GB2125409A - Genetic engineering - Google Patents

Genetic engineering Download PDF

Info

Publication number
GB2125409A
GB2125409A GB8320975A GB8320975A GB2125409A GB 2125409 A GB2125409 A GB 2125409A GB 8320975 A GB8320975 A GB 8320975A GB 8320975 A GB8320975 A GB 8320975A GB 2125409 A GB2125409 A GB 2125409A
Authority
GB
United Kingdom
Prior art keywords
sequence
dna
factor
recombinant
human
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Granted
Application number
GB8320975A
Other versions
GB2125409B (en
GB8320975D0 (en
Inventor
George Gow Brownlee
Kong Hong Choo
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
National Research Development Corp UK
Original Assignee
National Research Development Corp UK
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Priority claimed from GB838312490A external-priority patent/GB8312490D0/en
Application filed by National Research Development Corp UK filed Critical National Research Development Corp UK
Priority to GB8320975A priority Critical patent/GB2125409B/en
Publication of GB8320975D0 publication Critical patent/GB8320975D0/en
Publication of GB2125409A publication Critical patent/GB2125409A/en
Application granted granted Critical
Publication of GB2125409B publication Critical patent/GB2125409B/en
Expired legal-status Critical Current

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/14Hydrolases (3)
    • C12N9/48Hydrolases (3) acting on peptide bonds (3.4)
    • C12N9/50Proteinases, e.g. Endopeptidases (3.4.21-3.4.25)
    • C12N9/64Proteinases, e.g. Endopeptidases (3.4.21-3.4.25) derived from animal tissue
    • C12N9/6421Proteinases, e.g. Endopeptidases (3.4.21-3.4.25) derived from animal tissue from mammals
    • C12N9/6424Serine endopeptidases (3.4.21)
    • C12N9/644Coagulation factor IXa (3.4.21.22)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6876Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
    • C12Q1/6883Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for diseases caused by alterations of genetic material
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12YENZYMES
    • C12Y304/00Hydrolases acting on peptide bonds, i.e. peptidases (3.4)
    • C12Y304/21Serine endopeptidases (3.4.21)
    • C12Y304/21022Coagulation factor IXa (3.4.21.22)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q2600/00Oligonucleotides characterized by their use
    • C12Q2600/156Polymorphic or mutational markers

Landscapes

  • Chemical & Material Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Health & Medical Sciences (AREA)
  • Organic Chemistry (AREA)
  • Engineering & Computer Science (AREA)
  • Genetics & Genomics (AREA)
  • Wood Science & Technology (AREA)
  • Zoology (AREA)
  • Bioinformatics & Cheminformatics (AREA)
  • General Engineering & Computer Science (AREA)
  • General Health & Medical Sciences (AREA)
  • Biochemistry (AREA)
  • Proteomics, Peptides & Aminoacids (AREA)
  • Microbiology (AREA)
  • Analytical Chemistry (AREA)
  • Biomedical Technology (AREA)
  • Molecular Biology (AREA)
  • Biotechnology (AREA)
  • Pathology (AREA)
  • Immunology (AREA)
  • Biophysics (AREA)
  • Physics & Mathematics (AREA)
  • Medicinal Chemistry (AREA)
  • Micro-Organisms Or Cultivation Processes Thereof (AREA)
  • Preparation Of Compounds By Using Micro-Organisms (AREA)

Abstract

It has been a problem to find an alternative, less time-consuming, and more reliable source of factor IX, a polypeptide which is essential to the human blood-clotting process and necessary for the treatment of patients with Christmas disease. In order to aid in the solution of the problem, there is provided recombinant DNA containing a DNA sequence occurring in the human factor IX genome, and includes recombinant DNA comprising substantially the whole sequence of human factor IX genome, which is inserted in a cloning vehicle and transformed into a host, such as Escherichia coli. Other fragments of the sequence have also been cloned and the invention includes DNA molecules comprising part or all of the human factor IX DNA. There is also described cDNA derived from human factor IX RNA. Uses include the provision of an intermediate of value in the genetic engineering of a factor IX polypeptide precursor and thence manufacture of the factor IX polypeptide, and in making probes for use in diagnosing the presence of normal or abnormal factor IX DNA in patients with Christmas disease.

Description

SPECIFICATION Genetic engineering BACKGROUND OF THE INVENTION 1. Field of the invention This invention is in the field of genetic engineering relating to factor IX DNA.
2. Description of prior art Factor IX (Christmas factor or antihaemophilic factor B) is the zymogen of a serine protease which is required for blood coagulation via the intrinsic pathway of clotting (Jackson a Nemerson, Ann.Rev.Biochem. 49, 765--811, 1980). This factor is synthesised in the liver and requires vitamin K for its biosynthesis (Di Scipio a Davie, Biochem. 18, 899-904, 1979).
Human factor IX has been purified and characterised, but details of the amino acid sequence are fragmentary. It is a single-chain giycoprotein, with a molecular weight of approximately 60,000 (Suomela, Eur.J.Biochem.
71,145-154,1976). Like other vitamin Kdependent plasma proteins, human factor IX contains in the amino-terminal region approximately 12 gamma-carboxygiutamic acid residues (Di Scipio s Davie, Biochem. 18, 899-904, 1979) During the clotting process, and in the presence of Ca++ ions, factor IX is acted upon by activated factor IX (IXa) by the cleavage of two internal peptide bonds, releasing an activation glycopeptide of 10,000 daltons (Di Scipio et a/., J.Clin. Invest. 61, 1 528-1538, 1978). The activated factor IX (IXa) is composed of two chains held together by at least one disulphide bond.Factor IXa then participates in the next step in the coagulation cascade by acting on factor X in the presence of activated factor VEIL, Ca++ ions, and phospholipids (Lindquist etna/., J.Biol.Chem.
253,1902-1909,1978).
Individuals deficient in factor IX (Christmas disease or haemophilia B) show bleeding symptoms which persist throughout life. Bleeding may occur spontaneously or following injury. This may take place virtually anywhere. Bleeding into the joints is common, and after repeated haemorrhages, may result in permanent and crippling deformities. The condition is a sex-linked disorder affecting males. Its frequency in the population is approximately 1 in 30,000 males.
The current method of diagnosing Christmas disease involves measurement of the titre of factor IX in plasma by a combination of a clotting assay and in immunochemical assay. Treatment of haemorrhage in the disease consists of factor IX replacement by means of intravenous transfusion of human plasma protein concentrates enriched in factor IX. The enrichment of plasma in factor IX is a time-consuming process.
Summary of the invention After considerable research and experiment, important progress has now been made towards producing artificial human factor IX by recombinant DNA technology (genetic engineering). Thus, the cloning of DNA sequences which are substantially the same as extensive sequences occurring in the human factor IX genome has been achieved.
The invention arises from the finding that an extensive DNA sequence of the human factor IX genome can be obtained by a clever and laborious combination of chemical synthesis and artificial biosynthesis, starting from elementary nucleotide or dinucleotide "building blocks", as will be described below.
A major feature of the invention comprises recombinant DNA which comprises a cloning vehicle DNA sequence and a sequence foreign thereto (i.e. foreign to the vehicle) which is substantially the same as a sequence occurring in the human factor IX genome. A 11 873 nucleotide long part of such a foreign sequence has been identified and a very large part of it has been sequenced by the Maxam-Gilbert sequencing method. A 129 nucleotide length of this sequence is more than sufficient to characterise it unambiguously as coding for a specific protein and a particular such length is regarded herein as useful to characterise the whole sequence inserted in the cloning vehicle as one occurring in the human factor IX genome.Other cloned sequences can then be verified as belonging to the human factor IX genome by determining that part thereof is identical to a region of the firstmentioned sequence, i.e. the sequences have a common identity in an overlapping region.
A further feature of the invention therefore comprises recombinant DNA which comprises a cloning vehicle or vector DNA sequence and a DNA sequence foreign thereto which consists of or includes substantially the following sequence of 129 nucleotides (which should be read in rows of 30 across the page):- ATGTAACATG TAACATTAAG AATGGCAGAT GCGAGCAGTT TTGTAAAAAT AGTGCTGATA ACAAGGTGGT TTGCTCCTGT ACTGAGGGAT ATCGACTTGC AGAAAACCAG AAGTCCTGTG AACCAGCAG (1) The invention includes particularly recombinant DNA which comprises a cloning vehicle DNA sequence and a sequence foreign to the cloning vehicle, wherein the foreign sequence includes substantially the whole of an exon sequence of the human factor IX genome. The 129-nucleotide sequence described above corresponds substantially to such an exon sequence.Another such exon sequence which independently characterises the human factor IX DNA is the 203nucleotide sequence substantially as follows (again reading in rows of 30 across the page):- TGCCAThCC ATGTGGAAGA GTTTG7 CACAAACTTC TAAGCTCACC CGTGCTGAGG CTGTTT'CC TGATGTGGAC TATGTAAATT CTACTGAAGC TGAAACCATT TTGGATAACA TCACTCAAAG CACCCAATCA I | TTTAATGACT TCACTCGGGT TGTTGGTGGA GAAGATGCCA AACCAGGTCA ATTCCCTTGG CAG The intron sequences of the human factor IX genome are excised during the transcription process by which mRNA is made in human cells.
Only exon sequences are translated into protein.
DNA coding for factor IX has been prepared from human mRNA. This cDNA has been partly sequenced and found to contain the same 129and 203-nucleotide sequences set out above.
The invention also includes recombinant DNA which comprises a cloning vehicle sequence and a DNA sequence foreign to the cloning vehicle, wherein the foreign sequence comprises a DNA sequence which is complementary to human factor IX mRNA. Such a recombinant cDNA can be isolated from a library of recombinant cDNA clones derived from human liver mRNA by using an exon of the genomic human factor IX DNA (or part thereof) as a probe to screen this library and thence isolating the resulting clones.
The invention also includes recombinant DNA in which the foreign sequence is any fragment of human factor IX DNA, particularly of length at least 50 and preferably at least 75 nucleotides or base-pairs. It includes such recombinant DNA whether or not part of the 129 or 203-base-pair sequence defined above. It includes especially part or all of the exon sequences of human factor IX genomic DNA. Various short lengths up to about 11 kilobases (11,000 nucleotides or base-pairs) long have been prepared by use of various restriction endonucleases. Methods of isolating recombinant DNA from clones are well known and some are described hereinafter. The DNA of the invention can be single or double stranded form.
The recombinant human factor IX DNA of this invention is useful as a tool of recombinant DNA technology. Thus it is useful as the first stage in the production of artificial human factor IX and in the preparation of probes for diagnostic purposes.
In the production of the artificial human factor IX it is contemplated that appropriate cDNA or genomic clones will be introduced into a suitable expression vector in either mammalian or bacterial systems. For mammalian studies, the gene might be too long to be conveniently retained in one clone. Therefore a suitable artificial "minigene" will be designed and constructed from suitable parts of the cDNA and genomic clones. The minigene will be under the control of its own promoter or instead will be replaced by an artificial one, perhaps the mouse metallothioneine I promoter. The resultant 'minigene' will then be introduced into mammalian tissue culture cells e.g. a hepatoma cell line, and selection for clones of cells synthesising maximum amounts of biologically active factor IX will be carried out.
Alternatively "genetic farming" could be employed as has been demonstrated for mouse growth hormone (Palmiter eft at Nature 300, 611 1---615, 1982). The minigene would be micro-injected into the pronucleus of fertilised eggs, followed by in vivo cloning and selection for progeny producing the largest quantity of human factor IX in blood.
Alternatively, it is contemplated that the cDNA clone or selected parts of it will be linked to a suitable strong bacterial promotor, e.g. a Lac or Trp promotor or the lamdba PR or PL, and a factor IX polypeptide obtained therefrom.
The natural factor IX polypeptide is synthesised as a precursor containing both a signal and propeptide region. They are both normally cleaved off in the production of the definitive length protein. Even this product is merely a precursor. It is biologically inactive and must be gammacarboxylated at 12 specific N-terminal glutamic acid residues in the so called 'GLA' domain by the action of a specific vitamin K-dependent carboxylase. In addition, two carbohydrate molecules are added to the connecting peptide region of themolecule, but is remains unknown whether they are required for activity. The substrate for the carboxylase is unknown and could be the precursor factor IX polypeptide or alternatively the definitive length protein.
Therefore various relevant polypeptides both with and without the precursor domains will be "constructed" using genetic engineering methods in bacterial hosts. They will then be tested as substrates for the conversion of inactive to biologically active factor IV in vitro by the action of partially purified preparations of the carboxylase enzyme which can be isolated from liver microsomes or other suitable sources.
For diagnostic purposes, the recombinant human genomic factor IX DNA or recombinant human mRNA-derived factor IX DNA has a wide variety of uses. It can be cleaved by enzymes or combinations of two or more enzymes into shorter fragments of DNA which can be recombined into the cloning vehicle, producing "sub-clones".
These sub-clones can themselves be cleaved by restriction enzymes to DNA molecules suitable for preparing probes. A probe DNA (by definition) is labelled in some way, conveniently radiolabelled, and can be used to examine in detail mutations in the human DNA which ordinarily would produce factor IX. Several different probes have been produced for examining several different regions of the genome where mutation was suspected to have occurred in patients. Failure to obtain hybridisation from such a probe indicates that the sequence of the probe differs in the patient's DNA.
In particular it has been shown that Christmas disease can be detected or confirmed by such methodology. Useful probes can contain intron and/or exon regions of the genomic DNA or can contain cDNA derived from the mRNA.
The invention includes particularly probe DNA, i.e. which is labelled, and of a length suitable for the probing use envisaged. It can be singlestranded or double-stranded over at least the human factor IX DNA probing sequences thereof and such sequences will usually have a length of at least 1 5 nucleotides, preferably at least 19-30 nucleotides in order to have a reasonable probability of being unique They will not usually be larger than 5 kb and rarely longer than 10 kb.
The invention accordingly includes a DNA molecule, comprising part of the human factor IX DNA sequence, whether or not labelled, whether intron or exon or partly both. It also includes human cDNA corresponding to part of all of human factor IX mRNA. It includes particularly a solution of any DNA of the invention, which is a form in which it is conveniently obtainable by electroelution from a gel.
The invention includes, of course, a host transformed with any of the recombinant DNA of the invention. The host can be a bacterium, for example an appropriate strain of E.coli, chosen according to the nature of the cloning vehicle employed. Useful hosts may include strains of Pseudomonas, Bacillus subtilis and Bacillus stearothermophilus, other Bacilli, yeasts and other fungi and mammalian (including human) cells.
One process practised in connection with this invention for preparing a host transformed with the recombinant DNA of the invention is based on the following steps: (1) synthesising an oligodeoxynucleotide having a nucleotide sequence comprising that occurring in bovine factor IX messenger RNA coding for amino acids 70-75 or 348-352 of bovine factor IX, and labelling the oligodeoxynucleotide to form a probe; (2) preparing complementary DNA to a mixture of bovine mRNAs; (3) inserting the complementary DNA in a cloning vector to form a mixture of recombinant bovine cDNAs; (4) transforming a host with said mixture of recombinant bovine cDNAs to form a library of clones and multiplying said clones;; (5) probing the clones with the synthetic oligodeoxynucleotide probe obtained in step 1 and isolating the resultant recombinant bovine factor IX cDNA-containing clone; (6) digesting the recombinant bovine factor IX cDNA from said clone with one or more enzymes to produce a bovine factor IX cDNA molecule comprising a shorter sequence of bovine factor IX DNA, but preferably at least 50 base-pairs long; and (7) probing a library of recombinant human genomic DNA in a transformed-host with the shorter sequence bovine factor IX cDNA molecule, to hybridise the human genomic DNA to the said recombinant bovine factor IX DNA and isolating the resultant recombinant DNA-transformed host.
Brief description of the drawings Figure 1 shows the structure of a published amino-acid sequence of bovine factor IX polypeptide, the deduced sequence of the mRNA from which it would be translated and the structures of oligonucleotides (oligo-N 1 and N2) synthesised in the course of this invention; Figures 2 and 3 show the chemical formulae of "building blocks" used to synthesise the oligonucleotides referred to in Figures 1 and 11; Figure 4 is an elevational view, partly sectioned, showing an apparatus for synthesising oligonucleotides; Figure 5 shows the sequence of part of the bovine factor IX cDNA obtained in this invention; Figure 6 is a map showing the organisation of an approximately 27 kb length of human factor IX genomic DNA and is divided into five portions, showing (a) the exon regions; (b) the 11,873- nucleotide length sequenced;; (c) cDNA molecules obtained by restriction with various endonucleases, sub-cloned and subsequently used as probes; (d) DNA molecules obtained by restriction with various endonucleases; and (e) three regions of human factor IX genomic DNA derived from three clones in lambda phage vector.
Figure 7 shows the sequence of the DNA of Figure 6(b) and in parts the encoded protein; Figure 8 shows a restriction enzyme chart of the sequence shown in Figure 7; Figure 9 shows part of the sequence of the human factor IX cDNA and its encoded protein; Figure 10 shows the structure of a pair of complementary oligonucleotides (oligo N3 and N4) synthesised in the course of this invention; Figure 11 shows part of the DNA sequence of the vector pAT153/Pvull/8 of this invention, in the region where it differs from pAT153; Figure 12 is a diagram of plasmid pHIX17 of the invention showing the origin of the 1.4 kb fragment used for probing and initial sequencing; and Figure 1 3 shows the position of the major radioactive bands on probing a "Southern blot" of normal human DNA, cut by the restriction enzymes EcoRl(E), Hindlll(H), BglIl(B) and Bcll(Bc), with a sub-clone of the recombinant human factor IX DNA of this invention.
DESCRIPTION OF PREFERRED EMBODIMENTS 1. General description A recombinant DNA of the invention can be extracted by meats of probes from a library of cloned human genomic DNA. This is a known recombinant library and the invention does not, of course, extend to human genomic factor IX DNA when present in such a library. The probes used were of bovine factor IX cDNA (DNA complementary to bovine mRNA), which were prepared by an elaborate process involving firstly the preparation of recombinant bovine cDNA from a bovine mRNA starting material, secondly the chemical syntheses of oligonucleotides, thirdly their use to probe the recombinant bovine cDNA, in order to extract bovine factor IX cDNA and fourthly the preparation of suitable probes of shorter length from the recombinant bovine factor IX cDNA.The first probe tried appeared to contain an irrelevant sequence and the second probe tried not containing it, proved successful in enabling a single clone of the human genomic factor IX DNA to be isolated. This clone is designated lambda HlX-1. The steps involved are described in more detail in the sub-section "Examples" appearing hereinafter, and the second probe comprises the 247 base-pair DNA sequence of bovine factor IX cDNA indicated in Figure 5 of the drawings. The invention therefore provides specifically a recombinant DNA which comprises a cloning vehicle sequence and a DNA sequence foreign to the cloning vehicle, which recombinant DNA hybridises to a 247 base-pair sequence of bovine factor IX cDNA indicated in Figure 5 (by the arrows at each end thereof).
The cloning vehicle or vector employed in the invention can be any of those known in the genetic engineering art (but will be chosen to be compatible with the host). They include E.coli.
plasmids, e.g. pBR322, pAT153 and modifications thereof, plasmids with wider host ranges, e.g. RP4 plasmids specific to other bacterial hosts, phages, especially lambda phage, and cosmids. A cosmid cloning vehicle containing a fragment of phage DNA including its cos (cohesive-end site) inserted in a plasmid. The resultant recombinant DNA is circular and has the capacity to accommodate very large fragments of additional foreign DNA.
Fragments of human factor IX genomic DNA can be prepared by digesting the cloned DNA with various restriction enzymes. If desired, the fragments can be religated to a cloning vehicle to prepare further recombinant DNA and thereby obtain "sub-clones". In connection with this embodiment a new cloning vehicle has been prepared. This is a modified pAT1 53 plasmid prepared by ligating a BamHI and Hindlll double digest of pAT153 to a pair of complementary double sticky-ended oligonucleotides having a DNA sequence providing a BamHI restriction residue at one end, a Hindlll restriction residue at the other end and a Pvull restriction site in between.
While the invention is described herein with reference to human genomic factor IX DNA in particular, the invention includes human factor IX cDNA (complementary to human factor IX mRNA) which contains substantially the same sequences.
A library of human cDNA has been prepared and probed with human factor IX genomic DNA to isolate human factor IX cDNA from the library. For this purpose the probe DNA is conveniently of relatively short length and must include at least one exon sequence. The invention therefore includes a process of preparing a host transformed with recombinant DNA, comprising cloning vector sequences and a sequence of nucleotides comprised in cDNA complementary to human factor IX mRNA, which process comprises probing a library of clones containing recombinant DNA complementary to human mRNA with a probe comprising a labelled DNA comprising a sequence complementary to part or all of an exon region of the human factor IX genome.
2. Examples A. Bacteria used E.collK-12 strain MC 1061 (Casadaban s Cohen, J.Mol.Biol. 138, 179--207, 1980),E.coli K-i 2 strain HB 101 (Boyer s Roulland-Dussoix, J.Mol.Biol 41,459--472, 1969) and E,coll K-i 2 strain K803 which is a known strain used by genetic engineers.
B. Source and purification of bovine factor IX, antibovine factor IX antibody, and bovine mRNA Highly purified bovine factor IX and rabbit antibovine factor IX antiserum were gifts from Dr. M.
P. Esnouf. Analysis of the purified bovine factor IX on a denaturating polyacrylamide gel showed that it has a purity of greater than 99%. Specific antifactor IX immunoglobulins used for immunoprecipitation experiments were purified as described by Choo et a/., Biochem.J. 199, 527-535, 1 981, by passage of the crude antiserum through a Sepharose-4B column onto which pure bovine factor IX has been coupled.
Bovine mRNA was obtained from calf liver and isolated by the guanidine hydrochloride method (Chirgwin eta!., Biochem. 18, 5294-5299, 1979). The mRNA preparation was passaged through an oligo dT-cellulose column (Caton and Robertson, Nucl. Acids Res. 7, 1445-1456, 1979) to isolate poly(A) + mRNA.
Poly(A) + mRNA was translated in a rabbit reticulocyte cell-free system in the presence of 35S-cysteine as described by Pelham and Jackson (Eur. J.Biochem. 67, 247-256, 1976). At the end of the translation reaction, factor IX polypeptide was precipitated by the addition of specific anti-factor IX immunoglobulins. The immunoprecipitation procedure was as described by Choo etna!., Biochem.J. 181,285-294, 1979 The immunoprecipitated material was washed throughly and resolved on a two-dimensional SDS-polyacrylamide gel (Choo etal., Biochem.J.
181,285-294, 1979), by isoelectricfocussing in one dimension and electrophoresis in another.
Some polypeptides of known molecular weight were subjected to this procedure, to serve as reference points. The immunoprecipitated material showed 4 pronounced spots, all in the 50,000 molecular weight region and with separated isoelectric points. These predominant spots of molecular weight about 50,000 represent a single polypeptide chain plus a possible prepeptide signal sequence, a deduction compatible with published data (Katayama et awl., Proc. Natl.Acad.
Sci.USA 76, 4990--4994, 1979).
When the gel analysis was repeated for the same material but immunoprecipitated in the presence of unlabelled pure bovine factor IX, the 4 spots appeared at reduced intensity, indicating that the translation product is specifically competed for by pure factor IX. Thirdly, immunoprecipitation was performed using a control rabbit antiserum, i.e. from a rabbit which had not been immunised with factor IX. None of the 4 spots appeared. These results therefore indicate that the translation product was a factor IX polypeptide.
The specific immunological/cell-free translation assay established above was used to monitor the enrichment of factor IX mRNA on sucrose gradient centrifugations. Total poly(A) + mRNA was resolved by two successive separations by sucrose gradient centrifugations. When individual fractions from the gradient were assayed by the above method, a fraction of size 20-22 Svedberg units (approx. 2.5 kilobases of RNA) region was found to be enriched (approx. ten-fold) for the bovine factor IX mRNA. This enriched fraction was used in the subsequent cloning experiments.
C. Synthesis of specific bovine factor IX deoxyoligonucleotide mixtures Starting from a knowledge of the amino acid sequence of bovine factor IX (Katayama et al., Proc.Natl.Acad.Sci. USA 76, 49904994, 1 979), the synthesis of two mixtures of oligonucleotide probes was designed. These probes consisted of DNA sequences coding for two different regions of the protein. The regions selected were those known to differ in sequence in the analogous serine proteases, prothrombin, Factor C and Factors VII and X and were those corresponding to amino acids 70-75 and 348-352 respectively.The 70-75 region was particularly favourable in that the mixture of oligonucleotides synthesised, i.e. oligo N2A and oligo N2B, contained all 1 6 possible sequences that might occur in a 1 7 nucleotide long region of the mRNA corresponding to amino acids 70-75.
The oligo N2A-N2B mixture is hereinafter called "oligo N2" for brevity.
Figure 1 of the drawings shows the two selected regions of the known amino acid sequence of bovine factor IX, the corresponding mRNA and the oligonucleotides synthesised.
Since some of the amino acids are coded for by more than one nucleotide triplet, there are 4 ambiguities in the mRNA sequence shown for amino acids 70-75 and therefore 16 possible individual sequences.
The nucleotide mixtures oligo N1 and oligo N2 were synthesized using the solid phase phosphotriester method of Duckworth et al., Nucl.Acids Res. 9, 1691-1706, 1981, modified in two ways. Firstly, o-chlorophenyl rather than pchlorophenyl blocking groups were used for the phosphotriester grouping, and were incorporated in the mononucleotide and dinucleotide "building blocks". Figures 2 and 3 of the drawings show (a) dinucleotide and (b) mononucleotide "building blocks". DMT = 4,4' - dimethoxytrityl and B = 6 N-benzoyl-adenin-9-yl, 4-N-benzoylcytosin- 1 -yl, 2-N-isobutyrylguanin-9-yl or thymin-1 -yl, depending on the nucleotide selected.Secondly, the "reaction cell" used for the successive addition of mono- or dinucleotide "building blocks" was miniaturised so that the coupling step with the condensing agent 1-(mesitylene-2- sulphonyl)-3-nitro-1 ,2,4-triazole (MSNT) was carried out in a volume of 0.5ml pyridine containing 3.5 micromoles of polydimethylacrylamide resin, 1 7.5 micromoles of incoming dinucleotide (or 35 micromoles of mononucleotide) and 210 micromoles of MSNT.
Figure 4 of the drawings is an elevational view of the microreaction cell 1 and stopper 2 used for oligonucleotide synthesis, drawn 70% of actual size. The device comprises a glass-to-PTFE tubing joint 3 at the inlet end of the stopper 2. The stopper has an internal conduit 4 which at its lower end passes into a hollow tapered ground glass male member 5 and thence into a sintered glass outlet 6 to the stopper. The cell 1 has a ground glass female member 7 complementary to the member 5 of the stopper, leading to reaction chamber 8, the lower end of which terminates in a sintered glass outlet 9. This communicates with glass tubing 10 and a 1.2mm. "lnterflow"tap 11.
Further glass tubing 10, beyond the tap 11, leads to the outlet glass-to-PTFE tubing joint 12. Pairs of ears 1 3 on the stopper and cell enable them to be joined together by springs (not shown) in a liquid-tight manner.
After completion of the synthesis and deprotection, fractionation was carried out by high pressure liquid chromatography (Duckworth et al., see above) and the peak tubes corresponding to the product of correct chain length were located by labelling of fractions at their 5'-hydroxyl ends using [gamma-32p]-ATP and T4 polynucleotide kinase, followed by 20% 7M urea polyacrylamide gel electrophoresis. The position on the gel of the 17- and 14- oligonucleotides was determined by separately labelling, by the method described above, 17- and 14- nucleotide long "marker" oligonucleotides and subjecting these to the same gel electrophoresis.
D. Preparation of libraries of cDNA sequences for bovine mRNA Two different approaches were used for the generation of cloned cDNA library: (i) Mbol library First strand cDNA was synthesised using the sucrose gradient-enriched poly(A)+bovine mRNA as template. The conditions used were as described by Huddleston 8 Brownlee, Nucl. Acids Res. 10, 1029-1030, 1981, except that 2 micrograms of oligo N-1, 20-30 micrograms of the mRNA, 10 microcuries [alpha-32P]-dATP (Amersham, 3000 Ci/mmole), and 50 U of reverse transcriptase were used in a 50 microlitre reaction. "dNTP" in Figure 1 denotes the mixture of 4 deoxynucleoside triphosphates required for synthesis. Oligo N-i hybridises to the corresponding region on the mRNA (refer to Figure 1) and thereby acts as a primer for the initiation of transcription. It was used in order to achieve a further enrichment for factor IX mRNA.
At the end of the cDNA synthesis reaction, the cDNA was extracted with phenol and desalted on a Sephadex-G 100 column, before it was treated with alkali (0.1 M NaOH, 1 mM EDTA) for 30 min. at 600C to remove the mRNA strand. Second strand DNA synthesis was then carried out exactly as published (Huddleston 8 Brownlee, Nucl.Acids Res. 10, 1029--1038, 1981).
The double-stranded DNA was next cleaved with the restriction enzyme Mbol and ligated to the plasmid vector pBR322 which had been cut with BamH1 and treated with calf intestinal alkaline phosphatase to minimise vector selfreligation. Phosphatase treatment was carried out by incubating 5 micrograms of BamHI-cut pBR 322 plasmid with 0.5 microgram calf intestinal phosphatase (Boehringer; in 1 OmM Tris -- HCI buffer, pH 8.0) in a volume of 50 microlitres at 370C for 10 minutes, see Huddleston s Brownlee supra.
The ligated DNA was used to transform E.coli strain MC 1061. For transformation E.coli MC 1061 was grown to early exponential phase as indicated by an absorbancy of 0.2 at 600 nm and made "competent" by treating the pelleted bacteriai cells first with one half volume, followed by repelleting, and then with 1/50 volume of the original growth medium of 1 00mM CaCI2 15% v/v glycerol and 1 OmM PlPES-NaOH, pH 6.6 at OOC.
Cells were immediately frozen in a dry ice/ethanol bath to -70"C. For transformation, 200 microlitre aliquots were mixed with 10 microlitres of the recombinant DNA and incubated at OOC for 10 minutes followed by 370C for 5 minutes. 200 microlitres of L-broth (bactotryptone 1 Og., yeast extract 59., sodium chloride 10g., made up to 1 litre with deionised water) were then added and incubation continued for a further 30 minutes at 370C. The solution was then plated on the appropriate antibiotic agar (see below). A library of about 7,000 ampicillin-resistant colonies was thus obtained. They were ampicillin-resistant because they contained the beta-lactamase gene of pBR 322.Of these, aprox. 85% were found to be tetracycline-sensitive.
(ii) dC/dG tailed library In the preparation of this library, first strand cDNA was synthesised as described for the above library except that oligo do(12~181 was used as a primer to initiate cDNA synthesis. Following this, the cDNA was tailed with dCTP using terminal transferase and back copied with the aid of oligo dG(1218) primer and reverse transcriptase to give double stranded DNA, exactly according to the method of Land et a/., Nucl.Acids Res. 9, 2251-2266, 1981. After a further tailing with dCTP, this material was annealed by hybridisation to a dGTP-tailed pBR322 plasmid at the Pstl site. The hybrid DNA was used to transform E.coli strain MC 1061. A library of approximately 10,000 tetracycline resistant colonies was obtained.Of these, approximately 80% were found to be sensitive to ampicillin, due to insertion of DNA into the ampicillin-resistant gene at the Pstl site.
E. Isolation of specific bovine factor IX clones (i) From Mbol library The library of colonies, in an unordered fashion, was transferred onto 13 Whatman 541 filter papers and amplified with chloramphenicol, to increase the number of copies of the plasmid in the colonies, as described by Gergen et a/., Nucl.
Acids Res., 1, 2115-2136 (1979). The filters were pre-hybridised at 650C for 4h in 6 x NET (1 xNET = 0.15m NaCI, 1 mM EDTA, 1 5mM Tris HCI, pH 7.5), 5 x Denhardt's, 0.5% NP40 nonionic surfactant, and 1 microgram/ml. yeast RNA as described by Wallace et a/., Nucl. Acids Res. 9, 879-894(1981). Hybridisation was carried out at 47"C for 20h in the same solution containing 3 x 105cm (0.7 nanogram/ml) of labelled oligo N-2 probe.Labelling was done by phosphorylation of the oligonucleotides at the 5' hydroxyl end using [gamma-32P]-ATP and T4 phophokinase (Huddleston 8 Brownlee, Nucl.Acids Res. 10, 1029--1038, 1981). At the end of the hybridisation, filters were washed successively at 0-40C (2h), 250C (10 min), 370C (10 min) and47cC (10 min). After radioautography of the filters from this screening, one colony showed a positive signal above background. This colony was designated BIX-1 clone.
(ii) From dC/dG-tailed library Screening of this library, in an ordered array fashion, using oligo N-2 probe as described above has resulted in the identification of a positive clone. This was designated BIX--2 clone F. Sequence characterisation of bovine factor IX cDNA clones Characterisation of BlX-1 clone by restriction endonuclease cleavage indicated that it contained a DNA insert of about 430 base-pairs (data omitted, for brevity). Figure 5 shows part of the nucleotide sequence of the coding strand, determined by the Maxam-Gilbert method, extending over 304 nucleotides and provides direct evidence that it has the identity of a bovine factor IX sequence.Thus, nearly all of this 304 nucleotide sequence (corresponding to the amino acid residues 52-139) agrees with the nucleotide sequence predicted from the known bovine factor IX amino acid sequence data (Katayama et awl., Proc.Natl.Acad.Sci. 76, 4990-4994, 1 979). Over this region, there are no discrepancies between BlX-1 and these published data for factor IX, except at nucleotides 38-40 where the amino acid coded for is Asp instead of Thr. This amino acid change was similarly observed in a second, independent cDNA clone (BIX--2; see below). The remainder of the 304-nucleotide sequence, i.e. that shown in brackets in Figure 5, does not agree with the published bovine factor IX amino acid data of Katayama.
In Figure 5, the underlined portion denotes the sequence corresponding to the oiigo N-2 probe sequence, the asterisk denotes a nonsense codon, the brackets enclose a sequence which does not correspond to Katayama's amino acid data and the arrows indicate Hinfl restriction sites. The Katayama numbering system for amino acids is shown and this sequence is in the opposite orientation to the direction of transcription of the tetracycline-resistant gene of the plasmid.
By similar methods, BIX--2 clone was found to have a DNA insert of 102 nucleotides and this spans the nucleotide positions 7-108 as shown in Figure 5. The nucleotide sequences for BIX-1 and BIX-2 clones over this region (nucleotide 7-108) were identical.
G. Isolation of human factor IX gene (i) Initial clone -- lambda HIX- 1 A library of cloned human genomic DNA, namely a Haelil/Alul lambda phage Charon 4A library prepared by Lawn etna!., Cell, 15, 11 57-11 74, 1978, was used. 106 phage recombinants from this library were screened using the in situ plaque hybridisation procedure as described by T. Maniatis etna!., Cell, 15, 687, 1 978. Pre-hybridisation and hybridisation were carried out at 420C in 50% formamide.After hybridisation, filters were washed at room temperature with 2 x SSC (1 x SSC=0.15mM NaCI, 1 5mM sodium citrate, at pH 7.2) and 0.1% SDS, then at 650C with 1 x SSC and 0.1% SDS.
Two DNA molecules, being restriction fragments from the factor IX cDNA cloned in BlX-1, were radiolabelled and used as probes in the hybridisation. The first fragment corresponds to nucleotide numbers8 to 31 7 on the numbering system of Figure 5, and was isolated by Sau3Al digestion of BIX--1 plasmid DNA. The isolated DNA was labelled to high specific activity by incorporation of [alpha--32P] -dATP using a nicktranslation (Rigby et al., J. Mol.Biol. 1 13, 237-251, 1 977, modified, vide infra). Using this probe, 10 clones were isolated. These were plaque-purified and re-hybridised with a 247 nucleotide fragment from BIX1 clone.This fragment, derived from nucleotides 3-249 can be seen from Figure 5. It contains only sequences in agreement with the Katayama bovine factor IX amino acid sequence and was isolated by Hinfl digestion of BlX-1 plasmid DNA. Only a single clone gave a positive hybridisation signal with this 247-nucleotide probe. This clone was further plaque-purified and the resulting clone was designated "lambda HIX-1".
(ii) Subsequent genomic clones A sub-clone, pATIXcVll, of recombinant human factor IX cDNA from human liver mRNA, and prepared as described in Section L below, was linearised by digestion with Hindlil and BamHI.
The resulting 2 kb cDNA molecule was purified by 1% agarose gel electrophoresis. After electroelution, about 100 ng of this cDNA was nick-translated with [alpha 32p] dATP (see above) and used as a hybridisation probe to screen the Haelil/Alul lambda phage Charon 4A human genomic DNA library for further genomic clones, using standard stringent hybridisation conditions.
Two further human factor IX genomic clones, designated lambda HIX-2 and lambda HIX-3, were thus obtained.
H. Characterisation of human factor IX genomic clones (i) Restriction map The initial lambda HIX--1 clone was characterised by cleavage with various single and double digests with different restriction endonucleases and Southern blotting of fragments using the bovine factor IX cDNA probe (results omitted for brevity). The subsequently isolated lambda HIX-2 and 3 clones were characterised in the same way except that the human cDNA probe, pATIXcVII (see Section L below) was used for the Southern blots. From these results it emerged that the sequences in the factor IX genome corresponding to lambda HIX--2 and 3 overlapped with lambda HlX-1 as shown in Figure 6(e).In Section (d) of this Figure 6 are summarised the results of the analysis using the restriction enzymes EcoRI (E), Hindlll (H), Bgnl (B), BamHI (Ba) and Pvull (P), and this serves as a restriction enzyme map.
(ii) Sequencing Numerous sub-clones were isolated from a knowledge of the rectriction enzyme map as described in Section J(ii) below, the majority in a vector pAT153/Pvull/8. Examples of these subclones are shown in Figure 6(c) and a number were used and were of a convenient length for sequence analysis by the Maxam-Gilbert method (Maxam 8 Gilbert, Proc.Natl.Acad.Sci.USA 74, 56-564, 1980).
Initially sequencing was done on part of a 1.4 kb EcoRI restriction fragment from the sub-clone pHIX--17, see below and J(i). A 403-nucleotide (base-pair) length was sequenced, of which a 1 29-nucleotide length was identified as lying within an exon region. This is the 1 29-nucleotide sequence used above to define the factor IX DNA.
Subsequently, a region of 11 873 bases was sequenced in the central portion of the gene [see Figure 6(b)]. Figure 7 shows the sequence of one strand of the DNA. The nucleotides are arbitrarily numbered from 1 to 11873 in the 5' to 3' direction. The original 403-nucleotide sequence runs from Figure 7 nucleotides Nos. 4372 to 4774 and is indicated by 0--0'. The 1 29-nucleotide sequence lying within the 403 one, runs from Figure 7 nucleotides Nos. 4442 to 4570 and is indicated by J-J'. This corresponds exactly to the "w" exon.
In detail, the sequence of nucleotides Nos.
1-7830 contains two short exons (nucleotides 4442-4570 and 7140-7342 respectively) marked w and x in Figure 6(a), J-J' and J'-J" in Figures 7 and 9. These code for amino acids 85-127, and 128-195 respectively of the amino acid sequence predicted from the human factor IX cDNA clone (Figure 9). There are no differences in amino acid sequences predicted from the genomic and cDNA clones of the invention in these two exon regions.The sequence of the gene between residues 7831-11873 is less complete, containing several gaps, but is still a useful characterisation of the gene as it contains two "Alul repeat" sequences, nucleotides 7960-8155 and 96719938.A/ul sequences are found in many genes. The repetition is not exact but there is a typical degree of homology between them. This further characterisation provides a useful cross-check on the accuracy of the restriction enzyme map. This emerges more ciearly from the restriction enzyme chart of Figure 8.
Figure 8 is a chart produced by a computer analysis of the sequence data of the 11 873 nucleotide long sequence of Figure 7. Column 1 of Figure 8 gives the arbitrary nucleotide number allotted to the nucleotide of Figure 7. Column 2 apportions the nucleotide number as a fraction of the whole sequence. Column 3 shows the restriction enzymes which will cut the DNA within various short sequences of nucleotides shown in Column 4. The short sequences of Column 4 begin with the nucleotide numbered in Column 1. With the aid of this chart the positions of the restriction sites shown in Figure 6(d) and some of the sequences shown in Figure 6(c) can be determined very accurately. For example sequences ll-IV are produced by restriction at the following sites (denoted by the first nucleotide number at the 5' end of each site).
II 3624-4769 lil 6380-7378 IV 10589-11868 Particularly important sites are arrowed in Figure 8. Some of the relevant nucleotide numbers are shown in Figure 6(c), the number given being that of the nucleotide at the 5' end of each site.
Further sequence analysis of the sub-clones V, VI, VII and VIII shown in Figure 6(c) indicates that the factor IX gene is divided into at least 7 exon regions separated by at least 6 introns. The positions of the exons are shown in Figure 6(a) by the solid blocks labelled t, u, v, w, x, y and z. The "z" exon is much the longest and its 3'-end coincides with the 3'-end of the mRNA. The location of these exons relative to the cDNA sequence is discussed below (section L) and it is clear that the "t" exon shown in Figure 6(a) is not a marker for the 5'-end of the gene, as its sequence fails to match that of the extreme 5'-end of the cDNA clone (see below). This suggests that the factor IX gene will be longer at its 5'-end than the 27 kb region shown in Figure 6, and will contain at least one further exon.
Additionally, pHIX--17 DNA was digested with EcoRI. The digested material was resolved on 0.8% agarose gel and a 1.4 kb fragment was isolated in solution by electroelution. It can be stored in the usual manner. This 1.4 kb long molecule was used for the initial sequencing. Only about 1.0 kb is inserted DNA, the remaining 0.4 kb being of pBR322. A 403 nucleotide length of the inserted DNA was sequenced and is identified as 0--0' in Figure 7. The same 1.4 kb fragment was also labelled and used as a probe in Section M.
I. Construction of a vector pAT153/Pvull/8 A derivative of the plasmid pAT1 53 (Twig s Sherratt, Nature 283,216-218,1980) was prepared for subcloning of Pvull fragments of factor IX genomic clones, and for ease of characterisation of the resultant subclones. Two partially complementary synthetic deoxyoligonucleotides, oligo N3, and, oligo N4, were synthesised by the solid phase phosphotriester method described in Section C above. Each has "overhanging" BamHI and Hindlll recognition sequences and an internal Pvull recognition sequence. Figure 10 shows the structures of oligo N3 and oligo N4. BamHI and Hindlll cleave ds DNA to leave sticky or "overhanging" ends.For example Hindlll cleaves - AAGCTT -TTCGAA between the adenine-carrying nucleotides of each strand leaving the sticky-ended complementary strands: -A -TTCGA which are present in the oligo N3/N4 combination.
pAT1 53 was digested with Hindlll and BamHI and the 3393 nucleotide long linear fragment was separated from the 346 nucleotide shorter fragment by 0.7% agarose gel electrophoresis, followed by electroelution of the appropriate bands visualised by ethidium bromide fluorescence under UV light. After treatment with calf intestinal phosphatase, as described in Section D(i), the BamHI-Hindlll 3393-long fragment was ligated to an equimolar mixture of oligo N3 and oligo N4 which themselves had been pretreated, as a mixture, with T4 polynucleotide kinase and ATP, to phosphorylate their respective 5'-terminal OH groups.After transforming competent MC 1061 cells (see above) and plating on L-broth plates containing 20 micrograms/ml final concentration of ampicillin, 11 colonies were selected for further analysis. 1 ml plasmid preparation, see Holmes and Quigley, Analytical Biochem. 114, 193-197 (1981), was isolated from the 11 colonies. The plasmid DNA was then analysed for its ability to be linearised by the restriction enzymes BamHI, Hindííl and Pvull. Four clones were positive in this assay and one, labelled pAT1 53/Pvull/8, was selected for sequence analysis by the Maxam-Gilbert method across the newly constructed section of the plasmid. This part of the sequence is shown in Figure 11 along the unique restriction sites.The novel part of the plasmid sequence is underlined: the remainder is present in the parent plasmid pAT153. The vector allows blunt-end cloning (after treatment with phosphatase) into the inserted Pvull site. The cloned DNA can be excised, assuming that it lacks appropriate internal restriction sites, with BamHI/Hindlll, BamHI/Clal or BamHI/EcoRI double digests. The sites adjacent to the Pvull site are also convenient for end labelling with 32P for characterization of the ends of cloned DNA by the Maxam-Gilbert sequencing method.
J. Sub-cloning of human factor IX gene The following subcloning experiments were carried out as a first step towards sequencing of the factor IX gene, and to facilitate the isolation of a small DNA fragment to be used as a probe for the analysis of genomic DNA from haemophilia B patients (see sections M).
(i) Sub-cloning into pBR322 plasmid An approximately 11 kilobase Bglll fragment (see Figure 6) within the factor IX DNA insert in lambda HIX--1 clone was inserted into the BamHI site of pBR322. Transformation was carried out in the E.coli strain, HB 101. The resulting "subclone" was designated pHIX-1 7 (Figure 12).
(i) Sub-cloning into pA TI 53/Pvu11/8 (a) Piasmid DNA from pHIX--17 was prepared and cleaved with Pvull. Five discrete fragments, all derived from the DNA insert of pHIX--17, were isolated. The sizes of these fragments were approximately 1.3,1.2,1.1 and 1.0 kilobases.
These fragments were blunt-end iigated into the Pvull site of the pAT1 53/Pvull/8 vector and transformed into E.coli HB 101. Five clones of recombinant DNA which carried the 2.3, 1.3, 1.2, 1.1 and 1.0 kb fragments were obtained and these were designated pATIXPvu-1,2, 3, 4 and 5 respectively. Factor IX DNA from pATIXPvu-2 is abbreviated as IV and pATIXPvu-5 as III in Figure 6(c).
(b) Phage DNA from the lambda HIX--1 genomic clone was digested with EcoRI. Three different fragments (approximately 5, 2.3, 0.96, kb; see Figure 6), all derived from the insert into the phage, were isolated and inserted in pAT1 53/Pvull/8 vector at the EcoRI site and cloned in E.coli HB 101 to form sub-clones. The three resulting clones for each of these fragments were designated pATIXEco-1,2 and 4 respectively which are shown in the restriction map of Figure 6(d). pATIXEco-1 was further digested with both EcoRI and Bill, and the "overhanging ends" of the restriction sites filled in with deoxynucleotide triphosphates using the Klenow fragment of DNA polymerase I.After isolation of the resulting 1.1 kb fragment by agarose gel electrophoresis and electroelution, it was blunt-end ligated using T4 DNA ligase into the Pvull site of pAT1 53/Pvull and allowed to transform E.coli MC 1061. The resultant sub-clone was designated pATIXBE and the factor IX DNA sequence thereof is abbreviated as II in Figure 6(c).
(c) Phage DNA from lambda HIX--2 was digested with Hindlll and EcoRI giving a 1.8 kb and a 2.6 kb fragment amongst others. These fragments were eluted separately, filled in as described in (b) above, cloned as above into the Pvull site of pAT1 53/Pvull/8 and allowed to transform E.coli MC 1061. The resultant clones were designated pATlXHE-1, and the factor IX DNA sequence thereof is abbreviated as V in Figure 6(c), and pATIXEco-6 and the factor IX DNA sequence thereof is abbreviated as VI in Figure 6(c).
(d) Phage DNA from lambda HIX--3 was digested with EcoRI and Hind Ill and the fragments of 2.3 kb and 2.7 kb were sub-cloned exactly as described in (c) above. The resultant clones were designated pATIXEH--1, abbreviation Vll in Figure 6(c), and pATlXHE-2, abbreviation VIII in Figure 6(c).
K. Preparation of a library of cDNA clones from human liver mRNA Messenger RNA was extracted from a human liver and a 20--22 Svedberg unit enriched fraction of mRNA prepared exactly as described for bovine mRNA in Section B above, except that a 'translation assay' was not used. The first steps in the construction of the double-stranded DNA were carried out using the 'Stanford protocol' kindly supplied from Professor P Berg's department at Stanford University, USA. This itself is a modification of Wickens, Buell 8 Schimke (J.Biol.Chem. 253, 2483-2495, 1 978) and some further modifications, incorporated in the description given below were made in the present work.
For the first strand cDNA synthesis 6 micrograms of poly(A)+ 20-225 human mRNA was incubated with 5 microlitres of 1 Ox buffer (0.5 M Tris-chloride, pH 8.5 at room temperature, 0.4 M KCI, 0.008M MgCI2 and 4 mM dithiothreitol), 20 microlitres of a 2.5 mM mixture of each of the four deoxynucleoside triphosphates, 0.5 microlitres of oligo dTI12~181,1 microlitre (containing 0.5 microcurie) of [alpha-32P] -dATP, 2 microlitres of reverse transcriptase (14 units per microlitre) and the volume made up to 50 microlitres with deionized water. After incubation for 1 hour at 420C, the solution was boiled for 1 2 minutes and then rapidly cooled on ice.The second strand synthesis was carried out by adding directly to the above solution 20 microlitres of 5x second strand buffer (250 mM Hepes/KOH pH 6.9, 250 mM KCI, 50mM MgCI2l,4 microlitres of a 2.5 mM mixture of each of the four deoxynucleoside triphosphates, 10 microlitres of E.coli DNA polymerase 1(6 units per microlitre) and making the volume of the solution up to 100 microlitres with deionized water. After incubation for 5 hours at 1 50C, Sr nuclease digestion was carried out by addition of 400 microlitres of S1 nuclease buffer (0.03 M sodium acetate pH 4.4, 0.25 M NaCI, 1 mM ZnSO4) and 1 microlitre of S, nuclease (at 500 units per microlitre). After incubating for 30 minutes at 370C, 10 microlitres of 0.5M EDTA (pH 8.0) was added. Double stranded DNA was deproteinised by shaking with an equal volume of a phenol: chloroform (1:1) mixture, followed by ether extraction of the aqueous phase and precipitation of ds DNA by addition of 2 volumes of ethanol. After 1 6 hours at -200C, ds DNA was recovered by centrifugation.
DNA polymerase I "fill in" of S, ends was carried out by a further incubation of the sample dissolved in 25 microlitres of 50 mM tris-chloride, pH 7.5.
10 mM MgCl2, 5 mM dithiothreitol and containing 0.02 mM dNTP and 6 units of DNA polymerase I.
After incubating for 10 minutes at room temperature, 5 microlitres of EDTA (0.1 M at pH 7.4) and 3 microlitres of 5% sodium dodecyl sulphate (SDS) were added.
The following part of the protocol differs from the 'Stanford protocol'. The sample was fractionated on a "mini"-Sephacryl S400 column run in a disposable 1 ml pipette in 0.2 M NaCI, 10 mM tris-chloride, pH 7.5 and 1 mM EDTA. The first 70% of the "break-through" peak of radioactivity was pooled (0.4 ml) and deproteinised by shaking with an equal volume of n-butanol:chloroform (1 :4). To the aqueous phase was added 1 microgram of yeast RNA (BDH) as carrier followed by 2 volumes of ethanol. After 16 hours at -200C double stranded DNA was recovered by centrifugation for blunt-end ligation into calf intestinal phosphatase-treated Pvull-cut pAti 53/PvulI/8. using T4 DNA ligase (see I and J(ii) above).After performing a trial experiment, it was found that when the bulk of the sample was incubated with 200 nanograms of vector DNA in a suitable buffer (1 mM ATP, 50 mM Tris-chloride, pH 7.4, 10 mM MgCI2 and 1 2 mM dithiothreitol) and using 1 0 microlitres of T4 DNA ligase in a total volume of 0.2 ml, then on subsequent transformation of competent E.coli MC 1061 cells a total of 58,000 ampicillin-resistant colonies were obtained. Up to 20% of these were estimated to derive from "background" nonrecombinants derived by religation of the vector itself. This 20-225 cDNA library was amplified by growing the E.colifor a further 6 hours at 37 OC.
1 ml aliquots of this amplified library were stored at -200C in L broth containing 15% glycerol, before screening for factor IX cDNA clones.
L. Isolation and sequence analysis of human factor IX cDNA clones 6000 colonies of the amplified 20-22S human cDNA library were plated on each of ten 1 5 cm agar plates and after growing overnight were blotted into Whatman 541 filter paper. After preparing filters for hybridisation as described in section E(i) above, the immobilised colonies were probed with a 1.1 kb molecule of [alpha-32P] -nick translated human factor IX genomic DNA isolated from the pATIXBE subclone (Section J, above).
This linear 1.1 kb section of factor IX genomic cDNA A was isolated from pATIXBE by cleavage with the restriction enzymes BamHI and Hindlll, followed by separation of the 1.1 kb section from the vactor by 1.5% agarose gel electrophoresis. After electroelution, nick-translation was carried out as before and the material used in a hybridisation reaction for 16 hours at 650C in 3x SSC, 1 Ox Denhardts solution, 0.1% SDS and 50 micrograms/ml sonicated denatured E.coli DNA and 100 micrograms/ml of sonicated denatured herring sperm DNA.After hybridisation filters were washed at 650C successively in 3x SSC, 0.1% SDS (2 changes, half an hour each) and 2x SSC, 0.1% SDS (2 changes. half an hour each). After radioautography, 7 clones were selected as positive. but on dilution followed by re-screening by hybridisation as above, only 5 proved to be positive. Plasmid DNA was isolated from each of these 5 clones and one, designated pATIXcVII, was selected for sequence analysis as it appeared to be the longest of the 5 clones as judged by its electrophoretic mobility on 1% agarose gel electrophoresis. A second shorter clone, designated pATIXcVII was also selected for partial sequence analysis.
Sequencing was carried out by the Maxam Gilbert method and a 2778 nucleotide long section of sequence is shown in Figure 9.
Nucleotides 11 5-2002 were derived by sequencing clone pATIXcVII. (The actual extent of this clone is greater as it extends in a 5' direction to nucleotide 1 7. The sequence between 17 and 111 is inverted with respect to the remainder of the sequence presumably due to a cloning artefact.) Nucleotides 1-130 were derived from clone pATIXcVI which extends from nucleotides 1-1548 of Figure 9. The sequence from Nos.
2002-2778 was derived by isolating 4 additional clones designated pATlX1 08.1, pATIX108.2, pATIX108.3 and pATIXDB. The first 3 were derived from a mini-library (designated GGB108) of the cDNA clones constructed exactly as described in section K above except that sucrose density gradient centrifugation was used instead of chromatography on "Sephacryl" S-400 to fractionate the double-stranded DNA according to size. A fraction of m.w. from 1 kb-5 kb was selected and an amplified library of 10,000 independent clones containing approximately 20% background non-recombinant clones was obtained.Clone pATIXDB derived from another cDNA library (designated DB1 ) constructed as described in section K except that total poly A+ human liver mRNA was used as the starting material and sucrose density gradient centrifugation was used to fractionate the DNA according to size as in the construction of the mini-library GGB 108. The complexity of this library was 95,000 with an estimated background of non-recombinants of 50%. Clones pATIX108.1 and pATIX108.2 were selected from a group of 30 hybridization-positive clones isolated by Grunstein-Hogness screening of the mini library GGB108 using a 32P-nick translated probe derived from a Sau3Al restriction enzyme fragment, itself derived from nucleotides 1 796-2002 of clone pATIXcVII. From pATIX108.1 the sequence of nucleotides 2009-2756 was determined (Figure 9). Following this the sequence of a part of pATIX108.2, specifically nucleotides 1950-2086, provided the overlap with pATIXcVII. The remaining 28 hybridization positive clones were screened by carrying out a triple enzymatic digestion with the restriction enzymes EcoRI, BamHI and Hi/,dlll and screening the product of the digest for an EcoRI restriction fragment extending in the St direction trom the cut at position 2480.By this approach, clone pATIX1 08.3 was selected and sequenced from nucieotides 2642-2778. This clone was followed by three A nucleotides, which sequence was confirmed as a vestigial marker for the poly A tail, by the subsequent isolation of clone pATIXDB by a similar method. pATIXDB was sequenced from Nos. 2760-2778 and ended in 42 A nucleotides, thus marking the 3' end of the mRNA.
Figure 9 shows that the predicted amino acid sequence codes codes for a protein of 456 amino acids, but included in this are 41 residues of precursor amino acid sequence preceding the Nterminal tyrosine residue (Y) of the definitive length factor IX protein. The precursor section of the protein shows a basic amino acid domain (amino acids -1 to -4) as well as the more usual hydrophobic signal peptide domain (amino acids -21 to -36).
The definitive factor IX protein consists of 415 amino acids with 1 2 potential gammacarboxyglutamic acid residues at amino acids 7, 8, 15, 17,20,21,26,27,30,33,36 and 40. Two potential carbohydrate attachment sites occur at amino acid residues 1 57 and 1 67. The activation peptide encompasses residues 146180, which are cut out in the activation of Factor IX (see Background of Invention) by the peptide cleavage of an R-A and R-V bond. This leaves a light chain spanning residues 1-145 and a heavy chain spanning residues 181-415.
The exact location of the boundaries between exons (see Section H, above) and how they are joined in the mRNA is marked in Figure 9. The exons are marked t, u, v, w, x, y, z. It can be seen that there is a rough agreement between the exon domains and the protein regions. For example, the exon for the signal peptide is distinct from that of the GLA region. Also that of the activation peptide is separated from the serine protease domain.
The 3' non-coding region of the mRNA is extensive, consisting of 1 390 residues (including the UAAUGA double terminator 1389-1394 but excluding the poly A tail).
The factor IX cDNA is cleavable by the restriction enzyme Haelll to give a fragment from nucleotides 1 33-1440 i.e. a 1 307 nucleotide long region of DNA entirely encompassing the definitive factor IX protein sequence. The nucleotide sequence recognised by Haelll is GGCC. This fragment should be a suitable starting material for the expression of factor IX protein from suitable promoters in bacterial, yeast of mammalian cells. Another suitable fragment could be derived using the unique Stul site at residue 41 (corresponding to an early part of the hydrophobic signal peptide region) and linking it to a suitable promoter. The nucleotide sequence recognised by Stul is AGGCCT M.Southern Analysis of normal and patient Christmas disease DNA (i) Normal The standard (Southern) blotting procedure, Southern, J.Mol. Biol. 98, 503-517, 1975) was used. In a typical experiment, 10-20 micrograms of human genomic DNA (prepared from uncultured blood cells or cultured lymphocytic cells) were digested with one of a number of restriction endonucleases and loaded onto a single gel slot. Following electrophoresis on 0.8% agarose gel and transfer onto nitrocellulose it was hybridised with a probe of 32p~ labelled probe II or of 1.4 kb EcoRI fragment (see Section H).
Labelling of the probe was carried out by nick translation using the method of Rigby et al., supra, modified as follows. About 100 nanograms of the probe was mixed with 40 microcuries of [alpha 32p] dATP (activity about 3,000 Curies/mMole, obtained from Amersham International PLC) in 0.05M Tris-HCI, pH 7.5, 0.01 M MgCl2, 0.001 M dithiothreitol and dCTP, dGTP, dTTP each at a final concentration of 20 micromolar in a volume of 29 microlitres. To this was added 1 microlitre of "solution X" made up of a mixture of 6 units of DNA polymerase I (E.coli), 0.6 nanograms of pancreatic DNase I (Worthington), 1 microgram of crystalline BSA in 10 microlitres of 50% v/v glycerol containing 0.05M Tris-HCl, pH 7.5, 0.01 M MgCI2 and 0.001 M dithiothreitol.The mixture was incubated for 2 hours at 1 50C, after which high molecular weight DNA was purified by chromatography on G-1 00 "Sephadex". Figure 1 3 shows the major bands obtained with DNA from normal individuals probed with either probe II (Figure 6) or labelled 1.4 kb EcoRI fragment. With each of the 4 enzymes used, EcoRI, Hindlll, Bglll and Bull, a single major band of about 4.8, 5.2, 11 and 1.7 kb was obtained.
The fact that these restriction fragments had the same length as those observed in the restriction map of clone lambda HIX--1 confirmed that the conditions of Southern blotting were precise enough to detect the factor IX gene in total DNA preparations. This provides the basis for analysis of DNA from the blood of patients with Christmas disease.
(ii) Christmas patients with gene deletions The value of the probes of the invention for the assay of alterations of genes of some patients suffering from Christmas disease has been demostrated as follows. Two patients with severe Christmas disease, who also developed antibodies to factor IX, were selected for study. The DNA from 50 ml of blood was digested separately with EcoRI, Hindlll, Bglll and Bcll and Southern blots prepared for probing with 32P-nick translated probe II (Figure 6). No specific bands were observed with either patient under conditions where a control digest gave the pattern shown in Figure 13. Similarly no bands were observed in the patients when probe I, Ill or IV (Figure 6) was substituted for probe II.In order to control for possible mischance of some experimental artefact giving the observed 'negative' signal, a factor IX gene probe (this time pATlXcVIl - the cDNA probe) was mixed with an irrelevant autosomal gene probe which was specific for the human Al apolipoprotein (Shoulders and Baralle, Nucl.Acids Res. 10, 4873-4882. 1982). This experiment showed that patient 1 had normal Al apolipoprotein gene, characterised by a 12 kb band in an EcoRI digest, and confirmed that he lacked the 5.5 kb band observed with pATIXcVII and characteristic of the normal factor IX gene. It was concluded that both patients have a sequence of at least 1 8 kb deleted from their factor IX gene.
Two other patients, designated patients 3 and 4, who had also developed antibodies to factor IX gave bands in the normal or abnormal positions on Southern blots with some factor IX gene probes of the invention, but not with others. This suggested that these patients had less extensive deletions of the gene, possibly about 9 kb in length.
These results suggest that diagnosis of haemophiliacs and the heterozygous (carrier) females would be possible in families and this is now under examination. The altered pattern seen in the patient's DNA, whether absence of a band or the presence of a band in an abnormal position, serves as a "disease marker", which can be used to assess for its presence or absence in a suspected carrier. This same test can be applied to antenatal diagnosis, if DNA from foetai cells are available from an amniocentesis. "Genetic diagnosis" should considerably improve existing methods of antenatai diagnosis based on the assay of foetal factor IX protein levels, with the added advantage that the test can be carried out earlier in pregnancy. Genetic methods using natural polymorphisms within the factor IX gene as allelic markers should also make 100% carrier deletion a reality, thereby improving the existing somewhat unsatisfactory methods where probability values are offered to patients.

Claims (24)

1. Recombinant DNA which comprises a cloning vehicle DNA sequence and a DNA sequence foreign to the cloning vehicle, the foreign sequence comprising substantially the following 1 29-nucleotide sequence (read in rows of 30 across the page):- ATGTAACATG TAACATTAAG AATGGCAGAT GCGAGCAGTT TTGTAAAAAT AGTGCTGATA ACAAGGTGGT TTGCTCCTGT ACTGAGGGAT ATCGACTTGC AGAAAACCAG AAGTCCTGTG AACCAGCAG
2.Recombinant DNA which comprises a cloning vehicle DNA sequence and a DNA sequence foreign to the cloning vehicle, the foreign sequence comprising substantially the following 203-nucleotide sequence (read in rows of 30 across the page):- TGCCATTTCC ATGTGGAAGA GTTTCTG7TT CACAAACTTC TAAGCTCACC CGTGCTGAGG CTGTTTTTCC TGATGTGGAC TATGTAAATT CTACTGAAGC TGAAACCATT TTGGATAACA TCACTCAAAG CACCCAATCA TTTAATGACT TCACTCGGGT TGTTGGTGGA GAAGATGCCA AACCAGGTCA ATTCCCTTGG CAG
3. Recombinant DNA which comprises a cloning vehicle DNA sequence and a sequence foreign to the cloning vehicle, the foreign sequence being substantially the same as a sequence occurring in the human factor IX genome.
4. Recombinant DNA according to Claim 3 wherein the human factor IX sequence has a length of at least 50 nucleotides.
5. Recombinant DNA according to Claim 3 wherein the length of the human factor IX sequence is from 75 to 27,000 nucleotides.
6. Recombinant DNA which comprises a cloning vehicle sequence and a DNA sequence foreign to the cloning vehicle, wherein the foreign sequence includes substantially the whole of an exon sequence of the human factor IX genome.
7. Recombinant DNA which comprises a cloning vehicle sequence and a DNA sequence foreign to the cloning vehicle, wherein the foreign sequence comprises a DNA sequence which is complementary to the human factor IX mRNA.
8. Recombinant DNA according to Claim 3, 4 or 5, wherein the cloning vehicle is a modified pAT153 plasmid prepared by ligating a BamHI and Hindlll double digest of pAT153 to a pair of complementary double sticky-ended oligonucleotides having a DNA sequence providing a BamHI restriction residue at one end, a Hindlll restriction residue at the other end and a Pvull restriction site in between.
9. Recombinant DNA according to Claim 8 wherein the pair of complementary oligonucleotides are of formula:- 5' GATCCAGCTGA 3' 3' GTCGACTTCGA 5'
1 0. Recombinant DNA which comprises a cloning vehicle sequence and a DNA sequence foreign thereto which hybridises to a 247 basepair sequence of bovine factor IX DNA complementary to messenger RNA and indicated in Figure 5 by the arrows at each end thereof.
11. A host transformed with at least one molecule per cell of recombinant DNA claimed in any preceding claim.
12. A host according to Claim 11 in the form of E. coli.
13. A host according to Claim 11 in the form of mammalian tissue cells.
14. A process of preparing a host transformed with recombinant DNA as claimed in any one of Claims 1 to 7, which process comprises: (1) synthesising an oligodeoxynucleotide probe having a nucleotide sequence comprising that occurring in bovine factor IX messenger RNA coding for amino acids 70-75 or 348-352 of bovine factor IX and labelling the oligodeoxynucleotide to form a probe; (2) preparing complementary DNA to a mixture of bovine RNA; (3) inserting the complementary DNA in a cloning vehicle to form a mixture of recombinant bovine cDNAs; (4) transforming a host with said mixture of recombinant bovine cDNAs to form a library of clones and multiplying said clones;; (5) probing the clones with the synthetic oligodeoxynucleotide probe obtained in step 1 and isolating a resultant recombinant bovine factor IX cDNA-containing clone; (6) digesting the recombinant bovine factor IX cDNA from said clone with one or more enzymes to produce a bovine factor IX cDNA molecule containing a shorter sequence of bovine factor IX DNA; and (7) probing a library of recombinant human genomic DNA in a transformed host with the shorter sequence bovine factor IX cDNA molecule, to hybridise the human genomic DNA to the said recombinant bovine factor IX DNA and isolating the resultant recombinant DNA-transformed host.
1 5. A process of preparing a host transformed with recombinant DNA as claimed in Claim 1,2 or 7, which process comprises probing a library of clones containing recombinant DNA complementary to human mRNA with a probe comprising a labelled DNA comprising a sequence complementary to part or all of an exon region of the human factor IX genome.
1 6. A DNA molecule comprising an at least 1 5 nucleotide long sequence of part or all of substantially the 1 29-nucleotide sequence set forth in Claim 1.
1 7. A DNA molecule comprising an at least 1 5 nucleotide long sequence of part or all of substantially the 203-nucleotide sequence set forth in Claim 2.
18 A DNA molecule comprising an at least 1 5 nucleotide long sequence of part only of the DNA sequence of the human factor IX genome.
19. A DNA molecule comprising a sequence of length at least 1 5 nucleotides substantially the same as a sequence complementary to part or all of that occurring in human factor IX mRNA.
20. A DNA molecule according to any one of Claims 1 6 to 1 9 of length at least 50 nucleotides.
21. An artificial DNA molecule comprising a sequence substantially the same as a sequence of length at least 1 5 nucleotides occurring in the human factor IX genome.
22. An artificial DNA molecule according to Claim 21 comprising substantially only exon sequences.
23. A labelled diagnostic probe comprising a DNA molecule having a single-stranded or doublestranded probe sequence of from 1 5 to 1 0,000 nucleotides long of DNA sequence defined in Claim 16, 17, 18 or 19 or its complementary sequence.
24. A probe according to Claim 23 having a probe sequence from 20 to 5,000 nucleotides long.
GB8320975A 1982-08-04 1983-08-03 Genetic engineering Expired GB2125409B (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
GB8320975A GB2125409B (en) 1982-08-04 1983-08-03 Genetic engineering

Applications Claiming Priority (3)

Application Number Priority Date Filing Date Title
GB8222486 1982-08-04
GB838312490A GB8312490D0 (en) 1983-05-06 1983-05-06 Genetic engineering
GB8320975A GB2125409B (en) 1982-08-04 1983-08-03 Genetic engineering

Publications (3)

Publication Number Publication Date
GB8320975D0 GB8320975D0 (en) 1983-09-07
GB2125409A true GB2125409A (en) 1984-03-07
GB2125409B GB2125409B (en) 1985-11-13

Family

ID=27261689

Family Applications (1)

Application Number Title Priority Date Filing Date
GB8320975A Expired GB2125409B (en) 1982-08-04 1983-08-03 Genetic engineering

Country Status (1)

Country Link
GB (1) GB2125409B (en)

Cited By (11)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0195592A2 (en) * 1985-03-15 1986-09-24 Btg International Limited Factor IX protein
EP0218713A1 (en) * 1985-04-22 1987-04-22 Genetics Inst HIGH YIElD PRODUCTION OF ACTIVE FACTOR IX.
EP0236978A2 (en) * 1986-03-12 1987-09-16 BEHRINGWERKE Aktiengesellschaft Production of factor XIIIa by gene technology
EP0254076A1 (en) 1986-07-11 1988-01-27 Miles Inc. Improved recombinant protein production
US4994371A (en) * 1987-08-28 1991-02-19 Davie Earl W DNA preparation of Christmas factor and use of DNA sequences
US5171569A (en) * 1985-03-15 1992-12-15 National Research Development Corporation Factor IX preparations uncontaminated by plasma components or pox virus
EP0971724A1 (en) * 1997-02-14 2000-01-19 American Red Cross Expression of active human factor ix in mammary tissue of transgenic animals
US6746866B1 (en) 1986-03-12 2004-06-08 Aventis Behring Gmbh Preparation of factor XIIIa by gene manipulation
US6869790B1 (en) 1986-03-12 2005-03-22 Aventis Behring Gmbh Preparation of DNA encoding factor XIIIA
US7888321B2 (en) 2001-03-12 2011-02-15 Progenetics Llc Production of high levels of transgenic factor IX without gene rescue, and its therapeutic uses
US7977460B2 (en) 2003-05-19 2011-07-12 National Institute For Biological Standards And Control Compositions comprising coagulation factors IXA and VIII for the treatment of haemophilia A or B

Cited By (21)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0430930A1 (en) * 1985-03-15 1991-06-05 Btg International Limited Factor IX protein
JPS61263926A (en) * 1985-03-15 1986-11-21 ブリティッシュ・テクノロジー・グループ・リミテッド Factor ix protein
EP0195592A3 (en) * 1985-03-15 1987-06-24 National Research Development Corporation Factor ix protein
EP0195592A2 (en) * 1985-03-15 1986-09-24 Btg International Limited Factor IX protein
JPH082300B2 (en) 1985-03-15 1996-01-17 ブリティッシュ・テクノロジー・グループ・リミテッド Method for producing factor IX protein
US5171569A (en) * 1985-03-15 1992-12-15 National Research Development Corporation Factor IX preparations uncontaminated by plasma components or pox virus
EP0218713A1 (en) * 1985-04-22 1987-04-22 Genetics Inst HIGH YIElD PRODUCTION OF ACTIVE FACTOR IX.
EP0218713A4 (en) * 1985-04-22 1987-04-28 Genetics Inst HIGH YIElD PRODUCTION OF ACTIVE FACTOR IX.
US4770999A (en) * 1985-04-22 1988-09-13 Genetics Institute, Inc. High yield production of active Factor IX
EP0236978A2 (en) * 1986-03-12 1987-09-16 BEHRINGWERKE Aktiengesellschaft Production of factor XIIIa by gene technology
EP0236978A3 (en) * 1986-03-12 1988-12-21 Behringwerke Aktiengesellschaft Production of factor xiiia by gene technology
US6746866B1 (en) 1986-03-12 2004-06-08 Aventis Behring Gmbh Preparation of factor XIIIa by gene manipulation
US6869790B1 (en) 1986-03-12 2005-03-22 Aventis Behring Gmbh Preparation of DNA encoding factor XIIIA
US7220556B1 (en) 1986-03-12 2007-05-22 Zlb Behring Gmbh Preparation of factor XIIIa by gene manipulation
EP0254076A1 (en) 1986-07-11 1988-01-27 Miles Inc. Improved recombinant protein production
US4994371A (en) * 1987-08-28 1991-02-19 Davie Earl W DNA preparation of Christmas factor and use of DNA sequences
EP0971724A1 (en) * 1997-02-14 2000-01-19 American Red Cross Expression of active human factor ix in mammary tissue of transgenic animals
EP0971724A4 (en) * 1997-02-14 2003-01-08 American Nat Red Cross Expression of active human factor ix in mammary tissue of transgenic animals
US7419948B2 (en) 1997-02-14 2008-09-02 American Red Cross Treatment of hemophilia with human Factor IX produced in mammary tissue of transgenic mammals
US7888321B2 (en) 2001-03-12 2011-02-15 Progenetics Llc Production of high levels of transgenic factor IX without gene rescue, and its therapeutic uses
US7977460B2 (en) 2003-05-19 2011-07-12 National Institute For Biological Standards And Control Compositions comprising coagulation factors IXA and VIII for the treatment of haemophilia A or B

Also Published As

Publication number Publication date
GB2125409B (en) 1985-11-13
GB8320975D0 (en) 1983-09-07

Similar Documents

Publication Publication Date Title
EP0218713B1 (en) High yield production of active factor ix
EP0107278B1 (en) Molecular cloning of the gene for human anti-haemophilic factor ix
EP0200421B1 (en) Expression of factor vii activity in mammalian cells
EP0227462B1 (en) Novel peptide plasminogen activators
JP2610783B2 (en) Gene encoding polykringle plasminogen activator and vector containing the same
US4757006A (en) Human factor VIII:C gene and recombinant methods for production
KR950000303B1 (en) Tissue plasminogen activator (tpa) analogs
WO1985001961A1 (en) Production of factor viii and related products
JPS62111690A (en) Human protein c and its production
EP0182448A2 (en) Production of factor VIII and related products
AU621281B2 (en) Hybrid proteins
GB2125409A (en) Genetic engineering
AU615450B2 (en) Novel fibrinolytic enzymes
EP0299706A2 (en) Nonglycosylated plasminogen activator and method of preparation
CA1214125A (en) Human factor ix dna
RU2122583C1 (en) Method of preparing the protein showing factor vii-mediated activity in blood coagulation
EP0236040A2 (en) Amino acid modified prourokinase and method of preparation
Liang et al. Cloning and characterization of a cDNA encoding murine coagulation factor X
US5242819A (en) DNA molecules encoding hybrid proteins of tissue plasminogen activator and urokinase
US5580559A (en) Hybrid plasminogen activator
CA1312028C (en) Expression vectors containing the heat shock regulatory dna sequences from a heat shock protein 83 (hsp83) gene and inducible expression by use of the vectors
EP0462632A1 (en) Method for producing a desired human protein by recombinant DNA techniques
EP0373896A1 (en) Novel thrombolytic proteins, process for producing the same, and drugs containing the same as active ingredient

Legal Events

Date Code Title Description
732 Registration of transactions, instruments or events in the register (sect. 32/1977)
PE20 Patent expired after termination of 20 years

Effective date: 20030802