Genetic Diversity Analysis of Sus scrofa Population in Guizhou Based on Mitochondrial CytbGene

【Objective】 The objective of this study was to evaluate the genetic diversity and genetic structure of Sus scrofa in Guizhou,so as to provide theoretical basis for further conservation genetics research and population ecological management,and then lay a foundation of the research of Sus scrofa conservation biology and its adaptation to the environment.【Method】 The mitochondrial Cytb gene of Sus scrofa was amplified by PCR and sequenced.Combined with 55 mitochondrial Cytb gene sequences of Sus scrofa downloaded from GenBank in other 9 regions in China,Mega 7.0 software was used for base composition and genetic distance analysis,and DNAsp6 software was used for genetic diversity analysis.【Result】 The ratio of Cytb gene (1 140 bp) of Sus scrofa in Guizhou was similar with other region,and AT content was higher than GC content.The 11 sequences had 6 variation sites and 4 haplotypes.The haplotype diversity was 0.600,and the nucleotide diversity was 0.00118.Haplotype diversity and nucleotide diversity were only higher than those of Sus scrofa populations in Jiangxi and Northeastern region.The genetic distance within species was small,and the genetic relationship was close.The neutral test Tajima's D and Fu's Fs values were negative,and the difference was not significant.The mismatch distribution analysis showed a unimodal distribution,it showed that Sus scrofa population in Guizhou was relatwely stable in history.The haplotype diagram was constructed using Network,and the analysis of haplotype phylogenetic tree constructed by Mega 7.0,which showed the haplotypes of Sus scrofa in Guizhou were shared with populations reported in other region (Hap_1 and Hap_10).【Conclusion】 This study concluded that Sus scrofa population in Guizhou was experiencing an expansion phase,but the population genetic diversity was lower than the populations in other region in China,the genetic distance of intrapopulation was small,and moderate comparing with the populations from other region in China.Therefore,the conservation management on genetic biodiversity of Sus scrofa in Guizhou should be paid more attention.     

江淮水牛线粒体D-loop区和Cytb基因遗传多态性及系统发育分析

为研究安徽江淮水牛群体的分子种质特性,本试验测定了江淮水牛2个亚群共82个个体的线粒体D-loop区和细胞色素b基因完整序列,分析了序列遗传多态性及系统进化关系,并结合GenBank中已发表的141条中国水牛D-loop序列,进行了联合分析。结果在D-loop区内共发现核苷酸多态位点91个,组成104个单倍型,其中32个是在江淮水牛中新发现的单倍型。总体mtDNA D-loop区核苷酸多样性为(0.015 43±0.001 42),单倍型多样性为(0.948±0.009)。其中,江淮水牛的mtDNA D-loop区核苷酸多样性为(0.014 89±0.002 32),单倍型多样性为(0.955±0.013),表明其群体遗传多样性丰富,群体变异性水平与中国其他水牛群体接近。根据线粒体D-loop区单倍型构建系统树和进化网络,显示江淮水牛存在沼泽型水牛线粒体支系A和B,表明其具有2个线粒体母系来源,其中B支又分为b1和b2两个亚支;针对细胞色素b基因的进化分析也支持这一结论。这些研究结果为今后开展江淮水牛遗传资源的保护和利用提供了客观依据。     

基于线粒体控制区的鸡不同杂交组合遗传多样性研究

旨在探讨鸡不同杂交组合线粒体控制区（mtDNA D-loop区）的遗传多样性和单倍型特性。选取固始鸡和隐性白羽鸡及其正、反交F1代、藏鸡以及F2代等6个群体共387个个体的mtDNA D-loop区进行测序,分析其遗传规律和单倍型特性,并与不同红色原鸡亚种进行聚类,分析其母系起源。结果显示,6个群体D-loop区全序列大小为1 231 bp,共检测到28个多态位点和1个C碱基缺失,共构成19种单倍型,分为A、B、C和E 4个单倍型群,其中,固始鸡和反交F1代主要为A、C单倍型,固始鸡A、C单倍型比例分别为53.42%和46.58%,反交F1代A、C单倍型比例分别为50.75%和49.25%;隐性白羽鸡、正交F1代和F2代优势单倍型均为E单倍型,占比分别为48.89%、48.84%和50.00%。6个鸡群体单倍型多样度（Hd）在0.496~0.729之间,核苷酸多样度（Pi）在0.003 40~0.005 41之间,Hd值和Pi值最大的均为正交F1代,其次为隐性白羽鸡和F2代,固始鸡和反交F1代群体遗传多样性接近。聚类分析显示,A、B单倍型群与滇南亚种交叉聚为一枝;E单倍型群与印度亚种交叉聚为一枝;C单倍型群与印度亚种、指名亚种、印尼亚种以及滇南亚种聚为一枝。结果提示,mtDNA D-loop区遵循严格的母系遗传,后代的遗传多样性和单倍型比例与其母本基本一致;我国家鸡群体具有多个红色原鸡母系起源,且主要起源于原鸡滇南亚种。     

建昌马mtDNA D-loop区遗传多样性及系统进化分析

试验旨在以线粒体DNA(mitochondrial DNA,mtDNA)为切入点,研究建昌马的母系遗传多样性与系统进化。从建昌马(n=39)血液中提取基因组DNA,用PCR方法扩增mtDNA D-loop区并直接测序,分析其高变区247 bp序列信息,统计mtDNA D-loop区的单倍型及变异位点,计算单倍型多样性(haplotype diversity,Hd)、核苷酸多样性(nucleotide diversity,Pi)和平均核苷酸变异数(average number of nucleotide differences,K)。构建包括建昌马在内的19个品种马的NJ系统进化树,计算各品种间的遗传距离。结果显示,试验获得了清晰的PCR扩增产物,并通过直接测序方法获得了约1200 bp的序列。39匹建昌马mtDNA D-loop区247 bp序列(其中1个样品缺失1 bp)的AT碱基含量为61.45%,属AT碱基对富集区,检测到33个多态性位点,共显示26种单倍型,其中4种为共享单倍型,且Hap7和Hap1为优势单倍型,单倍型多样性为0.947,核苷酸多样性为0.02399,平均核苷酸变异数为5.901,显示丰富的母系遗传多样性;NJ系统进化树显示,建昌马分布在A、C、D、E、F、G共6个支系中,约50%的样品分布在A支系,显示出复杂的母系起源;建昌马与关中马的遗传距离最小(0.021),其次是三河马、文山马、韩国车巨马(0.024),与韩国济州岛马遗传距离最大(0.032)。本研究结果表明,建昌马的mtDNA D-loop高变区遗传多样性丰富,具有多个母系起源,且A支系占有明显优势,与关中马、文山马可能有共同的母系起源。     

关中驴线粒体DNA D-loop多态性分析

本文对 6头关中驴线粒体DNAD loop区 399bp的核苷酸序列进行了分析。结果发现 ,关中驴的D loop区核苷酸变异只有转换 1种形式。 6头关中驴D loop区的核苷酸序列组成 3种单倍型 ,单倍型比例为 5 0 .0 0 % ,说明关中驴mtDNA遗传多样性正逐步丧失 ,需要加强驴种质资源保护。以欧洲驴D loop序列为对照 ,关中驴 3种单倍型的核苷酸变异率分别为 4 .2 1%、4 .5 1%和 0 .2 5 %。在获得的 399bpD loop碱基序列中 ,共检测出核苷酸多态位点18个 ,多态位点比例为 4 .5 1%。从D loop区核苷酸序列的 3种单倍型分析 ,发现关中驴可能有 2种不同的母系起源     

唐古拉山牦牛群体的母系遗传多样性及遗传结构分析

[目的]从分子水平上探究青海省唐古拉山牦牛群体的母系遗传多样性、群体遗传结构及其遗传背景。[方法] 对52头唐古拉山牦牛个体mtDNA D-loop区序列进行测定后,使用生物信息学软件分析确定其核苷酸变异位点和单倍型数目,计算单倍型多样度和核苷酸多样度大小,并进行系统发育分析。[结果] 在619 bp唐古拉山牦牛D-loop区序列分析中,排除2处插入（缺失）后共检测到31处多态位点,包括单一多态位点5处和简约信息位点26处。根据序列间核苷酸变异共确定了13种单倍型,单倍型多样度和核苷酸多样度分别为0.821±0.043和0.007±0.004。与我国其他18个家牦牛品种和野牦牛相比,唐古拉山牦牛群体单倍型多样度和核苷酸多样度值均较低,表明该群体遗传变异较为贫乏,母系遗传多样性水平较低。以美洲野牛为外群,邻接法（即NJ法）构建的系统发育树结果显示：唐古拉山牦牛群体13种单倍型分布在A、B、C、D和E五种单倍型组中,且聚为2个大的母系分支（即I和II）,支系Ⅰ占比为77%,提示唐古拉山牦牛由2个母系支系组成,拥有2个母系起源且以支系Ⅰ为主。 [结论] 唐古拉山牦牛母系遗传多样性水平较低,由2个母系支系组成,以支系Ⅰ为主,推测其有2个母系起源。     

Genetic Diversity and Evolution of Danzhou Chicken Assessed with Mitochondrial Complete DNA D-loop Region Sequencing

The objective of this study was to determine the genetic diversity and evolution of Danzhou chicken.The complete mitochondrial DNA (mtDNA) D-loop regions of 36 Danzhou chickens were amplified,sequenced and analyzed.The sequencing reads were compared with the complete mtDNA D-loop sequence of several relative strains of chicken annotated in GenBank,and analyzed by bioinformatics methods.The genetic diversity and its evolutionary relationship in Danzhou chicken were analyzed.The results showed that the lengths of PCR products at the D-loop region were 1 210 bp,with 59.9% being A+T and 40.1% as C+G.The variable regions were 167-1 215 bp,and the high variable regions were mainly 167-367 bp.A total of 20 variable sites that defined 6 haplotypes were identified.The average haplotype diversity (Hd) and average number of nucleotide difference (k) were 0.571 and 6.449,respectively,the nucleotide diversity (Pi) was 0.00537,and the Tajima's D value of neutrality test was 1.61643.6 haplotypes could be grouped to 3 haplogroups (A,B and C) as determined by phylogenic analysis,with B clade,as the most abundant population.It concluded that the genetic diversity and haplotype diversity of Danzhou chicken were relatively low.Phylogenetic tree showed that the genetic composition of Danzhou chicken came from 3 maternal ancestors,Gallus gallus spadiceus,Gallus gallus bankiva and Gallus gallus jabouillei were potential ancestors.There was few influence of exotic lineage detected,which indicated that Danzhou chicken was a relatively conserved breed.     

浙江省本地及引进鹅种遗传多样性研究

本研究利用PCR和DNA克隆测序技术扩增并分析了浙江省5个地方鹅种和1个引进家鹅品种96个个体的线粒体DNA D环区(D-loop)全序列。结果表明:浙江省境内的家鹅线粒体DNA D-loop全序长为1 166～1 179 bp,共发现89个变异位点,定义了36种单倍型,群体总核苷酸多样度达到了0.007 25,单倍型多样度为0.862,说明鹅群的遗传资源较为丰富,其中磐石灰鹅的遗传多样性最丰富,朗德鹅的遗传多样性最匮乏,而且没有发现朗德鹅与其他本地鹅种之间的显著差异。同时,个体聚类图中同品种内的个体没有聚在一起,说明浙江省鹅品种的母系来源比较混杂,品种选育偏重于父系,应同时结合基因组水平对其遗传结构进行分析。     

基于线粒体ATP6及Cytb基因多态性研究藏山羊高原适应性

为了探究藏山羊ATP6和Cytb是否具有潜在的高海拔适应性突变，本研究利用藏山羊（n=157，来自西藏地区的8个群体，海拔高度>3 500 m）与低海拔山羊（n=104，来自欧亚大陆50个群体，海拔高度<1 000 m）两组261条ATP6和Cytb序列，对核苷酸组成、遗传多样性、单倍型网络以及基因突变对蛋白结构域功能影响进行比较分析。结果，在ATP6和Cytb中分别鉴定出33和67个单核苷酸多态性位点（SNPs），其中错义突变均为6个。值得注意的是，ATP6 m.8102A>G（Ile→Met；P=0.000 6）和Cytb m.14794A>G（Thr→Ala；P=0.007 7）是低海拔山羊群体特有的错义突变，由此形成的单倍体H27和Ha36与高原适应性呈显著负相关（H27，P=0.007 0；Ha36，P=0.012 3）。进一步分析推测，这两个突变阻碍了质子跨膜的正常功能，并影响了质子或电子在OXPHOS中的转移，从而导致了低海拔山羊和藏山羊之间呼吸作用效率的差异。本研究通过对线粒体ATP6和Cytb基因编码区多态性到功能的相关分析，初步推测了藏山羊高海拔低氧适应性机制，为高原适应性相关研究提供了一定的见解。     

A Genetic Diversity Analysis of Mitochondrial DNA D-loop Region in Four High Quality Chicken Breeds

This study was conducted to elucidate the genetic diversity of mitochondrial DNA (mtDNA) D-loop region in Qingyuan partridge chicken group 1,Qingyuan partridge chicken group 2,Yangshan chicken and Qingyuan Yellow feather black-bone chicken.The specific primers were designed according to mtDNA D-loop region of Gullus gullus spadiceus (accession No.:NC_007235.1) in GenBank.The sequence was analyzed after PCR amplification and sequencing,and the haplotype number,polymorphism number,haplotype diversity,nucleotide diversity and nucleotide mean difference were counted.The evolution divergence among breeds was calculated by Mega 5.10 software,and the phylogenetic tree was constructed.The results showed that the length of mtDNA D-loop region in four high quality chicken breeds was 591 bp,and 549 bp were used for subsequent analysis.The content of A,T,C and G were 27.2% to 27.3%,30.1% to 30.4%,29.5% to 29.8% and 12.8% to 12.9%,respectively,and the average content of G+C was 42.5%.There were 92 polymorphic sites which contained 14 singleton variable sites and 78 parsimony informative sites,and the percentage of transitions and transversions were 89.13% (82/92) and 10.87% (10/92),respectively.The haplotype diversity ranged from 0.682 to 0.835,and the nucleotide diversity ranged from 0.00849 to 0.01167.There were 32 haplotypes in all sequences,which could be divided into clades A,B,C and E,however,most of the individuals belonged to clades B (51.2%) and E (37.6%).The phylogenetic tree results showed that four high quality chicken breeds could be classified as 4 branches which were consistent with the haplotypes classification results.The results indicated that the four high quality chicken populations from Qingyuan had relatively high haplotype and nucleotide diversity and likely shared two or more common maternal lineages.     

Analyses of Genetic Diversity and Phylogeny of mtDNA D-loop from Yak in Karakoram-Pamir Area

This experiment was conducted to clarify the genetic diversity,genetic differentiation and phylogenetic status of yak in Karakoram-Pamir area.The mtDNA D-loop region sequence was selected as a molecular marker,and the sequence and genetic diversity of the mtDNA D-loop region of yak in Karakoram-Pamir area were analyzed by PCR direct sequencing and bioinformatics methods.The yak sequence in GenBank was used.The maximum likelihood method was used to construct the phylogenetic tree and the intermediary network relationship.The results showed that the mtDNA D-loop sequence of yak in Karakoram-Pamir area was rich in A and T bases,with AT content of 61.2%,and there were 63 polymorphic loci,accounting for 7.04% of the total number of nucleotides.The results indicated that A and T bases were rich in the mtDNA D-loop sequences at 61.2%.There were 63 mutation sites,accounting for 7.04% of all nucleotides,The average haplotype diversity (Hd) was 0.806,the average nucleotide diversity (π) was 0.01528,and the average nucleotide difference (K) was 13.509,indicating that the yak was rich in genetic diversity in Karakoram-Pamir area;Through phylogenetic analysis,there were two branches in yak in China,forming two branches and six small clades.The yak in Karakoram-Pamir area involved in this study had two different maternal origins.Additionally,yak in the Karakoram-Pamir area was less shared with other breeds of yak haplotypes.In the branch C,the yak group in the Karakoram-Pamir area accounts for a large proportion and was shared with wild yak.The yak population in Karakoram-Pamir area had a unique genetic background,which might be the result of early domestication of wild yaks.It was suggested to increase the identification of yak breeds and the formulation of breed standards in this area,and strengthen the protection of yak genetic resources in this area.According to the current situation of the population,wild blood yaks were introduced for purification and rejuvenation to prevent breed degeneration and decrease of genetic diversity.The introduction of foreign yak breeds and disorderly hybridization were reduced to ensure the characteristics of this breed of high-quality yak breed resources.     

不同类型肉鸡线粒体单倍型与遗传起源研究

旨在探讨鸡线粒体D-loop区单倍型特性以及与生长速度的相关性,并分析其遗传起源。选取不同类型肉鸡品种（配套系）6个,测定其生产性能,并对6个群体共计314个个体线粒体D-loop区全长进行测序,分析其单倍型特性;同时与不同红色原鸡亚种进行聚类,分析其母系起源。结果显示,6个群体D-loop区全序列共检测到37个突变位点,构成40种单倍型,分为A、B、C和E 4个单倍型群,其中AA肉鸡、罗斯308、禽雁麻鸡和裕禾1号肉鸡主要为E单倍型,占比分别为85.92%、50.00%、100.00%和70.21%;园丰麻鸡2号和港丰瑶黑麻鸡E单倍型占比相对较低,分别为15.00%和22.39%,园丰麻鸡2号B单倍型含量最高,占比66.67%,港丰瑶黑麻鸡C单倍型含量最高,占比40.30%。相关性分析显示,初生重与E单倍型比例之间呈极显著正相关（P<0.01）,与A、B和C单倍型比例之间均呈负相关;E单倍型比例与公母平均体重约1.8 kg时日龄之间呈显著负相关（P<0.05）,而与公母平均体重约1.8 kg时饲料转化比之间呈极显著负相关（P<0.01）。聚类分析显示,A、B单倍型所有个体均与原鸡滇南亚种聚为一枝;E单倍型所有个体均与原鸡印度亚种聚为一枝;C单倍型所有个体与原鸡印度亚种、滇南亚种、指名亚种以及印尼亚种交叉聚为一类。结果提示,线粒体单倍型与肉鸡生长速度之间相关显著,E单倍型与肉鸡生长速度具有较强的正相关;我国家鸡群体母系起源丰富,但主要起源于原鸡滇南亚种。     

4种鼢鼠线粒体DNA D-loop区全序列分析

采用PCR测序技术对采自甘肃境内的4种鼢鼠22个个体的线粒体DAND-loop区全序列进行了测定。结果表明：鼢鼠线粒体DNAD-loop序列长度为893、894、895、896或899bp,核苷酸位点突变类型有5种,即转换、颠换、插入、缺失及转换与颠换共存。碱基转换以T〈=〉C形式为主。其中T、C、A、G4种核苷酸的平均比例分别为34．1％、24．3％、30．1％、11．5％,A＋T含量（64．2％）明显高于G＋C含量（35．8％）。这4种鼢鼠22条线粒体DNAD-loop区发现20种单倍型,单倍型比例为81．82％,说明中国鼢鼠mtDNA遗传多态性很丰富。从系统发育树分析,4种鼢鼠明显聚为两类,推测鼢鼠可能有两个起源。     

贵州威宁黄牛线粒体DNA D-loop区全序列分析

为了解贵州威宁黄牛的遗传多样性及遗传背景，我们分析测定了19个个体线粒体DNA D-loop区序列。结果检测到8种单倍型，7种为普通牛血统的单倍型，1种为瘤牛血统的单倍型，表明威宁黄牛同时受普通牛和瘤牛的影响。本研究同时构建了19个威宁黄牛个体的系统发生树，结果发现它们明显分为普通牛血统单倍型组和瘤牛血统单倍型组两组。     

东帕米尔高原地区藏兔群体遗传进化分析

旨在利用分子遗传学方法检测东帕米尔高原地区极端环境对当地藏兔群体的遗传多样性、遗传结构及遗传分化的影响,为帕米尔高原物种多样性和遗传多样性的保护提供研究资料.本研究通过PCR扩增及测序技术测定东帕米尔高原地区藏兔的线粒体CO1与ND4基因序列,使用相关生物信息学软件进行数据分析.结果表明,东帕米尔高原地区4个采样点37...     

阿坝藏族羌族自治州若尔盖地区藏猪mtDNA D-Loop的遗传多样性分析

旨在通过获得和对比若尔盖地区藏猪mtDNA D-Loop高变区的部分序列,为该地区藏猪遗传资源的保护与利用提供参考。本试验收集了若尔盖地区9个乡镇共80头藏猪耳组织,以甘南州藏猪mtDNA D-Loop基因序列为模板设计引物,采用PCR扩增测序技术获得了80条核苷酸序列,并采用生物信息学的数据处理方法进行分析。结果表明,若尔盖地区藏猪mtDNA D-Loop高变区（435 bp）的A+T含量（56.46%）明显高于G+C含量（43.54%）,存在碱基偏倚性现象;在80条长度为435 bp的序列中,共检测到14个变异位点,鉴定了17个单倍型,单倍型多样度（Hd）、核苷酸多样度（Pi）和平均核苷酸差异数（k）分别为0.881、0.004 66和2.028,其中Hd、Pi和k在降扎乡藏猪群体中最高,Pi和k在占哇乡藏猪中最低;共享单倍型8个,特有单倍型9个,且若尔盖地区不同藏猪群体间特有单倍型数差异较大,其中,降扎乡藏猪的特有单倍型数量最多,占单倍型总数的17.65%（3/17）;Hap_1和Hap_15单倍型是4个乡镇（降扎乡、益哇乡、热尔乡和冻列乡）群体的共享单倍型,表明这4个乡镇藏猪群体存在两个共同的母系祖先单倍型。若尔盖地区藏猪的平均遗传距离为0.004 66,其中降扎乡和冻列乡藏猪间的遗传距离最大为0.006 90,包座乡和益哇乡藏猪间的遗传距离最小为0.002 16;构建的NJ分子系统进化树将若尔盖地区藏猪分为2支,而加入中国地方家猪、野猪和引种猪后,若尔盖地区藏猪在进化树中比较分散,说明该地区藏猪母源血统遗传复杂,彼此之间基因交流多。本研究进一步证实了若尔盖地区藏猪比西藏林芝、山南、日喀则、甘孜州、阿坝州藏猪的遗传多样性程度高,受到人工选择强度低,应强化对若尔盖地区藏猪遗传资源的保护与利用。     

D‐loop sequence mitochondrial DNA variability of Sarda goat and other goat breeds and populations reared in the Mediterranean area

To provide useful knowledge on goat breed origin and history, we studied the mitochondrial DNA (mtDNA) of 69 goats from five different breeds, Camosciata delle Alpi, Maltese, Nubian, Saanen and Sarda, and one population, the Tunisian. All goats analysed displayed a moderate haplotype and nucleotide diversity. The highest was in the Sarda – the autochthonous breed reared in Sardinia. On the basis of mtDNA control region sequences, animals showed a high genetic haplotype diversity, 35 haplotypes were each represented by a single sequence and only a few haplotypes were shared among the animals. New haplotypes of goats reared in the Mediterranean area were identified and the majority of Italian goats belonged to haplogroup A. This result confirmed worldwide distribution and diversity of haplogroup A.     

Lineage classification of canine inheritable disorders using mitochondrial DNA haplotypes

To estimate the maternal effects of dog breeds using mitochondrial DNA(mtDNA) haplotypes in the dogs with several clinical disorders, 600 base pairs of mtDNA D-loop region were amplified from 365 dogs and were determined for mtDNA sequences. The diversity of the 600-bp sequences was classified into 64 haplotypes, including 46 newly discovered haplotypes, and the haplotypes were grouped into four clusters I to IV. Lineage analysis using the mtDNA haplotype indicated that each dog breed genetically comprises one or a few mtDNA haplotypes. When the relationship between genetic background and occurrences of clinical diseases was estimated, canine lineage analysis using mtDNA haplotype revealed that the disorders distributed in the dominant mtDNA haplotypes of each dog breed, but no disorder closely associated with mtDNA haplotypes was detected.     

中国荷斯坦牛PIK3CB基因多态性及其与繁殖和产奶性状的关联分析

【目的】 探究磷脂酰肌醇-4,5-二磷酸3-激酶催化亚单位β（PIK3CB）基因多态性及其与中国荷斯坦牛繁殖和产奶性状的关系。【方法】 通过混池测序对中国荷斯坦牛PIK3CB基因进行单核苷酸多态性（SNP）位点筛选,采用竞争性等位基因特异性PCR （KASP）技术在1 160头健康泌乳中国荷斯坦牛中进行SNP分型并进行群体遗传学分析,采用线性模型进行SNP与11个繁殖和产奶性状基于单位点和单倍型组合的关联分析。【结果】 在PIK3CB基因中共检测到了17个SNPs,筛选出7个SNPs用于后续分析。关联分析发现,7个SNPs与多个目标性状存在显著或极显著的关联（P<0.05;P<0.01）;位于外显子区域的g.130433743 A>G位点AA基因型个体和位于可变剪接区域的g.130448069 G>A位点GG基因型个体,其经产牛首末次配种间隔、产奶量、乳蛋白量和乳脂量最低,体细胞评分最高,上述基因型个体具有较短的首末次配种间隔,而产奶性能相对较差;g.130387717 G>A位点AA基因型个体,其初配日龄和青年牛首末次配种间隔最低,产奶量、乳蛋白量和乳脂量最高,该基因型个体的繁殖和产奶性能均较好,上述3个SNPs位点可作为中国荷斯坦牛繁殖和产奶性状的候选位点重点关注。单倍型分析发现,PIK3CB基因的g.130387717 G>A、g.130430832 A>－、g.130433743 A>G、g.130433982 C>T、g.130446073 C>T和g.130448069 G>A 6个SNPs紧密连锁形成一个单倍型块,且与多个目标性状存在显著或极显著关联（P<0.05;P<0.01）,其中H2H3和H2H4单倍型组合个体的繁殖和产奶性能较好,为优势单倍型组合。【结论】 中国荷斯坦牛PIK3CB基因存在丰富的遗传变异,其多态性与繁殖和产奶性状存在关联,g.130433743 A>G、g.130448069 G>A和g.130387717 G>A位点可作为潜在分子标记,为中国荷斯坦牛的平衡育种提供理论依据。     

基于RAD-Seq技术的大围山微型鸡遗传进化分析

【目的】 在分子水平上探讨大围山微型鸡的遗传进化。【方法】 以大围山微型鸡与其他18个地方鸡品种及2个国外引进品种为研究对象,每个品种选取公鸡10只,母鸡20只,采血,提取全基因组DNA,进行简化基因组测序(RAD-Seq),鉴定21个品种基因组SNP,计算大围山微型鸡遗传统计量,分析遗传多样性和遗传结构、筛选受选择基因并进行功能富集分析。【结果】 在大围山微型鸡群体中鉴定出331 892个SNPs。大围山微型鸡的平均杂合度(Ho)为0.219、核苷酸多样度(Pi)为0.245,近交系数(Fis)为0.107,与其他18个地方鸡种相比遗传多样性呈中度多态。聚类分析发现,大围山微型鸡与瓢鸡、茶花鸡和藏鸡聚为一类,亲缘关系较近,且与瓢鸡的群体分化指数(Fst)最低(0.0929),亲缘关系最近,与河南斗鸡的Fst最高(0.2179),亲缘关系最远。共筛选出200个受选择基因。GO分析结果显示,这些受选择基因主要富集在运动、刺激应答、信号传导等生物学过程;KEGG分析结果表明,这些受选择基因主要富集在代谢、肌动蛋白细胞骨架的调节、MAPK等信号通路。【结论】 大围山微型鸡遗传多样性呈中度多态,与瓢鸡亲缘关系最近,本研究筛选出了200个受到选择的基因,这些基因在代谢、信号传导、颅骨发育等多个方面发挥作用。