CN105950727B - Lefteye flounder genotype detection primer and method based on microsatellite marker Paraoliva-1 - Google Patents

Lefteye flounder genotype detection primer and method based on microsatellite marker Paraoliva-1 Download PDF

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CN105950727B
CN105950727B CN201610332145.0A CN201610332145A CN105950727B CN 105950727 B CN105950727 B CN 105950727B CN 201610332145 A CN201610332145 A CN 201610332145A CN 105950727 B CN105950727 B CN 105950727B
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lefteye flounder
paraoliva
genotype
microsatellite
primer
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CN105950727A (en
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刘云国
刘凌霄
李瑶瑶
刘传林
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Linyi Xiaolu Biotechnology Co.,Ltd.
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Yantai University
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Abstract

The invention discloses a kind of lefteye flounder genotype detection primers and method based on microsatellite marker Paraoliva-1.The genomic DNA in Paralichthys olivaceus is extracted first and is diluted spare;The microsatellite core sequence contained in lefteye flounder DNA sequence dna is recycled, in its sequence design specific primers at both ends;Then PCR amplification is carried out using genomic DNA individual in the primer pair lefteye flounder difference proles or lefteye flounder group, PCR product is detected;It is analyzed using the band that product occurs, determines the genotype of each individual, and obtain the genetic polymorphism map of lefteye flounder.It is characteristic of the invention that the mapping genetic variations of lefteye flounder genetic marker Paraoliva-1 can be obtained efficiently, method is easy.

Description

Lefteye flounder genotype detection primer and method based on microsatellite marker Paraoliva-1
Technical field
The invention belongs to lefteye flounder (Paralichthys olivaceus) DNA molecular Genetic Markers, it is related to a kind of inspection Survey the technical method of lefteye flounder microsatellite marker Paraoliva-1, the specifically genotype of lefteye flounder microsatellite marker Paraoliva-1 Detection method.
Background technique
Lefteye flounder (Paralichthys olivaceus) belong to Pleuronectiformes (Pleuronectiformes), lefteye flounder section (Paralichthyidae), Paralichthys (Paralichthys), it is referred to as flatfish (Flatfish, Fluke) in China, it is left Flounder (Left-eyed flounder) tooth piece and step (Plaice) are the rare economic fish of marine products that cold aqueous, bottom is dwelt.At me There is extensive distribution in the Bohai and Yellow Seas of state and the East Sea.Lefteye flounder has growth fast, and individual is big, and reproductive capacity is strong, migratory small, returns The features such as Gui Xingqiang, particularly suitable in coastal development aquatic breeding.China artificial breeding of lefteye flounder and quotient since the eighties Product cultivation, occupies an important position in sea-farming at present.However, overfishing in recent years has made its stock number seriously decline Subtract, and the fast development of aquatic breeding, also the inheritance of Ya Xian natural population, germ plasm resource and genetic diversity are produced Immeasurable influence.Molecular labeling can be applied to the side such as analysis of genetic diversity, individual identification and genealogical identification of lefteye flounder Face.Although isoenzyme mark, RAPD label and AFLP labelling technique can be used for genetic structure and its heredity of research lefteye flounder Diversity, however since these labels belong to dominant inheritance label, detection efficiency is not as good as codominant markers such as microsatellite markers It is high.In addition, the shortcomings that isoenzyme mark is that polymorphism is low, the stability of RAPD label is bad, and AFLP marking operation is cumbersome, this Their application is all greatly limited a bit.And microsatellite sequence is distributed widely in eukaryotic gene group, its main feature is that type More, allele number is more, and polymorphism is high, codominance, mendelian inheritance pattern, and is randomly distributed in genome, Er Qiewei Satellite markers detection efficiency is high, as a result stable.Currently, although having developed some microsatellite markers in lefteye flounder, they The disadvantage is that allele is few, polymorphism is not high, limits its application, so there is an urgent need to obtain the microsatellite marker of high polymorphism To carry out the research and application of lefteye flounder genetic diversity, individual identification and genealogical identification etc..
Summary of the invention
The object of the present invention is to provide a kind of lefteye flounder DNA molecular Genetic Markers of high polymorphism, i.e. lefteye flounder microsatellite The rapid detection method of Paraoliva-1 is marked, to make up the deficiency of prior art.
Basic conception of the invention mainly utilizes the microsatellite core sequence contained in lefteye flounder DNA sequence dna, at its both ends Design specific primer simultaneously carries out PCR detection, thus the rapidly each individual hereditary variation in this microsatellite area of detection lefteye flounder, The primer (microsatellite marker Paraoliva-1) is obtained to the polymorphism map of lefteye flounder, is intuitively detected by map each The genotype of individual.Status and actual requirement based on the above background, the present invention obtain a microsatellite from lefteye flounder DNA sequence dna Label, is named as Paraoliva-1, microsatellite marker Paraoliva-1 can be used for lefteye flounder analysis of genetic diversity and pedigree Certification.
The present invention is completed according to following operational aspect: the genomic DNA and dilute first in extraction Paralichthys olivaceus It releases spare;The microsatellite core sequence contained in lefteye flounder genomic dna sequence is recycled, design specificity is drawn at its sequence both ends Object;Then PCR amplification is carried out using genomic DNA individual in the primer pair lefteye flounder difference proles or lefteye flounder group, PCR is produced Object carries out denaturing polyacrylamide gel electrophoresis detection, so that it is determined that the genotype of each individual, obtains the genetic polymorphism of lefteye flounder Property map.
Lefteye flounder genomic DNA is extracted, 100ng/ μ l is diluted to, 1 μ l is added in each PCR reaction, reacts total volume For 25 μ l.
DNA sequence dna containing microsatellite sequence are as follows:
1 catcgactct agaggaccgt acagatttga agatggtaga aactcagcac acagccagag
61 aacccctagg ggacctgtgg agagaacaaa gcacctcatg gttaggagag ccagagacct
121 ctgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt
181 gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt
241 gtcccgaaac ctggagacct gaccctcagc aactttttaa tgctagactg gaggccagat
301 gagggagagg gttggtccga ctggtttgta tgatga
Wherein microsatellite core sequence are as follows:
gtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgt gtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgtgt
Paraoliva-1 micro-satellite primers sequence are as follows:
Normal chain 5 '-CATCGACTCTAGAGGACCGTACA -3 ',
Minus strand 5 '-TCATCATACAAACCAGTCGGACCA -3 ', annealing temperature when using the primer are 60 DEG C.
Microsatellite core sequence and primer sequence are core of the invention, are presented in lefteye flounder Diversity Detection polymorphic Property.
The sample-adding parameter of PCR amplification are as follows: each PCR reaction total volume is 25 μ l, including 100ng lefteye flounder genomic DNA;10 × PCR Buffer, 2.5 μ l;Mg2+1.5mmol/L;Tag enzyme 1u;Each 0.1mmol/L of dNTP;Each 10pmol of above-mentioned primer; Add ddH2O to 25 μ l.Use the program parameter that PCR instrument is set when the primer are as follows: 94 DEG C of denaturation 2min;94 DEG C of 30sec, 60 DEG C 45sec, 72 DEG C of 40sec, the reaction carry out 35 circulations;72 DEG C of 5 min of extension, 4 DEG C of preservations.
The detecting step of PCR product: by PCR product with 15W invariable power electrophoresis in 8% denaturing polyacrylamide gel It is separated within 1.5 hours.After electrophoresis, 30min is impregnated with 10% glacial acetic acid solution first, then distilled water flushing 5min, then with 0.1% silver nitrate solution impregnate 30min, with 3% sodium carbonate liquor develop the color 5min, finally with 10% ice Acetum impregnates 5min, and the polymorphism map of lefteye flounder microsatellite marker Paraoliva-1 can be obtained.
Therefore, it is characteristic of the invention that the hereditary variation of the Paraoliva-1 microsatellite marker of lefteye flounder can be obtained efficiently Map, method are easy.Moreover, microsatellite marker meets Mendelian inheritance mould for other molecular genetic marker techniques Formula, is in codominant inheritance, and acquired results can intuitively detect the genotype of each individual of lefteye flounder;And it is applied to different proles Or genetic marker, genealogical identification and building of genetic map etc. between individual in lefteye flounder group.
Detailed description of the invention
Fig. 1 is microsatellite marker Paraoliva-1 of the present invention, and to lefteye flounder 20 individual test maps, (number 1-20 is 20 individuals of lefteye flounder).
Specific embodiment
Describe lefteye flounder Paraoliva-1 microsatellite core sequence DNA molecular genetic marker skill in detail below by embodiment Art method.The genomic DNA in Paralichthys olivaceus is extracted first and is diluted spare;Recycle what is contained in lefteye flounder DNA sequence dna micro- to defend Star core sequence, in its sequence design specific primers at both ends;Then the primer pair lefteye flounder difference proles or lefteye flounder group are used The genomic DNA of interior individual carries out PCR amplification, carries out denaturing polyacrylamide gel electrophoresis detection to PCR product, determines each The genotype of individual obtains the genetic polymorphism map of lefteye flounder.
1, the extraction of lefteye flounder genomic DNA: 100 μ g Paralichthys olivaceus are added in Eppendorf pipe, cell cracking is added The 5 μ l of Proteinase K of liquid 500 μ l and 20mg/ml, gently shake up, and 37 DEG C overnight.Then 600 μ are added in cracked sample L Fen Lv ︰ Fang ︰ isoamyl alcohol (25 ︰, 24 ︰ 1) mixed liquor, 12000rpm is centrifuged 10min after shaking 20min, takes supernatant.It adds Fen ︰ Lv Fang ︰ isoamyl alcohol mixed liquor repeats aforesaid operations 3 times.Supernatant is taken again, and the cooling dehydrated alcohol and 1/ of 2 times of volumes is added The sodium acetate of the 3mol/L of 10 volumes, 12000rpm are centrifuged 10min, discard supernatant liquid, retain DNA precipitating, then with 70% ethyl alcohol It washs the precipitating 2 times, after ethyl alcohol volatilization completely, with TE buffer solution DNA, and is diluted to 100ng/ μ l, 4 DEG C of preservations.
2, the design of micro-satellite primers: on the basis of lefteye flounder DNA sequence dna, using the sequence of microsatellite DNA two sides same Species are relative to the well-conserved of core sequence, accordingly in its design specific primers at both ends, amplify the site with it Microsatellite segment.Since microsatellite core sequence mutation rate is relatively high, the increasing of microsatellite DNA core sequence number of repetition is caused It adds deduct few, i.e. the variation of microsatellite DNA sequence length, this is the root for detecting microsatellite polymorphism.Microsatellite of the invention The specific primer sequence at area core sequence both ends are as follows: normal chain 5 '-CATCGACTCTAGAGGACCGTACA -3 ', minus strand 5 ' - TCATCATACAAACCAGTCGGACCA -3 ', annealing temperature when using the primer are 60 DEG C.
3, PCR amplification: being loaded first, and sample-adding amount is as follows: lefteye flounder genomic DNA (100ng/L), 1 μ l;10×PCR Buffer, 2.5 μ l;Mg2+(25mmo1/L), 1.5 μ l;Taq enzyme (5u/ μ l), 0.2 μ l;DNTP (each 2.5mmo/L), 1 μ l;Draw Object (each 10pmol/ μ l), 1 μ l;Add aqua sterilisa to 25 μ l.Secondly, carrying out PCR reaction, PCR amplification instrument program parameter are as follows: 94 DEG C denaturation 2min;94 DEG C of 30sec, 60 DEG C of 45sec, 72 DEG C of 40sec, 35 circulations;72 DEG C of extension 5min, 4 DEG C of preservations.
4, the detection of PCR product: PCR product is separated by electrophoresis on 8% denaturing polyacrylamide gel, electrophoresis apparatus function Rate is 15W, and electrophoresis time is 1.5 hours or so.After electrophoresis, 30min is impregnated with 10% glacial acetic acid solution first, then Distilled water flushing 5min, 0.1% silver nitrate solution impregnate 30min, 3% sodium carbonate liquor colour developing 5min, finally with 10% Glacial acetic acid solution impregnate 5min lefteye flounder can be obtained in the polymorphism map of Paraoliva-1 microsatellite core sequence, such as Fig. 1 It is shown.Fig. 1 the result shows that, 20 of lefteye flounder individual coamplifications go out 22 allele, illustrate microsatellite marker Paraoliva-1 With very high polymorphism, it is appropriate for the side such as lefteye flounder genetic diversity and genetic structure analysis, individual identification and genealogical identification The research and application in face.
<110>University Of Yantai
<120>based on the lefteye flounder genotype detection primer and method of microsatellite marker Paraoliva-1
<160> 1
<210> 1
<211> 336
<212> DNA
<213>lefteye flounder (Paralichthys olivaceus)
<220>
<221> repeat_region
<222> (123)...(242)
<400> 1
1 catcgactct agaggaccgt acagatttga agatggtaga aactcagcac acagccagag
61 aacccctagg ggacctgtgg agagaacaaa gcacctcatg gttaggagag ccagagacct
121 ctgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt
181 gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt gtgtgtgtgt
241 gtcccgaaac ctggagacct gaccctcagc aactttttaa tgctagactg gaggccagat
301 gagggagagg gttggtccga ctggtttgta tgatga

Claims (5)

1. one group of primer detected using microsatellite marker Paraoliva-1 to lefteye flounder genotype, which is characterized in that
Wherein the primer is sequence:
Normal chain 5 '-CATCGACTCTAGAGGACCGTACA -3 ',
Minus strand 5 '-TCATCATACAAACCAGTCGGACCA -3 ', annealing temperature when using the primer are 60 DEG C.
2. the method detected using microsatellite marker Paraoliva-1 to lefteye flounder genotype, which is characterized in that extract first Genomic DNA in Paralichthys olivaceus simultaneously dilutes spare;The microsatellite core sequence contained in lefteye flounder DNA sequence dna is recycled, is used Specific primer carries out PCR amplification to the genomic DNA of lefteye flounder Different Individual, and it is solidifying to carry out denaturing polyacrylamide to PCR product Gel electrophoresis detection, so that it is determined that genotype of the lefteye flounder Different Individual in Paraoliva-1 core sequence area, wherein the lefteye flounder The specific primer of microsatellite marker Paraoliva-1 are as follows:
Normal chain 5 '-CATCGACTCTAGAGGACCGTACA -3 ',
Minus strand 5 '-TCATCATACAAACCAGTCGGACCA -3 ', annealing temperature when using the primer are 60 DEG C.
3. the method that lefteye flounder genotype is detected using microsatellite marker Paraoliva-1 as claimed in claim 2, It is characterized in that, to the PCR amplification that the genomic DNA of different lefteye flounder individuals carries out, is loaded parameter are as follows: each PCR reaction is overall Product is 25 μ L, including 100ng lefteye flounder genomic DNA;10 × PCR Buffer, 2.5 μ L;Mg2+1.5 mmol/L;Taq enzyme 1u; dNTP 0.1mmol/L;Each 10 pmol of specific primer in claim 1;Finally plus ddH2O to 25 μ l;PCR instrument is set Program parameter are as follows: 94 DEG C of denaturation 2min;94 DEG C of 30sec, 60 DEG C of 45sec, 72 DEG C of 40sec, the reaction carry out 35 circulations; 72 DEG C of 5 min of extension, 4 DEG C of preservations.
4. the method that lefteye flounder genotype is detected using microsatellite marker Paraoliva-1 as claimed in claim 2, The step of being characterized in that, denaturing polyacrylamide gel electrophoresis detection is carried out to PCR product: PCR product is gathered in 8% denaturation It is separated within 1.5 hours in acrylamide gel with 15W invariable power electrophoresis, 30min is impregnated with 10% glacial acetic acid solution, so Distilled water flushing 5min afterwards, then with 0.1% silver nitrate solution impregnate 30min, with 3% sodium carbonate liquor develop the color 5min, most 5min is impregnated with 10% glacial acetic acid solution afterwards.
5. application of the method between lefteye flounder group on genetic polymorphism map construction described in claim 2-4 any one.
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