CN1557964A - In-situ polymerase chain reaction approach for detecting target gene on chip - Google Patents
In-situ polymerase chain reaction approach for detecting target gene on chip Download PDFInfo
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- CN1557964A CN1557964A CNA200410016012XA CN200410016012A CN1557964A CN 1557964 A CN1557964 A CN 1557964A CN A200410016012X A CNA200410016012X A CN A200410016012XA CN 200410016012 A CN200410016012 A CN 200410016012A CN 1557964 A CN1557964 A CN 1557964A
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Abstract
The present invention is method of performing in-situ PCR reaction on the surface of gene chip to detect the gene to be detected. The upstream primer in common PCR reaction is connected to the arm structure of poly(T), modified 5'-terminal amino radical is connected to aldehyde modified glass slide or other carrier, and the in-situ PCR reaction is performed on the chip. The said method can solve the problems of probe breaking and effective hybridization, and can realize the synchronous processing and in-situ detection. The present invention may be used in SNP detection, transgenic plant detection, disease detection, etc.
Description
Technical field
The present invention relates to the method that kind of chip in-situ polymerization enzyme chain reaction detects target gene, is a kind of method that in-situ polymerization enzyme chain reaction (PCR) detects target gene of carrying out on the gene chip surface specifically.
Background technology
Gene chip is meant a large amount of gene probe molecules is fixed in solid support (as silicon chip, glass, plastics and nylon membrane etc.) on, hybridize with the sample of mark then, the reaction result fluorescent method, enzyme linked immunosorbent assay, isotope method detects, carry out data gathering with instruments such as scanners again, carry out data analysis with computer software at last, utilize this technology to be fixed in a large amount of gene probes on the upholder simultaneously, so once can carry out check and analysis, thereby solve traditional nucleic acid blot hybridization technique complicated operation to a large amount of nucleic acid molecule, level of automation is low, the testing goal molecular amounts is few, the low deficiency that waits of efficient.At present, this technical applications mainly contains gene expression spectrum analysis, new gene discovery, transgenation and polymorphism analysis, genomic library mapping, medical diagnosis on disease and prediction, drug screening, gene sequencing etc.
Come the analyzing and testing sample with gene chip at present, all must increase and mark before testing sample and the chip hybridization, realize the reduction of the segmental length of testing gene and increase to be measured by increasing, the fragment length that generally is used for the gene chip detection is all about 200-300 base, and for the hybridization of big fragment and probe, owing to the existence of its secondary structure has influenced effective combination of itself and probe, thereby be a technical barrier of this detection means of gene chip to big segmental detection always.At present domestic have report to smash with machinery or non-limiting enzyme is cut and reduced segmental length, but these two kinds of method complicated operations, and, therefore all can not fundamentally solve detection problem to big fragment goal gene owing to be to interrupt at random so circulation ratio is bad to purpose is segmental.The method (application number 01133630.7) that proofreading PCR detects transgenation on a kind of solid phase carrier of inventions such as domestic Zhang Xianen proposes to utilize a pair of outer primer and inner primer that testing gene is carried out solid phase PCR and detects, and is to be template with clinical sample or with the primer extension product.Directly be template, correspondingly in solid phase PCR reaction have the problem that inner primer and outer primer vie each other and influenced the amplification efficiency of PCR with the clinical sample; Amplified production with outer primer is that template is being carried out solid phase PCR reaction then, has in fact still needed the preceding pre-amplification of sample hybridization, therefore neither a kind of very good detection method.And adopting hydrosulphonyl silane modification slide, commercial this slide is very few, has brought difficulty for the application of this method.
Summary of the invention
The present invention has proposed a kind of new detection method-chip original position PCR method with regard to the hybridization of big fragment and nucleic acid probe in the gene chip target gene has been detected, thereby the processing of sample, the synchronization and the in situ detection of mark have been realized, not only having saved amplification, the mark of sample before gene chip detects in the past but also solved the hybridization problem of big fragment testing gene sample and probe, is a kind of breakthrough in the gene chip hybridization technology.
The present invention adopts following technological line: design a pair of Auele Specific Primer according to target gene, 5 ' end of upstream primer is connected with long poly thymus pyrimidine (polyT) structure of 15-20 base, 5 ' end of this upstream primer is put on aldehyde group modified slide after amido modified again, genomic deoxyribonucleic acid (DNA) with testing sample is a template then, on chip, carry out original position PCR reaction, utilize the specificity of archaeal dna polymerase to realize to the segmental amplification of specific purpose, the dUTP that in the primer extension process, adds digoxigenin labeled, adopt traditional enzyme mark technology that extension products is detected subsequently, make detected result be presented in nylon membrane or nitrocellulose membrane surface by substrate colors, detected result can directly be estimated or with cheap optical scanner reading of data.Utilize present method can realize synchronous detection to multidigit point also can being used for detection to a plurality of SNP site.
Experimentation of the present invention is as follows:
Design of primers: follow annealing temperature (Tm value) principle about equally of each primer, with PrimerPremier5.0 software design primer, each testing gene designs a pair of primer.The preparation of chip: upstream primer 5 ' end is amido modified and be connected with the arm configuration of the poly (T) that 15-20 base grow, by Cartesian microarray manufacturing system dot matrix in aldehyde group modified wave carrier piece (purchasing) surface in genome company, fixing 48-72h under the room temperature.
Original position PCR reaction on the chip: preparation PCR reaction mixture, in mixed solution, add digoxigenin labeled-dUTP, mixed solution drips on the chip square formation, and cover plate (coverwell) mounting with department of Sigma company produces places PCR instrument internal reaction then.
After the wash-out of chip and colour developing: PCR finishes, shake flush away with washing lotion and remove free composition and non-specific hybridization molecule, then and anti digoxin antibody (anti-digoxigenin-AP) reaction, drip colour developing liquid (NBT/BCIP Stock Solution) and epiphragma it is developed the color on film.
Description of drawings
Fig. 1: the present invention-chip original position PCR detects the schematic diagram of target gene method
(1) behind the adding target gene, fixed Auele Specific Primer probe carries out hybridization on target gene and the chip;
(2) target gene and specific probe can complementary pairing just can carry out extension and are detected, and and the unmatched target gene of probe just can not extend thereby no signal appearance.
Fig. 2: with the inventive method plasmid pCAMBIA1301 is detected, to the figure as a result of its contained GUS, 35S, hptII, aadA gene test.Site the 2, the 4th, negative control, site 1,3,5,6 corresponds respectively to GUS, 35S promoter, hpt, aadA gene, and site 7 is positive controls.
Concrete embodiment
Utilize method provided by the invention to inquire into detection, 4 gene GUS, 35S promoter, hpt, aadA that contain in the plasmid have been made preliminary detection plasmid vector pCAMBIA1301 commonly used in the transgenic plant.The chip method of in situ PCR of utilization, the amplification and the markers step of the sample before traditional die detects have been reduced, can realize detection a step to 4 genes among the plasmid pCAMBIA1301, on detection time, shorten greatly, overcome the loaded down with trivial details of multistep PCR again, for biochip detecting of transgenic paddy rice and transgenic plant proposed a kind of feasibility method later comprehensively.The concrete step that detects is:
1, design of primers
At the conserved sequence of the normal 35S promoter that occurs, reporter gene hpt, aadA, gus gene in transgenic paddy rice, follow the roughly the same principle of annealing temperature (Tm value) of each primer, use
Primer Premier5.0 software design primer, sequence is as follows
| The primer title | Upstream primer | Downstream primer | Product length |
| ?GUS | ?5′-poly(T) 16GGT?CAG?TGG?CAG?TGA ?AGG?G-3′Tm=58.1 | ?5′-AGC?GTC?GCAGAA?CATTAC?AT-3′ ?Tm=55.8 | ?539bp |
| ?35S | ?5′-poly(T) 16TGG?AAA?AGG?AAG?GTG ?GCT?C-3′Tm=57.3 | ?5′-ATA?GTG?GGA?TTG?TGC?GTC ?AT-3′Tm=55 | ?209bp |
| ?HptII | ?5′-poly(T) 16GAT?GTT?GGC?GAC?CTC ?GTA?TT-3′Tm=57.5 | ?5′-TCG?TTA?TGT?TTA?TCG?GCA?CTT ?T-3′Tm=57.4 | ?517bp |
| ?AadA | ?5′-poly(T) 16GTT?GCT?GTC?TCC?CAG ?GTC?GG-3′Tm=62.5 | ?5′-CCT?TTG?CTC?GGA?AGA?GTA?TGA ?A-3′Tm=59.1 | ?298bp |
2, the preparation of chip
Upstream primer 5 ' end is amido modified and be connected with the arm configuration of the long poly (T) of 16 bases, with upstream primer deionized water dissolving (light absorption value 2O.D+40ulH2O), and mix with point sample damping fluid (2 * point sample damping fluid spotting solution of ArrayIt company) equal-volume, by Cartesian microarray manufacturing system dot matrix in aldehyde group modified wave carrier piece surface, fixing 72h under the room temperature.
3, the reaction of the original position PCR on the chip
The pcr amplification system is as follows
Every part of consumption of reagent
10 * damping fluid 1.5ul
dNTP(5∶2)(2.5mM)??????????????1.2ul
dig-dUTP???????????????????????0.5ul
Template (15ng/ul) 1.5ul
Primer (reverse, 10pmol/ul) 1ul * 4
Taq enzyme (1U/ul) 1ul
H
2O???????????????????????????5.3ul
Cumulative volume 15ul
Getting PCR mixed solution 50ul drips on the chip square formation, use the coverwell mounting then, place and adopt following program to circulate on the PCR instrument: 94 ℃ of pre-sex change 4min, 94 ℃ sex change 1min-58 ℃ annealing is extended 30s for 1min-72 ℃, totally 10 circulations, last 72 ℃ are extended 5min.
4, the wash-out of chip and colour developing
After PCR finishes, removing coverwell is placed among the washing lotion I (0.1 * SSC 0.1%SDS) room temperature and shakes and wash 10-30 minute, washing lotion II (100mM maleic acid (maleic acid), 150mM NaClPH7.5,0.3% (v/v) Tween 20) shakes and washes 5 minutes, drip 15-20ul antibody after blotting washing lotion on square formation, the lucifuge room temperature reaction is 30 minutes after the covered.After washing lotion II, detect the damping fluid flushing, blot after, drip colour developing liquid and epiphragma it developed the color on film, room temperature lucifuge colour developing 30min-2h.
Claims (4)
1. a chip original position PCR detects the method for target gene, it is characterized in that designing a pair of Auele Specific Primer according to target gene, 5 ' end of upstream primer is connected with the long poly thymus pyrimidine structure of 15-20 base, 5 ' end of this upstream primer is put on aldehyde group modified slide after amido modified again, genomic deoxyribonucleic acid with testing sample is a template then, on chip, carry out original position PCR reaction, utilize the specificity of archaeal dna polymerase to realize to the segmental amplification of specific purpose, the dUTP that in the primer extension process, adds digoxigenin labeled, adopt traditional enzyme mark technology that extension products is detected subsequently, make detected result be presented in nylon membrane or nitrocellulose membrane surface by substrate colors, detected result can directly be estimated or with cheap optical scanner reading of data, thereby realizes the processing of sample, mark synchronization and in situ detection.
2. detect the method for target gene by the described a kind of chip original position PCR of claim 1, it is characterized in that comprising the steps:
(1) design of primers: follow the roughly the same principle of annealing temperature (Tm value) of each primer, with PrimerPremier5.0 software design primer, a target gene designs a pair of primer;
(2) preparation of chip: upstream primer 5 ' end is amido modified and be connected with the arm configuration of the polyT that 15-20 base grow, by Cartesian microarray manufacturing system dot matrix in aldehyde group modified wave carrier piece surface, fixing 48-72h under the room temperature;
(3) reaction of the original position PCR on the chip: PCR mixing drop is used the cover plate mounting on the chip square formation, place PCR instrument internal reaction then;
(4) after the wash-out of chip and colour developing: PCR finishes, shake flush away with washing lotion and remove free composition and non-specific hybridization molecule, with the anti digoxin antibody reaction, drip colour developing liquid and epiphragma it is developed the color on film then.
3. detect the method for target genes by claim 1 or 2 described a kind of chip original position PCR, the concrete steps that it is characterized in that being used for the detection of plasmid vector pCAMBIA1301 are:
(1) design of primers: follow the roughly the same principle of annealing temperature (Tm value) of each primer, with PrimerPremier5.0 software design primer, sequence is as follows
The primer title Upstream primer Downstream primer Product length
?GUS ?5′-poly(T)
16?GGT?CAG?TGG ?CAG?TGA?AGG?G-3′ ?Tm=58.1
?5′-AGC?GTC?GCA?GAA?CAT ?TAC?AT?-3′ ?Tm=55.8 ?539bp
?35S ?5′-poly(T)
16?TGG?AAA?AGG ?AAG?GTG?GCT?C-3′ ?Tm=57.3
?5′-ATA?GTG?GGA?TTG?TGC ?GTC?AT-3′ ?Tm=55 ?209bp
?HptII ?5′-poly(T)
16?GAT?GTT?GGC ?GAC?CTC?GTA?TT-3′ ?Tm=57.5
?5′-TCG?TTA?TGT?TTA?TCG ?GCA?CTT?T-3′ ?Tm=57.4 ?517bp
?AadA ?5′-poly(T)
16?GTT?GCT?GTC ?TCC?CAG?GTC?GG-3′ ?Tm=62.5
?5′-CCT?TTG?CTC?GGA?AGA ?GTA?TGA?A-3′ ?Tm=59.1 ?298bp
(2) preparation of chip: upstream primer 5 ' end is amido modified and be connected with the arm configuration of the long polyT of 16 bases, upstream primer is mixed with deionized water dissolving and with point sample damping fluid equal-volume, by Cartesian microarray manufacturing system dot matrix in aldehyde group modified wave carrier piece surface, fixing 72h under the room temperature;
(3) reaction of the original position PCR on the chip: the pcr amplification system is as follows
Every part of consumption of reagent
10 * damping fluid 1.5ul
dNTP(5∶2)(2.5mM)?????????????????1.2ul
dig-dUTP??????????????????????????0.5ul
Template (15ng/ul) 1.5ul
Primer (reverse, 10pmol/ul) 1ul * 4
Taq enzyme (1U/ul) 1ul
H
2O??????????????????????????????5.3ul
Cumulative volume 15ul
Getting PCR mixed solution 50ul drips on the chip square formation, use the coverwell mounting then, place and adopt following program to circulate on the PCR instrument: 94 ℃ of pre-sex change 4min, 94 ℃ sex change 1min-58 ℃ annealing is extended 30s for 1min-72 ℃, totally 10 circulations, last 72 ℃ are extended 5min;
(4) wash-out of chip and colour developing
After PCR finishes, removing coverwell is placed among 0.1 * SSC 0.1%SDS washing lotion I room temperature and shakes and wash 10-30 minute, 100mM maleic acid, 150mM NaCl PH7.5,0.3v/v%Tween20 washing lotion II shake and wash 5 minutes, drip 15-20ul antibody after blotting washing lotion on square formation, the lucifuge room temperature reaction is 30 minutes after the covered; After washing lotion II, detect the damping fluid flushing, blot after, drip colour developing liquid and epiphragma it developed the color on film, room temperature lucifuge colour developing 30min-2h.
4. detect the method for target gene by the described a kind of chip original position PCR of claim 3, it is characterized in that described upstream primer deionized water dissolved light absorption value 2O.D+40ulH2O.
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Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN101638690B (en) * | 2009-08-31 | 2013-03-27 | 浙江省检验检疫科学技术研究院 | Polymerase chain reaction (PCR) chip method for detecting transgenic components |
| CN103931199A (en) * | 2011-11-14 | 2014-07-16 | 苹果公司 | Generation of multi -views media clips |
| CN113846159A (en) * | 2021-01-27 | 2021-12-28 | 北京百奥纳芯生物科技有限公司 | Special chip for detecting expression of breast cancer related gene |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN101392286B (en) * | 2007-11-19 | 2011-08-10 | 中国科学院上海微系统与信息技术研究所 | Method for directly detecting P53 gene mutation in lung cancer sample based on nano probe |
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Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN101638690B (en) * | 2009-08-31 | 2013-03-27 | 浙江省检验检疫科学技术研究院 | Polymerase chain reaction (PCR) chip method for detecting transgenic components |
| CN103931199A (en) * | 2011-11-14 | 2014-07-16 | 苹果公司 | Generation of multi -views media clips |
| CN113846159A (en) * | 2021-01-27 | 2021-12-28 | 北京百奥纳芯生物科技有限公司 | Special chip for detecting expression of breast cancer related gene |
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