WO1996038591A1 - IMPROVED METHOD FOR OBTAINING FULL-LENGTH cDNA SEQUENCES - Google Patents

IMPROVED METHOD FOR OBTAINING FULL-LENGTH cDNA SEQUENCES Download PDF

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WO1996038591A1
WO1996038591A1 PCT/US1996/008501 US9608501W WO9638591A1 WO 1996038591 A1 WO1996038591 A1 WO 1996038591A1 US 9608501 W US9608501 W US 9608501W WO 9638591 A1 WO9638591 A1 WO 9638591A1
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Prior art keywords
cdna
nucleic acid
pcr
sequence
primer
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PCT/US1996/008501
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French (fr)
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Karl J. Guegler
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Incyte Pharmaceuticals, Inc.
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Priority claimed from US08/459,046 external-priority patent/US6008039A/en
Application filed by Incyte Pharmaceuticals, Inc. filed Critical Incyte Pharmaceuticals, Inc.
Priority to EP96917035A priority Critical patent/EP0832282A1/en
Priority to AU59729/96A priority patent/AU5972996A/en
Priority to JP8536785A priority patent/JPH11506332A/en
Publication of WO1996038591A1 publication Critical patent/WO1996038591A1/en

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    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/10Processes for the isolation, preparation or purification of DNA or RNA
    • C12N15/1096Processes for the isolation, preparation or purification of DNA or RNA cDNA Synthesis; Subtracted cDNA library construction, e.g. RT, RT-PCR
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/435Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
    • C07K14/46Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans from vertebrates
    • C07K14/47Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans from vertebrates from mammals
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/435Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
    • C07K14/705Receptors; Cell surface antigens; Cell surface determinants
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
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    • 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
    • C12N9/6472Cysteine endopeptidases (3.4.22)
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    • 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
    • C12Q1/6844Nucleic acid amplification reactions
    • C12Q1/686Polymerase chain reaction [PCR]
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K48/00Medicinal preparations containing genetic material which is inserted into cells of the living body to treat genetic diseases; Gene therapy
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2319/00Fusion polypeptide

Definitions

  • the present invention is in the field of molecular biology and more particularly, in the field of recombinant DNA technology.
  • PCR has become a widely used nucleic acid amplification technique since it was first presented by Kary Mullis at the Cold Spring Harbor Symposium (Mullis K et al (1986) Cold Spring Harbor Symp Quant Biol 51: 263-273) .
  • PCR requires that a pair of primers be generated from known sequences.
  • sequence is available only from one end of a DNA segment.
  • Several methods have been developed to sequence an entire gene once a partial nucleotide sequence is available. As more partial cDNA sequences become available in the world' s genetic databanks, more efficient and economical methods will be sought for then obtaining the complete gene.
  • PCR has become a widely used technique to complete genes for which a partial sequence is already known.
  • Gene-specific primers and primers located in the vector into which the cDNAs have been cloned are used for this purpose.
  • this method is limited by the use of primers complementary to vector sequence which is common to all clones in the library. This results in an abundance of non-specific PCR-products which have to be cloned and sequenced. Multiple rounds of amplifications with nested primers might be required. These additional operations increase the incorporation of errors.
  • Gobinda, Turner and Bolander (1993) in PCR Methods and Applications 2:318-22 disclose "restriction-site PCR" as a direct method of retrieving unknown sequence which is adjacent to a known locus by using universal primers.
  • genomic DNA is amplified in the presence of restriction site oligonucleotides and a primer specific to the known region.
  • those products are subjected to a second round of PCR with the same restriction site oligonucleotides and another specific primer internal to the first one.
  • the products of the last round of PCR are transcribed with an appropriate RNA polymerase and sequenced with a reverse transcriptase and an end-labeled specific primer internal to the second specific PCR primer.
  • Gobinda et al. present data concerning Factor IX for which they identified a conserved stretch of 20 nucleotides in the 3' noncoding region of the gene.
  • Inverse PCR is the first method that reported successful acquisition of unknown sequences starting with primers based on a known region (Triglia T, Peterson MG, and Kemp DJ (1988) Nucleic Acids Res. 16:8186) .
  • Inverse PCR employs a strategy in which several restriction enzymes are used to generate a suitable fragment in the known region. The segment is then circularized by intramolecular ligation and used as a PCR template with divergent primers created from the known region.
  • the requirement of multiple restriction enzyme digestions followed by multiple ligations make the procedure slow and expensive (Gobinda et al. Supra) .
  • Capture PCR first disclosed by Lagerstrom M, Parik J, Malmgren H, Stewart J, Patterson U and Landegren ⁇ (1991) PCR Methods Applic. 1:111-19, is a method for PCR amplification of DNA fragments adjacent to a known sequence in human and YAC DNA. As noted by Gobinda et al. supra, that method also requires multiple restriction enzyme digestions and ligation of an engineered double-stranded primer before PCR. Although the restriction and ligation reactions are carried out simultaneously in this method, the requirement of extension reaction, immobilization of the extended product, two rounds of PCR and purification of template prior to sequencing render it cumbersome and time consuming as well.
  • cDNA complementary DNA
  • This cDNAs are subsequently cloned into a vector (plasmid or Lambda) and amplified by transfection into E.coli cells resulting in a so-called cDNA library.
  • plasmid or Lambda plasmid or Lambda
  • the enzymes used in converting mRNA into cDNA are limited in their ability to produce complete copies of the existing mRNAs. This requires the researcher to isolate multiple cDNA clones of the gene of interest using specific probes and analyze each of these isolates for a complete cDNA of the gene of interest. This process is called screening of cDNA libraries.
  • the method may be used for extending known DNA sequences of genomic or cDNA origin.
  • the method utilizes the polymerase chain reaction (PCR) and includes the steps of: a) combining a first and second PCR primer with nucleic acid from a cDNA library, or pools of cDNA libraries, expected to contain said partial cDNA, or said partial cDNA that has been extended, or a genomic library, under conditions suitable for synthesis of nucleic acid PCR products from the first and second primers, wherein said first and second primers are capable of annealing to opposite strands of the partial cDNA or genomic DNA and initiating nucleic acid synthesis in an outward manner and wherein the first primer is capable of being extended by DNA polymerase in an antisense direction and the second primer is capable of being extended in a sense direction, b) purifying the PCR products, and c) identifying extended nucleotide sequences derived from said partial cDNA or said
  • the method of identifying the extended nucleotide sequences comprises nucleic acid sequencing. In another embodiment of the present invention, the method proceeds with repeating steps 6a through 6c on the nucleotide sequences identified in step 6c.
  • a method for extending the nucleotide sequence of a partial complementary DNA (cDNA) using polymerase chain reaction (PCR) comprising the steps of a) combining a first and second PCR primer with nucleic acid from a cDNA library, or pools of cDNA libraries, expected to contain said partial cDNA, or said partial cDNA that has been extended, or a genomic DNA library, under conditions suitable for synthesis of nucleic acid PCR products from the first and second primers, wherein said first and second primers are capable of annealing to- opposite strands of the partial cDNA and initiating nucleic acid synthesis in an outward manner and wherein the first primer is capable of being extended by DNA polymerase in an antisense direction and the second primer is capable of being extended in a sense direction, b) purifying the PCR products, c) ligating the purified PCR products under conditions suitable for the formation of circular, closed nucleic acid, d) transforming a host
  • the present invention also provides a method for extending known genomic DNA sequences which may be used for the detection and amplification of 5' untranslated nucleotide sequences and/or promoter sequences .
  • an isolated DNA molecule comprising SEQ ID NO:11, the DNA for a novel human purinergic P2U receptor.
  • Figure 1 is a flow chart of the steps in the inventive method.
  • Figure 2 shows a typical plasmid obtained from the excision process of a lambdaZAP cDNA library. Typically 250-300 base pairs of the sequence are obtained in the high-throughput sequence operation. The clone is partially sequenced from the 5' end with T3 as a sequencing primer.
  • Figure 3 is a representation of the next step, in which pBLUESCRIPT SK plasmids in a cDNA library are used as a template and the two specially designed primers (XLR and XLS) amplify plasmids containing the gene of interest. Only plasmids containing priming sites for both XL-PCR primers and the gene of interest will be amplified during the XL-PCR reaction.
  • Figure 4 is a representation of the amplified DNA segments which have been obtained through the XL-PCR reaction and consequently purified after separating the products on an agarose gel.
  • the cDNA library used as a template should be synthesized by random priming to assure the availability in this step of different amplified length of DNA (3' end) between the XLS priming site and the T7 priming site in the vector.
  • the length of the 5' end (between the XLR priming site and the T3 priming site) in the vector will vary in size depending on how much of the mRNA of the gene of interest had been converted into cDNA during the cDNA library synthesis.
  • Figure 5 shows how the purified DNA segments containing the plasmid and the gene of interest are religated to form a circular plasmid and transformed into bacteria for amplification.
  • chemically competent E. coli cells were transformed and grown on petri dishes containing LB agar and 25 mg/L carbenicillin (2XCarb) for antibiotic selection.
  • Figure 6 shows schematically how pure samples of clones were obtained from the different E. coli colonies grown in the procedure shown in Figure 5 (also Step 1 purification, Step 2 religation and Step 3 transformation in Figure 6) . These clones are screened in Step 4 for additional sequence of the gene of interest at the 5' end. For this purpose the clones were analyzed by a PCR reaction employing the XLR primer and the T3 vector primer. The size of the resulting product will indicate how much additional sequence upstream of the XLR priming site each clone contains.
  • Figures 7A through 7H show the results of the inventive method, in which a partial sequence from Incyte clone 14770, which was similar to heat shock protein 90, was successively sequenced to obtain a full-length cDNA.
  • Figures 8A through 8F show the results of the inventive method, in which a partial sequence from Incyte clone 87058 which was similar to cathepsin was successively sequenced to obtain extensions of the cDNA.
  • the present method provides a way to utilize a genomic DNA library or a plasmid cDNA library (either obtained by cloning cDNAs directly into a plasmid vector or by converting a Lambda library into a plasmid library by known methods e.g. Lambda ZAP excision or Lambda ZIPLOCK conversion) which has been used for sequencing cDNAs, as a source to obtain much longer DNAs and in certain cases complete genes of partially known DNA sequences.
  • a genomic DNA library or a plasmid cDNA library either obtained by cloning cDNAs directly into a plasmid vector or by converting a Lambda library into a plasmid library by known methods e.g. Lambda ZAP excision or Lambda ZIPLOCK conversion
  • This new method utilizes PCR kits which enable the researcher to amplify long pieces of DNA.
  • the XL-PCR amplification kit (Perkin-Elmer) was employed. However, equivalent products may be available from other major suppliers.
  • This novel method allows one person to process multiple genes (up to 96 genes) at a time and obtain extended or complete sequence (possibly full-length) of the cDNAs of interest within 6-10 days. This compares very favorably with current competitive methods like screening with labelled probes which allow one worker to process only about 3-5 genes and obtain initial results in 14-40 days. This represents an increase in throughput of at least 1000%.
  • primer design and synthesis (based on a known partial sequence) can be performed in about two days.
  • the PCR amplification can be performed in 6-8 hours.
  • Multiple libraries can be pooled and therefore screened at the same time.
  • the next steps of purification and ligation take about one day.
  • transformation and growing up the bacteria take one day.
  • screening for clones with additional sequence of the genes of interest by PCR takes approximately five hours.
  • the next steps of DNA preparation and sequencing of the selected clones can be performed in about one day. This totals 6-7 days.
  • This method presumes that one already has partial cDNA sequences, either from a publicly available database or the scientist' s own earlier research, including but not limited to earlier preparation of a cDNA library whose cDNAs have been partially sequenced.
  • the cDNA library may have been prepared with oligo dT or random primers.
  • the difference between oligo dT and randomly primed libraries is that a randomly primed library will have more sequences which contain 5' ends of cDNAs.
  • a randomly primed library may be particularly useful for further work when the oligo dT library does not yield a complete gene. Random priming of the library also helps yield more cDNA sequences of different lengths. Library preparation techniques which promote longer insert sizes will in turn permit the sequencing of more complete cDNAs. Obviously, the larger the protein, the less likely it is that the complete cDNA will be found in a single plasmid.
  • Figure 2 shows a typical plasmid containing a cDNA which had been partially sequenced from the 5' end with T3 as a primer.
  • the top darkened portion represents the insert containing the gene of interest.
  • Step 1 PCR-amplification of cDNA-clones containing the ⁇ ene of interest
  • the first step of this method requires the design of two primers based on the known sequence.
  • the known sequence can be obtained by those skilled in the art either by a wet lab method or from the many publicly available DNA databases.
  • One primer is synthesized to be extended in an antisense direction (XLR) and the other in the sense direction (XLS or XLF) .
  • XLR antisense direction
  • XLS sense direction
  • XLF sense direction
  • the primers are designed to anneal to either end of the known sequence and to be extended "outward" from there to generate amplicons containing new, unknown sequences of the genes of interest. This is different from typical PCR, in which the primers are designed to amplify a known sequence in a direction "inward" toward each other.
  • primers need to be designed in a way displaying optimal criteria for extra long PCR.
  • a program like Oligo 4.0s can be employed for this purpose.
  • primers should be 22-30 nucleotides in length, consist of a GC content of 50% or more and anneal at 68°C-72°C to the target. Hairpin structures and primer-primer dimerizations must be avoided. Primers varying from the conditions described above may result in amplification of the desired targets providing extension conditions have been adjusted.
  • Figure 3 shows the next step, in which a cDNA library is used as a template and the two primers (XLR and XLS) amplify plasmids containing the gene of interest.
  • a cDNA library is used as a template and the two primers (XLR and XLS) amplify plasmids containing the gene of interest.
  • XLR and XLS primers
  • PCR enzymes which provide high fidelity and copy long sequences, such as that provided in the XL-PCR kit (Part No.
  • kit instructions should be followed, including suggestions to optimize concentrations of various reagents. In the examples disclosed infra, 25pMol of each primer worked well. Template (plasmid library) concentrations can be varied (see Examples infra for details) . It is essential to thoroughly resuspend the enzyme in solution prior to use, especially if the solution has been stored at -20°C. If the enzyme is not adequately resuspended, its effectiveness is impaired.
  • the preferred system is setup initially in two layers, employing Ampliwax" PCR Gems. However, efficiency can be increased by avoiding the use of these Gems and initiating amplification by using the "hot-start” technique by adding Magnesium, which is essential for amplification, at 82° C.
  • thermocycler MJ Research, Watertown, MA
  • Times and temperatures may be varied to optimize conditions in different thermocyclers.
  • Step 1 94° for 60 sec (initial denaturation)
  • Step 2 94° for 15 sec
  • Step 5 Repeat step 2-4 for 15 additional times
  • Step 6 94° for 15 sec
  • Step 7 65° for 1 min
  • Step 8 68° for 7 min + 15 sec/cycle
  • Step 9 Repeat step 6-8 for 11 additional times
  • Step 11 4° for 0.00 sec (to hold at 4°) At the end of these 28 cycles, 50 ⁇ l of the reaction mix is removed; on the remaining reaction mix, an additional 10 additional cycles are run, as outlined below:
  • Step 1 94° for 15 sec
  • Step 2 65° for 1 min
  • Step 3 68° for (10 min + 15 sec) /cycle
  • Step 4 Repeat step 1-3 for 9 additional times
  • Step 5 72° for 10 min
  • a 5-10 ⁇ l aliquot of the reaction mixture can be analyzed on a mini-gel to determine which reactions were successful.
  • Step 2 Purification of amplicons containing the ⁇ ene of interest
  • Figure 4 is a graphical representation of the amplified cDNA segments which have been separated on an agarose gel. Note that there are a variety of lengths of cDNA. Although the rest of the method could be performed using all extended cDNA species, the method can proceed optionally after selecting the largest products (likeliest to provide the remainder of the full-length gene) . Some of the larger species may in fact be hybrid clones which contain two cDNA inserts as a result of malfunction during the cDNA library construction which may represent an incomplete digestion with the restriction enzyme at the end of the cDNA synthesis. Such amplified hybrid clones, also called chimera, could result in overlooking the correct targeted extensions.
  • Successful reaction products should be purified on an agarose gel (preferentally low agarose concentrations 0.6-0.8% should be used) or other appropriate method.
  • An appropriate volume of reaction mixture should be loaded to obtain good separation of the products and to separate them from the plasmid library (template) still in the reaction mixture. Contamination with the template cDNA library will result in transformants which don't contain the desired gene and will require an extensive screening of many colonies.
  • the bands representing the genes of interest are then cut out of the gel and purified using a method like the QIAQuick gel extraction kit (Qiagen, Inc., Chatsworth, CA) .
  • Step 3 Cloning of amplicons containing the gene of interest Eventual overhangs are converted into blunt ends to facilitate religation and cloning of the products.
  • Klenow enzyme (3 units/reaction mixture) and dNTP' s (0.2 mM final concentration) are added and the reaction is incubated at room temperature for 30 min. The Klenow enzyme is then inactivated by incubating the reaction at 75° for 15 min.
  • Step 4 Screening of cloned products
  • each well contains 150ml of LB/2XCarb medium.
  • each row of the microtiter plate contains twelve clones from the same extension reaction.
  • the cells are grown over night at 37°C.
  • 5 ⁇ l of these overnight cultures are tranferred into a non-sterile 96-well plate (Falcon 3911 Microtest IIITM, Flexible Assay Plate, Becton Dickinson, Oxnard, CA) and diluted 1:10 with water. 5 ⁇ l of each dilution are then transferred into a PCR array (e.g., Cycleplate, Robbins Scientific Corp., Sunnyvale, CA) .
  • a PCR array e.g., Cycleplate, Robbins Scientific Corp., Sunnyvale, CA
  • Amplification generally was performed using the following conditions:
  • Step 1 9 °C for 60sec
  • Step 2 94°C for 20sec
  • Step 5 repeat steps 2-4 for an additional 29 times
  • Step 6 72°C for 180sec Step 7 4°C for ever
  • PCR products will allow direct determination of how much additional sequence the selected clones contain compared to the original partial cDNA. The efficiency of the method has been further improved by using the resulting PCR-products directly for sequencing thus avoiding the necessity of preparing plasmids.
  • the appropriate clones are selected and grown for plasmid preparation and sequencing. Plasmid preparations are made with standard kits familiar to those skilled in the art. Examples include the PROMEGA Magic
  • Sequencing is performed employing standard automated ABI sequencing equipment and protocols using either dye-primer or dye-terminator kits.
  • Sequence processing and assemblage of the sequencing data are performed using standard ABI software, including INHERITTM analysis and the Power assembler.
  • INHERITTM analysis and the Power assembler.
  • a THP-1 cDNA library constructed into the LambdaZAP vector (Stratagene) was converted into a plasmid library following the mass excision protocol. Plasmids of the excised libraries were prepared using the Quiagen Midi plasmid purification kit. 1.3 XL-PCR reaction set-up
  • the extension reactions were prepared following the instructions provided with the GeneAmp XL PCR Kit (Part No. N808-0182) from Perkin Elmer.
  • a two layer system was set up as follows: The lower reagent mix was prepared by pipetting the following components into a 0.2ml MicroAmp reaction tube.
  • Lower reagent mix preparation ⁇ Water 13.6 ⁇ l 3.3X buffer 12.0 ⁇ l dATP (lOmM) 2.0 ⁇ l dCTP (lOmM) 2.0 ⁇ l dGTP (lOmM) 2.0 ⁇ l dTTP (lOmM) 2.0 ⁇ l
  • the template DNA (excised library) was diluted to an appropriate concentration in water and then added to the upper mix. Mixing of the components is not necessary.
  • Step 1 94° for 60 sec (initial denaturation)
  • Step 2 94° for 15 sec
  • Step 4 68° for 7 min
  • Step 5 Repeat step 2-4 for 15 additional times
  • Step 8 68° for 7 min + 15 sec/cycle
  • Step 9 Repeat step 6-8 for 11 additional times Step 10 72° for 8 min
  • Step 11 4° for 0.00 sec (to hold at 4°)
  • Klenow enzyme (3 units/reaction) and dNTP's (0.2mM final concentration) were added and the reactions were incubated at room temperature for 30 min followed by incubation at 75° C for 15 min. The products were then ethanol precipitated and redissolved in 13 ⁇ l of ligation buffer containing ImM ATP.
  • T4-DNA ligase (15 units) and T4 Polynucleotide kinase (5 units) were added, and the reaction was incubated at room temperature for 3 hours. 3 ⁇ l of the ligation mixture were transformed into 40 ml of competent E.coli cells. After heatshocking the cells at 42° C for 45 seconds, 80 ⁇ l of SOC medium were added, and the cells were allowed to recover at 37° C for 1 hour. The whole transformation mixture then was plated on LB-agar/2XCarb-containing petri dish plates.
  • the 1.33 x concentrated PCR mix contained the following components: 10X PCR-buffer 2.0 ⁇ l
  • Step 1 94° C for 60sec
  • Step 2 94° C for 20sec
  • Step 3 55° C for 30sec
  • Step 4 72° C for 90sec
  • Step 5 repeat steps 2-4 for an additional 29 times Step 6 72° C for 180 sec Step 7 4° C for ever
  • the DNA of the selected clones was prepared using the WizardTM Minipreps DNA Purification System (Promega Corporation, Madison, WI) following the instructions of the manufacturer. Sequencing reactions were performed using the PRISMTM Ready Reaction DyeDeoxy Terminator Cycle Sequencing Kit (Part No 401628, Perkin Elmer, Applied Biosystems, Foster City, CA) . 1.9 Analysis of sequenced products
  • FIG. 14A-7H shows an alignment of the obtained sequences with the published human Hsp 90 nucleotide sequence.
  • Clones 14201.3 and 14201.5 contain part of the 5' untranslated region and therefore the full coding region of the gene has been obtained.
  • Example 2 For further method evaluation, a second known gene was selected. A partial sequence from a liver library was found to be related to that of the human cathepsin B gene (accession L16510, HUMCATHB, SEQ ID NO: 6) . This partial sequence (Incyte clone 87058, SEQ ID NO:7) initiated at base 1066 of the sequence with accession number L16510.
  • the extension reactions were prepared following the instructions provided with the GeneAmp XL PCR Kit (Part No. N808-0182) from Perkin Elmer. A two layer system was set up as described below. The lower reagent mix was prepared by pipetting the following components into a 0.2ml MicroAmp reaction tube. Lower reagent mix preparation:
  • the template DNA (excised library) was diluted to an appropriate concentration in water and then added to the upper mix. Mixing of the components is not necessary. Template (6.25ng/ ⁇ l) 40.0 ⁇ l
  • Step 1 94° for 60 sec (initial denaturation)
  • Step 2 94° for 15 sec
  • Step 5 Repeat step 2-4 for 15 additional times
  • Step 6 94° for 15 sec
  • Step 7 65° for 1 min
  • Step 8 68° for 7 min + 15 sec/cycle
  • Step 9 Repeat step 6-8 for 11 additional times
  • Step 11 4° for 0.00 sec (to hold at 4° ) 2.5 Purification of amplified products
  • T4-DNA ligase (15 units) and T4 Polynucleotide kinase (5 units) were added, and the reaction was incubated at room temperature for 3 hours.
  • the 1.33 x concentrated PCR mix contained the following components:
  • Step 1 94°C for 60sec Step 2 94°C for 20sec Step 3 55°C for 30sec Step 4 72°C for 90sec Step 5 repeat steps 2-4 for an additional 29 times Step 6 72°C for 180sec Step 7 4°C for ever
  • the DNA of the selected clones was prepared using the WizardTM Minipreps DNA Purification System (Promega Corporation, Madison, WI) following the instructions of the manufacturer. Sequencing reactions were performed using the PRISMTM Ready Reaction DyeDeoxy Terminator Cycle Sequencing Kit (Part No 401628, Perkin Elmer, Applied Biosystems, Foster City, CA) .
  • Figures 8A through 8F show an alignment of the obtained sequences with the published human Hsp 90 nucleotide sequence.
  • Clone 87058.16 contains part of the 5'UT and therefore the full coding region of the gene.
  • Example 3 In Example 3, a full length cDNA (Seq ID NO 11) of a novel P2U purinergic receptor homolog was obtained by the inventive method and is the subject of U.S. Patent Application 08/459,046 filed June 2, 1995, which is hereby incorporated by reference.
  • Incyte Clone 179696 was extended to full length using a modified XL-PCR (Perkin Elmer) procedure. Primers were designed based on known sequence; one primer was synthesized to initiate extension in the antisense direction (XLR) and the other to extend sequence in the sense direction (XLF) .
  • XLR antisense direction
  • XLF sense direction
  • the primers allowed the sequence to be extended "outward" from the known sequence, thus generating amplicons containing new, unknown nucleotide sequence comprising the gene of interest.
  • the primers were designed using Oligo 4.0 (National Biosciences Ine, Plymouth MN) to be 22-30 nucleotides in length, to have a GC content of 50% or more, and to anneal to the target sequence at temperatures about 68°-72° C. Any stretch of nucleotides which would result in hairpin structures and primer-primer dimerizations was avoided.
  • cDNA library was used as a template, and XLR (bases 278-298) and XLF (bases 587-610) primers were used to extend and amplify the 179696 sequence.
  • XLR bases 278-298
  • XLF bases 587-610
  • Step 3 65° C for 1 min
  • Step 4 68° C for 7 min
  • Step 5 Repeat step 2-4 for 15 additional cycles
  • Step 7 65° C for 1 min
  • Step 8 68° C for 7 min + 15 sec/cycle
  • Step 9 Repeat step 6-8 for 11 additional cycles
  • Step 1 94° C for 15 sec
  • Step 3 68° C for (10 min + 15 sec) /cycle
  • Step 4 Repeat step 1-3 for 9 additional cycles
  • Competent E. coli cells (in 40 ⁇ l of appropriate media) were transformed with 3 ⁇ l of ligation mixture and cultured in 80 ⁇ l of
  • Step 1 94° C for 60 sec
  • Step 2 94° C for 20 sec
  • Step 3 55° C for 30 sec
  • Step 4 72° C for 90 sec
  • Step 5 Repeat steps 2-4 for an additional 29 cycles
  • Step 6 72° C for 180 sec
  • Step 7 4° C (and holding)
  • the inventive method was used to obtain a novel full length cDNA from the partial sequence found in Incyte clone 08118 which was found to be somewhat homologous to the GenBank sequence of C5a anaphylatoxin receptor, a G-protein coupled surface receptor from dog (Perret J et al (1995) Biochem J 288:911-17) .
  • Example 3 Essentially the same method outlined in Example 3 above was used to extend the partial sequence of 8118 to obtain the full length sequence (Seq ID NO:12) of a novel C5a-like receptor homolog which is the subject of a U.S. Patent Application 08/462,355 filed June 5, 1995, and whose disclosure is incorporated by reference.
  • CTATTTATTC CTCGTCGGGC TCCCTTTGAC CTTTTTGAGA ACAAGAAGAA AAAGAACAAC 1140
  • GAGATTTTCC TTCGGGAGTT GATCTCTAAT GCTTCTGATG CCTTGGACAA GATTCGCTAT 240
  • CATGCTGTGG CAGATGTGTGTG GGGACGGCTG TAATGGTGGC TATCCTGCTG AAGCTTGGAC 300
  • ATCATTGTCC TCAACATGTT TGGCAGTGTC TTCCTGCTTA CTGCCATTAG CCTGGATCGC 360
  • GGCCAATTCA CAGATGACGA TCAAGTGCCA ACACCCCTCG TGGCAATAAC GATCACTAGG 1020
  • CTAGTGGTGG GTTTCCTGCT GCCCTCTGTT ATCATGATAG CCTGTTACAG CTTCATTGTC 1080

Abstract

A method for obtaining longer cDNA sequences is provided. The method utilizes a known genomic DNA sequence or a partial cDNA sequence, such as can be obtained from GenBank partial cDNAs. Two PCR primers are designed to correspond to the ends of the known partial sequence and to anneal to DNA in a cDNA library so as to initiate extension away from the known cDNA and the other primer. The primers are added to a cDNA library with appropriate enzymes and extend through additional DNA sequence to produce PCR products, which are subsequently purified and sequenced to provide new sequences. The new sequences are then compared with the known partial cDNA sequence for areas of overlap, and the sequence is extended beyond the overlapping areas to provide longer DNA sequence.

Description

IMPROVED METHOD FOR OBTAINING FOLL-LENGTH cDNA SEQUENCES
TECHNICAL FIELD
The present invention is in the field of molecular biology and more particularly, in the field of recombinant DNA technology.
BACKGROUND ART
PCR has become a widely used nucleic acid amplification technique since it was first presented by Kary Mullis at the Cold Spring Harbor Symposium (Mullis K et al (1986) Cold Spring Harbor Symp Quant Biol 51: 263-273) . PCR requires that a pair of primers be generated from known sequences. However, in many cases, sequence is available only from one end of a DNA segment. Several methods have been developed to sequence an entire gene once a partial nucleotide sequence is available. As more partial cDNA sequences become available in the world' s genetic databanks, more efficient and economical methods will be sought for then obtaining the complete gene.
PCR has become a widely used technique to complete genes for which a partial sequence is already known. Gene-specific primers and primers located in the vector into which the cDNAs have been cloned are used for this purpose. However, this method is limited by the use of primers complementary to vector sequence which is common to all clones in the library. This results in an abundance of non-specific PCR-products which have to be cloned and sequenced. Multiple rounds of amplifications with nested primers might be required. These additional operations increase the incorporation of errors.
Gobinda, Turner and Bolander (1993) in PCR Methods and Applications 2:318-22 disclose "restriction-site PCR" as a direct method of retrieving unknown sequence which is adjacent to a known locus by using universal primers. First, genomic DNA is amplified in the presence of restriction site oligonucleotides and a primer specific to the known region. Next, those products are subjected to a second round of PCR with the same restriction site oligonucleotides and another specific primer internal to the first one. Subsequently, the products of the last round of PCR are transcribed with an appropriate RNA polymerase and sequenced with a reverse transcriptase and an end-labeled specific primer internal to the second specific PCR primer. Gobinda et al. present data concerning Factor IX for which they identified a conserved stretch of 20 nucleotides in the 3' noncoding region of the gene.
Inverse PCR is the first method that reported successful acquisition of unknown sequences starting with primers based on a known region (Triglia T, Peterson MG, and Kemp DJ (1988) Nucleic Acids Res. 16:8186) . Inverse PCR employs a strategy in which several restriction enzymes are used to generate a suitable fragment in the known region. The segment is then circularized by intramolecular ligation and used as a PCR template with divergent primers created from the known region. However, the requirement of multiple restriction enzyme digestions followed by multiple ligations (even before PCR is started) make the procedure slow and expensive (Gobinda et al. Supra) .
Capture PCR, first disclosed by Lagerstrom M, Parik J, Malmgren H, Stewart J, Patterson U and Landegren ϋ (1991) PCR Methods Applic. 1:111-19, is a method for PCR amplification of DNA fragments adjacent to a known sequence in human and YAC DNA. As noted by Gobinda et al. supra, that method also requires multiple restriction enzyme digestions and ligation of an engineered double-stranded primer before PCR. Although the restriction and ligation reactions are carried out simultaneously in this method, the requirement of extension reaction, immobilization of the extended product, two rounds of PCR and purification of template prior to sequencing render it cumbersome and time consuming as well. Walking PCR, disclosed by Parker JD, Rabinovitch PS, and Burmer GC (1991) Nucleic Acids Res 19:3055-60, teaches a method for targeted gene walking via PCR. Although this method also permits retrieval of unknown sequence, Gobinda et al, supra, note that it requires oligomer-extension assay followed by identification and gel purification of the desired band prior to sequencing. Such extra steps again limit the applicability of the method.
The enzymes originally used in PCR were limited in their ability to reliably amplify long pieces of nucleic acids over 3kb. One of the explanations for this limitation seems to be the misincorporation of nucleotides resulting in non-basepairing mismatches which these enzymes often fail to extend.
Only the mixture of two enzymes, rTth DNA-Polymerase and Vent, the latter of which has so-called "proofreading" activity, and the optimization of amplification conditions finally overcame this limitation and made amplification of pieces of DNA of up to 40kb possible.
The most co mon way to identify genes expressed in a certain tissue at a certain time is the isolation of the mRNA of that particular tissue and the conversion of this mRNA into so-called cDNA (complementary DNA) . This cDNAs are subsequently cloned into a vector (plasmid or Lambda) and amplified by transfection into E.coli cells resulting in a so-called cDNA library. First and most important to researchers attempting to obtain a complete gene is that the enzymes used in converting mRNA into cDNA are limited in their ability to produce complete copies of the existing mRNAs. This requires the researcher to isolate multiple cDNA clones of the gene of interest using specific probes and analyze each of these isolates for a complete cDNA of the gene of interest. This process is called screening of cDNA libraries.
A major problem facing molecular biologists is finding the most efficient method to use to obtain a full-length cDNA from a partial sequence. Such sequences are appearing with increasing frequency in GenBank, from commercial cDNA libraries and privately prepared libraries. The inventive method disclosed herein is a contribution to that art. DISCLOSURE OF THE INVENTION
An improved method for extending the DNA sequence of a known fragment of DNA sequence is provided. The method may be used for extending known DNA sequences of genomic or cDNA origin. The method utilizes the polymerase chain reaction (PCR) and includes the steps of: a) combining a first and second PCR primer with nucleic acid from a cDNA library, or pools of cDNA libraries, expected to contain said partial cDNA, or said partial cDNA that has been extended, or a genomic library, under conditions suitable for synthesis of nucleic acid PCR products from the first and second primers, wherein said first and second primers are capable of annealing to opposite strands of the partial cDNA or genomic DNA and initiating nucleic acid synthesis in an outward manner and wherein the first primer is capable of being extended by DNA polymerase in an antisense direction and the second primer is capable of being extended in a sense direction, b) purifying the PCR products, and c) identifying extended nucleotide sequences derived from said partial cDNA or said genomic DNA. In one embodiment of the present invention, the method of identifying the extended nucleotide sequences comprises nucleic acid sequencing. In another embodiment of the present invention, the method proceeds with repeating steps 6a through 6c on the nucleotide sequences identified in step 6c. In another embodiment of the present invention, there is a method for extending the nucleotide sequence of a partial complementary DNA (cDNA) using polymerase chain reaction (PCR) , comprising the steps of a) combining a first and second PCR primer with nucleic acid from a cDNA library, or pools of cDNA libraries, expected to contain said partial cDNA, or said partial cDNA that has been extended, or a genomic DNA library, under conditions suitable for synthesis of nucleic acid PCR products from the first and second primers, wherein said first and second primers are capable of annealing to- opposite strands of the partial cDNA and initiating nucleic acid synthesis in an outward manner and wherein the first primer is capable of being extended by DNA polymerase in an antisense direction and the second primer is capable of being extended in a sense direction, b) purifying the PCR products, c) ligating the purified PCR products under conditions suitable for the formation of circular, closed nucleic acid, d) transforming a host cell with the circular, closed nucleic acid and culturing the transformed host cell under conditions suitable for growth, e) recovering said circular closed nucleic acid from the cultured, transformed host cell, and f) identifying extended nucleotide sequences derived from said partial cDNA or said genomic DNA.
The present invention also provides a method for extending known genomic DNA sequences which may be used for the detection and amplification of 5' untranslated nucleotide sequences and/or promoter sequences . . Also provided is an isolated DNA molecule comprising SEQ ID NO:11, the DNA for a novel human purinergic P2U receptor.
Also provided is an isolated DNA molecule comprising SEQ ID NO: 12, the DNA for a novel human C5a-like seven transmembrane receptor. These and other objects, advantages and features of the present invention will become apparent to those persons skilled in the art upon reading the details of the structure, synthesis, formulation and usage as more fully set forth below, reference being made to the accompanying figures forming a part hereof.
BRIEF DESCRIPTION OF DRAWINGS
Figure 1 is a flow chart of the steps in the inventive method. Figure 2 shows a typical plasmid obtained from the excision process of a lambdaZAP cDNA library. Typically 250-300 base pairs of the sequence are obtained in the high-throughput sequence operation. The clone is partially sequenced from the 5' end with T3 as a sequencing primer. Figure 3 is a representation of the next step, in which pBLUESCRIPT SK plasmids in a cDNA library are used as a template and the two specially designed primers (XLR and XLS) amplify plasmids containing the gene of interest. Only plasmids containing priming sites for both XL-PCR primers and the gene of interest will be amplified during the XL-PCR reaction.
Figure 4 is a representation of the amplified DNA segments which have been obtained through the XL-PCR reaction and consequently purified after separating the products on an agarose gel. For best results, the cDNA library used as a template should be synthesized by random priming to assure the availability in this step of different amplified length of DNA (3' end) between the XLS priming site and the T7 priming site in the vector. The length of the 5' end (between the XLR priming site and the T3 priming site) in the vector will vary in size depending on how much of the mRNA of the gene of interest had been converted into cDNA during the cDNA library synthesis.
Figure 5 shows how the purified DNA segments containing the plasmid and the gene of interest are religated to form a circular plasmid and transformed into bacteria for amplification. Here chemically competent E. coli cells were transformed and grown on petri dishes containing LB agar and 25 mg/L carbenicillin (2XCarb) for antibiotic selection.
Figure 6 shows schematically how pure samples of clones were obtained from the different E. coli colonies grown in the procedure shown in Figure 5 (also Step 1 purification, Step 2 religation and Step 3 transformation in Figure 6) . These clones are screened in Step 4 for additional sequence of the gene of interest at the 5' end. For this purpose the clones were analyzed by a PCR reaction employing the XLR primer and the T3 vector primer. The size of the resulting product will indicate how much additional sequence upstream of the XLR priming site each clone contains. Figures 7A through 7H show the results of the inventive method, in which a partial sequence from Incyte clone 14770, which was similar to heat shock protein 90, was successively sequenced to obtain a full-length cDNA.
Figures 8A through 8F show the results of the inventive method, in which a partial sequence from Incyte clone 87058 which was similar to cathepsin was successively sequenced to obtain extensions of the cDNA.
MODES FOR CARRYING OUT THE INVENTION Unless defined otherwise, all technical and scientific terms used herein have the same meaning as is commonly understood by one of skill in the art to which this invention belongs . All patents and publications referred to herein are incorporated by reference herein.
Before the present compounds, variants, formulations and methods for making and using such are described, it is to be understood that this invention is not limited to the particular compounds, variants, formulations or methods described, as such enzymes, formulations and methodologies may, of course, vary. The terminology used herein is for the purpose of describing particular embodiments only and is not intended to be limiting since the scope of protection will be limited only by the appended claims.
In the specification and appended claims, the singular forms "a", "an" and "the" include plural referents unless the context clearly dictates otherwise. Thus, for example, reference to "a high-fidelity PCR enzyme" includes mixtures of such enzymes and any other enzymes fitting the stated criteria, reference to the method includes reference to one or more methods for obtaining full-length cDNA sequences which will be known to those skilled in the art or will become known to them upon reading this specification.
The present method provides a way to utilize a genomic DNA library or a plasmid cDNA library (either obtained by cloning cDNAs directly into a plasmid vector or by converting a Lambda library into a plasmid library by known methods e.g. Lambda ZAP excision or Lambda ZIPLOCK conversion) which has been used for sequencing cDNAs, as a source to obtain much longer DNAs and in certain cases complete genes of partially known DNA sequences.
The steps disclosed herein are based on cDNA libraries but equally apply to genomic DNA libraries.
This new method utilizes PCR kits which enable the researcher to amplify long pieces of DNA. The XL-PCR amplification kit (Perkin-Elmer) was employed. However, equivalent products may be available from other major suppliers. This novel method allows one person to process multiple genes (up to 96 genes) at a time and obtain extended or complete sequence (possibly full-length) of the cDNAs of interest within 6-10 days. This compares very favorably with current competitive methods like screening with labelled probes which allow one worker to process only about 3-5 genes and obtain initial results in 14-40 days. This represents an increase in throughput of at least 1000%.
This increased efficiency is possible because of the inventive combination of steps shown in the flow chart (Figure 1) . First, primer design and synthesis (based on a known partial sequence) can be performed in about two days. The PCR amplification can be performed in 6-8 hours. Multiple libraries can be pooled and therefore screened at the same time. The next steps of purification and ligation take about one day. Then transformation and growing up the bacteria take one day. Then screening for clones with additional sequence of the genes of interest by PCR takes approximately five hours. The next steps of DNA preparation and sequencing of the selected clones can be performed in about one day. This totals 6-7 days. At the end of this time, one has usually obtained a much longer cDNA sequence, assuming such a longer cDNA existed in the libraries than what was initially sequenced. If the new sequence is a complete gene, then the goal has been reached. If the complete sequence has not been obtained, one still has a much longer sequence than before, and this longer sequence can be used to design primers to repeat the procedure on the same or another library. The choice of library is up to the researcher, but a preferred library is one that has been size-selected to include only larger cDNAs.
This method presumes that one already has partial cDNA sequences, either from a publicly available database or the scientist' s own earlier research, including but not limited to earlier preparation of a cDNA library whose cDNAs have been partially sequenced. The cDNA library may have been prepared with oligo dT or random primers. The difference between oligo dT and randomly primed libraries is that a randomly primed library will have more sequences which contain 5' ends of cDNAs. A randomly primed library may be particularly useful for further work when the oligo dT library does not yield a complete gene. Random priming of the library also helps yield more cDNA sequences of different lengths. Library preparation techniques which promote longer insert sizes will in turn permit the sequencing of more complete cDNAs. Obviously, the larger the protein, the less likely it is that the complete cDNA will be found in a single plasmid.
Figure 2 shows a typical plasmid containing a cDNA which had been partially sequenced from the 5' end with T3 as a primer. The top darkened portion represents the insert containing the gene of interest.
Step 1: PCR-amplification of cDNA-clones containing the σene of interest
The first step of this method requires the design of two primers based on the known sequence. The known sequence can be obtained by those skilled in the art either by a wet lab method or from the many publicly available DNA databases. One primer is synthesized to be extended in an antisense direction (XLR) and the other in the sense direction (XLS or XLF) . In effect, the primers are designed to anneal to either end of the known sequence and to be extended "outward" from there to generate amplicons containing new, unknown sequences of the genes of interest. This is different from typical PCR, in which the primers are designed to amplify a known sequence in a direction "inward" toward each other.
The primers need to be designed in a way displaying optimal criteria for extra long PCR. A program like Oligo 4.0s (National Biosciences, Inc., Plymouth MN) can be employed for this purpose. In general primers should be 22-30 nucleotides in length, consist of a GC content of 50% or more and anneal at 68°C-72°C to the target. Hairpin structures and primer-primer dimerizations must be avoided. Primers varying from the conditions described above may result in amplification of the desired targets providing extension conditions have been adjusted.
Figure 3 shows the next step, in which a cDNA library is used as a template and the two primers (XLR and XLS) amplify plasmids containing the gene of interest. In this step, it is very helpful to use PCR enzymes which provide high fidelity and copy long sequences, such as that provided in the XL-PCR kit (Part No.
N808-0182, Perkin Elmer, Applied Biosystems, Foster City, CA) . Generally, kit instructions should be followed, including suggestions to optimize concentrations of various reagents. In the examples disclosed infra, 25pMol of each primer worked well. Template (plasmid library) concentrations can be varied (see Examples infra for details) . It is essential to thoroughly resuspend the enzyme in solution prior to use, especially if the solution has been stored at -20°C. If the enzyme is not adequately resuspended, its effectiveness is impaired. The preferred system is setup initially in two layers, employing Ampliwax" PCR Gems. However, efficiency can be increased by avoiding the use of these Gems and initiating amplification by using the "hot-start" technique by adding Magnesium, which is essential for amplification, at 82° C.
Although various cycling conditions are detailed in the examples infra , the following cycling conditions have been found to be optimal with the MJ PCT200 thermocycler (MJ Research, Watertown, MA) . Times and temperatures may be varied to optimize conditions in different thermocyclers.
Step 1 94° for 60 sec (initial denaturation) Step 2 94° for 15 sec
Step 3 65° for 1 min
Step 4 68° for 7 min
Step 5 Repeat step 2-4 for 15 additional times
Step 6 94° for 15 sec Step 7 65° for 1 min
Step 8 68° for 7 min + 15 sec/cycle
Step 9 Repeat step 6-8 for 11 additional times
Step 10 72° for 8 min
Step 11 4° for 0.00 sec (to hold at 4°) At the end of these 28 cycles, 50 μl of the reaction mix is removed; on the remaining reaction mix, an additional 10 additional cycles are run, as outlined below:
Step 1 94° for 15 sec Step 2 65° for 1 min
Step 3 68° for (10 min + 15 sec) /cycle
Step 4 Repeat step 1-3 for 9 additional times
Step 5 72° for 10 min Next a 5-10 μl aliquot of the reaction mixture can be analyzed on a mini-gel to determine which reactions were successful.
Step 2: Purification of amplicons containing the σene of interest Figure 4 is a graphical representation of the amplified cDNA segments which have been separated on an agarose gel. Note that there are a variety of lengths of cDNA. Although the rest of the method could be performed using all extended cDNA species, the method can proceed optionally after selecting the largest products (likeliest to provide the remainder of the full-length gene) . Some of the larger species may in fact be hybrid clones which contain two cDNA inserts as a result of malfunction during the cDNA library construction which may represent an incomplete digestion with the restriction enzyme at the end of the cDNA synthesis. Such amplified hybrid clones, also called chimera, could result in overlooking the correct targeted extensions.
Successful reaction products should be purified on an agarose gel (preferentally low agarose concentrations 0.6-0.8% should be used) or other appropriate method. An appropriate volume of reaction mixture should be loaded to obtain good separation of the products and to separate them from the plasmid library (template) still in the reaction mixture. Contamination with the template cDNA library will result in transformants which don't contain the desired gene and will require an extensive screening of many colonies. The bands representing the genes of interest are then cut out of the gel and purified using a method like the QIAQuick gel extraction kit (Qiagen, Inc., Chatsworth, CA) . Step 3 : Cloning of amplicons containing the gene of interest Eventual overhangs are converted into blunt ends to facilitate religation and cloning of the products. For this purpose, Klenow enzyme (3 units/reaction mixture) and dNTP' s (0.2 mM final concentration) are added and the reaction is incubated at room temperature for 30 min. The Klenow enzyme is then inactivated by incubating the reaction at 75° for 15 min.
The products are then ethanol precipitated and redissolved in
13 μl of ligation buffer containing 1 mM ATP. 1ml T4-DNA ligase (15 units) and T4 Polynucleotide kinase (5 units) are added and the reaction is incubated at room temperature for 2-3 hours or overnight at 16°C.
3μl of the ligation mixture are transformed into 40ml of competent E.coli cells (prepared with a standard protocol) . 80μl of SOC medium are added and after 1 hour of recovery of the cells at 37°C the whole transformation mixture is plated on LB-agar 2XCarb-containing petri plates. Step 4 : Screening of cloned products
The next day 8 or 12 colonies are randomly picked from each plate and grown in individual wells of a sterile 96-well microtiter plate (e.g. 96 Well Cell Culture Cluster, Catalog No.
3799, Costar Corp., Cambridge, MA 02140), Each well contains 150ml of LB/2XCarb medium. Thus, each row of the microtiter plate contains twelve clones from the same extension reaction. The cells are grown over night at 37°C. The next day, 5 μl of these overnight cultures are tranferred into a non-sterile 96-well plate (Falcon 3911 Microtest III™, Flexible Assay Plate, Becton Dickinson, Oxnard, CA) and diluted 1:10 with water. 5μl of each dilution are then transferred into a PCR array (e.g., Cycleplate, Robbins Scientific Corp., Sunnyvale, CA) . To obtain a IX final concentration of PCR reagents, 15 μl of a 1.33X concentrated PCR mix are added to each well. Another way of efficient screening for extension products is the multiplex PCR method where multiple specific primers are pooled and submitted to the same reaction, therefore increasing the efficiency of setting up the screening mixtures. Addition of the PCR-template
(individual cultures) has been improved by the use of a 96-pin tool with which an aliquot of all 96 cultures grown as described above can be transferred into the PCR-screening mix in a matter of 1-2 minutes.
For PCR amplification, the final concentrations are IX for
PCR mix, 5 μM of each of a vector primer and one or both of the gene specific primers used for the original extension reaction and
0.75 units of Taq polymerase are added to each well.
Amplification generally was performed using the following conditions:
Step 1 9 °C for 60sec Step 2 94°C for 20sec
Step 3 55°C for 30sec
Step 4 72°C for 90sec
Step 5 repeat steps 2-4 for an additional 29 times
Step 6 72°C for 180sec Step 7 4°C for ever
Aliquots of these PCR reactions are run on agarose gels together with molecular weight markers. The size of the resulting
PCR products will allow direct determination of how much additional sequence the selected clones contain compared to the original partial cDNA. The efficiency of the method has been further improved by using the resulting PCR-products directly for sequencing thus avoiding the necessity of preparing plasmids. The appropriate clones are selected and grown for plasmid preparation and sequencing. Plasmid preparations are made with standard kits familiar to those skilled in the art. Examples include the PROMEGA Magic
MINIPREP and the AGTC alkaline lysis kit.
Sequencing is performed employing standard automated ABI sequencing equipment and protocols using either dye-primer or dye-terminator kits.
Sequence processing and assemblage of the sequencing data are performed using standard ABI software, including INHERIT™ analysis and the Power assembler. INDUSTRIAL APPLICABILITY
Example 1
For the initial method evaluation, a known gene was selected. A partial sequence of the human 90-kDa heat-shock protein gene (HUMHSP90, accession M16660) had been identified in a THP-1 library. This partial sequence (Incyte clone T-014201) initiated at base 1127 of the sequence with accession number M16660. 1.1 Primer design
Two primers were designed to perform the method described in the invention.
Primer 1 (XLR) 5' AGC TGT CCA TGA TGA ACA CAC G 3'
(1180-1159) Primer 2 (XLS) 5' AAT AGG CAC CAC ACC AAC TGA G 3'
(2011-2032) 1.2 Template preparation
A THP-1 cDNA library constructed into the LambdaZAP vector (Stratagene) was converted into a plasmid library following the mass excision protocol. Plasmids of the excised libraries were prepared using the Quiagen Midi plasmid purification kit. 1.3 XL-PCR reaction set-up
The extension reactions were prepared following the instructions provided with the GeneAmp XL PCR Kit (Part No. N808-0182) from Perkin Elmer. A two layer system was set up as follows: The lower reagent mix was prepared by pipetting the following components into a 0.2ml MicroAmp reaction tube.
Lower reagent mix preparation: Water 13.6 μl 3.3X buffer 12.0 μl dATP (lOmM) 2.0 μl dCTP (lOmM) 2.0 μl dGTP (lOmM) 2.0 μl dTTP (lOmM) 2.0 μl
Primer XLS (50μM) 1.0 μl
Primer XLR (50μM) 1.0 μl Mg(OAc)2 (25mM) .4 μl
Total lower reagent mix 40.0 μl
One AmpliWax™ gem was added to the tube. The wax was melted by incubating the reaction tubes at 75°C for 5 minutes. Then the tubes were cooled down to 4°C.
Upper reagent mix preparation: 3.3X buffer 18.0 ml rTth DNA Polymerase 2.0 ml
Total upper enzyme mix 20.0 μl
20 μl of the enzyme/buffer mix are added to each tube and kept separated from the lower mix by the wax layer. Addition of template:
The template DNA (excised library) was diluted to an appropriate concentration in water and then added to the upper mix. Mixing of the components is not necessary.
Template (6.25ng/ml) 40.0 μl
Final volume 100.0 μl
1.4 XL-PCR amplification
For amplification the following protocol was employed: Step 1 94° for 60 sec (initial denaturation)
Step 2 94° for 15 sec
Step 3 65° for 1 min
Step 4 68° for 7 min Step 5 Repeat step 2-4 for 15 additional times
Step 6 94° for 15 sec
Step 7 65° for 1 min
Step 8 68° for 7 min + 15 sec/cycle
Step 9 Repeat step 6-8 for 11 additional times Step 10 72° for 8 min
Step 11 4° for 0.00 sec (to hold at 4°)
1.5 Purification of amplified products
30 μl of the amplified products were run on a 0.7% agarose gel for 16 hours. Visible DNA bands were then cut out and purified using the QIAquick gel purification kit.
1.6 Cloning of amplified products
Klenow enzyme (3 units/reaction) and dNTP's (0.2mM final concentration) were added and the reactions were incubated at room temperature for 30 min followed by incubation at 75° C for 15 min. The products were then ethanol precipitated and redissolved in 13 μl of ligation buffer containing ImM ATP. T4-DNA ligase (15 units) and T4 Polynucleotide kinase (5 units) were added, and the reaction was incubated at room temperature for 3 hours. 3μl of the ligation mixture were transformed into 40 ml of competent E.coli cells. After heatshocking the cells at 42° C for 45 seconds, 80 μl of SOC medium were added, and the cells were allowed to recover at 37° C for 1 hour. The whole transformation mixture then was plated on LB-agar/2XCarb-containing petri dish plates.
1.7 Screening of cloned products
The next day 10 colonies were randomly picked and grown overnight in Falcon 2059 tubes (Becton Dickinson, Oxnard, CA) containing 3 ml of LB-broth with 2X Carb.
5 μl of the cultures were diluted 1:10 with water and 5 ml of this dilution were transferred into MicroAmp™ PCR tubes (Perkin Elmer, Applied Biosystems, Foster City, CA) .
15 μl of a 1.33X concentrated PCR mix were added to each well.
The 1.33 x concentrated PCR mix contained the following components: 10X PCR-buffer 2.0 μl
2mM dNTPs 2.0 μl
M13 rev primer (O.OlmM) 1.0 μl
Primer 2 (XLR, O.OlmM) 1.0 μl
Taq Polymerase 0.15 μl Water 8.85 μl
Final Volume 15.0 μl
The PCR cycling conditions were choosen as follows: Step 1 94° C for 60sec Step 2 94° C for 20sec Step 3 55° C for 30sec Step 4 72° C for 90sec
Step 5 repeat steps 2-4 for an additional 29 times Step 6 72° C for 180 sec Step 7 4° C for ever
Aliquots of the amplified products were run on a 0.8% agarose gel in parallel with the 1 kb DNA ladder (Life Technologies, Gaithersburg, MD 20897) . Appropriate plasmids containing different size inserts were selected for sequencing analysis. 1.8 Sequencing analyis of cloned products
The DNA of the selected clones was prepared using the WizardTM Minipreps DNA Purification System (Promega Corporation, Madison, WI) following the instructions of the manufacturer. Sequencing reactions were performed using the PRISMTM Ready Reaction DyeDeoxy Terminator Cycle Sequencing Kit (Part No 401628, Perkin Elmer, Applied Biosystems, Foster City, CA) . 1.9 Analysis of sequenced products
Three clones were selected for sequencing (14201.3, 14201.5, 14201.13) . The sequences obtained (SEQ ID NOS:3-5, respectively) were aligned using the DNASIS Multiple sequence alignment program. Clone 14201.3 initiated at base 24 of the published sequence
(HUMHSP90), clone 14201.5 initiated at base 13 of the published sequence and clone 14201.13 initiated at base 538 of the published sequence, the original clone (14201) initiated at base 1127 of the published sequence. Figure 7A-7H shows an alignment of the obtained sequences with the published human Hsp 90 nucleotide sequence. Clones 14201.3 and 14201.5 contain part of the 5' untranslated region and therefore the full coding region of the gene has been obtained. Example 2 For further method evaluation, a second known gene was selected. A partial sequence from a liver library was found to be related to that of the human cathepsin B gene (accession L16510, HUMCATHB, SEQ ID NO: 6) . This partial sequence (Incyte clone 87058, SEQ ID NO:7) initiated at base 1066 of the sequence with accession number L16510.
2.1 Primer design
Two primers were designed to perform the method described in the invention:
Primer 1 (XLR) 5' AAG CCA TTG TCA CCC CAG TCA G 3' (1103-1082)
Primer 2 (XLS) 5' GGT TCA CTG TGG AAT CGA ATC 3'
(1125-1145)
2.2 Template preparation A liver cDNA library constructed into the LambdaZAP vector (Stratagene) was converted into a plasmid library following the mass excision protocol. Plasmids of the excised libraries were prepared using the Quiagen Midi plasmid purification kit. 2.3 XL-PCR reaction set-up
The extension reactions were prepared following the instructions provided with the GeneAmp XL PCR Kit (Part No. N808-0182) from Perkin Elmer. A two layer system was set up as described below. The lower reagent mix was prepared by pipetting the following components into a 0.2ml MicroAmp reaction tube. Lower reagent mix preparation:
Water 13.6 μl
3.3 x buffer 12.0 μl dATP (lOmM) 2.0 μl dCTP (lOmM) 2.0 μl dGTP (lOmM) 2.0 μl dTTP (lOmM) 2.0 μl
Primer XLS (50U ) 1.0 μl
Primer XLR (50μM) 1.0 μl
Mg(OAc)2 (25μM) 4.4 μl
Total lower reagent mix 40.0 μl
One AmpliWaxVo gem was added to the tube. This was melted by incubating the reaction tubes at 75°C for 5 minutes. Then the tubes were cooled down to 4°C. Upper reagent mix preparation:
3.3X buffer 18.0 μl rTth DNA Polymerase 2.0 μl Total upper enzyme mix 20.0 μl
20 μl of the enzyme/buffer mix were added to each tube and kept separated from the lower mix by the wax layer. Addition of template:
The template DNA (excised library) was diluted to an appropriate concentration in water and then added to the upper mix. Mixing of the components is not necessary. Template (6.25ng/μl) 40.0 μl
Final volume 100.0 μl
2.4 XL-PCR amplification
For amplification the following protocol was employed:
Step 1 94° for 60 sec (initial denaturation) Step 2 94° for 15 sec
Step 3 65° for 1 min
Step 4 68° for 7 min
Step 5 Repeat step 2-4 for 15 additional times
Step 6 94° for 15 sec Step 7 65° for 1 min
Step 8 68° for 7 min + 15 sec/cycle
Step 9 Repeat step 6-8 for 11 additional times
Step 10 72° for 8 min
Step 11 4° for 0.00 sec (to hold at 4° ) 2.5 Purification of amplified products
30 μl of the amplified products were run on a 0.7% agarose gel for 16 hours. Visible DNA bands were then cut out and purified using the QIAQuick gel purification kit. 2.6 Cloning of amplified products Klenow enzyme (3 units/reaction) and dNTP's (0.2mM final concentration) were added, and the reactions were incubated at room temperature for 30 min followed by incubation at 75°C for 15 min .
The products were then ethanol precipitated and redissolved in 13 μl of ligation buffer containing ImM ATP. T4-DNA ligase (15 units) and T4 Polynucleotide kinase (5 units) were added, and the reaction was incubated at room temperature for 3 hours.
3 μl of the ligation mixture were transformed into 40 μl of competent E.coli cells. After heatshocking the cells at 42°C for 45 seconds, 80 μl of SOC medium were added; and the cells were allowed to recover at 37o C for 1 hour. The whole transformation 0 mixture then was plated on LB-agar 2x Carb-containing petri dishes. 2.7 Screening of cloned products
The next day 10 colonies were randomly picked and grown overnight in Falcon 2059 tubes (Becton Dickinson, Oxnard, CA 5 93030) containing 3 ml of LB-broth with 2X Carb.
5 μl of the cultures were diluted 1:10 with water and 5 μl of this dilution were transferred into MicroAmpTM PCR tubes (Perkin Elmer, Applied Biosystems, Foster City, CA) .
15 μl of a 1.33 x concentrated PCR mix were added to each o tube.
The 1.33 x concentrated PCR mix contained the following components:
10 x PCR-buffer 2.0 μl
2mM dNTPs 2.0 μl 5 M13 rev primer (O.OlmM) 1.0 μl
Primer 2 (XLR, O.OlmM) 1.0 μl
Taq Polymerase 0.15 μl water 8.85 μl
0 Final Volume 15.0 μl
The PCR cycling conditions were as follows: Step 1 94°C for 60sec Step 2 94°C for 20sec Step 3 55°C for 30sec Step 4 72°C for 90sec Step 5 repeat steps 2-4 for an additional 29 times Step 6 72°C for 180sec Step 7 4°C for ever
Aliquots of the amplified products were run on a 0.8% agarose gel in parallel with the lkb DNA ladder (Life Technologies, Gaithersburg, MD 20897) . Appropriate clones containing different size inserts were selected for sequencing analysis.
2.8 Sequencing analyis of cloned products
The DNA of the selected clones was prepared using the WizardTM Minipreps DNA Purification System (Promega Corporation, Madison, WI) following the instructions of the manufacturer. Sequencing reactions were performed using the PRISMTM Ready Reaction DyeDeoxy Terminator Cycle Sequencing Kit (Part No 401628, Perkin Elmer, Applied Biosystems, Foster City, CA) .
2.9 Analysis of sequenced products Three clones were selected for sequencing (87058.6, 87058.8, 87058.16) . The sequences obtained (SEQ ID NOS:8-10, respectively) were aligned using the DNASIS Multiple sequence alignment program and are shown in Figures 8A through 8F. Clone 87058.6 initiated at base 644 of the published sequence (HUMCATHB, SEQ ID NO:6), clone 87058.8 initiated at base 353 of the published sequence and clone 87058.16 initiated at base 58 of the published sequence, the original clone (87058, SEQ ID NO:7) initiated at base 1058 of the published sequence.
Figures 8A through 8F show an alignment of the obtained sequences with the published human Hsp 90 nucleotide sequence. Clone 87058.16 contains part of the 5'UT and therefore the full coding region of the gene. Example 3 In Example 3, a full length cDNA (Seq ID NO 11) of a novel P2U purinergic receptor homolog was obtained by the inventive method and is the subject of U.S. Patent Application 08/459,046 filed June 2, 1995, which is hereby incorporated by reference. Inherit™ and BLAST search and alignment tools were used to relate a partial sequence found in Incyte Clone 179696 from the placental cDNA library to the GenBank sequence of RNU09402, a G-protein coupled surface receptor from rat (Rice WR et al (1995) Am J Respir Cell Molec Biol 12:27-32) . The cDNA of Incyte 179696 was extended to full length using a modified XL-PCR (Perkin Elmer) procedure. Primers were designed based on known sequence; one primer was synthesized to initiate extension in the antisense direction (XLR) and the other to extend sequence in the sense direction (XLF) . The primers allowed the sequence to be extended "outward" from the known sequence, thus generating amplicons containing new, unknown nucleotide sequence comprising the gene of interest. The primers were designed using Oligo 4.0 (National Biosciences Ine, Plymouth MN) to be 22-30 nucleotides in length, to have a GC content of 50% or more, and to anneal to the target sequence at temperatures about 68°-72° C. Any stretch of nucleotides which would result in hairpin structures and primer-primer dimerizations was avoided.
The cDNA library was used as a template, and XLR (bases 278-298) and XLF (bases 587-610) primers were used to extend and amplify the 179696 sequence. By following the instructions for the XL-PCR kit and thoroughly mixing the enzyme, high fidelity amplification is obtained. Beginning with 25 pMol of each primer and the recommended concentrations of all other components of the kit, PCR was performed using the MJ PTC200 thermocycler (MJ Research, Watertown MA) and the following parameters: Step 1 94° C for 60 sec (initial denaturation) Step 2 94° C for 15 sec
Step 3 65° C for 1 min Step 4 68° C for 7 min
Step 5 Repeat step 2-4 for 15 additional cycles
Step 6 94° C for 15 sec
Step 7 65° C for 1 min Step 8 68° C for 7 min + 15 sec/cycle
Step 9 Repeat step 6-8 for 11 additional cycles
Step 10 72° C for 8 min
Step 11 4° C (and holding)
At the end of 28 cycles, 50 μl of the reaction mix was removed; and the remaining reaction mix was run for an additional
10 cycles as outlined below:
Step 1 94° C for 15 sec
Step 2 65° C for 1 min
Step 3 68° C for (10 min + 15 sec) /cycle Step 4 Repeat step 1-3 for 9 additional cycles
Step 5 72° C for 10 min
A 5-10 μl aliquot of the reaction mixture was analyzed by electrophoresis on a low concentration (about 0.6-0.8%) agarose mini-gel to determine which reactions were successful in extending the sequence. Although all extensions potentally contain a full length gene, some of the largest products or bands were selected and cut out of the gel. Further purification involved using a commercial gel extraction method such as QIAQuick™ (QIAGEN Ine,
Chatsworth CA) . After recovery of the DNA, Klenow enzyme was used to trim single-stranded, nucleotide overhangs creating blunt ends which facilitated religation and cloning.
After ethanol precipitation, the products were redissolved in
13 μl of ligation buffer. Then, lμl T4-DNA ligase (15 units) and lμl T4 polynucleotide kinase were added, and the mixture was incubated at room temperature for 2-3 hours or overnight at 16° C.
Competent E. coli cells (in 40 μl of appropriate media) were transformed with 3 μl of ligation mixture and cultured in 80 μl of
SOC medium (Sambrook J et al, supra) . After incubation for one hour at 37° C, the whole transformation mixture was plated on Luria Broth (LB) -agar (Sambrook J et al, supra) containing carbenicillin at 25 mg/L. The following day, 12 colonies were randomly picked from each plate and cultured in 150 μl of liquid LB/carbenicillin medium placed in an individual well of an appropriate, commercially-available, sterile 96-well microtiter plate. The following day, 5 μl of each overnight culture was transferred into a non-sterile 96-well plate and after dilution 1:10 with water, 5 μl of each sample was transferred into a PCR array.
For PCR amplification, 15 μl of concentrated PCR reaction mix (1.33X) containing 0.75 units of Taq polymerase, a vector primer and one or both of the gene specific primers used for the extension reaction were added to each well. Amplification was performed using the following conditions: Step 1 94° C for 60 sec Step 2 94° C for 20 sec Step 3 55° C for 30 sec Step 4 72° C for 90 sec Step 5 Repeat steps 2-4 for an additional 29 cycles Step 6 72° C for 180 sec Step 7 4° C (and holding)
Aliquots of the PCR reactions were run on agarose gels together with molecular weight markers. The sizes of the PCR products were compared to the original partial cDNAs, and appropriate clones were selected, ligated into plasmid and sequenced. Example 4
In this example, the inventive method was used to obtain a novel full length cDNA from the partial sequence found in Incyte clone 08118 which was found to be somewhat homologous to the GenBank sequence of C5a anaphylatoxin receptor, a G-protein coupled surface receptor from dog (Perret J et al (1995) Biochem J 288:911-17) . Based on the partial cDNA sequence, primers (XLR = GAAAGACAGCCACCACCACCACG and XLF = AGAAAGCAAGGCAGTCCATTCAGG ) were designed. Essentially the same method outlined in Example 3 above was used to extend the partial sequence of 8118 to obtain the full length sequence (Seq ID NO:12) of a novel C5a-like receptor homolog which is the subject of a U.S. Patent Application 08/462,355 filed June 5, 1995, and whose disclosure is incorporated by reference.
While the present invention has been described with reference to specific enzymes and sequences, particularly PCR enzyme, and formulations containing such, those skilled in the art understand that various changes may be made and equivalents may be substituted without departing from the true spirit and scope of the invention. In addition, many modifications may be made to adapt a particular situation, material, enzyme, process, process step or steps and still carry out the objective, spirit and scope of the invention. All such modifications are intended to be within the scope of the claims appended hereto.
SEQUENCE LISTING
(1) GENERAL INFORMATION:
(i) APPLICANT: INCYTE PHARMACEUTICALS, INC.
(ii) TITLE OF INVENTION: IMPROVED METHOD FOR OBTAINING
FULL LENGTH cDNA SEQUENCES
(iii) NUMBER OF SEQUENCES: 12
(iv) CORRESPONDENCE ADDRESS:
(A) ADDRESSEE: INCYTE PHARMACEUTICALS, INC.
(B) STREET: 3330 Hillview Avenue
(C) CITY: Palo Alto
(D) STATE: CA
(E) COUNTRY: USA
(F) ZIP: 94304
(v) COMPUTER READABLE FORM:
(A) MEDIUM TYPE: Floppy disk
(B) COMPUTER: IBM PC compatible
(C) OPERATING SYSTEM: PC-DOS/MS-DOS
(D) SOFTWARE: PatentIn Release #1.0, Version #1.30
(vi) CURRENT APPLICATION DATA:
(A) APPLICATION NUMBER: To Be Assigned
(B) FILING DATE: Filed Herewith
(vii) PRIOR APPLICATION DATA:
(A) APPLICATION SERIAL NO: US 08/487,112
(B) FILING DATE: 7-JUN-1995
(vii) PRIOR APPLICATION DATA:
(A) APPLICATION SERIAL NO: US 08/462,355
(B) FILING DATE: 5-JUN-1995
(vii) PRIOR APPLICATION DATA:
(A) APPLICATION SERIAL NO: US 08/459,046
(B) FILING DATE: 2-JUN-1995
(vii) PRIOR APPLICATION DATA:
(A) APPLICATION SERIAL NO: US 08/566,334
(B) FILING DATE: l-DEC-1995
(vii) PRIOR APPLICATION DATA:
(A) APPLICATION SERIAL NO: US 60/006,809
(B) FILING DATE: 15-NOV-1995
(viii) ATTORNEY/AGENT INFORMATION:
(A) NAME: Luther, Barbara J.
(B) REGISTRATION NUMBER: 33954
(C) REFERENCE/DOCKET NUMBER: HP-001-1 PCT
(ix) TELECOMMUNICATION INFORMATION: (A) TELEPHONE: 415-855-0555 (B) TELEFAX: 415-852-0195 (2) INFORMATION FOR SEQ ID NO:l:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 2543 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: GenBank HUMHSP90
(B) CLONE: Accession No. M16660
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:l:
CTCCGGCGCA GTGTTGGGAC TGTCTGGGTA TCGGAAAGCA AGCCTACGTT GCTCACTATT 60
ACGTATAATC CTTTTCTTTT CAAGATGCCT GAGGAAGTGC ACCATGGAGA GGAGGAGGTG 120
GAGACTTTTG CCTTTCAGGC AGAAATTGCC CAACTCATGT CCCTCATCAT CAATACCTTC 180
TATTCCAACA AGGAGATTTT CCTTCGGGAG TTGATCTCTA ATGCTTCTGA TGCCTTGGAC 240
AAGATTCGCT ATGAGAGCCT GACAGACCCT TCGAAGTTGG ACAGTGGTAA AGAGCTGAAA 300
ATTGACATCA TCCCCAACCC TCAGGAACGT ACCCTGACTT TGGTAGACAC AGGCATTGGC 360
ATGACCAAAG CTGATCTCAT AAATAATTTG GGAACCATTG CCAAGTCTGG TACTAAAGCA 420
TTCATGGAGG CTCTTCAGGC TGGTGCAGAC ATCTCCATGA TTGGGCAGTT TGGTGTTGGC 480
TTTTATTCTG CCTACTTGGT GGCAGAGAAA GTGGTTGTGA TCAGAAAGCA CAACGATGAT 540
GAACAGTATG CTTGGGAGTC TTCTGCTGGA GGTTCCTTCA CTGTGCGTGC TGACCATGGT 600
GAGCCCATTG GCATGGGTAC CAAAGTGATC CTCCATCTTA AAGAAGATCA GACAGAGTAC 660
CTAGAAGAGA GGCGGGTCAA AGAAGTAGTG AAGAAGCATT CTCAGTTCAT AGGCTATCCC 720
ATCACCCTTT ATTTGGAGAA GGAACGAGAG AAGGAAATTA GTGATGATGA GGCAGAGGAA 780
GAGAAAGGTG AGAAAGAAGA GGAAGATAAA GATGATGAAG AAAAGCCCAA GATCGAAGAT 840
GTGGGTTCAG ATGAGGAGGA TGACAGCGGT AAGGATAAGA AGAAGAAAAC TAAGAAGATC 900
AAAGAGAAAT ACATTGATCA GGAAGAACTA AACAAGACCA AGCCTATTTG GACCAGAAAC 960
CCTGATGACA TCACCCAAGA GGAGTATGGA GAATTCTACA AGAGCCTCAC TAATGACTGG 1020
GAAGACCACT TGGCAGTCAA GCACTTTTCT GTAGAAGGTC AGTTGGAATT CAGGGCATTG 1080
CTATTTATTC CTCGTCGGGC TCCCTTTGAC CTTTTTGAGA ACAAGAAGAA AAAGAACAAC 1140
ATCAAACTCT ATGTCCGCCG TGTGTTCATC ATGGACAGCT GTGATGAGTT GATACCAGAG 1200 TATCTCAATT TTATCCGTGG TGTGGTTGAC TCTGAGGATC TGCCCCTGAA CATCTCCCGA 1260
GAAATGCTCC AGCAGAGCAA AATCTTGAAA GTCATTCGCA AAAACATTGT TAAGAAGTGC 1320
CTTGAGCTCT TCTCTGAGCT GGCAGAAGAC AAGGAGAATT ACAAGAAATT CTATGAGGCA 1380
TTCTCTAAAA ATCTCAAGCT TGGAATCCAC GAAGACTCCA CTAACCGCCG CCGCCTGTCT 1440
GAGCTGCTGC GCTATCATAC CTCCCAGTCT GGAGATGAGA TGACATCTCT GTCAGAGTAT 1500
GTTTCTCGCA TGAAGGAGAC ACAGAAGTCC ATCTATTACA TCACTGGTGA GAGCAAAGAG 1560
CAGGTGGCCA ACTCAGCTTT TGTGGAGCGA GTGCGGAAAC GGGGCTTCGA GGTGGTATAT 1620
ATGACCGAGC CCATTGACGA GTACTGTGTG CAGCAGCTCA AGGAATTTGA TGGGAAGAGC 1680
CTGGTCTCAG TTACCAAGGA GGGTCTGGAG CTGCCTGAGG ATGAGGAGGA GAAGAAGAAG 1740
ATGGAAGAGA GCAAGGCAAA GTTTGAGAAC CTCTGCAAGC TCATGAAAGA AATCTTAGAT 1800
AAGAAGGTTG AGAAGGTGAC AATCTCCAAT AGACTTGTGT CTTCACCTTG CTGCATTGTG 1860
ACCAGCACCT ACGGCTGGAC AGCCAATATG GAGCGGATCA TGAAAGCCCA GGCACTTCGG 1920
GACAACTCCA CCATGGGCTA TATGATGGCC AAAAAGCACC TGGAGATCAA CCCTGACCAC 1980
CCCATTGTGG AGACGCTGCG GCAGAAGGCT GAGGCCGACA AGAATGATAA GGCAGTTAAG 2040
GACCTGGTGG TGCTGCTGTT TGAAACCGCC CTGCTATCTT CTGGCTTTTC CCTTGAGGAT 2100
CCCCAGACCC ACTCCAACCG CATCTATCGC ATGATCAAGC TAGGTCTAGG TATTGATGAA 2160
GATGAAGTGG CAGCAGAGGA ACCCAATGCT GCAGTTCCTG ATGAGATCCC CCCTCTCGAG 2220
GGCGATGAGG ATGCGTCTCG CATGGAAGAA GTCGATTAGG TTAGGAGTTC ATAGTTGGAA 2280
AACTTGTGCC CTTGTATAGT GTCCCCATGG GCTCCCACTG CAGCCTCGAG TGCCCCTGTC 2340
CCACCTGGCT CCCCCTGCTG GTGTCTAGTG TTTTTTTCCC TCTCCTGTCC TTGTGTTGAA 2400
GGCAGTAAAC TAAGGGTGTC AAGCCCCATT CCCTCTCTAC TCTTGACAGC AGGATTGGAT 2460
GTTGTGTATT GTGGTTTATT TTATTTTCTT CATTTTGTTC TGAAATTAAA GTATGCAAAA 2520
TAAAGAATAT GCCGTTTTTA TAC 2543
(2) INFORMATION FOR SEQ ID NO:2:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 261 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA (vii) IMMEDIATE SOURCE:
(A) LIBRARY: THP-1
(B) CLONE: 14201
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:
AAGAAAAAGA ACAACATCAA ACTCTATGTC CGCCGTGTGT TCATCATGGC AGCTGTGATG 60
AGTTGATACC AGAGTATCTC AATTTTATCC GTGGTGTGGT TGACTTGAGG TCTGCCCCTG 120
AACATCTCCC GGAAATGCTC CAGCAGAGCA AAATCTTGAA AGGCATTCGC AAAAACATTG 180
TTAAGAGTGC CTTAGCTCTT CTCTAGCTGG CAGAAGCAAG GGGATTTCAA GAAATTCTTT 240
TGGGGGGATT TCTTAAAAAT T 261 (2) INFORMATION FOR SEQ ID NO:3:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 478 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: THP-1
(B) CLONE: 14201.3
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:3: GCTGGGTATC GGAAAGCAAG CCTACGTTGC TCACTATTAC GTATAATCCT TTTCTTCAAG 60
ATGCCTGAGG AAGTGCACCA TGGAGAGGAG GAGGTGGAGA CTTTTGCCTT TCAGGCAGAA 120
ATTGCCCAAC TCATGTCCCT CATCATCAAT ACCTCCTATT CCAACAAGGA GATTTCCTCG 180
GGAGTTGATC TCTAATGCTT CTGATGCCTC GGACAAGATT CGCTATGAAG CCTGACAGAC 240
CCTTCGAAGT GGTCAGCGGC AAGAGCTGAA AATTGACATC ATCCCCAACC CTCAGGAACG 300
TCCCTGTACT TTGGGTAGAC ACAGGCATTG GCATAAACAA AGCTGACCTC ATATTATTCG 360
GGGAACCATT GCCAAGTCTT GTCTAAAAGC ATTCATGGAG GCTCTCAGGT TGGCGCAGAC 420
ATCTCCAGAT TGGCAGGTGG GTGTTGGCTT TATTCTGCCC ACTTGGTGGC AGAGAAAT 478 (2) INFORMATION FOR SEQ ID NO:4:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 508 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: CDNA (vii) IMMEDIATE SOURCE:
(A) LIBRARY: THP-1
(B) CLONE: 14201.5
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:4:
GTTGGGACTG TCTGGGTATC GGAAAGCAAG CCTACGTTGC TCACTATTAC GTATAATCCT 60
TTTCTTTTCA AGATGCCTGA GGAAGTGCAC CATGGAGAGG AGGAGGTGGA GACTTTTGCC 120
TTTCAGGCAG AAATTGCCCA ACTCATGTCC CTCATCATCA ATACCTCCTA TTCCAACAAG 180
GAGATTTTCC TTCGGGAGTT GATCTCTAAT GCTTCTGATG CCTTGGACAA GATTCGCTAT 240
GAGAGCCTGA CAGACCCTTC GAAGTTGGAC AGTGGTAAAG AGCTGAAAAT TGACATCATC 300
CCCAACCCTC AGGAACGTAC CCTGACTTTG GGTAGACACA GGCATCGGCA TGACCAAAAG 360
CTGATCTCAT AATAATTGGG AACCATTGCA AGTCTGGTAC TAAAGCATTC ATGGAGGCTC 4 0
TTCAGGCTGG TGCAGACATC TCCATGATTG GGCAGCTTGG GTGTTGCTTT ATTCTGCCTC 480
CTTGGTGGCA GAGAAAGTGT TGTGATCA 508 (2) INFORMATION FOR SEQ ID NO:5:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 547 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: THP-1
(B) CLONE: 14201.13
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:5:
TTGAGAGTAT GTCGAGTTAC TGTGGAGGTT CCTTCACTGC GTGCTGACAT GGTGAGCCCA 60
TGGGAGCGGT ACCAAGTGAT CCTCCATCTC AAAGAAGATC AGACAGAGTA CCTAGAGAGA 120
GGCGGATCAA AGAGTAGTGA TGAGCATCCT CAGATCATAG GCTATCCCAT CACCCTTTTT 180
TGGAGAAGGA CGAGAGAAGG AATTAGGATG ATGAGGCAGA GGAAGAGAAT GGTGAGAATG 240
AAGAGGAGTA ACGATGATGA AGAAACCCCA AGATCGATGA TGTGGTTCAG ATGAGGGGAT 300
GACAGCGGTA GATAAGAAGA AGAAACTAGA ATCATCGGAT CATGACAGGA AGAACTAACA 360
GATCATCTTT CGGCCAGAAT CCCTGATGTC ATCACCCAAG AGGGTATGGA GATTTCTACA 420
TGCAGCTCAC TTTACTGGGC AAGACACTTG GCAGCAACAC TTTTCTGTAG AAGGCCATTG 480 CATCACGCAT TGCTATTCTT CCCTCGCCGT CTCCTTTGAC CTGGTCTGGC ATCATGGTGT 540 CTTGATC 547
(2) INFORMATION FOR SEQ ID NO:6:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 1996 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: GenBank HUMCATHB
(B) CLONE: Accession No. L16510
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:6:
TCCGGCAACG CCAACCGCTC CGCTGCGCGC AGGCTGGGCT GCAGGCTCTC GGCTGCAGCG 60
CTGGGCTGGT GTGCAGTGGT GCGACCACGG CTCACGGCAG CCTCAGCCAC CCAGATGTAA 120
GCGATCTGGT TCCCACCTCA GCCTCCCGAG TAGTGGATCT AGGATCCGGC TTCCAACATG 180
TGGCAGCTCT GGGCCTCCCT CTGCTGCCTG CTGGTGTTGG CCAATGCCCG GAGCAGGCCC 240
TCTTTCCATC CCCTGTCGGA TGAGCTGGTC AACTATGTCA ACAAACGGAA TACCACGTGG 300
CAGGCCGGGC ACAACTTCTA CAACGTGGAC ATGAGCTACT TGAAGAGGCT ATGTGGTACC 360
TTCCTGGGTG GGCCCAAGCC ACCCCAGAGA GTTATGTTTA CCGAGGACCT GAAGCTGCCT 420
GCAAGCTTCG ATGCACGGGA ACAATGGCCA CAGTGTCCCA CCATCAAAGA GATCAGAGAC 480
CAGGGCTCCT GTGGCTCCTG CTGGGCCTTC GGGGCTGTGG AAGCCATCTC TGACCGGATC 540
TGCATCCACA CCAATGCGCA CGTCAGCGTG GAGGTGTCGG CGGAGGACCT GCTCACATGC 600
TGTGGCAGCA TGTGTGGGGA CGGCTGTAAT GGTGGCTATC CTGCTGAAGC TTGGAACTTC 660
TGGACAAGAA AAGGCCTGGT TTCTGGTGGC CTCTATGAAT CCCATGTAGG GTGCAGACCG 720
TACTCCATCC CTCCCTGTGA GCACCACGTC AACGGCTCCC GGCCCCCATG CACGGGGGAG 780
GGAGATACCC CCAAGTGTAG CAAGATCTGT GAGCCTGGCT ACAGCCCGAC CTACAAACAG 840
GACAAGCACT ACGGATACAA TTCCTACAGC GTCTCCAATA GCGAGAAGGA CATCATGGCC 900
GAGATCTACA AAAACGGCCC CGTGGAGGGA GCTTTCTCTG TGTATTCGGA CTTCCTGCTC 960
TACAAGTCAG GAGTGTACCA ACACGTCACC GGAGAGATGA TGGGTGGCCA TGCCATCCGC 1020
ATCCTGGGCT GGGGAGTGGA GAATGGCACA CCCTACTGGC TGGTTGCCAA CTCCTGGAAC 1080
ACTGACTGGG GTGACAATGG CTTCTTTAAA ATACTCAGAG GACAGGATCA CTGTGGAATC 1140 GAATCAGAAG TGGTGGCTGG AATTCCACGC ACCGATCAGT ACTGGGAAAA GATCTAATCT 1200
GCCGTGGGCC TGTCGTGCCA GTCCTGGGGG CGAGATCGGG GTAGAAATGC ATTTTATTCT 1260
TTAAGTTCAC GTAAGATACA AGTTTCAGGC AGGGTCTGAA GGACTGGATT GGCCAAACAT 1320
CAGACCTGTC TTCCAAGGAG ACCAAGTCCT GGCTACATCC CAGCCTGTGG TTACAGTGCA 1380
GACAGGCCAT GTGAGCCACC GCTGCCAGCA CAGAGCGTCC TTCCCCCTGT AGACTAGTGC 1440
CGTGGGAGTA CCTGCTGCCC AGCTGCTGTG GCCCCCTCCG TGATCCATCC ATCTCCAGGG 1500
AGCAAGACAG AGACGCAGGA TGGAAAGCGG AGTTCCTAAC AGGATGAAAG TTCCCCCATC 1560
AGTTCCCCCA GTACCTCCAA GCAAGTAGCT TTCCACATTT GTCACAGAAA TCAGAGGAGA 1620
GATGGTGTTG GGAGCCCTTT GGAGAACGCC AGTCTCCAGG TCCCCCTGCA TCTATCGAGT 1680
TTGCAATGTC ACAACCTCTC TGATCTTGTG CTCAGCATGA TTCTTTAATA GAAGTTTTAT 1740
TTTTCGTGCA CTCTGCTAAT CATGTGGGTG AGCCAGTGGA ACAGCGGGAG CCTGTGCTGG 1800
TTTGCAGATT GCCTCCTAAT GACGCGGCTC AAAAGGAAAC CAAGTGGTCA GGAGTTGTTT 1860
CTGACCCACT GATCTCTACT ACCACAAGGA AAATAGTTTA GGAGAAACCA GCTTTTACTG 1920
TTTTTGAAAA ATTACAGCTT CACCCTGTCA AGTTAACAAG GAATGCCTGT GCCAATAAAA 1980
GGTTTCTCCA ACTTGA 1996 (2) INFORMATION FOR SEQ ID NO:7:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 294 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: LIVER
(B) CLONE: 87058
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:7:
CGGCACGAGC CAACTCCTGG AACACTGACT GGGGTGACAA TGGCTTCTTT AAAATACTCA 60
GAGGACAGGT TCACTGTGGA ATCGAATCAG AAGTGGTGGC TGGAATTCCA CGCACCGTTC 120
AGTACTGGGA AAAGTCTAAT CTGCCGTGGG CCTTCGTGCC AGTCCTGGGG GCGAGATGGG 180
GGTAGAAATG CATTTTATTC TTTAAGTTCA CGTAAGATAC AAGTTTCAGA CAGGGGTCTA 240
AGGCCTGGTT GCCAAAATCA GACCTGTTTT TCAAGGGGCC CAAGTCCTGG GTTC 294 (2) INFORMATION FOR SEQ ID NO:8:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 552 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: Liver
(B) CLONE: 87058.6
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:8:
GTGAAGCTTG GAACTTCTGG ACAAGAAAAG GCCTGGTTTC TGGTGGCCTC TATGAATCCC 60
ATGTAGGGTG CAGACCGTAC TCCATCCCTC CCTGTGAGCA CCACGTCAAC GGCTCCCGGC 120
CCCCATGCAC GGGGGAGGGA GATACCCCCA AGTGTAGCAA GATCTGTGAG CCTGGCTACA 180
GCCCGACCTA CAAACAGGAC AAGCACTACG GATACAATTC CTACAGCGTC TCCAATAGCG 240
AGAAGGACAT CATGGCCGAG ATCTACAAAA ACGGCCCCGT GGAGGGAGCT TTCTCTGTGT 300
ATTCGGACTT CCTGCTCTAC AAGTCAGGAG TGTACCAACA CGTCACCGGA GAGATGATGG 360
GTGGCCATGC CATCCGCATC CTGGGCTGGG GAGTGGAGAA TGGCACAACC TACTGGCTGG 420
TTGGCAACTC CTGGAACACT GACTGGGGTG ACAATGGGTT CACTGTGGAA TCGAATCAGA 480
AGTGGTGGTG GAATTCCACG CACGATCAAG TGCTGGGAAA AGATCTTAAT CTGCCGGGGC 540
TGTCGGCCAG TC 552 (2) INFORMATION FOR SEQ ID NO:9:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 559 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: Liver
(B) CLONE: 87058.8
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:9: GAGGTACCTT CCTGGGTGGG CCCAAGCCAC CCCAGAGAGT TATGTTTACC GAGGACCTGA 60 AGCTGCCTGC AAGCTTCGAT GCACGGGAAC AATGGCCACA GTGTCCCACC ATCAAAGAGA 120 TCAGAGACCA GGGTCCTGTG GCTCCTGCTG GGCCTTCGGG GCTGTGGAAG CCATCTCTGA 180 CCGGATCTGA TCCACACCAA TGCGCACGTC AGCGTGGAGG TGTCGGCGGA GGACTGCTCA 240
CATGCTGTGG CAGATGTGTG GGGACGGCTG TAATGGTGGC TATCCTGCTG AAGCTTGGAC 300
TTCTGGACAA GAAAAGGCCC TGGTTTCTGG TGGCCTCTAT GATCCCATGT AGGGTGTAGA 360
CCGTACTCCA TCCCTCCCTG TGAAGCACCA CGTCAACGGT TCCCGGGCCC CATGCACGGG 420
GAGGGAGATA CCCCCAAGTG TAACAAGATC TGTGAGCCTG GGTACAGTCC CGACCACAAA 480
CAGGAAAAGC ACTACGGATA CAATTCCTCA GGTCTCCAAT AGTGAGAAGG GACATCATGC 540
CGAGATCTAC AATAACGGC 559 (2) INFORMATION FOR SEQ ID NO:10:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 622 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: Liver
(B) CLONE: 87058.16
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:10:
CGGTTGAGAT TCGGACAGTC CGAAAACGTC CGGCAAGTCA CCCGCTCCGC TGGCGCAGGC 60
TGGGTGCAGG CTCTCGGTGC AGGCTGGGTG GATCTAGGAT CCGGCTTCCA ACATGTGGCA 120
GTTCTGGGCC TCCCTCTGTG CCTGCTGGTG TTGGACAATG CCCGGAGGAG GCCTCTTTCC 180
ATCCCCTGTC GGATGAGCTG GTCACTATGT CAACAAACGG AATACCACGT GGAGGCCGGG 240
AACAACTTCT ACAACGTGGA CATGAGCTAC TTGAGAGGTA TGTGGTACCT TCCTGGGTGG 300
GCCCAAGCCA CCCCAGAGAG TTTGTTTACC GAGGACCTGA GCTGCCTGCA AGCTTCGAAG 360
GACGGGAACA ATGGCCACAG TGTCCCACCA TCAAAGAGAT CAGAGACAGG GCTCCTGTGG 420
TCCTGCTGGG CCTCCGGGGC TGTGGAAGCA TCTCTGACCG GATCTGCATC CACACCAATG 480
GCACGTCAGC GTGGTGGTGT CGGGGAGGAC CTGATCACCT TTGTGGTAGC ATGTGTGGGG 540
GACGGCTGTA ATGGTGGTTA TCCTGTGAAG CTGGGCCTTC TAGAAAGAAA AGGCTGTTTT 600
GGTGGCCTTA TGACTCCCAT GT 622
(2) INFORMATION FOR SEQ ID NO:11:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 984 base pairs (B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA
(vii) IMMEDIATE SOURCE:
(A) LIBRARY: Placenta
(B) CLONE: 179696
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:11:
ATGGAATGGG ACAATGGCAC AGACCAGGCT CTGGGCTTGC CACCCACCAC CTGTGTCTAC 60
CGCGAGAACT TCAAGCAACT GCTGCTCCCA CCTGTGTATT CGGCGGTGCT GGCGCCTGCC 120
CTCCCGCTGA ACATCTGTGT CATTACCCAG ATCTGCACGT CCCGCCGGGC CCTGACCCGC 180
ACGGCCGTGT ACACCCTAAA CCTTGCTCTG CCTGACCTGC TATATGCCTG CTCCCTGCCC 240
CTGCTCATCT ACAACTATGC CCAAGGTGAT CACTGGCCCT TTGGCGACTT CGCCTGCCGC 300
CTGGTCCGCT TCCTCTTCTA TGCCAACCTG CACGGGAGGA TCCTCTTCCT CACCTGCATC 360
AGCTTCCAGC GCTACCTGGG CATCTGCCAC CCGCTGGCCC CCTGGCACAA ACGTGGGGGC 420
CGCCGGGCTG CCTGGCTAGT GTGTGTAGCC GTGTGGCTGG CCGTGACAAC CCAGTGCCTG 480
CCCACAGCCA TCTTCGCTGC CACAGGCATC CAGCGTAACC GCACTGTCTG TTATGACCTC 540
AGCCCGCCTG CCCTGGCCAC CCACTATATG CCCTATGGGA TGGCTCTCAC TGTCATCGGC 600
TTCCTGCTGC CCTTTGCTGC CCTGCTGGCC TGCTACTGTC TCCTGGCCTG CCGCCTGTGC 660
CGCCAGGATG GCCCGGCAGA GCCTGTGGCC CAGGAGCGGC GTGGCAAGGC GGCCCGCATG 720
GCCGTGGTGG TGGCTGCTGT CTTTGGCATC AGCTTCCTGC CTTTTCACAT CACCAAGACA 780
GCCTACCTGG CAGTGCGCTC GACGCCGGGC GTCCCCTGCA CTGTATTGGA GGCCTTTGCA 840
GCGGCCTACA AAGGCACGCG GCCGTTTGCC AGTGCCAACA GCGTGCTGGA CCCCATCCTC 900
TTCTACTTCA CCCAGAAGAA GTTCCGCCGG CGACCACATG AGCTCCTACA GAAACTCACA 960
GACAAATGGC AGAGGCAGGG TCGC 984 (2) INFORMATION FOR SEQ ID NO:12:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 1446 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: cDNA (vii) IMMEDIATE SOURCE: (A) LIBRARY: Mast Cell
(B) CLONE: 8118
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:12:
ATGGCGTCTT TCTCTGCTGA GACCAATTCA ACTGACCTAC TCTCACAGCC ATGGAATGAG 60
CCCCCAGTAA TTCTCTCCAT GGTCATTCTC AGCCTTACTT TTTTACTGGG ATTGCCAGGC 120
AATGGGCTGG TGCTGTGGGT GGCTGGCCTG AAGATGCAGC GGACAGTGAA CACAATTTGG 180
TTCCTCCACC TCACCTTGGC GGACCTCCTC TGCTGCCTCT CCTTGGCCTT CTCGCTGGCT 240
CACTTGGCTC TCCAGGGACA GTGGCCCTAC GGCAGGTTCC TATGCAAGCT CATCCCCTCC 300
ATCATTGTCC TCAACATGTT TGGCAGTGTC TTCCTGCTTA CTGCCATTAG CCTGGATCGC 360
TGTCTTGTGG TATTCAAGCC AATCTGGTGT CAGAATCATC GCAATGTAGG GATGGCCTGC 420
TCTATCTGTG GATGTATCTG GGTGGTGGCT TTTGTGTTGT GCATTCCTGT GTTCGTGTAC 480
CGGGAAATCT TCACTACAGA CAACCATAAT AGATGTGGCT ACAAATTTGG TCTCTCCAGC 540
TCATTAGATT ATCCAGACTT TTATGGGGAT CCACTAGAAA ACAGGTCTCT TGAAAACATT 600
GTTCAGCCGC CTGGAGAAAT GAATGATAGG TTAGATCCTT CCTCTTTCCA AACAAATGAT 660
CATCCTTGGA CAGTCCCCAC TGTCTTCCAA CCTCAAACAT TTCAAAGACC TTCTGCAGAT 720
TCACTCCCTA GGGGTTCTGC TAGGTTAACA AGTCAAAATC TGTATTCTAA TGTATTTAAA 780
CCTGCTGATG TGGTCTCACC TAAAATCCCC AGTGGGTTTC CTATTGAAGA TCACGAAACC 840
AGCCCACTGG ATAACTCTGA TGCTTTTCTC TCTACTCATT TAAAGCTGTT CCCTAGCGCT 900
TCTAGCAATT CCTTCTACGA GTCTGAGCTA CCACAAGGTT TCCAGGATTA TTACAATTTA 960
GGCCAATTCA CAGATGACGA TCAAGTGCCA ACACCCCTCG TGGCAATAAC GATCACTAGG 1020
CTAGTGGTGG GTTTCCTGCT GCCCTCTGTT ATCATGATAG CCTGTTACAG CTTCATTGTC 1080
TTCCGAATGC AAAGGGGCCG CTTCGCCAAG TCTCAGAGCA AAACCTTTCG AGTGGCCGTG 1140
GTGGTGGTGG CTGTCTTTCT TGTCTGCTGG ACTCCATACC ACATTTGGGG AGTCCTGTCA 1200
TTGCTTACTG ACCCAGAAAC TCCCTTGGGG AAAACTCTGA TGTCCTGGGA TCATGTATGC 1260
ATTGCTCTAG CATCTGCCAA TAGTTGCTTT AATCCCTTCC TTTATGCCCT CTTGGGGAAA 1320
GATTTTAGGA AGAAAGCAAG GCAGTCCATT CAGGGAATTC TGGAGGCAGC CTTCAGTGAG 1380
GAGCTCACAC GTTCCACCCA CTGTCCCTCA AACAATGTCA TTTCAGAAAG AAATAGTACA 1440
ACTGTG 1446

Claims

1. A method of extending the sequence of a partial complementary DNA (cDNA) using polymerase chain reaction (PCR) , comprising the steps of: a) combining a first and second PCR primer with nucleic acid from a cDNA library expected to contain said partial cDNA, or a genomic library, under conditions suitable for synthesis of nucleic acid PCR products from the first and second primers, wherein said first and second primers are capable of annealing to opposite strands of the partial cDNA or genomic DNA and initiating nucleic acid synthesis in an outward manner and wherein the first primer is capable of being extended by DNA polymerase in an antisense direction and the second primer is capable of being extended in a sense direction. b) purifying the PCR products, and c) identifying extended nucleotide sequences derived from said partial cDNA or said genomic DNA.
2. The method of Claim 1 wherein identifying extended sequences comprises nucleic acid sequencing.
3. The method of Claim 2 further comprising extending the nucleotide sequences of step 6c by repeating steps 6a through 6c on the nucleotide sequences identified in step 6c.
4. A method of extending the nucleotide sequence of a partial complementary DNA (cDNA) using polymerase chain reaction (PCR), comprising the steps of: a) combining a first and second PCR primer with nucleic acid from a cDNA library expected to contain said partial cDNA, or a genomic library, under conditions suitable for synthesis of nucleic acid PCR products from the first and second primers, wherein said first and second primers are capable of annealing to opposite strands of the partial cDNA or genomic DNA and initiating nucleic acid synthesis in an outward manner and wherein the first primer is capable of being extended by DNA polymerase in an antisense direction and the second primer is capable of being extended in a sense direction. b) purifying the PCR products, c) ligating the purified PCR products under conditions suitable for the formation of circular closed nucleic acid, d) transforming a host cell with the circular closed nucleic acid and culturing the transformed host cell under conditions suitable for growth, e) recovering said circular closed nucleic acid from the cultured, transformed host cell, f) identifying extended nucleotide sequences derived from said partial cDNA or said genomic DNA.
5. The method of Claim 4 wherein identifying extended sequences comprises nucleic acid sequencing.
6. The method of Claim 4 wherein culturing the transformed host cell under conditions suitable for growth comrpises culturing in the presence of selective antibiotic conditions.
7. The method of Claim 4 wherein said host cell is E.coli .
8. The method of Claim 4 wherein after step 4b and prior to step 4c, the purified PCR products are treated under conditions sutiable for converting nucleic acid overhangs to blunt ends.
PCT/US1996/008501 1995-06-02 1996-06-03 IMPROVED METHOD FOR OBTAINING FULL-LENGTH cDNA SEQUENCES WO1996038591A1 (en)

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AU59729/96A AU5972996A (en) 1995-06-02 1996-06-03 Improved method for obtaining full-length cdna sequences
JP8536785A JPH11506332A (en) 1995-06-02 1996-06-03 Improved method for obtaining full-length cDNA sequences

Applications Claiming Priority (10)

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US08/459,046 US6008039A (en) 1995-06-02 1995-06-02 Polynucleotide encoding a novel purinergic P2U receptor
US08/459,046 1995-06-02
US46235595A 1995-06-05 1995-06-05
US08/462,355 1995-06-05
US48711295A 1995-06-07 1995-06-07
US680995P 1995-11-15 1995-11-15
US56633495A 1995-12-01 1995-12-01
US60/006,809 1995-12-01
US08/566,334 1995-12-01
US08/487,112 1995-12-01

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WO2000052200A1 (en) * 1999-02-26 2000-09-08 Shanghai Biorigin Gene Development Co., Ltd. METHOD FOR LARGE SCALE cDNA CLONING AND SEQUENCING BY CIRCULATING SUBTRACTION
WO2000060076A2 (en) 1999-04-02 2000-10-12 Corixa Corporation Compositions for the treatment and diagnosis of breast cancer and methods for their use
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