CN105296640B - SNP marker for tracing to the source and its application on No. 6 chromosomes of one pig - Google Patents

SNP marker for tracing to the source and its application on No. 6 chromosomes of one pig Download PDF

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CN105296640B
CN105296640B CN201510785895.9A CN201510785895A CN105296640B CN 105296640 B CN105296640 B CN 105296640B CN 201510785895 A CN201510785895 A CN 201510785895A CN 105296640 B CN105296640 B CN 105296640B
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吴潇
唐雪明
武国干
吕贝贝
蒋玮
王金斌
李鹏
白蓝
刘华
赵凯
王荣谈
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Shanghai Academy of Agricultural Sciences
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Abstract

The invention discloses the SNP marker for being used to trace to the source on No. 6 chromosomes of a pig and its applications, the SNP marker is obtained by ncbi database sequence alignment, it is identified by Ecol30I restriction enzymes, total 578bp, there are one bases to replace at 232nd bit base, for 232C or 232T, sequence is as shown in SEQ ID NO.1.By analyzing SNP marker in the distribution situation for testing group's allelic in the experiment group including 10 pig varieties or strain, it was found that gene frequency of the SNP marker of the present invention in different kinds or strain is close, rich polymorphism, gene frequency distributional difference is small between kind or strain, and heterozygosity is both greater than 0.3, which can be used as DNA source tracing of pork products.

Description

SNP marker for tracing to the source and its application on No. 6 chromosomes of one pig
Technical field
The invention belongs to field of food safety, and in particular on No. 6 chromosomes of a pig for the SNP marker traced to the source and It is applied.
Background technology
With the development of society, the link in agri-food supply chains is being continuously increased, from farm, pasture to food enterprise plus Work, packaging, storage, transport and sale, there are the security risk of food, food-safety problem often has the links of food supply Occur.Therefore need to carry out meat products can tracing management, establish the retrospect system of links from the place of production to dining table, to The information that accurate and detailed article is provided for consumer is conducive to operator and finds in time present in each link Hidden danger.Since the food security crisis of mid-term the 1990s, the retrospect of meat product has been used as a kind of safety Control measure are paid much attention to by multiple countries of the world.Meat product traceability system strengthens government department to meat product quality The ability to supervise of safety, therefore many countries establish meat product traceability system one after another and exist to reduce in meat product quality safety Risk.
Meat product tracing technology has label tracing technology, isotopic traceability technology, mineral element fingerprint tracing technology, organic Object tracing technology iris feature technology and DNA marker tracing technology (or DNA tracing technologies) etc., wherein DNA tracing technologies because Detection means is simple, quickly, the features such as being difficult to forge become the widely applied quick tracing technology in countries in the world.With other labels Method is compared, and DNA marker is put into superiority with peculiar:It directly occurs with DNA form, in each tissue, each of organism Developmental stage can detect, and not influenced by environmental factor, and marker number is more, and organism whole gene group is spread.
SNP marker refers to the variation of single nucleotide acid on the same site of genome, normally behaves as two allele, suitable High throughput automated analysis, so identifying molecular labeling of greatest concern as animal identification.
But the SNP marker traced to the source for meat product is different from general SNP marker, for single SNP marker, it must Must at least have following characteristics:(1) degree of variation is high, close in kind or strain allelic frequency;(2) equipotential base between kind Because distribution frequency difference is small;(3) heterozygosity is more than or equal to 0.3.
In long-term breeding work, researcher has accumulated a large amount of SNP marker, since single SNP labels of tracing to the source are nothings Method is completed to trace to the source, and could realize and traces to the source therefore, it is necessary to one group of mutually independent SNP marker.With existing 13 known SNP points Son label is as label combination of tracing to the source, in the pig groups introduced by height selection, when being traced to the source using the group echo, and meeting There is the case where certain individuals cannot distinguish between.
In addition, in long-term breeding work, a large amount of SNP marker of accumulation often integrated distribution in certain chromosomes On, and other part chromosome, such as No. 5, No. 6, No. 8, No. 14, No. 15 and No. 18 chromosome etc. then lack SNP marker, are easy to lead Cause cascade phenomenon occur between molecular labeling, cannot be independent mutually between molecular labeling, the detection range for experiment of tracing to the source is reduced, is caused Practical detectable range is less than expected detectable range.Therefore, the requirement that DNA traces to the source is carried out to pork product in order to meet, needed The SNP marker for tracing to the source on other chromosomes is developed, trace to the source detection range and accuracy are improved.
Invention content
The purpose of the present invention is to provide the SNP marker for being used to trace to the source on No. 6 chromosomes of a pig and its applications, can To be widely used in DNA source tracing of pork products and its detection, the safety for being especially used for pork product is traced to the source, perfect existing mark Note combination, improves accuracy in detection of tracing to the source, expands the scale of tracing to the source.
To achieve the above object, technical scheme is as follows:
SNP marker on No. 6 chromosomes of pig for tracing to the source, the DNA sequence dna such as SEQ ID of the SNP marker Shown in NO.1, total 578bp, there are one bases to replace at the 232nd bit base, is 232C or 232T.
Further, the SNP marker is identified by Ecol30I restriction enzymes.
The SNP marker is obtained by ncbi database sequence alignment, and including 10 pig varieties or In the experiment group (amounting to 245 individuals) of strain, the SNP marker is analyzed in the distribution feelings for testing group's allelic Condition finds that gene frequency of the molecular labeling in different kinds and strain is close, rich polymorphism, kind or strain Between gene frequency distributional difference it is small, the preliminary judgement SNP marker can be used as DNA source tracing of pork products.
The preparation method of the SNP marker traced to the source for pork DNA, using PCR-Ecol30I-RFLP methods It carries out, includes the following steps:
(1) the DNA sequence dna information that No. 6 chromosomes of pig are searched on NCBI, designs forward and reverse primer
Detach the DNA fragmentation of No. 6 chromosome of pig;
(2) sequence alignment is carried out online using ncbi database, there are the sites that base substitutes for searching;
(3) foundation of PCR-Ecol30I-RFLP detection methods and the detection in replacement site;
(4) the ear tissue sample for acquiring 10 kinds and strain, amounts to 245 individuals;
(5) detection SNP marker is in the distribution of experiment group, statistical analysis, and further whether verification experimental verification is applicable in In pork product is traced to the source.
Wherein, in the method for above-mentioned acquisition SNP marker, on described separation No. 6 chromosomes of pig DNA fragmentation just, Reverse primer sequences are as follows:
Forward primer:5 '-CTTTACCGTTCTGCCCTTTC-3 ' (as shown in SEQ ID NO.2);
Reverse primer:5 '-TCCTCTGCCTGCCTTTGA-3 ' (as shown in SEQ ID NO.3).
During DNA traces to the source, the site as soon as often increase is traced to the source can further expand the number of detection sample, accurately Property also with regard to higher, ideal SNP site should be generally evenly distributed on the different chromosome of pig, and in existing SNP site lack Label of tracing to the source on weary No. 6 chromosome.
The present invention detects the existing SNP marker on No. 6 chromosomes of pig by ncbi database sequence alignment, In experiment group including 10 pig varieties or strain, distribution of the SNP marker in experiment group allelic is analyzed Situation finds that gene frequency of the molecular labeling in different kinds or strain is close, rich polymorphism, kind or product Gene frequency distributional difference is small between system, and heterozygosity is both greater than 0.3, and the preliminary judgement SNP marker can be used as pork production During product DNA traces to the source and the safety of pork product is traced to the source.
It is combined to improve existing SNP marker, improves the accuracy in detection for experiment of tracing to the source, expand scale of tracing to the source, it will The Novel SNP molecular marker site that the present invention obtains on No. 6 chromosomes of pig and other existing published SNP marker sites It is combined together and (amounts to 14 SNP sites) and carry out experiment of tracing to the source.
The present invention increases market pig source, 300 from different pig farms is picked altogether in slaughterhouse in experiment of tracing to the source Individual selects 100 individuals at random from 300 individuals, detects the genotype of 14 SNP sites in 100 individuals, statistics The genotype results of each individual find that 100 individuals possess respectively different genotype, can realize individual differentiation;Meanwhile 20 parts of muscle samples of picking in this 100 individuals at random, the genotype in 14 SNP marker sites of same detection statistics, so 100 individual genotype of heel are compared, and discovery can be found completely the same with 20 parts of muscle samples genotype Individual finds the source individual of 20 parts of pig muscles by tracing to the source in 100 individuals, therefore, it is determined that the SNP points of the present invention Son label can be used for pork product and trace to the source.
Compared with prior art, beneficial effects of the present invention:
The SNP marker of the present invention is located on No. 6 chromosomes of pig, can further improve the detection covering surface of label, Improve the accuracy traced to the source, and the DNA for expanding pig traces to the source the detection range of SNP marker.
Specific implementation mode
Technical scheme of the present invention is described in further detail below in conjunction with specific embodiment.
The lookup of 1 molecular labeling of embodiment
(1) design of primers
With the DNA sequence dna (Genbank of No. 6 chromosomes of pig:FN673773) it is template, the DNA pieces of design primer separation pig Section (using the DNA of a Shen agriculture pig as the template of PCR amplification), primer is as follows:
Forward primer:5 '-CTTTACCGTTCTGCCCTTTC-3 ' (as shown in SEQ ID NO.2);
Reverse primer:5 '-TCCTCTGCCTGCCTTTGA-3 ' (as shown in SEQ ID NO.3).
PCR react total volume be 20 μ l, wherein pig genomic DNA about 100ng, (Promega companies) containing 1 × buffer, 1.5mmol/L MgCl2, dNTP (Shanghai Sheng Gong biotech firms) final concentration of 150 μm of ol/L, the final concentration of 0.2 μm of ol/ of primer L, 2U Taq archaeal dna polymerases (Promega companies).
PCR amplification:94 DEG C of 4min, (94 DEG C of 30s, 60 DEG C of annealing 30s, 72 DEG C of 30s) cycle 30 times, last 72 DEG C of extensions 10min。
PCR reaction products are detected with 1% agarose gel electrophoresis.PCR reaction products are examined with 1% agarose gel electrophoresis It surveys.
(2) cloning and sequencing is analyzed
The DNA fragmentation of obtained No. 6 chromosome of pig is cloned as follows.
The purifying of PCR product:The gel containing target fragment is cut from Ago-Gel in the UV lamp, is put into 1.5ml In Ependorff pipes, purified with PCR product purification kit (Tiangeng biochemical technology Co., Ltd).
Connection reaction:The PCR product of purifying is connect with pMD18-T carriers (Dalian treasured biotech firm), connection reaction is total Volume is 10 μ l, and including 5 μ l solution I (Dalian treasured biotech firm), (the precious biology in Dalian is public for the carrier T of 0.5 μ l Department), the purified pcr product of 2.5 μ l, be eventually adding 2 μ l aqua sterilisas set 4 DEG C of water-baths stay overnight.
Conversion:Take 100-120 μ l competent cells (Tiangeng biochemical technology Co., Ltd) in 1.5ml under germ-free condition In Ependorff pipes, mixing is added in the connection product of 5 μ l, places 30min on ice, 42 DEG C of heat shock 90s not shake therebetween Dynamic Ependorff pipes, ice bath 3-4min after taking-up are added the LB liquid medium of 400 μ l antibiotic-frees, 37 DEG C keep flat 1h after fall Set culture.
Bacterium colony PCR identifications:Bacterial strain after bacterium colony PCR identifications is in 37 DEG C of overnight incubations of LB culture mediums, and picking is multiple immediately Clone is sent to the sequencing of Shanghai life work biology Co., Ltd.
After tested, this is located on No. 6 chromosomes of pig, sequence such as SEQ ID through the spliced total 578bp of pig DNA sequence Shown in NO.1.It finds that there are a bases to replace at its 232nd base through analysis, is 232C or 232T.Pass through molecular biology Software is analyzed and ncbi database analysis, it is found that the replacement of the base at the 232nd base leads to Ecol30I-RFLP (Restriction Fragment Length Polymorphism, the i.e. sites Ecol30I-RFLP) polymorphism.
(3) foundation of PCR-Ecol30I-RFLP detection methods and the detection in replacement site
10 μ l of endonuclease reaction total volume, wherein 1 × buffer, 10 μ l, PCR product 3-5 μ l, restriction enzyme Ecol30I is 0.5 μ l (5U), uses H2O supplies 10 μ l, 37 DEG C of water-bath 4h, weigh 0.6g agaroses be dissolved in 15.75ml DEPC (on Hai Shenggong biotech firms) in processing water, be added after slightly cooling 5ml 5 × formaldehyde gel buffer solution and 4.25ml 37% Formalin, mixing glue detect digestion result after electrophoresis.As a result, it has been found that:There is C allele in SEQ ID NO.1 sequences 363bp and 215 two segment, T allele have tri- segments of 133bp, 230bp and 215bp, the two allele to constitute Three kinds of genotype, CC, CT, TT, also, replaced in the 232nd bit base of the SEQ ID NO.1 sequences, base is C or T.
The distribution situation of 2 allele of embodiment
(1) design of group is tested
Test group:Acquire Pietrain (21), Shen Nong (17), great Bai (43), great Shen (52), long Shen (16), The ear group of Du Shen (23), Pi great Shen (11), Shen of growing up (25), Du great Shen (17) and Du's (20) individuals of Pi great Shen It knits, extracts DNA, amount to 245 DNA samples.
The purpose of experiment group is to detect distribution situation of the SNP marker in different cultivars.
(2) genetic test
Forward primer:5 '-CTTTACCGTTCTGCCCTTTC-3 ' (as shown in SEQ ID NO.2);
Reverse primer:5 '-TCCTCTGCCTGCCTTTGA-3 ' (as shown in SEQ ID NO.3).
(condition such as embodiment 1) is expanded, it is all to detect experiment group with identical PCR-Ecol30I-RFLP methods Idiotype.
(3) statistical analysis
All idiotypes of record experiment group, and gene frequency and heterozygosity are calculated, as a result such as the following table 1.
Table 1
As known from Table 1:Gene frequency of the SNP marker of the present invention in each kind is close, rich polymorphism; Between kind or strain, the distributional difference of gene frequency C and T are small;The heterozygosity H of all kinds or strain is all higher than 0.3, Therefore it was initially believed that the DNA that the SNP marker can be used for pork product traces to the source and traces to the source with safety.
3 SNP marker availability of embodiment is traced to the source verification experimental verification
The SNP marker of the present invention can be used for by tentative confirmation in traceability label, in order to ensure in label of tracing to the source In availability, the present invention resamples in different location again, with existing 13 SNP markers (as described in Table 2) It is used in combination (totally 14 SNP markers), carries out availability and trace to the source verification experimental verification, meanwhile, only to be divided with existing 13 SNP Son label trace to the source verification experimental verification work to ratio.
In the ear tissue and each 100 parts of muscle sample for reviving slaughterhouse random acquisition pig individual, (each pig individual is adopted simultaneously Collect ear tissue sample and muscle sample), ear tissue sample number E1-E100, muscle sample number M1-M100 extract muscle sample and ear respectively The DNA of tissue sample is spare.
The pig of the present invention is detected in 20 muscle samples selected in 100 individual ear tissue samples and at random The genotype (amounting to 14 SNP marker sites) of Ecol30I SNP sites and existing published 13 SNP sites, system The genotype results of each individual of meter.According to digestion banding pattern, a band is denoted as 1, two bands occurs and is denoted as 2, three bands are denoted as 3. Record sequence is ranked sequentially according to 2 site of table, and the SNP marker site as II enzymes of Pvu of ADAMTS-1 genes identify is 1, Its genotype record result just makes number one, and the SNP marker site of I enzymes of the Eam1104 identification of ADD1 genes is 2, Genotype record result just comes second, and so on, the Ecol30I SNP molecule marks on No. 6 chromosomes of pig of the application Note site comes finally, and genotype results are indicated as the 14th number from left to right, and individual genotype can indicate For:21232223331221.
Table 2
The genotype in 14 SNP marker sites of each individual of statistics and meat sample, 100 individuals and 20 parts of muscle samples The genotype Statistical Comparison result of product is respectively such as the following table 3 and table 4.
In table 3, No. 82 individuals and No. 91 individual genotype are closely similar, and two individual preceding 13 tag values are equal Unanimously, only difference is that the 14th label is different.It can be seen that tracing back merely with existing 13 SNP markers When source, it may appear that the case where genotype repeats, the 14th is labeled as New SNP marker provided by the invention, illustrates that the present invention is added SNP marker after, so that it may with smoothly by this, genotype distinguishes in two, the addition of Novel SNP molecular marker of the invention The further perfect scale of tracing to the source for combination of tracing to the source, improves the accuracy traced to the source pork DNA with SNP marker.
The genotype results in 14 SNP marker sites of 20 parts of muscle samples with 100 individual genotype into Row compares analysis (comparison result is referring to table 4), and discovery can find the individual completely the same with 20 parts of muscle samples genotype, The source individual for finding 20 parts of pig muscles in 100 individuals by tracing to the source, realizes that meat sample is traced to the source to the accurate of individual.
Illustrate in conjunction with table 3 and table 4, experiment of tracing to the source, 100 individuals, 20 parts of muscle samples are carried out using 14 SNP markers Possess different genotype with 14 SNP marker detections, can realize individual differentiation.
Table 3
Number Genotype Number Genotype Number Genotype
E1 33332332132312 E35 33333232131333 E68 23311222133233
E2 21211233132122 E36 21333321323233 E69 2331333333321
E3 33333232331122 E37 22213233131321 E70 21231233333212
E4 23311232111313 E38 31221211121112 E71 21121333332231
E5 23113332231331 E39 22333231121222 E72 21231122211122
E6 23332221321323 E40 33332223111333 E73 31313113323221
E7 33231232321333 E41 21233113113323 E74 23131113231123
E8 23332222131122 E42 33311312333123 E75 31332213331113
E9 21123123221121 E43 21233112131322 E76 23333333321313
E10 31313211221112 E44 33112113133132 E77 23311232333322
E11 21211332123112 E45 21312233331233 E78 22131232333331
E12 12121313131112 E46 33212323222112 E79 12133233222322
E13 33312232313213 E47 31212333333311 E80 31211212311131
E14 32112212111321 E48 21232312331232 E81 21231222322321
E15 23113132231113 E49 33333232133221 E82 21231233333333
E16 23132311121122 E50 31133211131323 E83 21231233331332
E17 23123232113212 E51 33332333331233 E84 33331332333323
E18 32132231321322 E52 21133232323221 E85 31311222112211
E19 21213132321113 E53 21232132123113 E86 12132112133222
E20 21211212331333 E54 21232332321113 E87 23223212322223
E21 23313332323311 E55 21213232131213 E88 21231233333111
E22 33312233233213 E56 33132122332312 E89 23213331133212
E23 23111212323112 E57 33132312131132 E90 23311222132221
E24 13133331223213 E58 31231221331213 E91 21231333233331
E25 32113232321113 E59 31332333113313 E92 31212212123113
E26 21222223333333 E60 21313232321133 E93 33311232311132
E27 33312232132112 E61 31313133231332 E94 32131332233331
E28 32111222322223 E62 32132211313331 E95 23312332323112
E29 32311213123112 E63 33313233213333 E96 13332223323113
E30 32113213123221 E64 21321332221312 E97 21211132323332
E31 33123311113312 E65 32112213231223 E98 21332212132211
E32 11232131332231 E66 31213133321133 E99 32131331321113
E33 33131232232112 E67 32131133113321 E100 23313231323332
E34 31222212111132
Table 4
Number Genotype Corresponding individual Number Genotype Corresponding individual
M1 31213133321133 E66 M11 32131331321113 E99
M2 21333321323233 E36 M12 31221211121112 E38
M3 23123232113212 E17 M13 11232131332231 E32
M4 21123123221121 E9 M14 33212323222112 E46
M5 33123311113312 E31 M15 31332213331113 E75
M6 13133331223213 E24 M16 32131133113321 E67
M7 21121333332231 E71 M17 23131113231123 E74
M8 33112113133132 E44 M18 23213331133212 E89
M9 31313211221112 E10 M19 31212333333311 E47
M10 31231221331213 E58 M20 33131232232112 E33

Claims (3)

1. the SNP marker on No. 6 chromosomes of pig for tracing to the source, the DNA sequence dna such as SEQ ID NO.1 of the SNP marker Shown, total 578bp, there are one bases to replace at the 232nd bit base, is 232C or 232T;The SNP marker is by Ecol30I Restriction enzyme identifies.
2. the primer pair for expanding the SNP marker on No. 6 chromosomes of pig described in claim 1 for tracing to the source, special Sign is comprising forward primer, reverse primer, specific base sequence are as follows:
Forward primer:As shown in SEQ ID NO.2;
Reverse primer:As shown in SEQ ID NO.3.
3. application of the SNP marker described in claim 1 in DNA source tracing of pork products, wherein utilize claim 2 The primer pair amplifies go out the SNP marker sequence fragment.
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