A kind of method of identifying the animal hide
Technical field
The present invention relates to a kind of method of identifying animal species, particularly a kind of molecule labelling method is identified the method for animal skins, relates in particular to the method that a kind of molecule labelling method is identified donkey hide.
Background technology
Donkey-hide gelatin is Chinese traditional Chinese patent drug, be to be that raw material boils and forms by donkey hide, donkey-hide gelatin contains 18 seed amino acids and the multiple trace element that benefits human body, residence removes disease body-building in one, have enriching blood, stop blooding, promote hematopoiesis, enhance immunity power promotes medical health care function widely such as the absorption of calcium and storage, especially its enrich blood, hematopoiesis function be better than similar in, the Western medicine product.
When the purchase donkey hide, need identify at present, prevent to pretend to be donkey hide with horse skin, mule hide and ox-hide etc. to donkey hide.The evaluation of donkey hide is usually used in donkey hide and identifies as Chinese crude drug, general mass spectrum or stratographic analysis, the isodynamic enzymes etc. of adopting are based on the Analysis and Comparison of Protein of Nutrient Mycelia method, but because the difference on protein constitutes between the animal individual, there is certain error in these methods, are difficult to standardization.State-of-the-art method is to use the molecular species authentication method, identifies with molecule labelling method, can detect simultaneously rapidly, accurately and efficiently and identify a large amount of samples.Molecular species is identified the meat evaluation that has been applied in the Food Science, usually differentiate horseflesh, beef, mutton and pork etc. with little satellite method, but the evaluation of donkey meat is report not still, and this is because donkey meat seldom is used for food processing, the having little significance of evaluation.
The inventor has consulted domestic and international lot of documents, proposes to come donkey hide is identified that with cytochrome b gene PCR-RFLP method this authentication method also belongs to blank at present.
Summary of the invention
The purpose of this invention is to provide a kind of method of identifying animal species, a kind of method of molecule labelling method evaluation animal skins is provided especially, a kind of method of molecule labelling method evaluation donkey hide especially is provided, filled up the blank of molecule labelling method evaluation donkey hide.
The present invention has selected mitochondrial cytochrome B gene PCR-RFLP finger-print as appraisal basis, its reason: the one, because the genomic DNA severely degrade in the outmoded dry hide, at the molecule labelling method such as the RAPD of genomic DNA, little satellite etc. are difficult to use.The 2nd, because mitochondrial cytochrome B gene has high conservative property, within species, there is variation hardly, and between species, have the difference of mononucleotide, and can detect easily with the PCR-RFLP method, be a kind of marker gene that species are identified that can be used for.Because cytochrome b gene has the zone of one section high conservative between different plant species, can be used for the cytochrome b gene conservative fragments of a pair of all species of primer amplification detecting, exempted the trouble of using different primers to increase to each species.And because chondriogen has more copy number in cell, even genomic DNA degraded fully, mitochondrial DNA also may also exist, and can increase out with PCR method with comparalive ease.
The objective of the invention is to finish by the following technical programs:
A kind of evaluation animal species is especially identified to may further comprise the steps the method for animal skins: adopt the dna molecular marker method to identify; Described dna molecular marker method is that cytochrome b gene (cytB) PCR-restriction fragment length polymorphism (PCR-RFLP) method is identified;
Described method comprises and makes Fig. 3 or finger-print shown in Figure 4 is identified;
Described preparation method also comprises:
Extract animal skins sample DNA, and as the pcr amplification template;
According to animal skins sample DNA, design and synthesize primer:
B15’-CCATCCAACATCTCAGCATGATGAAA-3’,
B25’-GCCCCTCAGAATGATATTTGTCCTCA-3’;
Obtain cytochrome b gene PCR product with known PCR method amplification, described PCR product is a cytochrome b gene 359bpDNA segment, and its sequence is a nucleotide sequence shown in Figure 5; Described DNA is meant increase at least DNA of cytochrome B (cyt B) gene once of PCR; Described DNA is meant the DNA of pcr amplification secondary cell pigment B gene; Described DNA is meant the DNA of three cytochrome B of pcr amplification (cyt B) gene segment;
With restriction enzyme incising cell pigment B gene PCR product; The described restricted restriction endonuclease of cutting enzyme can be one of Hinf I, Hae III, Alu I, MboI, Taq I and Mse I or its combination;
Electrophoresis PCR product obtains described dna fingerprinting; Described pcr amplification product dna content can be 10-500ng/ul.
Described animal skins as the extracting method of donkey hide, horse skin, ox-hide, mule hide DNA, can be extracted a sample total DNA by known clinical sample DNA extraction kit instructions; The improved dry hide DNA extraction of also available the present invention method is extracted, and the DNA that this extraction obtains can be used as the template that pcr amplification of the present invention is used, and extracts the method for described DNA, may further comprise the steps:
Clip hide sample is removed hair and other attachment of hide outside surface, and remove inside surface pollution layer, hide is sheared tiny particulate;
Take by weighing the skin sample that cuts and place the Eppendorf pipe, wash 2~3 times, inhale and anhydrate and impurity with vibration of deionized water distilled water or piping and druming;
Add digestive juice in described Eppendorf pipe, Proteinase K and SDS spend the night, and described digestive juice is 10mmol/L Tris HCl, and PH can be 8.0,1mmol/LCaCl
2, 4M urea, 0.5%SDS, 0.2mg/ml Proteinase K;
Centrifugal, get supernatant and put into another centrifuge tube;
Add isopyknic phenol: chloroform: isoamylol, volume ratio can be 25: 24: 1, the extracting sample, during described extracting preferably fast, low temperature, be preferably in 5 minutes; Can operate on ice;
Centrifugal, draw supernatant;
Add isopyknic chloroform: isoamylol, volume ratio can be 24: 1, the extracting sample, during described extracting preferably fast, low temperature, be preferably in 5 minutes; Can operate on ice;
Centrifugal, draw supernatant;
Add the NaAc solution of 3mol/L, add an amount of absolute ethyl alcohol behind the mixing, mixing placed-5 ℃~-20 ℃ more than 30 minutes.
Centrifugal, abandoning supernatant;
Add 70% ethanol, centrifugal, supernatant discarded;
Drying is dissolved in the sediment of drying in an amount of pure water; 0-10 ℃ of standby or-20 ℃ of long preservation of temporary transient preservation get extract.
The extracting method of described animal skins DNA, also comprise quality with the DNA of conventional biological method method Detection and Extraction, especially use the quality of the DNA of 1.0% agarose gel electrophoresis Detection and Extraction, use λ DNA/Hind III Marker (mark) as molecular weight standard, the point sample electrophoresis detection; With observing under the known uviol lamp or taking pictures with gel imaging system; Also available DNA micro quantitative determination instrument detects DNA concentration, and described animal skins DNA electrophoresis pattern is shown in Figure 1;
With the DNA that is extracted is template, carry out PCR design and synthetic primer, amplification acquisition cytochrome b gene fragment, promptly obtain the segment of described DNA, its method can be: inquire about the mitochondrial genomes dna sequence dna of animals such as donkey, ox, horse, mule from GenBank, intercepting cytochrome b gene sequence wherein; And according to the cytochrome b gene sequence that intercepts, with the synthetic one couple of PCR primers of known method design;
For guaranteeing that a pair of primer can amplify the cytochrome b gene fragment of all animals, also can adopt following method: the PCR primer designs according to conserved sequence, at first use known software, as Clustal W software, the zooblast pigment B gene order that will identify is carried out the multisequencing comparison and is aimed at (align), find between conserved region, adopt the PCR primer-design software, as Oligo 6.0 PCR primer-design softwares, design primer in this is interval, press the known method synthetic primer, this primer sequence is as follows:
B15’-CCATCCAACATCTCAGCATGATGAAA-3’
B25’-GCCCCTCAGAATGATATTTGTCCTCA-3’
Described cytochrome b gene fragment (Cyt B) pcr amplification method may further comprise the steps:
Can be through pcr amplification condition optimizing repeatedly, determine that suitable pcr amplification condition is: each PCR reaction volume contains template DNA, 10mM Tris-HCl (pH8.3), 50mM KCl, 4 kinds of dNTPs of 0.2mM, 2.0mM MgCl2 and 2.0 Taq of unit archaeal dna polymerases;
In pcr amplification reaction condition amplifying cells pigment B genetic fragment routinely; Produce the dna fragmentation of the described 359bp of Fig. 5 behind the described pcr amplification, i.e. cytochrome b gene;
In order to improve specificity, avoid producing non-specific amplification, can adopt known warm start mode, or directly adopt the Taq archaeal dna polymerase of warm start type;
Because the outmoded degree varies sample of each hide sample, the DNA concentration difference of extraction is very big, amplification for the first time may bar have have by force a little less than, have have non-specific amplification or background is higher; It is quantitative to carry out PCR, promptly according to the result of the pcr amplification first time, determine the quantity of To Template DNA in the DNA sample, adjust the template amount of pcr amplification for the second time more in view of the above, also can repeatedly adjust, carry out more times pcr amplification, obtain the consistent amplified band of strength ratio, can guarantee after further enzyme is cut, to obtain restriction enzyme mapping clearly, thereby obtain judging that the identification rate of sample institute species is 100%.
The restriction fragment length polymorphism of described DNA (Restriction fragment lengthpolymorphism, RFLP) method may further comprise the steps:
PCR product with restriction enzyme incising cell pigment B genetic fragment; The restriction enzyme of the described pcr amplification product of described Fig. 5 provides a large amount of experiments, filters out the restriction enzyme that can be used for differentiating, as Hinf I, Hae III, Alu I, MboI, Taq I and Mse I etc., preferably restriction endonuclease is HinfI and Hae III;
Described reaction volume contains damping fluid 10x buffer R+, restriction endonuclease and PCR product D NA.Can cut reaction conditions by known enzyme carries out; Get the PCR-RFLP product;
Described PCR-RFLP product can obtain collection of illustrative plates with the known gel electrophoresis method; Described collection of illustrative plates can be analyzed the RFLP band spectrum that produces, and then judge sample institute species according to band spectrum with gel imaging analysis system scan input computing machine;
Experiment showed, only needs just can identify all species with 2 kinds of restriction endonuclease Hinf I and Hae III in detection.
Described preparation method detects and the identification experiment product after comprising that also reaction finishes; The quality of the DNA of available conventional biological method method Detection and Extraction, especially use the quality of the DNA of 1.0% agarose gel electrophoresis Detection and Extraction, with λ DNA/Hind III Marker as molecular weight standard, the point sample electrophoresis detection, and with observing under the known uviol lamp or taking pictures with gel imaging system; Also available DNA micro quantitative determination instrument detects DNA concentration.As: the animal skins DNA that extracts detected or purifying after detect, described purifying mode is an electrophoresis, sees shown in Figure 1; The PCR product is detected and discriminating, and described purifying, the mode of evaluation are electrophoresis, see shown in Figure 2; PCR product enzyme is cut the back detection and differentiated that described purifying, the mode of evaluation are electrophoresis, see Fig. 3, collection of illustrative plates shown in Figure 4.
Described preparation method also comprises with the animal skins dna direct order-checking of described extraction or with the method that checks order behind Fig. 5 gene fragment clone and identifying.
If high to the accuracy requirement of differentiating, perhaps other sample extremely, or carry out PCR-RFLP with 2 kinds of restriction endonuclease HinfI and Hae III and analyze can not differentiate the time can adopt direct order-checking or the method that checks order again behind this gene fragment clone is identified;
Described direct order-checking: the pcr amplification product of described sample directly can be checked order, or with checking order behind the conventional gel electrophoresis purifying; Also available conventional sequenator carries out as automatic sequencer;
Order-checking again behind the described gene fragment clone: the method that can adopt conventional clone, order-checking; Also can be: the PCR product is mixed with plasmid vector pGEM-T (available from Shanghai bio-engineering corporation), add the T4DNA ligase, with the connection product that obtains with efficiently express the attitude Escherichia coli and mix, with bacterium liquid shop LB agar plate, described agar plate contains ampicillin, 0.5mM IPTG, 40mg/ml X-Gal, and heat in advance.With dull and stereotyped overnight incubation, according to blue hickie screening recon.Recon (hickie) bacterium colony is picked out access to be contained in the LB nutrient culture media of ampicillin, shaken cultivation is spent the night, and known alkaline cracking process extracts plasmid DNA, with EcoR I digested plasmid DNA, agarose gel electrophoresis reclaims DNA and inserts fragment, again with described restriction endonuclease digestion; Carry out rflp analysis, after the 359bp fragment of definite section type cytochrome b gene that is obtained, check order with dideoxy chain termination;
The cytochrome b gene sequence of animals such as the sequence measured and the donkey among the GenBank, horse, ox is compared, and its gene order is consistent with which kind of animal, and which kind of animal this sample just belongs to.
This method is as discrimination method, except generally being used to differentiate animal species, also be used to differentiate the animal hide, especially the donkey hide that has higher medical value, also can be used as the judging standard of production quality control, can prevent to pretend to be donkey hide, as the donkey hide of purchase, the donkey hide in the raw material processing procedure, the judging standard of the donkey hide that uses of feeding intake with horse skin, mule hide and ox-hide etc., when especially conduct is used to make the raw material of medicine, use dna molecular of the present invention to identify the quality control standard of donkey hide.
A kind of application of dna fingerprinting aspect the evaluation of donkey hide Chinese crude drug of identifying donkey hide describedly is accredited as the finger-print that the cytochrome b gene PCR-restriction fragment length polymorphism finger-print preparation method makes donkey hide identified.
Discrimination method of the present invention, the DNA that the different animals dry hide is extracted is consistent, only has the difference (see figure 1) of concentration, and its PCR product D NA collection of illustrative plates also is consistent (see figure 2), but the DNA collection of illustrative plates after enzyme is cut can come the different animals difference, thereby identifies the donkey hide (see figure 3).
Animal DNA standard molecular weight of the present invention is to reach known dna molecular quantity measuring method and to obtain from known references and Genebank.
The present invention has the following advantages:
1, animal skins DNA extraction method of the present invention, pcr amplification has obtained the fragment of the 359bp of cytochrome b gene conservative region, by the digestion with restriction enzyme that filters out, obtained dna fingerprinting with agarose gel electrophoresis, judge sample institute species etc. according to the dna fingerprinting that obtains, proved that this method can guarantee that the skin sample identifies that accuracy rate is 100%.
2, because the similarity of different animals cytochrome b gene conservative region fragment, therefore, the present invention is used to differentiate the animal hide, especially has the animal hide of higher medical value, can prevent effectively the phenomenon of pretending to be with other animal skins from can provide reliable assurance for products material.As prevent that ox-hide, horse skin from pretending to be donkey hide, for the ass-hide glue certified products provides reliable credit foundation.Therefore the present invention not only is used for the donkey-hide gelatin raw material, and the present invention also can be used for identifying the discriminating of other animal species.
3, verified the validity of this authentication method through Blind Test (blind test).
4, the key method difficult point of this research has 2 points: the one, and the extraction of hide sample DNA, it is too outmoded or rot DNA severely degrade, the problem that is difficult to extract to overcome some hide; Two are to locate the molecule labelling method that is suitable for distinguishing donkey, horse, ox, and have enough sensitivity, can correctly detect the hide sample, and no matter this hide sample is fresh hide, still outmoded dry hide or the hide that rots.The inventor proposes donkey hide to be identified with cytochrome B (cyt B) gene pyramiding polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) fingerprint spectrum method identification rate is 100%.
5, the present invention also carries out qualitative analysis to the quality (outmoded or rotten degree) that detects leather, and the check and the handle that are applied to raw material are shut, to guarantee the quality of product.Because leather is when outmoded in various degree or rotten, the degraded that DNA can be in various degree the difference of different sharpness can occur, even can't measure in collection of illustrative plates.
6, the present invention identifies maturation, uses feasible; Method is easy, is easy to grasp, and can promptly detect a large amount of samples simultaneously; The method good stability is to the detection rate of accuracy reached 100% of donkey hide.Except that differentiating the donkey hide kind, also can distinguish the quality of donkey hide, the skin sample that rots and but do not have dna fingerprinting to show should be got rid of outside the raw material of donkey-hide gelatin.
7, the present invention differentiates the donkey-hide gelatin raw material, belongs to initiative both at home and abroad.It can be widely applied in the kind discriminating of animal tcm material.
8, this method can be used as the quality standard that donkey-hide gelatin manufacturer raw material is purchased and fed intake, and can be used as the foundation of including pharmacopeia in, improves the donkey-hide gelatin quality of production, promotes the raising of the existing modernization level of donkey-hide gelatin.
Description of drawings
The dna content collection of illustrative plates that Fig. 1 extracts from different animal dry hides for the present invention.
Wherein, M: represent λ DNA/Hind III Marker molecular weight standard;
Numeral 1,7,10,17: for the epiderm-like numbering, different animals is unanimity as a result;
N and L contrast: the DNA that representative is extracted from fresh beef and donkey meat.
Fig. 2 is that the present invention is from different zooblast pigment B gene 359bp fragment PCR amplified production collection of illustrative plates
Wherein, M: represent Gene Ruler 100bp DNA Ladder (100bp dna molecular amount standard)
Numeral 1~10 is represented the detected sample Article Number, symbol sample O: the mule skin, and J: the hinny skin, N: beef, L: donkey meat, different animals is unanimity as a result;
-1: blank.
Fig. 3 cuts finger-print for different animals HinfI of the present invention and Hae III enzyme
Wherein, M represents molecular weight standard;
N1, N2, N3 represent ox, and M1, M2 represent horse, and L1, L2 represent donkey, and J1, J2 represent hinny (Jue Hinnies).
Fig. 4 differentiates the enzyme of species for Blind Test of the present invention and cuts finger-print
Wherein, M: be molecular weight standard;
1~No. 17 is sample, and Niu is known beef sample contrast, and Lv is known donkey meat sample contrast; The known horse skin sample contrast of Ma.
Fig. 5 is cytochrome b gene pcr amplification product 359bpDNA of the present invention sequence table
Wherein:
Marker is a standard molecular weight; Donkey represents donkey; Horse represents horse;
Cattle represents ox; Pig represents pig.
Embodiment
Embodiment 1
Identify the preparation method of the dna fingerprinting of donkey hide
Material:
The skin sample provides donkey hide, ox-hide, horse skin, mule hide sample by the Donga donkey-hide gelatin, and every kind of animal is got the skin sample of 20 individualities.
Molecular biology reagent:
Proteinase K, RNA enzyme, dna ligase, Hinf I, Hae III, Alu I, MboI, TaqI, Mse I, EcoR I, Bam HI, Hind III restriction endonuclease, all adopt Shanghai to give birth to worker bio-engineering corporation product, the Taq archaeal dna polymerase is a Promega company product, and other general reagents are homemade AR level reagent.
Experimental facilities and instrument:
The PCR instrument, agarose gel electrophoresis groove and electrophoresis apparatus, gel imaging system, constant temperature shaking table, thermostat water bath, supercentrifuge, and other molecular biology experiment common instrument.
Preparation process:
1, DNA extraction
Clip hide sample is removed the pollution layer of outside surface attachment, inside surface, cuts into tiny particulate; Get 25 milligrams of microparticle skin samples and place the Eppendorf pipe, each sample is established 3 and is repeated sample; The digestive juice, 0.5%SDS, the 0.2mg/ml Proteinase K that in each Eppendorf pipe, add 1mL; 54 ℃ were spent the night 10 hours; Described digestive juice comprises 10mmol/L Tris HCl (pH8.3), 1mmol/LCaCl
2, 4M urea; Centrifugal 5 minutes of described Eppendorf pipe 8000rpm gets the 1mL supernatant, puts into a centrifuge tube; Add phenol in the centrifuge tube: chloroform: isoamylol mixed liquor extracting sample with supernatant isopyknic 25: 24: 1 (volume ratio); Centrifugal 5 minutes of described extracting sample 8000rpm draws 4/5 volume supernatant; The chloroform that adds isopyknic 24: 1 (volume ratio): isoamylol mixed liquor extracting sample; Centrifugal 5 minutes of described extracting sample 8000rpm draws 4/5 volume supernatant; Add 1/10 volume 3mol/L NaAc solution, add 2 times of volume absolute ethyl alcohols behind the mixing, mixing, place-20 ℃ 30 minutes.Then, centrifugal 10 minutes of 12000rpm, abandoning supernatant; Add 1mL70% ethanol, centrifugal 3 minutes of 12000rpm, abandoning supernatant; Vacuum drying is dissolved in the 100ul pure water with the sediment of drying; 4 ℃ of preservations are standby.With the quality of the DNA of 1.0% agarose gel electrophoresis Detection and Extraction, with λ DNA/Hind III Marker as molecular weight standard, point sample amount 5ul, sample-loading buffer 2ul, 30 minutes time; Take pictures with gel imaging system and to see Fig. 1, detect DNA concentration, be used for pcr amplification with conventional DNA micro quantitative determination instrument.
Test results and analysis:
DNA extraction by animal donkey, horse, ox, mule dry hide, obtain the DNA of hide sample, it is better that electrophoresis detection shows that most of skin sample obtains the DNA quality, can satisfy the needs of follow-up work, small part skin sample dna degradation is more serious, as long as but can amplify the target gene fragment.The advantage of mitochondrial cytochrome B genetic fragment PCR-RFLP method just is to have higher sensitivity, can overcome the problem of sample DNA severely degrade.Even genomic DNA is degraded fully, when not coming out or getting the wrong sow by the ear based on the method amplification of genomic DNA with little satellite method or RAPD method etc., and agarose gel electrophoresis and DNA quantitative instrument all can not detect under the situation that DNA exists, also can amplify mitochondrial cytochrome B genetic fragment, thereby detect sample institute species.
2, PCR design of primers and synthetic, cytochrome b gene (Cyt B) 359bp fragment PCR amplification
From GenBank, inquire about the mitochondrial genomes dna sequence dna of donkey, ox, horse animal, intercepting cytochrome b gene sequence wherein, adopt Oligo 6.0 PCR primer-design softwares to design and synthesize primer according to sequence, can amplify the fragment of cytochrome b gene 359bp with described primer amplification, primer sequence is as follows:
B15’-CCATCCAACATCTCAGCATGATGAAA-3’,
B25’-GCCCCTCAGAATGATATTTGTCCTCA-3’
Primer concentration is 5.0umol/L, and the tubule that is packed as 50ul is preserved;
The pcr amplification condition is: each PCR reaction volume is 50ul, contains 10x Taq enzyme buffer liquid 5ul, 25mM MgCl
2Solution 4ul, 10mM mixing dNTPs 1ul, 5.0uM 5 '-primer B11ul, 5.0uM 3 '-primer B2l ul, 10ng/ul template DNA 5ul, 5U/ul Taq archaeal dna polymerase 0.4ul, surplus sterilization deionization distilled water;
The PCR reaction conditions is: 94 ℃ of pre-sex change, 2min; 94 ℃ of 30 circulations, 30s; 55 ℃, 30s; 72 ℃, 40s; Extend 72 ℃, 2min.
Amplified production is detected with 1.5% agarose gel electrophoresis in the reaction back, and described PCR produces the dna fragmentation of 359bp shown in Figure 5.
Test results and analysis:
Pcr amplification has obtained the fragment of the 359bp of cytochrome b gene conservative region, obtains the consistent amplified band of strength ratio and sees Fig. 2.
When extracting DNA in the above-mentioned experiment, each sample is done 6 repetitions.The DNA that extracts is merged dissolving, to improve the concentration of template DNA.During pcr amplification, each sample is done 12 repetitions, and will there be the pcr amplification product of amplified band to merge, use isopyknic phenol: chloroform: isoamylol (25: 24: 1) extracting once adds the 10M ammonium acetate and the two volumes absolute ethyl alcohol of 1/4 volume, and mixing is placed on-20 degrees centigrade of half an hour, centrifugal 15 minutes of 12000rpm, carefully pour out supernatant, will precipitate once, will precipitate with the dissolving of 50ul sterilization deionization distilled water with the washing of 500ul 70% ethanol.After like this PCR product being concentrated again enzyme cut, can guarantee to obtain finger-print more clearly after next step enzyme is cut.
3, the restriction fragment length polymorphism (Restriction fragment lengthpolymorphism, RFLP) analyze:
Described each pcr amplification product is used Hinf I, Hae III, Alu I, MboI, Taq I and Mse I, Hinf I and Hae III digestion with restriction enzyme respectively.Reaction volume 50ul, the required sample size of enough twice electrophoresis wherein contains 5ul damping fluid (10x buffer R+), the described restriction endonuclease of 2ul, with 43ul PCR product D NA, mixing and centrifugal back 37 ℃ of digestion were spent the night 12 hours, handled 25 minutes with the deactivation restriction endonuclease for 80 ℃.
Described PCR-RFLP product 3% agarose gel electrophoresis, and develop the color with ethidium bromide (EB), the electrophoresis pattern that obtains, and with gel imaging analysis system scan input computing machine, analyze the RFLP band spectrum that produces, filtering out in detection only needs just can identify all species with Hinf I and 2 kinds of restriction endonucleases of Hae III.
Test results and analysis:
This experiment screening can be judged the restriction endonuclease of sample institute species according to the dna fingerprinting that is obtained.The standard one of screening restriction endonuclease is between the species evident difference to be arranged and not there are differences between the individuality within the species, to guarantee that the accuracy that detects is 100%; The 2nd, easy, in this detection, only need just can identify all species with 2 kinds of restriction endonucleases.Through a large amount of tests, determine that only restriction endonuclease is Hinf I and Hae III, obtain the dna fingerprinting of Fig. 3 of difference species.
The explanation of Fig. 3 collection of illustrative plates: this method can be distinguished donkey, Ma Heniu.After extracting the DNA of skin sample, the cytochrome b gene 359bp fragment that pcr amplification produces uses two kinds of different enzymes to cut, and produces different band spectrums.Wherein, Hinf I enzyme is cut and horse can be distinguished, but the bands of a spectrum of ox and donkey are identical, and M1, M2 are horse (molecular weight is 234bp), other be donkey or ox.Wherein weak band is the PCR product of complete degestion not above the master tape, can judge on molecular weight, does not influence the judgement of following two band spectrums.
Wherein, Hae III enzyme is cut and ox (molecular weight is 258bp) can be distinguished, but the bands of a spectrum of horse and donkey are similar, and N1, N2, N3 are ox, other be donkey or horse.
This method assurance skin sample identifies that accuracy rate is 100%.
6, dna clone and order-checking
Identify with direct order-checking or with the method that checks order again behind this gene fragment clone.
Described direct order-checking is: directly check order after the pcr amplification product of each sample is used the agarose gel electrophoresis purifying, order-checking can be carried out with conventional automatic sequencer.
Check order again behind the described gene fragment clone and be: 20ng PCR product is mixed with 50ng plasmid vector pGEM-T (described plasmid vector is available from Shanghai bio-engineering corporation), adding the 3U dna ligase spends the night 4 ℃ of connections, 2ul is connected product to be mixed with the efficient competence Escherichia coli of 100ul, 0 ℃ of ice bath 2min, bacterium liquid is all spread the LB agar plate, and (described agar plate contains the 100mg/ml ampicillin, 0.5mM IPTG, 40mg/ml X-Gal, and heat in advance to 37 ℃).Flat board 37 ℃ of overnight incubation, is screened recon according to blue hickie.Recon (hickie) bacterium colony is picked out access 5ml to be contained in the LB nutrient culture media of 50mg/ml ampicillin, 37 ℃ of shaken cultivation are spent the night, conventional alkaline bleach liquor cleavage method is extracted plasmid DNA, cut the 1ug plasmid DNA with 10U EcoR I enzyme, 1.2% agarose gel electrophoresis reclaims and inserts fragment, again with restriction endonuclease commonly used, as Hae III and Hinf I restriction endonuclease digestion carrying out rflp analysis, after the 359bp fragment of definite section type cytochrome b gene that is obtained, check order with dideoxy chain termination.The cytochrome b gene sequence of donkey among sequence and the GenBank, horse, ox is compared, and its gene order is consistent with which kind of animal, and which kind of animal this sample just belongs to.This method identification rate is 100%.
Embodiment 2
A kind of application of dna fingerprinting aspect the evaluation of donkey hide Chinese crude drug of identifying donkey hide describedly is accredited as the finger-print that the cytochrome b gene PCR-restriction fragment length polymorphism finger-print preparation method makes donkey hide identified.
1) inventor is to twice provides before and after the Donga donkey-hide gelatin company 17 skin samples that belong to donkey, horse, ox, pig species individuality respectively, by manufacturer numbering but do not indicate skin sample institute species, carry out the validity of Blind Test (blindtest) with verification method, assay method is with above-mentioned embodiment, result such as Fig. 4 have proved that this method can correctly judge hide institute species.
Test results and analysis:
Can judge that according to Hinf I restriction enzyme mapping among Fig. 44,5,7,8,9, No. 10 is horse, other be donkey or ox.Can judge 1,2,11, No. 12 for ox according to Hae III restriction enzyme mapping among the figure, other are donkey or horse.
Comprehensive above analysis result can judge 1,2,11, No. 12 be ox, 4,5,7,8,9, No. 10 is horse, 3,13,15,16, No. 17 be donkey (359bp).
It is serious that No. 6 and No. 14 sample horse skins rot, and do not amplify band, can't judge.Among the figure 5,9,11, No. 13 band spectrums a little less than, but do not influence judgement.
Above-mentioned 19 samples have been carried out repeated experiments 6 times, all shown identical result, fidelity factor reaches 100%, and illustration method has good repeatability and stability sees the following form:
Table: the test result and the fidelity factor of Blind Test sample repeated experiments
Sample | Lv | ?Nu | ?1 | ?2 | ?3 | ?4 | ?5 | ?6 | ?7 | ?8 | ?9 | ?10 | ?11 | ?12 | ?13 | ?14 | ?15 | ?16 | ?17 |
Multiplicity | 6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 |
Positive number of times | 6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?0 | 6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?6 | ?0 | ?6 | ?6 | ?6 |
Fidelity factor % | 100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 | ?100 |
2) the different places of production donkey hide sample collecting and detection have been carried out.
Purpose is that accuracy, stability and the reappearance to method verified, gathers 126 in donkey hide sample altogether, and 40 of horse skins, 26 of mule hides, 33 on ox-hide repeat time experiment to each sample 10, all can obtain identical result, fidelity factor 100%.It is clear that all donkey hide sample amplification and enzyme are cut band spectrum, judge accurate, accuracy rate 100%.The collection of illustrative plates of this method preparation is not subjected to the influence of geographical population, and the kind inner height is true and consistent, has good stability.Extremely other sample that is provided is owing to rot seriously to be difficult to distinguish.See Table 2
Table 2: to domestic different donkey hides place of production test result of samples
Gather ground | Donkey hide | Horse skin | Mule hide | Ox-hide | Add up to |
Xinjiang | ????20 | ????3 | ????3 | | ????26 |
The Inner Mongol | ????8 | ????4 | ????2 | | ????14 |
Gansu | ????11 | ????3 | ????2 | | ????16 |
Qinghai | ????10 | ????4 | ????1 | | ????15 |
Shanxi | ????9 | ????2 | ????2 | ????4 | ????17 |
Henan | ????15 | ????3 | ????3 | ????3 | ????24 |
Hebei | ????16 | ????5 | ????2 | ????6 | ????29 |
Shandong | ????37 | ????16 | ????11 | ????20 | ????84 |
Add up to | ????126 | ????10 | ????16 | ????33 | ????225 |
Detect accuracy rate (%) | ????100 | ????97.5 | ????100 | ????93.9 | ????/ |