CN106755342A - Based on the ring mediated isothermal amplification that color judges(LAMP)Technology for detection chestnut phytophthora Heisui River germ - Google Patents

Based on the ring mediated isothermal amplification that color judges(LAMP)Technology for detection chestnut phytophthora Heisui River germ Download PDF

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CN106755342A
CN106755342A CN201611084928.8A CN201611084928A CN106755342A CN 106755342 A CN106755342 A CN 106755342A CN 201611084928 A CN201611084928 A CN 201611084928A CN 106755342 A CN106755342 A CN 106755342A
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germ
phytophthora
heisui river
primer
lamp
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纪睿
曾丹丹
廖太林
郑小波
张正光
周锐
吴军
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P R OF CHINA KUNSHAN ENTRY-EXIT INSPECTION AND QUARANTINE BUREAU
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P R OF CHINA KUNSHAN ENTRY-EXIT INSPECTION AND QUARANTINE BUREAU
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    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6844Nucleic acid amplification reactions
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6876Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
    • C12Q1/6888Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms
    • C12Q1/6895Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms for plants, fungi or algae

Abstract

The invention discloses a kind of ring mediated isothermal amplification judged based on color(LAMP)The molecular detecting method and its primer of technology for detection chestnut phytophthora Heisui River germ, primer sequence is respectively as shown in the ID NO. 6 of SEQ ID NO. 1 to SEQ.Detection architecture of the invention is under 62 °C of isothermys, can be quick, it is convenient, efficiently, it is high special, chestnut phytophthora Heisui River germ is detected with sensitivity, and do not need complex instrument, for the detection of chestnut phytophthora Heisui River germ provides new technology platform, the Site Detection to chestnut phytophthora Heisui River germ can preferably be met, suitable for the inspection and quarantine and the investigation of disease of entry and exit plant and plant product, quick diagnosis and monitoring etc., to preventing chestnut phytophthora Heisui River incoming China of germ significant, simultaneously, the foundation of system of the present invention is also for the detection of other pathogens provides technological guidance and theoretical foundation.

Description

Based on ring mediated isothermal amplification (LAMP) technology for detection chestnut phytophthora Heisui River that color judges Germ
Technical field
The present invention relates to a kind of detection chestnut phytophthora Heisui River germ (Phytophthora lateralis Tucker et Mibrath LAMP primer), and using the molecular detecting method of primer detection chestnut phytophthora Heisui River germ, belong to biological Technical field.
Background technology
Chestnut phytophthora Heisui River germ is one to be used for a kind important crushing phytopathogen, can cause serious chestnut black canker And root, the stem rot of many planting fruit-trees[1].Because the disease causes harm weight, propagation soon, and prevent and treat and eradicate extremely difficult, the cause of disease Bacterium has caused the great attention of many countries such as European Union, takes measures to prevent that its is incoming one after another.In recent years, due to international nursery stock And its allocation and transportation of plant packaging material are increased, the most probably incoming China of the pathogen, once it is incoming, will be to China's agricultural Industry, ecological environment etc. are caused a significant threat.Because there is not a report that chestnut phytophthora Heisui River germ occurs in China, State General Administration for Quality Supervision in List the germ in new revision within 2007《Enter the territory plant quarantine harmful organism register》In.In order to prevent the pathogen incoming China, it is necessary to quickly and accurately detected to it, therefore for chestnut phytophthora Heisui River germ detection We conducted a series of Research.
Chestnut phytophthora Heisui River germ [Phytophthora cambivora (Petri) Buisman] is subordinate to phycomycete circle (Chromista), oomycota (Oomycota), Peronosporales (Peronosporales), pythiaceae (Pythiaceae), Phytophthora (Phytophthora), it is the important phytopathogen of a class, its geographical distribution and host range are very extensive.Germ mycelium Coralliform, produces mycelia to expand body on butter bean culture medium.Sporangium width egg shape, it is sub- it is spherical, fall pyriform or ellipse, spore Capsule is without mastoid process, base portion blunt circle.48~83 × 32~61 μm of sporangium size, average 59~64 × 40~45 μm;Length-width ratio 1.4~ 1.8.Sporangium internal layer goes out, sporangiophore Dan Sheng, and branch or sympodium are not given birth to.Heterothallism.Oogonium is spherical, most of oogonium Outer wall has excipuliform to swell, 30~58 μm of diameter, average 40.5 ± 5.5 μm, 2 μm of the thickness average out to of oogonium wall.Egg spore is expired Device, 35~39 μm of diameter, average 33.8 ± 5.6 μm.Spermary side is given birth to, generally extension, unicellular or double cells, about 60% hero Device is double cells.16.6~29.4 μm of spermary length, average 27.3 μm (double cellular types), 19.3 μm (unicellular type).Germ is most 2 DEG C of low growth temperature, 22~24 DEG C of optimum growth temperature, 32 DEG C of maximum growth temperature[1]
The classification of traditional pathogen, identification are based primarily upon morphological characteristic, Pathogenicity etc., cumbersome, time-consuming, Sensitivity is low, easily by artificially and the factors such as environment are disturbed[2], additionally, also having black using serological method detection chestnut phytophthora The report of edema bacterium[2], but detection time is more long, and detection process is complicated, it is impossible to meet the demand of quick detection.
Loop-mediated isothermal amplification technique (Loop-mediated isothermalamplification, LAMP) is Japan A kind of new nucleic acid amplification technologies that can invent of Rong Yan plants of formula[3], because its simple to operate, quick, specific high, low cost The advantages of, as the new nucleic acid amplification technologies that can substitute regular-PCR.Design 4 kinds of spies in 6 regions that it is directed to target gene Different primer, causes self-loopa strand replacement reaction, 60~65 DEG C of 60~70min of scope in the presence of Bst Large fragment polymerases It is interior, it is accompanied by accessory substance while a large amount of synthesis target dnas --- the magnesium pyrophosphate precipitation of white is produced[4].Due to LAMP amplifications Process relies on identification 6 isolated areas of target sequence, so atopic is very strong, and amplification process is in constant temperature Under carry out, common water-bath or the equipment for having stable thermal source just can meet reacts requirement, and testing cost substantially reduces.
The selection of target gene is one of key factor of LAMP detections.At present, the conventional target gene of Molecular Detection has Internal Transcribed Spacer (Internal transcribed space, ITS), but many scholars think that the target does not have There are enough variant sites to distinguish all of phytophthora kind[5].The modulation GTP (GTP) that the present invention is selected combines egg White gene (Ypt1) is a gene related to proto-oncogene Ras (Rat sarcoma), in yeast, the gene code one The individual gtp binding protein related to Ras.Ypt1 genes include multiple intrones, and noncoding region has enough specificity Site, and its sequence is conservative in kind of inner height, is highly suitable as the Molecular Detection target of phytophthora[6]
Bibliography
1.Erwin,D.C.;Ribeiro,O.K.Phytophthora lateralis.In:Phytophthora diseases worldwide.American Phytopathological Society,St.Paul(US),1996,pp 365-367.
2.Daniells J,Davis D,Peterson R,et al..Goldfinger:not as resistant to Sigatoka/yellow sigatoka as first thought.Infomusa, 1995,4 (1):6.
3.Notomi,T.,Okayama,H.,Masubuchi,H.,Yonekawa,T.,Watanabe,K.,Amino,N., and Hase,T.Loop-mediated isothermal amplification of DNA.Nucleic Acids Research,2000,28:e63-e63.
4.6.Yasuyoshi Mori,Kentaro Nagamine,Norihiro Tomita,and Tsugunori Notomi.Detection of Loop-Mediated Isothermal Amplification Reaction by Turbidity Derived from Magnesium Pyrophosphate Formation.Biochemical and Biophysical Research Communications,2001,289:e150-e154.
5.White,T.J.,Bruns,T.,Lee,S.,and Taylor,J.Amplification and direct sequencing of fungal ribosomal RNA genes for phylogenetics.1990,Pages 315- 322in:PCR Protocols:A Guide to Methods and Applications.M.A.Innis, D.H.Gelfand,J.J.Sninsky,and T.J.White,eds.Academic Press,San Diego,CA.
6.Chen Y,Roxby R.Characterization of a Phytophthora infestans gene involved in vesicle transport.Gene,1996,181(1-2):89-94.
The content of the invention
The technical problems to be solved by the invention are needed for solving the detection method of chestnut phytophthora Heisui River germ in the prior art Cycle is long, waste time and energy, cumbersome, poor specificity and PCR detection techniques need thermal cycler instrument, high cost, it is impossible to quick detection The problem of chestnut phytophthora Heisui River germ, so that there is provided the new molecular detecting method of chestnut phytophthora Heisui River germ, to chestnut phytophthora black canker Bacterium carries out LAMP detections, and the method detection cycle short (only needing 80min), high specificity, sensitivity is high, can visually observe detection knot Fruit and to be not required to expensive instrument cost low, easy to operation.
The selection of modulation gene and the screening of primer are the key factors of LAMP detections.At present, Molecular Detection is extensive Application is the target based on ribosomes transcribed spacer (ITS), but by ITS sequence does not have enough variant sites to distinguish institute Some phytophthora kinds, it is therefore desirable to excavate out new Molecular Detection target.First, search pertinent literature and have chosen tRNA (transhipments RNA) the availability such as EF1 α (translation elongation factor), Ypt1 (GTP binding-protein gene), beta microtubule protein genes Target, then Screening target gene successively, final choice Ypt1 as detection chestnut phytophthora Heisui River germ target gene.Again to Many set primers of target gene design are tested and verified, select the LAMP primer of a set of detection chestnut phytophthora Heisui River germ.
The present invention provide technical scheme be:
The present invention chooses modulation gene, designs and screen the LAMP primer for detecting chestnut phytophthora Heisui River germ, its Including four specific primers F3, B3, FIP, BIP and two rings primer LF and LB, primer sequence respectively as SEQ ID NO.1 extremely Shown in SEQ ID NO.6, table 1 below is specifically shown in.
The chestnut phytophthora Heisui River germ LAMP primer sequence of table 1
Meanwhile, the present invention also puies forward a kind of method using above-mentioned primer detection chestnut phytophthora Heisui River germ altogether, and its process is:Carry The DNA of testing sample is taken as template, LAMP amplified reactions are carried out using described primer, after reaction, visually seen under ordinary light Examine, result judgement is carried out with the color change of hydroxynaphthol blue (hydroxynaphthol blue, HNB);Under ordinary light, sky blue Testing result is represented to detect chestnut phytophthora Heisui River germ in positive (+), i.e. sample, purple represents that testing result is negative (-), Chestnut phytophthora Heisui River germ (Fig. 1) is not detected by sample.
The method of above-mentioned detection chestnut phytophthora Heisui River germ, its LAMP reaction system is:2.5μL 10×ThermoPol Buffer (0.1%Trion-X, 20mM Tris-HCl, 10mM KCl, 10mM (NH4) SO4, pH 8.8), 4 μ L MgSO4 (50mM), 4 μ L glycine betaines (5M), 3.5 μ L dNTPs (10mM), inner primer FIP and BIP (20 μM) each 2 μ L, outer primer F3 and B3 (10 μM) each 0.5 μ L, ring primer LF and LB (10 μM) the μ L Bst archaeal dna polymerases of each 1 μ L, 2 μ L HNB (2.4mM), 1 (8U μ L-1), the μ L of template DNA 2.
The method of above-mentioned detection chestnut phytophthora Heisui River germ, its LAMP response procedures is:62 DEG C, 80min.
Beneficial effect
The present invention compared with prior art, has the advantages that:
(1) practicality is good.Common PCR reaction carries out gel electrophoresis to product and easily causes product diffusion, and this is experiment One main source of chamber contamination;And ethidium bromide (EB) has severe toxicity, can accumulate carcinogenic;Long-term observation uviol lamp also can be to reality The personnel of testing cause a certain degree of injury.And LAMP reactions need to only be carried out in thermostat water bath, reaction passes through HNB after terminating Color change just can direct judged result, whole operation process is simple and easy to apply, it is adaptable to the port of chestnut phytophthora Heisui River germ Quarantine and the quick diagnosis of disease.
(2) constant-temperature amplification.Unlike PCR methods have to thermal cycle, the dependence to thermal cycler instrument is thus broken away from, as long as The thermal source LAMP reactions for having stabilization can just occur, and greatly extend the scope that LAMP is used, and why LAMP can be constant Thermal source under react because with the addition of glycine betaine in LAMP reaction solutions, double-stranded DNA is in the dynamic equilibrium unwind In, amplification is realized in the presence of Bst archaeal dna polymerases.
(3) accuracy is high.Because traditional chestnut phytophthora Heisui River germ detection technique is to be identified according to morphological feature, Time-consuming, sensitivity is low, easily by artificially and the factors such as environment are disturbed;And the present invention is according to chestnut phytophthora Heisui River germ Ypt1 sequences, guard very much in genome of the sequence in the germ of chestnut phytophthora Heisui River, using Bioedit softwares that chestnut phytophthora is black The Ypt1 sequences of edema bacterium and the Ypt1 sequences of other phytophthoras are compared, the specific LAMP of design chestnut phytophthora Heisui River germ Primer.LAMP reactions recognize 6 isolated areas on target sequence by 4 primer specificities, are recognized relative to common PCR primers For 2 isolated areas of target sequence, specificity and sensitivity are all higher.
Under 62 DEG C of isothermys, energy is quick, convenient, efficient, height specifically, is with sensitivity detected for detection architecture of the invention To chestnut phytophthora Heisui River germ, and complex instrument is not needed, for the detection of chestnut phytophthora Heisui River germ provides new technology platform, energy Preferably meet to the Site Detection of chestnut phytophthora Heisui River germ, it is adaptable to chestnut epidemic disease in the inspection and quarantine of enter and leave the border plant and plant product High sensitivity, the quick detection of mould Heisui River germ, while can be used for the investigation of chestnut phytophthora black canker, quick diagnosis and monitoring etc., To preventing chestnut phytophthora Heisui River incoming China of germ significant, meanwhile, the foundation of system of the present invention is also other pathogens Detection provide technological guidance and theoretical foundation.
Brief description of the drawings
Fig. 1 LAMP reactions add the experiment of HNB chromogenic reactions, wherein ,-:Negative reaction is presented purple;+:Positive reaction is in Existing sky blue.
Fig. 2 chestnut phytophthoras Heisui River germ Ypt1 gene nucleic acids sequence and primer location.
The versatility checking of Fig. 3 primers;
Wherein 1:P.cambivora(ATCC 38811);2:P.cambivora(CBS 111329);3:P.cambivora (CBS 114093);4:Negative control.
The inter-species specificity verification of Fig. 4 primers;
Wherein 1:Chestnut phytophthora Heisui River germ P.cambivora, 2-4:Deodar Phytophthora Root Rot P.lateralis, 5,6: Robur sudden death pathogen P.ramorum, 7:Soybean phytophthora P.sojae, 8:Phytophthora infestans P.infestans, 9:Big hero phytophthora P.megasperma,10:Melon phytophthora P.melonis, 11:Phytophthora capsici P.capsici, 12:Clover phytophthora P.medicaginis,13:Phytophthora drechsleri P.drechsleri, 14:Palm mould P.palmivora, 15:Peronophythora Litchii Peronophthora litchi,16:Phytophthora cactorum P.cactorum, 17:Ramie mould P.boehmeriae, 18:Hidden ground phytophthora P.cryptogea,19:Phytophthora nicotianae P.nicotianae, 20:Negative control.
The specificity among genus checking of Fig. 5 primers;
Wherein 1:Chestnut phytophthora Heisui River germ P.cambivora;2:Fusarium graminearum Fusarium graminearum;3:Point Fusariumsp F.oxysporum;4:Layer goes out Fusariumsp F.proliferatum;5:Scouring rush's Fusariumsp F.equiseti;6:Eggplant corruption sickle Spore bacterium F.solani;7:Oat Fusariumsp F.avenaceum;8:Yellow Fusariumsp F.culmorum;9:Tack anthrax-bacilus Colletotrichum truncatum;10:Colletotrichum gloeosporioides Penz C.gloeosporioides;11:More main rod spore bacterium Corynespora cassiicola;12:Soybean charcoal rot bacterium Macrophomina phaseolina;13:Cercospora kikuchii Cercospora kikuchii;14:Rhizoctonia solani Kuhn Rhizoctonia solani;15:Chinese ilex Caionectria bacterium Calonectria ilicicola;16:Fusarium oxysporum Bipolaris maydis;17:Aspergillus oryzae Aspergillus oryzae;18:Pyricularia oryzae Magnaporthe grisea;19:Southern stem canker of soybean Diaporthe phaseolorum var.meridionalis;20:The northern stem canker Diaporthe of soybean phaseolorum var.caulivora;21:Brown stem rot bacterium Phialophora gregata;22:Soybean intends stem point Seed rot disease bacterium Phomopsis longicolla;23:Soybean rest fungus Phakopsora pachyrhiz;24:Negative control.
The sensitivity technique of Fig. 6 chestnut phytophthoras Heisui River germ LAMP detection method;
Wherein 1-8:100ng·μL-1、10ng·μL-1、1ng·μL-1、100pg·μL-1、10pg·μL-1、1pg·μL-1、100fg·μL-1、10fg·μL-1The chestnut Heisui River phytophthora DNA of concentration gradient is used as reaction template;10:Negative control.
Specific embodiment
Embodiment 1:Modulation gene is chosen, the LAMP primer for detecting chestnut phytophthora Heisui River germ is designed and screen, And set up LAMP detection architectures
(1) selection of modulation gene and the design of primer and screening
The selection of modulation gene and the screening of primer are the key factors of LAMP detections.At present, Molecular Detection is extensive Application is the target based on ribosomes transcribed spacer (ITS), but by ITS sequence does not have enough variant sites to distinguish institute Some phytophthora kinds, it is therefore desirable to excavate out new Molecular Detection target.First, search pertinent literature and have chosen tRNA (transhipments RNA) the availability such as EF1 α (translation elongation factor), Ypt1 (GTP binding-protein gene), beta microtubule protein genes Target.By taking target Ypt1 as an example, the Ypt1 gene orders and other phytophthora kinds of chestnut phytophthora Heisui River germ are downloaded from GeneBank Ypt1 gene orders, the Ypt1 gene orders of all downloads are analyzed using Bioedit softwares then, and use PrimerExplore V4 software Photographing On-line primers, choose suitable according to primer length, primer free energy and G/C content etc. Primer is tested, and therefrom versatility is good in screening kind, and inter-species high specificity, specificity among genus are strong, sensitivity primer high.According to Secondary other targets of screening, final choice Ypt1 is used as the target gene (Fig. 2) for detecting chestnut phytophthora Heisui River germ.Again to the target Many set primers of base design carry out test of many times and checking, select that a set of versatility is good, and high specificity, sensitivity is high, can be quick, The accurate primer for detecting chestnut phytophthora Heisui River germ, sequence is as follows:
Detection primer is to ((F3, B3, FIP, BIP, LB))
F3 (positive outer primer):CCTAGGTCCACCATGGCTA(SEQ ID NO.1);
B3 (reverse outer primer):CGTGTCCCACTACAATTCCG(SEQ ID NO.2);
FIP (positive inner primer) (F1C+F2):
TCCAGCTCGATCGTGCGAATTT-TTGACCTCCAGGCTGACG(SEQ ID NO.3);
BIP (reverse inner primer) (B1C+B2):
CGGCAAGACCATCAAGCTCCA-CCAGTTAGCTCCATGAAGCA(SEQ ID NO.4);
LF (positive ring primer):GCACAACAACGAGCACGATAA(SEQ ID NO.5);
LB (reverse ring primer):GATTGTGCGTGCATTCCCG(SEQ ID NO.6).
(2) chestnut phytophthora Heisui River germ LAMP detection architectures are set up
Chestnut phytophthora Heisui River germ LAMP reaction systems:2.5 μ 10 × ThermoPol of L Buffer (0.1%Trion-X, 20mM Tris-HCl, 10mM KCl, 10mM (NH4) SO4, pH 8.8), 4 μ L MgSO4 (50mM), 4 μ L glycine betaines (5M), 3.5 μ L dNTPs (10mM), inner primer FIP and BIP (20 μM) each 2 μ L, outer primer F3 and B3 (10 μM) each 0.5 μ L, ring primer LF and LB (10 μM) the μ L Bst archaeal dna polymerases of each 1 μ L, 2 μ L HNB (2.4mM), 1 (8U μ L-1), 2 μ L template DNAs.By above-mentioned mixing Thing is placed in the PCR reaction tubes of 0.2mL and is slightly vortexed on vortice, is then centrifuged for ensuring not having drop on tube wall.Will Reaction tube is placed in 62 DEG C of isothermal reaction 80min in water-bath.
Embodiment 2:Prepare DNA profiling
The template that the DNA of sample reacts as LAMP is extracted, detailed process is as follows:
(1) prepared by strain culturing and hypha powder
LBA (butter bean culture medium (Zheng little Bo phytophthoras and its agriculture of investigative technique China will be gone to for examination phytophthora bacteria strain Industry publishing house .1997)) on flat board, other bacterial strains go to PDA (potato glucose solid medium (Erwin, D.C.; Ribeiro,O.K.Phytophthora lateralis.In:Phytophthora diseases Worldwide.American Phytopathological Society, St.Paul (US), 1996, pp 365-367)) it is flat On plate, 10 pieces of 2 × 2mm mycelia blocks are cut from colony edge after 25 DEG C of dark culturing 3d, the bacterial strain of phytophthora goes to the training of V8 liquid Base (Zheng little Bo phytophthoras and its investigative technique Chinese agriculture publishing house .1997) is supported, other bacterial strains go to PDB (potato Portugals Grape sugar liquors culture medium) in, 25 DEG C of 5~7d of shaken cultivation are collected by filtration mycelia, and chilled draining grinds to form hypha powder, -20 DEG C Save backup.
(2) extraction of genomic DNA
A small amount of hypha powder, plus 900 μ L 2%CTAB extract solutions and 90 μ L 10%SDS are taken, whirlpool is mixed, in 60 DEG C of water-baths 1h, it is middle to be turned upside down several times per 10min.12000rpm·min-1Centrifugation 10min, take supernatant add isometric phenol/chloroform/ Isoamyl alcohol (25:24:1), overturn and mix, 12000rpmmin-1Centrifugation 10min;Supernatant is transferred in new pipe, add etc. The chloroform of volume, gently overturns and mixes, 12000rpmmin-1Centrifugation 5min.Supernatant is taken to be transferred in new pipe, plus 2 times of volumes Absolute ethyl alcohol and 1/10 volume 3molL-1NaAc (pH 5.2), -20 DEG C staticly settle (>1h).12000rpm·min-1 Centrifugation 10min, incline supernatant, and precipitation is washed 2 times with 70% ethanol, and room temperature is dried.Plus appropriate sterilizing ultra-pure water or TE (pH 8.0) dissolution precipitation (contains 20 μ gml-1RNase), after 37 DEG C for the treatment of 1h, -20 DEG C save backup.
Embodiment 3:The specificity of detection LAMP primer and sensitivity
(1) specific detection
Bacterial strain uses therefor of the present invention and relevant information are shown in Table 2.Using all for examination bacterium in the primer pair table 2 designed by the present invention The genomic DNA of strain carries out LAMP amplified reactions, and the chestnut phytophthora Heisui River germ of the chromogenic reaction result display separate sources of HNB is anti- Guan Juncheng sky blues are answered, is positive findings, negative control reaction tube does not change colour, be still purple (Fig. 3).Chestnut phytophthora Heisui River germ Reaction tube be in sky blue, be positive findings, the reaction tube of other phytophthoras, fungi and negative control is in purple, is cloudy Property result (Fig. 4,5), as a result show that the primer has specificity well, can by chestnut phytophthora Heisui River germ and its allied species and Other correlation kinds are distinguished.
The strains tested of table 2 and LAMP testing results
Note:NJAU represents Agricultural University Of Nanjing;CAIQ represents Chinese Jian Ke institutes;* to indicate and (only provide bacterial strain without bacterial strain DNA)+expression there occurs that LAMP is expanded;- indicate without amplification.
(2) sensitivity technique
The sensitivity of above-mentioned set up detection architecture is determined in the reaction system of 26 μ L, by 10 times of gradient dilutions The genomic DNA of chestnut phytophthora Heisui River germ is (from 100ng μ L-1To 10fg μ L-1) LAMP amplifications are carried out for template, in 62 DEG C 80min is reacted under isothermy.Fig. 6 shows the HNB visualization colour developing figures of sensitivity technique result, when there is LAMP amplifications, Positive reaction is changed into sky blue, and what LAMP amplifications did not occurred is still purple.Testing result shows that lowest detection sensitivity is 100pg·μL-1
<110>P. R. of China Kunshan Entry-exit Inspection and Quarantine Bureau
<120>Based on the ring mediated isothermal amplification that color judges(LAMP)Technology for detection chestnut phytophthora Heisui River germ
<160> 6
<210> 1
<211> 19
<212> DNA
<400> 1
CCTAGGTCCACCATGGCTA 19
<210> 2
<211> 20
<212> DNA
<400> 2
CGTGTCCCACTACAATTCCG 20
<210> 3
<211> 41
<212> DNA
<400> 3
TCCAGCTCGATCGTGCGAATTT-TTGACCTCCAGGCTGACG 40
<210> 4
<211> 42
<212> DNA
<400> 4
CGGCAAGACCATCAAGCTCCA-CCAGTTAGCTCCATGAAGCA 41
<210> 5
<211> 21
<212> DNA
<400> 5
GCACAACAACGAGCACGATAA 21
<210> 6
<211> 19
<212> DNA
<400> 6
GATTGTGCGTGCATTCCCG 19

Claims (4)

1. a kind of LAMP primer for detecting chestnut phytophthora Heisui River germ, it is characterised in that:It include four specific primer F3, B3, FIP, BIP and two rings primer LF and LB, primer sequence is respectively as shown in the ID NO. 6 of SEQ ID NO. 1 to SEQ.
2. it is a kind of based on color judge chestnut phytophthora Heisui River germ LAMP detection method, it is characterised in that:Extract testing sample DNA as template, carry out LAMP amplified reactions using the primer described in claim 1, after reaction, visually seen under ordinary light Examine, result judgement is carried out with the color change of hydroxynaphthol blue;Under ordinary light, sky blue represents that testing result is the positive, i.e. sample In detect chestnut phytophthora Heisui River germ, purple represents that testing result is feminine gender, i.e., chestnut phytophthora Heisui River germ is not detected by sample.
3. LAMP detection method according to claim 2, it is characterised in that:Its LAMP amplification reaction system is:2.5 μL 10×ThermoPol Buffer(0.1% Trion-X, 20 mM Tris-HCl, 10 mM KCl, 10 mM(NH4)SO4, pH 8.8), 4 μ L MgSO4(50 mM), 4 μ L glycine betaines(5 M), 3.5 μ L dNTPs(10 mM), inner primer FIP and BIP (20 μM)Each 2 μ L, outer primer F3 and B3(10 μM)Each 0.5 μ L, ring primer LF and LB(10 μM)Each 1 μ L, 2 μ L HNB (2.4 mM), 1 μ LBstDNA polymerases(8 U·μL-1), the μ L of template DNA 2.
4. LAMP detection method according to claim 3, it is characterised in that:Its LAMP amplified reaction program is:62 DEG C, 80min。
CN201611084928.8A 2016-11-30 2016-11-30 Based on the ring mediated isothermal amplification that color judges(LAMP)Technology for detection chestnut phytophthora Heisui River germ Pending CN106755342A (en)

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