人类基因组中单核苷酸多态性的检测技术

随着人类基因组测序工作的完成,单核苷酸多态性作为继限制性片段长度多态性和微卫星多态性这2种遗传标记之后的第3代遗传标记,已成为人类后基因组时代的主要研究内容之一。系统地介绍了人类基因组中单核苷酸多态性的传统检测方法、新的方法以及基于生物信息学的方法,并对SNP检测技术的发展进行了展望。     

基于生物信息学的SNP候选位点搜寻方法

单核苷酸多态性（Single Nucleotide Polymorphism,SNP)是人类基因组中最常见的遗传多态,在遗传学研究的很多方面具有重要的作用。它的搜寻正受到广泛关注。近年来,国际上出现了一种基于生物信息学的发掘SNP新方法,本对方法的两种策略及其各自所存在的问题作一介绍。     

鸡6个功能基因microRNA靶标区域SNP的生物信息学预测

GDF-8、IGF-I,IGF-III、IGF2R、,IGFBP2和GHR是鸡的重要经济性状候选基因.利用miRanda和Targetscan软件预测6个基因3'UTR潜在的microRNA靶标,并发掘靶标区域SNP位点.结果表明:在6个基因的26个microRNA靶标区域,共检测到125个SNP位点,在靶标及其5'和3'邻接等长侧翼区分别检测到47个,44个和35个SNPs位点,其中12个SNP定位于靶标种子序列互补区.种子序列互补区及其3'侧翼区的SNP位点可能会影响microRNA的调控,导致家禽的表型变异.     

鸡MD基因5＇侧翼区多态性与鸡生长和体组成性状的相关研究

苹果酸脱氢酶（Malate Dehydrogenase,MD）是一种氧化还原性酶,参与体内多种能量代谢反应.它可以催化苹果酸氧化脱羧生成丙酮酸和CO2,并使NADP＋还原成NADPH,NADPH是脂肪酸合成所必需的载体,棕榈酸可以利用生成的NADPH来合成长链脂肪酸,MD的活性与脂肪酸合成效率之间存在密切的相关,MD也参与体内骨骼肌、心肌的能量代谢,并对肌纤维的生长有一定的调节作用.根据鸡MD基因的5侧翼区序列设计一对引物,用直接测序的方法在侧翼区检测多态性位点,在235bp（GenBank登录号：U49693）处发现一个SNP位点,此位点是一个限制性内切酶（SphⅠ酶）发生变化的位点.以东北农业大学高低脂双向选择系的第8世代肉鸡和东农F2资源群体为实验材料,用PCR-RFLP的方法进行基因型分析,建立适合的统计模型,进行基因型与生长和体组成性状的相关分析.结果表明：在高低脂系第8世代肉鸡中AA基因型个体的腹脂重和腹脂率显著高于BB基因型个体（P＜0.05）;BB基因型个体的大胸肌重和大胸肌率显著高于AA基因型个体（P＜0.05）.在东农F2资源家系中BB基因型个体的大胸肌重和大胸肌率显著高于AA和AB基因型个体（P＜0.05）;AA基因型个体的肝脏重和肝脏率显著高于BB基因型个体（P＜0.05）.综上所述,MD基因可能是影响鸡生长和体组成性状的主效基因或与控制生长和体组成性状的主效基因相连锁.     

鸡6个功能基因microRNA靶标区域SNP的生物信息学预测

GDF-8、IGF-I、IGF-III、IGF2R、IGFBP2和GHR是鸡的重要经济性状候选基因。利用miRanda和Targetscan软件预测6个基因3′UTR潜在的microRNA靶标, 并发掘靶标区域SNP位点。结果表明: 在6个基因的26个microRNA靶标区域, 共检测到125个SNP位点, 在靶标及其5′和3′邻接等长侧翼区分别检测到47个、44个和35个SNPs位点, 其中12个SNP定位于靶标种子序列互补区。种子序列互补区及其3′侧翼区的SNP位点可能会影响microRNA的调控, 导致家禽的表型变异     

奶牛CRP基因SNP的生物信息学分析

利用PCR-SSCP方法检测了CRP基因在中国荷斯坦奶牛群体中的单核苷酸多态性,并用各种网络分析软件分析了单核苷酸改变对其功能的影响。结果表明:CRP基因在P1引物扩增片段中存在PCR-SSCP多态性并引起编码氨基酸的改变。经测序分析可知,位于P1引物扩增片段内存在G→T突变,该突变位点使编码的氨基酸发生Q→H的改变。对引起编码氨基酸的P1位点进一步进行生物信息学分析发现,由于编码的改变引起新的转录结合们点vaccinia-term-s的产生,但没有引起其它CRP二三级结构的变化。这一分析结果可为奶牛CRP基因突变所产生的性状功能的改变提供分子水平的解释。     

鸡MD基因5'侧翼区多态性与鸡生长和体组成性状的相关研究

苹果酸脱氢酶(Malate Dehydrogenase,MD)是一种氧化还原性酶,参与体内多种能量代谢反应.它可以催化苹果酸氧化脱羧生成丙酮酸和CO2,并使NADP+还原成NADPH,NADPH是脂肪酸合成所必需的载体,棕榈酸可以利用生成的NADPH来合成长链脂肪酸,MD的活性与脂肪酸合成效率之间存在密切的相关,MD也参与体内骨骼肌、心肌的能量代谢,并对肌纤维的生长有一定的调节作用.根据鸡MD基因的5侧翼区序列设计一对引物,用直接测序的方法在侧翼区检测多态性位点,在235bp(GenBank登录号U49693)处发现一个SNP位点,此位点是一个限制性内切酶(SphⅠ酶)发生变化的位点.以东北农业大学高低脂双向选择系的第8世代肉鸡和东农F2资源群体为实验材料,用PCR-RFLP的方法进行基因型分析,建立适合的统计模型,进行基因型与生长和体组成性状的相关分析.结果表明在高低脂系第8世代肉鸡中AA基因型个体的腹脂重和腹脂率显著高于BB基因型个体(P＜0.05);BB基因型个体的大胸肌重和大胸肌率显著高于AA基因型个体(P＜0.05).在东农F2资源家系中BB基因型个体的大胸肌重和大胸肌率显著高于AA和AB基因型个体(P＜0.05);AA基因型个体的肝脏重和肝脏率显著高于BB基因型个体(P＜0.05).综上所述,MD基因可能是影响鸡生长和体组成性状的主效基因或与控制生长和体组成性状的主效基因相连锁.     

SNP与Hbb基因多态性的关联性

目的从单核苷酸多态性（single nucleotide polymorphism,SNP）水平探索小鼠生化标记基因Hbb多态性的形成机理。方法从DNA、RNA和蛋白多肽3个方面分析研究Hbb基因的多态性。结果基因组DNA中有4个SNP位点与Hbbd/s多态性相关：分别为外显子1中的2个T（G）,外显子2中的G（A）和外显子3中的A（G）;RNA水平有4个SNP位点与Hbbd/s多态性相关：分别对应为外显子1中的2个T（G）,外显子2中的G（A）和外显子3中的A（G）;蛋白多肽水平第13、20和139位氨基酸残基,即Cys/Gly、Ser/Ala和Thr/Ala间的转换与Hbb/s多态性相关,分别对应于外显子1中的2个T（G）和外显子3中的A（G）。结论第13、20和139位氨基酸残基,即Cys/Gly、Ser/Ala和Thr/Ala间的转换可能是Hbbd/s多态性的形成原因。     

拷贝数变异: 基因组多样性的新形式

基因拷贝数变异是指DNA片段大小范围从kb到Mb的亚微观突变, 是一可能具有致病性、良性或未知临床意义的基因组改变。Fosmid末端配对序列比较策略、比较基因组杂交芯片是当前较多使用的检测手段。染色体非等位的同源重排、非同源突变和非b DNA结构是造成基因组拷贝数变异的重要原因。拷贝数变异可导致不同程度的基因表达差异, 对正常表型的构成及疾病的发生发展具有一定作用。文章在总结基因拷贝数变异的认识过程和研究策略的基础上, 分析了拷贝数变异的形成和作用机制, 介绍了第一代人类基因组拷贝数变异图谱, 阐述了拷贝数变异研究的临床意义, 提示在探索疾病相关的遗传变异时不能错失拷贝数变异这一基因组多样性的新形式。     

鸡MD基因5′侧翼区多态性与鸡生长和体组成性状的相关研究(英文)

苹果酸脱氢酶(MalateDehydrogenase,MD)是一种氧化还原性酶,参与体内多种能量代谢反应。它可以催化苹果酸氧化脱羧生成丙酮酸和CO2,并使NADP+还原成NADPH,NADPH是脂肪酸合成所必需的载体,棕榈酸可以利用生成的NADPH来合成长链脂肪酸,MD的活性与脂肪酸合成效率之间存在密切的相关,MD也参与体内骨骼肌、心肌的能量代谢,并对肌纤维的生长有一定的调节作用。根据鸡MD基因的5′侧翼区序列设计一对引物,用直接测序的方法在侧翼区检测多态性位点,在235bp(GenBank登录号:U49693)处发现一个SNP位点,此位点是一个限制性内切酶(SphⅠ酶)发生变化的位点。以东北农业大学高低脂双向选择系的第8世代肉鸡和东农F2资源群体为实验材料,用PCR-RFLP的方法进行基因型分析,建立适合的统计模型,进行基因型与生长和体组成性状的相关分析。结果表明:在高低脂系第8世代肉鸡中AA基因型个体的腹脂重和腹脂率显著高于BB基因型个体(P<0.05);BB基因型个体的大胸肌重和大胸肌率显著高于AA基因型个体(P<0.05)。在东农F2资源家系中BB基因型个体的大胸肌重和大胸肌率显著高于AA和AB基因型个体(P<0.05);AA基因型个体的肝脏重和肝脏率显著高于BB基因型个体(P<0.05)。综上所述,MD基因可能是影响鸡生长和体组成性状的主效基因或与控制生长和体组成性状的主效基因相连锁。     

Single nucleotide polymorphisms in chicken lmbr1 gene were associated with chicken growth and carcass traits

Lmbr1 is the key candidate gene controlling vertebrate limb development, but its effects on animal growth and carcass traits have never been reported. In this experiment, lmbr1 was taken as the candi-date gene affecting chicken growth and carcass traits. T/C and G/A mutations located in exon 16 and one A/C mutation located in intron 5 of chicken lmbr1 were detected from Silky, White Plymouth Rock broilers and their F2 crossing chickens by PCR-SSCP and sequencing methods. The analysis of vari-ance (ANOVA) results suggests that T/C polymorphism of exon 16 had significant association with eviscerated yield rate (EYR), gizzard rate (GR), shank and claw rate (SCR) and shank girth (SG); A/C polymorphism of intron 5 was significantly associated with SCR, liver rate and head-neck weight (HNW), while both sites had no significant association with other growth and carcass traits. These results demonstrate that lmbr1 gene could be a genetic locus or linked to a major gene significantly affecting these growth and carcass traits in chicken.     

Single nucleotide polymorphisms in chicken lmbr1 gene were associated with chicken growth and carcass traits

Lmbr1 is the key candidate gene controlling vertebrate limb development, but its effects on animal growth and carcass traits have never been reported. In this experiment, lmbr1 was taken as the candidate gene affecting chicken growth and carcass traits. T/C and G/A mutations located in exon 16 and one A/C mutation located in intron 5 of chicken lmbr1 were detected from Silky, White Plymouth Rock broilers and their F₂ crossing chickens by PCR-SSCP and sequencing methods. The analysis of variance (ANOVA) results suggests that T/C polymorphism of exon 16 had significant association with eviscerated yield rate (EYR), gizzard rate (GR), shank and claw rate (SCR) and shank girth (SG); A/C polymorphism of intron 5 was significantly associated with SCR, liver rate and head-neck weight (HNW), while both sites had no significant association with other growth and carcass traits. These results demonstrate that lmbr1 gene could be a genetic locus or linked to a major gene significantly affecting these growth and carcass traits in chicken. Supported by the State Major Basic Research Development Program (Grant No. G20000161) and Beijing Natural Science Foundation (Grant No. 5011002)     

Single nucleotide polymorphisms in caprine calpastatin gene

The calpains and calpastatin (CAST) make up a major cytosolic proteolytic system, the calpain-calpastatin system, found in mammalian tissues. The relative levels of the components of the calpain-calpastatin system determine the extent of meat tenderization during postmortem storage. Calpastatin (CAST) is a protein inhibitor of the ubiquitous calcium-dependent proteases, μ-calpain, and m-calpain. Polymorphisms in the bovine, ovine and pig CAST gene have been associated with meat tenderness but little is known about how caprine CAST gene may affect goat meat quality traits. In this study we selected different parts of the CAST gene: (1) that have been previously reported to be polymorphic, intron 5 and 12 and 3’UTR; (2) first time explored (exon 3, 7 and 8 and part of intron 7 and 8) to investigate polymorphic status of caprine CAST gene. Using comparative sequencing ten novel SNPs located in exon 3 and intron 5, 7 and 8 were identified. Previously reported SNPs in intron 5, 3’UTR and intron 12 were absent. Sequence analysis revealed a non synonymous amino acid variation in exon 3, which would result in Lys/Arg substitution in the corresponding protein sequence. Considerable variation was detected in intronic regions. Twenty-four InDel were also recognized in intronic regions (15) and 3’UTR (9). All the sequences shared high homology with published bovine and ovine sequences. Three PCR-RFLP loci have been established for further analyzing genetic polymorphism in indigenous goats.     

黑柄炭角菌的单核苷酸多态性研究

以SNPs作为分子标记,对黑柄炭角菌的生活史和遗传多样性进行研究。基于黑柄炭角菌的基因组文库,在两个菌株（X-WC和X-LY）的34个片段（19,680bp）中共发现193个SNPs,SNP发生率为0.981%。193个SNPs位点都有两个可变的核苷酸,其中132个转换,61个颠换,转换与颠换比率为2.16。此外,对两个菌株序列进行比较,发现了41个插入/缺失位点。从34个片段中选择4个片段,分别比较菌株内的SNPs情况。X-WC的菌株内SNP发生率为每个核苷酸1.308%（30/2293）,X-LY的菌     

Single nucleotide polymorphisms in the equine transferrin gene

Single nucleotide polymorphisms (SNPs) in exons 13, 15 and 16 of equine transferrin for common, rare and mutant variants were investigated. Compared with previous work a further 13 SNPs have been identified, allowing for the two previously identified clades to be subdivided into 11 groups. A combination of one or more of eight SNPs can be used to classify the equine variants into these 11 groups, since most are co-inherited. Putative sites of glycosylation in exons 13 and 16 showed no polymorphism, suggesting that presence or absence of sugar moieties does not lead to electrophoretic variation between the variants. Using the 26 SNPs currently identified in transferrin it is still not possible to differentiate variants F1 from F2, or D from H2, which represent 75% of the variants occurring in Thoroughbred equine population. This suggests that further SNPs exist in equine transferrin. The significance of the high level of variation in exon 15 is discussed.     

Single nucleotide polymorphisms in the human E-cadherin gene

We report four DNA variants in the gene coding for the cell adhesion molecule E-cadherin. The polymorphisms affect codons 115, 133, 582 and the 3-noncoding region.     

Single nucleotide polymorphisms and recombination rate in humans

Levels of heterozygosity for single nucleotide polymorphisms vary by more than one order of magnitude in different regions of the human genome. Regional differences in the rate of recombination explain a substantial fraction of the variation in levels of nucleotide polymorphism, consistent with the widespread action of natural selection at the molecular level.     

Single nucleotide polymorphisms and linkage disequilibrium in sunflower

Genetic diversity in modern sunflower (Helianthus annuus L.) cultivars (elite oilseed inbred lines) has been shaped by domestication and breeding bottlenecks and wild and exotic allele introgression⁻the former narrowing and the latter broadening genetic diversity. To assess single nucleotide polymorphism (SNP) frequencies, nucleotide diversity, and linkage disequilibrium (LD) in modern cultivars, alleles were resequenced from 81 genic loci distributed throughout the sunflower genome. DNA polymorphisms were abundant; 1078 SNPs (1/45.7 bp) and 178 insertions-deletions (INDELs) (1/277.0 bp) were identified in 49.4 kbp of DNA/genotype. SNPs were twofold more frequent in noncoding (1/32.1 bp) than coding (1/62.8 bp) sequences. Nucleotide diversity was only slightly lower in inbred lines (θ = 0.0094) than wild populations (θ = 0.0128). Mean haplotype diversity was 0.74. When extraploted across the genome (~3500 Mbp), sunflower was predicted to harbor at least 76.4 million common SNPs among modern cultivar alleles. LD decayed more slowly in inbred lines than wild populations (mean LD declined to 0.32 by 5.5 kbp in the former, the maximum physical distance surveyed), a difference attributed to domestication and breeding bottlenecks. SNP frequencies and LD decay are sufficient in modern sunflower cultivars for very high-density genetic mapping and high-resolution association mapping.     

Single nucleotide polymorphisms and disease gene mapping

Single nucleotide polymorphisms are the most important and basic form of variation in the genome, and they are responsible for genetic effects that produce susceptibility to most autoimmune diseases. The rapid development of databases containing very large numbers of single nucleotide polymorphisms, and the characterization of haplotypes and patterns of linkage disequilibrium throughout the genome, provide a unique opportunity to advance association strategies in common disease rapidly over the next few years. Only the careful use of these strategies and a clear understanding of their statistical limits will allow novel genetic determinants for many of the common autoimmune diseases to be determined.     

鸡单核苷酸多态性与高清晰度QTL图谱的构建

作为一种重要的经济动物和模式动物, 鸡SNP多样性的研究以及鸡主要经济性状QTL定位的研究近年来成绩斐然。文章综述了上述研究成果, 并就SNP标记在鸡QTL精细定位方面的研究前景进行了展望。