CN102605095A - PCR (polymerase chain reaction) kit for rapidly detecting reindeer-derived deer product and preparation method thereof - Google Patents
PCR (polymerase chain reaction) kit for rapidly detecting reindeer-derived deer product and preparation method thereof Download PDFInfo
- Publication number
- CN102605095A CN102605095A CN2012101085582A CN201210108558A CN102605095A CN 102605095 A CN102605095 A CN 102605095A CN 2012101085582 A CN2012101085582 A CN 2012101085582A CN 201210108558 A CN201210108558 A CN 201210108558A CN 102605095 A CN102605095 A CN 102605095A
- Authority
- CN
- China
- Prior art keywords
- primer
- pcr
- deer
- reinder
- pcr reaction
- 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
Images
Landscapes
- Measuring Or Testing Involving Enzymes Or Micro-Organisms (AREA)
Abstract
The invention provides a PCR (polymerase chain reaction) kit for rapidly detecting a reindeer-derived deer product and a preparation method thereof. According to the invention, the specific molecular fragment of mitochondrial DNA of a reindeer is amplified by adopting a PCR technology, so that the kit is prepared and used for detecting whether a detected sample contains reindeer composition or not and detecting a mixed sample. The kit and the preparation method have the characteristics that operation is simple, sensitivity is high, speed is rapid, and the like.
Description
Technical field:
The present invention discloses the PCR test kit of a kind of rapid detection reinder source property deer product, particularly detects the composition that whether contains the reinder product in the deer product.Be used for quick and precisely discerning the deer product, belong to the biological detection reagent kit technical field.
Background technology:
The deer product is some tissue or organs of deer, mainly includes: pilose antler, the deer heart, deer kidney, deer tire, deer's sinew, deer whip, deer's tail, venison and deer blood etc.Because the deer product is rare traditional Chinese medicine mostly, cost an arm and a leg, so see repeatly on the market with low-quality goods and pretend to be famous and precious deer product.
At present, traditional method is adopted in the evaluation of deer product mostly, mainly comprises macroscopical identification, microscopical identification and physics and chemistry evaluation.Though traditional authentication method is simple, quick, cost is low, influences the factor a lot (like human factor, environmental factors, trophic factor) of traditional authentication method, thereby can not judge the situation of poor quality of deer product exactly.Such as in the course of processing of deer product, its proterties, microstructure, physico-chemical property etc. usually change, and utilize traditional authentication method to identify that erroneous judgement may appear in the deer product.Yet molecular assay method (based on the method for DNA) does not receive the influence of these factors, and has characteristics such as accuracy is big, highly sensitive, good stability, highly versatile.
Summary of the invention:
The present invention provides the PCR test kit of a kind of rapid detection reinder source property deer product, has solved the problem that whether contains the reinder composition in the deer product.
The present invention also provides the preparation method of the PCR test kit of above-mentioned rapid detection deer product, adopts single step reaction to differentiate the reinder derived component in the deer product through a PCR method reaction system.
The PCR test kit of rapid detection reinder provided by the invention source property deer product is characterized in that:
Comprise DNA extraction liquid, PCR reaction solution and negative standard substance:
Described DNA extraction liquid:
(1) low salt buffer (pH 7.6-7.8): 12-13 part Tris alkali (Tutofusin tris), 32-35 part Na
2EDTA (EDTA Disodium), 7-8 part MgCl
2, 4-5 part NaCl, surplus part is water;
(2) cell pyrolysis liquid: 4-6 part SDS sodium lauryl sulphate, 4-6 part Triton X-100 (polyoxyethylene glycol is to the iso-octyl phenyl ether), 1000 parts of low salt buffers;
Described PCR reaction solution:
DdH2O, 10 * PCR Buffer, dNTPs, upstream primer, downstream primer, Taq enzyme;
Concrete primer sequence is:
Upstream primer: 5 '-GGAGTAATCCAGGTCGGTTTCTATC-3 '
Downstream primer: 5 '-TAGGGCGGGATATGTTTGTGTATC-3 '
Negative standard substance: be aseptic double-distilled water.
The preparation method of the PCR test kit of rapid detection reinder according to the invention source property deer product may further comprise the steps:
1) DNA extraction liquid
(1) low salt buffer (pH 7.6-7.8): 12-13 part Tris alkali (Tutofusin tris), 32-35 part Na
2EDTA (EDTA Disodium), 7-8 part MgCl
2, 4-5 part NaCl, surplus part is water;
(2) cell pyrolysis liquid: 4-6 part SDS sodium lauryl sulphate, 4-6 part Triton X-100 (polyoxyethylene glycol is to the iso-octyl phenyl ether), 1000 parts of low salt buffers;
2) PCR reaction solution.
(1) design of primers: at the plastosome 16S of reinder rRNA gene region, design a pair of Auele Specific Primer, comprise a upstream primer and a downstream primer.Sequence is following:
Upstream primer: 5 '-GGAGTAATCCAGGTCGGTTTCTATC-3 '
Downstream primer: 5 '-TAGGGCGGGATATGTTTGTGTATC-3 '
(2) PCR reaction solution:
DdH2O 9.3ul, 10 * PCR Buffer 1.5ul, dNTPs (100 uM) 2.0ul, upstream primer (20 uM) 0.5ul, downstream primer (20 uM) 0.5ul, Taq enzyme (5U/ul) 0.2ul.
(3) negative standard substance: be aseptic double-distilled water.
The method of use that reinder of the present invention source property deer product P CR detects:
(1) from sample to be checked, extracts genomic dna;
(2) preparation PCR reaction system:
DNA 1ul and the negative control got in the step (1) join in the PCR reaction solution, increase with the PCR appearance;
(3) set response procedures and carry out pcr amplification, response procedures is all following:
94℃ 5min;94℃ 30s,60℃ 30s,72℃ 30s,30?cycles;72℃ 5min。
(4) get 5 μ l PCR products after reaction finishes and analyze observations under the uv lamp at 1% agarose gel electrophoresis.
The result judges: if amplify the fragment that length is 141bp, explain and contain the reinder derived components in the test sample.
Positively effect of the present invention is: adopt the special molecular fragment of the Mitochondrial DNA of round pcr amplification reinder, the generate a reagent box is used for detecting test sample and whether contains the reinder composition, and can detect biased sample; Have simple to operate, highly sensitive, characteristics such as speed is fast.
Description of drawings
Fig. 1 is a specificity between the kind of primer;
Fig. 2 is the interior versatility of the kind of primer.
Embodiment
Below in conjunction with the practical implementation instance, further set forth the present invention:
Embodiment 1: the composition of test kit and preparation
1) preparation of DNA extraction liquid
(1) low salt buffer (pH 7.6): 800ml dissolved in distilled water 1.21gTris alkali (Tutofusin tris), 3.38g Na
2EDTA (EDTA Disodium), 0.76g MgCl
2, 0.47gNaCl.Add concentrated hydrochloric acid and transfer pH to desirable value, adding distil water is settled to 1L.
(2) cell pyrolysis liquid: add 1g SDS (sodium lauryl sulphate), 1ml Triton X-100 (polyoxyethylene glycol is to the iso-octyl phenyl ether) in the 200ml low salt buffer.
Process for extracting: 200ul anticoagulation and 400ul low salt buffer join in the 1.5ml centrifuge tube, and fully the centrifugal 10min of 1000RPM behind the mixing abandons supernatant; Add the 500ul low salt buffer, behind the mixing under room temperature the centrifugal 5min of 1000RPM, repeat once; Careful sucking-off supernatant adds the 300ul cell pyrolysis liquid, behind the mixing in 65 ℃ of water-bath 10min; Add the saturated NaCl of 75ul, fully the centrifugal 5min of 12000RPM behind the mixing transfers to supernatant in the new 1.5ml centrifuge tube; Add 2 times of volume absolute ethyl alcohols, in the centrifugal 2min of 10000RPM, abandon supernatant behind the abundant mixing; Add 500ul ice bath 70% ethanol, put upside down mixing and abandon supernatant in the centrifugal 1min of 10000RPM in the back for several times; Dry 5min in 65 ℃ of baking ovens dissolves 15min in 65 ℃ of water-baths behind the adding 100ul ddH2O.
2) PCR reaction solution
(1) design of primers: adopt Bioedit 7.0.9.0 software to carry out sequence alignment according to the plastosome sequence of having announced in the GenBank DB.Utilize Oligo 6.0 softwares in the plastosome 16S of reinder rRNA gene region design specific primers.Comprise a upstream primer and a downstream primer.Primer will have specificity between kind of interior versatility and kind.Sequence is following:
Upstream primer: 5 '-GGAGTAATCCAGGTCGGTTTCTATC-3 '
Downstream primer: 5 '-TAGGGCGGGATATGTTTGTGTATC-3 '
(2) PCR reaction solution:
DdH2O 9.3ul, 10 * PCR Buffer 1.5ul, dNTPs (100 uM) 2.0ul, upstream primer (20 uM) 0.5ul, downstream primer (20 uM) 0.5ul, Taq enzyme (5U/ul) 0.2ul.
(3) negative standard substance: be aseptic double-distilled water.
The foundation of embodiment 2:PCR optimum reaction condition.
For a PCR reaction, most important reaction conditions is exactly an annealing temperature, therefore sets the top condition of PCR reaction from this aspect.Specificity and the interior generally adopted principle of kind between the setting of optimum reaction condition at first should be followed and plant, the temperature when selecting expanding effect the most desirable then on this basis is set at the optimal reaction temperature of primer.
1) extraction of DNA
From blood, extracted the genomic dna of reinder according to the method for embodiment 1.
2) preparation of PCR reaction system:
The DNA 1ul that extracts in the step 1) is joined in the PCR reaction solution among the embodiment 1, constitute the reaction system of 15ul.
3) setting of PCR reaction optimum annealing temperature.
The gradient scope of annealing temperature is 54-68 ℃, whenever establishes a gradient at a distance from 2 ℃, is reflected on the Eppendorf AG instrument and increases.
Program is following:
94 ℃ of 5min; 94 ℃ of 30s, 54-68 ℃ of 30s, 72 ℃ of 30s, 72 ℃ of 5min, 30 circulations of increasing.
Get 5 μ l PCR products after reaction finishes and in 1% sepharose, carry out electrophoresis detection, write down experimental result in the gel imaging system, confirm the optimum annealing temperature of every pair of primer according to the brightness of band in the gel.
4) establishment of best PCR reaction conditions.
The final PCR optimum reaction condition of establishing is: 94 ℃ of 5min; 94 ℃ of 30s, 60 ℃ of 30s, 72 ℃ of 30s, 72 ℃ of 5min, 30 circulations of increasing.
Embodiment 3: the specificity test of test kit
1) proves that primer has specificity between kind.
(A) To prove the present invention has a species-specific primers, in accordance with the method of Example 1 was extracted deer, red deer, Tarim red deer, red deer, reindeer, deer, Eld's deer, white-lipped deer, elk, fallow deer, pigs , cattle, sheep, chicken genomic DNA, a DNA extraction system for preparing a PCR reaction, sterile water as a negative control.
(2) preparation of PCR reaction system: the DNA 1ul that gets step (1) extraction joins in the PCR reaction solution among the embodiment 1, constitutes the 15ul system.
(3) according to response procedures: 94 ℃ of 5min; 94 ℃ of 30s, 60 ℃ of 30s, 72 ℃ of 30s, 72 ℃ of 5min, 30 circulations of increasing.Carry out pcr amplification.
(4) The results shown in Figure 1: N: deer; C: red deer; Y: Tarim red deer; E: red deer; R: Reindeer; 1: Sambar; 2: Eld; 3: white-lipped deer; 4: elk; 5 : fallow deer; 6: Pig; 7: Cattle; 8: Sheep; 9: chicken; 10: negative control; M: Marker? I (600,500,400,300,200,100? bp);
In all species, genomic DNA PCR reaction, only reindeer genomic DNA fragment was amplified 141bp specificity, and deer, red deer, Tarim red deer, red deer, sambar, Eld's deer, white-lipped deer, elk, fallow deer, pigs, cattle, sheep, chicken genomic DNA was negative, indicating that the present invention is a species-specific primers.
2) prove versatility in the kind of primer.
Primer also must have kind of an interior versatility simultaneously except between planting, having the specificity, therefore versatility in the kind of primer is also assessed.
1) extracted the genomic dna of 9 reinder according to the method for embodiment 1, the DNA of extraction is used to prepare the PCR reaction system, and sterilized water is as negative control.
(2) preparation of PCR reaction system: the DNA 1ul that gets step (1) extraction joins in the PCR reaction solution among the embodiment 1, constitutes the 15ul system.
(3) according to response procedures: 94 ℃ of 5min; 94 ℃ of 30s, 60 ℃ of 30s, 72 ℃ of 30s, 72 ℃ of 5min, 30 circulations of increasing.Carry out pcr amplification.
(4) result such as Fig. 2: reinder (1-9), 10: negative control; M:Marker I (600,500,400,300,200,100 bp); The genomic dna of 9 reinder has all amplified the purpose fragment of 141bp.Explain that primer of the present invention has versatility in planting.
Claims (3)
1. the PCR test kit of a rapid detection reinder source property deer product is characterized in that comprising following primer:
Upstream primer: 5 '-GGAGTAATCCAGGTCGGTTTCTATC-3 '
Downstream primer: 5 '-TAGGGCGGGATATGTTTGTGTATC-3 '.
2. the PCR test kit of the described rapid detection reinder of claim 1 source property deer product is characterized in that comprising DNA extraction liquid, PCR reaction solution and negative standard substance;
Described DNA extraction liquid:
(1) low salt buffer (pH 7.6-7.8): 12-13 part Tris alkali (Tutofusin tris), 32-35 part Na
2EDTA (EDTA Disodium), 7-8 part MgCl
2, 4-5 part NaCl, surplus part is water;
(2) cell pyrolysis liquid: 4-6 part SDS sodium lauryl sulphate, 4-6 part Triton X-100 (polyoxyethylene glycol is to the iso-octyl phenyl ether), 1000 parts of low salt buffers;
Described PCR reaction solution:
DdH2O, 10 * PCR Buffer, dNTPs, upstream primer, downstream primer, Taq enzyme;
Concrete primer sequence is:
Upstream primer: 5 '-GGAGTAATCCAGGTCGGTTTCTATC-3 '
Downstream primer: 5 '-TAGGGCGGGATATGTTTGTGTATC-3 '
Negative standard substance: be aseptic double-distilled water.
3. the preparation method of the PCR test kit of the described rapid detection reinder of claim 2 source property deer product may further comprise the steps:
1) DNA extraction liquid
(1) low salt buffer (pH 7.6-7.8): 12-13 part Tris alkali (Tutofusin tris), 32-35 part Na
2EDTA (EDTA Disodium), 7-8 part MgCl
2, 4-5 part NaCl, surplus part is water;
(2) cell pyrolysis liquid: 4-6 part SDS sodium lauryl sulphate, 4-6 part Triton X-100 (polyoxyethylene glycol is to the iso-octyl phenyl ether), 1000 parts of low salt buffers;
2) PCR reaction solution:
(1) design of primers: at the plastosome 16S of reinder rRNA gene region, design a pair of Auele Specific Primer, comprise a upstream primer and a downstream primer; Sequence is following:
Upstream primer: 5 '-GGAGTAATCCAGGTCGGTTTCTATC-3 '
Downstream primer: 5 '-TAGGGCGGGATATGTTTGTGTATC-3 '
(2) PCR reaction solution:
DdH2O 9.3ul, 10 * PCR Buffer 1.5ul, dNTPs (100 uM) 2.0ul, upstream primer (20 uM) 0.5ul, downstream primer (20 uM) 0.5ul, Taq enzyme (5U/ul) 0.2ul;
(3) negative standard substance: be aseptic double-distilled water.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN2012101085582A CN102605095A (en) | 2012-04-15 | 2012-04-15 | PCR (polymerase chain reaction) kit for rapidly detecting reindeer-derived deer product and preparation method thereof |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN2012101085582A CN102605095A (en) | 2012-04-15 | 2012-04-15 | PCR (polymerase chain reaction) kit for rapidly detecting reindeer-derived deer product and preparation method thereof |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CN102605095A true CN102605095A (en) | 2012-07-25 |
Family
ID=46522859
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CN2012101085582A Pending CN102605095A (en) | 2012-04-15 | 2012-04-15 | PCR (polymerase chain reaction) kit for rapidly detecting reindeer-derived deer product and preparation method thereof |
Country Status (1)
| Country | Link |
|---|---|
| CN (1) | CN102605095A (en) |
Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102876805A (en) * | 2012-10-25 | 2013-01-16 | 苏州市红冠庄国药饮片有限公司 | Primer system for PCR (polymerase chain reaction) identification for deer, pig, cow, sheep, horse, donkey, rabbit and chicken |
| CN103525935A (en) * | 2013-10-22 | 2014-01-22 | 张敏 | Identification primers for penis cervi of New Zealand wapiti and penis cervi of sika deer as well as PCR (Polymerase Chain Reaction) identification method |
-
2012
- 2012-04-15 CN CN2012101085582A patent/CN102605095A/en active Pending
Non-Patent Citations (2)
| Title |
|---|
| 查代明,邢秀梅,杨福合: "水鹿的分子鉴定", 《特产研究》 * |
| 查代明: "《基于线粒体DNA序列的鹿产品分子检测》", 《中国优秀硕士学位论文全文数据库医药卫生科技辑(月刊)》 * |
Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102876805A (en) * | 2012-10-25 | 2013-01-16 | 苏州市红冠庄国药饮片有限公司 | Primer system for PCR (polymerase chain reaction) identification for deer, pig, cow, sheep, horse, donkey, rabbit and chicken |
| CN102876805B (en) * | 2012-10-25 | 2013-10-09 | 苏州市红冠庄国药饮片有限公司 | Primer system for PCR (polymerase chain reaction) identification for deer, pig, cow, sheep, horse, donkey, rabbit and chicken |
| CN103525935A (en) * | 2013-10-22 | 2014-01-22 | 张敏 | Identification primers for penis cervi of New Zealand wapiti and penis cervi of sika deer as well as PCR (Polymerase Chain Reaction) identification method |
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| CN102605098A (en) | Multiplex-polymerase chain reaction (PCR) kit for rapidly detecting deer product and preparation method thereof | |
| CN103898235A (en) | DNA (deoxyribonucleic acid) barcoding based molecular identification method of leech | |
| CN109554507B (en) | Detection method of H5 and H7N9 subtype highly pathogenic avian influenza virus | |
| CN109234462A (en) | A kind of reverse transcription recombinase-mediated isothermal amplification detection method of avian influenza virus | |
| CN102329888A (en) | Fluorescent quantitative PCR (Polymerase Chain Reaction) testing method for cccDNA (covalently closed circular deoxyribonucleic acid) of hepatitis B virus and kit thereof | |
| CN102618653A (en) | Polymerase chain reaction (PCR) kit capable of rapidly detecting cervus derived products and preparation method | |
| WO2016075277A1 (en) | Novel fish virus and method for detection | |
| CN103540680A (en) | Dual reverse transcription-polymerase chain reaction (RT-PCR) detection method for identifying H9N2 subtype avian influenza virus | |
| CN104988246A (en) | Eriocheir sinensis white spot syndrome virus specificity PCR detection kit and method | |
| CN102605095A (en) | PCR (polymerase chain reaction) kit for rapidly detecting reindeer-derived deer product and preparation method thereof | |
| CN101629217A (en) | RT-LAMP detection kit and detection method of swine influenza virus | |
| CN102605097A (en) | Polymerase chain reaction (PCR) kit for rapidly detecting red deer-derived deer product | |
| CN109207643A (en) | A kind of real-time fluorescence quantitative RT-PCR detection method of avian influenza virus | |
| CN101376909B (en) | A segment of sequence and a restriction enzyme site for differentiating canine distemper viral vaccine strain and wild strain | |
| CN102534052B (en) | Nucleic-acid sequence-based amplification (NASBA) method for detecting swine influenza virus (SIV) | |
| CN108531651A (en) | A kind of specific primer and its application for detecting and differentiating FAdV-4 and FAdV-8b | |
| CN102605096A (en) | Polymerase chain reaction (PCR) kit for rapidly detecting sambar-derived deer product and preparation method thereof | |
| CN109722492B (en) | Method for detecting H5 and H7N9 subtype highly pathogenic avian influenza virus and H9 subtype avian influenza virus | |
| CN102329891B (en) | RT-LAMP (reverse transcription-loop-mediated isothermal amplification) primer group for detecting H9 subtype avian influenza virus as well as detection method and application thereof | |
| CN101845515B (en) | Method for detection of swine influenza A H1N1 virus based on pyrosequencing technology | |
| CN102618652A (en) | PCR (Polymerase chain reaction) kit for rapidly detecting Tarim wapiti-derived deer's products and preparation method for PCR kit | |
| CN101921869B (en) | Method for identifying virulent strain and attenuated strain in Newcastle disease virus by pyrosequencing technology | |
| CN109055613A (en) | I type astrovirus ring mediated isothermal amplification detection primer group of chicken, kit and its detection method | |
| CN101921868B (en) | Method for determining avian influenza virus subtype by pyrosequencing technology | |
| CN109628643B (en) | Rapid detection method for H5 subtype avian influenza virus |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| C06 | Publication | ||
| PB01 | Publication | ||
| C10 | Entry into substantive examination | ||
| SE01 | Entry into force of request for substantive examination | ||
| C02 | Deemed withdrawal of patent application after publication (patent law 2001) | ||
| WD01 | Invention patent application deemed withdrawn after publication |
Application publication date: 20120725 |