CN107475415A - A kind of SNP primer pairs of the method for screening the high long oyster parent shellfish of glycogen content and its correlation - Google Patents

Abstract

The present invention relates to a kind of method for screening the high long oyster parent shellfish of glycogen content and its SNP primer pairs of correlation.By 486 individual whole-genome associations, 67 SNP signals significantly correlated with glycogen content on long No. 6 chromosomes of oyster are identified.1 SNP site at the scaffold1243_53489 bases of the region, develops its corresponding detection method, the results showed that can simply detect the SNP site rapidly using this method.Site CC genotype individuals are compared to TT genotype individuals simultaneously.The close shellfish of CC genotype is screened, instructs oyster breeding.Long oyster site upstream and downstream 500kb nucleotide sequence is as shown in SEQ ID No.1.Beneficial effect of the present invention carries out genotype identification, raising filial generation glycogen content to close shellfish before being seed breeding.This result of study acquisition SNP marker confidence level is higher, and effect is more stable.

Description

A kind of SNP of the method for screening the high long oyster parent shellfish of glycogen content and its correlation draws Thing pair

Technical field

The invention belongs to genetic engineering and genetic breeding field, is related to a kind of long oyster glycogen content correlation of screening The primer pair of SNP marker and its application.

Background technology

Oyster is a kind of important marine living resources, and one of most important sea-farming shellfish in the world.China Oyster culture scale and yield be all sure to occupy first place in the world for many years, but the average price of oyster outlet is only other countries' oyster production The 1/3 of product.This explanation China oyster can only market one's own products mostly, it is difficult into high-end market.Improve the warp of China's oyster culture Ji benefit, realizes industry from the poorly efficient transition and upgrade to high yield and high efficiency of high yield, the product quality for improving oyster is to need solution badly Certainly the problem of.And the content height of the nutriment such as glycogen is one of most important characteristic of oyster.The content of glycogen not only influences male Oyster coefficient of condition and yield, while the main taste compound of delicate flavour is used as, oyster consumption mouthfeel is affected, directly determines oyster product Quality.The genetic improvement for carrying out the Nutrient Quality Traits such as glycogen is the important way for solving the poorly efficient present situation of China's oyster industry high yield Footpath.

In aquatic livestock breeding research starting evening, the research to growth traits is focused primarily upon at present, method is mostly using biography The selection of system, hybridization, cycle length, slowly effect.Quality trait research to long oyster is also rare.In the last few years, genomics Development, the breeding technique such as molecular marking supplementary breeding and full-length genome selection have also obtained fast development, substantially increased male The genetic breeding of oyster is horizontal, not only makes it possible the breeding of the complicated quality trait such as glycogen, while also will being obviously improved property The Breeding Efficiency and precision of shape.Blindness can be reduced using molecular marker assisted selection simultaneously, shortens the breeding time limit, raising is educated The efficiency of kind.And the method that molecular labeling is obtained currently with genome sequencing mainly includes QTL positioning and full-length genome pass Join the method for analysis.Although QTL localization methods can the fast positioning chromosome segment associated with character, in character parsing side Face has the characteristics of degree of accuracy is high.But its linkage analysis based on limited meiosis, the region of the genome large fragment of positioning All it is chained together, it is difficult to be accurately positioned.And whole-genome association method can then overcome this shortcoming, in full-length genome In the range of to hereditary variation gene carry out population interconnection analysis, by associated bit point location in the section of very little, significantly improve The degree of accuracy of positioning and precision, the heredity parsing for the complex character that is particularly suitable for use in.In recent years, with non-mode biology full-length genome The completion of sequencing, positioned using GWAS technique study complexity Quantitative Trait Genes into fashion trend.

Although GWAS has played important function in the agro-ecology of crop and livestock and poultry is studied, in aquatic livestock also only There is a small amount of report.Such as in Atlantic salmon quality research, fillet fat content is associated using 5,650 SNP markers Analysis.And in terms of the research of the aquatic livestock reported at present, especially bivalve shellfish association analysis is concentrated mainly on candidate gene. But this method is to carry out the exploitation of pleomorphism site on known functional gene according to prior information, marks relative number Mesh is few, differs and surely obtains main effect site, and can not have a comprehensive understanding to the genetic regulation mechanism of phenotype.With length The completion of oyster genome sequencing and the acquisition of high density genetic linkage mapses so that carry out GWAS analyses and be possibly realized. The present invention is based on long oyster genome, and carrying out full-length genome by two generation sequencing technologies resurveys sequence, and is carried out for glycogen content Whole-genome association, obtain the main effect pleomorphism site and key gene of control glycogen content.The present invention is in full-length genome On the basis of resurveying sequence, magnanimity SNP marker is developed, parsing determines the hereditary basis of oyster glycogen content, filtered out and glycogen content Extremely significantly correlated cluster SNP marker, the screening for glycogen phenotype.Compared with the SNP site developed in the past, what GWAS was obtained SNP signal confidence level is higher, while has simplicity, portable strong feature.

The content of the invention：

It is an object of the invention to provide a kind of SNP marker related to long oyster glycogen content, for the molecule mark of long oyster Remember that assisted Selection provides reference.

Specific acquisition SNP methods are as follows：(1) experiment material collection and homogeneity raise and train：It is wild to collect 486 long oyster Raw individual, carries out homogeneous cultivation.(2) measure of phenotypic data：Sugar is carried out to different long oyster individuals using anthrone colorimetric hair Former assay.(3) Genotyping：Using two generation sequencing technologies platforms, full-length genome is carried out to 486 oysters and resurveys sequence, is sieved Look into SNPs sites and carry out individual parting, obtain effective SNPs sites for association analysis, build the haplotype collection of illustrative plates of oyster. (4) association analysis：Whole-genome association is carried out using mixed linear model, obtains 67 SNP significantly associated with character Site (P-value<10^-6), in the range of long oyster genome scaffold 1,243 16,015-67,096kb.Pass through LD Block is analyzed, 67 SNP site close linkages (LD ＞ 0.7).Whole-genome association Manhattan figure is shown in accompanying drawing 2.Then choosing In the base on scaffold1243_53,489kb, P-value is 2.67 × 10 for fetch bit^-7, as this project candidate SNP locus. Two base forms of T and C be present in the site.Other 66 in the range of scaffold 1243 16,015-67,096kb SNP site all applies identical authentication method.

The present invention is achieved by the following technical programs：

A kind of SNP marker related to long oyster glycogen content：The mark is located at long oyster genome scaffold1243_ At 53,489kb base, there are two base forms of T and C in this base.The sequence such as SEQ of the site upstream and downstream 500kb Shown in ID No.1.It is as follows to predominantly detect step：

1) long oyster genomic DNA is extracted, 10-20ng/uL is diluted to using aqua sterilisa or TE buffer solutions；

2) it is template to take long oyster genomic DNA described in step 1), and reaction system is prepared using primers F and R：Genome DNA 1uL, universal PC R mix 5uL, primers F and each 0.2uL of R, distilled water 3.6uL is (if genomic DNA concentration≤5ng/ for sterilizing UL, 4.6uL genomic DNAs can be added and be not added with the distilled water that sterilizes.Another reaction system can amplify on year-on-year basis)；

3) response procedures of PCR amplifications are：

It is for the above-mentioned PCR forward and reverse primer sequences expanded：

F：5’-TAGTATTAAGGCACATGCCG-3’；

R：5’-ATGATGTTTACTTGTTTGCTTG-3’.

4) after the PCR reactions described in step 3) terminate, add saturated fluorescence dyestuff Lcgreen and internal standard (mixed in equal amounts High temperature internal standard and low temperature internal standard, i.e., two double chain oligonucleotides with different G/C contents, high and low temperature internal standard final concentration are respectively 2.5uM) each 1uL, by 95 DEG C of annealing 5-10min；

5) room temperature is naturally cooling to after the annealing described in step 4), carries out high-resolution melting curve analysis, identification is treated The genotype of long oyster SNP marker, specific method are described in test sample sheet：

A) melting curve of all samples to be tested is corrected using interior target melting curve；

B) a point group is carried out to all sample to be tested melting curves after correction, if melting curve derivation figure is unimodal and peak value More than 77.5 DEG C, then SNP genotype is CC to corresponding abscissa temperature, if melting curve is asked, figure is unimodal and peak value corresponds to abscissa Temperature be less than 77.5 DEG C then SNP genotype be TT, be after the melting curve derivation it is bimodal if SNP genotype be TC；

C) long oyster SNP marker genotype described in each sample to be tested is judged.

Required high and low interior label sequence during SNP genotype identifications, wherein, high temperature interior label sequence is：

Low temperature interior label sequence is：

Target specific method is in acquisition：

1) it is single-stranded to synthesize four oligonucleotides for authorized company：

GWNB+：5’-GCGGTCAGTCGGCCTAGCGGTAGCCAGCTGCGGCACTGCGTGACGCTCAG-3’

GWNB-：5’-CGCCAGTCAGCCGGATCGCCATCGGTCGACGCCGTGACGCACTGCGAGTC-3’

DWNB+：5’-ATCGTGATTTCTATAGTTATCTAAGTAGTTGGCATTAATAATTTCATTTT-3’

DWNB-：5’-TAGCACTAAAGATATCAATAGATTCATCAACCGTAATTATTAAAGTAAAA-3’

2) dissolving four single-stranded nucleotides with sterilizing distilled water makes final concentration of 10uM；

3) four single-stranded nucleotides are mixed in equal volume, obtain the internal standard that high and low temperature internal standard final concentration is respectively 2.5uM.

The potential application of the SNP marker related to long oyster glycogen content：Up to the present, in addition to this patent, in oyster In, there has been no the report based on whole-genome association exploitation SNP marker.This result of study is marked relative to single SNP in the past The exploitation of note, confidence level is higher, and the scope of suited-community is wider, and effect is more stable.Before seed breeding, taken by non-lethality Sample extracts oyster genomic DNA, judges close shellfish genotype using SNP marker and its authentication method as described above, passes through sieve CC genotype parent shellfishes are selected to effectively improve the long oyster glycogen content of offspring.The present invention provides judges SNP according to PCR primer melting curve The method of genotype, as shown in figure 1, when be unimodal after melting curve derivation and peak value correspond to abscissa temperature more than 77.5 DEG C when SNP genotype is CC, when be unimodal after melting curve derivation and peak value correspond to abscissa temperature less than 77.5 DEG C when SNP genotype For TT, SNP genotype is TC when being bimodal after melting curve derivation.

Brief description of the drawings

1. Fig. 1 is the PCR primer melting curve derivation figure in the above-mentioned scaffold1243_53,489 sites included；2. Fig. 2 It is the Manhattan figure of above-mentioned long oyster glycogen content whole-genome association.

Embodiment：

Further explain the present invention with reference to embodiments, but embodiment does not do any type of limit to the present invention It is fixed.

Embodiment 1：

A) collection of sample：288 individuals of wild population of seedling are incubated in collection Jiangnan simultaneously, and it is dissected, takes closed shell Flesh and remaining tissue, are saved backup with liquid nitrogen flash freezer after -80 DEG C.

B) DNA extraction：Extract the genomic DNA of 288 samples and use Uv-spectrophotometric Determination concentration, according to Genomic DNA is diluted to 10ng/uL by measure concentration using aqua sterilisa；

C) SNP site genotype detection：The genomic DNA of dilution in step 1) is taken to enter as template using primers F and R Performing PCR expands, and reaction system is as follows：Genomic DNA 1uL, primers F and R each 0.2uL, PCR mix 5uL, sterilize distilled water 3.6uL；

PCR amplification response procedures be：

After described PCR reactions terminate, saturated fluorescence dyestuff Lcgreen and each 1uL of internal standard is added, by 95 DEG C of DEG C of annealing 8min；

Forward primer is F：5’-TAGTATTAAGGCACATGCCG-3’；

Reverse primer is R：5’-ATGATGTTTACTTGTTTGCTTG-3’；

Reaction adds 1 μ l internal standards (internal standard is same as above) and 1 μ l LC-green dyestuffs after terminating, 95 DEG C are denatured after brief centrifugation 10min, it is cooled to room temperature.

Room temperature is naturally cooling to after annealing, carries out high-resolution melting curve analysis, test sample is treated in identification

A) melting curve of all samples to be tested is corrected using interior target melting curve；

B) a point group is carried out to all sample to be tested melting curves after correction, after melting curve derivation is unimodal and peak value SNP genotype is CC when corresponding abscissa temperature is more than 77.5 DEG C, and after melting curve derivation be unimodal and peak value corresponds to horizontal seat It is TT to mark SNP genotype when temperature is less than 77.5 DEG C, and SNP genotype is TC when being bimodal after melting curve derivation.

C) long oyster SNP marker genotype described in each sample to be tested is judged.

Required high and low interior label sequence during SNP genotype identifications, wherein,

High temperature interior label sequence is：

Low temperature interior label sequence is：

Target specific method is in acquisition：

1) it is single-stranded to synthesize four oligonucleotides for authorized company：

GWNB+：5’-GCGGTCAGTCGGCCTAGCGGTAGCCAGCTGCGGCACTGCGTGACGCTCAG-3’

GWNB-：5’-CGCCAGTCAGCCGGATCGCCATCGGTCGACGCCGTGACGCACTGCGAGTC-3’

DWNB+：5’-ATCGTGATTTCTATAGTTATCTAAGTAGTTGGCATTAATAATTTCATTTT-3’

DWNB-：5’-TAGCACTAAAGATATCAATAGATTCATCAACCGTAATTATTAAAGTAAAA-3’

2) dissolving four single-stranded nucleotides with sterilizing distilled water makes final concentration of 10uM；

3) four single-stranded nucleotides are mixed in equal volume, obtain the internal standard that high and low temperature internal standard final concentration is respectively 2.5uM.

D) HRM partings:Take out 96 hole PCR reaction plates and be put into the progress HRM detections of the machines of LightScanner 96, collect 55 Fluorescence signal between DEG C -95 DEG C, operation finishes carries out interpretation of result according to melting curve, counts the genotype of each individual.

E) interpretation of result:After detection, only the 102nd idiotype is C/C, and 136 idiotypes are T/C, 49 Individual idiotype is T/T, and 1 idiotype is NN.

F) detection and association analysis of glycogen content：288 wild individual glycogen contents are detected using anthrone colorimetry. Data are shown in figure, and the order of different genotype glycogen content is CC>TC>TT.CC genotype glycogen content is compared to TT types, sugar Former content significantly improves 8.6%.So the parting in the site significantly associates with glycogen content.By screening CC in breeding Type individual, can significantly improve offspring's glycogen content.

Table 1：288 individual glycogen contents and Genotyping analysis.

Sequence table (1) SEQ ID NO.1 information sequence characteristic length：1001bp

Type：Nucleic acid

Chain：It is single-stranded

Topological structure：It is linear

Molecule type：DNA

Source：Long oyster

Sequence description：

AATATTCAAATACATGTATATGATGCAAGTTTTCTTCTTTATGCTACATCTTACATA

CAACACATGAACATACACTGCAGATAAATGCAGAATGAGTGATTTTCCCTGTTTTGTGAATTCTTTGACATGCAGAA ATATTAGAGTTATTTCCCTTTTAACACAAGATATTCTTGTACAAAAGAGGACTCCGAATGTCTCCTTTGTGGTCTCT TTTTTGTGCATTCAAATTCTCTTTTTGATGGTATGGTCATATTATAAGTATAGATACCACTTAGGAAATGCATCAAA ACATGATAAAGATATGGCAAAATTAAAATATTTCAAGACAAGATTAATTTATGACATGGAAAACATCTGTTCAGTTA AATAATATTTTAATTTGGTTTTTGATGCAACGTTCAAGTCTGAGATATTTATTAACAGGTATGGAACCACAATGGAA ACACACATGAAGAATTTAGTATTAAGGCACATGCCGCCCAATTTACAAACTATGGACTTCAAGCAAACAAGTAAACA TCATATCCTTAACCAGTTACTTTCAACTAAATGTTATCATTTGACTTTTATCCCAATTTTAAAGAGTCAGTTTGAAA ATGAAAATTTTCAGTAATCTGCTTCTCTTCGTCAACAGCAATCCGCCCTAACTTGGACAGTTACGTGTTCCTGCGTG TGAACGAGGACACTGACGGAGTTCTAGTGGAGGAGGAAACGTTAGACACGGGGTGAGTTATCCTGATGACACACGTG TGTATGTAGCCGACTTACTGTACAGGAAATGTACACGTCAAGGATTTAATTTCCTGAAGTTTGTGTAGAGAAGTCTG ATGAATACCGGTACATGATGAAGTCTGTTTCGTGGGAATTATATTTCATTGCCTGCACATTTATACAATTTGATTCT CTTGATTTATTCTGTTTTTTAAAATGGGGCCAATGTCATATAAATTATATGTATAACCCAACAATAACTTTAATATC ATTGTTGTAAAATATTAACA。

By 486 individual whole-genome associations, 67 on long No. 6 chromosomes of oyster and sugar are identified The significantly correlated SNP signal of former content.1 SNP site at the scaffold1243_53489 bases of the region, is developed Its corresponding detection method, the results showed that can simply detect the SNP site rapidly using this method.Site CC genes simultaneously Type individual is compared to TT genotype individuals, and glycogen content significantly improves 8.6%.Subsequently can be with it, screening CC bases Because of the close shellfish of type, oyster breeding is instructed.Long oyster site upstream and downstream 500kb nucleotide sequence such as SEQ ID No.1 It is shown.The invention provides a SNP marker and its potential application significantly correlated with long oyster glycogen content, its advantage It is that genotype identification can be carried out to close shellfish before seed breeding, improves filial generation glycogen content.

Sequence table

<110>The Institute of Oceanology of the Chinese Academy of Sciences

<120>A kind of SNP primer pairs of the method for screening the high long oyster parent shellfish of glycogen content and its correlation

<141> 2017-09-20

<160> 1

<170> SIPOSequenceListing 1.0

<210> 1

<211> 1001

<212> DNA

<213> gene

<220>

<221> gene

<222> (1)..(1001)

<400> 1

aatattcaaa tacatgtata tgatgcaagt tttcttcttt atgctacatc ttacatacaa 60

cacatgaaca tacactgcag ataaatgcag aatgagtgat tttccctgtt ttgtgaattc 120

tttgacatgc agaaatatta gagttatttc ccttttaaca caagatattc ttgtacaaaa 180

gaggactccg aatgtctcct ttgtggtctc ttttttgtgc attcaaattc tctttttgat 240

ggtatggtca tattataagt atagatacca cttaggaaat gcatcaaaac atgataaaga 300

tatggcaaaa ttaaaatatt tcaagacaag attaatttat gacatggaaa acatctgttc 360

agttaaataa tattttaatt tggtttttga tgcaacgttc aagtctgaga tatttattaa 420

caggtatgga accacaatgg aaacacacat gaagaattta gtattaaggc acatgccgcc 480

caatttacaa actatggact tcaagcaaac aagtaaacat catatcctta accagttact 540

ttcaactaaa tgttatcatt tgacttttat cccaatttta aagagtcagt ttgaaaatga 600

aaattttcag taatctgctt ctcttcgtca acagcaatcc gccctaactt ggacagttac 660

gtgttcctgc gtgtgaacga ggacactgac ggagttctag tggaggagga aacgttagac 720

acggggtgag ttatcctgat gacacacgtg tgtatgtagc cgacttactg tacaggaaat 780

gtacacgtca aggatttaat ttcctgaagt ttgtgtagag aagtctgatg aataccggta 840

catgatgaag tctgtttcgt gggaattata tttcattgcc tgcacattta tacaatttga 900

ttctcttgat ttattctgtt ttttaaaatg gggccaatgt catataaatt atatgtataa 960

cccaacaata actttaatat cattgttgta aaatattaac a 1001

Claims (5)

1. a kind of screen the related SNP primer pairs of the long oyster parent shellfish of high glycogen content, it is characterised in that：

Forward primer is F：5’-TAGTATTAAGGCACATGCCG-3’；

Reverse primer is R：5’-ATGATGTTTACTTGTTTGCTTG-3’.

A kind of 2. method for screening the long oyster parent shellfish of high glycogen content as claimed in claim 1, it is characterised in that：

One SNP marker is obtained by whole-genome association, it is located at long oyster genome scaffold1243_53, At 489kb bases；There are two base forms of T and C in the site, carry out the SNP marker site base to close shellfish before seed breeding Because type identifies that the order of different genotype glycogen content is CC>TC>TT, by screening the close shellfish of site CC genotype, improve The glycogen content of progeny population,

It is as follows including step：

(1) extraction of the long oyster genome, specially extracts long oyster genomic DNA, uses aqua sterilisa or TE buffer solutions It is diluted to 10-20ng/uL；

(2) the long oyster genomic DNA is template, prepares reaction system：Genomic DNA 1uL, universal PC R mix 5uL, draws Each 0.2uL of thing F and R, sterilizing distilled water 3.6uL；The reaction system can amplify on year-on-year basis；

(3) response procedures of PCR amplifications are：

(4) after the PCR reactions described in terminate, saturated fluorescence dyestuff Lcgreen and each 1uL of internal standard is added, is moved back by 95 DEG C -98 DEG C Fiery 5-10min；

(5) room temperature is naturally cooling to after annealing, carries out high-resolution melting curve analysis, test sample is treated in identification

A) melting curve of all samples to be tested is corrected using interior target melting curve；

B) a point group is carried out to all sample to be tested melting curves after correction, after melting curve derivation be unimodal and peak value is corresponding SNP genotype is CC when abscissa temperature is more than 77.5 DEG C, and after melting curve derivation be unimodal and peak value corresponds to abscissa temperature SNP genotype is TT when degree is less than 77.5 DEG C, and SNP genotype is TC when being bimodal after melting curve derivation.

C) long oyster SNP marker genotype described in each sample to be tested is judged.

3. the method for the high long oyster parent shellfish of glycogen content of screening according to claim 2, it is characterised in that：

In the step (5), the high temperature internal standard and low temperature internal standard of mixed in equal amounts are inside designated as, i.e., two have the double of different G/C contents Chain oligonucleotides, high and low temperature internal standard final concentration are respectively 2.5 μM.

4. the method for the high long oyster parent shellfish of glycogen content of screening according to claim 3, it is characterised in that：

Required high and low interior label sequence during SNP genotype identifications, wherein,

High temperature interior label sequence is：

Low temperature interior label sequence is：

5. the method for the high long oyster parent shellfish of glycogen content of screening according to claim 3, it is characterised in that：

Target specific method is in acquisition：

1) it is single-stranded to synthesize four oligonucleotides for authorized company：

GWNB+：5’-GCGGTCAGTCGGCCTAGCGGTAGCCAGCTGCGGCACTGCGTGACGCTCAG-3’GWNB-：5’- CGCCAGTCAGCCGGATCGCCATCGGTCGACGCCGTGACGCACTGCGAGTC-3’DWNB+：5’- ATCGTGATTTCTATAGTTATCTAAGTAGTTGGCATTAATAATTTCATTTT-3’DWNB-：5’- TAGCACTAAAGATATCAATAGATTCATCAACCGTAATTATTAAAGTAAAA-3 ' 2) dissolves four lists with sterilizing distilled water Chain nucleotides makes final concentration of 10uM；

3) four single-stranded nucleotides are mixed in equal volume, obtain the internal standard that high and low temperature internal standard final concentration is respectively 2.5uM.