用4个微卫星标记分析7个绵羊群体之间的遗传关系

分析了4个微卫星基因座BM143、OarHH35、OarAE101、BMS2508在7个绵羊群体（小尾寒羊、湖羊、乌珠穆沁羊、萨福克羊、多赛特羊、夏洛来羊、多赛特公羊×小尾寒羊母羊F1代杂种羊）286只绵羊中的遗传多态性。结果表明,这4个微卫星标记在7个绵羊群体中的等位基因数分别为9、11、14和9,其多态信息含量/有效等位基因数/杂合度分别为0.7073/3.7231/0.7314、0.8267/6.4399/0.8447、0.5743/2.5178/0.6028、0.6172/3.0712/0.6744,其中OarHH35的遗传变异最大,OarAE101最小。7个绵羊群体中小尾寒羊的遗传变异最大,湖羊的最小。基于Nei氏DA距离和DS标准遗传距离,采用UPGMA方法构建了系统发生树。该发生树将中国地方品种（小尾寒羊、乌珠穆沁羊、湖羊）和法国的夏洛来羊归为一类,将F1杂种羊、英国品种（萨福克羊和多赛特羊）归为另一类。绵羊微卫星基因分型技术为检查品种（群体）之间的遗传关系提供了一个有用的工具。 Abstract：The genetic polymorphisms of four microsatellite loci BM143,OarHH35,OarAE101,and BMS2508 were analyzed in 286 sheep of seven sheep populations (Small Tail Han sheep, Hu sheep, Ujumqin sheep, Suffolk sheep, Dorset sheep, Charolais sheep, F1 of Dorset♂ × Small Tail Han sheep♀). The numbers of alleles for BM143,OarHH35,OarAE101,and BMS2508 are 9, 11, 14 and 9 in seven sheep populations, respectively. The polymorphism information content/number of effective alleles/ heterozygosity of BM143,OarHH35,OarAE101 and BMS2508 were 0.7073/3.7231/0.7314, 0.8267/6.4399/0.8447,0.5743/2.5178/0.6028,0.6172/3.0712/0.6744 in 286 sheep, respectively. The results revealed the greatest genetic variation at OarHH35 locus and the lowest at OarAE101, the greatest genetic variation in Small Tail Han sheep and the lowest in Hu sheep among seven sheep populations. In the unweighted pair group method with arithmetic mean (UPGMA) dendrograms based on Nei's DA distance and Nei's DS standard genetic distance, the Chinese native breeds (Small Tail Han sheep, Ujumqin sheep, Hu sheep) were grouped together, then with Charolais sheep. The F1 crossbred sheep, and the two British native sheep (Suffolk sheep, Dorset sheep) also clustered together. Microsatellite genotyping in sheep provided a useful tool for examining the genetic relationships among breeds(populations).     

近交系小鼠微卫星DNA多态性的研究

随机选择位于小鼠不同染色体上的微卫星引物42对,用PCR技术对C3H、C57、BALB/c、DBA、TA2、T739、B615、BACB/c－nu－nu和SCID等9种实验室常用近交系小鼠微卫星DNA多态性进行了研究。结果显示有信息的40对引物中,9种近交系小鼠在各基因座上均出现一条清晰条带,28个基因座表现为多态性。其中D3Mit22、D7Nds1、D11Mit12、D12Nds2、D15Mit17、D16Mit3、D16Mit4基因座表现为显著多态性。T739、B615和TA2的遗传背景相近,其相似系数分别为90％和85％;其次为TA2、SCID和B615,其相似系数分别为80％和82.5％。结果表明所检测的小鼠符合近交要求,筛选出的引物能典型地反映9个近交系小鼠的品系特异性和遗传背景,可用于常规检测小鼠品系来源和遗传背景等。 Abstract：Forty-two microsatellites DNA loci on different chromosomes in nine kinds of inbred strain mice including C3H,C57,BALB/c,DBA,TA2,T739,B615,BALB/c-nu-nu and SCID were investigated by PCR analysis.It showed that all these mice tested display single allelic gene band with forty pairs of informative primers.Twenty-eight loci are polymorphisms,among which the polymorphisms of D3Mit22,D7Nds1,D11Mit12,D12Nds2,D15Mit17,D16Mit3,and D16Mit4 loci are significant.The genetic background of T739 was similarity with that of B615 and TA2 ,the similarity indices were 90％ and 85％ respectively;and that of TA2 was similarity with SCID and B615,the similarity indices were 80％ and 82.5％.These results suggest that these mice tested meet the request of inbred strain.Screened primers showing marked polymorphisms topically reflect the speciality of strains and genetic backgrounds,which could be used in determining the strains origin and genetic background of mice.     

近交系小鼠微卫星DNA多态性的研究

随机选择位于小鼠不同染色体上的微卫星引物42对,用PCR技术对C3H、C57、BALB/c、DBA、TA2、T739、B615、BACB/c－nu－nu和SCID等9种实验室常用近交系小鼠微卫星DNA多态性进行了研究。结果显示有信息的40对引物中,9种近交系小鼠在各基因座上均出现一条清晰条带,28个基因座表现为多态性。其中D3Mit22、D7Nds1、D11Mit12、D12Nds2、D15Mit17、D16Mit3、D16Mit4基因座表现为显著多态性。T739、B615和TA2的遗传背景相近,其相似系数分别为90％和85％;其次为TA2、SCID和B615,其相似系数分别为80％和82.5％。结果表明所检测的小鼠符合近交要求,筛选出的引物能典型地反映9个近交系小鼠的品系特异性和遗传背景,可用于常规检测小鼠品系来源和遗传背景等。 Abstract：Forty-two microsatellites DNA loci on different chromosomes in nine kinds of inbred strain mice including C3H,C57,BALB/c,DBA,TA2,T739,B615,BALB/c-nu-nu and SCID were investigated by PCR analysis.It showed that all these mice tested display single allelic gene band with forty pairs of informative primers.Twenty-eight loci are polymorphisms,among which the polymorphisms of D3Mit22,D7Nds1,D11Mit12,D12Nds2,D15Mit17,D16Mit3,and D16Mit4 loci are significant.The genetic background of T739 was similarity with that of B615 and TA2 ,the similarity indices were 90％ and 85％ respectively;and that of TA2 was similarity with SCID and B615,the similarity indices were 80％ and 82.5％.These results suggest that these mice tested meet the request of inbred strain.Screened primers showing marked polymorphisms topically reflect the speciality of strains and genetic backgrounds,which could be used in determining the strains origin and genetic background of mice.     

PCR扩增近交系大鼠微卫星位点DNA多态性的研究

本实验选取大鼠7条染色体上的微卫星位点合成了10对引物,利用聚合酶链反应(PCR)扩增技术对国内北京和哈尔滨等4家单位提供的6个品系(SHR、SHRSP、LEW、RCS、WKY和F344)的8个近交系大鼠群体进行了DNA多态性分析的研究.结果表明:9个微卫星位点具有显著多态性;不同品系个体之间具有多态性;同一群体不同个体之间除SHR(哈)的SMST位点和WKY(哈)的AGT位点出现一定的差异外,其他均没有差异;不同地区同一品系的不同个体之间也存在一定的差异.该方法能有效地对近交系与杂交系、品系与品系、品系与亚系加以区分.因此,本实验为开展近交系大鼠遗传作图、基因定位和为实验动物的遗传背景监测提供可靠的信息,为大鼠遗传基因的研究提供了一个快捷简便、特异准确的方法。 Abstract:In the experiment,It were selected that 20 primers were assigned on 7 chromosomes of inbred rat.DNA polymorphism of 8 colonies from 6 inbred rat strains(SHR、SHRSP、WKY、LEW、RCS、F344)were studied in national Beijing and Harbin using PCR-analyzed microsatellites.The results indicated that there were remarkable polymorphism in 9 microsatellite loci;There is a polymorphism among the various rat strains;and no polymorphism in the same rat strains except SMST locus of SHR(Harbin)and AGT locus of WKY(Harbin)and there is a little difference among the same inbred rat strains in different areas.The method of PCR-analyzed microsatellites can be used for distinguishing between inbred and outbred、different strains、strain and substrain.and it provides a lot of information for genetic mapping,gene location and heredity probe of the inbred rat strains,and a speedy、convenient method for genetic research of the inbred rat.     

我国6个地方绵羊品种微卫星DNA多态性研究

利用聚丙烯酰胺凝胶电泳技术研究了我国蒙古羊、乌珠穆沁羊、哈萨克羊、阿勒泰羊、滩羊和藏绵羊 6个地方绵羊品种 17个微卫星标记的多态性 ,以探讨其遗传多样性、起源分化及群体间的遗传亲缘关系。结果表明微卫星标记不同位点间遗传多样性差异极显著 (P <0 0 1) ,群体间多态信息含量 (PIC)、近交程度 (Fis)和观察杂合度 (Obs .Het)差异不显著 ,但基因多样性 (genediversity)和期望杂合度 (Exp .Het)差异显著 (P <0 0 5 )。所研究的我国 6个地方绵羊品种与欧洲品种具有相似的遗传多样性 ,但具有较高的近交系数。个体和群体的聚类分析结果提示我国地方绵羊品种可能起源于两类祖先。群体间的聚类分析结果还表明 ,蒙古羊与乌珠穆沁羊分化不明显且具有较近的遗传亲缘关系 ,蒙古羊与藏绵羊间分化明显且具有较远的遗传亲缘关系。滩羊、阿勒泰羊以及藏绵羊间也具有较近的遗传亲缘关系。所研究的我国 6个地方绵羊品种的遗传分化 (Fst)与西班牙绵羊品种接近 ,但明显小于欧洲其他绵羊品种     

微卫星DNA的多态性及其应用

微卫星DNA是广泛存在于各种真核生物基因组中的短串联重复序列,具有突变速率快、多态性高等特点,本分析了微卫星的多态性及其形成机制,并简要介绍其在亲缘关系鉴定、种群遗传结构分析、基因图谱以及基因诊断等方面的应用。     

山羊群体遗传多样性的微卫星分析

为了保护和合理利用我国地方山羊品种遗传资源提供理论基础,本研究利用国际农粮组织和国际家畜研究所推荐的10对微卫星引物,结合荧光标记PCR,检测了中国9个地方山羊品种和1个引进山羊品种的遗传多样性。所研究的10个品种中7个呈现出高度多态,3个呈现出中度多态。并共检测到119个等位基因,有效等位基因数在1.4641~9.2911之间,座位平均杂合度在0.2618~0.7672之间,品种平均杂合度在0.5196~0.7024之间,其中SRCRSP23位点和河西绒山羊(HXR)平均杂合度最高。聚类关系(NJ和UPGMA)和主成分分析结果与其起源、育成历史及地理分布基本一致。     

蒙古山羊和哈萨克山羊GOLA-DRB3基因的HaeⅢ酶切多态性分析

采用限制性内切核酸酶HaeⅢ对蒙古山羊和哈萨克山羊GOLA-DRB3基因外显子2的285bp扩增产物进行了PCR-RFLP多态性分析,共检测到17种基因型,由A、B、C、D、E、F和H等7个复等位基因控制;通过酶切图谱分析发现蒙古山羊和哈萨克山羊的GOLA-DRB3基因外显子2的154、168和220位碱基表现出多态性。并对基因型频率和等位基因频率进行了统计分析,结果表明,GOLA-DRB3基因的部分基因型频率和等位基因频率在两个群体之间差异显著（P＜0.10或P＜0.05）或极显著（P＜0.01）; χ2适合性检验结果表明,蒙古山羊和哈萨克山羊的GOLA-DRB3基因外显子2的HaeⅢ酶切位点均未达到Hardy-Weinberg平衡状态（P＜0.01）。 Abstract:The exon2 of GOLA-DRB3 gene was amplified and a uniform fragment of 285bp was obtained in Mongolian Goat and Kazakh Goat.The 285bp PCR product was digested with restriction endomuclease HaeⅢ and genetic polymorphism was investigated by PCR-RFLP.Seventeen kinds of genotypes were found in two populations,which were controlled by seven alleles.There are significant differences in some genotypic frequencies and gene frequencies between the two populations（P＜0.10,P＜0.05,P＜0.01）;The results of χ2 test showed that genotypes of GOLA-DRB3 gene in two populations did not fit with Hardy-Weinberg equilibrium（P＜0.01）.     

微卫星多态性检测技术及其在保护遗传学中的应用

微卫星是一种新型的分子遗传标记,具有只需极少量样品即可进行PCR扩增等优点,使之极其适合于保护遗传化学研究。阐释了微卫星的结构、微卫星多态检测技术的原理,简要论述了微卫生多态检测技术的优点及其应用,并介绍了一种分离动物微卫星位点的富集方法。     

海参微卫星DNA的多态性

微卫星DNA(microsatellite DNA)广泛存在于真核生物的基因组中。由于其具有突变频率快、多态性丰富、呈共显性遗传、通用性等特点,已成为近年来被广泛应用的分子遗传标记。本研究对10个海参微卫星DNA进行了克隆与测序。结果表明:90%的微卫星DNA序列存在长度多态性,这为进一步研究海参的分子标记辅助育种奠定了基础。     

Genetic polymorphism of goat kappa-casein (CSN3) in different breeds and characterization at DNA level

Data on genetic differences at CSN3 in goat breeds including a DNA based typing method and the mutations responsible for variation on protein and DNA level are presented here. Isoelectric focusing (IEF) in ultrathin polyacrylamide gels with carrier ampholytes was used to demonstrate CSN3 polymorphism in milk samples of Italian (Orobica n=88; Ionica n=68) and German goat breeds (Bunte Deutsche Edelziege n=244; Weisse Deutsche Edelziege n=134; Toggenburger n=25; Thüringer Waldziege n=70). A further CSN3 band was found presenting a more cathodic migration than CSN A. After chymosin action, the genetic polymorphism was also observed in the para-kappa-casein fraction. The new allele CSN3(B) was spread mainly in Orobica (37%), Bunte Deutsche Edelziege (11%) and Ionica (10%). CSN3(B) occurred in low frequency (<3%) in Thüringer Waldziege and in Weisse Deutsche Edelziege, and could not be demonstrated in milk samples of Toggenburger. The populations were in Hardy-Weinberg equilibrium at CSN3. The codominant genetic control of CSN3(B) was confirmed by genetic studies. Discrimination of CSN3 alleles A and B was also obtained by DNA SSCP analysis. Sequencing of CSN3(B) revealed four transitions at position 247, 309, 471, and 591 compared with CSN3(A). From these transitions, the following amino acid substitutions are deduced: 44 Gln --> Arg, 65 Val --> Ile, 119 Val --> Ile, and 159 Ser --> Pro. Among the four mutations, only the 44 Gln --> Arg can be revealed by milk protein IEF analysis while at DNA level three further genetic variants should exist in addition to CSN3(A) and CSN3(B).     

Genetic diversity in Swiss goat breeds based on microsatellite analysis

Genetic diversity in eight Swiss goat breeds was estimated using PCR amplification of 20 bovine microsatellites on 20-40 unrelated animals per breed. In addition, the Creole breed from the Caribbean and samples of Ibex and Bezoar goat were included. A total of 352 animals were tested. The bovine microsatellites chosen amplified well in goat. The average heterozygosity within population was higher in domestic goat (0.51-0.58) than in Ibex (0.17) and Bezoar goat (0.19). Twenty-seven per cent of the genetic diversity in the total population could be attributed to differences between the populations. However, with the exclusion of Ibex from the total population, this proportion dropped to 17%. Principal component analysis showed that all Swiss goat breeds are closely related, whereas the Creole breed, Ibex and Bezoar goat are clearly distinct from all eight Swiss breeds.     

Genetic relationships among twelve Chinese indigenous goat populations based on microsatellite analysis

Twelve Chinese indigenous goat populations were genotyped for twenty-six microsatellite markers recommended by the EU Sheep and Goat Biodiversity Project. A total of 452 goats were tested. Seventeen of the 26 microsatellite markers used in this analysis had four or more alleles. The mean expected heterozygosity and the mean observed heterozygosity for the population varied from 0.611 to 0.784 and 0.602 to 0.783 respectively. The mean F_ST (0.105) demonstrated that about 89.5% of the total genetic variation was due to the genetic differentiation within each population. A phylogenetic tree based on the Nei (1978) standard genetic distance displayed a remarkable degree of consistency with their different geographical origins and their presumed migration throughout China. The correspondence analysis did not only distinguish population groups, but also confirmed the above results, classifying the important populations contributing to diversity. Additionally, some specific alleles were shown to be important in the construction of the population structure. The study analyzed the recent origins of these populations and contributed to the knowledge and genetic characterization of Chinese indigenous goat populations. In addition, the seventeen microsatellites recommended by the EU Sheep and Goat Biodiversity Project proved to be useful for the biodiversity studies in goat breeds.     

中国绒山羊遗传多样性现状和系统发生关系的微卫星分析

为了调查中国绒山羊遗传资源现状, 作者应用联合国粮农组织和国际家畜研究所推荐的19对微卫星引物并结合荧光PCR技术, 对9个中国地方产绒山羊群体和1个西非山羊品种进行了遗传多样性检测。14个微卫星座位在10个山羊群体中显示为高度多态, 可作为山羊遗传多样性分析的有效标记。多态信息含量和遗传杂合度等数据表明: 目前中国地方产绒山羊群体的遗传多样性较为丰富, 并且大部分保种场较好地保存了这些地方资源。采用非加权配对算术平均法构建的聚类图和采用主成分分析法得到的散点图均显示, 中国山羊与西非山羊为不同的2类; 中国产绒山羊中河谷山羊、河西绒山羊与其他山羊的遗传距离较远; 其他山羊又大致分为2类: 一类由辽宁绒山羊、新疆山羊、柴达木山羊、陕北山羊组成, 另一类由内蒙古绒山羊组成。此研究结果为开展我国地方绒山羊种质特性研究及资源保护和利用提供了科学依据。     

东北大口鲇2个群体的微卫星DNA多态分析

利用磁珠富集法克隆制备的24个大口鲇（Silurus meriaionalis Chen）微卫星标记,对黑龙江野生群体与松花江养殖群体2个东北大口鲇（S．soldatovi）的地理种群的等位基因频率（P）、观测杂合度（Ho）、期望杂合度（He）、多态信息含量（PIC）和有效等位基因数（Ne）等进行了遗传检测,以遗传偏离指数（d）检验Hardy—Weinberg平衡,并以Nei氏遗传分化系数（GST）和AMOVA分析（ФST）群体遗传变异的来源。同时,使用PHYLIP3．63软件绘制基于Nei氏遗传距离的个体间UPGMA系统树。结果表明：24个微卫星标记在东北大口鲇的2个群体中共扩增出1357条多态性片段,片段长度为1024385bp,总体平均等位基因8．875个,可以用于东北大口鲇遗传多样性的评估。并发现8个可区分这2个种群的遗传标记;黑龙江群体的P、Ho、He、PIC和Ne依次为0．165、0．435、0．758、0．742和5．019,松花江群体为0．147、0．299、0．847、0．764和5．944,在这些多样性参数上,方差分析也显示2地理种群差异不显著,在大多数位点并无显著差异,仅HLJcf37位点具有显著差异：在多个位点偏离Hardy—Weinberg平衡,2群体呈现不同程度的杂合体过度,纯合体完全缺失现象,其原因有待证实;群体遗传变异分析证实2群体间遗传分化较弱,其98％以上的变异是由群体内个体间的遗传变异引起的,群体间的变异对总变异影响不显著。UPGMA系统树也显示出个体间遗传距离小,亲缘关系很近。结果表明,人工繁殖没有对东北大口鲇的遗传多样性产生影响,该种群遗传分化小,种质资源状况良好。     

Genetic relationships between 14 native Spanish breeds of goat

Summary. The genetic distances separating 14 Spanish goat breeds are calculated from gene frequency data of 14 genetic blood markers (GSH, Ke, Hb, Dia, Ct, MDH, CA, X, NP, Alp, Am, Cp, Tf and Al).
Working from the matrix of Nei's genetic distances we drew a dendrogram demonstrating a great genetic similarity among populations from Negra Serrana, Zamorana, Guadarrama, Retinta, Blanca Andaluza, Berciana and Pirenaica on one hand; and Canaria, Murciana, Blanca Celtibérica, Verata, Palmera, Malaguena and Granadina on the other.
We discuss the similarities and differences within our classification using gene frequency data of the blood genetic markers studied, and classifications based chiefly on morphological and production data.     

Genetic diversity and population structure in multiple Chinese goat populations using a SNP panel

Information about genetic diversity and population structure among goat breeds is essential for genetic improvement, understanding of environmental adaptation as well as utilization and conservation of goat breeds. Here, we measured genetic diversity and population structure in multiple Chinese goat populations, namely, Nanjiang, Qinggeda, Arbas Cashmere, Jining Grey, Luoping Yellow and Guangfeng goats. A total of 193 individuals were genotyped for about 47 401 autosomal single nucleotide polymorphisms (SNPs). We found a high proportion of informative SNPs, ranging from 69.5% in the Luoping Yellow to 93.9% in the Jining Grey goat breeds with an average mean of 84.7%. Diversity, as measured by expected heterozygosity, ranged from 0.371 in Luoping Yellow to 0.405 in Jining Grey goat populations. The average estimated pair‐wise genetic differentiation (F_ST) among the populations was 8.6%, ranging from 0.2% to 16% and indicating low to moderate genetic differentiation. Principal component analysis, genetic structure and phylogenetic tree analysis revealed a clustering of six Chinese goat populations according to geographic distribution. The results from this study can contribute valuable genetic information and can properly assist with within‐breed diversity, which provides a good opportunity for sustainable utilization of and maintenance of genetic resource improvements in the Chinese goat populations.     

Erythrocyte potassium polymorphism in 14 Spanish goat breeds

Summary. The existence of polymorphism for erythrocyte potassium (Ke) is confirmed in certain Spanish breeds of goat. A statistical boundary is established between two caprine populations: low (LK) and high (HK) red cell potassium, the dividing line being set at 45 m-equiv/l of Ke. Both types are shown to be controlled genetically by an autosomal locus with two alleles K ^L and K ^h, being K ^L dominant over K ^h. The gene frequencies of K ^L and K ^h are determined in 14 native Spanish breeds of goat.     

罗伯逊易位群体遗传结构的DNA指纹分析

用微卫星探针（GGAT）4得到了罗伯逊易位猪群体内共9个家猪品种的DNA指纹图。1－9品种依次为：13／17罗伯逊易位纯合子猪群体、13／17罗伯逊易位杂合子猪群体、13／17罗伯逊易位杂合子猪互交所得到的正常核型猪群体（杂交0号）、丹系长白猪群体、加系双肌臂杜洛克猪群体、加系双肌臀大约克猪群体、加系双肌臀长白猪群体、丹系长白猪与13／17易位杂合子猪产生的杂交后备猪群体（杂交1号）、杜洛克猪与13／17易位杂合子猪产生的杂交后备猪群体（杂交2号）。根据指纹带型计算了每个群体的相似系数（F）、平均等位基因频率（Q）、最底平均杂合率（H）和遗传距离指数（D）。9个品种的相似系数介于0．546－0．931,根据各品种之间的遗传距离指数作出矩阵图,并据此绘制出品种间亲缘关系树状聚类图。