哈萨克羊DRB1基因外显子3多态性及生物信息学分析     

王元元  严国  罗成  齐江姣  周光普  谭君  高剑峰 《中国畜牧兽医》2018,(3)

试验旨在研究白细胞表面抗原DRB1基因外显子3多态性与哈萨克羊布鲁氏菌病易感性的相关性。运用混合DNA池结合PCR产物直接测序方法,对哈萨克羊DRB1基因外显子3进行多态性分析,经卡方检验分析每个SNP位点的等位基因频率、基因型频率及其多态性与布鲁氏菌病易感性的相关性,利用生物信息学分析软件对PCR扩增所获序列进行RNA二级结构及蛋白质的二级结构和抗原表位分析。结果表明,在282bp的外显子3序列中共检测到7个SNPs,分别为:T10C、C119T(Trp→Arg)、G215C(Gln→Glu)、A238G、T245G(Ser→Ala)、G256A、C259T,这些位点在病例组和对照组之间的等位基因频率及各基因型间不存在显著性差异(P0.05);进一步分析发现,各突变位点均引起RNA二级结构和最小自由能的改变,各错义突变位点均未引起蛋白质二级结构和抗原表位的改变。由此得出,DRB1基因外显子3的7个SNPs位点(T10C、C119T、G215C、A238G、T245G、G256A和C259T)与哈萨克羊布鲁氏菌病易感性无相关性。  相似文献   

哈萨克羊DRB1基因外显子3多态性及生物信息学分析     

王元元  严国  罗成  齐江姣  周光普  谭君  高剑峰 《中国畜牧兽医》2018,45(3):721-729

试验旨在研究白细胞表面抗原DRB1基因外显子3多态性与哈萨克羊布鲁氏菌病易感性的相关性。运用混合DNA池结合PCR产物直接测序方法,对哈萨克羊DRB1基因外显子3进行多态性分析,经卡方检验分析每个SNP位点的等位基因频率、基因型频率及其多态性与布鲁氏菌病易感性的相关性,利用生物信息学分析软件对PCR扩增所获序列进行RNA二级结构及蛋白质的二级结构和抗原表位分析。结果表明,在282 bp的外显子3序列中共检测到7个SNPs,分别为：T10C、C119T（Trp→Arg）、G215C（Gln→Glu）、A238G、T245G（Ser→Ala）、G256A、C259T,这些位点在病例组和对照组之间的等位基因频率及各基因型间不存在显著性差异（P > 0.05）;进一步分析发现,各突变位点均引起RNA二级结构和最小自由能的改变,各错义突变位点均未引起蛋白质二级结构和抗原表位的改变。由此得出,DRB1基因外显子3的7个SNPs位点（T10C、C119T、G215C、A238G、T245G、G256A和C259T）与哈萨克羊布鲁氏菌病易感性无相关性。  相似文献   

中国美利奴羊OLA-DQB1基因exon2遗传多态性与布鲁氏菌病易感性的关联分析     

王文文  许万云  胡梦薇  李建华  刘朋涛  高剑峰 《中国畜牧兽医》2015,42(6):1495-1503

本试验采用PCR-SSCP方法对148只布鲁氏菌阴性和60只布鲁氏菌阳性中国美利奴羊白细胞表面抗原DQB1(OLA-DQB1)基因exon 2单核苷酸多态性(SNPs)进行了检测,之后挑选不同等位基因进行PCR产物测序,旨在确定该基因的多态性位点,并对每个SNP位点的等位基因频率、基因型频率进行统计分析,从而分析其多态性与布鲁氏菌病易感性的相关性.测序结果表明,在270 bp的序列内共检测到43个SNPs,其中G196A位点的等位基因频率在病例组和对照组中的分布存在极显著差异(P< 0.01),其基因型频率存在显著差异(P< 0.05);C211T位点的等位基因频率在病例组和对照组中存在显著差异(P< 0.05).由此表明,OLA-DQB1基因exon 2多态性与中国美利奴羊布鲁氏菌病易感性呈显著相关.  相似文献   

哈萨克羊iNOS基因多态性与布鲁氏菌病的相关性分析     

张凡  徐杰  李刚  周永顺  何营  韩凯  陈福龙  高剑峰 《中国畜牧兽医》2021,48(3):1102-1111

试验旨在探讨哈萨克羊诱导型一氧化氮合酶（iNOS）基因多态性与布鲁氏菌病的相关性。使用虎红平板凝集试验（RBPT）方法对231只哈萨克羊血清进行布鲁氏菌病血清学检测,参考GenBank中绵羊iNOS基因序列,针对其第6、7、8外显子及其邻近内含子片段设计引物,利用PCR-SSCP技术和DNA测序技术对231只哈萨克羊的iNOS基因进行多态性检测,分析其SNPs与哈萨克羊布鲁氏菌病易感性的相关性。结果表明,67只哈萨克羊为布鲁氏菌感染阳性,阳性检出率为29.00%。在哈萨克羊iNOS基因的外显子6和8片段上未检测到多态位点,在外显子7片段上检测出F7-T18054C和F7-C18084T 2个多态位点,在F7-T18054C多态位点上检测到3种基因型（TC、TT、CC）,优势等位基因和基因型分别是C型和CT型,其等位基因频率和基因型频率分别是0.660和0.446。在F7-C18084T多态位点上检测到2种基因型（CT、CC）,优势等位基因频率和基因型分别是C和CC型,其等位基因和基因型频率分别是0.946和0.892。F7-C18084T属于低度多态（PIC<0.25）,F7-T18054C属于中度多态（0.25 < PIC < 0.5）。相关性分析表明,F7-T18054C和F7-C18084T多态位点与布鲁氏菌病易感性无显著相关性（P>0.05）。试验结果表明,哈萨克羊iNOS基因F7-T18054C和F7-C18084T多态位点与布鲁氏菌病易感性不存在相关性。  相似文献   

中国美利奴羊TLR2基因多态性及其与布鲁氏菌病的相关性分析     

罗成  王元元  王会敏  谭君  周光普  高剑峰 《中国畜牧兽医》2018,45(5):1145-1152

试验旨在研究Toll样受体2（Toll-like receptor,TLR2）基因的多态性及其与中国美利奴羊布鲁氏菌病易感性的相关性。利用生物信息学方法对NCBI上公布的绵羊TLR2基因序列进行比对,选出多态位点丰富的片段进行扩增,运用PCR-SSCP的方法对206个中国美利奴布鲁氏菌病阴性样本和80个中国美利奴羊布鲁氏菌病阳性样本进行TLR2基因的多态性检测,然后对不同等位基因的PCR产物进行测序,确定该基因的多态性位点,经卡方检验分析每个SNP位点的等位基因频率、基因型频率及其多态性与布鲁氏菌病易感性的相关性,利用生物信息学软件分析RNA二级结构及蛋白质的二级结构。结果表明,在279 bp的序列中共检测到3个SNPs,分别为：C1731T、G1737C和G1749T,均未引起对应氨基酸的改变,属于无义突变。这些位点在病例组和对照组之间的等位基因频率及基因型频率均不存在显著差异（P>0.05）。各突变位点均能引起RNA二级结构和最小自由能的改变,而蛋白质的二级结构均未改变。由此得出,中国美利奴羊TLR2基因的3个SNPs位点（C1731T、G1737C和G1749T）与中国美利奴羊布鲁氏菌病易感性无相关性。  相似文献   

中国美利奴羊TLR2基因多态性及其与布鲁氏菌病的相关性分析     

罗成  王元元  王会敏  谭君  周光普  高剑峰 《中国畜牧兽医》2018,(5)

试验旨在研究Toll样受体2(Toll-like receptor,TLR2)基因的多态性及其与中国美利奴羊布鲁氏菌病易感性的相关性。利用生物信息学方法对NCBI上公布的绵羊TLR2基因序列进行比对,选出多态位点丰富的片段进行扩增,运用PCR-SSCP的方法对206个中国美利奴布鲁氏菌病阴性样本和80个中国美利奴羊布鲁氏菌病阳性样本进行TLR2基因的多态性检测,然后对不同等位基因的PCR产物进行测序,确定该基因的多态性位点,经卡方检验分析每个SNP位点的等位基因频率、基因型频率及其多态性与布鲁氏菌病易感性的相关性,利用生物信息学软件分析RNA二级结构及蛋白质的二级结构。结果表明,在279bp的序列中共检测到3个SNPs,分别为:C1731T、G1737C和G1749T,均未引起对应氨基酸的改变,属于无义突变。这些位点在病例组和对照组之间的等位基因频率及基因型频率均不存在显著差异(P0.05)。各突变位点均能引起RNA二级结构和最小自由能的改变,而蛋白质的二级结构均未改变。由此得出,中国美利奴羊TLR2基因的3个SNPs位点(C1731T、G1737C和G1749T)与中国美利奴羊布鲁氏菌病易感性无相关性。  相似文献   

哈萨克绵羊DRB1基因外显子1和4多态性与布鲁氏菌病的相关性研究     

马雪珍  徐杰  高剑峰  李刚 《中国畜牧兽医》2020,47(12):3844-3851

试验旨在对哈萨克绵羊DRB1基因外显子1和4多态性与布鲁氏菌病的相关性进行研究。使用虎红平板凝集试验（RBPT）对试羊的血清进行血清学检测，参考GenBank中绵羊MHC ClassⅡ区DRB1基因序列（登录号：NC_040271.1），对其外显子1和4片段设计引物，采用PCR-SSCP和DNA测序技术对230只哈萨克绵羊的DRB1基因进行多态性检测，分析其多态位点与哈萨克绵羊布鲁氏菌易感性之间的关系。RBPT检测发现66只哈萨克绵羊为布鲁氏菌感染阳性，阳性检出率为28.7%。外显子1片段存在一个SNP位点（F1-G22A），测序确定两种基因型（GG、GA），优势等位基因和基因型分别为G、GG，F1-G22A多态位点的易感基因型为GA。卡方检验表明，哈萨克绵羊DRB1基因F1-G22A多态位点与布鲁氏菌易感性的相关性不显著（P>0.05）。通过生物信息学在线软件分析得出，F1-G22A多态位点导致了RNA二级结构的改变和最小自由能的降低，引起了蛋白质二级结构的改变。DRB1基因外显子4片段未发现SNPs。由此得出，哈萨克绵羊DRB1基因F1-G22A多态位点与布鲁氏菌易感性可能存在一定的相关性。  相似文献   

中国美利奴羊eNOS基因exon8多态性及其与布鲁氏菌病易感性相关性分析     

许万云  王会敏  李建华  汪文伦  胡梦薇  高剑峰 《中国畜牧兽医》2015,42(12):3294-3299

本试验旨在研究内皮型一氧化氮合酶(eNOS)基因exon8多态性与中国美利奴羊布鲁氏菌病易感性的相关性。利用生物信息学方法对人和中国美利奴羊eNOS基因exon8序列进行比对,并对NCBI SNP数据库上人eNOS基因exon8多态性进行了统计分析。通过PCR-SSCP对101只中国美利奴羊阴性样本和61只中国美利奴羊阳性样本eNOS基因exon8的多态性进行检测,然后对不同等位基因进行PCR产物测序,旨在确定该基因exon8多态性位点,并对SNP位点的等位基因频率、基因型频率进行统计分析。在eNOS基因exon8序列142 bp处检测到一个新的SNP位点(ss974768653:A142G),该位点在病例组和对照组之间的等位基因频率及各基因型间不存在显著差异性(P >0.05)。eNOS基因exon8 A142G多态性位点与中国美利奴羊布鲁氏菌病易感性可能无相关性。  相似文献   

贵州黑山羊DQB2基因Exon1遗传变异分析     

《中国畜牧杂志》2016,(9)

研究了贵州黑山羊MHC-DQB2基因的多态性,以便发挥MHC-DQB2基因在山羊抗病育种中的作用。采用构建DNA池并通过PCR直接测序的方法对164只贵州黑山羊的DQB2基因Exon1进行遗传变异分析;应用生物信息学软件分析基因频率、RNA二级结构、蛋白质二级结构和抗原表位。在其第1外显子中筛选得到4个SNPs,分别为G23A(Arg→Gln)、G45A(同义突变)、T90C(同义突变)、C109A(Gln→Lys),其中,T90C突变位点的最小自由能最低,其RNA二级结构最稳定。G23A和C109A 2个突变位点均引起RNA二级结构、蛋白质二级结构和抗原表位的改变。结果表明:贵州黑山羊MHC-DQB2基因的第1外显子具有较丰富的遗传多样性。  相似文献   

贵州地方山羊THRSP外显子1多态性分析     

《黑龙江畜牧兽医》2016,(19)

为了分析贵州山羊甲状腺激素应答蛋白(THRSP)基因的多态性,试验采用PCR产物直接测序法筛选出贵州地方山羊THRSP基因外显子1中对山羊肉质性状有显著影响的单核苷酸多态性(SNPs)位点。结果表明:在2个山羊品种中均检测到THRSP基因的2个SNPs位点分别为A341G、G365A,均为同义突变;位点G365A的A和G等位基因频率在2个品种间的差异较大。利用在线软件预测突变前后的mRNA二级结构及理化特性。说明THRSP基因外显子1的A341G和G365A位点的突变均能引起mRNA结构发生显著改变。  相似文献   

Polymorphisms and Its Genetic Variation Analysis of DQB2 Gene Exon 2 in Kazakh Sheep     

WANG Yuan-yuan  YAN Guo  LUO Cheng  QI Jiang-jiao  ZHOU Guang-pu  TAN Jun  GAO Jian-feng 《中国畜牧兽医》2017,44(12):3543-3553

This study was aimed to investigate the association between the polymorphism of DQB2 gene exon 2 and the susceptibility to Kazakh sheep brucellosis. The DQB2 gene exon 2 of Kazakh sheep lymphocyte antigen was amplified by PCR-SSCP method from 146 healthy and 28 infected with Brucella Kazakh sheep, and the single nucleotide polymorphisms (SNP) was analyzed, then the different alleles were selected for cloning and sequencing. In order to analyze its correlation with brucellosis susceptibility, the differences in gene frequency and genotype frequency of each SNP locus were analyzed by Chi-square test. Bioinformatics softwares were used to analyze the secondary structure of mRNA, the secondary structure, tertiary structure and epitope of protein. The sequencing result showed that 33 SNPs were detected in 270 bp DNA sequence, the gene frequencies of C9G and A180G were extremely significantly different in case group and control group (P<0.01), and its genotype frequencies presented significantly difference (P<0.05). Similarly, A13T and C133G loci were significant difference in case group and control group (P<0.05). Further analysis result showed that the minimum free energy of the A180G mutation site was the lowest and its mRNA secondary structure was the most stable; Both A13T and C133G mutation sites caused the changes of mRNA secondary structure, protein secondary, tertiary structure and antigenic epitope of protein, respectively. The results showed that the polymorphism of DQB2 gene exon 2 might be significantly correlated with brucellosis susceptibility in Kazakh sheep.  相似文献   

The Correlation Between Polymorphisms of Exon1 and Exon4 of DRB1 Gene and Brucellosis in Kazakh Sheep     

MA Xuezhen  XU Jie  GAO Jianfeng  LI Gang 《中国畜牧兽医》2007,47(12):3844-3851

The purpose of this experiment was to study the correlation between exon 1 and 4 polymorphisms of DRB1 gene and brucellosis in Kazakh sheep.Using RBPT serological tests to try sheep serum,reference in GenBank sheep MHC Class Ⅱ area DRB1 gene sequences (Accession No.:NC_040271.1),the exon 1 and 4 pieces designed primers,using PCR-SSCP and DNA sequencing technology to 230 Kazak sheep DRB1 gene polymorphism detection,analyze its polymorphism loci and the relationship between the Kazak sheep Brucella susceptibility.The results showed that 66 Kazakh sheep were positive for Brucella in RBPT test,and the positive detection rate was 28.7%.There was one SNP locus (F1-G22A) in exon 1 fragment,and sequencing determined two genotypes (GG and GA),the dominant allele and genotype were G and GG respectively,and the susceptibility genotype of the polymorphisms of F1-G22A was GA.Chi-square test showed that there was no significant correlation between the polymorphisms of DRB1 gene F1-G22A and Brucella susceptibility in Kazakh sheep (P>0.05).According to the analysis of bioinformatics online software,the F1-G22A polymorphic sites lead to the change of RNA secondary structure and the decrease of minimum free energy,and lead to the change of protein secondary structure.No SNPs were found in DRB1 exon 4 fragment.Therefore,there might be a certain correlation between the polymorphisms of DRB1 gene F1-G22A and Brucella susceptibility in Kazakh sheep.  相似文献   

The Correlation Analysis between Chinese Merino Sheep OLA-DQB1 Gene Exon 2 Genetic Polymorphism and Brucellosis Susceptibility     

WANG Wen-wen  XU Wan-yun  HU Meng-wei  LI Jian-hua  LIU Peng-tao  GAO Jian-feng 《中国畜牧兽医》2015,42(6):1495-1503

The single nucleotide polymorphisms (SNPs) of ovine lymphocyte antigen DQB1 (OLA-DQB1) gene exon 2 was amplified by PCR-SSCP method from 148 healthy and 60 infected with Brucella Chinese Merino sheep and then PCR products of different alleles were sequenced to determine the polymorphism loci of the gene.The differences in gene frequency and genotype frequency of each SNP loci were analyzed statistically to analyze its correlation with brucellosis susceptibility.The sequencing result showed that 43 SNPs were detected in 270 bp DNA sequence,the gene frequencies of G196A allele had extremely significant difference in case and control samples (P< 0.01),and its genotype frequencies presented significant difference (P< 0.05).Similarly,C211T allele was significantly different in case and control samples (P< 0.05).The results showed that the polymorphism of OLA-DQB1 gene exon 2 might be a significant association gene with brucellosis susceptibility.  相似文献   

The Polymorphisms of Chinese Merino Sheep eNOS Gene exon8 and its Association with Brucellosis Susceptibility     

XU Wan-yun  WANG Hui-min  LI Jian-hua  WANG Wen-lun  HU Meng-wei  GAO Jian-feng 《中国畜牧兽医》2015,42(12):3294-3299

The association of Chinese Merino sheep eNOS gene exon8 polymorphisms with brucellosis susceptibility was studied in this research.The sequences of human and Chinese Merino sheep eNOS gene exon8 were aligned by the bioinformatics methods,and the polymorphisms of human eNOS gene in the NCBI SNP database were statistically analyzed.The polymorphisms of 101 Chinese Merino sheep negative samples and 61 Chinese Merino sheep positive samples were detected by PCR-SSCP method,and then the PCR products of different alleles were sequenced,aiming to determine exon8's polymorphism loci,and the allele frequency and genotype frequency of SNP loci were statistically analyzed.A novel SNP locus (ss974768653:A142G) was detected at the 142 bp of eNOS gene exon8,and the locus had no difference in allele frequency and each genotype between negative and positive groups (P >0.05).There might be no correlation between the A142G polymorphism locus of Chinese Merino sheep eNOS gene exon8 and brucellosis susceptibility.  相似文献