CN104830991A - Primer and kit for detecting PDGFRA (platelet-derived growth factor receptor alpha) gene D842V polymorphic sites and PCR (polymerase chain reaction) method of primer and kit - Google Patents

Primer and kit for detecting PDGFRA (platelet-derived growth factor receptor alpha) gene D842V polymorphic sites and PCR (polymerase chain reaction) method of primer and kit Download PDF

Info

Publication number
CN104830991A
CN104830991A CN201510290644.3A CN201510290644A CN104830991A CN 104830991 A CN104830991 A CN 104830991A CN 201510290644 A CN201510290644 A CN 201510290644A CN 104830991 A CN104830991 A CN 104830991A
Authority
CN
China
Prior art keywords
primer
probe
keeping gene
gene gapdh
pcr
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Granted
Application number
CN201510290644.3A
Other languages
Chinese (zh)
Other versions
CN104830991B (en
Inventor
高劲松
张英杰
李星颐
王箫笛
魏潇
魏奇
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
SHENYANG EUGENOM BIOLOGICAL TECHNOLOGY Co Ltd
Original Assignee
SHENYANG EUGENOM BIOLOGICAL TECHNOLOGY Co Ltd
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by SHENYANG EUGENOM BIOLOGICAL TECHNOLOGY Co Ltd filed Critical SHENYANG EUGENOM BIOLOGICAL TECHNOLOGY Co Ltd
Priority to CN201510290644.3A priority Critical patent/CN104830991B/en
Publication of CN104830991A publication Critical patent/CN104830991A/en
Application granted granted Critical
Publication of CN104830991B publication Critical patent/CN104830991B/en
Active legal-status Critical Current
Anticipated expiration legal-status Critical

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6876Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
    • C12Q1/6883Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for diseases caused by alterations of genetic material
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • 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
    • C12Q1/6858Allele-specific amplification
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q2600/00Oligonucleotides characterized by their use
    • C12Q2600/106Pharmacogenomics, i.e. genetic variability in individual responses to drugs and drug metabolism
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q2600/00Oligonucleotides characterized by their use
    • C12Q2600/156Polymorphic or mutational markers

Abstract

The invention discloses a primer and a kit for detecting PDGFRA (platelet-derived growth factor receptor alpha) gene D842V polymorphic sites and a PCR (polymerase chain reaction) method of the primer and the kit. The primer comprises a wild specific sense primer, a mutant type specific sense primer, and a reverse primer shared by the wild specific sense primer and the mutant type specific sense primer. The wild specific sense primer has an SEQ No.17 sequence, the mutant type specific sense primer has an SEQ No.14 sequence, and the shared reverse primer has an SEQ No.16 sequence. The kit has the advantages of simplicity in detection, quickness, accuracy, low cost and the like, and powerful tools are provided for scientific research and clinic analysis of the PDGFRA gene D842V polymorphic sites.

Description

Detect the primer of PDGFRA gene D842V pleomorphism site, test kit and PCR method thereof
Technical field
The present invention relates to molecular biology field of gene detection, specifically provide a kind of primer, test kit and the PCR method thereof that detect PDGFRA gene D842V pleomorphism site, for the rapid detection of PDGFRA gene D842V pleomorphism site.
Background technology
Thr6 PDGF BB (PDGF) is a kind of angiogenic factors, PDGF is the former and important angiogenesis factor of the potent mitogenesis of multiple mesenchymal cell as inoblast, vascular smooth muscle cell, renal glomerulus vascular cell, neurogliocyte, endotheliocyte etc., by thrombocyte, histocyte and some tumour cell produce.Platelet derived growth factor receptor (PDGFR) is a kind of receptor tyrosine protein kinase family member, the chemotactic of cell, division and proliferation can be promoted, positive important is played in the physiological processs such as body growth growth, trauma repair, and closely related with the generation of tumour.PDGFRA is the one of PDGFR, is promoting to play a significant role in the propagation of tumour cell, invasion and attack and vasculogenesis etc.The activation of PDGFR path relates to crucial downstream signaling pathway, comprises RAS-MAPK approach and PI3K approach etc.
PDGFRA gene is by mankind's rice chromosome genes encoding (4q12), PDGFRA full length gene about 65 kb, be made up of 23 exons, 5 immunoglobulin-like regions wherein outside exon 3 ~ 10 coding born of the same parents, exons 11 encode transmembrane district, exons 13 ~ 15 and exons 17 ~ 21 are encoded 2 Tyrosylprotein kinase districts in born of the same parents respectively.The protein of PDGFRA genes encoding is platelet derived growth factor receptor (platelet2derived growth factor recep tor alpha, PDGFRA), PDGFRA is a kind of single transmembrane glycoprotein, be made up of 1089 amino acid, 593 ~ 954 belong to Tyrosylprotein kinase district.
PDGFRA transgenation often betides 12 exons and 18 exons.Imatinib (imatinib mesylate, Gleevec) Tyrosylprotein kinase in PDGFR downstream is acted on, clinical studies show imatinib is used for the treatment of gastrointestinal stromal tumor, brain tumor and melanoma Be very effective, but the D842V sudden change of PDGFRA gene extron 18 can cause gastrointestinal stromal tumor patient to imatinib initial drug-resistant.In gastrointestinal stromal tumor patient, the case of about 7% carries PDGFR transgenation, and wherein 1/3 case has PDGFRA to suddenly change, and sudden change mainly occurs on the exons 18 of encoding active structural domain, and PDFGR α transgenation and C-KIT transgenation are separate.Select the patient of targeted drug Therapeutic cancer should carry out the abrupt climatic change of this gene, whether can to monoclonal antibody class drug resistant to help doctor to understand patient.
At present to the detection of transgenation and gene pleiomorphism, common have direct sequencing; Gene chip hybridization method; PCR-RFLP method; Pcr amplification product capillary electrophoresis analysis method; PCR-SSCP; PCR high-resolution fusion curve analytical technology; PCR-Taqman MGB(Minor Groove Binder) probe method; AS-PCR method; Cast-PCR method etc.It is high more or less also to there is instrument price in these methods, and operation easier is large, and there is certain false negative and false positive, testing cost is high, and clinical popularity is low, can not detect the shortcomings such as clinical samples on a large scale simultaneously.
As: 1) direct sequencing is the gold standard of mutation analysis, can find known and unknown mutation site, but the mutator gene DNA profiling number that the sensitivity of this method detection transgenation is 20%(and goal gene accounts for 20% of wild-type DNA profiling number).Also there is complicated operation, the cycle is long simultaneously, and analysis speed is slow, the normal needs time of 2 days, and this method is open pipe operation, greatly increases the possibility of pollution, be not suitable for the detection to extensive sample, also need expensive instrument simultaneously, exist in shortcomings such as basic unit not easily implement.
2) regular-PCR-RFLP method and technology is easy; low price; the test in laboratory of suitable a small amount of sample; but RFLP only can detect the sudden change of restriction enzyme site; can not detect without restriction enzyme site; waste time and energy, also there is PCR primer pollution and cause false-positive risk, see [Mol Diagn Ther. 2010 Jun 1; 14 (3): 163-9, United States Patent 20120135406].
3) chip technology has the features such as high-throughput, microminiaturization, automatization compared with traditional instrument detection method, is applicable to full genome mutated scanning, and the mutational site being not suitable for individual gene is detected, and precision is low, expensive.
4) PCR high-resolution fusion curve analytical technology; the catastrophe of energy high throughput testing gene; reagent cost is lower; but because its fluorescent signal is from dyestuff; specificity is affected, and detecting instrument is the fluorescent PCR instrument of upgrade version, and price is high; universal limited, see [Clin Chim ACqa. 2012 Nov 12; 413 (21-22): 1781-5; United States Patent 20110045479].
5) PCR-Taqman MGB probe method is applicable to known mutations site, usually need two probes, and the synthesis price of Taqman MGB probe is several times of general T aqman probe, sees [J Clin Microbiol. 2010 Aug; 48 (8): 2909-15; United States Patent 20090311679], and allelotrope or the mutational site of the content less (1 in >=1,000) in sample can not be detected.
6) although PCR-SSCP method is simple, this method is open detection system, easily cause the pollution of PCR primer, and operation steps is many, wastes time and energy.
7) allele-specific primers pcr amplification method (AS-PCR); this method detects transgenation or the most simple and quick method (Wu D Y, Ugozzoli L, the Pal B K of SNP at present; Wallace R B., Proc Natl Acad Sci USA 1989; 86:2757-2760), its principle is the base mispairing of primer 3' terminal bases and template, and the efficiency of its PCR will decline 10 3-10 6.6doubly (Chen, X., and Sullivan, P F, The Pharmacogeonomics Journal 2003,3,77-96).Although the party's ratio juris is simple, still can there is non-specific amplification in the primer of mispairing; amplification situation looks type (the Ayyadevara S relevant with the base sequence around detection site of sudden change; Thaden J J, Shmookler Reis R J., Anal Biochem 2000; 284:11-18), also with the impact of allelotrope variable that exists in sample.In order to increase the specificity of AS-PCR, many scientists have done a lot of effort.A large amount of experiments proves, the method is it is crucial that two special primers of design and 3' terminal mutation site base complementrity or mispairing, and design of primers is bad, by causing the intersection of high background to increase, can cause higher false positive.Although many people make great efforts this drawback to overcome; as the TaqMAMA method of report; 3 ' penultimate or the 3rd introduce mutating alkali yl; really the specificity of reaction can be increased; but still false positive cannot be eliminated completely, and in the judgement of homozygote and heterozygote, lack standard; there will be chaotic situation, see [J Virol Methods. 2008 Nov; 153 (2): 156-62; Genomics. 2004 Feb; 83 (2): 311-20].Simple AS-PCR, carry out electrophoresis again after usually adopting PCR reaction to terminate, from there being reactionless band to carry out judged result, although this method does not need expensive instrument, electrophoretic procedures, adds the opportunities for contamination of PCR, and time and effort consuming.Possessor has done improvement to the method to the greatest extent, adopt fluorescent quantitative PCR technique, but what obtain is not the result of " all or none " formula, always have the generation of nonspecific reaction, namely all can increase in same primer pair wild-type and saltant type site, just its Ct(Cycle threshold obtained) different, therefore the concept of Δ Ct is just introduced, i.e. Δ Ct=wild Ct-sudden change Ct, but calculation of complex, be greater than homozygote Ct value as wanted Δ Ct value and be judged to saltant type homozygote, Δ Ct value is less than heterozygote Ct value, be judged to heterozygote, the introducing of Δ Ct value not only increases operation steps, also confusion can be caused, because the established standards of Δ Ct value cannot accurately be located, the operation of different personnel, different samples and different detecting instruments all can have different numerals, very large difficulty is brought to clinical application, practical application is still limited, see [Chinese patent CN101235415, CN101565742A].
8) U.S. LIFE company adopts a kind of MGB to close the method for probe; be called Cast-PCR(Competitive allele specific Taqman PCR); with MGB probe, the site do not detected is closed; then the method testing goal site of allele specific primer quantitative fluorescent PCR is used; although this improves the specificity of detection, owing to adding to close probe into a MGB, cost certainly will be increased; how much can bring interference to reaction efficiency, see [Exp Mol Pathol. 2012 Jun; 92 (3): 275-80; United States Patent 20100221717; CN102428190A].Someone adopts the PCR primer of the base (Anal Biochem.2005,340:287-294) of lock nucleic acid (LNA) (Plant Method 2007,3:2) or modification, and AS-PCR detection sensitivity can be made to improve.But, these approaches increases the overall cost of analysis, and depth optimization need be carried out to reaction.
A kind of PDGFRA gene mutation detection liquid-phase chip (patent No. CN 101984072 A) of domestic Guangzhou Yishan Biotechnology Co., Ltd. application, the D842V catastrophe of liquid-phase chip technology to PDGFRA gene of employing detects.
Chip technology has the features such as high-throughput, microminiaturization, automatization compared with traditional instrument detection method, is applicable to full genome mutated scanning, and the mutational site being not suitable for individual gene is detected, and precision is low, expensive.And common fluorescent quantitative PCR technique designs the most key site-specific primer, also only carry out according to the rule of design of primers, the screening objective indicator of the good special primer of neither one, the most key is, and their result judges, still fuzzy, do not have the concept of " all or none ", nonspecific like this shortcoming still cannot overcome.The fluorescence quantifying PCR method of two probe, due to needs two probes, and is usually Taqman-MGB probe, considerably increases reagent cost, and the design of probe and optimization, condition is very high.Although high-resolution fusion curve analytical technology reagent cost is low, fluorescence dye is nonspecific display, the success or failure of the experience of reaction condition optimization in advance, different instruments costly and operator often determination result.
Therefore, how to carry out simply detecting accurately to the D842V sudden change of PDGFRA gene, become people's problem demanding prompt solution.
Summary of the invention
Given this, the invention provides a kind of primer, test kit and the PCR method thereof that detect PDGFRA gene D842V pleomorphism site, high with the result interpretation complexity, the detecting instrument price that at least solve test kit existence in the past, operation easier is large, there is certain false negative and false positive, testing cost is high, and clinical popularity is low, can not detect one or more problems such as clinical samples on a large scale simultaneously.
Scheme provided by the invention is specially: a kind of primer detecting PDGFRA gene D842V pleomorphism site, it is characterized in that, described primer comprises: the downstream primer that wild-type specific upstream primer, saltant type specific upstream primer and wild-type specific upstream primer and saltant type specific upstream primer share;
And described wild-type specific upstream primer has SEQ No.17 sequence, described saltant type specific upstream primer has SEQ No.14 sequence, and described shared downstream primer has SEQ No.16 sequence.
One aspect of the present invention additionally provides a kind of reagent detecting PDGFRA gene D842V pleomorphism site, it is characterized in that: described reagent contains above-mentioned primer.
The present invention additionally provides a kind of test kit detecting PDGFRA gene D842V pleomorphism site on the other hand, it is characterized in that: described test kit is also containing above-mentioned primer.
Preferably, also comprise in described test kit with described primer with the use of probe, wherein, described probe is Taqman probe, has SEQ No.15 sequence.
Further preferably, described test kit also comprises PCR reaction tubes, dNTPs and Taq enzyme mixed solution, PCR damping fluid, the upstream primer detecting house-keeping gene GAPDH, the downstream primer detecting house-keeping gene GAPDH, the probe detecting house-keeping gene GAPDH, positive quality control product and blank;
The upstream primer of described detection house-keeping gene GAPDH has SEQ No.19 sequence; The downstream primer of described detection house-keeping gene GAPDH has SEQ No.20 sequence; The probe of described detection house-keeping gene GAPDH has SEQ No.21 sequence.
Further preferably, the probe of the upstream primer of described saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is coated in T-shaped PCR reaction tubes in advance; And be coated in advance in A type PCR reaction tubes with the probe of the upstream primer of described wild-type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH.
Further preferably, in described T-shaped PCR reaction tubes, the concentration and probe concentration of the upstream primer of saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 50nM-2um, 50nM-2uM, 50nM-400nM, 1pm-20pm, 1pm-20pm, 0.05pm-5pm; And the concentration and probe concentration of the upstream primer of wild type specificity upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 50nM-2um, 50nM-2uM, 50nM-400nM, 1pm-20pm, 1pm-20pm, 0.05pm-5pm in described A type PCR reaction tubes.
Further preferred, in described T-shaped PCR reaction tubes, the concentration and probe concentration of the upstream primer of saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 500nM, 500nM, 100nM, 5pm, 5pm, 2.5pm; And the concentration and probe concentration of the upstream primer of wild type specificity upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 500nM, 500nM, 100nM, 5pm, 5pm, 2.5pm in described A type PCR reaction tubes.
Present invention also offers the PCR method of above-mentioned primer and reagent, it is characterized in that: PCR reaction is undertaken by two step amplification cycles programs, and the cycle number of the first step amplification is less than the cycle number of second step amplification, the annealing temperature that the annealing temperature that the described the first step increases increases higher than described second step.
Preferably, the condition of described PCR reaction is: 37 DEG C of 2min, 95 DEG C of 2min denaturations; The first step increases, 95 DEG C of sex change 5s, and 55 DEG C ~ 68 DEG C annealing 32s, circulate 10 ~ 15 times; Second step, 95 DEG C of sex change 5s, 50 DEG C ~ 65 DEG C annealing, extend 32s, circulates 30 ~ 50 times, collection fluorescent signal; Further preferably, the condition of described PCR reaction is: 37 DEG C of 2min, 95 DEG C of 2min denaturations; The first step increases, 95 DEG C of sex change 5s, and 63 DEG C of annealing 32s, circulate 15 times; Second step, 95 DEG C of sex change 5s, 60 DEG C of annealing, extend 32s, circulates 40 times, collection fluorescent signal.
The primer of detection PDGFRA gene D842V pleomorphism site provided by the invention and test kit thereof, greatly can increase the ability that allele-specific primers PCR distinguishes not isoallele site, the non-specific possibility of intersecting amplification between different loci is made to drop to minimum, the amplification of real " all or none " formula can be accomplished, not only there is good specificity, also there is extraordinary sensitivity, the genotype distribution situation in 1ng genomic dna can be detected.
The primer of detection PDGFRA gene D842V pleomorphism site provided by the invention and test kit thereof, have the following advantages:
1) by for a change making the people on primer sequence detected result really accomplish to judge result " all or none ", enormously simplify the difficulty of result interpretation, reducing the possibility of makeing mistakes, for scientific research and clinical application are provided convenience.
2) the mixing of Taq enzyme and dNTPs, ensured the stability of dNTPs, made it can stand repeatedly the test of multigelation.
3) shift to an earlier date the pre-assigned damping fluid that can directly use, user is convenient.
4) primer and probe are coated in PCR reaction tubes in advance, avoid the possibility that site mismatch appears in operator, and also save a large amount of operating time.
5) in the present invention primer and test kit to have specificity good, detection highly sensitive, detection speed is fast, and whole process can complete in 1 hour 20 minutes.
6) only use a conventional Taqman probe in test kit, such as do not close probe without other, reduce costs.
7) this test kit has and detects the advantage such as simple, quick, accurate, inexpensive.
Accompanying drawing explanation
Fig. 1 is pcr amplification graphic representation when designing wild-type and mutant primers;
Fig. 2 is the pcr amplification graphic representation in T site;
Fig. 3 is the pcr amplification graphic representation in A site;
Fig. 4 is the pcr amplification graphic representation in AT site.
Fig. 5 is the pcr amplification graphic representation of house-keeping gene GAPDH.
Embodiment
With concrete case, the present invention is further expalined below, but is not limited to protection scope of the present invention.
If do not specialize, the conventional means that technique means used in embodiment is well known to those skilled in the art, product used is commercial.
The explanation of relational language in the present invention to give a definition:
" allelotrope " generally refers to region of DNA section, in the same, physical on homologous chromosomes, controls the one pair of genes of contrast character.In some cases, allelotrope can correspond to the replacement of the mononucleotide on specific physics locus.In other situation, allelotrope can correspond to Nucleotide (single or multiple) and insert or disappearance.
" allele-specific primers " refers to the complementary with target alleles, can extend special PCR reaction when PCR.Allele-specific primers can be designed to detect few primer very special to 1 nucleotide difference in target sequence, and this primer can comprise allele-specific nucleotide part, 3 ' end target specificity part and tail.
" MGB group " refers to minor groove binding.When the 3 ' end with oligonucleotide is puted together, MGB group can play a role as inextensible enclosure portion.MGB is the molecule that can be incorporated in the ditch of double-stranded DNA, usually adopts its synthetic method of DPI3(see U.S. Patent number 6,084,102; With 6,727,356).
" detection probes " refers to: instruction amplification multi-signal transduction molecule in any one.Such as, SYBR Green and other DNA binding dye are all detection probes.Some detection probes can be sequence-specific, such as Taqman probe (U.S. Patent number 5, 538, 848), multiple stem toroidal molecule beacon (U.S. Patent number 6, 103, 476 and 5, 925, 517 and Tyagi and Kramer, Nature Biotechnology, 1996, 14:303-308), acaulescence or Linear Beacon (WO99/21881), PNA Molecular Beacons TM (U.S. Patent number 6, 355, 421 and 6, 593, 091), the linear PNA beacon (people such as Kubista, 2001, SPIE4264:53-58), non-FRET probe (U.S. Patent number 6, 150, 097), Sunrise/Amplifluor probe (U.S. Patent number 6, 548, 250), stem ring and the double-strand Scorpion TM probe (people such as Solinas, 2001, NucleicAcidsResearch29:E96 and U.S. Patent number 6, 589, 743), ring probe (the U.S. Patent number 6 heaved, 590, 091), false knot probe (U.S. Patent number 6, 589, 250), cyclicon (U.S. Patent number 6, 383, 752), MGB Eclipse TM probe (Epoch Biosciences), hairpin probe (U.S. Patent number 6, 596, 490), peptide nucleic acid(PNA) (PNA) probe.Detection probes can comprise fluorescent reporter molecule, such as, 6-Fluoresceincarboxylic acid (6-FAM) or Tetrachlorofluorescein (TET), with quencher molecule part, such as tetramethylrhodamin (TAMRA), Black Hole Quenche RS (Biosearch), Iowa Black (IDT), QSY quencher (Molecular Probes) and Dabsyl and Dabcel sulfonate/carboxylate salt quencher (Epoch).
" share Auele Specific Primer " and refer to the primer matched with allele-specific primers in PCR reaction, it can use with the allele-specific primers pairing of different loci.
" polysaccharase of thermostability " refer to thermostability or the enzyme of heat resistance, mainly referring to archaeal dna polymerase, when pcr amplification, can not there is inactivation in this enzyme at an elevated temperature.
" Tm " or " melting temperature (Tm) " of oligonucleotide refers to temperature during molecule and the complementary sequence hybridization of in section of DNA 50%.Tm value can use the formula known to calculate (see, people such as Maniatis, T.: Molecular cloning, Cold Spring Harbor, N.Y.:1982).
" sensitivity " refers to the minimum (copy number) that can be detected template.
" specificity " refers to the ability distinguishing matching template and mispairing template.Specificity is mated through being often expressed as Δ Ct=Ct mispairing-Ct.
" selectivity " refers to that AS-PCR measures and can be used for measuring minority (normally suddenling change) allelotrope in mixture and without the degree from most (being often wild-type) allelic interference.Selectivity is through being often expressed as ratio or percentage.Such as, the mensuration that can detect 1 mutagenesis template when existence 100 wild-type template is referred to as the selectivity with 1: 100 or 1%.
" Ct " value refers to cycle threshold, represents cycle number when pcr amplification curve becomes exponential growth flex point from baseline.
When " Delta Ct " or " Δ Ct " refers to signal by fixed threshold, two different samples or reaction between cycle number difference.Δ Ct is when reaching exponential amplification, two different samples or reaction between cycle number difference.Δ Ct can be used for identifying the specificity between coupling primer and mismatched primers.
The present invention relates to primer and the test kit of rapid detection PDGFRA gene D842V pleomorphism site.Specifically, the present invention is based on Past-PCR(Perfect allele-specific Taqman PCR) on the basis of method, be successfully applied to PDGFRA gene D842V pleomorphism site and detect.So-called Past-PCR is combined into by detecting gene polymorphism sites or the high specific AS-PCR method of sudden change and the Fluorescence PCR assay of Taqman probe, it only uses a Taqman probe, under most of the cases, this probe is conventional Taqman probe, only in portion gene because being rich in the special sequence of AT base, adopt the probes such as Taqman-MGB or LNA, in addition without the need to any extra closed probe or reporter probe, Past-PCR method is by the two kinds of method perfect adaptations of AS-PCR and Taqman fluorescent PCR, and make both advantages obtain performance extremely, be in particular in AS-PCR method, when not increasing any cost, successfully non-specific amplification is eliminated by design of primers and unique verification method, result is made to judge to present " complete and nothing " mode, namely have and just have, just do not have, make the judgement of result simply and accurately, this is to the maximum improvement of the AS-PCR method in past, also be effectively making up that AS-PCR method is that This is what people generally disapprove of, thus the advantage of AS-PCR method performed to ultimate attainment, the tidemark that the method can reach.As everyone knows, Taqman fluorescent PCR has stopping property and detects the process after finishing without the need to reaction, not only save the time, and decrease the risk of PCR primer pollution, the second time identification target sequence of probe has ensured the specificity and reliability that detect, also can be used for, to the detection by quantitative of gene, reaching the advantages such as criterion for clinical use.Past-PCR method has the two-fold advantage of AS-PCR method and Taqman fluorescence PCR method, and be these two kinds of methods combining together time, detect the most simplification formation that component can reach, therefore, we call it as perfect allele-specific Taqman PCR.
Based on Past-PCR method, invented the test kit for detecting gene PDGFRA gene D842V pleomorphism site, it basic composition is: the allele-specific primers of (a) high special; (b) fluorescent detection probe; C another Auele Specific Primer that () and allele-specific primers match.
Wherein, the primer of detection PDGFRA gene D842V pleomorphism site provided by the invention, comprising: the downstream primer that wild-type specific upstream primer, saltant type specific upstream primer and wild-type specific upstream primer and saltant type specific upstream primer share;
And described wild-type specific upstream primer has SEQ No.17 sequence, described saltant type specific upstream primer has SEQ No.14 sequence, and described shared downstream primer has SEQ No.16 sequence.
Additionally provide the detection reagent containing above-mentioned primer and test kit simultaneously, detect PDGFRA gene D842V pleomorphism site in the past to solve to there is operation easier large, there is certain false negative and false positive, testing cost is high, clinical popularity is low, simultaneously can not detect the problems such as clinical samples on a large scale, achieve and detect simple, quick, accurate, cheap desirable, for scientific research and clinical gene type and gene mutation analysis provide strong instrument.
Preferably, also comprise in described test kit with described primer with the use of probe, wherein, described probe is Taqman probe, has SEQ No.15 sequence, only uses a probe in whole test kit, other without other such as closed probes etc., reduce the cost of test kit.
Further preferably, described test kit also comprises PCR reaction tubes, dNTPs and Taq enzyme mixed solution, PCR damping fluid, the upstream primer detecting house-keeping gene GAPDH, the downstream primer detecting house-keeping gene GAPDH, the probe detecting house-keeping gene GAPDH, positive quality control product and blank;
The upstream primer of described detection house-keeping gene GAPDH has SEQ No.19 sequence; The downstream primer of described detection house-keeping gene GAPDH has SEQ No.20 sequence; The probe of described detection house-keeping gene GAPDH has SEQ No.21 sequence; Wherein, by dNTPs and Taq enzyme mixing, the stability of dNTPs can be ensured, make it can stand repeatedly the test of multigelation; Detecting the upstream primer of house-keeping gene GAPDH, downstream primer and probe is for as internal reference, for preventing occurring false negative when detecting; Positive quality control product is AT type human gene group DNA; Blank is sterilizing ultrapure water.
Further preferably, the probe of the upstream primer of described saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is coated in T-shaped PCR reaction tubes in advance, and with described wild-type specific upstream primer, described shared downstream primer, described probe, the upstream primer of described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and the probe of described detection house-keeping gene GAPDH are coated in A type PCR reaction tubes in advance, be coated in PCR reaction tubes in advance by the reaction consumption of the best, in each reaction tubes, actual bag is by six oligonucleotides, namely one for allelic a kind of specific upstream primer, , a probe (being generally Taqman probe), , a shared specific Down Stream primer, article one, detect the upstream primer of house-keeping gene GAPDH, article one, detect the downstream primer of house-keeping gene GAPDH and the probe of a detection house-keeping gene GAPDH.Like this in order to detect the different gene pleiomorphism in a site, often need to wrap respectively and managed above PCR reaction tubes by two pipes or two, the downstream primer of their middle probes, shared specific Down Stream primer, the upstream primer detecting house-keeping gene GAPDH, detection house-keeping gene GAPDH and the probe of detection house-keeping gene GAPDH are the same, different is only other specific upstream primer of qualification allelotrope different shaped, bag is avoided the possibility that site mismatch appears in operator so in advance, and has saved a large amount of operating time.
Further preferably, in described T-shaped PCR reaction tubes, the concentration and probe concentration of the upstream primer of saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 50nM-2um, 50nM-2uM, 50nM-400nM, 1pm-20pm, 1pm-20pm, 0.05pm-5pm; And the concentration and probe concentration of the upstream primer of wild type specificity upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 50nM-2um, 50nM-2uM, 50nM-400nM, 1pm-20pm, 1pm-20pm, 0.05pm-5pm in described A type PCR reaction tubes.Optimum is, in described T-shaped PCR reaction tubes, the concentration and probe concentration of the upstream primer of saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 500nM, 500nM, 100nM, 5pm, 5pm, 2.5pm; And the concentration and probe concentration of the upstream primer of wild type specificity upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 500nM, 500nM, 100nM, 5pm, 5pm, 2.5pm in described A type PCR reaction tubes.
Owing to introducing the base of mispairing in allele-specific primers, make its react time decrease in efficiency, different primer decline degree is different, usually 10 to 20 effects that just can reach when not having mispairing that circulate will be increased, ensure the sensitivity detected, preferred PCR reaction is undertaken by two step amplification cycles programs, and the cycle number of the first step amplification is less than the cycle number of second step amplification, the annealing temperature that the annealing temperature that the described the first step increases increases higher than second step, the first step amplification uses higher anneal temperature, second step amplification uses comparatively low temperature thermal oxidation, specificity when object is primer annealing when increasing the first step amplification, thus ensure that Past-PCR detects the object of high degree of specificity, specifically the condition of preferred described PCR reaction is: 37 DEG C of 2min, 95 DEG C of 2min denaturations, the first step increases, 95 DEG C of sex change 5s, and 55 DEG C ~ 68 DEG C annealing 32s, circulate 10 ~ 15 times, second step, 95 DEG C of sex change 5s, 50 DEG C ~ 65 DEG C annealing, extend 32s, circulates 30 ~ 50 times, collection fluorescent signal, the condition of more preferred PCR reaction is: 37 DEG C of 2min, 95 DEG C of 2min denaturations, the first step increases, 95 DEG C of sex change 5s, and 63 DEG C of annealing 32s, circulate 15 times, second step, 95 DEG C of sex change 5s, 60 DEG C of annealing, extend 32s, circulates 40 times, collection fluorescent signal.
Concrete testing process is:
1) detected sample is put into respectively be coated with wild-type special primer respectively in advance, the downstream primer shared, probe, detect the upstream primer of house-keeping gene GAPDH, detect the downstream primer of house-keeping gene GAPDH and detect probe and the saltant type special primer of house-keeping gene GAPDH, the downstream primer shared, probe, detect the upstream primer of house-keeping gene GAPDH, detect the downstream primer of house-keeping gene GAPDH and detect in probe two groups of PCR reaction tubess of house-keeping gene GAPDH, and add PCR damping fluid, dNTPs and Taq enzyme mixed solution, sterilizing ultrapure water and genomic dna, cover tightly pipe lid, quantitative real time PCR Instrument reacts, and collect fluorescent signal,
2) if detect the sample amplification curve that only has saltant type reaction tubes to have logarithm to increase at FAM passage, while the VIC passage amplification curve that has logarithm to increase, can judge that sample is as T-shaped, i.e. saltant type homozygote;
If detect the sample amplification curve that only has wild-type reaction tubes to have logarithm to increase at FAM passage, while the VIC passage amplification curve that has logarithm to increase, can judge that sample is as A type, i.e. wild-type homozygote;
If detect the amplification curve that sample saltant type and wild-type reaction tubes all have logarithm to increase at FAM passage, while the VIC passage amplification curve that has logarithm to increase, can judge that sample is as AT type, i.e. heterozygote;
If detection sample saltant type and wild-type reaction tubes are at FAM passage all without the amplification curve that logarithm increases, possible sample or operation have problems, or sample DNA concentration is too low, should again extract sample DNA and test.
Each component introduction in testing process is described in detail in detail below:
(1) allele-specific primers:
The allele-specific nucleotide partial complementarity of allele-specific primers in an allelotrope site of gene, but is not complementary to another allelotrope site of this gene.Typically, the allele-specific nucleotide part of allele-specific primers is positioned at the last bit base that 3 ' of allele-specific primers is held.In some cases, allele-specific nucleotide part also can be positioned at other base positions of allele-specific primers 3 ' end.
In some cases, allele-specific primers is except 3 ' termini-complementary changes to some extent in allelotrope site, we usually will introduce the base of mispairing in other positions of primer, as held penultimate or the 3rd to introduce base mispairing at primer 3 ', or second and the continuous mispairing of the 3rd; For different SNP or mutational site, hold at primer 3 ' on the basis of penultimate or the 3rd introducing base mispairing, also can increase the requirement that base mispairing meet atopic in other site of primer, more away from 3 ' end, the base number increasing mispairing is more, can reach at most at 5 ' end.Its T of length Main Basis of allele-specific primers mvalue decides, typically its T mbe worth about 5-20 DEG C lower than the annealing temperature of PCR circulation.
Article two, detect the allele-specific upstream primer of corresponding gene pleiomorphism, except its base difference of site that 3 ' end detects, all the other sequences are identical as far as possible, the T of two primers mbe worth also consistent as far as possible.
Low T mallele-specific primers (ASP) have higher specificity.Generally, allele-specific primers is short oligonucleotide, and its length is about 15-30, its T mabout 40 DEG C to 60 DEG C, lower than the annealing/elongating temperature of the PCR cycling condition used in amplification procedure about 5 DEG C to 20 DEG C.
Due to the design of allele-specific primers and screening very important, good primer needs to select from numerous primer to be selected, and therefore we establish the method for a screening, and the concrete screening process of its allele-specific primers is as follows:
(1) design peripheral primer and pcr amplification: first in the upstream and downstream of transgenation point to be checked or SNP site, design a pair pcr amplification primer, then use this to primer, conventional PCR reaction is carried out to goal gene, wherein expanding fragment length can at tens to many kilobases pair, and preferred length is 200 to 500 base pairs;
(2) clone PCR products: by the PCR primer amplified, utilizes the method that AT clones, and in the carrier T plasmid of recombinating common, obtains recombinant plasmid, and the recombinant plasmid wherein obtained can carry out sequence verification, thus guarantees the exactness of PCR primer;
(3) build recombinant mutant: the information provided according to information biology, adopt molecule clone technology, by the sequence of mutant, build up in recombinant plasmid obtained above, the recombinant mutant of structure is carried out sequence verification sequence, thus guarantee its exactness;
(4) design and screen specific primer on the mutated site: designing two allele-specific primerses, 3 ' end of a primer is complementary with mutant nucleotide sequence, and 3 ' end of another primer is complementary with normal sequence; Then respectively with allele-specific primers and the common downstream primer pairing of corresponding Standard PCR, using the above-mentioned recombinant mutant built as reaction template, utilize quantitative real time PCR Instrument, to reaction system, screen; Wherein, reaction can adopt fluorescence dye, as SYBR GREEN, also can adopt specific Taqman fluorescence probe, and the standard being 0.1 microgram complete genome DNA according to added sample size is screened, and its concrete screening content is as follows:
(a) setting PCR reaction conditions: the annealing temperature first setting PCR reaction is completely the same, actual temp is 55 DEG C ~ 68 DEG C, PCR cycle index is 40 times, the enzyme of PCR reaction and buffer system immobilize after all optimizing, and simultaneously the setting of this reaction conditions conveniently detects several genes sudden change;
(b) specificity screening: adopt the primer of saltant type with the recombinant plasmid of wild-type for template, its Ct of the primer filtered out is greater than 40;
Wherein the determination reason of cycle threshold is as follows, mutant primers at wild-type template generation non-specific amplification than wild primers in many 19 circulations of wild-type template generation specific amplification, when detecting according to clinical practice, added sample size is the standard of 0.1 microgram complete genome DNA, we are by following formula, and copy number=(DNA measures ng × 6.022 × 10 23)/(length bp × 10 9× 660), wherein the length of complete genome DNA is 3,000,000,000 pairs of bases, and therefore the copy number of 0.1 microgram complete genome DNA is: 3.09 × 10 4be reflected in the quantitative cycle threshold of Ct(of quantitative fluorescent PCR) be probably 21, we obtain second screening index like this, namely use the primer of saltant type, when the recombinant plasmid of wild-type is template, the Ct of gained should be greater than 40, can ensure that detection there will not be false positive, both amplification efficiency differences are 40-21=19 circulation, and namely amplification efficiency differs more than 19 circulations, will become the objective indicator that we judge allele-specific primers specificity quality.We know when primer 3 ' is held with template mispairing, extend efficiency and will decline 10 3-10 6.6doubly, be converted into reaction cycle number then to decline about 13 to 27 circulations, Here it is, and we can filter out the theoretical foundation of desirable primer, because do not carry out primer screening, 19-13=6 circulation, certainly will produce false positive, the specificity of this primer is just bad, and 19-27=-8, false positive can not be produced, have the scope of 8 cycle numbers to screen primer for us.According to this requirement, we design a series of allele-specific primers, set about from length, near the artificial base mispairing of introducing of 3 ' end, add its downstream primer matched, utilize the wild-type and saltant type recombinant plasmid that build, carry out the intersection screening of quantitative fluorescent PCR reaction respectively, namely when increasing by the template of mutant primer and wild-type, more than multiplex 19 cycle numbers are wanted with the reaction of wild-type template with wild primers, vice versa, and so such primer just possesses the specificity of height.
C () susceptibility is screened: the Auele Specific Primer filtered out is done sensitivity test with recombination mutation type plasmid, and Auele Specific Primer detection sensitivity being less than 10-1000 copy screens, and is required mutant-specific primers.
By the screening of above several respects, the allele-specific primers obtained will possess high degree of specificity and extremely sensitive desirable primer.
(2) detection probes:
In some cases, the T of detection probes mvalue is approximately 60 DEG C to 70 DEG C, and the best is 65 DEG C, and probe length is according to its T mvalue determines.Although there is multiple multi-form probe available, Taqman probe (Applied Biosystems, Foster City) is usually first-selected.In some special cases, as detected AT too high levels in sequence, can adopt and improve T mthe probe of the types such as the Taqman-MGB of value.
The Auele Specific Primer shared, in some cases, the T of the Auele Specific Primer shared mvalue is approximately 50 DEG C to 70 DEG C, and the best is 60 DEG C, and its length is by its T mvalue determines, generally between 15-25 base.
(3) other compositions:
The archaeal dna polymerase that the present invention uses is Taq enzyme, and mutant, derivative or fragment, may also be other hot resistant DNA polymerase, in some cases, also can adopt Hotstart Taq enzyme, to increase the special of reaction and high efficiency.
The primer provided for PDGFRA gene D842V pleomorphism site provided in the present invention and test kit, mainly for the shortcoming of allele-specific primers pcr amplification method, utilize molecule clone technology, build the recombinant plasmid containing gene wild-type to be checked and saltant type in advance respectively, with this recombinant plasmid for positive template, screening determine specifically respectively with two special primers of 3' terminal mutation site or wild site base complementrity, once the specific primer sequences filtered out, it will be the key element of our detection system.The said products of the present invention, can be used for the quantitative real time PCR Instrument of any model, and reagent cost is worked as with nowadays quantitative fluorescent PCR Reagent evaluation on the market, therefore overcomes the deficiency that other adopt allele-specific primers pcr amplification methods preferably.
The invention has the advantages that: described test kit has simple to operate, cost is low, result judges easily simple, highly sensitive, and the mutator gene DNA template number that this test kit detection transgenation sensitivity can reach 1%(and goal gene accounts for 1% of wild-type DNA profiling number); And the mutator gene DNA template number that the sensitivity detecting transgenation in direct Sequencing is 20%(and goal gene accounts for 20% of wild-type DNA template number); Taqman probe technique has ensured that the stopped pipe that is detected as of test kit reacts, effectively avoid false-positive generation, its detection specificity is also fully guaranteed, and detect quick and convenient, whole testing process only has 80 minutes, direct Sequencing then needs the time of 2 days, and is open pipe operation, and the possibility that PCR primer is polluted increases.
PCR(Past-PCR in the present invention) implementation step:
1. the structure of positive plasmid
In the upstream and downstream design one couple of PCR primers of PDGFRA gene D842V pleomorphism site to be detected, the length of its amplified fragments can in the scope of 500bp, be template with gDNA, adopt conventional PCR method, amplify this fragment, by the mode that AT clones, be cloned in the plasmid of order-checking by this fragment, the pCR2.1 Topo carrier T test kit of usual Invitrogen, operation by specification carries out, also can with the carrier T test kit of other producers, the carrier T plasmid even can prepared with oneself.The positive colony obtained, through sequence verification, prove the exactness of sequence, then the Quickchange test kit of Stratagene company is adopted, design another genotyping primer in corresponding site, by the method for Quickchange, obtain other positive colony of this saltant type, operation by specification carries out, and the positive plasmid obtained must be all next step the use of being correctly allowed for access through sequence verification.The quantitative plasmid of Taqman, and be used as template to verify susceptibility, linear dynamic range, the specificity of given assay method.
2. the design of allele-specific primers (ASP) and screening
At the transgenation base position of primer 3 ' termini-complementary in correspondence, and introduce base mispairing primer 3 ' end penultimate or the 3rd, or second and the continuous mispairing of the 3rd; For different SNP or mutational site, hold on the basis of penultimate or the 3rd introducing base mispairing at primer 3 ', also can increase the requirement that base mispairing meets atopic in other site of primer, more away from 3 ' end, the base number increasing mispairing is more, can reach maximum allelotrope 1 Auele Specific Primers at 5 ' end.
The screening of ASP utilizes the wild-type and saltant type recombinant plasmid that build, carry out the intersection screening of quantitative fluorescent PCR reaction respectively, namely when increasing by the template of mutant primer and wild-type, more than multiplex 19 cycle numbers are wanted with the reaction of wild-type template with wild primers, vice versa, and so such primer just possesses the specificity of height.The Auele Specific Primer filtered out is done sensitivity test with corresponding recombinant plasmid, detection sensitivity is less than the sensitivity requirement that namely 10-1000 the primer copied reach detection, the primer meeting above-mentioned two conditions is exactly the ASP primer that we select, and can carry out next step detection.
3. amplifing reagent prepares and adds detected sample
(1) from test kit, take out each moiety, room temperature slowly melts PCR damping fluid, dNTPs and Taq enzyme mixed solution, positive quality control product, blank, puts upside down and shakes up.Each reaction tubes need add PCR damping fluid, Taq enzyme (dNTPs), sterilizing ultrapure water and DNA sample.Cover tightly pipe lid, after brief centrifugation, transfer to pcr amplification district.
(2) advise that the analysis of sample, positive quality control product, blank is carried out in each PCR reaction all simultaneously, the loading methods of positive quality control product and blank is with sample Adding Way.
4. reaction conditions
In each reaction tubes, (scope of reaction final volume can at 10-50 μ l, and the best is at 20-25 μ l reaction volume) comprises PCR damping fluid (10mM Tris-HCl pH8.3,50mM KCl, 0.1%Triton X-100,2.0mM MgCl 2), 10-100ng DNA or 1,000, the plasmid DNA of 000 copy, the general specificity T aqman probe that 50nM-400nM mono-is common, the general reverse specific Down Stream primer that a 50nM-2uM is common, the different allele-specific upstream primer of 50nM-2uM, 1pm-20pm detects the upstream primer of house-keeping gene GAPDH, 1pm-20pm detects the downstream primer of house-keeping gene GAPDH, 0.05pm-5pm detects the probe of house-keeping gene GAPDH, adds 1.5 units of Taq polymerase, 200 μMs of dNTPs.
1), cycling condition is arranged
For making fluorescence curve more attractive in appearance, advise collecting fluorescent signal from second step.
2), instrument sense channel is selected
Fluorescence signal acquisition temperature is set to 60 DEG C, and concrete method to set up please refer to corresponding instrument working instructions.
3), type of detection setting: blank is set to " NTC ", and positive quality control product and sample to be checked are set to " Unknown ".
5. interpretation of result
If detect the sample amplification curve that only has saltant type reaction tubes to have logarithm to increase at FAM passage, while the VIC passage amplification curve that has logarithm to increase, can judge that sample is as T-shaped, i.e. saltant type homozygote; If detect the sample amplification curve that only has wild-type reaction tubes to have logarithm to increase at FAM passage, while the VIC passage amplification curve that has logarithm to increase, can judge that sample is as A type, i.e. wild-type homozygote; If detect the amplification curve that sample saltant type and wild-type reaction tubes all have logarithm to increase at FAM passage, while the VIC passage amplification curve that has logarithm to increase, can judge that sample is as AT type, i.e. heterozygote; Because present method result is " all or none ", result very easily judges, which pipe responds, and which pipe is exactly positive.
Specific embodiment
Below for the situation to PDGFRA gene D842V polymorphic position point mutation detection, specifically the present invention is further detailed explanation.
Embodiment 1: the wild-type detected for PDGFRA gene D842V pleomorphism site and the preparation of saltant type positive plasmid
First we recall the gene order before and after PDGFRA gene D842V pleomorphism site from gene pool, and pleomorphism site double underline is marked, in the upstream and downstream appropriate location (indicating with boldface type and underscore) of PDGFRA gene D842V pleomorphism site, design a pair cloning primer, amplified fragments is 120bp, mutational site comprises in it, and gene order shows below, SEQ No.1:
agctacagatggcttgatcctgagtcatttcttccttttccatgcagtgtgt ccaccgtgatctggctgctc gcaacgtcctcctggcacaaggaaaaattgtgaagatctgtgactttggcctggccagag a catcatgcatgattc gaactatgtgtcgaaaggcagtgt acgtcctcacttccctcactggtcaggctcatcctccttcactttaatctctaaagtcaggtgttgcttctagagattcggtgcctgttttttaaaacatcaatagattt
Experimental procedure is as follows:
1) genomic dna is extracted
With the genome DNA extracting reagent kit of domestic Tian Gen company or Qiagen company, extract genomic dna, concrete operation step by specification carries out.The DNA sample prepared, measures concentration through ultraviolet spectrophotometer, its concentration is adjusted to 50ng/ μ l, be stored in-20 DEG C, or directly carry out reaction below.
2) AT clone obtains positive plasmid
First at catastrophe point upstream and downstream design cloning primer, in table 1:
Table 1. PDGFRA gene D842V pleomorphism site Wild type clone primer
In the PCR amplification system of 2 × PCR Master Mix (Fermentas) of 12.5 μ l, add 10 μMs of upstream primers and 10 μMs of downstream primers, and genomic dna 50ng, add water to cumulative volume 25 μ l, PCR reaction conditions is set as 95 DEG C of denaturation 3min, 95 DEG C of sex change 10s, 60 DEG C of annealing and extension 30s, 35 circulations altogether, get 15 μ l reaction product after reaction terminates, carry out the gel electrophoresis of concentration 2.5%, electrophoresis terminates rear observation, band conforms to the size of prediction, shows to increase successfully.Adopt the pCR2.0 TOPO carrier T of Life company of the U.S., by its operation instructions, by the mode that TA clones, obtain PDGFRA gene D842V pleomorphism site wild-type positive plasmid, concrete gene order is as follows, wherein pleomorphism site is shown as A type, is illustrated as wild-type, and it is correct that order-checking proves that institute obtains plasmid.
SEQ No.4:agctacagatggcttgatcctgagtcatttcttccttttccatgcagtgtgtccaccgtgatctggctgctcgcaacgtcctcctggcacaaggaaaaattgtgaagatctgtgactttggcctggccagag a catcatgcatgattcgaactatgtgtcgaaaggcagtgtacgtcctcacttccctcactggtcaggctcatcctccttcactttaatctctaaagtcaggtgttgcttctagagattcggtgcctgttttttaaaacatcaatagattt
3) rapid mutation method obtains mutant plasmid
Then, adopt the method (Quickchange, QC) producing rapid mutation, design mutant primer, primer sequence is in table 2.
Table 2. PDGFRA gene D842V pleomorphism site mutant clones primer
According to reaction conditions and the step of (Stratagene company) Quickchange test kit, complete the structure of mutant, the recombinant plasmid obtained, concrete gene order is as follows, through sequence verification wherein pleomorphism site be shown as T-shaped, for saltant type, then saltant type and wild plasmid are put-20 DEG C respectively and save backup.
SEQ No.7:agctacagatggcttgatcctgagtcatttcttccttttccatgcagtgtgtccaccgtgatctggctgctcgcaacgtcctcctggcacaaggaaaaattgtgaagatctgtgactttggcctggccagag t catcatgcatgattcgaactatgtgtcgaaaggcagtgtacgtcctcacttccctcactggtcaggctcatcctccttcactttaatctctaaagtcaggtgttgcttctagagattcggtgcctgttttttaaaacatcaatagattt
Embodiment 2: the design of allele-specific primers (ASP) and specificity screening
For PDGFRA gene D842V pleomorphism site, design wild-type and a series of sudden change Idiotype primer as follows:
PDGFRA-D842V-WT-R: cacatagttcgaatcatgcatgaagt(SEQ No.8)
PDGFRA-D842V-mut-R: cacatagttcgaatcatgcatgaaga(SEQ No.9)
PDGFRA-D842V-mut-R1: acatagttcgaatcatgcatgaaga(SEQ No.10)
PDGFRA-D842V-mut-R2: catagttcgaatcatgcatgaaga(SEQ No.11)
PDGFRA-D842V-mut-R3: cacatagttcgaatcatgcatgatca(SEQ No.12)
PDGFRA-D842V-mut-R4: acatagttcgaatcatgcatgatca(SEQ No.13)
PDGFRA-D842V-mut-R5: catagttcgaatcatgcatgatca(SEQ No.14)
Design and synthesis Taqman specific probe simultaneously:
SEQ No.15:FAM-ccaggccaaagtcacagatcttcacaat-BHQ1, relevant primer and probe synthesize in Sangon Biotech (Shanghai) Co., Ltd..
Then match with PDGFRA-D842V-F:5 '-ccaccgtgatctggctgctc-3 ' (SEQ No.16) primer of above-mentioned 7 primers and PDGFRA gene D842V pleomorphism site respectively, add Taqman specific probe, adding wild-type recombinant plasmid about 30,000 copy that aforementioned structure obtains is template, quantitative real time PCR Instrument carries out primer specificity screening, reaction conditions is set as the first step 95 DEG C of 2min denaturations, 95 DEG C of 5s, 63 DEG C of 30s totally 15 circulations, do not collect fluorescent signal, second step 95 DEG C of 5s, 60 DEG C of 30s totally 40 circulations, collect fluorescent signal, the results are shown in Figure 1.
Wherein, in Fig. 1,1 ~ 7 curve represents PDGFRA-D842V-WT-R respectively, PDGFRA-D842V-mut-R, PDGFRA-D842V-mut-R1, PDGFRA-D842V-mut-R2, PDGFRA-D842V-mut-R3, PDGFRA-D842V-mut-R4, the pcr amplification curve of PDGFRA-D842V-mut-R5, from Fig. 1, we find out that No. 1 wild primers produces amplified signal 9 circulations, the specificity of 2-6 primer is poor, non-specific amplification is produced respectively at 9-11 circulation time, same wild primers (No. 1) amplification efficiency difference is less than 19 circulations, No. 7 primer meets our requirement, at 40 circulation times, still do not increase, 19 circulations are differed by more than with wild primers amplification efficiency.In order to have better comparability with mutant primer, we with reference to the primer of No. 7 Primer redesign wild-type are: catagttcgaatcatgcatgatct(SEQ No.17).
Embodiment 3:ASP sensitivity is screened
Match with the common downstream primer SEQ No.16 of PDGFRA gene D842V pleomorphism site respectively with mutant primers again, use saltant type recombinant plasmid, according to 10 6, 10 5, 10 4, 10 3, 10 2, 10,0 makes gradient dilution, adds Taqman specific probe, in the enterprising line sensitivity checking of quantitative real time PCR Instrument.Sudden change Idiotype primer can detect 100 mutant copied, and therefore this primer is exactly filter out by our method the best primer detecting PDGFRA gene D842V pleomorphism site, is shown in Table 3.
Embodiment 4: prefabricated PCR(Past-PCR of the present invention) reaction tubes
According to the requirement of two reaction tubess in each mutational site, namely a pipe detects wild type site, and another pipe detects mutational site, is coated in advance by the primed probe of suitable concentration in the milky PCR reaction tubes of 0.2ML.
In order to prevent occurring false negative when detecting, in each reaction tubes, be coated with the upstream primer, downstream primer and the probe that detect house-keeping gene GAPDH all in advance, wherein, GAPDH gene order is as follows:
cctccgggaaactgtggcgtgatggccgcggggctctccagaacatcatccctgcctctactggcgctgccaaggctgtgggcaaggtcatccctgagctgaacgggaagctcactggcatggccttccgtgtccccactgccaacgtgtcagtggtggacctgacctgccgtctagaaaaacctgccaaatatgatgacatcaagaaggtggtgaagcaggcgtcggagggccccctcaagggcatcctgggctacactgagcaccaggtggtctcctctgacttcaacagcgacacccactcctccacctttgacgctggggctggcattgccctcaacg(SEQ No.18)
The upstream primer sequence detecting house-keeping gene GAPDH is: ggctgtgggcaaggtcatc(SEQ No.19)
The downstream primer sequence detecting house-keeping gene GAPDH is: ctccgacgcctgcttcaccac (SEQ No.20)
The probe sequence detecting house-keeping gene GAPDH is: ccttccgtgtccccactgccaacgt (SEQ No.21)
Wherein, the probe 5 ' end detecting house-keeping gene GAPDH uses HEX fluorescent mark, 3 ' end BHQ mark, and because HEX and VIC belongs to same Air conduct measurement, and many instruments often adopt VIC to indicate, and therefore describe with VIC in literary composition.
In PCR reaction tubes, concrete details is in table 3.
The component of table 3. prefabricated PDGFRA gene D842V pleomorphism site Past-PCR reaction tubes and concentration
Because we are coated on the probe of saltant type and wild-type upstream primer, probe, common downstream primer, the upstream and downstream primer detecting house-keeping gene GAPDH and detection house-keeping gene GAPDH in the differential responses pipe of the number of finishing in advance, effectively prevent the operate miss of user, substantially increase operation efficiency simultaneously, greatly facilitate actual use clinically.
Embodiment 5: the checking of sample
Gather the peripheral blood of normal population or mouth desquamated cells sample, and with the genome DNA extracting reagent kit of Qiagen company, extraction genomic dna, concrete operation step by specification carries out.The DNA sample prepared, measures concentration through ultraviolet spectrophotometer, its concentration is adjusted to 100ng/ μ l for subsequent use.
We, with this mutant-specific primers filtered out, compare with wild primers simultaneously, and on same PCR Sptting plate, every two reaction tubess detect a gene locus, and one of them is mutational site, and another is wild type site.10mM Tris-HCl pH8.3 is comprised, 50mM KCl, 0.1%Triton X-100,2.0mM MgCl in each reaction tubes 20 μ l reaction volume 2100ng human gene group DNA, 100nM specificity T aqman probe, 500nM shares specific Down Stream primer, 500nM wild-type specific upstream primer or saltant type specific upstream primer, 5pm detects the upstream primer of house-keeping gene GAPDH, 5pm detects the downstream primer of house-keeping gene GAPDH, and 2.5pm detects the probe of house-keeping gene GAPDH, adds 1.5 unit Taq archaeal dna polymerases, 200 μMs of dNTPs, all the other are deionized water.
The first step PCR reaction conditions is: 37 DEG C of 2min, 95 DEG C of 2min denaturations, then 95 DEG C of 5s, 63 DEG C of 30s, 15 circulations, and this step does not collect fluorescence; Second step PCR reaction conditions is: 95 DEG C of 5s, 60 DEG C of 30s, totally 40 circulations, and this step collects fluorescence.For convenience's sake, PDGFRA gene D842V polymorphism normal locations is regarded as wild-type (A site) by us, and PDGFRA gene D842V polymorphism mutation site (T site), if the amplification curve that the reaction tubes of correspondence has logarithm to increase at FAM passage, simultaneously the VIC passage amplification curve that has logarithm to increase, is just judged as the homozygous genotype of correspondence; As the amplification curve that two Guan Jun have logarithm to increase at FAM passage, simultaneously the VIC passage amplification curve that has logarithm to increase, be then heterozygous.
1, carry out mutation allele homozygote (T site) according to the method described above to detect, its concrete gene order is:
SEQ No.22:ctggccagag t catcatgcat
The FAM passage pcr amplification graphic representation collected, as shown in Figure 2, wherein, the representative of a curve detects the amplification curve in saltant type PCR reaction tubes, and the representative of b curve detects the amplification curve in wild-type PCR reaction tubes.
2, carry out wild allele genic homozygote (A site) according to the method described above to detect, its concrete gene order is:
SEQ No.23:ctggccagag a catcatgcat
The FAM passage pcr amplification graphic representation collected, as shown in Figure 3, wherein, the representative of c curve detects the amplification curve in wild-type PCR reaction tubes, and the representative of d curve detects the amplification curve in saltant type PCR reaction tubes.
3, carry out heterozygosis (AT type) according to the method described above to detect, its concrete gene order is:
SEQ No.24:ctggccagag a/t catcatgcat
The FAM passage pcr amplification graphic representation collected, as shown in Figure 4, wherein, the representative of e curve detects the amplification curve in wild-type PCR reaction tubes, and the representative of f curve detects the amplification curve in saltant type PCR reaction tubes.
Meanwhile, above-mentioned 3 are detected in cases, and when the amplification curve that VIC passage house-keeping gene GAPDH has logarithm to increase, as shown in Figure 5, the FAM passage amplification curve that has logarithm to increase simultaneously, then this experimental result is effective.
Therefore, from above-mentioned detection experiment, the detected result of this test kit is the result of " all or none ", even detected sample is mutation allele homozygote, in two PCR reaction tubess, only have the amplification curve that saltant type PCR reaction tubes all has logarithm to increase at FAM passage and VIC passage, and wild-type PCR reaction tubes has no amplification curve at FAM passage; If detected sample is wild allele genic homozygote, in two PCR reaction tubess, only have the amplification curve that wild-type PCR reaction tubes all has logarithm to increase at FAM passage and VIC passage, and saltant type PCR reaction tubes has no amplification curve at FAM passage; If detected sample is heterozygote, the fluorescent signal that two PCR reaction tubess all have logarithm to increase at FAM passage and VIC passage.The detected result interpretation of this test kit is simple, the detected result decreasing test kit in the past needs the process of carrying out the series of complex calculating such as Δ Ct, reduce false determination ratio, also effectively prevent the generation that there is false negative false positive phenomenon in test kit detected result in the past simultaneously.In addition test kit provided by the invention can be used for the quantitative real time PCR Instrument of any model, and detecting instrument is simple, and cost is low, for scientific research and clinical PDGFRA gene D842V pleomorphism site somatotype and gene mutation analysis provide strong instrument.
Sequence table
You Jinuo bio tech ltd, <110> Shenyang
<120> detects the primer of PDGFRA gene D842V pleomorphism site, test kit and PCR method thereof
<130> 2015
<160> 24
<170> PatentIn version 3.3
<210> 1
<211> 282
<212> DNA
<213> artificial sequence
<400> 1
agctacagat ggcttgatcc tgagtcattt cttccttttc catgcagtgtgtccaccgtg 60
atctggctgc tcgcaacgtc ctcctggcac aaggaaaaat tgtgaagatctgtgactttg 120
gcctggccag agacatcatg catgattcga actatgtgtc gaaaggcagtgtacgtcctc 180
acttccctca ctggtcaggc tcatcctcct tcactttaat ctctaaagtcaggtgttgct 240
tctagagatt cggtgcctgt tttttaaaac atcaatagat tt 282
<210> 2
<211> 20
<212> DNA
<213> artificial sequence
<400> 2
ccaccgtgat ctggctgctc 20
<210> 3
<211> 24
<212> DNA
<213> artificial sequence
<400> 3
acactgcctt tcgacacata gttc 24
<210> 4
<211> 282
<212> DNA
<213> artificial sequence
<400> 4
agctacagat ggcttgatcc tgagtcattt cttccttttc catgcagtgtgtccaccgtg 60
atctggctgc tcgcaacgtc ctcctggcac aaggaaaaat tgtgaagatctgtgactttg 120
gcctggccag agacatcatg catgattcga actatgtgtc gaaaggcagtgtacgtcctc 180
acttccctca ctggtcaggc tcatcctcct tcactttaat ctctaaagtcaggtgttgct 240
tctagagatt cggtgcctgt tttttaaaac atcaatagat tt 282
<210> 5
<211> 26
<212> DNA
<213> artificial sequence
<400> 5
ctggccagag tcatcatgca tgattc 26
<210> 6
<211> 26
<212> DNA
<213> artificial sequence
<400> 6
gaatcatgca tgatgactct ggccag 26
<210> 7
<211> 282
<212> DNA
<213> artificial sequence
<400> 7
agctacagat ggcttgatcc tgagtcattt cttccttttc catgcagtgtgtccaccgtg 60
atctggctgc tcgcaacgtc ctcctggcac aaggaaaaat tgtgaagatctgtgactttg 120
gcctggccag agtcatcatg catgattcga actatgtgtc gaaaggcagtgtacgtcctc 180
acttccctca ctggtcaggc tcatcctcct tcactttaat ctctaaagtcaggtgttgct 240
tctagagatt cggtgcctgt tttttaaaac atcaatagat tt 282
<210> 8
<211> 26
<212> DNA
<213> artificial sequence
<400> 8
cacatagttc gaatcatgca tgaagt 26
<210> 9
<211> 26
<212> DNA
<213> artificial sequence
<400> 9
cacatagttc gaatcatgca tgaaga 26
<210> 10
<211> 25
<212> DNA
<213> artificial sequence
<400> 10
acatagttcg aatcatgcat gaaga 25
<210> 11
<211> 24
<212> DNA
<213> artificial sequence
<400> 11
catagttcga atcatgcatg aaga 24
<210> 12
<211> 26
<212> DNA
<213> artificial sequence
<400> 12
cacatagttc gaatcatgca tgatca 26
<210> 13
<211> 25
<212> DNA
<213> artificial sequence
<400> 13
acatagttcg aatcatgcat gatca 25
<210> 14
<211> 24
<212> DNA
<213> artificial sequence
<400> 14
catagttcga atcatgcatg atca 24
<210> 15
<211> 28
<212> DNA
<213> artificial sequence
<400> 15
ccaggccaaa gtcacagatc ttcacaat 28
<210> 16
<211> 20
<212> DNA
<213> artificial sequence
<400> 16
ccaccgtgat ctggctgctc 20
<210> 17
<211> 24
<212> DNA
<213> artificial sequence
<400> 17
catagttcga atcatgcatg atct 24
<210> 18
<211> 342
<212> DNA
<213> artificial sequence
<400> 18
cctccgggaa actgtggcgt gatggccgcg gggctctcca gaacatcatccctgcctcta 60
ctggcgctgc caaggctgtg ggcaaggtcatccctgagctgaacgggaagctcactggca 120
tggccttccg tgtccccact gccaacgtgt cagtggtgga cctgacctgccgtctagaaa 180
aacctgccaa atatgatgac atcaagaaggtggtgaagcaggcgtcggagggccccctca 240
agggcatcct gggctacact gagcaccagg tggtctcctc tgacttcaacagcgacaccc 300
actcctccac ctttgacgct ggggctggca ttgccctcaa cg 342
<210> 19
<211> 19
<212> DNA
<213> artificial sequence
<400> 19
ggctgtgggc aaggtcatc 19
<210> 20
<211> 21
<212> DNA
<213> artificial sequence
<400> 20
ctccgacgcc tgcttcacca c 21
<210> 21
<211> 25
<212> DNA
<213> artificial sequence
<400> 21
ccttccgtgt ccccactgcc aacgt 25
<210> 22
<211> 21
<212> DNA
<213> artificial sequence
<400> 22
ctggccagag tcatcatgca t 21
<210> 23
<211> 21
<212> DNA
<213> artificial sequence
<400> 23
ctggccagag acatcatgca t 21
<210> 24
<211> 22
<212> DNA
<213> artificial sequence
<400> 24
ctggccagag atcatcatgc at 22

Claims (10)

1. one kind is detected the primer of PDGFRA gene D842V pleomorphism site, it is characterized in that, described primer comprises: the downstream primer that wild-type specific upstream primer, saltant type specific upstream primer and wild-type specific upstream primer and saltant type specific upstream primer share;
And described wild-type specific upstream primer has SEQ No.17 sequence, described saltant type specific upstream primer has SEQ No.14 sequence, and described shared downstream primer has SEQ No.16 sequence.
2. detect a reagent for PDGFRA gene D842V pleomorphism site, it is characterized in that: described reagent contains primer according to claim 1.
3. detect a test kit for PDGFRA gene D842V pleomorphism site, it is characterized in that: described test kit contains primer according to claim 1.
4. according to the test kit detecting PDGFRA gene D842V pleomorphism site described in claim 3, it is characterized in that: described test kit also comprise with primer described in claim 1 with the use of probe, wherein, described probe is Taqman probe, has SEQ No.15 sequence.
5. according to the test kit detecting PDGFRA gene D842V pleomorphism site described in claim 4, it is characterized in that: described test kit also comprises PCR reaction tubes, dNTPs and Taq enzyme mixed solution, PCR damping fluid, the upstream primer detecting house-keeping gene GAPDH, the downstream primer detecting house-keeping gene GAPDH, the probe detecting house-keeping gene GAPDH, positive quality control product and blank;
The upstream primer of described detection house-keeping gene GAPDH has SEQ No.19 sequence; The downstream primer of described detection house-keeping gene GAPDH has SEQ No.20 sequence; The probe of described detection house-keeping gene GAPDH has SEQ No.21 sequence.
6. according to the test kit detecting PDGFRA gene D842V pleomorphism site described in claim 5, it is characterized in that: the probe of the upstream primer of described saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is coated in T-shaped PCR reaction tubes in advance; And be coated in advance in A type PCR reaction tubes with the probe of the upstream primer of described wild-type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH.
7. according to the test kit detecting PDGFRA gene D842V pleomorphism site described in claim 6, it is characterized in that: in described T-shaped PCR reaction tubes, the concentration and probe concentration of the upstream primer of saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 50nM-2um, 50nM-2uM, 50nM-400nM, 1pm-20pm, 1pm-20pm, 0.05pm-5pm; And the concentration and probe concentration of the upstream primer of wild type specificity upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 50nM-2um, 50nM-2uM, 50nM-400nM, 1pm-20pm, 1pm-20pm, 0.05pm-5pm in described A type PCR reaction tubes.
8. according to the test kit detecting PDGFRA gene D842V pleomorphism site described in claim 7, it is characterized in that: in described T-shaped PCR reaction tubes, the concentration and probe concentration of the upstream primer of saltant type specific upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 500nM, 500nM, 100nM, 5pm, 5pm, 2.5pm; And the concentration and probe concentration of the upstream primer of wild type specificity upstream primer, described shared downstream primer, described probe, described detection house-keeping gene GAPDH, the downstream primer of described detection house-keeping gene GAPDH and described detection house-keeping gene GAPDH is respectively 500nM, 500nM, 100nM, 5pm, 5pm, 2.5pm in described A type PCR reaction tubes.
9. the PCR method of primer or the arbitrary test kit of claim 3 ~ 8 described in a claim 1, it is characterized in that: PCR reaction is undertaken by two step amplification cycles programs, and the cycle number of the first step amplification is less than the cycle number of second step amplification, the annealing temperature that the annealing temperature that the described the first step increases increases higher than described second step.
10. according to PCR method according to claim 9, it is characterized in that, the condition of described PCR reaction is: 37 DEG C of 2min, 95 DEG C of 2min denaturations; The first step increases, 95 DEG C of sex change 5s, and 55 DEG C ~ 68 DEG C annealing 32s, circulate 10 ~ 15 times; Second step, 95 DEG C of sex change 5s, 50 DEG C ~ 65 DEG C annealing, extend 32s, circulates 30 ~ 50 times, collection fluorescent signal; Or the condition of described PCR reaction is: 37 DEG C of 2min, 95 DEG C of 2min denaturations; The first step increases, 95 DEG C of sex change 5s, and 63 DEG C of annealing 32s, circulate 15 times; Second step, 95 DEG C of sex change 5s, 60 DEG C of annealing, extend 32s, circulates 40 times, collection fluorescent signal.
CN201510290644.3A 2015-05-29 2015-05-29 Detect primer, kit and its PCR method of PDGFRA gene D842V polymorphic sites Active CN104830991B (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
CN201510290644.3A CN104830991B (en) 2015-05-29 2015-05-29 Detect primer, kit and its PCR method of PDGFRA gene D842V polymorphic sites

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
CN201510290644.3A CN104830991B (en) 2015-05-29 2015-05-29 Detect primer, kit and its PCR method of PDGFRA gene D842V polymorphic sites

Publications (2)

Publication Number Publication Date
CN104830991A true CN104830991A (en) 2015-08-12
CN104830991B CN104830991B (en) 2018-04-27

Family

ID=53809186

Family Applications (1)

Application Number Title Priority Date Filing Date
CN201510290644.3A Active CN104830991B (en) 2015-05-29 2015-05-29 Detect primer, kit and its PCR method of PDGFRA gene D842V polymorphic sites

Country Status (1)

Country Link
CN (1) CN104830991B (en)

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN105463112A (en) * 2016-01-13 2016-04-06 武汉海吉力生物科技有限公司 Primers and probes and kit for detecting human PDGFRA gene D842V mutation
CN106636333A (en) * 2016-09-28 2017-05-10 广东凯普生物科技股份有限公司 PDGFRA gene mutation detection kit
CN107904290A (en) * 2017-11-09 2018-04-13 上海赛安生物医药科技股份有限公司 PDGFRA detection in gene mutation system and its kit
CN113943790A (en) * 2021-10-25 2022-01-18 北京华夏时代基因科技发展有限公司 Method for detecting ApoE single nucleotide polymorphism

Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN104328182A (en) * 2014-10-30 2015-02-04 武汉百泰基因工程有限公司 Primer, probe, locked nucleic acid probe, kit and detection method for detecting PDGFRA gene hotspot mutation
CN104531881A (en) * 2015-01-09 2015-04-22 湖南圣湘生物科技有限公司 Fluorescence PCR detection kit for human K-RAS gene mutation

Patent Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN104328182A (en) * 2014-10-30 2015-02-04 武汉百泰基因工程有限公司 Primer, probe, locked nucleic acid probe, kit and detection method for detecting PDGFRA gene hotspot mutation
CN104531881A (en) * 2015-01-09 2015-04-22 湖南圣湘生物科技有限公司 Fluorescence PCR detection kit for human K-RAS gene mutation

Non-Patent Citations (2)

* Cited by examiner, † Cited by third party
Title
赵静等: "ARMS技术联合Taqman探针检测100例非小细胞肺癌EGFR基因突变", 《中国肺癌杂志》 *
陈吉宝等: "等位基因特异PCR技术的研究与应用", 《植物遗传资源学报》 *

Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN105463112A (en) * 2016-01-13 2016-04-06 武汉海吉力生物科技有限公司 Primers and probes and kit for detecting human PDGFRA gene D842V mutation
CN105463112B (en) * 2016-01-13 2019-04-23 武汉海吉力生物科技有限公司 For detecting primer, probe and the kit of mankind PDGFRA gene D842V mutation
CN106636333A (en) * 2016-09-28 2017-05-10 广东凯普生物科技股份有限公司 PDGFRA gene mutation detection kit
CN107904290A (en) * 2017-11-09 2018-04-13 上海赛安生物医药科技股份有限公司 PDGFRA detection in gene mutation system and its kit
CN113943790A (en) * 2021-10-25 2022-01-18 北京华夏时代基因科技发展有限公司 Method for detecting ApoE single nucleotide polymorphism

Also Published As

Publication number Publication date
CN104830991B (en) 2018-04-27

Similar Documents

Publication Publication Date Title
CN104862402B (en) Detect primer, kit and its PCR method of ApoE gene pleiomorphisms
CN104894256A (en) Primers and kit for detecting acetaldehyde dehydrogenase 2 gene rs671 polymorphism site, and PCR (polymerase chain reaction) method thereof
JPH09512428A (en) Detection of mutations by resorbase cleavage
CN104962609B (en) Detect primer, kit and its PCR method of CYP2C9 and VKORC1 gene pleiomorphisms
CN105331733B (en) Polymorphic detection probe, amplification primers and its application of EGFR gene
CN104372093A (en) SNP (single-nucleotide polymorphism) detection method based on high-flux sequencing
CN104846106A (en) Primer and kit for detecting BRAF gene V600E mutation sites, and PCR method of kit
KR20110036646A (en) Method of detecting variation and kit to be used therein
CN104862401A (en) Primers for detecting hot-spot mutation sites of KRAS gene, kit and PCR (polymerase chain reaction) method for primers or kit
EP3607064A1 (en) Method and kit for targeted enrichment of nucleic acids
CN113614246A (en) Methods and compositions for identifying tumor models
JP2013081450A (en) Probe for detecting polymorphism, method of detecting polymorphism, method of evaluating efficacy of drug, and reagent kit for detecting polymorphism
CN105624296A (en) Universal fluorescent hairpin primers for detecting gene polymorphism on basis of ARMS (amplification refractory mutation system) fluorescent PCR (polymerase chain reaction) process
CN104830991A (en) Primer and kit for detecting PDGFRA (platelet-derived growth factor receptor alpha) gene D842V polymorphic sites and PCR (polymerase chain reaction) method of primer and kit
CN104818340A (en) Primers and kit for detecting JAK2 gene V617F site polymorphism, and PCR (polymerase chain reaction) method thereof
CN104830992A (en) Primer and kit for detecting methylenetetrahydrofolate reductase C677T polymorphic sites and PCR (polymerase chain reaction) method of primer and kit
CN105695614A (en) Method for identifying polymorphism of human breast cancer genes BRCA1 rs8176318 by aid of NsiI
CN104846108A (en) Primer, kit as well as PCR method for detecting of D816V mutation site of C-KIT gene
CN108251511A (en) The detection kit and detection method of a kind of EGFR genetic mutation
WO2018186947A1 (en) Method and kit for targeted enrichment of nucleic acids
CN105420349A (en) Method and kit for determining mutated nucleic acid bases
CN108913774A (en) C-KIT somatic mutation gene detection KIT and detection method thereof
CN104846107A (en) Primers and kit for detecting mutation of site M918T of RET gene and PCR (Polymerase Chain Reaction) method of primer and kit
JP4836710B2 (en) Method and kit for detecting microsatellite unstable cells
CN105695615A (en) Method for identifying polymorphism of human breast cancer genes RAD51 rs7180135 by aid of BccI

Legal Events

Date Code Title Description
C06 Publication
PB01 Publication
C10 Entry into substantive examination
SE01 Entry into force of request for substantive examination
GR01 Patent grant
GR01 Patent grant