CN101403004A - Rapid diagnosis reagent kit and detection method for vibrio vulnficus gene - Google Patents
Rapid diagnosis reagent kit and detection method for vibrio vulnficus gene Download PDFInfo
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- CN101403004A CN101403004A CNA200810198808XA CN200810198808A CN101403004A CN 101403004 A CN101403004 A CN 101403004A CN A200810198808X A CNA200810198808X A CN A200810198808XA CN 200810198808 A CN200810198808 A CN 200810198808A CN 101403004 A CN101403004 A CN 101403004A
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Abstract
The invention discloses a rapid diagnosis kit and a detection method of genes of vibrio vulnificus. The kit consists of two pairs of primers, DNA polymerase, stabilizing solution, reaction solution, sample pre-treatment solution, color development solution and positive comparison solution, wherein, the seven solutions are respectively placed in containers. The rapid diagnosis kit of genes of the invention applies six sections and four primers and can judge whether target materials exist only according to the amplification, thus being high in specificity. The rapid diagnosis kit of genes of the invention is high in speed, high in efficiency and sensitivity, can amplify the reaction with only constant temperature, without special reagents or equipment, and is low in detection cost. The rapid diagnosis kit of genes of the invention is simple and convenient in identification. Pyrophosphate ions separated out from the dNTP are combined with Mg<2+> in the reaction solution to produce a by-product which is the sediment of magnesium pyrophosphate which can be identified by naked eyes. Furthermore, after the color development solution is added, the color development differences of negative and positive results are notable and the identification is more obvious and reliable.
Description
Technical field
The present invention relates to biological detection reagent, be specifically related to a kind of vibrio vulnficus gene quick diagnosis reagent kit and detection method thereof.
Background technology
At present Vibrio vulnificus there is multiple detection method, from identifying and the automatic biochemical evaluation with pathogenic micro-organism isolation identification, morphology, immunology detection technology, nucleic acid probe, polymerase chain reaction (PCR) technology equimolecular biological detection method [food safety detection and modern biotechnology to differential protein, Chemical Industry Press, 2004].Wherein the cause of disease detection of nucleic acids all improves a lot at aspects such as rapidity, security, accuracy and susceptibilitys, these new technologies are attempted to break through microbiologies such as traditional morphology, biochemical reaction and are detected old model, do not need microorganism is separated purification, and directly its gene and gene product are carried out rapid detection with the enrichment liquid of sample or sample, and combine with Protocols in Molecular Biology and information biology means, to accurately, fast, the direction of sensitivity and automatization develops.
With polymerase chain reaction (PCR) technology is that the cause of disease nucleic acid detection technique of representative also exists some problems in actual applications, as the special instrument of common polymerase chain reaction (PCR) Technology Need, and there are easy crossed contamination and the loaded down with trivial details shortcoming of operating process.And fluorescence real-time quantitative polymerase chain reaction (real time PCR) though technology has solved the problem of crossed contamination preferably, and has simplified operating process, needs more complicated quantitative assay instrument, therefore is not suitable for field quick detection.And the cost of fluorescent probe is higher in the real-time quantitative polymerase chain reaction PCR technology, has strengthened the difficulty of applying.The immunology detection technology is fast and convenient with low cost, but requires the monoclonal antibody of high quality high stability, otherwise because of accuracy is not enough, can only be the auxiliary detection means at present.So in time use the newest fruits of biotech development significant to satisfying improving constantly of pathogenic micro-organism detection requirement.Wherein isothermal duplication (Isothermal Amplification) nucleic acid Fast Detection Technique is the rapid progress on the cause of disease nucleic acid detection technique, the loop-mediated isothermal amplification technique of now having set up (loop-mediated isothermal amplication of DNA, be called for short LAMP) have a lot of superiority, and do not see that useful loop-mediated isothermal amplification technique detects the gene quick diagnosis kit of Vibrio vulnificus at present yet.
Summary of the invention
The objective of the invention is deficiency, a kind of vibrio vulnficus gene quick diagnosis reagent kit based on loop-mediated isothermal amplification technique that cost is low, easy to use, detection speed is fast, specificity is high that detects is provided at the prior art existence.
Another object of the present invention provides the detection method of above-mentioned vibrio vulnficus gene quick diagnosis reagent kit.
Above-mentioned purpose of the present invention is achieved by following technical solution:
One, vibrio vulnficus gene quick diagnosis reagent kit of the present invention is made up of two pairs of primers, BstDNA polysaccharase, reaction solution, stable liquid, sample pretreatment liquid, colour developing liquid and positive control solution, more than seven kinds of liquid place container respectively, wherein:
Described two pairs of primers are:
Outer primer F3:TGAGAACGGTGACAAAACGG;
Outer primer B3:GAGCTTATCGCCTTCCCAAT;
Inner primer FIP:AGGCCCCAAACTTGGTTCCAATTTTTTGCGGGTGGTTCGGTTA;
Inner primer BIP:AGCCGAGTRGCATCCGATCGTTTTGCTAAGTTCGCACCACACT;
Contain 1.6~2mmol dNTP, 20~25mmolTris-HCl, 10~12.5mmol Repone K, 10~12.5mmol ammonium sulfate, 8~10mmol sal epsom, 1~1.25ml TritonX-100,0.8~1mol trimethyl-glycine, each 1.6~2mol of inner primer FIP/BIP and each 0.2~0.25mol of outer primer F3/B3 in above-mentioned every 1L reaction solution; Preferred ratio is to contain 2mmol dNTP, 25mmol Tris-HCl, 12.5mmol Repone K, 12.5mmol ammonium sulfate, 10mmol sal epsom, 1.25ml TritonX-100,1mol trimethyl-glycine, each 2mol of inner primer FIP/BIP and each 0.25mol of outer primer F3/B3 in every 1L reaction solution.
Tris-HCl, the 1~2mmol EDTA and the 10~12ml Triton X-100 that contain 10~20mmol pH 8.0 in above-mentioned every 1L sample pretreatment liquid.Preferred ratio is to contain 20mmol Tris-HCl (pH 8.0), 2mmol EDTA and 12ml TritonX-100 in every 1L sample pretreatment liquid.
Above-mentioned colour developing liquid is preferably fluorescence dye SYBR Green I or EvaGreen;
Aforementioned stable liquid is preferably paraffin oil.
Above-mentioned positive control is vibrio vulnficus gene group DNA.
Two, the production technique of gene quick diagnosis kit of the present invention
1, with behind inner primer FIP/BIP and the outer primer F3/B3 synthesizing and purifying, quantitatively preparation, concentration detects, the sampling quality inspection;
2, reaction solution is aseptic subpackaged, and determine the quality inspection of sampling with carrying out concentration according to experiment;
3, stable liquid is aseptic subpackaged, the sampling quality inspection;
4, with the positive control sample preparations, packing, sampling quality inspection;
5, assembling test kit.
Three, the detection method of gene quick diagnosis kit of the present invention
1, sample preparation
Testing sample is increased behind the bacterium centrifugal in centrifuge tube, remove supernatant, add sample pretreatment liquid in the precipitation and mix, cooled on ice after the boiling water bath deactivation, behind the high speed centrifugation, supernatant is the sample template DNA;
2, loop-mediated isothermal amplification technique reaction process
In reaction tubes, add reaction solution 38~40 volume %, big fragment 0.9~1.8 volume % of Bst archaeal dna polymerase, stable liquid 52~54.5 volume %, sample template DNA 4.5~9 volume %, 63~65 ℃ of isothermal reaction 45~90min.Described volume percent is meant the volume percent that accounts for four component cumulative volumes.
3, post-reaction treatment
In above-mentioned reaction tubes and positive controls, add colour developing liquid respectively, mixing, the sample sets colour developing is identical with control group then positive, otherwise negative.
Principle of the present invention is the special inside and outside primer (being inner primer FIP/BIP and outer primer F3/B3) of two couples that utilizes the Bst archaeal dna polymerase and design according to target-gene sequence, six isolated areas on the specific recognition target sequence, start the endless chain replacement(metathesis)reaction, start complementary strand in target DNA district synthetic, and result's complementary sequence on same chain goes round and begins again and is formed with the very stem of polycyclic Cauliflower structure-circular DNA mixture.In the LAMP reaction process, pyrophosphate ion of separating out from dNTP and the Mg the reaction soln
2+In conjunction with, produce by product---magnesium pyrophosphate milky white precipitate, can be by the visual inspection result of determination.The LAMP reaction is to finish in 45~90 minutes under constant temperature (63~65 ℃) condition.This comparatively gentle temperature condition and do not have temperature cycle that required instrument is oversimplified, overcome conventional P CR inherent detection time long, pollute easily and detect shortcoming such as cost height.In addition, this detection method is lower to testing staff's technical quality requirement, and actually operating is very easy, does not need special reagent and plant and instrument, helps setting up rapid screening system with low cost.The LAMP method is a kind of gene amplification method of easy, quick, high degree of specificity.Constant temperature gene amplification technology and round pcr (comprising the fluorescence real-time quantitative PCR technology) are compared, can find that this technology is equivalent to or is better than round pcr on methodology indexs such as sensitivity, specificity and sensing range, and do not rely on any special plant and instrument and can realize on-the-spot high-throughput rapid detection, and detect cost far below fluorescent quantitative PCR technique.Domestic do not have the test kit of this respect to sell at present as yet.At present in the national standard with microorganism separation and Culture and morphology be accredited as main, in conjunction with the passing method that biochemical analysis and serological typing are identified, preliminary evaluation needs 2~3 days, finishes probation report and needs 10~15 days; Adopt gene quick diagnosis kit of the present invention only to need 2 hours.And, having added colour developing liquid in the reaction solution of the present invention, qualification result is more visual and clear.
Compared with prior art, the present invention has following beneficial effect:
1. gene quick diagnosis kit of the present invention only needs just energy amplified reaction of a steady temperature, does not need special reagent and equipment, and it is low to detect cost; 2. gene quick diagnosis kit of the present invention is used six sections, four primers, and whether the existence that just can judge target substance according to whether increasing to be, so has high specific; 3. gene quick diagnosis kit of the present invention amplification fast and efficient can be finished amplification less than 1 hour, and the productive rate height; 4. gene quick diagnosis kit of the present invention is highly sensitive, and amplification template only needs 10 copies or still less; 5. gene quick diagnosis kit of the present invention is identified easy, pyrophosphate ion of separating out from dNTP and the Mg the reaction soln
2+In conjunction with, produce by product-magnesium pyrophosphate precipitation, can identify by visual inspection, and after adding colour developing liquid, yin and yang attribute colour development difference as a result is remarkable, checking rate height, more obviously reliable.
Embodiment
The preparation of embodiment 1 test kit
(1) in the following sequence through the synthetic oligomerization picodna primer of dna synthesizer:
Outer primer F3:TGAGAACGGTGACAAAACGG;
Outer primer B3:GAGCTTATCGCCTTCCCAAT;
Inner primer FIP:AGGCCCCAAACTTGGTTCCAATTTTTTGCGGGTGGTTCGGTTA;
Inner primer BIP:
AGCCGAGTRGCATCCGATCGTTTTGCTAAGTTCGCACCACACT;
(2) purchase archaeal dna polymerase: BstDNApolymerase (big fragment) places container.
(3) preparation reaction solution: the prescription of reaction solution contains each 0.25mol preparation of 2mmol dNTP, 25mmol Tris-Cl, 12.5mmol Repone K, 12.5mmol ammonium sulfate, 10mmol sal epsom, 1.25ml TritonX-100,1mol trimethyl-glycine, each 2mol of inner primer FIP/BIP and outer primer F3/B3 by every 1L solution, places container.
(4) preparation sample pretreatment liquid: the prescription of sample pretreatment liquid contains 20mmol Tris-HCl (pH 8.0), 2mmol EDTA and 12ml Triton X-100 preparation by every 1L solution, places container.
(5) purchase stable liquid: paraffin oil places container;
(6) purchase colour developing liquid: SYBR Green I places container.
(7) extract positive control: vibrio vulnficus gene group DNA places container.
(8) above-mentioned 7 containers are dressed up test kit, encapsulation.
Preparation technology is summarized as follows:
1, with behind inner primer FIP/BIP and the outer primer F3/B3 synthesizing and purifying, quantitatively preparation, concentration detects, the sampling quality inspection;
2, reaction solution is aseptic subpackaged, and determine the quality inspection of sampling with carrying out concentration according to experiment;
3, with the stable liquid packing, the sampling quality inspection;
4, with the positive control sample preparations, packing, sampling quality inspection;
5, assembling test kit.
The preparation of embodiment 2 test kits
The prescription of reaction solution is: contain 1.6mmol dNTP, 20mmolTris-HCl, 10mmol Repone K, 10mmol ammonium sulfate, 8mmol sal epsom, 1ml TritonX-100,0.8mol trimethyl-glycine, each 1.6mol of inner primer FIP/BIP and each 0.2mol of outer primer F3/B3 in every 1L reaction solution;
The prescription of sample pretreatment liquid is: Tris-HCl, the 1mmol EDTA and the 10ml Triton X-100 that contain 10mmol pH8.0 in every 1L sample pretreatment liquid.
Colour developing liquid is EvaGreen.
Other are with embodiment 1.
The application of embodiment 3 vibrio vulnficus gene quick diagnosis reagent kits
1, sample preparation (template DNA extraction)
(1) adopts the about 200ml of aseptic technique water sampling (or samples such as settling, ooze), can staticly settle or the centrifugal 1min removal of 1000r/min large particulate matter if any impurity;
(2) will pass through aperture 0.22 μ m~0.45 μ m membrane filtration through precipitation or centrifuged sample (supernatant), and take off filter membrane and place the 15ml aqua sterilisa, fully wash-out;
(3) get the 5ml elution samples, the centrifugal 2min of 10000rpm obtains bacterial sediment;
(4) in above-mentioned bacterial sediment, add 100 μ l sample pretreatment liquid and mix, boil in the boiling water after 10 minutes and placed cooled on ice immediately 10 minutes, centrifugal 2 minutes of 10000rpm, supernatant is the sample template DNA.
2, the reaction process of loop-mediated isothermal amplification technique
1) in 200 μ l reaction tubess preparation reaction system: reaction solution 22 μ l, Bst archaeal dna polymerase 0.5 μ l (4U), stable liquid 30 μ l, template DNA 2.5 μ l.
2) with the reaction tubes for preparing in 64 ℃ of isothermal reaction 1h.
3, post-reaction treatment
In above-mentioned reaction product, add 2 μ l SYBR Green I, mixing, also add SYBR Green I mixing in the heliotropism control tube (vibrio vulnficus gene group DNA) simultaneously, if the same shows green with control tube of reaction tubes is then positive, if reaction tubes manifests orange then negative.
Claims (7)
1, a kind of vibrio vulnficus gene quick diagnosis reagent kit is characterized in that being made up of Bst archaeal dna polymerase, reaction solution, stable liquid, sample pretreatment liquid, colour developing liquid and positive control solution, more than five kinds of liquid place container respectively,
Two pairs of primers are in the reaction solution:
Outer primer F3:TGAGAACGGTGACAAAACGG;
Outer primer B3:GAGCTTATCGCCTTCCCAAT;
Inner primer FIP:AGGCCCCAAACTTGGTTCCAATTTTTTGCGGGTGGTTCGGTTA;
Inner primer BIP:AGCCGAGTRGCATCCGATCGTTTTGCTAAGTTCGCACCACACT;
Contain 1.6~2mmol dNTP, 20~25mmol Tris-HCl, 10~12.5mmol Repone K, 10~12.5mmol ammonium sulfate, 8~10mmol sal epsom, 1~1.25ml TritonX-100,0.8~1mol trimethyl-glycine, each 1.6~2mol of inner primer FIP/BIP and each 0.2~0.25mol of outer primer F3/B3 in every 1L reaction solution;
Tris-HCl, the 1~2mmol EDTA and the 10~12ml Triton X-100 that contain 10~20mmol pH 8.0 in every 1L sample pretreatment liquid;
Above-mentioned positive control is vibrio vulnficus gene group DNA.
2,, it is characterized in that described colour developing liquid is SYBRGreen I or EvaGreen according to the described test kit of claim 1.
3,, it is characterized in that containing in described every 1L sample pretreatment liquid Tris-HCl, 2mmol EDTA and the 12ml TritonX-100 of 20mmol pH 8.0 according to the described test kit of claim 1.
4,, it is characterized in that containing in described every 1L reaction solution 2mmol dNTP, 25mmol Tris-HCl, 12.5mmol Repone K, 12.5mmol ammonium sulfate, 10mmol sal epsom, 1.25ml TritonX-100,1mol trimethyl-glycine, each 2mol of inner primer FIP/BIP and each 0.25mol of outer primer F3/B3 according to the described test kit of claim 1.
5,, it is characterized in that described stable liquid is paraffin oil according to the described test kit of claim 1.
6, a kind of method that detects Vibrio vulnificus is characterized in that using the described test kit of claim 1, follows these steps to carry out:
(1) testing sample is increased behind the bacterium centrifugally in centrifuge tube, remove supernatant, add sample pretreatment liquid in the precipitation and mix, cooled on ice after the boiling water bath deactivation, behind the high speed centrifugation, supernatant is the sample template DNA;
(2) in reaction tubes, add reaction solution 38~40 volume %, big fragment 0.9~1.8 volume % of Bst archaeal dna polymerase, stable liquid 52~54.5 volume %, sample template DNA4.5~9 volume %, isothermal reaction;
(3) in above-mentioned reaction tubes and positive controls, add colour developing liquid respectively, mixing, the sample sets colour developing is identical with control group then positive, otherwise negative.
7,, it is characterized in that in the step (2) that the reaction conditions of isothermal reaction is 63~65 ℃ of temperature, reaction times 45~90min according to the described detection method of claim 6.
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CN111041112A (en) * | 2015-09-02 | 2020-04-21 | 上海产业技术研究院 | Rapid constant-temperature detection method of vibrio vulnificus, primer set and application |
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CN101082579A (en) * | 2006-05-29 | 2007-12-05 | 广州华峰生物科技有限公司 | Gene rapid diagnosis method based on annular mediated isothermal amplification technology |
CN101082581A (en) * | 2006-05-30 | 2007-12-05 | 广州华峰生物科技有限公司 | Colon bacillus 0157 gene rapid diagnosis reagent kit of annular mediated isothermal amplification technology |
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CN111041112A (en) * | 2015-09-02 | 2020-04-21 | 上海产业技术研究院 | Rapid constant-temperature detection method of vibrio vulnificus, primer set and application |
CN111057779A (en) * | 2015-09-02 | 2020-04-24 | 上海旺旺食品集团有限公司 | Rapid constant-temperature detection method for vibrio vulnificus and application |
CN111057779B (en) * | 2015-09-02 | 2022-08-26 | 上海旺旺食品集团有限公司 | Rapid constant-temperature detection method for vibrio vulnificus and application |
CN111041112B (en) * | 2015-09-02 | 2022-09-20 | 上海产业技术研究院 | Rapid constant-temperature detection method of vibrio vulnificus, primer set and application |
CN107034266A (en) * | 2016-01-29 | 2017-08-11 | 清华大学 | For detecting that the primer of wound infection pathogen is combined and integrating device |
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