Substances causing differentiation
A DNA construct is described which contains a fusion gene under the control of a promoter. The fusion gene comprises at least one resistance gene and at least one reporter gene and is slightly toxic to a host cell transfected with that DNA construct. That DNA construct can be encoded on a plasmid or a virus. Further, a method is described for using the DNA construct to identify substances that may cause a differentiation in eukaryotic cells.
This application is a continuation of U.S. application Ser. No. 10/431,705, filed May 8, 2003, which is continuation of International Patent Application PCT/EP01/12660 filed on Oct. 31, 2001, designating the US, and published in German, which claims priority of German patent application DE 100 56 059.8 filed on Nov. 11, 2000, all which are incorporated herein by reference in their entireties.
BACKGROUND OF THE INVENTION1. Field of the Invention
The present invention relates to a method for identifying substances causing differentiation in eukaryotic cells, to DNA constructs, plasmids, viruses and cell lines used in said method, and to a method of preparing a pharmaceutical composition.
2. Description of the Related Art
Differentiation of cells from stem cells is a general biological phenomenon during embryonic development, but also plays a very large part in regeneration processes in the adult organism (e.g., skin regeneration, formation of blood, regeneration of intestinal epithelia, liver regeneration after poisoning or alcohol abuse, etc.). As in all important biological processes, disruptions may cause chronic diseases or may be lethal.
During tumorigenesis, there is very frequently, if not always, a “back”-differentiation of cells, i.e. cells revert to an undifferentiated, embryonic state. Despite great improvements in the methods for early diagnosis and therapy of tumor diseases, mortality is still very high and affected patients suffer immensely. Therefore, finding and developing novel and more effective cancer medicaments (cytostatics) is of extraordinary importance for health policy and have, from the perspective of the pharmaceutical industry, a very large growth potential on the drugs market.
Since many genetic modifications occur on the path from a normal healthy cell to a tumor cell, there are in principle also many possibilities of interfering with the metabolism of tumor cells and thus preventing growth and dissemination. Thus, the largest class of cytostatics leads to damage of cellular DNA. After cell division, this causes lethal mutations, or the cell dies as a direct result of the triggering of the so-called programmed cell death (apoptosis). This affects all rapidly growing cells, i.e. not only tumor cells but also healthy growing cells.
Another class of cytostatics is that of the antimetabolites which halt the metabolism of rapidly growing cells. A third class of cytostatics damages the so-called spindle fiber apparatus of dividing cells, thereby inhibiting cell division or killing the cells directly. A fourth and relatively new class is that of anti-angiogenetic substances which interfere with the ability of tumor cells to induce new blood vessels for their own supply.
A relatively new class of cytostatics, which is relevant in context with the present invention, interferes with the expression pattern of genes which have been partly switched off during tumorigenesis. These are frequently so-called tumor suppressor genes and differentiation genes. The renewed induction and expression of said genes usually leads to a loss of growth advantages of a cancer cell and may also make it easier for the immune system to attack said cell.
The fact that such differentiation-causing substances interfere with the state of methylation of so-called “CpG is-lands” has been known for a long time. CpG islands are found particularly frequently in the 5′-regulatory sequences of genes and play an important part in genomic imprinting, i.e. in regulating paternal versus maternal gene expression. It is possible to switch off genes by methylating the CpG islands present in promoters. If the DNA methylase mainly responsible for methylation is inactive, lethal disruptions in development occur, as can be shown in a knockout model in mice.
It is therefore assumed nowadays that there is a genetically controlled equilibrium of methylation and demethylation in embryogenesis. A disruption of this equilibrium is often present in tumor cells. Thus, it has been found that it is possible to switch off promoters of tumor suppressor genes by methylation of the CpG islands, which is why, for example, the hypomethylation-inducing substance 5′-azacytidine (Aza) acts as a potent cytostatic agent in many types of tumor.
Another mechanism important for differentiation is the influence of histone acetylation. Histones are DNA-binding proteins which can regulate chromatin structure and also influence gene expression. This takes place preferably via biochemical modifications of said histones, for example by acetylation or phosphorylation. Thus, the substance trichostatin A (TSA) is known as a specific inhibitor of histone deacetylase. Recently, it was shown that deacylation of histone H4 leads to chromatin condensation and thereby can suppress gene expression. Accordingly, inhibition of histone deacetylase by TSA leads to chromatin decondensation and can thereby remove suppression of gene expression.
It must be assumed that there are still many other, as yet unknown mechanisms which can be used by tumor cells to switch off expression of differentiation genes and tumor suppressor genes dangerous to them.
While for some classes of cytostatics there are already very good assay systems which also can be used to identify novel compounds, there is, however, a lack of methods for identifying, as mentioned above, such substances capable of causing differentiation. However, this novel class of cytostatics is particularly interesting, because it has great potential for controlling tumors and is associated with substantially fewer side effects than the traditional cytostatics.
The following widespread in vitro test systems are available for identifying substances which cause DNA damage and could therefore potentially be used as cytostatics: the Ames test, or else Salmonella typhimurium test (STY), is based on the mutagenicity of substances in bacteria, while the SOS-Chromotest is based on inducing the bacterial SOS system by genotoxic agents. Both tests have comparable sensitivities, but have the fundamental disadvantage that genotoxic action of substances can vary in bacteria and higher organisms.
For this reason, the Micronucleus test, the single cell gel test (SCG test), also known as comet assay, and the test for sister chromosome exchange (SCE test), which are based on eukaryotic cell systems, have been developed. In the literature, a cell line, A4/4, which contains a lacZ gene under the control of the heavy metal-inducible metallothionein promoter has been described. The authors report that the promoter is switched off during cultivation but can be induced again by the demethylating substance 5′-azacytidine (Biard et al. 1992 Cancer Res 52:5213-5218).
The previously known assay systems for identifying DNA-damaging agents, however, are not suited to identify substances causing differentiation, since the mechanism is completely different.
The reporter cell line described by Biard et al. has the decisive disadvantage of being an inducible system. The demethylating action of substances can be visualized only if the inducer for the promoter is used at the same time. The authors have chosen the metallothionein promoter which is induced by heavy metals such as cadmium and zinc. There are hundreds of indications in the literature for heavy metals themselves inducing gene expression. As a result, the gene expression-causing action of the heavy metals required for the system superimposes the demethylating action of some substances, i.e. unspecific, false negative or false positive results are very easily possible. The cell line was prepared for the purpose of being able to find demethylating substances. These substances may cause differentiation but are, as explained above, not the only substances capable thereof. Since there are, after 1992, no further publications regarding this cell line, it is neither known whether this cell line is stable nor whether it is suitable for detecting other differentiation processes as well.
SUMMARY OF THE INVENTIONIn view of the above, it is an object of the present invention to provide a method of the type mentioned at the beginning, which can be used to identify in a rapid, simple and reliable manner substances causing differentiation, and auxiliary substances which can be used in said method.
This object is achieved by a DNA construct which comprises a fusion gene under the control of a promoter, wherein said fusion gene comprises at least one resistance gene and at least one reporter gene and is slightly toxic to a host cell transfected with said DNA construct so that said promoter is switched off when expression of the resistance gene is not required for growth of the transfected host cells, since, for example, the nutrient medium lacks the appropriate antibiotic.
Further objects of the invention are a plasmid having such a DNA construct, a virus having an expression cassette containing said DNA construct or coding therefor, i.e. a DNA virus or a retrovirus, and a eukaryotic cell, in particular human cell, which is stably transfected with said plasmid or infected with said virus, in particular the cell line U87-HGFP which was deposited in accordance with the Budapest Treaty at the DSMZ in Braunschweig, Germany, under deposition number DSMZ ACC 2473 on Nov. 9, 2000, and a method of using said DNA construct and/or said plasmid and/or said virus and/or said cell for identifying substances which cause differentiation in eukaryotic cells.
A further object is a method for identifying substances which are capable of causing differentiation in eukaryotic cells, comprising the steps:
a) incubating the novel cells in a culture medium containing a selection substance corresponding to the resistance gene,
b) inoculating a culture medium lacking said selection sub-stance with the incubated cells from step a) and incubating the inoculated cells for approx. 5 to approx. 100, preferably approx. 24, hours,
c) adding a substance to be identified to said culture medium of the cells from step b) and incubating further for approx. 1 to approx. 5, preferably approx. 2, days, and
d) checking the incubated cells from step c) for increased reporter gene expression compared to cells from step b).
The present invention completely solves the problem of identifying substances causing differentiation.
In this connection, preference is given to selecting the promoter from CMV promoter, RSV promoter, cellular promoters of tumor suppressor genes and promoters of differentiation genes, to selecting the reporter gene from GFP, LacZ, luciferase, to selecting the resistance gene from hygromycin gene, neomycin gene, puromycin gene, and/or to the fusion gene containing at least one gene coding for a polypeptide capable of developing an action toxic to the host cell, such as, for example, GFP, which itself is slightly toxic or cytosine deaminase or thymidine kinase which convert the prodrugs 5′-fluorocytosine and ganciclovir, respectively, into toxic substances.
The cell line also includes a fusion gene under the control of the human cytomegalovirus promoter (CMV promoter). This promoter is usually extremely strong in cells and therefore need not be induced, in contrast to the metallothionein promoter of the prior art. Moreover, it is known that the promoter can be switched off under certain conditions, in particular in vivo.
The fusion gene here consists of the resistance gene for the antibiotic hygromycin (hygro) and green fluorescent protein (GFP). Transfection of the glioblastoma cell line U87 with this construct generated the cell line U87-HGFP, after selection using the antibiotic hygromycin. This cell line expresses the fusion gene in the presence of the antibiotic, this being very clearly visible in fluorescence microscopy on the basis of GFP fluorescence. If the antibiotic is removed for just a few days, the cell downregulates the CMV promoter, since the fusion protein is slightly toxic to the cells. As the inventors observed, the said fusion protein accumulates in particular cell compartments (probably the ER). Treating said cells with the differentiation-causing substances 5′-azacytidine and/or trichostatin A at very low concentrations results in very strong upregulation of the CMV promoter, visible due to increased GFP fluorescence, within just two days.
Up until now, no cell line has been described or known in which substances causing differentiation can be detected using an expression unit consisting of CMV promoter and hygromycin-GFP fusion. The system is very reliable, with the presence of hygromycin during routine cultivation of the cell line preventing the loss of said expression unit. The cell line has the intrinsic capability of virtually completely downregulating the CMV promoter only a few days after removing hygromycin. The promoter is upregulated again when adding substances causing differentiation.
The advantage compared to the known system is, inter alia, the use of a fusion gene which combines a plurality of proper-ties: (I) positive selectability by the hygromycin gene, i.e. the expression unit is retained in a stable manner when adding the antibiotic; (II) negative selectability, i.e. in the absence of hygromycin B the toxic effect of the GFP gene selects for cells in which the promoter is switched off; (III) identifiability due to intrinsic fluorescence of GFP. These properties render the system very stable and reliable.
The system needs no inducer except the differentiation substance to be tested and is therefore unaffected by disruptions or superpositions by an inducer.
The system has proved to be capable of finding not only demethylation but also histone acetylation.
Using the GFP as reporter, it is possible to observe the promoter activity, and thus the action of substances causing differentiation, both in living cells and in fixed cells (fluorescence microscopy) and to quantify it exactly and reproducibly by means of flow cytometry.
According to another object, it is also possible in the novel method to use other reporter expression units consisting of a promoter (CMV promoter, RSV promoter, cellular promoters of tumor suppressor genes or differentiation genes), a selection marker (hygromycin gene, neomycin gene, puromycin gene, etc.) fused to a reporter (GFP, LacZ, luciferase), and a “toxic” gene (e.g. GFP, cytosine deaminase, HSV thymidine kinase).
Cytosine deaminase or thymidine kinase would then additionally need toxic but not lethal concentrations of the pro-drugs 5′-fluorocytosine and ganciclovir, respectively. This would select for cells which down-regulate the promoter.
These constructs may also be transfected in cell lines other than U87, or the studies may also be carried out in vivo, i.e. on transgenic animals.
The cell line U87-HGFP, which is still a further object of the invention, has a particular advantage in that the promoter can be switched off within a short time and reliably. Furthermore, the method can be automated, making it possible to screen many substances in a short time.
The cell line has the further advantage of being a tumor cell line so that the substances are searched for in a cancer cell which is thus not only a model system but also, at the same time, a test system. Another advantage is the fact that these cells differentiate with addition of the appropriate substances, and this can be seen due to the change in morphology.
A substance identified in this way is thus not only capable of reactivating a downregulated promoter but can also force a cancer cell to differentiate and is thus a potential cytostatic.
Against this background as another object, the invention also relates to a method of using a substance identified by the novel method for preparing a pharmaceutical composition for treating malignant and benign tumor diseases, and to a method for preparing a pharmaceutical composition, which comprises the novel method and mixing the identified substance with a pharmaceutically acceptable carrier.
Further advantages arise from the description and the attached drawings.
It is obvious that the features mentioned above and still to be illustrated below can be used not only in the combinations indicated in each case but also in other combinations or on their own, without leaving the scope of the present invention.
BRIEF DESCRIPTION OF THE DRAWINGS
[I and IV] show dot plots referred to DNA staining of treated and untreated cells. In order to exactly define a population of (2N+4N) nuclei, a region (R1) was utilized. [II and V] show dot plots referred to BrdU incorporation into DNA. The values 200 and 400 on the linear scale of FL3-A fluorescence correspond to the amount of 2N and 4N DNA in the nuclei. All events shown correspond to the R1 region. [III and VI] show an isotype control for establishing the quadrants for the dot plots of BrdU incorporation. The anti-isotype antibody represents nonspecific binding and was used as a negative control for the anti-BrdU antibody. The percentages of cells in different phases of the cell cycle were determined using the dot plots of BrdU incorporation (in quadrant: bottom left region=G1−G0; bottom right region=G2; top left region=S; top right region=M).
1) Cloning of pCMV-HygroEGFP
Intermediate Plasmid 1 Called pScriptpolyA (3595 bp).
Starting plasmid pCRScript SK(+) AmpR+ cut with EcoRV and HindIII, and subsequent ligation with SmaI/HindIII fragment which contains a 625 bp HSV thymidine kinase polyadenylation signal from pTKneo (blunt end ligation).
Intermediate 2: pCMVA (4260 bp).
Insertion of a 670 bp hCMV promoter fragment from pL15Tk [cut with PstI, blunt-ended using T4 DNA polymerase] into intermediate 1, pScriptpolyA, cut with SrfI (blunt end ligation).
Intermediate 3: pCMV-EGFP (4975 bp).
Ligating of the EGFP reading frame from plasmid pEGFP (Clontech) cut with BamHI/NotI (end filled in using Klenow polymerase) into vector pCMVA opened with PstI (intermediate 2, blunt-ended using T4 DNA polymerase) (blunt end ligation).
Final pCMV-HygroEGFP (6052 bp).
Ligation of a 1026 bp PCR fragment containing the open reading frame of the hygromycin resistance gene from pTkHygro (Stopcodon removed by said PCR) into AgeI-opened vector pCMV-EGFP (blunt-ended by filling in ends using Klenow polymerase) (blunt end ligation).
The plasmid is depicted in
2) Materials and Methods
Cell Lines
U87H-GFP is a cell line derived from the human glioblastoma cell line U87 after stable transfection with plasmid pCMV-hygroEGFP. This plasmid which is integrated into the genomic DNA is derived from PCR-Script™ (Stratagene) and carries a fusion gene downstream of the human CMV promoter. This fusion gene contains the gene for resistance to hygromycin, which is linked to the gene coding for the enhanced green fluorescent protein (EGFP). The resulting gene (called H-GFP) codes for a protein which imparts resistance to hygromycin B and which can be readily detected by fluorescence microscopy and flow cytometry analysis. In contrast, the parent cell line U87 does not contain any plasmid and can be used as a negative control.
U87H-GFP and the parent line U87 were cultured in Dulbecco's Modified Eagle's Medium, (D-MEM, low glucose, Gibco, BRL) supplemented with 10% fetal calf serum (Seromed), 100 units/ml penicillin, 100 μg/ml streptomycin and 1 μg/ml amphotericine B (Gibco, BRL) at 37° C. in a humidified atmosphere containing 5% CO2. For the U87H-GFP cell line, the culture medium was supplemented with 600 units/ml hygromycin B (Calbiochem).
U87H-GFP and the parent cells were seeded at 1-2×105 cells/well on 6-well plates (Nuclon, NUNC), using D-MEM without hygromycin B, and incubated for adhesion for 24 h. This was followed by adding 5-azacytidine and trichostatin A (Sigma Chemicals, Co.) at different final concentrations (2.5-5-10-20-40 μM for Aza; from 10 nM to 3 μM for TSA) to the culture medium. After two days of treatment, fluorescence microscopy and flow cytometry analyses were carried out.
Fluorescence Microscopy
Approximately 105 cells of each cell line were seeded on polylysine-coated coverslips, treated with different concentrations of Aza and TSA for 48 h and then fixed in 5% formaldehyde at room temperature for 30 min. This was followed by analyzing all samples under a fluorescence microscope (Axiophot, Zeiss, Germany) and recording various images which correspond to the different final concentrations of each medicament (
Flow Cytometry Analyses of Cells Expressing the Hygromycin-EGFP Fusion Gene.
In order to prepare samples for FACS analysis, cells were incubated in the 6-well plates in 0.05% trypsin containing 0.5 mM EDTA (Gibco, BRL) at 37° C. for 5 min, followed by stopping the trypsin action by adding two volumes of culture medium. The cells were harvested, centrifuged at 500×g for 5 min and resuspended in 1 ml complete D-MEM. In order to stain dead cells, propidium iodide (final concentration 10 μg/ml) was added to each sample. The cells were then again centrifuged and resuspended in phosphate-buffered saline (PBS 1 x, pH 7.4), before analyzing them by means of FACS.
The cells were analyzed using FACScalibur (Becton Dickinson) with the flow rate corresponding to approximately 500 events/s.
In order to exactly define a cell population and to exclude cell debris and aggregates, a region of interest was established on the dot plot (FSC compared to SSC). In the two-parameter histogram of propidium iodide, dead cells were distinguished by comparison to forward angle light scatter (FSC). The fluorescence intensity of individual cells was measured on a logarithmic scale, each logarithmic histogram representing 2×104 counted events. The fluorescence intensity mean value (MFI) was the parameter used for defining the increase in the fluorescence intensity in each cell population.
Cell Cycle Analysis
U87H-GFP and the parent cells were seeded at 5×103/cm2 in T25 flasks (Nuclon, NUNC), using D-MEM without hygromycin B for both cell lines. Half of the flasks were treated with 5 μM Aza and the other, as a negative control, without any medicaments. After 42 h, BrdU was added to the medium (final concentration of 10 μM), and 6 h later the cells were prepared for cell cycle analysis.
The cells were harvested, centrifuged at 500×g for 5 min and fixed in chilled 70% strength ethanol for 20 min. BrdU incorporation into the DNA was detected by using 3×105 cells of each Aza-treated or untreated cell line.
PBS 1 x/0.5% BSA (washing buffer) was added, and the cells were centrifuged at 500×g for 5 min. The pellet was then resuspended in a denaturing solution (HCl 1M, PBS 0.5×BSA 0.5%) and washed again after 20 min. This was followed by re-suspending the pellet in 0.1M sodium borate (Na2B4O7), pH 8.5, for 2 min and then adding the washing buffer. After this passage, the total volume of each sample was divided into two halves (one half being used for the isotype antibody, the other one for the BrdU antibody), centrifuged at 500×g for 5 min, resuspended in the buffer containing the anti-isotype or anti-BrdU monoclonal antibodies (Becton Dickinson) and, after 30 min, washed with PBS 1 x/0.5% BSA. The supernatant was discarded and the pellet resuspended in RNAse A (final concentration 100 μg/ml); the DNA was stained by also adding to the solution 7-AAD (Via-PROBE, Becton Dickinson). After 1 h (in the dark), the samples were washed and then resuspended in PBS 1 x/0.5% BSA. DNA fluorescence of the nuclei (approximately 104 nuclei were analyzed for each cell population) was measured by means of the abovementioned FACScan flow cytometer (Becton Dickinson) and the percentages of cells in the G0 and G1, S, G2 and M phases of the cell cycle were analyzed on the basis of the FACScan software programs.
3) Results
The cell line U87H-GFP contains the plasmid pCMV-hygroEGFP in which activation of the hCMV promoter is usually regulated at a low level. Said plasmid imparts to the cell line resistance to hygromycin B and a basic green fluorescence compared to the parent cell line. The hCMV promoter was shown as being completely repressed by methylation of the 5′-CpG site of cytosine (Prosh S. et al. 1996 Biol Chem Hoppe Seyler 377(3):195-201). In order to estimate the property of the promoter of being able to be activated by medicaments interfering with the DNA methylation state and chromatin condensation, U87H-GFP and the parent line U87 were kept in the presence of Aza and TSA for several days. Prior to the experiment, hygromycin B was removed from the medium in order to obtain a decrease in basic activation of the hCMV promoter and furthermore to detect promoter activation by Aza and TSA.
Furthermore, a change in the morphology of the cells was observed at high concentrations of TSA and Aza, indicating that these substances may force the tumor cells U87 back into differentiation.
The abscissae correspond to an arbitrary scale which refers to the logarithm of fluorescence intensity, and the ordinates represent the relative cell number. When comparing the control, which had not been treated with the reporter cell line, with the reporter cell line, which had been treated with the abovementioned final concentration, we obtained a shift in the fluorescence profile in the direction of higher intensity. The shift is already clearly-visible with additions of 2.5 μM Aza (
At a final concentration of 100 nM, TSA does not induce in any way an increase in H-GFP gene expression (profile d), but attains a saturation threshold at a final concentration of 1 μM (profile 1). It was not possible to use final TSA concentrations of more than 3 μM, since these proved highly toxic and drastically reduced the number of living cells, as was observed by means of FACS (data not shown).
The parent cell line is likewise sensitive to Aza (
The histogram in
TSA can also cause amplification of the H-GFP gene, as
In order to further investigate whether TSA can act synergistically with Aza, as has been shown for other tumor cell lines (Cameron E. E. et al. 1999 Nat Genet 21:103-107), we used TSA in combination with Aza for 48 h (
Effects of 5-Azacytidine on the Cell Cycle.
U87H-GFP and the parent cells were treated with 5 μM Aza for two days in order to study the effect of cytosine analog on the cell cycle. As
4) Statistical Analysis
The P values were calculated using the program “Anova, 1-faktorielle-Varianz-Analyse” with MS Excel. The P values <0.05 were regarded as statistically significant.
Table 1 shows the cell cycle analysis: 5-azacytidine influences the cell cycle only in the parent cell line U87 but not in U87H-GFP. The percentages of the cells in the G1-G0, S, G2 and M phases of the cell cycle were obtained as described in
Apart from an increased number of cells in the G2 phase, U87H-GFP exhibited no significant differences in the cell cycle when treated with 5 μM Aza. In contrast, there were significant changes in the cell cycle phases of U87 when kept in a culture containing 5 μM Aza for 2 days. A reduced number of cells in the G1-G0 and M phases was associated with an increased number in the G2 and S phases.
Claims
1. A DNA construct, comprising a fusion gene under the control of a promoter, wherein said fusion gene comprises a resistance gene and a reporter gene and is slightly toxic to a host cell transfected with said DNA construct.
2. The DNA construct of claim 1, wherein the promoter is selected from the group consisting of: a CMV promoter, an RSV promoter, cellular promoters of tumor suppressor genes and promoters of differentiation genes.
3. The DNA construct of claim 2, wherein the reporter gene is selected from the group consisting of: GFP, LacZ and luciferase.
4. The DNA construct of claim 3, wherein the resistance gene is selected from the group consisting of: a hygromycin gene, a neomycin gene and a puromycin gene.
5. The DNA construct of claim 2, wherein the resistance gene is selected from the group consisting of a hygromycin gene, neomycin gene and puromycin gene.
6. The DNA construct of claim 1, wherein the reporter gene is selected from the group consisting of: GFP, LacZ and luciferase.
7. The DNA construct of claim 6, wherein the resistance gene is selected from the group consisting of: a hygromycin gene, a neomycin gene and a puromycin gene.
8. The DNA construct of claim 1, wherein the resistance gene is selected from the group consisting of: a hygromycin gene, neomycin gene and puromycin gene.
9. The DNA construct of claim 1, wherein the fusion gene comprises a gene coding for a polypeptide capable of developing an action toxic to the host cell.
10. A plasmid, comprising a DNA construct of claim 1.
11. A plasmid, comprising a DNA construct of claim 2.
12. A plasmid, comprising a DNA construct of claim 6.
13. A plasmid, comprising a DNA construct of claim 8.
14. A plasmid, comprising a DNA construct of claim 9.
15. A virus, comprising an expression cassette which comprises the DNA construct of claim 1 or codes therefor.
16. A virus, comprising an expression cassette which comprises the DNA construct of claim 2 or codes therefor.
17. A virus, comprising an expression cassette which comprises the DNA construct of claim 6 or codes therefor.
18. A virus, comprising an expression cassette which comprises the DNA construct of claim 8 or codes therefor.
19. A virus, comprising an expression cassette which comprises the DNA construct of claim 9 or codes therefor.
20. A virus, comprising an expression cassette which comprises the DNA construct of claim 10 or codes therefor.
21. A virus, comprising an expression cassette which comprises the DNA construct od claim 14 or codes therefor.
22. A eukaryotic cell, comprising the plasmid of claim 10.
23. The eukariotic cell of claim 22, wherein said cell is a human cell.
24. The eukariotic cell of claim 22, wherein said cell is from the cell line U87-HGFP which was deposited in accordance with the Budapest Treaty at the DSMZ in Brunswick, Germany, under deposition number DSMZ ACC 2473 on Nov. 9, 2000.
25. A eukaryotic cell, comprising the virus of claim 15.
26. The eukaryotic cell of claim 25, wherein said cell is a human cell.
27. The eukaryotic cell of claim 25, wherein said cell is from the cell line U87-HGFP which was deposited in accordance with the Budapest Treaty at the DSMZ in Brunswick, Germany, under deposition number DSMZ ACC 2473 on Nov. 9, 2000.
28. A method for identifying a compound capable of causing differentiation in eukaryotic cells, comprising:
- a) incubating cells of claim 22 in a culture medium containing a selection substance corresponding to the resistance gene;
- b) inoculating a culture medium lacking said selection substance with the incubated cells from step a);
- c) incubating the culture medium inoculated with the cells from step b) for about 5 hours to about 100 hours;
- d) checking the incubated cells from step c) for expression of the reporter gene;
- e) adding said compound to said culture medium of the cells from step c);
- f) incubating said culture medium with the cells and said compound for about 1 day to about 5 days;
- g) checking the incubated cells from step f) for expression of the reporter gene compared to cells from step d); and
- e) identifying the compound that causes the increase in the expression of said reporter gene as the compound that causes differentiation in eukaryotic cells.
29. The method of claim 28, wherein said incubating of the culture medium inoculated with the cells in step c) is for about 24 hours.
30. The method of claim 28, wherein said incubating of said culture medium with the cells and said compound in step f) is for about 2 days.
31. A method for identifying a compound capable of causing differentiation in eukaryotic cells, comprising:
- a) incubating cells of claim 25 in a culture medium containing a selection substance corresponding to the resistance gene;
- b) inoculating a culture medium lacking said selection substance with the incubated cells from step a);
- c) incubating the culture medium inoculated with the cells from step b) for about 5 hours to about 100 hours;
- d) checking the incubated cells from step c) for expression of the reporter gene;
- e) adding said compound to said culture medium of the cells from step c);
- f) incubating said culture medium with the cells and said compound for about 1 day to about 5 days;
- g) checking the incubated cells from step f) for expression of the reporter gene compared to cells from step d); and
- e) identifying the compound that causes the increase in the expression of said reporter gene as the compound that causes differentiation in eukaryotic cells.
32. The method of claim 31, wherein said incubating of the culture medium inoculated with the cells in step c) is for about 24 hours.
33. The method of claim 31, wherein said incubating of said culture medium with the cells and said compound in step f) is for about 2 days.
34. A method for preparing a pharmaceutical composition, comprising the steps of the method of claim 28 and further comprising mixing the identified compund with a pharmaceutically acceptable carrier.
35. A method for preparing a pharmaceutical composition, comprising the steps of the method of claim 31 and further comprising mixing the identified compound with a pharmaceutically acceptable carrier.
Type: Application
Filed: Jul 27, 2006
Publication Date: Feb 1, 2007
Inventors: Jan-Heiner Kuepper (Kusterdingen), Reinhard Kandolf (Hechingen), Ralph Meyer (Waldbockelheim)
Application Number: 11/495,182
International Classification: A61K 48/00 (20060101); C07H 21/04 (20060101); C12P 21/06 (20060101); C12N 7/00 (20060101); C07K 14/47 (20070101);