CN1715408A - Using pig slow contraction type troponin coded gene TNN 11 as genetic marker of pig productive character - Google Patents
Using pig slow contraction type troponin coded gene TNN 11 as genetic marker of pig productive character Download PDFInfo
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Abstract
The present invention belongs to the field of molecular biological technology and breeding of pit, and is especially the detection technology of single nucleotide polymorphism (SNP) of the third intron in the pig slow-twitch troponin 1 coding gene. The detection includes the following steps: extracting genome DNA from pig blood, designing primer, PCR proliferation, PCR product cloning, sequencing, sequence comparison and analysis, detecting single nucleotide polymorphism (SNP), and analysis of marker and character correlativity. The present invention discloses the DNA sequence of the third intron in the pig slow-twitch troponin 1 coding gene and the SNP typing detecting technology, and provides new marker for the auxiliary molecular marker selection of pig.
Description
Technical field
The present invention relates to Protocols in Molecular Biology and the breeding field of pig, be specifically related to detection method pig and mutational site production traits genes involved TNNI1 gene the 3rd intron.
Background technology
The breeding value that phenotypic number by the production traits estimates is carried out animal selection breeding, has promoted the genetic improvement of Livestock Production proterties greatly.Since the nineties, along with the progress of Protocols in Molecular Biology and in the pig Application for Field, progressively having occurred is the molecular marker assisted selection and the infiltration equimolecular breeding technique of core with the molecule marker, and these technology combine with conventional breeding, have quickened the pig breeding process greatly.The gene or the mark that can be applied to molecular marker assisted selection must have bigger genetic contribution to objective trait, be major gene or mark, therefore seeking prerequisite and the basis that these major genes and closely linked with it molecule marker become molecular marker assisted selection, also is the research emphasis and the urgent problem of for some time pig biology field at present and in the future.
Have a plurality of being found and applying for a patent of functional gene inside that are positioned at present with the closely linked molecule marker of the production traits.For example, at traditional pig breeding in the works, because the human consumer to the interest of lean meat, therefore selects mainly to emphasize to reduce fat.Fat reduces mainly to reduce with the thickness of backfat to be weighed.Yet the thickness of backfat descends and has caused the decline of intramuscular fat equally, and the last deposition site of fat is a muscle, so the acceptance level of intramuscular fat and taste and muscle is proportionate.For preventing that intramuscular fat from further descending, must find the molecule marker that influences this proterties, because intramuscular fat is difficult in the live body vacuum metrics.Gerbens etc. have confirmed to be arranged in the relation of muscle tissue special candidate gene heart fat acid binding protein and pig intramuscular fat content and other production traits on No. 6 karyomit(e)s of pig, and this gene has been applied patent, and its patent No. is WO 97/35878; In addition, Rothschild etc. have found the molecule marker relevant with lean ratio in the leptin acceptor gene, and its patent No. is US.Pat.Nos.5972621.
According to ATP enzyme group method, myofiber is divided into I type (slow contraction type) and II type (fast shrinkage type) myofiber two big main types (Staronet al.1986.Correlation between myofibrillar ATPase activity and myosin heavy chain composition in rabbitmuscle fibers.Histochemistry.86:19-23).I fiber type sarcoplasm myohaemoglobin and cytopigment are many, and the vascularity density around the myofiber is big, have higher line plastochondria enzyme concn, and sarcostyle ATP enzyme and Starch phosphorylase activity is low, only can carry out the aerobic oxidation metabolism, and is corresponding with red muscle fiber; The IIA fiber type can carry out glycolysis in the II type, can carry out aerobic oxidation again, is osculant; The IIB fiber type only can carry out the glycolysis metabolism, corresponding with white muscle fiber (Karlsson et al.1999.Skeletal muscle fibres as factors for pork quality.Livest Prod Sci.3:255-269).I type (red muscle fiber) is than II type (white muscle fiber) fiber finer, and a little less than the acid producing ability, pH value and lipid content are higher, improves muscle I fiber type ratio and helps improving yellowish pink, tender degree and succulence.
The troponin complex body belongs to independently multigene family, and it and tropomyosin and Actin muscle-actomyosin sarcostyle interacts and participated in Ca
2+The voluntary muscle of mediation shrinks.This complex body comprises 3 protein that are closely connected: TnC (TnC), Troponin I (TnI) and TnT (TnT), its expression product all shows the myofiber specificity.TnI is an actin binding protein, and the TnI gene family comprises 3 hypotypes: 2 skeletal muscle hypotypes, that is: fast shrinkage type of TnI-and TnI-slow contraction type, 1 myocardium hypotype, that is: TnI-heart-type.(1990.cDNA sequence such as Wade, tissue-specific expression, and chromosomal mapping of the hunan slow-twitchskeletal muscle isoform of troponin I.Genomics.7:346-357) at first isolated the cDNA full length sequence that the people shrinks skeletal muscle TNNI1 gene slowly, as if with this cDNA is tissue specificity regulation and control and developmental regulation in probe in detecting rodent and the people sarcoplast, found that the TNNI1 signal only is confined to contain in the muscle tissue of slow contraction type skeletal muscle fiber.
Biologically, the production traits is embodied in the particular organization of animal, such as, muscle tissue is corresponding to lean meat production.Therefore, in improvement of breed in the works, the selective pressure of various levels all can put in the different tissues.And also do not disclose fully about the relation between specific expression gene in the different tissues and the individual production performance.The invention provides interior heritable variation of muscle specific expressing gene-slow contraction type muscle troponin (TNNI1) encoding gene the 3rd intron and the relation between pig growth, trunk and the meat production traits.
Summary of the invention
The portion gene group dna sequence dna that the objective of the invention is to clone pig TNNI1 gene is sought the mutational site of TNNI1 gene and the detection method of gene pleiomorphism, for the molecular breeding of pig provides assisted selection method.
The invention provides the genome nucleotide sequence that Large White, landrace, Tongcheng pig, peaceful pig and painted face in Beijing opera pig comprise the 455bp of pig TNNI1 gene the 3rd intron, its sequence such as SEQ ID NO.1, SEQ ID NO.2, SEQ ID NO.3, SEQ ID NO.4 is shown in the SEQ ID NO.5; Carrying out Cluster W comparison by the above-mentioned sequence of 5 pig kinds (Large White, landrace, Tongcheng pig, peaceful pig and painted face in Beijing opera pig) provides the 5 place's single nucleotide polymorphism (SNP) that are positioned at this 455bp amplified fragments inside, and its SNP site as shown in Figure 1.
The step for preparing this gene fragment is as follows: selecting three place of china kinds (Tongcheng pig, peaceful pig and painted face in Beijing opera pig) and 2 external (abroad) kinds (Large White, landrace) is test materials, from pig blood, extract DNA, according to pig TNNI1 gene cDNA sequence (GeneBank accession number: AY282922), the design primer, its sequence is respectively shown in sequence table SEQ IDNO.6 and SEQ ID NO.7, pcr amplification, PCR product purification, cloning and sequencing, sequence comparing analysis.
The invention provides XbaI-RFLP (restriction fragment length polymorphism) the genotyping method of identifying the above-mentioned sequence 383bp C/T of place variation.Its step comprises: according to pig TNNI1 gene cDNA sequence (GeneBank accession number: AY282922) with the above-mentioned SEQ ID NO.1-SEQ ID NO.5 sequence that is obtained, the design primer, its primer sequence is respectively shown in sequence table SEQ ID NO.8 and SEQ IDNO.9, in the pig genomic dna, carry out pcr amplification, pcr amplified fragment XbaI enzyme cutting somatotype and detection.
The present invention further provides and utilized definite different genotype individuality of XbaI-RFLP method and the correlationship between the production traits.
Sequence table, description of drawings
1, sequence table SEQ ID NO.1: the nucleotide sequence that is external pig kind " Large White ";
2, sequence table SEQ ID NO.2: the nucleotide sequence that is external pig kind " landrace ";
3, sequence table SEQ ID NO.3: the nucleotide sequence that is Chinese Pigs kind " Tongcheng pig ".
4, sequence table SEQ ID NO.4: the nucleotide sequence that is Chinese Pigs kind " peaceful pig ".
5, sequence table SEQ ID NO.5: the nucleotide sequence that is Chinese Pigs kind " painted face in Beijing opera pig ".
6, sequence table SEQ ID NO.6: be the used forward primer of preparation SEQ ID NO.1-SEQ ID NO.5 specific gene fragment.
7, sequence table SEQ ID NO.7: be the used reverse primer of preparation SEQ ID NO.1-SEQ ID NO.5 specific gene fragment.
8, sequence table SEQ ID NO.8: be the forward primer of implementing pig TNNI1 gene the 3rd intron C/T variation XbaI-RFLP (restriction fragment length polymorphism) genotyping method.
9, sequence table SEQ ID NO.9: be the reverse primer of implementing pig TNNI1 gene the 3rd intron C/T variation XbaI-RFLP (restriction fragment length polymorphism) genotyping method.
Fig. 1: five pig kind TNNI1 gene order comparison results and SNP site.
Fig. 2: the gene fragment agarose gel electrophoretogram that comprises pig TNNI1 gene the 3rd intron.
Sepharose concentration is 1.5%; M swimming lane: DNA Marker DL2,000; Swimming lane 1-4 represents sequence table SEQ ID NO.6 and the amplified fragments of primer shown in the SEQID NO.7 in different pig kinds, and clip size is 455bp.
Fig. 3: TNNI1 gene XbaI-RFLP detected result.
Agarose gel concentration is 2.5%; Swimming lane M is DL 2000 Markers; 1,4,5,8,9 swimming lanes are the AA genotype, 188bp; 3,7 swimming lanes are the AB genotype, 188bp, 111bp, 77bp; 2,6 swimming lanes are the BB genotype, 111bp, 77bp.
The method according to this invention can be used for being developed to diagnostic method or kit, thereby utilizes these methods to select to carry favourable allelic pig in breeding plan, selects preferably effect thereby can reach.
Embodiment
Embodiment 1; The acquisition of gene fragment and the foundation of pleiomorphism detecting method
Selecting 2 external pig kinds (Large White, landrace) and 3 Chinese Pigs kinds (Tongcheng pig, peaceful pig, painted face in Beijing opera pig) is test materials, according to pig TNNI1 gene cDNA sequence (GeneBank accession number: AY282922), design following primer, primer sequence is as follows:
Forward primer F
1: TCACTGCCTCCCGCAAACT
Reverse primer R
1: GAGCCTTCTCAGCCTCTCGC
In five pig kinds (Large White, landrace, Tongcheng pig, peaceful pig and painted face in Beijing opera pig) genomic dna, carry out pcr amplification with this primer, the PCR reaction system is 25 μ l, wherein template DNA is 50ng, dNTPs concentration is 200 μ mol/L, every primer concentration is 0.4 μ mol/L, (Biostar International Canada), adds deionized water to cumulative volume 25 μ l to the Taq archaeal dna polymerase of 3U; PCR response procedures: 94 ℃ of pre-sex change 4min; 94 ℃ of sex change 50s, 64 ℃ of annealing 50s, 72 ℃ of extensions 1min, totally 35 circulations then; Last 72 ℃ are extended 10min.
Behind the PCR product of different pig kinds purified (UNIQ-10 pillar DNA glue reclaims test kit and gives birth to worker biotech company available from Shanghai), the clone, carry out sequencing, sequencing is given birth to worker biotech company by Shanghai and is finished.The PCR product sequence of different pig kinds is carried out sequence alignment through ClusterW software, and comparison result is seen Fig. 1 between sequence.Above-mentioned amplified fragments size is 455bp, co-exists in 5 nucleotide variations, and the C/T variation that wherein is arranged in this segmental 383bp place has showed, outer pig difference between species, and has caused XbaI enzyme cutting site (↓ TCTAGA) polymorphism.In view of the above, design following primer, and adopt the XbaI-RFLP method to carry out the SNP somatotype, primer sequence is as follows:
Forward primer F
2: GAGTGGTAGGAGATTGACGGA
Reverse primer R
2: GTAGCGAGCCTTCTCAGCC
The PCR reaction system is 20 μ l, and wherein template DNA is 50ng, and dNTPs concentration is 200 μ mol/L, and every primer concentration is 0.5 μ mol/L, and (Biostar International Canada), adds deionized water to cumulative volume 25 μ l to the Taq archaeal dna polymerase of 1U; The PCR response procedures is: 94 ℃ of pre-sex change 4min; 94 ℃ of sex change 50s, 60 ℃ of annealing 50s, 72 ℃ of extensions 1min, totally 35 circulations then; Last 72 ℃ are extended 10min.
Get that 8.5 μ l PCR products add 0.5 μ l (10U/ μ l) restriction enzyme and 1 μ l, 10 * buffer (contains 10 * BSA), 37 ℃ of XbaI enzyme cutting 4h, get 5 μ l enzymes and cut product with agarose or polyacrylamide gel electrophoresis detection, under ultraviolet lamp or silver dye that the back is observed and the record enzyme is cut the result.This amplified fragments size is 188bp, the XbaI enzyme cutting pleomorphism site is positioned at this segmental 111bp place, if the base at 111bp place is C, then there is not the Xbal restriction enzyme site, have only a 188bp fragment (A allelotrope) with the XbaI enzyme cutting detected result, when this site was T, the result caused the generation of an Xbal restriction enzyme site, enzyme is cut and is obtained two fragments, and length is respectively 111bp and 77bp (B allelotrope).
Embodiment 2: the polymorphism of molecule marker in different swinerys distributes
Detect the XbaI-RFLP polymorphism of pig TNNI1 the 3rd intron in 3 external swinerys (Large White, landrace, duroc) and 6 Chinese swinerys (Tongcheng pig, peaceful pig, eight eyebrow pigs, Huainan pig, plum mountain pig, painted face in Beijing opera pig), detected result is as shown in table 1.In the several pig kinds that detected, Da Bai, the long white and allelic gene frequency of the dominant A of duroc group are respectively 0.804,0.825 and 0.883, and the allelic gene frequency of B of advantage is respectively 1,0.865,0.679 and 0.636 in painted face in Beijing opera, Mei Shan, the peaceful and eight eyebrow pigs, A allelotrope and the allelic frequency of B are approaching in Tongcheng pig and Huainan pig, and the allelic gene frequency of A is respectively 0.522 and 0.52.
The distribution results of table 1 TNNI1 gene XbaI enzyme cutting polymorphism in different pig kinds
Kind | Quantity | The AA genotype | The AB genotype | The BB genotype | The A gene frequency | The B gene frequency |
The peaceful pig eight eyebrow pig Huainan Swine plum mountain pig Erhualians of Large White Landrace duroc Tongcheng pig | 28 20 30 23 28 11 25 26 36 | 17 13 23 5 3 1 7 0 0 | 11 7 7 12 12 6 10 7 0 | 0 0 0 6 13 4 8 19 36 | 0.804 0.825 0.883 0.478 0.321 0.364 0.480 0.135 0 | 0.196 0.175 0.117 0.522 0.679 0.636 0.520 0.865 1 |
Embodiment 3: the association analysis of the molecule marker and the production traits
In order to determine whether the TNNI1 gene pleiomorphism is relevant with the pig phenotypic difference, 295 Da Bai * Mei Shan F2 that selects pig genetics and breeding key lab of the Ministry of Agriculture of Hua Zhong Agriculture University to set up is a test materials for resource colony, the XbaI-RFLP method that adopts embodiment 2 to be set up is carried out polymorphism and is detected, and analyzes the correlationship of pig TNNI1 gene XbaI-PFLP different genotype and pig production character.Adopt SAS statistical software (SASInstitute Inc, Version 8.0) glm program to carry out single mark variance analysis, adopt the reg program to calculate additive effect of gene and dominant effect simultaneously, and carry out test of significance, the model that adopts is:
Y
ijkl=μ+G
i+F
j+S
k+Y
l+b
ijklX
ijkl+e
ijkl
Y
IjBe the proterties phenotypic number, μ is a mean value, G
iFor the genotype effect (comprises additive effect of gene and dominant effect; Additive effect is represented AA, AB and BB genotype respectively with-1,0 and 1, and dominant effect is with 1, and-1 and 1 represents AA, AB and BB genotype respectively); S
k, Y
l, F
jBe fixed effect, be respectively sex, year, family effect, b
IjklFor slaughter weight or butcher the regression coefficient of age in days, carcass trait is concomitant variable with the slaughter weight, and the meat proterties is a concomitant variable to butcher age in days, and concomitant variable is not considered in growth; e
IjklBe the residual error effect.
295 that are detected big * plum F2 for individuality in, the AA genotype has 74, the AB genotype has 154, the BB genotype has 67.Statistic analysis result between the different genotype and the production traits is summarized in table 2 and 3.
As can be seen from Table 2, the XbaI-RFLP genotype not simultaneously, birth weight, skin rate, bone rate, fat meat rate, thin fertile ratio, eye muscle height, eye muscle area, thickness of backfat proterties exist significantly or utmost point significant difference.This site between birth weight, skin rate, bone rate, fat meat rate, thin fertile ratio, eye muscle area, 6-7 lumbar vertebrae between the thickness of backfat and chest lumbar vertebrae the thickness of backfat mainly based on the additivity mode of action, but effect direction and interracial phenotypic effect and not quite identical.The A allelotrope that derives from the Da Bai kind is reducing between fat meat rate, 6-7 lumbar vertebrae between the thickness of backfat and chest lumbar vertebrae in the thickness of backfat, birth weight and thin fertile ratio have been improved, this is consistent with Da Bai kind phenotypic effect direction, and opposite with the variety effect direction on skin rate, bone rate, eye muscle area character.This site dominant effect on the shoulder thickness of backfat and the high proterties of eye muscle is remarkable, is respectively-0.099 ± 0.041 and-0.142 ± 0.047.
The statistical analysis table of table 2 TNNI1 gene XbaI-RFLP genotype and growth, carcass trait
Proterties | The TNNI1-XbaI-RFLP genotype (μ ± SE) | Genetic effect (μ ± SE) | |||
The AA genotype | The AB genotype | The BB genotype | Additive effect | Dominant effect | |
The long rib of the birth weight dressing percentage skin rate bone rate lactones rate fat meat thin fertile ratio trunk of rate lean meat percentage is counted between the average skin depth shoulder of the eye muscle height eye muscle area thickness of backfat chest lumbar vertebrae thickness of backfat between the average thickness of backfat triadic mean of thickness of backfat buttocks thickness of backfat 6-7 lumbar vertebrae | 1.190±0.026 a 71.679±0.504 10.639±0.212 Aa 13.416±0.254 2.963±0.074 20.891±0.52 A 54.912±0.431 2.961±0.105 Aa 91.398±0.482 14.729±0.084 8.582±0.094 a 28.052±0.539 a 0.389±0.011 3.546±0.083 ab 1.957±0.062 a 1.794±0.072 2.418±0.064 2.686±0.068 a | 1.145±0.018 ab 72.078±0.344 10.191±0.144 ABa 13.046±0.174 3.065±0.051 21.838±0.355 AB 54.861±0.294 2.739±0.071 ABa 91.158±0.329 14.695±0.058 8.864±0.064 b 29.149±0.368 ab 0.391±0.008 3.395±0.057 a 2.007±0.043 ab 1.832±0.049 2.399±0.044 2.702±0.046 a | 1.098±0.027 b 72.058±0.532 9.516±0.222 Bb 12.712±0.268 2.980±0.078 23.031±0.549 B 54j34±0.454 2.474±0.11 Bb 90.354±0.508 14.700±0.089 8.573±0.099 a 30.064±0.569 b 0.373±0.012 3.638±0.088 b 2.138±0.066 b 1.798±0.076 2.524±0.067 2.901±0.072 b | -0.047±0.019 * 0.204±0.374 -0.570±0.157 ** -0.372±0.188 * -0.013±0.055 1.070±0.386 ** -0.260±0.318 -0.243±0.078 ** -0.513±0.357 -0.013±0.063 -0.006±0.07 1.033±0399 * -0.008±0.008 0.045±0.062 0.092±0.046 * -0.002±0.054 0.053±0.047 0.107±0.05 * | -0.000±0.013 -0.113±0.250 -0.052±0.105 0.020±0.126 -0.050±0.037 -0.061±0.258 -0.135±0.213 -0.011±0.052 -0.146±0.239 0.009±0.042 -0.142±0.047 ** -0.061±0.267 -0.005±0.005 -0.099±0.041 * -0.020±0.031 -0.018±0.036 -0.036±0.032 0.046±0.034 |
Annotate: above numerical value is least square mean value standard error; Contain same letter and represent that difference is not remarkable, the lowercase alphabet differential is different significantly, and capitalization represents that difference is extremely remarkable; The additive effect negative value represents that B allelotrope reduces the proterties phenotypic number:
*Expression p<0.05,
*Expression p<0.01 (following table together).
As can be seen from Table 3, during TNNI1 gene XbaI-RFLP different genotype, biceps muscle of thigh pH value and longissimus dorsi muscle colour significant difference, longissimus dorsi muscle pH value difference heteropole significance.For longissimus dorsi muscle muscle pH value, this site additive effect and dominant effect are all remarkable, are respectively-0.031 ± 0.016 and 0.022 ± 0.011; Longissimus dorsi muscle muscle colour additive effect is remarkable, and its value is 0.558 ± 0.257; The A allelotrope that derives from the Da Bai kind has improved longissimus dorsi muscle muscle pH value, has reduced longissimus dorsi muscle muscle colour simultaneously.
The statistical analysis table of table 3 TNNI1 gene XbaI-RFLP genotype and meat proterties
Proterties | The TNNI1-XbaI-RFLP genotype (μ ± SE) | Genetic effect (μ ± SE) | |||
The AA genotype | The AB genotype | The BB genotype | Additive effect | Dominant effect | |
Longissimus dorsi muscle pH biceps muscle of thigh pH complexus pH percentage of water loss is waterpower longissimus dorsi muscle colour biceps muscle of thigh colour longissimus dorsi muscle marble grain biceps muscle of thigh marble grain intramuscular fat intramuscular moisture | 6.394±0.021 Aa 6.448±0.015 a 6.443±0.015 6.202±0.441 91.587±0.609 19.818±0.347 a 19.145±0.134 3.449±0.022 4.129±0.021 3.154±0.065 73.883±0.089 | 6.318±0.015 Bb 6.406±0.010 b 6.448±0.010 6.905±0.302 90.554±0.417 20.435±0.237 ab 19.132±0.092 3.412±0.015 4.106±0.014 3.128±0.044 73.728±0.061 | 6.331±0.023 ABb 6.416±0.016 ab 6.434±0.015 6.846±0.466 90.717±0.644 20.932±0.367 b 19.334±0.142 3.402±0.023 4.086±0.022 3.075±0.068 73.804±0.094 | -0.031±0.016 * -0.016±0.011 -0.004±0.011 0.321±0.327 -0.435±0.451 0.558±0.257 * 0.096±0.099 -0.024±0.016 -0.022±0.015 -0.038±0.048 -0.040±0.066 | 0.022±0.011 * 0.013±0.008 -0.005±0.007 -0.190±0.220 0.299±0.304 -0.031±0.173 0.053±0.067 0.007±0.011 0.001±0.010 -0.008±0.032 0.058±0.044 |
Sequence table SEQ UENCE LISTING
<110〉Hua Zhong Agriculture University
<120〉pig slow contraction type troponin encoding gene TNNI1 is as the genetic marker of pig production character
<130>
<141>2004-06-25
<160>9
<170>PatentIn version 3.1
<210>1
<211>455
<212>DNA
<213〉pig (Sus scrofa)
<220>
<221>gene
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tcactgcctc ccgcaaactc ctgctgaagg tgtgctgggt cctggttttg gggagatgtc 60
caggggaggc agaggggcac agggcagcct tgggggttgg gggaagggtc atgggagggt 120
gacagggggc caaagcctgg gaggaggcag gaccagcttc agggcacaat cccccatctc 180
ccgatctccc aatctcccaa tctcccagtg ggagcctggg agaagagctt tattttgcta 240
agagtctttg aagctctggg ggcgcaaaga gagtggtagg agattgacgg acaggagaga 300
aagaggaaga ctgaggccag ctcggtccag ctgggctctg cctttcctgc gggctggccc 360
cctcacctgg ctctgtccca tccagagcct gatgctggcc aaggccaagg agtgctggga 420
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gacagggggc caaagcctgg gaggaggcag gaccagcttc agggcacaat cccccatctc 180
ccgatctccc aatctcccaa tctcccagtg ggagcctggg agaagagctt tattttgcta 240
agagtctttg aagctctggg ggcgcaaaga gagtggtagg agattgacgg acaggagaga 300
aagaggaaga ctgaggccag ctcggtccag ctgggctctg cctttcctgc gggctggccc 360
cctcacctgg ctctgtccca tccagagcct gatgctggcc aaggccaagg agtgctggga 420
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ggcagggggc caaagcctgg gaggaggcag gaccagcttx agggcacaat cccccatctc 180
ccgatctccc aatctcccaa tctcccagtg ggagcctggg agaagagctt tattttgcta 240
agagtctttg aagctctggg ggcgcaaaga gagtggtaggagattgacgg acaggagaga 300
aagagggaga ctgaggccag ctcggtccag ctgggctctg cctttcctgx gggctggccc 360
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gacagggggc caaagcctgg gaggaggcag gaccagcttc agggcacaat cccccatctc 180
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aagaggaaga ctgaggccag ctcggtccag ctgggctctg cctttcctgc gggctggccc 360
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acagggggc caaagcctgg gaggaggcag gaccagcttc agggcacaat cccccacctc 180
ccgatctccc aatctcccaa tctcccagtg ggagcccggg agaagagctt tattttgcta 240
agagtctttg aagctctggg ggcgcaaaga gagtggtagg agattgacgg acaggagaga 300
aagaggaaga ctgaggccag ctcggtccag ctgggctctg cctttcctgc gggctggccc 360
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<220>
<221>gene
<222>(1)..(19)
<223>
<400>6
tcactgcctc ccgcaaact 19
<210>7
<211>20
<212>DNA
<213〉pig (Sus scrofa)
<220>
<221>gene
<222>(1)..(20)
<223>
<400>7
gagccttctc agcctctcgc 20
<210>8
<211>21
<212>DNA
<213〉pig (Sus scrofa)
<220>
<221>gene
<222>(1)..(21)
<223>
<400>8
gagtggtagg agattgacgg a 21
<210>9
<211>19
<212>DNA
<213〉pig (Sus scrofa)
<220>
<221>gene
<222>(1)..(19)
<223>
<400>9
gtagcgagcc ttctcagcc 19
Claims (5)
1, comprise the specific gene fragment of pig slow contraction type troponin encoding gene TNNI1 the 3rd intron, its nucleotide sequence is shown in sequence table SEQ ID NO.1, SEQ ID NO.2, SEQ ID NO.3, SEQ IDNO.4, SEQ ID NO.5.
2, according to the described dna sequence dna of claim 1, the primer sequence that obtains this dna sequence dna is shown in sequence table SEQ ID NO.6 and SEQ ID NO.7.
3, according to the described dna sequence dna of claim 1, it is characterized in that: there is a base mutation C383-T383 at sequence table SEQ ID NO.1, SEQID NO.2, SEQ ID NO.3, SEQ ID NO.4, SEQ ID NO.5 sequence 383 bit base places, cause Xba I-RFLP polymorphism.
4, a kind of molecular marker method of screening pig production character, according to following steps:
From pig blood, extract genomic dna, according to the sequences Design primer shown in pig TNNI1 gene cDNA sequence and the sequence table SEQ ID NO.1-SEQ ID NO.5, the sequence of this primer is shown in sequence table SEQ IDNO.8 and SEQ ID NO.9, in the pig genomic dna, carry out pcr amplification, pcr amplified fragment XbaI enzyme cutting somatotype and detection with this primer.
5, each described pig production character genes involved TNNI1 application in the pig marker assisted selection of claim 1-4.
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Cited By (3)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
CN102146372A (en) * | 2011-01-24 | 2011-08-10 | 四川农业大学 | Method for cloning complete sequence of goat TNNC2 gene coding region |
CN107058543A (en) * | 2017-04-26 | 2017-08-18 | 山东农业大学 | Distinguish primer and its application of animal muscle protein TNNC1 genes |
CN107130037A (en) * | 2017-06-02 | 2017-09-05 | 西北农林科技大学 | The method and dedicated kit of a kind of TNNI1 genes auxiliary detection ox Growth and carcass character |
Families Citing this family (1)
Publication number | Priority date | Publication date | Assignee | Title |
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CN105969880B (en) * | 2016-06-21 | 2020-08-07 | 北京农学院 | Quadruple PCR (polymerase chain reaction) detection method for meat components and application |
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Cited By (5)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
CN102146372A (en) * | 2011-01-24 | 2011-08-10 | 四川农业大学 | Method for cloning complete sequence of goat TNNC2 gene coding region |
CN102146372B (en) * | 2011-01-24 | 2012-09-05 | 四川农业大学 | Method for cloning complete sequence of goat TNNC2 gene coding region |
CN107058543A (en) * | 2017-04-26 | 2017-08-18 | 山东农业大学 | Distinguish primer and its application of animal muscle protein TNNC1 genes |
CN107058543B (en) * | 2017-04-26 | 2021-02-05 | 山东农业大学 | Primer for distinguishing animal muscle protein TNNC1 gene and application thereof |
CN107130037A (en) * | 2017-06-02 | 2017-09-05 | 西北农林科技大学 | The method and dedicated kit of a kind of TNNI1 genes auxiliary detection ox Growth and carcass character |
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