牛TLR4基因5′侧翼区的遗传变异与乳房炎的关联

TLR4基因通过识别病原体激活免疫细胞, 在天然免疫和适应性免疫防御中起着重要的作用。以中国荷斯坦奶牛、三河牛和中国西门塔尔牛为研究对象, 扩增477 bp的目的片断, 测序后发现扩增片段的245 bp处G→C的转换使得MspⅠ酶切位点产生, 形成新的等位基因。因此采用RFLP-MspⅠ方法检测该等位基因的多态性, 结果表明, 在3个群体中A、B两个等位基因均有分布, 处于中度多态。经c²适合性检验, 三河牛在该位点未达到Hardy-Weinberg平衡状态(P<0.05)。利用SAS 8.2软件采用最小二乘法拟合线性模型将该基因座不同基因型与奶牛乳房炎进行了关联分析, 结果表明品种和泌乳月效应对乳房炎的影响较大, 各基因型效应差异均不显著(P>0.05)。     

奶牛TLR4基因的多态性与乳房炎的相关性研究

TLR4通过识别病原体而激活免疫细胞,在先天免疫和适应性免疫防御中起着重要作用。以中国荷斯坦奶牛、三河牛和中国西门塔尔牛为研究对象,以TLR4为乳房炎抗性的候选基因,分别扩增316bp和382bp2个片段,分别采用SSCP和RFLP-AluⅠ方法来检测TLR4基因的多态性。结合测序发现:在intron1的第4,525bp处的A→G的突变,和exon3的第1,397bp处的T→C突变,使得产生多态。2个位点的A、B等位基因在3个群体中都有分布,且处于中度多态。χ2适合性检验表明,3个群体在这2个位点的突变达到Hardy-Weinberg平衡状态(P>0.05)。运用SAS8.0软件采用最小二乘法拟合线性模型,将基因座不同基因型与奶牛乳房炎进行了关联分析,结果表明:T4CRBR1的AA基因型为乳房炎抗性基因型(P<0.05),A等位基因为乳房炎抗性的有利基因,T4CRBR2的各基因型个体间的体细胞评分差异不显著(P>0.05)。     

TNF-α基因多态性及其与奶牛乳房炎的相关性分析

以417头中国荷斯坦奶牛为研究对象,根据体细胞评分(Somatic cell score,SCS)的大小将该奶牛群体划分为感染牛群(100头)和健康牛群(317头)。通过PCR-RFLP和CRS-RFLP方法检测了肿瘤坏死因子α(Tumor necrosis factor-alpha,TNF-α)基因在荷斯坦奶牛群体中的多态性,并分析这些多态位点和奶牛乳房炎的相关性。研究发现了3个单核苷酸多态位点(Single-nucleotide polymorphism,SNP):第2外显子39bp处G→A的突变;第4外显子293bp处C→T的突变;5′侧翼区(5′-flanking region,5′UTR)C→G的突变。这3个突变位点分别是DraⅠ、AfaⅠ和DdeⅠ限制性内切酶的酶切多态位点,其中DraⅠ为创造酶切位点。经过基因型分析与χ2检验表明:3个酶切多态位点在荷斯坦奶牛群中均未达到Hardy-Weinberg平衡状态。运用SPSS13.0软件,采用最小二乘拟合线性模型分析3个酶切多态位点与SCS的关系,结果表明:AA基因型个体在DraⅠ酶切位点中的SCS显著大于BB及AB基因型个体(P0.05),BB基因型表现出乳房炎抗性。AfaⅠ酶切位点中BB基因型个体的SCS显著大于AA及AB基因型个体(P0.05),AA基因型表现出乳房炎抗性。DdeⅠ酶切位点中,AB基因型个体的SCS显著低于AA基因型个体(P0.05),AB基因型为优良基因型。因此BB、AA、AB基因型分别为DraⅠ、AfaⅠ、DdeⅠ酶切位点中的优良基因型,可作为分子标记应用于奶牛乳房炎抗性筛选。     

CXCR2基因多态性与奶牛乳房炎和乳品质的关联

采用PCR-SSCP技术研究了荷斯坦牛、西门塔尔牛和通江黄牛3个品种共160头个体CXCR2基因多态性与乳房炎抗性性状和对牛奶品质性状的遗传效应。结果表明: CXCR2基因有3个SNP多态位点, 分别位于序列的第685 bp、777 bp和861 bp位点, 确定了5个等位基因A、B、C、E和F。685 bp位点表现为BC和CC基因型, 777 bp位点表现为AA和AB基因型, 861 bp位点为CC和BC基因型。与奶牛乳房炎敏感性有关的基因型主要是BC、CC和FF, 可能对乳房炎有抗性的是AA、AB和EE基因型。据不同基因型对乳品质的遗传效应分析来看, AA、AB和EE基因型的乳品质性状极显著或显著优于其他基因型。     

荷斯坦牛Nramp1基因遗传多态性及其与乳房炎相关性的研究

利用PCR-SSCP技术检测了344头中国荷斯坦牛Nramp1基因exon 11的基因多态性, 并分析了其不同基因型与乳房炎及产奶量性状的关系。结果表明: 实验群体发现3种基因型AA、AB、BB, 其中A等位基因为优势等位基因, 等位基因频率为0.767, 而B等位基因频率则为0.233。经χ2适合性检验, 群体处于Hardy-Weinberg平衡状态(P>0.05)。测序结果显示: 扩增片段分别在200 bp(C/G)和254 bp(T/G)存在碱基突变, 并导致了氨基酸改变, 分别为丙氨酸替换为脯氨酸(Ala356Pro)、亮氨基酸替换为蛋氨酸(Leu374Met)。通过构建最小二乘线性模型, 进行Nramp1基因多态性与产奶量、体细胞评分(SCS)的相关性分析表明, AA型个体的SCS最小二乘均值显著低于BB﹑AB型(P<0.05), 而AA型﹑AB个体的产奶量最小二乘均值显著高于BB型(P<0.01, P<0.05), AA基因型可作为乳房炎抗性的优良基因型。因此, 可将Nramp1作为奶牛乳房炎候选基因应用于分子标记辅助选择育种。     

κ中国荷斯坦奶牛κ-酪蛋白基因第四外显子多态性与产奶性状的关联分析

摘要: 以544头中国荷斯坦奶牛为研究对象, 以k-酪蛋白基因为产奶性状的候选基因, 扩增779 bp的片段, 结合测序结果采用PCR-RFLP方法来检测k-酪蛋白基因3个位点的多态性。结果在exon 4的第10 891 bp、10 927 bp和10 988 bp处分别发生了T/C、C/A错义突变和G/A同义突变, 据此分别选择了TaqⅠ、HindⅢ、 PstⅠ等 3种限制性内切酶检测了其多态性。发现3个位点的A、B等位基因在群体中都有分布, 且处于低度多态; A 和B 等位基因的频率分别为86.03%和13.97%; AA, AB和BB基因型频率分别为73.71%, 24.63%和1.66%; c2适合性检验表明, 该群体在这3个位点的突变达到Hardy-Weinberg平衡状态(P > 0.05); BB和AB基因型个体乳脂率显著高于AA基因型个体(P<0.05), AB基因型个体脂蛋白比显著高于AA基因型个体(P < 0.05), 但不同基因型对产奶量和乳蛋白率没有显著影响; 3个位点的酶切多态性在所研究群体中是紧密连锁的。说明在中国荷斯坦奶牛群体中, κ-酪蛋白B等位基因可作为改良奶牛乳脂率性状的分子遗传标记。     

牛α1-AT基因5’侧翼区新SNPS的鉴定及其与产奶性状的相关性

以中国荷斯坦奶牛(Chinese Holstein dairy cattle)为对象,以α1 抗胰蛋白酶基因(α1-AT)为候选基因,扩增5′侧翼区668 bp和999 bp的片段并进行测序.首次发现,在+3 142 bp处P1和+4 408 bp处P2分别发生C-T、T-C突变.随后采用PCR-RFLP方法对随机采自6个牛场,共计294头牛进行了检测,遗传变异和产奶性状分析结果显示：2个位点的等位基因在群体中都有分布,且处于中度多态.P1位点A和B等位基因的频率分别为50.34%和49.66%; AA、AB和BB基因型频率分别为23.81%、53.06%和23.13%;P2位点E和F等位基因的频率分别为30.61%和69.39%, EE、EF和FF基因型频率分别为11.90%、37.41%和50.68%. χ2适合性检验表明,该群体在P1位点的突变达到Hardy-Weinberg平衡状态（P>0.05）,在P2位点未达到平衡.基因与产奶性状关联分析表明,AB基因型个体产奶量与脂蛋比显著高于AA基因型个体(P＜0.05);FF基因型个体乳蛋白率显著高于EF基因型个体(P＜0.05);9种单倍型组合与乳脂率、乳蛋白率、体细胞数、产奶量及脂蛋比均存在不同程度相关性.     

DGAT1基因K232A突变位点在3个中国荷斯坦母牛群体中的基因型频率分布及其与产奶量的相关性

二脂酰甘油酰基转移酶1(acylCoA:diacylglycerol acyltransferase,DGAT1)基因是影响奶牛产奶性状的主效基因之一,其第八外显子上的第232位的赖氨酸转化为丙氨酸(K232A)的错义突变是影响产奶量、乳脂和乳蛋白含量的因果突变.本研究利用GenBank中已公布的牛DGAT1基因DNA序列,于K232A位点两端设计引物,采用PCR-RFLP方法鉴定来自新疆和江西的3个中国荷斯坦母牛群体共454个个体DGAT1基因K232A突变位点的基因型,使用SAS9.0软件分析供试群体基因型分布及其与产奶量的相关性.研究结果表明:K等位基因为441 bp的PCR扩增片段,A等位基因为完全切开的202bp和239bp两片段.新疆1、新疆2和南昌金牛3个荷斯坦母牛群体在该位点上K等位基因的频率分别为51.9%、42.4%和27.2%;A等位基因的频率分别为48.1%、57.6%和72.8%.DGAT1基因K232A突变位点与三个母牛群体日平均产奶量的相关性分析发现在3个群体中KK型个体产奶量均低于AA型个体,但不同基因型个体间产奶量差异在统计学上没有显著差异.本研究为进一步探讨DGAT1基因在中国奶牛群体中的遗传效应及分子标记辅助选择培育良种奶牛提供参考.     

三河牛β-乳球蛋白基因型及其启动子序列特点

[目的]分析三河牛β-乳球蛋白(β-Lg)的基因型,并探索其启动子序列与乳中含量的关系。[方法]采用聚丙烯酰胺凝胶电泳(PAGE)检测乳中β-Lg遗传变异体及其相对表达量,并通过PCR扩增,比对不同遗传变异体启动子的序列差异。[结果]三河牛(n=62)乳清中β-Lg有AA、AB和BB共3种基因型,频率依次为0.290、0.403和0.307,A和B两种等位基因频率接近;对37个纯合型β-Lg启动子的部分序列进行PCR扩增(636 bp)和测序,并与普通牛β-Lg基因序列(GenBank登录号：U31361.1)比对,共检测到6个突变位点,其中-430、-362、-216和-204位点基本上是等位基因特异的,且有3个突变点在3种转录因子结合基序中;建立了三河牛乳中β-Lg含量的高效液相色谱测定方法,发现β-Lg含量在AA型中极显著高于AB型(P<0.01),但AA、AB型与BB型之间均无显著差异。[结论]三河牛β-Lg A和B两种等位基因频率接近,其启动子-430、-362、-216和-204位点具有等位基因特异性,并可能影响等位基因表达。     

奶牛β-Lg基因第1外显子PCR-SSCP多态性与泌乳性能的相关性

采用PCR-SSCP技术并结合测序对233头奶牛β乳球蛋白(β-Lg)基因5’端部分序列和外显子1全部序列进行了多态性研究,分析了该基因与奶牛泌乳性状的相关性。结果表明:β-Lg基因5’端和外显子1共存在2个等位基因3种基因型,BB型为优势基因型,B为优势等位基因。该群体在这一位点上偏离Hardy-Weinberg平衡状态,多态信息含量(PIC)为0.3548。测序结果显示,与普通牛该基因序列(X14710)相比,B等位基因在2073 bp、2202 bp和2206 bp处发生了G→C、C→T和A→G的碱基突变,其中2202 bp处的C→T突变导致第11位氨基酸由苏氨酸变为异亮氨酸,而A等位基因在3个位点上与X14710相同。最小二乘法分析表明,BB型305 d乳蛋白量显著高于AA型和AB型(P<0.05);AB型305 d乳脂量显著高于AA型(P<0.05),BB型与AB型之间差异不显著(P>0.05);等位基因B为高乳蛋白量和乳脂量的优势基因,可作为奶牛选育的分子遗传标记。     

Haplotype analysis of TLR4 gene and its effects on milk somatic cell score in Chinese commercial cattle

Bovine mastitis is a very complex and common disease of dairy cattle and a major source of economic losses to the dairy industry worldwide. In this study, the bovine TLR4 was taken as a candidate gene for mastitis resistance. This study aimed to analyze the associations of single nucleotide polymorphisms (SNP) or haplotype and somatic cell score (SCS) in 404 Chinese commercial dairy cattle including Chinese Holstein, Sanhe cattle and Chinese Simmental breeds. The polymerase chain reaction and sequencing methods were used for detecting genotype and allele frequency distribution of the two SNPs (rs8193062, rs8193064), statistical results showed that T allele at rs8193062 and C allele at rs8193064 were the predominate alleles. Moreover, six SNPs, including two SNPs (rs8193062, rs8193064) and four SNPs (rs8193060, rs8193069, rs29017188, rs8193046) which were chosen according the polymorphism level for the same cattle populations in previous studies, were used for haplotype analysis, the results revealed that twenty-one haplotypes were found in the mentioned animals, of which, Hap1 (30.5 %) and Hap2 (30.4 %) were the most common haplotypes. Hap2, Hap4 and Hap12 might negatively effect on milk SCS, whereas Hap13 might positively effect on milk SCS. The results in this study might assist in marker assisted selection and provided some reference to be implemented in breeding programs to improve the mastitis resistance of dairy cattle.     

Toll-Like Receptor 2 Gene Polymorphism and its Relationship with SCS in Dairy Cattle

Toll-like receptor 2 (TLR2) plays an important role in the innate immune response to a variety of pathogens. In this study, bovine TLR2 gene was taken as a candidate gene for mastitis resistance. Through PCR-SSCP analysis and sequencing, three missense mutations at T385 G, G398A, and G1884A were detected in the coding region that encoded extracellular domain. Altogether 240 dairy cattle of three breeds (Holstein, Simmental, and Sanhe cattle) were genotyped and allele frequencies were determined. The effects of TLR2 polymorphisms on somatic cell score (SCS) were analyzed and significant association was found between T385 G and SCS. The mean of genotype GG was significantly lower than those of genotype TT and TG. No significant associations were found with SCS for G398A and G1884A. Information provided in this research will be useful in further studies to determine the role of TLR2 gene in the mastitis resistance.     

A coding SNP of <Emphasis Type="Italic">LHX4</Emphasis> gene is associated with body weight and body length in bovine

Heterozygous mutations in LHX4 are associated with combined pituitary hormone deficiency. In this study, the polymorphism of LHX4-HaeIII locus was revealed in 822 individuals from four Chinese cattle breeds. The PCR–RFLP analysis showed that there were three genotypes: GG, GA, AA. The frequencies of genotype GG ranged from 0.6620 to 0.9789 in analyzed populations. The genotypic frequencies of LHX4 locus in the four populations all agreed with Hardy–Weinberg equilibrium (P > 0.05). Distributions of genotypic frequencies of different breeds (QC, NY, JX, CH) at this locus were found to be significantly different based on a χ ² test (P < 0.001). The genetic diversity analysis revealed the JX cattle possessed intermediate genetic diversity, and the other three Chinese cattle breeds belonged to poor genetic diversity. Correlation analysis with growth traits in the NY breed indicated that: the animals with genotype GA had greater body weight than those with genotype GG (P < 0.05); the animals with GA genotype owned significantly longer body length than the ones with GG genotype (P < 0.05) at 18 and 24 months.     

Single nucleotide polymorphism of CACNA2D1 gene and its association with milk somatic cell score in cattle

The objective of the present study was to identify polymorphisms of the CACNA2D1 gene, and to analyze associations between these polymorphisms and mastitis in several cattle breeds. Through PCR-RFLP methods and DNA sequencing, an allelic variant corresponding to the A→G mutations and Aspartic (Asp) to Glycine (Gly) amino acid replacement at positions 526745 in the exon 25 of bovine CACNA2D1 gene could be detected. Two alleles, A and G, and three genotypes, AA, AG and GG were defined. Genetic character in the studied populations indicated that the A526745G loci of CACNA2D1 gene was moderate polymorphism and fitted with Hardy-Weinberg equilibrium (P > 0.05). The effects of CACNA2D1 polymorphisms on somatic cell score (SCS) were analyzed and significant association was found between A526745G and SCS. The mean of genotype GG was significantly lower than those of genotype AG and AA (P = 0.0469). Information provided in this research could be useful in further studies to determine the role of CACNA2D1 gene in the mastitis resistance.