CN109022591A - One kind SNP marker relevant to Macrobrachium rosenbergii body measurement trait and its application - Google Patents

One kind SNP marker relevant to Macrobrachium rosenbergii body measurement trait and its application Download PDF

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CN109022591A
CN109022591A CN201810907437.1A CN201810907437A CN109022591A CN 109022591 A CN109022591 A CN 109022591A CN 201810907437 A CN201810907437 A CN 201810907437A CN 109022591 A CN109022591 A CN 109022591A
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macrobrachium rosenbergii
body measurement
snp
measurement trait
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冯艺
陈文强
李镇养
李浩杰
袁启志
张志浩
陈文坚
杨虹
刘咸
陈建酬
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Foshan University
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Abstract

The invention discloses one kind SNP markers relevant to Macrobrachium rosenbergii body measurement trait and its application that belong to molecular marker breeding technical field.The SNP marker corresponds to the site Macrobrachium rosenbergii ND1 gene T574C, and base is T or C herein.SNP marker of the invention is related to Macrobrachium rosenbergii body measurement trait (carapace is high, uromere is high, periproct is high), it is a new molecular labeling, by the genotype of determination Macrobrachium rosenbergii SNP site to be measured to which the body measurement trait (carapace is high, uromere is high, periproct is high) to Macrobrachium rosenbergii carries out early stage breeding, production cost can effectively be saved and accelerate genetic progress, preferably serve the breeding of Macrobrachium rosenbergii, not only it had been able to satisfy the huge market demand, but also with very big Economic Application value and scientific research value.

Description

One kind SNP marker relevant to Macrobrachium rosenbergii body measurement trait and its application
Technical field
The invention belongs to molecular marker breeding technical fields, in particular to a kind of relevant to Macrobrachium rosenbergii body measurement trait SNP marker and its application.
Background technique
Molecular mark (Marker Assisted Selection, MAS) is using molecular labeling and to determine mesh The characteristics of marking the gene close linkage of character is screened and important economic characters (such as weight, growth in animals and plants breeding process Speed, resistance etc.) relevant molecular labeling, and building has the breeding population of related molecular marker in breeding process, with Achieve the purpose that a kind of breeding method of selection target character, accuracy high feature strong with Objective can be significantly Breeding efficiency is improved, the breeding time limit is shortened.
Mononucleotide loci polymorphism (Single Nucleotide Polymorphisms, SNP) is on genome by list The nucleotide variation that a nucleotide generates has the characteristics that distributed quantity is more, rich polymorphism, be after microsatellite molecular marker it Another important molecular genetic marker, referred to as third generation molecular genetic marker afterwards.The label is widely used to animals and plants mark Remember the fields such as assistant breeding, the assignment of genes gene mapping, genetic diversity Journal of Sex Research.
ND1 gene is the gene for encoding nadh dehydrogenase subunit 1,1 (NADH of nadh dehydrogenase subunit Dehydrogenase subunit 1, ND1) gene be mtDNA protein coding gene, including cytochrome b, cytochromes The coded sequence of 7 subunits of 3 subunits of oxidizing ferment, 2 subunits of ATP enzyme and nadh dehydrogenase is responsible for the egg of coding White is the subunit I of nadh dehydrogenase.Nadh dehydrogenase is the main composition of electron transport chain complex I, by direct in respiratory chain It participates in hydrogen and electron transmission and goes to participate in energetic supersession effect by oxidative phosphorylation generation ATP.Thus, it influences to a certain extent The acquisition of animal exogenous nutrition substance, assimilation utilize and the activity of the vital metabolics such as transhipment and then the character of animal risen decisive Effect.It is more about species ND1 gene diversity Journal of Sex Research both at home and abroad, such as three tail swallowtail butterflies (Bhutanitis thaidina), nothing The discussion of the phylogeographies and genetic development such as web gecko (Gekko swinhonis), tree toad (Hylid).Currently, Hou Lingling Have found chicken NDl Gene A 4589G mutation and caecum length, 8 week old chest depths, 8 week old keel lengths and 8 week old shins length, leg flesh length There is significant correlation respectively with the influence of leg flesh width, glucose, lactic dehydrogenase, abdominal fat, abdominal fat and subcutaneous fat thickness.
Macrobrachium rosenbergii, also known as Malaysian prawn, fresh water prawn, big long-armed prawn are under the jurisdiction of Arthropoda, hapalonychia Guiding principle, Decapoda, Palaemonidae, pond crayfish category are one of tropical fresh water shrimps largest in the world, and with growing, fast, feeding habits are wide, resistance to The features such as high temperature, premunition are strong, the culture-cycle is short, mouthfeel is fresh and tender and rich in nutrition content and by consumers.It originates in In the India Pacific region, various types of fresh water or salt-fresh water waters are lived in, is supported later by the shifting of many countries and regions numerous It grows, becomes local main freshwater aquiculture shrimps.Currently, Macrobrachium rosenbergii is up to more than 60 ten thousand mu, but Roche in the cultured area of China The breeding quantity of pond crayfish is far from meeting its huge industry size and huge seed demand, therefore, the early stage of Macrobrachium rosenbergii Breeding seems very urgent and significant.
Summary of the invention
To overcome the above insufficient or defect in the prior art, the present invention provides one kind and Macrobrachium rosenbergii body measurement trait phase The SNP marker and its application of pass, can be by the genotype of determination Macrobrachium rosenbergii SNP site to be measured to Macrobrachium rosenbergii Body measurement trait (carapace is high, uromere is high, periproct is high) carries out early stage breeding, limits without age, the gender etc. by Macrobrachium rosenbergii, The early stage breeding that can be effectively used for Macrobrachium rosenbergii promotes the breeding process of Macrobrachium rosenbergii.
The technical solution used in the present invention is:
A kind of SNP marker relevant to Macrobrachium rosenbergii body measurement trait, the SNP marker are located at Macrobrachium rosenbergii The site ND1 gene T574C, base is T or C herein.
Application of the SNP marker in Macrobrachium rosenbergii early stage breeding.
A kind of method of Macrobrachium rosenbergii body measurement trait early stage breeding, for according to the base in the site Macrobrachium rosenbergii ND1 gene T574C Because type carries out early stage breeding to Macrobrachium rosenbergii body measurement trait, include the following steps:
(1) design specific amplification contains the primer pair of the genetic fragment in the site Macrobrachium rosenbergii ND1 gene T574C;
(2) genomic DNA of Macrobrachium rosenbergii to be measured is extracted;
(3) PCR amplification, detection amplification gained are carried out with genomic DNA of step (1) the resulting primer pair to Macrobrachium rosenbergii The genotype of the SNP site of genetic fragment;
(4) early stage breeding is carried out to Macrobrachium rosenbergii body measurement trait based on the genotype of SNP site.
As a further improvement of the foregoing solution, the primer sequence of the PCR amplification is
ND1-F:5 '-GATAAAGTAGGCTATGCTGG-3 ' (SEQ ID № 1),
ND1-R:3 '-CCTCCTCTGTACTCGGTATT-5 ' (SEQ ID № 2).
As a further improvement of the foregoing solution, the amplification instrument that the PCR amplification uses is BIO-RAD T100PCR instrument.
The beneficial effects of the present invention are: the present invention provides a kind of SNP molecule marks relevant to Macrobrachium rosenbergii body measurement trait Note and its application, the SNP marker are located at the site Macrobrachium rosenbergii ND1 gene T574C, and base is T or C herein.Sieve The nucleotide sequence of ND1 gene is significant related to the body measurement trait of Macrobrachium rosenbergii from 5 ' 574 bit base T or C of end in family name pond crayfish, i.e., (carapace is high, uromere is high, tail for SNP marker and Macrobrachium rosenbergii body measurement trait on the site Macrobrachium rosenbergii ND1 gene T574C Section is high) it is related, it is a new molecular labeling, by the genotype of determination Macrobrachium rosenbergii SNP site to be measured to Roche natural pond Shrimp body measurement trait (carapace is high, uromere is high, periproct is high) carries out early stage breeding, can effectively save production cost and accelerate heredity into Exhibition, preferably serves the early stage breeding of Macrobrachium rosenbergii, has not only been able to satisfy the huge market demand, but also have very big Economic Application Value and scientific research value.
Detailed description of the invention
Fig. 1 is the PCR products electrophoresis map of Macrobrachium rosenbergii ND1 Gene Partial segment;
Fig. 2 is 574 mutational site genotype mutations sequence alignment of Macrobrachium rosenbergii ND1 gene.
Specific embodiment
The present invention is specifically described below with reference to embodiment, in order to technical field personnel to of the invention Understand.It is necessary to it is emphasized that embodiment is only intended to, the present invention will be further described herein, should not be understood as to this The limitation of invention protection scope, fields person skilled in the art, according to foregoing invention content non-to made by the present invention The modifications and adaptations of matter should still fall within protection scope of the present invention.Mentioned raw materials following simultaneously are unspecified, For commercial product;The processing step or preparation method not referred in detail be processing step known to a person skilled in the art Or preparation method.
The source of the Macrobrachium rosenbergii cultured population of test: Guangdong (GD) adopts 47 samples;Adopt 76 samples in Guangxi 1 (GX1) Product;Adopt 35 samples in Guangxi 2 (GX2);44 samples are adopted in Hainan (HN), are provided by the seedling base of three water-white golden breeding companies, Raised under identical environmental condition 106, in July, 2017 random acquisition at shrimp.
Embodiment
One, the detection of SNP marker
1. design primer: design specific amplification contains the primer of the genetic fragment in the site Macrobrachium rosenbergii ND1 gene T574C It is right.
Using software Primer 5.0, with the ND1 gene (GenBank:NC_006880.1) of Macrobrachium rosenbergii in GenBank The specificity amplification primer for making Reference Design, the primer sequence expanded are
Upstream F:5 '-GATAAAGTAGGCTATGCTGG-3 ' (SEQ ID № 1), 20bp;
Downstream R:3 '-CCTCCTCTGTACTCGGTATT-5 ' (SEQ ID № 2), 20bp.
Optimum temperature is 48.8 DEG C, product length 542bp, and by Guangzhou, Sheng Gong bioengineering Co., Ltd is synthesized.
2. the extraction of Macrobrachium rosenbergii genomic DNA
Use the whole blood kit of OMEGAD, the specific steps are as follows:
(1) each sample takes the blood sample of 150 μ L, and buffer Elution Buffer is added, and vortex mixes 10s;
(2) the Buffer GL lysate of 500 μ L is added in each sample, shakes up 20s manually, stands 20min;
(3) after the GL2 lysate of 100 μ L is added, there is white opacity in solution, after vortex mixes 60s, 13000 × g high speed It is centrifuged 15min, the phenomenon that separation of solid and liquid after centrifugation;
(4) supernatant after centrifugation is transferred in adsorption column, 10000 × g high speed centrifugation 1min, is outwelled in absorption column tube Waste liquid;
(5) the HB Buffer that 500 μ L are added binds liquid, after 10000 × g is centrifuged 1min, outwells useless in absorption column tube Liquid;
(6) the Wash Buffer cleaning solution of 650 μ L is added, 10000 × g high speed centrifugation 1min is outwelled in absorption column tube Waste liquid;
(7) (6) step is repeated;
(8) the Elution Buffer dilution of 70 DEG C of preheatings is added, 1000 × g is centrifuged after being incubated at room temperature 3min;
(9) liquid that centrifugation is obtained rejoins in adsorption column, and 1000 × g is centrifuged after being incubated at room temperature 3min, carries out pair The label answered, -20 DEG C of preservations.
3. amplification and detection: carrying out PCR amplification, detection amplification with genomic DNA of the primer pair of design to Macrobrachium rosenbergii The genotype of the SNP site of gained genetic fragment.
Take 40 samples at random in the genome extracted, every 4 samples take 2 μ L to mix, are divided into 10 groups, carry out PCR respectively Amplification amounts to 10 samples.
Program: the PCR SuperMix of full formula gold is used.
System: DD H2O:22 μ L;Mix:25 μ L;
Upstream primer: 1 μ L;Downstream primer: 1 μ L;DNA:1 μ L.
Using BIO-RAD T100PCR instrument, wherein program setting: A, 94 DEG C of initial denaturation 5min;B, 94 DEG C of denaturation 30s;C, 48.8 DEG C of annealing 30s;D, 72 DEG C of extension 1min;E, B~D30 circulation;F:72 DEG C of extension 5min;G:4 DEG C of constant temperature saves.
With 0.8g BIOWEST agarose, 1.0% agarose is made in 1 × TAE liquid of 80ml and 8 μ L Goldview It is solidifying.With 5 μ L product point samples, using the full formula gold DNA Marker DL2000 of 5 μ L as reference, in BIO-RAD Powerpac electrophoresis In instrument, use 1 × TAE liquid as room temperature electrophoresis.(wherein, voltage: 150V;Electric current 400mA;Time: 20min.) after electrophoresis, It observes and photographs to record under Tanon gel imaging system.Determine single and clearly bright purpose band occur (such as Fig. 1 institute Show) after send to Guangzhou Sheng Gong biotech firm and be sequenced, Genotyping is carried out according to sequencing result, obtains Fig. 2.
Two, the association analysis of SNP site genotype and character
The relevance of linear analogue analysis SNP site genotype and character is carried out using SAS9.0 software Mixed program, In, phenotypic number is represented with body measurement trait (carapace is high, uromere is high, periproct is high) when analysis, as follows using model:
Model: Yijkx=p+Bj+Gk+Eijkl+Fx+bjk:
YijkxFor the observation of Carcass Traits, p is group's mean, BjIt is sex-effects, GkFor genotype effects.
EijklFor random error.FxFor family stochastic effects.bjkFor the regression coefficient for influencing slaughter traits.With GLM program The least squares means and standard error of different genotype slaughter trait are calculated, while carrying out significance test.
The gene frequency of its SNP site and the association analysis of body measurement trait are as shown in table 1 below.
The gene frequency of 1 SNP site of table and the association analysis of body measurement trait
As shown in Table 1, which is that the carapace height, uromere height, periproct height of the Macrobrachium rosenbergii of TT type are significantly higher than TC Type (P < 0.05).Body measurement trait (carapace height, uromere of the nucleotide sequence from 5 ' 574 bit base T or C of end and Macrobrachium rosenbergii It is high, periproct is high) significant correlation.
Above-described embodiment is the preferred embodiment of the present invention, all with similar technique of the invention and made equivalence changes, It should belong to protection category of the invention.
SEQUENCE LISTING
<110>Foshan Science &. Technology College
<120>a kind of SNP marker relevant to Macrobrachium rosenbergii body measurement trait and its application
<130> 2018.08.01
<160> 2
<170> PatentIn version 3.5
<210> 1
<211> 20
<212> DNA
<213>artificial sequence
<400> 1
gataaagtag gctatgctgg 20
<210> 2
<211> 20
<212> DNA
<213>artificial sequence
<400> 2
cctcctctgt actcggtatt 20

Claims (6)

1. a kind of SNP marker relevant to Macrobrachium rosenbergii body measurement trait, which is characterized in that the SNP marker is located at The site Macrobrachium rosenbergii ND1 gene T574C, base is T or C herein.
2. a kind of application of SNP marker relevant to Macrobrachium rosenbergii body measurement trait, which is characterized in that by claim 1 institute The SNP marker stated is applied in Macrobrachium rosenbergii early stage breeding.
3. a kind of method of Macrobrachium rosenbergii body measurement trait early stage breeding, which is characterized in that SNP site according to claim 1 Genotype to Macrobrachium rosenbergii body measurement trait carry out early stage breeding.
4. according to the method described in claim 3, it is characterized by comprising the following steps:
(1) design specific amplification contains the primer pair of the genetic fragment in the site Macrobrachium rosenbergii ND1 gene T574C;
(2) genomic DNA of Macrobrachium rosenbergii to be measured is extracted;
(3) PCR amplification, detection amplification gained genetic fragment are carried out with genomic DNA of the primer pair of step (1) to Macrobrachium rosenbergii SNP site genotype;
(4) early stage breeding is carried out to Macrobrachium rosenbergii body measurement trait based on the genotype of SNP site.
5. according to the method described in claim 4, it is characterized in that, the sequence of the primer pair of the PCR amplification such as SEQ ID № 1 Shown in 2.
6. according to the method described in claim 4, it is characterized in that, the amplification instrument that uses of the PCR amplification is BIO-RAD T100PCR instrument.
CN201810907437.1A 2018-08-10 2018-08-10 One kind SNP marker relevant to Macrobrachium rosenbergii body measurement trait and its application Pending CN109022591A (en)

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Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN109797226A (en) * 2019-02-26 2019-05-24 中国水产科学研究院珠江水产研究所 A kind of Macrobrachium rosenbergii classification method based on EST-SSR label
CN110029174A (en) * 2019-04-22 2019-07-19 浙江省淡水水产研究所 A kind of SSR marker related to Macrobrachium rosenbergii weight
CN112375827A (en) * 2020-03-24 2021-02-19 扬州大学 SNP marker related to growth of macrobrachium rosenbergii as well as typing method and application thereof
CN114410801A (en) * 2022-01-26 2022-04-29 广西壮族自治区药用植物园 SNP marker influencing growth traits of macrobrachium rosenbergii and application thereof
CN114480675A (en) * 2022-03-04 2022-05-13 广西壮族自治区药用植物园 GP gene SNP marker and application thereof

Non-Patent Citations (3)

* Cited by examiner, † Cited by third party
Title
AGARWAL ET AL.: "SNP mining in transcripts and concomitant estimation of genetic variation in Macrobrachium rosenbergii stocks", 《CONSERVATION GENETICS RESOURCES》 *
GENBANK: "Macrobrachium rosenbergii mitochondrion, complete genome", 《GENBANK》 *
THANH ET AL.: "Single nucleotide polymorphisms in the actin and crustacean hyperglycemic hormone genes and their correlation with individual growth performance in giant freshwater prawn Macrobrachium rosenbergii", 《AQUACULTURE》 *

Cited By (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN109797226A (en) * 2019-02-26 2019-05-24 中国水产科学研究院珠江水产研究所 A kind of Macrobrachium rosenbergii classification method based on EST-SSR label
CN110029174A (en) * 2019-04-22 2019-07-19 浙江省淡水水产研究所 A kind of SSR marker related to Macrobrachium rosenbergii weight
CN110029174B (en) * 2019-04-22 2023-01-10 浙江省淡水水产研究所 SSR (simple sequence repeat) marker related to quality of macrobrachium rosenbergii bodies
CN112375827A (en) * 2020-03-24 2021-02-19 扬州大学 SNP marker related to growth of macrobrachium rosenbergii as well as typing method and application thereof
CN112375827B (en) * 2020-03-24 2023-10-27 扬州大学 SNP (single nucleotide polymorphism) marker related to growth of macrobrachium rosenbergii as well as typing method and application thereof
CN114410801A (en) * 2022-01-26 2022-04-29 广西壮族自治区药用植物园 SNP marker influencing growth traits of macrobrachium rosenbergii and application thereof
CN114480675A (en) * 2022-03-04 2022-05-13 广西壮族自治区药用植物园 GP gene SNP marker and application thereof

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