CN103409420A - Y-chromosome specific molecular marker of Nile tilapia, and genetic sex determination method and supermale producing method both based on molecular marker - Google Patents
Y-chromosome specific molecular marker of Nile tilapia, and genetic sex determination method and supermale producing method both based on molecular marker Download PDFInfo
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Abstract
The invention discloses a Y-chromosome specific molecular marker of Nile tilapia, wherein the nucleotide sequence of the Y-chromosome specific molecular marker is as shown in SEQ ID No.4; the Y-chromosome specific molecular marker can be commonly used for a plurality of strains of Nile tilapia; a genetic sex determination method of Nile tilapia is established based on the molecular marker, so that normal female fish XX, normal male fish XY, converted female fish XY, converted female fish YY and supermale fish YY can be differentiated from each other economically, rapidly and accurately; large-scale production of supermale fish fry can be realized through mating of YY supermale fish and the normal female fish XX based on the genetic sex determination method; as a result, the yield of culture is improved remarkably, the culture cost is reduced and the economic benefit is enhanced; besides, a method of producing the YY supermale fish through mating of the supermale fish YY and the converted female fish YY is also established by using the Y-chromosome specific molecular marker.
Description
Technical field
The invention belongs to the molecular breeding technical field, relate to tilapia sex specific molecular marker, based on the tilapia genetic sex identification method of this molecule marker and the method for producing the supermale fish based on this molecule marker.
Background technology
Tilapia claims again African crucian, originate in the African continent and the Atlantic coast degree of saltiness water waters, the Middle East, belonging to Osteichthyes Perciformes Callichthyidae, is tropic fishes, has that reproductivity is strong, growth is fast, feeding habits are wide, feed request is low, lower oxygen concentration resistance, adaptability and an advantage such as disease resistance is strong.In recent decades, along with countries in the world are introduced tilapia in succession, its one of main cultured fishes kind that become international.At present, the tilapia breed variety of China has Mozambique tilapia, bolti, Oreochromis aureus etc., is mainly wherein bolti.China is the first producing country of tilapia and export State.
Because tilapia is short sexual cycle, breeding is fast, female slower than male growth, for fear of tilapia excessive multiplication in cultivation, obtains fast, individual large, the neat specification of growth, marketable fish that output is high, need to carry out single male Tilipia production.The method that obtains at present single male Tilipia on producing mainly contains three kinds: one, sex-reversal method, and namely with male hormone, to process fry and obtain full milter, the method is simple and easy to do, but has the suspicion of hormone residues, does not meet the requirement of pollution-free healthy cultivation; Two, species hybridization method, as bolti ♀ * Oreochromis aureus ♂, the method is pollution-free, the marketable fish performance is good, but needs the parent very pure, and obtaining male ratio is only generally 90-95%, still have a considerable amount of rauns, also have crossing barrier to a certain degree, the breeding cycle is long, and numerous seedling amount is on the low side; Three, three series mating method, claim again hereditary male Tilipia technology (Genetically Male Tilapia, GMT), being about to sex-reversal and hybridizing method combines, with (the XX ♀ of former system, XY ♂), transform system (XY ♀, YY ♀) and malely isozygoty that to be that (YY ♂) is supporting produce hereditary complete male tilapia.Concrete grammar is as follows: the undifferentiated juvenile fish seedling of sex is carried out to feminized treatment, transform raun (XY ♀) by the filial generation Test Identification; To transform raun (XY ♀) with former be milter (XY ♂) mating, by filial generation Test Identification YY supermale fish; By YY supermale fish with transform raun (XY ♀) mating and carry out feminized treatment, by filial generation Test Identification YY, transform raun; YY is transformed to raun and the mating of YY supermale fish, obtain full YY supermale fish; By YY supermale fish and former be raun (XX ♀) mating, produce full milter.Above-mentioned three line for hybrid seed production program comparision complexity, in a single day required time is also longer, but obtains YY supermale fish and YY conversion raun, just can obtain in a large number YY supermale fish (YY ♀ * YY ♂), is a kind of relatively method of science.But because prior art can only judge parent's genotype for sex ratio according to tester after the test cross experiment, complex operation is time-consuming, labour intensity is large, seriously hindered applying of GMT, therefore, the key of three series mating method is how to distinguish quickly and efficiently normal raun XX ♀, normal milter XY ♂, transform raun XY ♀, transform raun YY ♀ and supermale fish YY ♂.
Development and maturation along with molecular marking technique, by analyzing with the closely linked molecule marker of target gene, judge molecular marker assisted selection (the Marker-Assisted Selection whether target gene exists, MAS) technology is identified for the genetic sex of tilapia, and its key is to filter out the special molecule marker of tilapia sex.By hero (female) the property specific DNA molecule marker chain with sex chromosome (sex) in screening tilapia genome, by the MAS technology, can greatly simplify the Production Flow Chart of GMT, reduce production costs, increase the benefit.Contriver place seminar is in early-stage Study, bolti Y chromosome specific molecular marker NtY1 and NtY2 and X chromosome specific molecular marker NtX1 have been filtered out, and based on above-mentioned molecule marker, set up the genetic sex identification method (Chinese patent ZL201010501061.8) of bolti, also developed on this basis another bolti sex specific molecular marker (called after marker2 in the present invention).But above-mentioned sex specific molecular marker is all not ideal enough, slightly far away with the distance in bolti sex determination site, be only applicable to screen the bolti strain of this mark, and can not be common to the bolti of multiple strain.
Summary of the invention
In view of this, one of purpose of the present invention is to provide a kind of bolti Y chromosome specific molecular marker, can be common to the bolti of multiple strain; Two of purpose is to provide a kind of method of carrying out the evaluation of bolti genetic sex based on above-mentioned molecule marker, can distinguish economical, quickly and accurately normal raun XX ♀, normal milter XY ♂, transforms raun XY ♀, transform raun YY ♀ and supermale fish YY ♂; Three of purpose is to provide a kind of method based on above-mentioned molecule marker fast and efficient production supermale fish, realizes the large-scale production of full milter fry by YY supermale fish, to cultivate route, significantly improves cultured output, reduces aquaculture cost, increases economic efficiency.
After deliberation, the invention provides following technical scheme:
1. bolti Y chromosome specific molecular marker, its nucleotide sequence is as shown in SEQ ID No.4.
2. the molecule marking method identified of bolti genetic sex comprises the following steps:
A.PCR amplification: get the fin ray of bolti to be measured, extract genomic dna; The gained genomic dna of take is template, adopt the upstream primer shown in SEQ ID No.1 and the downstream primer shown in SEQ ID No.2, pcr amplification bolti sex specific molecular marker: the nucleotide sequence of X chromosome specific molecular marker is as shown in SEQ ID No.3, and the nucleotide sequence of Y chromosome specific molecular marker is as shown in SEQ ID No.4;
B. result judgement: from the genomic dna of bolti to be measured, only amplifying the X chromosome specific molecular marker, judge that this bolti to be measured is the raun in heredity, the sex chromosome genotype is XX; From the genomic dna of bolti to be measured, only amplifying the Y chromosome specific molecular marker, judge that this bolti to be measured is the supermale fish in heredity, the sex chromosome genotype is YY; From the genomic dna of bolti to be measured, amplifying simultaneously X chromosome specific molecular marker and Y chromosome specific molecular marker, judge that this bolti to be measured is the milter in heredity, the sex chromosome genotype is XY.
3. the molecule marking method that adopts the bolti genetic sex to identify is produced the method for supermale fish, comprises the following steps:
A. in the post-coitum of bolti raun XX and milter XY generation, carried out to feminized treatment, the molecule marking method that adopts the bolti genetic sex to identify, filtering out the sex chromosome genotype is the conversion raun of XY;
B. XY is transformed to raun and the mating of bolti XY milter, the molecule marking method that adopts the bolti genetic sex to identify, from filtering out the supermale fish that the sex chromosome genotype is YY the offspring; Separately get XY conversion raun and bolti XY milter post-coitum for carrying out feminized treatment, the molecule marking method that adopts the bolti genetic sex to identify, filtering out the sex chromosome genotype is the conversion raun of YY;
C. YY supermale fish and YY are transformed to the raun mating, obtain full YY supermale fish;
D. YY supermale fish offspring is carried out to feminized treatment, obtain YY and transform raun;
E. repeating step C and D, transform the raun mating by YY supermale fish and YY and produce YY supermale fish.
After adopting aforesaid method to guarantee to continue acquisition YY supermale fish, by YY supermale fish and the mating of bolti XX raun, can produce in a large number complete male marketable fish.
Beneficial effect of the present invention is: genetic linkage analysis shows, in the situation that get rid of natural sex, reverse interference, bolti X of the present invention and Y chromosome specific molecular marker (difference called after sdX and sdY in the present invention) are 0cM with the genetic distance in bolti sex determination site, obviously be better than the described bolti X of Chinese patent ZL201010501061.8 and Y chromosome specific molecular marker NtX1 and NtY2, and another bolti sex specific molecular marker marker2 of filtering out of this seminar, can be common to the bolti of multiple strain, as to from Hainan, 98 tail boltis of 4 different lines of four the tilapia nurseries in Guangxi and Guangdong carry out the double blinding check, genetic sex and phenotypic sex identify that the rate of coincideing is 90%~100%, based on the bolti genetic sex identification method of X of the present invention and Y chromosome specific molecular marker sdX/sdY structure, can distinguish economical, quickly and accurately normal raun XX ♀, normal milter XY ♂, transform raun XY ♀, transform raun YY ♀ and supermale fish YY ♂, based on the YY ♀ of above-mentioned bolti genetic sex identification method foundation and the method for YY ♂ mating production YY supermale fish, can fast and efficient production YY supermale fish, and then realize the large-scale production of full milter fry by YY supermale fish and normal raun XX ♀ mating, significantly improve cultured output, reduce aquaculture cost, increase economic efficiency.
The accompanying drawing explanation
In order to make purpose of the present invention, technical scheme and beneficial effect clearer, the invention provides following accompanying drawing and describe:
Fig. 1 is the sequence alignment figure of X of the present invention and Y chromosome specific molecular marker.
The result that Fig. 2 carries out the genetic sex evaluation for application X of the present invention and Y chromosome specific molecular marker to 5 tail bolti raun XX, 5 tail bolti milter XY and 5 tail bolti supermale fish YY, M means DNA molecular amount standard DL2000.
Fig. 3 for application X of the present invention and Y chromosome specific molecular marker to result that 19 tail XX ♀ * XX ♂ bolti filial generation carries out the genetic sex evaluation, wherein 1-19 is XX ♀ * XX ♂ filial generation, XX, XY, YY are contrast, and M means DNA molecular amount standard DL2000.
Fig. 4 for application X of the present invention and Y chromosome specific molecular marker to result that 19 tail XX ♀ * YY ♂ bolti filial generation carries out the genetic sex evaluation, wherein 1-19 is XX ♀ * YY ♂ filial generation, XX, XY, YY are contrast, and M means DNA molecular amount standard DL2000.
Fig. 5 for application X of the present invention and Y chromosome specific molecular marker to result that 19 tail YY ♀ * YY ♂ bolti filial generation carries out the genetic sex evaluation, wherein 1-19 is YY ♀ * YY ♂ filial generation, XX, XY, YY are contrast, and M means DNA molecular amount standard DL2000.
Fig. 6 is X of the present invention and Y chromosome specific molecular marker and the sex determination site linkage map on sex chromosome.
Embodiment
Below in conjunction with accompanying drawing, the preferred embodiments of the present invention are described in detail.The experimental technique of unreceipted actual conditions in preferred embodiment, usually according to normal condition, the molecular cloning experiment guide (third edition for example, J. the work such as Pehanorm Brooker, Huang Peitang Deng Yi, Science Press, 2002) described in condition, or the condition of advising according to manufacturer.
One, the acquisition of bolti sex specific molecular marker
1, the extraction of genomic dna
The clip bolti (is the Japanese strain bolti of this laboratory introduction, its female parent draws from Egyptian, male parent is drawn from Malaysia) fin ray 10mg, put homogenate in lysate [10mM Tris-HCl (pH8.0)+100mM EDTA (pH8.0)+100mM NaCl+5mg/ml SDS] 600 μ l, adding final concentration is the Proteinase K of 20mg/ml and the ribonuclease A (RnaseA) that final concentration is 100 μ g/ml, 55 ℃ of water-bath digestion are to clarification, add again phenol-chloroform-primary isoamyl alcohol (volume ratio is 25:24:1) mixed solution 600 μ l, after fully mixing in 12000rpm centrifugal 10 minutes, draw supernatant liquor, again add phenol-chloroform-primary isoamyl alcohol (volume ratio is 25:24:1) mixed solution extracting DNA, centrifugal, draw supernatant liquor, add ice ethanol 1000 μ l precipitation DNA, centrifugal, abandon supernatant liquor, the DNA precipitation is 70% washing with alcohol through volume fraction, after seasoning, with the TE damping fluid, dissolve and make the solution (OD that concentration is 20ng/ μ l
260/ OD
280=1.76~1.80) ,-20 ℃ save backup.
2, the interval screening of PCR random amplification sex determination sex specific molecular marker
Research to the different lines bolti shows, genetic linkage group LG1(Cnaani and Kocher, 2008; Lee et al., 2011; Lee et al., 2003), LG3(Campos-Ramos et al., 2001; Carrasco et al., 1999; Foresti et al., 1993; Harvey et al., 2003; Harvey et al., 2002; Ocalewicz et al., 2009) and LG23(Eshel et al., 2011; 2012) corresponding karyomit(e) is likely all sex chromosome, but which LG correspondence karyomit(e) on earth, at present final conclusion not also.Based on early-stage Study achievement and bolti genomic dna sequence, the contriver be chosen in LG23 32 pairs of primers of Random Design on 3 adjacent Scaffold7,101 and 29 (be respectively Scaffold716 to, Scaffold1016 to, Scaffold2910 to), respectively pcr amplification is carried out in XX, XY, YY bolti genome pond, screening sex specific molecular marker.Found that, (upstream primer F1 sequence is as shown in SEQ ID No.1 for 1 pair of primer on Scaffold101, downstream primer R1 sequence is as shown in SEQ ID No.2) have an obvious sex-specific, can in XX and XY individuality, amplify the X chromosome specific band of a long 1422bp, simultaneously in XY and YY individuality, amplify the Y chromosome specific band of a long 982bp, and all the other 31 pairs of primers do not have sex-specific.
3, the clone of sex specific molecular marker and sequential analysis
Get respectively the sepharose that contains above-mentioned X chromosome specific band, Y chromosome specific band, reclaim the purpose fragment, it is cloned into to the pMD-19T carrier, transform again competent escherichia coli cell, with blue hickie sieve method screening positive clone, picking hickie list bacterium colony, identify positive colony by the PCR method, then check order.
The X chromosome specific molecular marker that order-checking is obtained (sequence as shown in SEQ ID No.3, called after sdX) and Y chromosome specific molecular marker (sequence as shown in SEQ ID No.4, called after sdY) carry out the sequence alignment analysis.As shown in Figure 2, the sequence difference of X and Y chromosome specific molecular marker mainly contains 3 places: with the X chromosome specific molecular marker, compare, 1. the Y chromosome specific molecular marker has inserted the 36bp sequence at the 514bp place to result; 2. at the 738bp place, lacked the 4bp sequence; 3. at the 838bp place, lacked the 472bp sequence.
Two, the molecule marking method of bolti genetic sex evaluation
The molecule marking method that the bolti genetic sex is identified comprises the following steps:
The A.PCR clone: the fin ray of clip bolti to be measured, extract genomic dna; The gained genomic dna of take is template, adopts the upstream primer F1 shown in SEQ ID No.1 and the downstream primer R1 shown in SEQ ID No.2 to carry out pcr amplification; The pcr amplification parameter is: 94 ℃ of denaturations 3 minutes, and then 30 seconds, 72 ℃ of 30 seconds, 58 ℃ annealing of 94 ℃ of sex change were extended 30 seconds, totally 38 circulations, last 72 ℃ were extended 10 minutes; Gained PCR product carries out 1.5% agarose gel electrophoresis;
B. result judgement: the X chromosome specific band (being X chromosome specific molecular marker sdX of the present invention) that only amplifies long 1422bp when the genomic dna from bolti to be measured, judge that this bolti to be measured is the raun in heredity, the sex chromosome genotype is XX; When the genomic dna from bolti to be measured, only amplify the Y chromosome specific band (being Y chromosome specific molecular marker sdY of the present invention) of long 982bp, judge that this bolti to be measured is the supermale fish in heredity, the sex chromosome genotype is YY; When the genomic dna from bolti to be measured, amplify simultaneously the X chromosome specific band of long 1422bp and the Y chromosome specific band of long 982bp, judge that this bolti to be measured is the milter in heredity, the sex chromosome genotype is XY.
The application aforesaid method carries out the genetic sex evaluation to 5 tail bolti raun XX, 5 tail bolti milter XY and 5 tail bolti supermale fish YY, the results are shown in Figure 2, in all XX individualities, all only amplified the X chromosome specific band of long 1422bp, in all YY individualities, all only amplified the Y chromosome specific band of long 982bp, and in the XY individuality, amplified simultaneously the X chromosome specific band of long 1422bp and the Y chromosome specific band of long 982bp, consistent with notional result.
The application aforesaid method carries out the genetic sex evaluation to 19 tail bolti XX ♀ * XX ♂ filial generation, the results are shown in Figure 3, in all boltis to be measured and contrast XX individuality, all only amplified the X chromosome specific band of long 1422bp, and in contrast XY individuality, amplified simultaneously the X chromosome specific band of long 1422bp and the Y chromosome specific band of long 982bp, in contrast YY individuality, only amplified the Y chromosome specific band of long 1422bp, illustrate that this 19 tail bolti to be measured is the XX raun in heredity, consistent with notional result.
The application aforesaid method carries out the genetic sex evaluation to 19 tail bolti XX ♀ * YY ♂ filial generation, the results are shown in Figure 4, in all boltis to be measured and contrast XY individuality, the X chromosome specific band of long 1422bp and the Y chromosome specific band of long 1070bp have all been amplified simultaneously, and in contrast XX individuality, only amplified the X chromosome specific band of long 1422bp, in contrast YY individuality, only amplified the Y chromosome specific band of long 982bp, illustrate that this 19 tail bolti to be measured is the XY milter in heredity, consistent with notional result.
The application aforesaid method carries out the genetic sex evaluation to 19 tail bolti YY ♀ * YY ♂ filial generation, the results are shown in Figure 5, in all boltis to be measured and contrast YY individuality, all only amplified the Y chromosome specific band of long 1422bp, and in contrast XX individuality, only amplified the X chromosome specific band of long 1422bp, in contrast XY individuality, the X chromosome specific band of long 1422bp and the Y chromosome specific band of long 982bp have been amplified simultaneously, illustrate that this 19 tail bolti to be measured is the YY supermale fish in heredity, consistent with notional result.
Three, the genetic linkage analysis in bolti sex specific molecular marker and sex determination site
3 XX ♀ * XY ♂ of Japanese strain bolti that this laboratory is introduced normally cultivate family and carry out linkage analysis.Each individual phenotypic sex confirms by tissue slice, and genetic sex adopts respectively bolti sex specific molecular marker sdX/sdY, NtX1/NtY2, marker2 to identify.Utilize JoinMAP4.0 to carry out the genetic linkage analysis of sex determination site (sex-determining loci, SD) and above sex specific molecular marker, the results are shown in Table 1 and Fig. 6.
The genetic linkage analysis in table 1 bolti sex specific molecular marker and sex determination site
Annotate: the individual individuality of having got rid of the natural sex reverse of restructuring; The LOD threshold value is 3.0; Genetic distance and LOD value are calculated by Joinmap4.0.
As shown in Table 1, bolti sex specific molecular marker sdX/sdY, NtX1/NtY2 and marker2 apart from the genetic distance in sex determination site be respectively 0,1.89,1.08cM, sex specific molecular marker sdX/sdY of the present invention obviously is better than the sub-mark of another two component.
Four, based on the sex specific molecular marker, the bolti of different sources is carried out to the genetic sex evaluation
Adopt sex specific molecular marker sdX/sdY of the present invention, to from Hainan (HN1, HN2), the 98 tail boltis (62 tail phenotype rauns and 36 tail phenotype milters) of 4 different lines of four tilapia nurseries of Guangxi (THS) and Guangdong (NG) carry out the genetic sex evaluation, result is shown as 59 tail rauns and 39 tail milters.With the phenotypic evaluation result, carry out the matching analysis, discovery has 5 coda gene type sexes and the phenotypic sex qualification result is misfitted, and wherein 4 tail phenotype rauns are accredited as the XY milter, and 1 tail phenotype milter is accredited as the XX raun; The bolti of 4 different lines, the identical rate of genetic sex and phenotypic sex is 90%~100%, and what the rate of coincideing was minimum is the HN2 family, and the highest is HN1 family (table 2), and the reason misfitted may be due to due to tilapia generation sex reversal.From the above results, sex specific molecular marker sdX/sdY of the present invention is applicable to the bolti of this Laboratory culture and the bolti of 4 different sources strains, has universality.
The genetic sex qualification result of 4 different sources family boltis of table 2
| Phenotypic sex | HN1(28) | HN2(22) | THS(25) | NG(23) |
| Raun | (19♀:0♂) | (13♀:1♂) | (13♀:2♂) | (13♀:1♂) |
| Milter | (0♀:9♂) | (1♀:7♂) | (0♀:10♂) | (0♀:9♂) |
| The |
100% | 93% | 87% | 93% |
| The |
100% | 88% | 100% | 100% |
| |
100% | 90% | 93% | 96% |
Five, based on the sex specific molecular marker, produce the method for supermale bolti
Based on sex specific molecular marker sdX/sdY of the present invention, carry out the evaluation of bolti genetic sex, the method for producing the supermale bolti comprises the following steps:
A. in bolti raun XX and milter XY post-coitum generation, carried out to the estradiol dipping bath in latter 5 days in hatching, the molecule marking method that adopts bolti genetic sex of the present invention to identify, from filtering out the conversion raun that the sex chromosome genotype is XY the sexual maturity female individuals;
B. XY is transformed to raun and the mating of bolti XY milter, the molecule marking method that adopts bolti genetic sex of the present invention to identify, from filtering out the supermale fish that the sex chromosome genotype is YY the sexual maturity offspring; Separately XY is transformed to raun and bolti XY milter post-coitum in hatching, carrying out the estradiol dipping bath in latter 5 days, the molecule marking method that adopts the bolti genetic sex to identify, from filtering out the conversion raun that the sex chromosome genotype is YY the sexual maturity female individuals;
C. YY supermale fish and YY are transformed to the raun mating, obtain full YY supermale fish;
D. YY supermale fish offspring is carried out to feminized treatment, obtain YY and transform raun;
E. repeating step C and D, transform the raun mating by YY supermale fish and YY and produce YY supermale fish.
After adopting aforesaid method to guarantee to continue acquisition YY supermale fish, by YY supermale fish and the mating of bolti XX raun, can produce in a large number complete male marketable fish.
Finally explanation is, above preferred embodiment is only unrestricted in order to technical scheme of the present invention to be described, although the present invention is described in detail by above preferred embodiment, but those skilled in the art are to be understood that, can to it, make various changes in the form and details, and not depart from the claims in the present invention book limited range.
Claims (3)
1. bolti Y chromosome specific molecular marker, is characterized in that, nucleotide sequence is as shown in SEQ ID No.4.
2. the molecule marking method identified of bolti genetic sex comprises the following steps:
A.PCR amplification: get the fin ray of bolti to be measured, extract genomic dna; The gained genomic dna of take is template, adopt the upstream primer shown in SEQ ID No.1 and the downstream primer shown in SEQ ID No.2, pcr amplification bolti sex specific molecular marker: the nucleotide sequence of X chromosome specific molecular marker is as shown in SEQ ID No.3, and the nucleotide sequence of Y chromosome specific molecular marker is as shown in SEQ ID No.4;
B. result judgement: from the genomic dna of bolti to be measured, only amplifying the X chromosome specific molecular marker, judge that this bolti to be measured is the raun in heredity, the sex chromosome genotype is XX; From the genomic dna of bolti to be measured, only amplifying the Y chromosome specific molecular marker, judge that this bolti to be measured is the supermale fish in heredity, the sex chromosome genotype is YY; From the genomic dna of bolti to be measured, amplifying simultaneously X chromosome specific molecular marker and Y chromosome specific molecular marker, judge that this bolti to be measured is the milter in heredity, the sex chromosome genotype is XY.
3. the molecule marking method that adopts the described bolti genetic sex of claim 2 to identify is produced the method for supermale fish, comprises the following steps:
A. in the post-coitum of bolti raun XX and milter XY generation, carried out to feminized treatment, the molecule marking method that adopts the bolti genetic sex to identify, filtering out the sex chromosome genotype is the conversion raun of XY;
B. XY is transformed to raun and the mating of bolti XY milter, the molecule marking method that adopts the bolti genetic sex to identify, from filtering out the supermale fish that the sex chromosome genotype is YY the offspring; Separately get XY conversion raun and bolti XY milter post-coitum for carrying out feminized treatment, the molecule marking method that adopts the bolti genetic sex to identify, filtering out the sex chromosome genotype is the conversion raun of YY;
C. YY supermale fish and YY are transformed to the raun mating, obtain full YY supermale fish;
D. YY supermale fish offspring is carried out to feminized treatment, obtain YY and transform raun;
E. repeating step C and D, transform the raun mating by YY supermale fish and YY and produce YY supermale fish.
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| CN110055335A (en) * | 2018-12-14 | 2019-07-26 | 中山大学 | A kind of microsatellite molecular marker primer, kit and rapid identification method identifying the female milter of star continent red tilapia |
| CN110250116A (en) * | 2019-08-05 | 2019-09-20 | 广东海洋大学 | A kind of method of quickly breeding YY supermale bolti |
| CN110938626A (en) * | 2019-12-12 | 2020-03-31 | 西南大学 | Specific molecular marker of sex chromosome of Oreochromis aureus, genetic sex identification based on molecular marker and method for producing unisex fish |
| CN112655600A (en) * | 2019-12-06 | 2021-04-16 | 海南勤富实业有限公司 | Method for quickly cultivating tilapia mossambica in early stage |
| CN116042863A (en) * | 2023-03-13 | 2023-05-02 | 内江师范学院 | Method for detecting nile tilapia allele expression level based on double-fluorescence-labeled probe |
| CN116804225A (en) * | 2023-07-24 | 2023-09-26 | 西部(重庆)科学城种质创制大科学中心 | Ji Shi tilapia sex chromosome specific molecular marker, detection primer, kit and application thereof |
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| CN110055335A (en) * | 2018-12-14 | 2019-07-26 | 中山大学 | A kind of microsatellite molecular marker primer, kit and rapid identification method identifying the female milter of star continent red tilapia |
| CN110055335B (en) * | 2018-12-14 | 2023-03-24 | 中山大学 | Microsatellite molecular marker primer, kit and rapid identification method for identifying female and male tilapia in stellera |
| CN110250116A (en) * | 2019-08-05 | 2019-09-20 | 广东海洋大学 | A kind of method of quickly breeding YY supermale bolti |
| CN112655600A (en) * | 2019-12-06 | 2021-04-16 | 海南勤富实业有限公司 | Method for quickly cultivating tilapia mossambica in early stage |
| CN110938626A (en) * | 2019-12-12 | 2020-03-31 | 西南大学 | Specific molecular marker of sex chromosome of Oreochromis aureus, genetic sex identification based on molecular marker and method for producing unisex fish |
| CN116042863A (en) * | 2023-03-13 | 2023-05-02 | 内江师范学院 | Method for detecting nile tilapia allele expression level based on double-fluorescence-labeled probe |
| CN116804225A (en) * | 2023-07-24 | 2023-09-26 | 西部(重庆)科学城种质创制大科学中心 | Ji Shi tilapia sex chromosome specific molecular marker, detection primer, kit and application thereof |
| CN116804225B (en) * | 2023-07-24 | 2024-02-13 | 西部(重庆)科学城种质创制大科学中心 | Ji Shi tilapia sex chromosome specific molecular marker, detection primer, kit and application thereof |
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