CN105274211A - Method and kit for determination of human NEFM gene polymorphism rs12515 site polymorphism - Google Patents
Method and kit for determination of human NEFM gene polymorphism rs12515 site polymorphism Download PDFInfo
- Publication number
- CN105274211A CN105274211A CN201510615157.XA CN201510615157A CN105274211A CN 105274211 A CN105274211 A CN 105274211A CN 201510615157 A CN201510615157 A CN 201510615157A CN 105274211 A CN105274211 A CN 105274211A
- Authority
- CN
- China
- Prior art keywords
- fragment
- amplified production
- cut
- site
- upstream primer
- 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.)
- Pending
Links
Classifications
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Q—MEASURING 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
- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
- C12Q1/6844—Nucleic acid amplification reactions
- C12Q1/6858—Allele-specific amplification
Landscapes
- Chemical & Material Sciences (AREA)
- Life Sciences & Earth Sciences (AREA)
- Organic Chemistry (AREA)
- Engineering & Computer Science (AREA)
- Zoology (AREA)
- Wood Science & Technology (AREA)
- Proteomics, Peptides & Aminoacids (AREA)
- Health & Medical Sciences (AREA)
- Biophysics (AREA)
- Chemical Kinetics & Catalysis (AREA)
- Immunology (AREA)
- Microbiology (AREA)
- Molecular Biology (AREA)
- Analytical Chemistry (AREA)
- Physics & Mathematics (AREA)
- Biotechnology (AREA)
- Biochemistry (AREA)
- Bioinformatics & Cheminformatics (AREA)
- General Engineering & Computer Science (AREA)
- General Health & Medical Sciences (AREA)
- Genetics & Genomics (AREA)
- Measuring Or Testing Involving Enzymes Or Micro-Organisms (AREA)
Abstract
The invention discloses a method and a kit for determination of human NEFM gene polymorphism rs12515 site polymorphism. The method is as follows: providing to-be-tested human genomic DNA; providing upstream and downstream primers for amplification of sequences nearby human NEFM gene polymorphism rs12515 site, wherein the upstream primer has a mismatched base T; taking the to-be-tested human genomic DNA as a template, using the upstream and downstream primers for PCR amplification reaction to obtain an amplification product containing ATTAAY fragment, wherein Y is to be confirmed base C or T on the human NEFM gene polymorphism rs12515 site; providing a restriction endonuclease; using the restriction endonuclease for enzyme digestion of the amplification product to obtain a corresponding enzyme digestion product; and according to the resulting enzyme digestion product, determining whether the to be confirmed base Y on the human NEFM gene polymorphism rs12515 site is C or T. The restriction endonuclease is restriction endonuclease which only be capable of cutting one of ATTAAT fragment or ATTAAC fragment. The determination method is fast and reliable, and can greatly reduce the determination cost.
Description
Technical field
The present invention relates to the method measuring single nucleotide polymorphism.
Background technology
SNP (single nucleotide polymorphism) refers to and comprises the forms such as the displacement of single base, insertion and disappearance by the mutant dna sequence that the change of single core thuja acid causes.Gene pleiomorphism is individual inherent hereditary feature, does not change with environment, neither the special or non-specific clinical manifestation of certain disease, and therefore its application does not exist Diagnosis and Treat effect.
Genetic polymorphism detection is widely used in genetic arts and medical field, is exemplified below: 1. study the genetics such as the origin of species and evolution phenomenon.According to genovariation situation, obtain the information of biomacromolecule, infer organic evolution history, illustrate spore relation.Be applied in archeology to determine the sibship of ancient human's heritable variation feature and different population.2. research polymorphic with population genetics etc. genetics research.Polymorphic also closely related with various characteristics of human body, comprise height, body weight, the colour of skin, Facial Features etc.3. may be used for prophylaxis in preventive medicine field.By the tolerance of researching human body to poisonous substance, find to be easy to, to the individuality of certain poisonous substance generation toxic action, avoid this individuality and toxicant exposure in time, protect this Susceptible population.Such as, carry out polymorphic detection to the crowd preparing to be engaged in the organic solvents such as Contact benzene, examination goes out easily to occur the individuality that hematotoxicity, neurotoxicity etc. are reacted, and makes it away from organic solvents such as benzene, protects this type of Susceptible population to encroach on from poisonous substance.4. may be used for medicament selection in pharmacology and dosage is determined.Can judge that diseased individuals is responsive to certain poisonous side effect of medicine by polymorphic detection, thus avoid using this kind of medicine to exempt its toxic action.By judging the individual level of response determination drug dose to effect of drugs, reduce drug dose and side effect thereof.
Neurofilaments (Neurofilaments, NFS) is cytoskeletal elements main in eukaryotic cells, is mainly present in neurone.It can be divided into three kinds of subunits by molecular weight difference, namely molecular weight is the lower molecular weight neurofilaments (Neurofilment of 68kd, lightpolypeptide, NEFL), median size molecular weight neurofilaments (Neurofilament, the mediumpolypeptide of 150kd size, NEFM), with the high molecular neurofilament (Neurofilament, heavypolypeptid, NEFH) of 200kd.Often kind of subunit is all individual gene product, plays important effect in cytoskeleton.
Middle-molecular-weihydroxyethyl neurofilaments gene is also called chain gene in neurofilaments, is the more a kind of cytoskeleton gene of Recent study, is positioned chromosome 8p 21, has 4 exons.There are some researches show that NEFM gene pleiomorphism may be relevant with the protein function of its coding.NEFM gene rs12515 site is positioned at UTR-3 region, there are some researches show this polymorphic function that may affect NEFM.
NEFM gene rs12515 site is polymorphic, two kinds of allele C and T is there is in crowd, form the genotype of three kinds of NEFM genes: CC type (two allelotrope bases of human genome rs12515 polymorphic site are C), CT type (two allelotrope bases of human genome rs12515 polymorphic site are respectively C and T) and TT type (two allelotrope bases of human genome rs12515 polymorphic site are T).
Polymerase chain reaction-restriction fragment length polymorphic (PCR-RFLP) technology is a kind of quick, easy, accurate, low cost mensuration SNP (single nucleotide polymorphism) genotypic classical way.The method carries out amplified reaction by primer to template, forms sufficient amount and stable amplified production, by cutting and detect the fragment length of digestion products to the enzyme of amplified production, finally determines SNP.So far, not yet find that there is restriction enzyme and can identify base sequence containing NEFM gene rs12515 polymorphic site, PCR-RFLP technology can not be taked to detect.Therefore need to develop new detection technique.
Summary of the invention
The object of this invention is to provide the reliable means of the mensuration people NEFM gene rs12515 loci polymorphism of the diagnosis of a kind of non-diseases or therapeutic purpose.
According to a first aspect of the invention, provide a kind of method measuring people NEFM gene rs12515 loci polymorphism, comprising:
Human gene group DNA to be measured is provided;
There is provided upstream primer and the downstream primer of amplification people NEFM gene rs12515 location proximate sequence, wherein upstream primer has base mismatch T;
With described human gene group DNA to be measured for template, utilize upstream primer and downstream primer to carry out pcr amplification reaction to obtain containing ATTAAY fragment, wherein Y is base C undetermined on people NEFM gene rs12515 site or T;
Restriction enzyme is provided;
Utilize restriction enzyme to carry out enzyme to gained amplified production and cut (reaction) to obtain corresponding digestion products; And
Determine that the base Y undetermined on people NEFM gene rs12515 site is C or T according to gained digestion products, wherein, restriction enzyme is the restriction enzyme that only can cut one of ATTAAT fragment and ATTAAC fragment.
According to embodiments of the invention, on gained amplified production, two base AA of being separated by between base mismatch T and the Y of upstream primer.Surprisingly, so arrange base mismatch endonuclease reaction will be made to carry out extremely smooth, there will not be enzyme to cut the phenomenons such as insufficient.Further, so arrange upstream primer base mismatch and PCR reaction is well on, improve sensitivity and the specific degree of PCR, this may be relevant with making the secondary structural change of extension increasing sequence after base mismatch.
In an alternate embodiment of the present invention where, on gained amplified production, upstream primer terminal bases is adjacent with Y.
In a preferred embodiment of the invention, on gained amplified production, upstream primer terminal bases is not adjacent with Y.Such as, upstream primer end can be ... TA structure.Be difficult to the imagination, the upstream primer with this design can promote endonuclease reaction unexpectedly further greatly, and this may have certain to associate with amplification bonding force.
In a preferred embodiment of the invention, restriction enzyme can adopt the AseI or its isoschizomers that only can cut ATTAAT fragment.This fermentoid is cheap, greatly can reduce cost of determination.
According to embodiments of the invention, gained digestion products comprises three kinds of clip types: have total fragment length do not cut off amplified production, cut off after have compared with the amplified production of long segment and after cutting off, there is amplified production (comparatively short-movie section can not effectively observe usually) compared with short-movie section.The clip types comprised by observation (judgement) digestion products determines that the base undetermined on people NEFM gene rs12515 site is C or T.Such as, when adopting AseI enzyme, judge compared with the observations of these two fragments of long segment according to total fragment with after cutting off: if observe digestion products only have a kind of there is total fragment length do not cut off amplified production, then base undetermined is C; Only have one to have the cut-out product of comparatively long segment (being less than total fragment length) if observe digestion products, then base undetermined is T; If observe said two devices, then base undetermined not only comprises C but also comprise T.
In one embodiment of the invention, the clip types that judgement (or observation) digestion products comprises is schemed to contrast to carry out with reference after being taken pictures by gel electrophoresis associating ultraviolet lamp.In this case, preferably reference figure is that amplified production obtains and only has first with reference to picture position and second with reference to picture position after the gel electrophoresis standard setting time after ultraviolet lamp is taken pictures, wherein first with reference to picture position for be the amplified production of the total fragment length do not cut off, second with reference to picture position then for be cut off after there is amplified production compared with long segment.Such as, the present invention adopt with reference to figure be by 151bp and 116bp synthesized two base fragments simultaneously after gel electrophoresis same time ultraviolet lamp take pictures and form.Compared with the compound reference figure of conventional DNAladder, owing to have employed, only there are two specific reference figure with reference to picture position, this method of the present invention intuitively can be observed rapidly or judge the clip types that digestion products comprises, and avoids erroneous judgement to greatest extent simultaneously.Preferably carry out electrophoresis by after concentrated for digestion products 1 ~ 2 times of concentration after endonuclease reaction, increase brightness of image, improve judgment accuracy.
In a preferred embodiment of the invention, make total fragment length of amplified production between 100 to 300bp by designing the length of upstream primer and downstream primer, and the fragment length of upstream primer is at least 35bp, preferred length 40 ~ 60bp (amplified reaction especially smoothly fully between this dominant area), makes enzyme fall Partial Fragment length earnestly and accounts for the per-cent of total fragment length more than 20%.This design of the present invention has the electrophoresis ultraviolet photo of the amplified production compared with long segment position after can making to have not cutting off amplified production and cutting off of total fragment length is distinguished significantly.But if total fragment is long, then electrophoretic mobility shift is by not obvious; Too short, image can thicken a slice, cannot accurately distinguish.The fragment length scope of upstream primer ensure that pcr amplification reaction can carry out smoothly, the amplification that there will be when avoiding base mismatch not foot phenomenon.
In a preferred embodiment of the invention, by controlling the scope of annealing temperature in pcr amplification program between 55 ~ 70 DEG C, preferable temperature 60 ~ 69 DEG C (this temperature can improve the specificity of amplified reaction), make the PCR primer purity of design higher.This design of the present invention can make pcr amplification product band clear, occurs, be easy to electrophoresis identification without assorted band.But if temperature is too low, then few the and assorted band of specific band is too much, is difficult to after electrophoresis distinguish and judges; If temperature is too high, then affects pcr amplification efficiency and make specific amplified production very few, affect observing effect.
In a preferred embodiment of the invention, by controlling to extend the scope of time between 10 ~ 60s in pcr amplification program, preferred time 15 ~ 30s (this time can improve the efficiency of amplified reaction and the specificity of amplified production), make the PCR reaction times of design shorter, amplified production purity is higher.This design of the present invention can make pcr amplification product band clear, occurs, be easy to electrophoresis identification, and the PCR time is shorter without assorted band.But if the time is too short, then specific band can not increase completely and make amplified production less, be difficult to after electrophoresis distinguish judgement; If overlong time, then increase the occurrence probability of non-specific band, occur that assorted band affects observing effect.
In the present invention, PCR reacted constituent can comprise DNA profiling, upstream and downstream primer, TaqDNApolymerase (archaeal dna polymerase or also can be called " Taq enzyme "), damping fluid, Mg
2+deng.In a preferred embodiment of the invention, TaqDNApolymerase and TaqAntibody can be used in pcr amplification reaction.TaqAntibody is the monoclonal antibody of TaqDNApolymerase, it suppresses DNA polymerase activity after being combined with TaqDNApolymerase, both avidity is very high, even if the activity of TaqDNApolymerase still can be closed at 65 DEG C, the non-specific amplification that therefore can effectively suppress the non-specific annealing of primer and primer dimer to cause, has high amplification sensitivity and specificity.TaqAntibody only needs to get final product complete deactivation at 95 DEG C of heating 30s, and release TaqDNApolymerase is active, ensure that subsequent PCR amplification reaction can be carried out smoothly.
The Tris-HCl damping fluid that pH value is 8.1 ~ 8.7 can be added in PCR reaction, adjust PCR solution ph when 72 DEG C of extensions between 6.8 ~ 7.8, thus make Taq enzyme play activity better in slight alkali environment.In addition, gelatin (0.01%) can also be added in PCR solution to reduce the adsorption of PCR pipe to Taq enzyme, stabilized enzyme activity and provide protection, promote PCR reaction.
In addition, Mg in PCR solution
2+when concentration is between 1.5 ~ 2.0mmol/L, can well control PCR react productive rate and specificity.
The final concentration that PCR reacts primer is generally about 0.1 ~ 1 μM, and the too high meeting of concentration causes non-specific amplification, and too low then amplified production very little.
In addition, can also add solubility promoter methyl-sulphoxide (DMSO) and ammonium sulfate to reduce base mispairing level in PCR reaction, the amplification efficiency of GC template is rich in raising.This with the secondary structure eliminating primer and template, may reduce DNA melting temperature(Tm) and makes DNA sex change completely relevant.
According to a further aspect in the invention, provide a kind of test kit for measuring people NEFM gene rs12515 loci polymorphism, it comprises:
For upstream primer and the downstream primer of pcr amplification people NEFM gene rs12515 location proximate sequence, wherein upstream primer has base mismatch T to obtain containing the amplified production of ATTAAY fragment, and wherein Y is base C undetermined on people NEFM gene rs12515 site or T; And
Only can cut the restriction enzyme of one of ATTAAT fragment and ATTAAC fragment.
Can also comprise other composition in mentioned reagent box, such as PCR reacts Mix and (comprises 4 kinds of dNTP mixtures, Mg
2+, TaqDNApolymerase, TaqAntibody, damping fluid, DMSO and ammonium sulfate) and for implement measure specification sheets etc.
It will be understood by those skilled in the art that unless there are obvious conflict, the correlated characteristic of a first aspect of the present invention and second aspect can combine mutually.
Mensuration means of the present invention are not only fast and reliable, and cost of determination reduces greatly.
Accompanying drawing explanation
Fig. 1 describes the digestion products electrophoresis ultraviolet photo that method according to the present invention obtains.Wherein Marker is: standard reference position; Swimming lane 1:CC genotype; Swimming lane 2:TC genotype; Swimming lane 3:TT genotype.
Embodiment
Describe the present invention below.It will be appreciated by those skilled in the art that following detailed description only for illustration of and non-limiting the present invention.
(1) acquisition of DNA to be measured
Gather different crowd peripheral blood, after extracting genomic dna, carry out the mensuration of NEFM gene rs12515 loci polymorphism below.
For the selection of DNA to be measured, the not special restriction of the present invention.Both can be obtain in vitro sample from the body fluid of human body or tissue, the genome of degradation treatment in advance can also be through.For convenience of implementation, usually preferably in vitro sample is extracted from blood.Wherein said tissue comprises the tissue containing all or at least NEFM gene in human body, and with whether express this NEFM gene and have nothing to do.The method extracting DNA from body fluid and/or tissue well known to a person skilled in the art, and can with reference to conventional molecular biology manual, such as " practical flow cytometry icones ", " molecular cloning " the 2nd edition etc.
(2) design of primers and synthesis
Search Gene database and the snp database of NCBI website, obtain NEFM gene complete sequence and rs12515 polymorphic site information respectively.Rs12515 polymorphic site y front and rear part base sequence (base sequence represents with 5' → 3', capital and small letter same meaning) following (SEQIDNO:1):
Upstream primer and the downstream primer of base mismatch is introduced according to above-mentioned sequences Design.On final gained amplified production, two base AA of being separated by between base mismatch T and the Y of upstream primer.
In the present invention, upstream primer has base mismatch T, and length is 35 ~ 60bp.Primer in one of them embodiment is as follows:
Upstream primer: 5'GTATTATGCAAAGTACCAACTGAGCCAAAAACAAT
taA3'(SEQIDNO:2),
Downstream primer: 5'ACTGTGCATGTCAACGAGGTTCTCCCA3'(SEQIDNO:3), wherein upstream primer underscore base is base mismatch.
(3) pcr amplification product is prepared
Formulate pcr amplification program and condition according to upstream primer and downstream primer feature and PCR corresponding reagent, prepare pcr amplification product.In one of them embodiment, get genomic dna (50 ~ 80ng), upstream and downstream primer (final concentration is 0.1 ~ 1 μM), 2 × PCRMix7.5 μ L (comprise 4 kinds of dNTP mixtures, Mg
2+, TaqDNApolymerase, TaqAntibody, damping fluid, DMSO and ammonium sulfate) and distilled water jointly form 15 μ L reaction systems, adjustment pH value of solution be about 7.3.PCR reaction conditions is: 95 DEG C of denaturation 30s, and DEG C annealing 30s → 72 DEG C, 95 DEG C of sex change 30s → 61 extend 20s totally 30 circulations, and 72 DEG C extend 7min.Stable amplified production is obtained after PCR reaction.
(4) endonuclease reaction
The present invention adopts the price of restriction endonuclease AseI very cheap, as shown in table 1.
Table 1NEB company AseI endonuclease recognition sequence and price thereof
In one of them embodiment, get PCR primer 10 μ L, add the restriction enzyme A seI5U, 2 μ L10 × enzyme cutting buffering liquids and the 7.5 μ L distilled waters that identify ATTAAT sequence and form 20 μ L reaction systems, in 37 water-baths, enzyme cuts 4 ~ 12h, obtain digestion products, digestion products is observed through 1 times of concentrated rear electrophoresis.
(5) electrophoresis test
In one of them embodiment, if PCR primer can not be cut after AseI enzyme is cut, be still 151bp, if be cut open, occur that (cut generation sticky end due to AseI enzyme makes its complementary strand bases number different to 116bp with 35bp, therefore after cutting, fragment length is as the criterion with strand base number in gene order and calculates), be wherein difficult in 35bp fragment electrophoretic figure differentiate.
By digestion products in 2 ~ 4% sepharoses under 3 ~ 8V/cm condition, electrophoresis 30 ~ 80min, mensuration of taking pictures under ultraviolet lamp.Restriction enzyme digestion and electrophoresis figure is shown in Fig. 1, and the presence or absence according to 151bp and 116bp fragment judges genotype: CC type is 151bp fragment, and TC type has 151bp and 116bp two kinds of fragments, and TT type is 116bp fragment.
Here implements some embodiments of the present invention.
Embodiment 1 is extracted human peripheral leucocytes DNA and is measured rs12515 polymorphism
1 materials and methods
1.1 main agents and instrument
Reagent: 2 × PCRMix (comprises 4 kinds of dNTP mixtures, Mg
2+, TaqDNApolymerase, TaqAntibody, damping fluid, DMSO and ammonium sulfate), restriction enzyme A seI (NEB company), agarose (Biowest company), primer is synthesized by Shanghai Sangon company.
Instrument: 9600 type PCR instrument (PE company), miniature electrophoresis chamber (PharmaciaBiotech, EPS1000), GelDoc2000 gel imaging instrument (Bio-RAD company).
1.2 extract DNA as testing gene group DNA profiling from peripheral blood leucocyte
EDTA-K
2anticoagulant tube gathers human peripheral 1mL, white corpuscle separation is carried out with reference to leukocytic separation method in " practical flow cytometry icones ", white corpuscle genomic dna is extracted with reference to NaCl salting-out method in " molecular cloning ", and as human gene group DNA's template to be measured.1.3 sequences are searched and design of primers
NEFM gene order and rs12515 polymorphic site information is searched to design primer in NCBI website, specific as follows:
Upstream primer: 5'GTATTATGCAAAGTACCAACTGAGCCAAAAACAAT
taA3'(SEQIDNO:2),
Downstream primer: 5'AACTGTGCATGTCAACGAGGTTCTCCCA3'(SEQIDNO:3).1.4PCR amplification
Get genomic dna (50 ~ 80ng), upstream and downstream primer (final concentration is 0.1 ~ 1 μM), 2 × PCRMix7.5 μ L (comprise 4 kinds of dNTP mixtures, Mg
2+, TaqDNApolymerase, TaqAntibody, damping fluid, DMSO and ammonium sulfate), sterilizing distilled water supplies 15 μ L reaction systems, adjustment pH value of solution be about 7.3.
PCR reaction conditions is: 95 DEG C of denaturation 30s, and DEG C annealing 30s → 72 DEG C, 95 DEG C of sex change 30s → 61 extend 20s totally 30 circulations, and 72 DEG C extend 7min.Stable amplified production is obtained after PCR reaction.
1.5 enzymes cut qualification
Get PCR primer 10 μ L, add 5U restriction endonuclease AseI, 2 μ L10 × enzyme cutting buffering liquids and 7.5 μ L distilled waters and form 20 μ L reaction systems, in 37 DEG C of water-baths, enzyme cuts 12h, obtains digestion products, and digestion products is observed through 1 times of concentrated rear electrophoresis.
Above-mentioned digestion products under 3% sepharose 5V/cm condition, electrophoresis 35min, qualification Polymorphic type of taking pictures under ultraviolet lamp.
2 results
2.1PCR amplification
Sequence (it is arranged in SEQIDNO:1 base sequence 463-613 place, altogether 151bp) after amplification, the amplified production sequence obtained following (SEQIDNO:4):
In amplification after product sequence, underscore part is respectively the sequence corresponding to upstream, downstream primer, and y represents the polymorphic i.e. SNP site rs12515 of C/T.
2.2 enzymes cut result
Product Sequence after restriction endonuclease AseI enzyme is cut is as follows respectively:
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 116bp (this fragment downstream sequence forms sticky end because enzyme is cut and reduces by 2 bases than upstream sequence) sequence (SEQIDNO:5):
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 35bp (this fragment downstream sequence forms sticky end because enzyme is cut and increases by 2 bases than upstream sequence) sequence (SEQIDNO:6):
gtattatgcaaagtaccaactgagccaaaaacaat35
Take pictures under ultraviolet lamp after digestion products electrophoresis qualification, result is shown in Figure 1.Wherein, after the amplification of rs12515 site, there is 151bp segment, cut rear electrophoresis through AseI enzyme and there will be 151bp, 116bp and 35bp tri-kinds of segments (wherein 35bp not easily differentiates in electrophorogram).
Enzyme is cut rear genotype and is judged: as shown in Figure 1, CC type is 151bp fragment, and TC type has 151bp and 116bp two kinds of fragments, and TT type is 116bp fragment.
The polymorphic result in 2.3NEFM gene rs12515 site
Detect 20 routine personnel altogether, detected result finds that CC type 6 example, TC type 9 example and TT type 5 example appear in rs12515 site.
Embodiment 2 human peripheral whole blood sample measures NEFM gene rs12515 polymorphism
Main agents and instrument are with embodiment 1; Peripheral blood Whole Blood Genomic DNA is extracted with reference to phenol-chloroform extraction process in " molecule clone technology ", and as human gene group DNA's template to be measured.
Sequence searches same embodiment 1, PCR, and to react the upstream primer adopted be SEQIDNO:7, and downstream primer is SEQIDNO:8.
Upstream primer: 5'GAGATGTATTATGCAAAGTACCAACTGAGCCAAAACAAT
taA3'(SEQIDNO:7);
Downstream primer: 5'TTAACATCGATCAACATAAGATTGCAAACTGT3'(SEQIDNO:8).
Get genomic dna (50 ~ 80ng), upstream and downstream primer (final concentration is 0.1 ~ 1 μM), 2 × PCRMix10 μ L (comprise 4 kinds of dNTP mixtures, Mg
2+, TaqDNApolymerase, TaqAntibody, damping fluid, DMSO and ammonium sulfate), sterilizing distilled water supplies 20 μ L reaction systems, adjustment pH value of solution be about 7.3.
PCR reaction conditions is: 95 DEG C of denaturation 3min, and DEG C annealing 30s → 72 DEG C, 95 DEG C of sex change 30s → 63 extend 20s totally 30 circulations, and 72 DEG C extend 10min.
Endonuclease reaction is with embodiment 1.After digestion products is concentrated through 1 times under 3% sepharose 5V/cm condition, electrophoresis 45min, qualification of taking pictures under ultraviolet lamp.
Result:
Sequence (it is arranged in SEQIDNO:1 base sequence 458-639 place, altogether 182bp) after amplification, the amplified production sequence obtained following (SEQIDNO:9):
In amplification after product sequence underscore part be upstream, sequence corresponding to downstream primer, y represents the polymorphic i.e. SNP site rs12515 of C/T.
Product Sequence after restriction endonuclease AseI enzyme is cut is as follows respectively:
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 142bp (this fragment downstream sequence forms sticky end because enzyme is cut and reduces by 2 bases than upstream sequence) sequence (SEQIDNO:10):
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 40bp (this fragment downstream sequence forms sticky end because enzyme is cut and increases by 2 bases than upstream sequence) sequence (SEQIDNO:11):
gagatgtattatgcaaagtaccaactgagccaaaaacaat40
To take pictures under ultraviolet lamp after digestion products electrophoresis qualification, after the amplification of rs12515 site, occur 182bp segment, cut rear electrophoresis through AseI enzyme and there will be 182bp, 142bp and 40bp (wherein 40bp not easily differentiates in electrophorogram) three kinds of segments.
Enzyme is cut rear genotype and is judged: CC type is 182bp fragment, and TC type has 182bp and 142bp two kinds of fragments, and TT type is 142bp fragment.
Detect 25 routine personnel altogether, detected result finds that CC type 7 example, TC type 12 example and TT type 6 example appear in rs12515 site.
Embodiment 3 human peripheral blood clot sample measures NEFM gene rs12515 polymorphism
Main agents and instrument are with embodiment 1; Blood clot genomic dna is extracted with reference to phenol-chloroform extraction process in " molecule clone technology ".
It is SEQIDNO:12 that PCR reacts the upstream primer adopted, and downstream primer is SEQIDNO:13.
Upstream primer: 5'CTTGAGATGTATTATGCAAAGTACCAACTGAGCCAAAACAAT
ta3'(SEQIDNO:12);
Downstream primer: 5'GCAAGTACTGCTGTGACGTTTAACATCGAT3'
(SEQIDNO:13)
Pcr amplification is except annealing temperature is 65 DEG C, and remaining reaction condition is with embodiment 1; Endonuclease reaction is with embodiment 1.After digestion products is concentrated through 1 times under 2.5% sepharose 5V/cm condition, electrophoresis 45min, qualification of taking pictures under ultraviolet lamp.
Result:
Sequence (it is arranged in SEQIDNO:1 base sequence 455-658 place, altogether 204bp) after amplification, the amplified production sequence obtained following (SEQIDNO:14):
In amplification after product sequence underscore part be upstream, sequence corresponding to downstream primer, y represents the polymorphic i.e. SNP site rs12515 of C/T.
Product Sequence after restriction endonuclease AseI enzyme is cut is as follows respectively:
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 161bp (this fragment downstream sequence forms sticky end because enzyme is cut and reduces by 2 bases than upstream sequence) sequence (SEQIDNO:15):
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 43bp sequence (this fragment downstream sequence forms sticky end because enzyme is cut and increases by 2 bases than upstream sequence) (SEQIDNO:16):
cttgagatgtattatgcaaagtaccaactgagccaaaaacaat43
To take pictures under ultraviolet lamp after digestion products electrophoresis qualification, after the amplification of rs12515 site, occur 204bp segment, cut rear electrophoresis through AseI enzyme and there will be 204bp, 161bp and 43bp (wherein 43bp not easily differentiates in electrophorogram) three kinds of segments.
Enzyme is cut rear genotype and is judged: CC type is 204bp fragment, and TC type has 204bp and 161bp two kinds of fragments, and TT type is 161bp fragment.
Polymorphic result, detects 46 routine personnel altogether, and detected result finds that CC type 13 example, TC type 21 example and TT type 12 example appear in rs12515 site.
Embodiment 4 human oral mucosa cells measures NEFM gene rs12515 polymorphism
Main agents and instrument are with embodiment 1; Oral Mucosal Cells genomic dna is extracted with reference to phenol-chloroform extraction process in " molecule clone technology ".
It is SEQIDNO:17 that PCR reacts the upstream primer adopted, and downstream primer is SEQIDNO:18.
Upstream primer: 5'GGGATGTCTTGAGATGTATTATGCAAAGTACCAACTGAGCCAAAAACAAT
ta3'(SEQIDNO:17);
Downstream primer: 5'GACTATGTTTCCAATATGACCTTTATTGAGCAA3'
(SEQIDNO:18)
Pcr amplification is except annealing temperature is 68 DEG C, and remaining reaction condition is with embodiment 1; Endonuclease reaction is with embodiment 1.After digestion products is concentrated through 1 times under 2.5% sepharose 5V/cm condition, electrophoresis 45min, qualification of taking pictures under ultraviolet lamp.
Result:
Sequence (it is arranged in SEQIDNO:1 base sequence 448-687 place, altogether 240bp) after amplification, the amplified production sequence obtained following (SEQIDNO:19):
In amplification after product sequence underscore part be upstream, sequence corresponding to downstream primer, y represents the polymorphic i.e. SNP site rs12515 of C/T.
Product Sequence after restriction endonuclease AseI enzyme is cut is as follows respectively:
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 190bp (this fragment downstream sequence forms sticky end because enzyme is cut and reduces by 2 bases than upstream sequence) sequence (SEQIDNO:20):
When this polymorphic site contains T allelotrope, PCR primer enzyme can be formed after cutting and cut fragment 50bp (this fragment downstream sequence forms sticky end because enzyme is cut and increases by 2 bases than upstream sequence) sequence (SEQIDNO:21):
gggatgtcttgagatgtattatgcaaagtaccaactgagccaaaaacaat50
To take pictures under ultraviolet lamp after digestion products electrophoresis qualification, after the amplification of rs12515 site, occur 240bp segment, cut rear electrophoresis through AseI enzyme and there will be 240bp, 190bp and 50bp (wherein 50bp not easily differentiates in electrophorogram) three kinds of segments.
Enzyme is cut rear genotype and is judged: CC type is 240bp fragment, and TC type has 240bp and 190bp two kinds of fragments, and TT type is 50bp fragment.
Polymorphic result, detects 64 routine personnel altogether, and detected result finds that CC type 18 example, TC type 30 example and TT type 16 example appear in rs12515 site.
Claims (10)
1. measure a method for people NEFM gene rs12515 loci polymorphism, comprising:
Human gene group DNA to be measured is provided;
There is provided upstream primer and the downstream primer of amplification people NEFM gene rs12515 location proximate sequence, wherein upstream primer has base mismatch T;
With described human gene group DNA to be measured for template, utilize upstream primer and downstream primer to carry out pcr amplification reaction to obtain containing the amplified production of ATTAAY fragment, wherein Y is base C undetermined on people NEFM gene rs12515 site or T;
Restriction enzyme is provided;
Utilize restriction enzyme to carry out enzyme to gained amplified production to cut to obtain corresponding digestion products; And
Determine that the base Y undetermined on people NEFM gene rs12515 site is C or T according to gained digestion products,
Wherein, restriction enzyme is the restriction enzyme that only can cut one of ATTAAT fragment and ATTAAC fragment.
2. method according to claim 1, wherein on gained amplified production, two base AA of being separated by between base mismatch T and the Y of upstream primer.
3. method according to claim 2, wherein on gained amplified production, upstream primer terminal bases is adjacent with Y.
4. method according to claim 2, wherein on gained amplified production, upstream primer terminal bases is not adjacent with Y.
5. method according to claim 1, wherein restriction enzyme is AseI or its isoschizomers that only can cut ATTAAT fragment.
6. method according to claim 1, wherein gained digestion products comprises three kinds of clip types: have total fragment length do not cut off amplified production, cut off after have compared with the amplified production of long segment and after cutting off, there is amplified production compared with short-movie section, by judging that the clip types that digestion products comprises determines that the base Y undetermined on people NEFM gene rs12515 site is C or T.
7. method according to claim 6, wherein judge clip types that digestion products comprises taken pictures by gel electrophoresis associating ultraviolet lamp after with reference to scheming to contrast to carry out.
8. method according to claim 7, wherein reference figure is that amplified production obtains and only has first with reference to picture position and second with reference to picture position after the gel electrophoresis standard setting time after ultraviolet lamp is taken pictures, wherein first with reference to picture position for be the amplified production of the total fragment length do not cut off, second with reference to picture position then for be cut off after there is amplified production compared with long segment.
9. method according to claim 1, wherein make total fragment length of amplified production between 100 to 300bp by designing the length of upstream primer and downstream primer, and the fragment length of upstream primer is at least 35bp, makes enzyme fall Partial Fragment earnestly and account for the per-cent of the length of total fragment more than 20%.
10., for measuring a test kit for people NEFM gene rs12515 loci polymorphism, it comprises:
For upstream primer and the downstream primer of pcr amplification people NEFM gene rs12515 location proximate sequence, wherein upstream primer has base mismatch T to obtain containing the amplified production of ATTAAY fragment, and wherein Y is base C undetermined on people NEFM gene rs12515 site or T; And
Only can cut the restriction enzyme of one of ATTAAT fragment and ATTAAC segments-segment.
Priority Applications (1)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
CN201510615157.XA CN105274211A (en) | 2015-09-24 | 2015-09-24 | Method and kit for determination of human NEFM gene polymorphism rs12515 site polymorphism |
Applications Claiming Priority (1)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
CN201510615157.XA CN105274211A (en) | 2015-09-24 | 2015-09-24 | Method and kit for determination of human NEFM gene polymorphism rs12515 site polymorphism |
Publications (1)
Publication Number | Publication Date |
---|---|
CN105274211A true CN105274211A (en) | 2016-01-27 |
Family
ID=55144038
Family Applications (1)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
CN201510615157.XA Pending CN105274211A (en) | 2015-09-24 | 2015-09-24 | Method and kit for determination of human NEFM gene polymorphism rs12515 site polymorphism |
Country Status (1)
Country | Link |
---|---|
CN (1) | CN105274211A (en) |
Citations (1)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
CN101570778A (en) * | 2008-05-01 | 2009-11-04 | 夏昭林 | Method and kit for detecting polymorphism of ADPRT gene |
-
2015
- 2015-09-24 CN CN201510615157.XA patent/CN105274211A/en active Pending
Patent Citations (1)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
CN101570778A (en) * | 2008-05-01 | 2009-11-04 | 夏昭林 | Method and kit for detecting polymorphism of ADPRT gene |
Non-Patent Citations (2)
Title |
---|
E HOFSLI等: ""Identification of novel neuroendocrine-specific tumour genes",第1330–1339页", 《BRITISH JOURNAL OF CANCER》 * |
未知: ""rs12515 ss14793"", 《NCBI DBSNP》 * |
Similar Documents
Publication | Publication Date | Title |
---|---|---|
CN105274212A (en) | Method and kit for determination of human POT1 gene rs1034794 site polymorphism | |
CN105274204A (en) | Method and kit for determination of human PLIN1 gene rs894160 site polymorphism | |
KR101676912B1 (en) | PNA probe set for identifying ginseng cultivars and method for identifying ginseng cultivars using the same | |
CN100415884C (en) | DNA molecular marking method for researching fish genetic relation | |
CN105274213A (en) | Method and kit for determination of human PLIN1 gene rs894160 site polymorphism | |
CN105256008A (en) | Method and kit used for determining human PON1 gene rs662 site polymorphism | |
CN101638683A (en) | Dual-PCR method for detecting tomato TY-1 gene and Mi gene at the same time | |
CN105331682A (en) | Human PON1 gene rs854560 site polymorphism detection method and kit | |
CN105256006A (en) | Method and kit used for determining human TERF1 gene rs201882345 site polymorphism | |
CN105274215A (en) | Method and kit for determining rs854560 site polymorphism of PON1 gene | |
CN105274211A (en) | Method and kit for determination of human NEFM gene polymorphism rs12515 site polymorphism | |
CN105316406A (en) | Method and kit for measuring human NEFM gene rs12515 site polymorphism | |
CN105274203A (en) | Method and kit for determination of human NEFL gene rs1059111 site polymorphism | |
CN104120124B (en) | SCAR marker for specifically detecting wheat stripe rust and detection method | |
CN105274216A (en) | Method and kit for determining rs2979704 site polymorphism of human NEFL gene | |
CN105256012A (en) | Method and kit used for determining human NEFL gene rs1059111 site polymorphism | |
CN105274217A (en) | Method and kit for determining rs3093816 site polymorphism of human CCNH gene | |
CN105087818A (en) | Method and kit for determining POT1 gene rs1034794 locus polymorphism | |
CN105274208A (en) | Technology for determination of human PLIN1 gene rs2289487 site polymorphism | |
CN105274207A (en) | Method and kit for determination of human CDKN1B gene rs34329 site polymorphism | |
CN105274210A (en) | Method and kit for determination of human PLIN1 gene rs2289487site polymorphism | |
CN105755166A (en) | GBA gene L444P mutation detection kit | |
CN105296612A (en) | Method and kit for determining polymorphism of human TERT gene rs4975605 site | |
CN105274206A (en) | Method and kit for determination of human TERT gene rs2853669 site polymorphism | |
CN105274209A (en) | Method and kit for determination of human TERF1 gene rs3863242 site polymorphism |
Legal Events
Date | Code | Title | Description |
---|---|---|---|
C06 | Publication | ||
PB01 | Publication | ||
C10 | Entry into substantive examination | ||
SE01 | Entry into force of request for substantive examination | ||
RJ01 | Rejection of invention patent application after publication | ||
RJ01 | Rejection of invention patent application after publication |
Application publication date: 20160127 |