex Flp cells were seeded in <NUM>-well tissue culture treated plates at a density of 4e4 cells/well for <NUM>-hours and transduced with adenoviruses Ad5-MLP-TET01a, Ad5-MLP-TET01b, Ad5-MLP-TET02 or standard E1-E3 deleted Ad5 (Ad5-MLPwt) in the presence of doxycycline <NUM>. 2ug/ml or DMSO <NUM> T-Rex Flp cells were infected with MLP mutant or MLP-wt Ad5 in the presence of doxycycline or DMSO. Total viral and cellular DNA was harvested <NUM>-days post infection. Viral genome copy was quantified by QPCR using TaqMan® probes. Ad5 of known titres were used for generating the standard curve and data is presented (<FIG>) as increase in genome copy above the initial viral load used for infection. Data representative of triplicate biological replicates and presented as mean ± SEM **P≤<NUM>; unpaired, two tailed Student's.

To determine the effect of MLP repression on inhibiting adenovirus production and virus spreading, adenovirus with wild-type MLP or TET01b modification was engineered to express the EGFP reporter, with and without Ad5 TPL fused to the EGFP initiation codon. EGFP reporter was expressed from the virus E1 deleted region and under control of the CMV promoter. Adenoviruses expressing EGFP were used to infect a monolayer of Flp-In T-REx <NUM> cells treated with doxycycline or DMSO at MOI <NUM> and EGFP expression was monitored at <NUM>-days by fluorescence microscopy and flow cytometry. While viral spreading i. e EGFP expression across the cell monolayer was not inhibited in the control adenovirus with wild-type MLP, virus spreading of adenoviruses with MLP TET01b was blocked in Flp-In T-REx <NUM> cells in the absence of doxycycline, indicating repression of virion replication (<FIG>).

Following <NUM>-days post infection, cells were harvested for flow cytometry to determine the relative proportion of EGFP expressing cells within the gated population. In line with results from fluorescent microscopy, the proportion of cells expressing EGFP was comparable in Flp-In T-REx <NUM> cells treated with doxycycline or DMSO following infection with the control adenovirus (<FIG>). However, whilst the population of EGFP positive cells were lower from infection with MLP TET01b modified adenoviruses in cells treated with doxycycline compared to the control virus, presumably due to variation in infectivity and replication, cells treated with DMSO showed a significantly lower popular of EGFP expressing cells, indicating that EGFP is only expressed from cells transduced by viruses from the first-round infection.

To determine whether fusion of Ad5 TPL exons to the initiation codon of EGFP affected gene expression, plasmids engineered to expression EGFP, with and without the leader sequence, under the control of the CMV promoter were transfected into HEK293 cells and EGFP expression determined by flow cytometry at <NUM> hours post-transfection. The results are shown in <FIG>. Whilst the promoter-less control plasmid showed background levels of EGFP, there were no significant differences in the levels of EGFP expression from plasmid containing the TPL sequence.

To assess whether protein expression is increased following MLP repression, MLP TET01b modified adenoviruses expressing the EGFP reporter from the CMV promoter, with and without Ad5 TPL, were infected into Flp-In T-REx <NUM> cells treated with doxycycline or DMSO at an MOI <NUM>, and EGFP expression was measured by flow cytometry <NUM>, <NUM> and <NUM>-hours post-infection. The results are shown in <FIG>. While MLP TET01b adenovirus expressing EGFP containing the TPL showed an increase in median fluorescence intensity (MFI) compared EGFP lacking the TPL sequence, repression of the adenovirus MLP from infection in the DMSO treated cells resulted in a further ~<NUM>-fold increase in EGFP expression compared to virus infection into cells treated with doxycycline, which enables virion production.

Similarly, a ~<NUM>-fold increase in EGFP expression was observed in HEK293 cells when adenovirus MLP was repressed by transient expression of the repressor TETR (see <FIG>). Plasmid expressing TETR from the CMV promoter was transfected into HEK293 cells treated with doxycycline or DMSO. Subsequently, cells were infected with adenovirus containing MLP TET01b modification and expressing EGFP (with and without the TPL exons) from the CMV promoter or transfected using Lipofectamine with a CMV expression plasmid that transcribed EGFP. EGFP expression was determined by flow cytometry <NUM>-hours post transduction with the virus and plasmid. Results showed comparable levels of EGFP expression, as determined by MFI, from HEK293 cells transduced with the EGFP expressing adenoviruses or plasmid DNA. However, -<NUM>-fold increase in EGFP expression was only observed from infection with the MLP TET01b modified adenovirus expression EGFP with the TPL exons in cells treated with DMSO, which allowed repression of Ad MLP TET01b by TETR, indicating enhance protein production by cap-independent translation as this effect was not observed in the EGFP coding sequence without the TPL exons.

Adenoviruses with MLP TET01b modification was further engineered to express the repressor TETR from a splice acceptor sequence under direct control of the virus internal MLP, position at the E3-deleted region of the virus, to construct TERA. The results are shown in <FIG>.

To assess repression of viral structural proteins from TERA, control adenovirus E1/E3 deleted or TERA was used for infection of HEK293 cells in the presence of doxycycline or DMSO, at an MOI <NUM> or <NUM>. Adenovirus capsid proteins from cellular lysate and growth medium were probed using anti-Ad5 antibodies by Western blot <NUM>-hours post infection. Comparable levels of adenovirus structural proteins were detected from TERA and the control virus when doxycycline was present in the growth medium, from both cell lysates and culture media. However, in the treated DMSO group, structural proteins from TERA were undetectable from the blot. Presumably, in the absence of doxycycline, TERA infection into HEK293 cells enabled production of viral MLP transcribed TETR to self-repression of its own MLP and a blockade in the production of capsid proteins.

In a doxycycline dose-escalation study to assess production of TERA in HEK293 cells, control adenovirus with the wildtype MLP or TERA was used for infection of HEK293 cells at MOI <NUM> and <NUM>, treated with DMSO or doxycycline dose of <NUM>, <NUM>, <NUM> and <NUM>µg/mL. The results are shown in <FIG>. Comparable levels of Ad5 major structural proteins were detected for the control adenovirus infection in cells treated with DMSO or doxycycline, while capsid proteins expressed from TERA increased with increasing with increasing doses of doxycycline up to <NUM>µg/mL, consistent for both MOI assessed.

To assess virus replication of TERA, control E1/E3 deleted adenovirus or TERA was used to infect a monolayer of HEK293 cells at MOI <NUM>, <NUM> and <NUM>, in the presence of doxycycline, and total genomic DNA was extracted from growth media and cellular lysate at time-point <NUM>, <NUM>, <NUM> and <NUM>-hours post viral infection. Abundance of adenovirus genomic DNA was determined by QPCR. The results are shown in <FIG>.

For all three infection MOI assessed, virus replication of TERA was comparable to the control adenovirus, where the relative abundance of viral genome increased sharply at <NUM>, with ><NUM>-log increases in total viral genomes at <NUM> post-infection.

Genome replication of TERA during MLP repression was further assessed by QPCR. The virus TERA or control E1/E3 deleted adenovirus was used for infecting HEK293 cells in the presence of doxycycline or DMSO at an MOI of <NUM> and <NUM> and total genomic DNA was harvested at time-point <NUM>, <NUM>, <NUM>, <NUM>, and <NUM>-hours post infection viral genome quantification by QPCR. Similarly, while virus replication of TERA was comparable to the control virus, DNA replication from TERA significantly increased after <NUM>-hours post infection in HEK293 cells treated with the DMSO control group compared to infection into cells cultured with doxycycline. Presumably, repression of the virus MLP inhibited TERA from completion of its replicative life-cycle, thereby enabling exponential viral genome amplification.

To assess EGFP reporter expression from TERA under control of the CMV promoter, TERA engineered to express EGFP, with and without the Ad5 TPL exons, were used to infect HEK293 cells and EGFP expression is compared to expression from E1/E3 control adenovirus and method of transient transfection with a CMV expression plasmid.

While E1/E3 adenovirus and TERA exhibited increase EGFP expression compared to expression from a CMV plasmid vector, TERA expressing EGFP containing Ad5 TPL exons enhanced production above levels observed from both E1/E3 control vector and TERA without the TPL exons. Presumably, self-repression of TERA MLP by the virally encoded TETR resulted in repression of Ad5 late mRNA transcripts and enabling cap-independent translation of the prevailing TPL EGFP mRNAs.

Additionally, Western blot confirmed that EGFP expression using the control E1/E3 adenovirus and TERA, in the presence of doxycycline, was accompanied with contaminating adenovirus proteins. In contrast, the absence of doxycycline enabled repression of Ad5 structural proteins in TERA while EGFP expression was maintained.

To compare production of a model secretory protein using TERA against a method of transient expression from plasmid DNA, TERA and plasmid vector (pCMV-BiTE) were engineered to express a Bi-Specific T-Cell Engager (BiTE) against tumour specific antigen EpCAM under the control of the CMV promoter. The results are shown in <FIG>.

Virus TERA expressing BiTE containing the Ad5 TPL exons or plasmid pCMV-BiTE was used to transduce HEK293 cells at MOI <NUM> or <NUM>. 75µg DNA per well, respectively, and protein harvested from growth media at time-point <NUM>, <NUM> and <NUM>-hours post-transduction and probed using anti-6x His antibodies. Western blot showed significant increase in BiTE expressing from TERA compared to production from using the CMV expression plasmid in all three time-point of harvest.

<FIG> shows Western blot detection of BiTE protein expressed from TERA compared to E1/E3 deleted adenovirus. HEK293 cells, cultured in the absence of doxycycline, were infected with adenoviruses E1/E3-deleted or TERA-expressing BiTE under control of the CMV promoter (with and without Ad5 TPL exons) at MOI <NUM> and BiTE protein expression was measured at <NUM>-hours post-infection from growth medium. TERA exhibited increase production of BiTE compared to control adenovirus; however, ~<NUM>-fold increase in BiTE production was observed from infection with TERA expressing BiTE containing the Ad5 TPL exons. Additionally, while viral structural proteins were detected from infection with the E1/E3 deleted virus control, virus capsid proteins were undetectable following infection by TERA. Amplification of the viral genomic DNA was confirmed to be maintained and comparable to the control virus by QPCR analysis.

To evaluate the use of TERA for delivery of helper-functions and rAAV DNA for the production rAAV viral vectors, E1/E3 deleted control adenovirus and TERA was modified in the virus E1 deleted region to encode an rAAV genome, AAV2 ITRs flanking an EGFP expression cassette under control of the CMV promoter. The results are shown in <FIG>.

rAAV encoding EGFP transgene was produced by an established Helper-free triple transfection method, or via infection with control E1/E3 deleted adenovirus or TERA. HEK293 cells were triple-transfected with plasmid encoding <NUM>) rAAV genome encoding EGFP, <NUM>) AAV2 Rep and Cap, and <NUM>) Ad5 Helper, or transduced with plasmid encoding AAV2 Rep and Cap, and control E1/E3 deleted adenovirus or TERA, in the presence of doxycycline or DMSO. Recombinant viruses were harvested from cellular lysates and growth media <NUM>-hours post transduction and viral genomes, from encapsulated adenovirus and rAAV, were quantified by QPCR using primer and probe sets directed against adenovirus DNA encoding Fibre, or CMV promoter encoded by both rAAV and adenoviruses.

<FIG> shows quantification of encapsulated adenovirus genomes from cellular lysate and growth medium. While significant levels of adenoviruses were detected following infection with the control adenovirus and TERA in HEK293 cells treated with DMSO and doxycycline, respectively, presence of adenoviruses were below the lowest standard and detection range of the assay from HEK293 cells, absent of doxycycline, when transduced with TERA or Helper-free production method. In contrast, significant levels of recombinant viruses from all samples were detected by QPCR assay using primer and probe sets directed against the encoded CMV promoter, present in both adenoviruses and rAAVs (<FIG>).

Since virus quantification used QPCR primers and probe directed against the encoded CMV promoter detected both rAAV and the adenoviral delivery vectors, total rAAV from each production method and conditions were determined by subtraction of overall adenovirus particles contamination detected (<FIG>). E1/E3 deleted adenovirus produced rAAV that were comparable or above the Helper-free production system by triple transfection, which was also accompanied with significant levels of adenovirus contamination. In contrast, HEK293 cells infected with TERA-AAV, in the absence of doxycycline, yielded -<NUM>-fold increase in rAAV compared to Helper-free plasmid transfections with adenovirus contamination beyond the limit of the QPCR detection. (<FIG>) Adenovirus particles contamination in growth medium was further confirmed by Western blot using antibodies directed against Ad5 capsid protein. In line with results from QPCR analysis, adenovirus structural proteins were undetectable from Helper-free production method or infection with TERA (MOI <NUM> and <NUM>) in HEK293 cells absent of doxycycline, while adenovirus proteins were readily detected from TERA infection in the presence of doxycycline, enabling active MLP, and from the E1/E3 control virus.

To determine rAAV particles with an encapsulated rAAV genome, rAAV capsids produced from methods of Helper-free plasmid transfection, or via TERA infection into plasmid Rep and Cap transfected HEK293 cells, were quantified. <FIG> shows total rAAV2 capsids and DNase-I resistant genome encapsulated particles determined by ELISA directed toward formed-AAV2 viral capsids and quantification of rAAV genome by QPCR, respectively. <FIG> shows per cell basis, TERA MOI <NUM> infection produced significantly higher amounts of rAAV2 capsids and DNase-I resistant genome encapsulated rAAVs, compared to Helper-free production method. Overall, Helper-free rAAV2 production and TERA produced genome encapsulated particles accounting to ~<NUM>% and -<NUM>% of total rAAV2 capsid particles, respectively.

Claim 1:
An adenoviral vector comprising a repressible Major Late Promoter (MLP) and a plurality of adenoviral late genes, wherein the MLP comprises one or more repressor elements which are capable of regulating or controlling transcription of the adenoviral late genes, wherein the one or more repressor elements are inserted between the MLP TATA box and the +<NUM> position of transcription, and wherein the one or more repressor elements are ones which are capable of being bound by a repressor protein and wherein the repressor protein is the tetracycline repressor, the lactose repressor, the ecdysone repressor, rat glucocorticoid receptor or human estrogen receptor.