The gene PRV-1 and its use Description 5 The invention relates to a nucleotide sequence which encodes the PRV-1 gene, to recombinant DNA which contains this nucleotide sequence, to vectors which contain the recombinant DNA and to cells which are transformed with these vectors, and also to a PRV-1 10 polypeptide, to antibodies against this polypeptide, to a process for detecting the PRV-1 polypeptide and to drugs which comprise the PRV-1 polypeptide or antibodies which are directed against the PRV-1 polypeptide. 15 Polycythemia rubra vera (erythremia), also termed polycythemia vera or p. vera, is a malignant hematological disease in which there is an increased formation of erythroid, granulocytic and megakaryocytic cells. The disease is of clonal origin and arises as a 20 result of the mutation of a single hematopoietic precursor cell. In Germany, the incidence of p. vera is from 4 to 6 per million inhabitants. If left untreated, the disease leads to death within 18 months. Treatment by means of blood-letting or chemotherapy extends the 25 average survival time to more than 13 years. P. vera is diagnosed by means of clinical criteria. The clinical picture includes headaches, pruritus, splenomegaly in two thirds of the patients, bleeding or thromboses, hypertension in a third of the 30 patients, gout, which is brought about by an increase in the production of uric acid, and, in some cases, septic ulcers. The most important laboratory finding is an increase in the values for hemoglobin, hematocrit, erythrocyte count and total erythrocyte volume, and 35 also a neutrophilic granulocytosis or thrombocytosis in many cases. Since, on the one hand, most of the criteria are rather diffuse and, on the other hand, not all the patients fulfill these criteria, it is - 2 frequently difficult to distinguish p. vera from other myeloproliferative diseases, such as chronic granulocytic leukemia or essential thrombocytosis, and thereby confirm the diagnosis. To date, the molecular 5 cause of p. vera is completely unknown. Since, however, p. vera takes a severe course if it is not treated, accurate diagnosis is important. An object of the invention was therefore to find the molecular cause of polycythemia rubra vera and 10 to create the possibility of diagnosing it. This object was achieved by isolating a gene which is expressed specifically in association with p. vera and not in healthy control individuals. This gene is designated the PRV-1 gene (polycythemia rubra vera). 15 A similar nucleotide sequence is disclosed in International application WO 98/50552. One part of the subject matter of the invention therefore relates to a polynucleotide which encodes the PRV-1 gene and essentially comprises the sequence ID 20 No. 1. The polynucleotides of the present invention can be single-stranded or double-stranded DNA or RNA. If they are RNA, it is then clear to the skilled person that "U" nucleotides are present in place of "T" nucleotides. "Polynucleotide" is understood as meaning 25 nucleic acids which contain 15 or more nucleotides. The nucleotide sequence according to the invention is depicted in figure 1. The invention therefore relates to a polynucleotide which corresponds to the sequence shown in figure 1 and also to a 30 polynucleotide whose nucleotide sequence exhibits minor differences. Within the meaning of the present application, minor differences are understood as meaning those sequences in which a few, preferably not more than 50 and particularly preferably not more than 35 25, nucleotides can be exchanged, with, however, the function of the gene encoded by the nucleotide sequence being unaffected. The skilled person is familiar with the fact that a base triplet encoding an amino acid can be replaced with another triplet which encodes the same - 3 amino acid. In addition to this, regions which are of less importance can be deleted and/or mutated to a minor extent. In a particular embodiment, the polynucleotide comprises nucleotides 36 to 1346 of 5 sequence No. 1, that is the coding region of the PRV-1 gene. Other embodiments comprise nucleotides 36 to 1262 or 36 to 1238 of sequence No. 1. This region presumably encodes the active region of the PRV-1 polypeptide. Finally, the polynucleotide of the invention can also 10 comprise nucleotides 39 to 1346, 39 to 1262 or 39 to 1238 of sequence No. 1, such that the codon which encodes the starting methionine is not present. A preferred embodiment is a polynucleotide which comprises nucleotides 99 to 1346, 99 to 1262 or 99 to 15 1238 of sequence No. 1. This results in the codons at the 5' end which encode the signal peptide of the PRV-1 polypeptide not being present. The polynucleotide according to the invention can also be a fragment of the PRV-1 gene. As a rule, 20 the fragment possesses more than 100 nucleotides, preferably, however, more than 300 nucleotides. The fragments can also be used as primers or as probes, in particular for PCR; in this case, the fragments can be truncated to fit the purpose. Usually, primers have a 25 length of between 10 and 30 nucleotides and probes have a length of between 15 and 50 nucleotides. The PRV-1 gene is an endogenous gene whose expression in healthy individuals is, however, restricted to only a few organs. Normally, it is 30 expressed in the main in the hematopoietic organs, i.e. in bone marrow and fetal liver, and weakly expressed in the spleen, but not expressed in heart, muscle, pancreas or kidney. In patients who are suffering from p. vera, this gene is very strongly overexpressed in 35 the hematopoietic cells, in particular. The PRV-1 gene encodes a protein which exhibits the protein sequence shown in Figure 2. The signal peptide, which is present in the protein sequence of all surface molecules and normally removed when the - 4 protein is processed, is divided of f by a hyphen. The protein has the sequence ID No. 2. Another aspect of the invention is consequently an essentially pure polypeptide having the sequence No. 2 or a polypeptide 5 having the sequence No. 2 but lacking the signal peptide (i.e. amino acids 22 to 437 of sequence No. 2). Other embodiments encompass amino acids 1 to 409, 22 to 409, 1 to 401 or 22 to 401 of sequence No. 2 (what is probably the active region of the protein). 10 With regard to biological activity, the polypeptide according to the invention is preferably glycosylated; it is most preferably N-glycosylated. It can then be glycosylated at at least one of the amino acids Asn-46, Asn-189 and Asn-382 of the PRV-1 15 polypeptide (the amino acid numbers refer to the sequence No. 2) . The invention also encompasses fragments of the polypeptides according to the invention which are N-glycosylated. The fragments are at least 50 amino acids in length, preferably at least 20 100 amino acids and most preferably at least 150 amino acids. In another embodiment, a polypeptide can be 0 glycosylated. It is clear to the skilled person that particular amino acids can be replaced with other amino 25 acids without impairing the biological activity of the protein. Such modified forms of the polypeptides according to the invention are also part of the subject matter of the invention (variants) . The amino acid replacements are those which do not have a negative 30 effect on the biological activity of the protein. The skilled person can make use of well known rules for selecting the replacements. Depending on the method of preparation, the PRV-1 polypeptide can, for example, possess a glycosyl 35 phosphatidylinositol anchor. This is then bonded to the amino acids which correspond to amino acids 407 to 409 in sequence ID No. 2. A GPI anchor is used to anchor a protein by means of a lipid on the outside of the cell membrane. However, for reasons which have not so far - 5 been conclusively elucidated, it is frequently observed that GPI-linked proteins are also released into the medium. This is referred to as "shedding". To date, it has not been clarified whether this is a specific 5 process, i.e. such proteins are cleaved from the membrane by enzymes in a controlled manner, or whether it represents a non-specific loss of the anchor. It is consequently very probable that PRV-1 is to be found both on the cell membrane and extracellularly. The 10 secreted form, which is not membrane-bound, is probably more important for the effect of the polypeptide as a growth factor and growth inhibitor since, as a growth factor, this form is able to diffuse and reach other cells. 15 It is clear to the skilled person that he can influence the attachment of the protein to the cell membrane by manipulating these C-terminal amino acids. This particularly concerns the preparation of defined DNA constructs which are intended for expressing the 20 PRV-1 polypeptide or fragments of this polypeptide. The codons which encode these amino acids can be mutated or deleted. The gene encodes a surface receptor of the uPAR/Ly6 family. This receptor family can transduce 25 mitogenic signals, i.e. signals which stimulate cell division. It is therefore assumed that overexpression of the PRV-1 gene, inter alia on the bone marrow cells of p. vera patients, contributes to hyperproliferation of these cells. 30 It has been found that PRV-1 is not expressed on granulocytes in healthy individuals or in patients suffering from other myeloproliferative diseases, e.g. suffering from chronic granulocytic leukemia, acute granulocytic leukemia, essential thrombocytosis or 35 secondary erythrocytosis. In order to be able to use the polypeptide encoded by the PRV-1 gene for analyses and detection methods, it is expediently generated from recombinant DNA, with the recombinant DNA preferably comprising the - 6 nucleotide sequence ID No. 1 or at least the coding region of the PRV-1 gene, that is nucleotides 36 to 1346 of sequence ID No. 1, or else at least nucleotides 39 to 1262 or 39 to 1238, functionally linked to a 5 promoter. However, the recombinant DNA can also comprise only a fragment of sequence No. 1. The invention furthermore relates to a vector which contains the recombinant DNA for the PRV-1 polypeptide, or a fragment thereof, and to a host cell 10 which is transfected or transformed with this vector. The host cells may be prokaryotic, for example bacteria such as E. coli. However, the polypeptides which are expressed are then not glycosylated. Preference is therefore given to eukaryotic host cells, which are 15 able to glycosylate the expressed protein post translationally and modify it in other ways. Examples of eukaryotic host cells are insect cells, such as Sf9 cells, for expression following infection with recombinant baculoviruses, and mammalian cells, such as 20 293 cells, COS cells, CHO cells and HeLa cells. These examples are not exhaustive. It is also possible to use yeast cells as host cells. It is clear to the skilled person that the glycosylation pattern can differ depending on the host cell. The biological activity of 25 the expression product can therefore also vary. Particular preference is given to host cells which glycosylate the expression product in such a way that the biological activity of the protein is retained. Another aspect of the invention is a process 30 for preparing a polypeptide according to the invention. In this process, a DNA encoding the polypeptide according to the invention is caused to be expressed in a host cell. The culture medium or the cells is/are employed for the subsequent isolation of the 35 polypeptide depending on whether the expressed polypeptide is secreted by the host cell into the culture medium or remains in the cell. After that, the polypeptide according to the invention is concentrated and/or purified using methods which are known in the - 7 state of the art, for example chromatographic methods. Methods for purifying proteins are described, for example, in Scopes, R., Protein Purification: Principles and Practice (3rd edition), Springer Verlag 5 (1994) . In one particular embodiment, the process according to the invention encompasses the step in which glycosylated polypeptide is concentrated and/or purified. This step can take place either before the polypeptide according to the invention has been 10 essentially purified or after it has already been essentially purified. In the latter case, the glycosylated moiety of the purified polypeptide is then separated off and isolated. In the most preferred embodiment of the process, N-glycosylated polypeptide 15 is specifically isolated. In another embodiment of the process, polypeptide is isolated which is glycosylated at at least one of the amino acids Asn-46, Asn-189 and Asn-382 of sequence No. 2. The PRV-1 polypeptide which is isolated from 20 granulocytes or produced recombinantly can be employed both for diagnosing polycythemia vera and for treating the disease. One therapeutic possibility is that of "antisense therapy". This method employs an "antisense" 25 RNA molecule, that is an RNA which is complementary to the PRV RNA. Since the PRV-1 RNA has the sequence 5' AAAAGCAGAAAGAGATTACCAGCC-3' (seq. ID No. 3) at its beginning, the requisite antisense PNA directed against this sequence would possess the following nucleotide 30 sequence: 5'-GGCTGGTAATCTCTTTCTGCTTTT-3' (seq. ID No. 4) . This antisense RNA is incorporated into a vector and introduced into the p. vera cells. This RNA is introduced, for example, by means of transfection, with the vector used for the transfection preferably being 35 configured such that it is introduced specifically into the p. vera cells. Expression of the antisense RNA results in it no longer being possible for the PRV-1 mRNA to be translated into a polypeptide. Cells which - 8 have been treated in this way do not then form any PRV 1 protein. The invention therefore also relates to a process for detecting p. vera which is characterized in 5 that the PRV-1 polypeptide, or an epitope thereof, is detected and the extent of the expression is determined. Overexpression of this receptor on mature cells outside of the bone marrow, e.g. on granulocytes, is a 10 strong indication of the presence of the disease p. vera. This overexpression is expediently detected by means of an immunoassay using antibodies which are directed against the PRV-1 receptor. Suitable test methods are the known immunoassay variants which make 15 use of PRV-1 polypeptide-specific antibodies together with other labeled antibodies which can be immobilized or in solution. The labeling can be effected in a manner known per se, for example using radioactive isotopes, by means of fluorescence or luminescence, 20 using enzymes, by means of color-forming reactions or using other groups which are suitable for the determination. These variants are known to the skilled person and do not require any more detailed explanation here. According to the invention, ELISA tests are 25 particularly preferred. The antibodies which are required for specifically detecting the PRV-1 receptor can likewise be prepared in a manner which is known per se. Both monoclonal and polyclonal antibodies are suitable, with 30 preference being given to using monoclonal antibodies. Peptides which are derived from the protein can also be used for preparing antibodies. Within the context of the present invention, success was achieved using the peptides having the sequences: 35 a) KVSDLPRQWTPKN (amino acids 34 to 46) [seq. ID No. 5], and - 9 b) SAREKRDVQPPASQH (amino acids 391 to 405) [seq. ID No. 6]. The polyclonal antibodies are normally produced 5 by immunizing a suitable host (rabbit) with the PRV-1 polypeptide, where appropriate bound to an immunological support (adjuvant), and eliciting an immune response. Monoclonal antibodies can be generated in a manner known per se using the hybridoma technique. 10 The antibodies can be purified by means of affinity purification. The preparation and purification of antibodies are described, for example, in "Antibodies: A Laboratory Manual" by Harlow and Lane, Cold Spring Harbor Laboratory Press. 15 Furthermore, such polyclonal or monoclonal antibodies which are directed against PRV-1 can also be used for treating the disease. In another embodiment, the PRV-1 receptor can be detected using an RT-PCR method. For this, RNA is 20 first of all isolated from the PRV-1-overexpressing cells, which are as a rule granulocytes. A reverse transcription is then performed in a manner known per se using an RT primer. The RT primer is preferably a primer which has the following nucleotide sequence (SEQ 25 ID No. 7): ATTAGGTTATGAGGTCAGAGGGAGGTT. In this way, the specific PRV-1 RNA is 30 transformed into DNA. This DNA is then amplified in a PCR reaction in a manner known per se. The following two primers are preferably employed for the amplification cycles: 35 As the sense primer (SEQ ID No. 8) GCAGAAAGAGATTACCAGCCACAGACGG. As the antisense primer (SEQ ID No. 9) - 10 GAATCGTGGGGGTAATAGAGTTAGCAGG. The skilled person is readily able to use the 5 disclosed sequence to find other primers which are also suitable. Since the RNA is used as the starting material for this method, the PCR signal is only positive when the PRV-1 gene is also expressed. As explained above, 10 this is only the case when the patient is suffering from p. vera. PRV is not expressed in granulocytes of healthy patients. Consequently, the absence of any RT-PCR signal indicates that no p. vera is present. The quantification in the RT-PCR method is preferably 15 effected using the TaqMan@ technology. This quantification requires a probe in addition to primers. The preferred sequence of the probe is 5'-TTCTTGTTGAACCACACCAGACAAATCGG- 3 ' (SEQ ID NO:10). Quantitative RT-PCR for detecting the PRV-1 transcript 20 is therefore also part of the subject matter of this invention. In another alternative, it is also possible to use a blotting method, preferably a Northern Blot, for diagnosing p. vera. For such a method, the RNA is 25 isolated from granulocytes and then examined for the expression of PRV-1 using a blotting method, for example Northern blotting. The cDNA sequence of SEQ ID No. 1, or a segment of the sequence, can be used as the probe. Hybridization then only occurs if the 30 granulocytes are derived from a patient suffering from p. vera since only then is there any expression on the granulocytes. The absence of hybridization indicates that the individual from whom the granulocytes are derived does not have p. vera. 35 It is also possible to use a fragment of the gene for the Northern blot hybridization. Such a fragment is normally more than 100 bases in length, preferably more than 300 bases in length. Alternatively, various different fragments of the gene, - 11 which can be used as probes in the Northern blot, can be prepared by digesting the gene with restriction endonucleases. If the fragments are derived from the cDNA, they are then present as double strands which 5 have to be separated into the single strands for the hybridization. Suitable examples are the Bam HI-PstI fragment from base pair 420 to base pair 831, or the PstI-PstI fragment from base pair 831 to base pair 1900. 10 PRV-1 mRNA, and consequently the expression of PRV-1, can also be detected by first of all reverse transcribing the mRNA in an RT-PCR reaction and then amplifying the cDNA; the amplified DNA is then detected with a probe in a hybridization method. 15 In the case of a positive diagnosis, the disease has to be treated since it otherwise leads to death within a relatively short period of time. For this treatment, it is possible to use specific antibodies which are directed against PRV-1 and to 20 which cytotoxic components can be bonded, where appropriate. The invention therefore furthermore relates to a drug which, in addition to the customary excipients, comprises antibodies which are directed against the 25 PRV-1 receptor. Since the PRV-1 receptor is overexpressed in p. vera, many antibodies are bound on the surface of the affected granulocytes when they come into contact with the anti-PRV-1 antibody. The binding of many antibodies 30 to these cells stimulates the immunological cells to destroy these granulocytes. In this way, it is possible to eliminate the p. vera cells specifically. Surprisingly, it has also been found that the PRV-1 polypeptide exhibits haematopoietic activity. The 35 PRV-1 polypeptide is able to stimulate certain hematopoietic precursor cells to form erythroid colonies. It is particularly the N-glycosylated PRV-1 polypeptides which display this function. The polypeptides according to the invention which are - 12 preferred are therefore the N-glycosylated PRV-1 polypeptides, and fragments thereof, which display the growth factor activity. Another aspect of the invention is therefore a 5 drug which, in addition to a pharmaceutically tolerated excipient, comprises the PRV-1 polypeptide or a biologically active fragment thereof. The PRV-1 polypeptide is preferably glycosylated PRV-1 polypeptide and, even more preferably, N-glycosylated 10 PRV-1 polypeptide or a biologically active fragment thereof. The invention also relates to drugs which comprise at least one polynucleotide according to the invention. The present invention furthermore relates to 15 the use of PRV-1 polypeptide, or a biologically active fragment thereof or a biologically active variant thereof, as a growth factor in vivo and ex vivo. The PRV-1 polypeptide, or a biologically active fragment thereof or a biologically active variant thereof, can 20 be used for treating all pancytopenias and pancytopathies in the bone marrow and in the circulation (change in the cellular constituents of the peripheral blood and bone marrow). The polypeptides of the present invention can, for example, be used for 25 treating anemias in the case of kidney failure, chemotherapy or whole body radiation, for treating neutropenias and thrombocytopenias during chemotherapy or whole body radiation, for the ex-vivo treatment of peripheral or bone marrow stem cells for expansion 30 (multiplication) and retransfusion into the patients, and for treating sepsis, systemic inflammatory response syndrome (SIRS) or regional inflammatory reactions. The polypeptides of the present invention, or drugs which comprise them, can be administered in a wide variety of 35 ways. The forms of administration comprise intravenous, intramuscular, subcutaneous, intraperitoneal, oral, transdermal and transmucosal administration. The polynucleotides according to the invention can also be used for treating pancytopenias and - 13 pancytopathies. In this case, the aim is to express a PRV-1 polypeptide, or a functional fragment thereof, in cells of the affected patient. Gene therapy methods are first and foremost used in this connection. Cells can 5 be isolated from the patient and transfected with a polynucleotide according to the invention (ex-vivo manipulation), after which they are then returned to the patient. It is also possible to conceive of methods in which the polynucleotides according to the invention 10 gain access into the target cells by means of viral transfer. Expression of the inserted nucleic acids then leads to haematopoietic activity. Surprisingly, it was also found that, at higher concentration, the PRV-1 polypeptide has an inhibitory 15 effect on the growth of cells. Thus, it was observed, for example, that adding an increased quantity of PRV-1 protein virtually completely stops the formation of erythroid and granulocytic/monocytic colonies. This effect resembles the action of Interferon-a, which is 20 used, inter alia, therapeutically in chronic myeloid leukemia (CML) and in p. vera. An endogenous inhibitory substance possesses great advantages as compared with a chemical cytostatic agent, such as hydroxyurea, which was used when Interferon-a was not yet available and is 25 to some extent still used. A disadvantage of Interferon-a is that this active compound has very severe side effects. The patients feel as if they were suffering from a serious influenza. The present invention makes available a hematopoiesis-inhibiting 30 substance, with the inhibitory activity being concentration-dependent. Another aspect of the invention is therefore the use of a PRV-1 polypeptide, as described in this application, for inhibiting the growth of cells, in 35 particular its use as a cytostatic agent. Preference is given to the polypeptide being used for inhibiting the growth of hematopoietic cells. The invention also relates to the use of a polypeptide according to the invention for producing a drug for treating - 14 proliferative diseases. These diseases are, in particular, the myeloproliferative diseases, p. vera, essential thrombocythemia, myelofibrosis, CML and also all leukemias and lymphomas and also solid tumors. 5 Another aspect of the invention is the use of a polynucleotide, as described in this application, of a biologically active fragment or of a biologically active variant thereof, for inhibiting the growth of cells. The polynucleotide can be incorporated into a 10 suitable vector and transfected into suitable target cells. After the PRV-1 polypeptide, or a biologically active fragment thereof, or a biologically active variant thereof, has been expressed in an appropriate concentration, the growth-inhibiting effect comes into 15 operation. In the same way, the polynucleotide can be incorporated into a viral vector, after which appropriate target cells are infected virally, leading to PRV-1 being expressed. The invention also relates to the use of a polynucleotide of this application for 20 producing a drug for treating proliferative diseases, such as the myeloproliferative diseases, p. vera, essential thrombocythemia, myelofibrosis, CML and also all leukemias and lymphomas and also solid tumors. The invention also relates to kits for 25 detecting either polycythemia vera or disturbances of the hematopoietic system. These kits comprise a polynucleotide according to the invention and/or a polypeptide according to the invention and/or one or more antibodies according to the invention. In addition 30 to this, the kit can also comprise a container or compositions which are suitable for implementing detection reactions. Examples of such compositions are buffer solutions, reagents for blocking membranes, hybridization solutions, secondary antibodies, 35 substrate solutions for detection reactions, etc. The kit is preferably used for implementing PCR reactions, RT-PCR, Northern blots, Southern blots, Western blots and ELISA, RIA or similar reactions.
- 15 The following examples are given in explanation. Example 1 5 Characterizing the PRV gene The following experiments were carried out in order to characterize the gene: 10 - the following protocol was used to isolate granulocytes from stored blood or from blood obtained by bleeding p. vera patients: - an equal volume of 3% dextran solution in 0.9% NaC1 was added to the blood and the mixture was left to 15 stand at room temperature (RT) for 20 minutes. - The mixture separated into two phases. The upper, light-colored phase was removed and centrifuged for 10 minutes at 1800 g and at RT. - The supernatant was discarded and the cell 20 pellet was resuspended in the same volume of 0.9% NaCl. - In each case 35 ml of the cells in NaCl were layered on 15 ml of Ficoll-Hypaque. - The cells on the Ficoll-Hypaque were then centrifuged for 60 minutes at 1800 g and at RT without 25 using the brake. - A cell pellet and two layers with an interphase were formed. - The layers and interphase were aspirated off and the cell pellet was resuspended for 30 seconds in 30 10 ml of ice-cold 0.2% NaCl, and 10 ml of ice-cold 1.6% NaCl were added immediately after 30 seconds. - The cells were centrifuged down for 10 minutes at 1800 g and at RT. - They were then washed once in 10 ml of PBS and 35 centrifuged down. - The cell pellet contained 95-99%-pure granulocytes. - RNA was isolated from these cells using standard methods.
- 16 - 10 mg of this RNA were examined for the expression of PRV-1 in a Northern blot. The entire cDNA sequence shown in SEQ ID No. 1 was used as a probe. This experiment was performed on 39 p. vera 5 patients and 29 control samples of stored blood. The PRV-1 probe was found to hybridize strongly in the case of the p. vera patients. No hybridization was observed in healthy control samples. 10 Example 2 PRV-1 possesses growth factor activity Embryos were removed from a pregnant mouse 13.5 15 days after fertilization. The fetal livers were removed. The cells contained in them were stained using antibodies and enriched for particular cells, and depleted for other cell types, by means of column chromatography. This results in a cell mixture which is 20 enriched for certain hematopoietic precursor cells (colony forming units-erythroid, CFU-E). Thus, while in all approximately 2% of the fetal liver consists of CFU-E, 30-40% of the enriched cells consist of CFU-E. These CFU-Es were transfected using a 25 retrovirus. To do this, a packaging cell line, designated 293-T, was itself transfected 48 hours previously. 293-T cells are an established human embryonic kidney cell line. 293-T cells are stably transfected with several genes from a retrovirus. If 30 these 293-T cells are now transfected with two plasmids, termed pOS and pKAT, the 293-T cells then produce a retrovirus which is able to infect murine fetal liver cells. If the 293-T cells are transfected with an empty pOS vector and pKAT, a wild-type 35 retrovirus, which only expresses retroviral proteins, is then produced. On the other hand, cloning a human gene, e.g. PRV-1, into the pOS vector results in the production of a retrovirus which expresses this protein - 17 when it has infected cells. The 293-T cells secrete the retrovirus into the cell culture medium. After two days, the cell culture medium from the transfected 293-T cells which contains the 5 retrovirus is harvested and filtered once through a 0.45 gm filter. In order to transfect the fetal liver cells, these latter cells are mixed with the filtered cell culture medium, which contains the retrovirus, and centrifuged for 2 hours at 1800 rpm and 20 0 C in the 10 added presence of Polybren. The transfected fetal liver cells were then cultured in a medium (Methocult, from Cell Systems) which contains, in addition to the usual salts and amino acids, fetal calf serum, 0.0001-0.4 IU of erythropoeitin (EPO)/ml and methyl cellulose (0.8%). 15 The CFU-Es require EPO in order to form hematopoietic colonies. The methyl cellulose solidifies the medium in the form of a jelly, thereby fixing individual cells in this jelly so that, in contrast to being in a liquid medium, they cannot move. It is therefore possible to 20 observe whether a hematopoietic colony is or is not formed from a single cell. CFU-Es form erythroid colonies, that is colonies which contain red blood cells and their precursor cells. After three days, a count is taken of the 25 number of hematopoietic colonies which have developed. Various mixtures are compared. The mixtures were not all examined in each experiment; mixtures 1-3 are very similar controls and each of them can be compared individually with mixture 4. 30 Mixture 1: Cells which were not transfected with a retrovirus; Mixture 2: Cells which were transfected with an empty pOS vector; 35 Mixture 3: Cells which were transfected with a "green fluorescent protein" (GFP), a protein which is not hematopoietically active.
- 18 Mixture 4: Cells which were transfected with pOS PRV-1 (vector + gene according to the invention) . 5 Table 1: The table lists the results obtained from three experiments which were performed as described. The figures in each case indicate the number of colonies. 10 Mixture 1 Mixture 2 Mixture 3 Mixture 4 un- empty vector GFP PRV-1 transfected (pOS) (pOS-GFP) (pOS-PRV-1) Experiment 1 116 156 80 326 Experiment 2 271 273 410 Experiment 3 120 131 291 The experiments demonstrate that CFU-Es which were transfected with PRV-1 form very many more colonies (up to three times as many) than do the 15 various control CFU-Es. This result indicates that PRV 1 is a growth factor for CFU-E. Example 3 20 Solubility of the PRV-1 growth factor A further experiment was carried out in order to investigate whether PRV-1 is a soluble growth factor or whether cell-cell contact is required. It is not 25 only a retrovirus which is produced by the packaging cell line 293-T after it has been transfected with the pOS and pKAT vectors. In addition, the 293-T cells also synthesize the protein encoded by the gene cloned in pOS, i.e. PRV-1 in the present case. If the gene 30 product is a soluble protein, it is secreted into the medium which surrounds the packaging cell line 293-T. If the 293-T cells are transfected only with the pOS - 19 vector, without pKAT, no retroviruses are then formed. The cell culture medium then only contains the soluble protein produced by the cells. Medium which is derived from pOS-PRV-1-transfected cells, and which does not 5 contain any retrovirus, is mixed with CFU-Es and the whole is plated out in the methyl cellulose medium; the resulting colonies are then counted. The following results were obtained: 10 Table 2: Solubility of PRV-1. The figures in each case indicate the number of colonies. Mixture 1 Mixture 2 Mixture 3 Mixture 4 un- empty vector GFP PRV-1 transfected (pOS) (pOS-GFP) (pOS-PRV-1) Experiment 4 137 187 557 In this experiment, too, CFU-Es which were 15 treated with PRV- 1-containing medium formed very many more hematopoietic colonies than did control cells. It can be concluded from this result that PRV-1 is a soluble growth factor. 20 Example 4 PRV-1 also has an inhibitory, cytostatic effect. The experiments were carried out on peripheral 25 blood cells. Since a small number of precursor cells are also circulating in the peripheral blood in healthy individuals, it is possible to culture hematopoietic colonies from peripheral blood cells in a suitable medium (methyl cellulose) . 40 ml of peripheral venous 30 blood were withdrawn from a healthy donor (while initially introducing heparin or EDTA as an anticoagulant) , 15 ml of Ficoll/Hypaque were added to the blood and the mixture was centrifuged at 1 600 rpm for 40 minutes without braking. This results in the 35 production of a density gradient which fractionates the - 20 blood into its cellular constituents. After the centrifugation, what are termed the mononuclear cells, which also include the stem cells, are to be found at the interphase between serum and Ficoll. This 5 interphase was removed and washed in PBS (isotonic salt solution) . This yields purified mononuclear cells, approximately 0.1% of which are hematopoietic stem cells. 10 The mononuclear cells were taken up in a particularly rich medium (IMDM) which contained an added concentration of 3% FCS (fetal calf serum) . This 3% FCS/IMDM subsequently contained the modifications, i.e. PRV-1 was or was not added to it. 15 The mononuclear cells in IMDM were added, at a density of 7 x 10 5 cells/ml, to a commercially available medium supplied by Stem Cell Technologies (Methocult), which contained IMDM and 30% FCS, 1% BSA (bovine serum albumin), mercaptoethanol, 2 mM L-glutamine, 3 IU EPO 20 (erythropoietin)/ml and 1.0% methyl cellulose. The cells grew for 14 days in this medium. The few stem cells which are present in this mixture are able to develop into hematopoietic colonies. Usually, between 100 and 200 hematopoietic colonies develop for every 25 7 x 105 cells employed. A cell line which expresses a very high quantity of PRV-1 was also constructed. The PRV-1 which is produced by these cells is altered such that it no longer possesses a lipid anchor. The expression product 30 consists of the amino acids 1-401 of the sequence SEQ ID No:2; the amino acids 402-437 are therefore missing. This altered PRV-1 is therefore not, like wild-type PRV-1, incorporated into the cell membrane by means of a lipid anchor, but is instead completely 35 secreted from the cells. As in example 3, the cell line consisted of 293 cells which do not produce any retrovirus but which express protein (PRV-1). For the hematopoietic colony assays, the mononuclear blood cells were now taken up either in - 21 IMDM medium, which had been incubated for 48 hours with untransfected cells (293), or in medium which had been incubated for 48 hours with cells which were expressing the altered PRV-1 (293-GPI-less-PRV-1) . The ability of 5 these cells to form hematopoietic colonies was then investigated. The number of erythroid (red) and myeloid (white) blood cell colonies was determined after 14 days. The experiment was repeated three times and also carried out on different days and using different blood 10 donors. Duplicates were also evaluated within the experiment. The following results were obtained: Experiment 1 Cell Donor 1 Donor 2 supernatant Red White Red White colonies colonies colonies colonies 293 248/221 70/114 127/161 25/66 293-GPI-less- 7/3 0/0 31/19 0/0 PRV-1 15 Experiment 2 Cell Donor 1 Donor 2 supernatant Red White Red White colonies colonies colonies colonies 293 99/91 20/19 49/33 8/1 293-GPI-less- 0/0 0/0 0/0 0/0 PRV-1 Experiment 3 20 Cell Donor 1 Donor 2 supernatant Red White Red White colonies colonies colonies colonies - 22 293 107/207 22/30 24/32 5/8 293-GPI-less- 4/3 0/6 0/1 3/0 PRV-1 It can be concluded from this data that a higher dose of PRV-1 than that used in example 3 possesses a cytostatic effect. 5 Example 5 The growth factor PRV-1 is N-glycosylated 10 Granulocytes were isolated from a patient suffering from p. vera, and protein extracts were prepared from these cells using a standard protocol. These protein extracts were treated in accordance with the protocol for the "N-Glycosidase F Deglycosylation 15 Kit" supplied by Boehringer Mannheim. In detail, this means that a "denaturation buffer" was added to the protein extracts and the mixtures were heated at 95 0 C for 3 minutes, after which they were treated either with "reaction buffer" or with "reaction buffer" plus 20 N-glycosidase. Each mixture was incubated overnight at 370C and the proteins were analyzed on a PAGE gel electrophoresis followed by a Western blot. The PRV-1 protein was detected with an antibody directed against a protein having the amino acid sequence ID No. 5. The 25 results show that while PRV-1 protein purified from granulocytes is 60-65 kDa in size, it is only 40 kDa in size after having been digested with N-glycosidase. This clearly proves that PRV-1 is glycosylated on asparagine residues (asparagine = N).