藏鸡和两种低地鸡线粒体全基因组序列 的测定和比对

藏鸡生活在青藏高原, 它对高原低氧具有一定的遗传适应能力. 丝羽乌骨鸡和寿光鸡都是低地鸡种, 缺乏对低氧环境的遗传适应能力. 鸡的线粒体基因组总长16785 bp, 共编码37个基因, 这些基因的编码产物均与线粒体的呼吸作用和氧化磷酸化相关, 它们的突变均有可能影响线粒体的功能, 因此均可被选为藏鸡低氧遗传适应的候选基因. 测定比较藏鸡和低地鸡的线粒体基因组, 可以为进一步研究藏鸡的低氧遗传适应机理提供线索. 本研究测定和比较了藏鸡、丝羽乌骨鸡和寿光鸡的线粒体全基因组序列, 发现藏鸡线粒体基因组总长为16784~16786 bp, 丝羽乌骨鸡为16785 bp, 寿光鸡为16784 bp; 比对后共发现突变(包括单核苷酸多态性(SNP)、单碱基缺失和插入)120个, 其中tRNA基因突变4个, rRNA基因突变10个, D-LOOP区突变39个, 基因间隔区突变1个, 编码蛋白质亚基的碱基突变66个(包括同义突变48个, 错义突变18个).     

藏鸡和两种低地鸡线粒体全基因组序列 的测定和比对

藏鸡生活在青藏高原, 它对高原低氧具有一定的遗传适应能力. 丝羽乌骨鸡和寿光鸡都是低地鸡种, 缺乏对低氧环境的遗传适应能力. 鸡的线粒体基因组总长16785 bp, 共编码37个基因, 这些基因的编码产物均与线粒体的呼吸作用和氧化磷酸化相关, 它们的突变均有可能影响线粒体的功能, 因此均可被选为藏鸡低氧遗传适应的候选基因. 测定比较藏鸡和低地鸡的线粒体基因组, 可以为进一步研究藏鸡的低氧遗传适应机理提供线索. 本研究测定和比较了藏鸡、丝羽乌骨鸡和寿光鸡的线粒体全基因组序列, 发现藏鸡线粒体基因组总长为16784~16786 bp, 丝羽乌骨鸡为16785 bp, 寿光鸡为16784 bp; 比对后共发现突变(包括单核苷酸多态性(SNP)、单碱基缺失和插入)120个, 其中tRNA基因突变4个, rRNA基因突变10个, D-LOOP区突变39个, 基因间隔区突变1个, 编码蛋白质亚基的碱基突变66个(包括同义突变48个, 错义突变18个).     

鸡含锰超氧化物歧化酶cDNA克隆及序列分析

 为弄清鸡含锰超氧化物歧化酶 (manganese containingsuperoxidedismutase ,MnSOD)的cDNA序列 ,以开展动物锰营养学的深入研究 ,根据已知鸡MnSOD的N端氨基酸序列设计简并引物 ,应用 3′RACE(rapidamplificationofcDNAends)技术 ,扩增克隆了鸡心肌MnSOD 990bp的 3′cDNA片段 .再根据 3′RACE片段测序结果设计引物进行 5′RACE ,结果获取了一个与 3′RACE片段相互重叠的鸡心肌MnSOD 52 1bp的 5′RACE片段 ,并对其进行了克隆测序 .最后根据 3′RACE片段和 5′RACE片段序列信息进行拼接 ,从而获取鸡MnSODcDNA的全序列信息 .研究结果表明 :鸡MnSODcDNA全长为 110 8个核苷酸 ,其中 5′非翻译区 2 5个核苷酸 ,编码区 675个核苷酸 ,3′非翻译区 4 0 8个核苷酸 ,编码一个长 2 2 4个氨基酸残基的蛋白质前体 .其中信号肽长 2 6个氨基酸残基 ,成熟肽长 198个氨基酸残基 ,分子量为 2 2kD .与人、大鼠、线虫、果蝇等真核生物MnSOD氨基酸序列的同源性分别为82 4 %、84 .7%、62 .4 %、59.3% .     

利用微卫星技术分析中国部分地方鸡种的遗传结构

利用7个微卫星标记对鹿苑鸡、固始鸡、藏鸡、白耳鸡、仙居鸡、茶花鸡、大骨鸡、北京油鸡、狼山鸡、河南斗鸡、泰和乌骨鸡和萧山鸡等12个中国地方鸡种的等位基因频率、基因杂合度、平均基因杂合度、多态信息含量以及群体间的亲缘关系进行分析。研究结果表明,12个地方鸡种在7个微卫星座位上的基因频率存在一定的差异;鹿苑鸡的平均基因杂合度最高,为0．5929;茶花鸡的平均遗传杂合度最低,为0．3514。平均多态信息含量也出现了类似的结果,说明鹿苑鸡的遗传多样性最丰富。模糊聚类分析结果表明,12个地方鸡种间,泰和乌骨鸡与河南斗鸡的亲缘关系相对较近,而固始鸡与其他11个地方鸡种的亲缘关系相对较远。12个地方鸡种可以聚为3类：泰和乌骨鸡、河南斗鸡、狼山鸡、大骨鸡、萧山鸡、北京油鸡、鹿苑鸡聚为第1个类群;茶花鸡、藏鸡、仙居鸡、白耳鸡聚为第2类群;固始鸡为第3类群。     

鸡二价金属转运蛋白1 cDNA的克隆与序列分析

鸡二价金属转运蛋白1（divalent metal transporter 1, DMT1）在动物胃肠道锰吸收过程中起重要作用.根据哺乳动物Dmt1同源蛋白氨基酸序列的保守性设计引物,应用3′RACE(rapid amplification of cDNA ends)技术,扩增并克隆获得鸡小肠Dmt1 cDNA 3′端1 289bp和1 092bp的2种片段,发现其3′端翻译区和非翻译区存在差异. 根据鸡Dmt1 cDNA 3′端片段的测序结果设计引物,扩增获得1个与3′端片段部分重叠的鸡Dmt1 cDNA 5′端907 bp片段,并对其进行了克隆测序. 根据鸡小肠Dmt1 3′RACE片段和5′RACE片段序列信息进行拼接,从而获得鸡小肠Dmt1 cDNA全序列信息.结果表明,鸡小肠Dmt1 cDNA有2种形式,1种全长为1 972个核苷酸,其中5′非翻译区为104个核苷酸,编码区1 695个核苷酸,3′非翻译区为173个核苷酸,编码1个含564个氨基酸残基的蛋白质;另1种形式为1 775个核苷酸,其中5′非翻译区为104个核苷酸,编码区1 593个核苷酸,3′非翻译区为78个核苷酸,编码1个含530个氨基酸残基的蛋白质.据鸡Dmt1 cDNA推测出的2种形式蛋白质的氨基酸序列与人、大鼠和小鼠的Dmt1蛋白具有高度同源性,它们的同源性分别为82%、82%、80%,和 84%、84%、83%. 对推测氨基酸序列进行疏水性和跨膜区分析表明,Dmt1蛋白为1种跨膜整合蛋白,具有膜转运蛋白糖基化位点和底物结合位点的保守序列.     

家鸡腺苷琥珀酸裂解酶基因多态性与肌苷酸含量的关联及其与红原鸡的亲缘关系

根据腺苷琥珀酸裂解酶(adenylosuccinate lyase, ADSL)基因外显子2的序列设计引物, 用PCR-SSCP的方法对隐性白羽鸡、丝羽乌骨鸡、白耳鸡、藏鸡以及红色原鸡两个亚种进行了单核苷酸多态性分析, 并检测到了多态性, 表现为3种基因型, 对两种纯合子进行直接测序, 结果发现3484位碱基处发生C→T突变。对3种基因型的肌肉肌苷酸含量的最小二乘分析结果显示TT型(突变型)个体的肌肉肌苷酸含量极显著地高于CT型、显著地高于CC型个体, CT型个体也稍高于CC型, 但差异不显著, 初步推测该位点可能与肌肉肌苷酸含量有关。根据该多态位点的基因频率, 基于Nei氏的遗传距离运用NJ聚类法构建系统发生树, 进行家鸡与原鸡的亲缘关系分析, 结果发现, 丝羽乌骨鸡与白耳鸡的亲缘关系最近, 藏鸡和中国红原鸡亚种的亲缘关系也较近, 中国地方家鸡品种与中国红原鸡亚种的亲缘关系较近,而与泰国红色原鸡的亲缘关系较远,隐性白羽鸡与原鸡亲缘关系最远, 初步得出中国家鸡有自己独自的血缘来源的结论。     

鸡8个功能基因5′-侧翼区与内含子的SNP多样性比较

本研究旨在探讨鸡功能基因5′-侧翼区的单核苷酸多态性(SNP)水平。作者以白来航鸡、隐性白洛克鸡、杏花鸡、丝羽乌骨鸡、固始鸡、红色原鸡为材料,扩增了GH、DDBC1、RIKEN、RASGRP3、IGF1、THRSP、VIP及PRL共8个基因的5′-侧翼区DNA序列。扩增序列全长为8,399bp,SNP的总数为161个,平均每52bp出现一个SNP。8个功能基因5′-侧翼区核苷酸多样性的θ均值和π均值分别为0.00620±0.00110和0.00559±0.00100。比较检验表明,5′-侧翼区的SNP多样性显著低于内含子区域。5′-侧翼区是基因表达的一个重要调控区域,在分子进化和系统发生过程中承受着比内含子区域更大的选择压,其较低的SNP多样性是适应性较好的表现。Tajima检验与Fu和Li检验表明,与鸡繁殖性状显著关联的VIP基因和PRL基因很可能是人工选择或自然选择的目的基因。     

三个品种家鸡催乳素基因cDNA的克隆及序列分析

从粤黄鸡、毛丝乌骨鸡及伊莎蛋鸡的垂体中快速抽提总RNA,根据国外已发表的肉用仔鸡乳素基因cDNA的序列,设计并合成了能与特定载体末端互补的1对引物,经反转录－聚合酶链式反应（RT－PCR）方法扩增获得了特异性片段。将扩增片段与线性化质粒pBSSK连接,克隆后进行序列分析,与已报道的肉用仔鸡、矮脚鸡和火鸡催乳素基因的核苷酸序列及推导的氨基酸序列进行了比较。结果表明,不同品种间核苷酸同源性介于93．97％－99．87％之间,其中丝毛乌骨鸡与矮脚鸡间的同源性最高为99．87％。推导的相应氨基酸序列的同源性在98．25％－100％之间,也是丝毛乌骨鸡与矮脚鸡间的同源性最高,为100％。在粤黄鸡、丝毛乌骨鸡和伊莎蛋鸡中,发现前两者的催乳素前体的cDNA片段推导的 氨基酸序列中信号肽裂触位点跟肉用仔鸡,矮脚鸡及火鸡的一样,为Leu-Pro-IIe-Cys,而伊莎蛋鸡的信号肽裂解位点则不一样,为Pro-Pro-IIe-Cys。此位点的差异可能导致催乳素前体翻译加工的不同,使伊莎蛋鸡无就巢性。这3个家鸡品种与国外的肉用仔鸡、矮脚鸡催乳素氨基酸序列还在以下位置出现差异：71、141、150、175。在肉用仔鸡、丝毛乌骨鸡催乳素氨基酸序列中还发现了一个肝素结合位点175－181（L－R－R－D－S－H－K）。     

番木瓜环斑病毒华南强株系cDNA文库的构建及其基因组3'端区域结构的研究

以λ-ZAPⅡ噬菌体为载体,构建了番木瓜环斑病毒华南强株系(PRV-SM)基因组cDNA文库。以PCR扩增的外壳蛋白(CP)基因为探针筛选出阳性克隆。酶谱和序列分析确定,其中两个阳性克隆除重叠部分外为长达2676个核苷酸的基因组3′端区域。其中包括棱内含体蛋白b(NIb)基因的1607个棱苷酸,CP基因的858个核苷酸和基因组3′端非编码区的211个核苷酸(不包括polyA尾巴)。PRV-SM的NIb含有依赖于RNA的RNA聚合酶的8个特征性保守序列,可能是参与基因组RNA复制的核心亚基。与其他株系比较,NIb的氨基酸变化主要集中在其C端和N端。PRV-SM 3′端非编码区有一段28个核苷酸的正向重复序列,能在其内形成茎环二级结构,并且在各株系间具有高度保守性。NIb,CP和3′端非编码区的总的序列比较表明,SM株系与国外报道的其他株系亲缘关系相对较远。     

辣椒多聚半乳糖醛酸酶基因CaPG的克隆与序列分析

以耐贮辣椒品系P98为材料,采用RACE方法,首次获得辣椒果实多聚半乳糖醛酶(PG)基因的全长cDNA,命名为CaPG,登录号为FJ596175.序列分析结果表明,该基因cDNA长1 668 bp,5′非编码区为119 bp,3′非编码区为442 bp,CDS长1 107 bp,编码368个氨基酸.Blast比对发现,该基因核苷酸序列与已报道的番茄和番木瓜PG基因具有84%和85%的相似性.聚类分析表明,该基因与番茄和番木瓜的亲缘关系较近,与拟南芥PG基因的亲缘关系较远.     

Phylogenetic analysis in chicken breeds inferred from complete cytochrome b gene information

Complete cytochrome b (cyt b) gene (1140 bp) nucleotide sequences were used to investigate characteristics of the genetic constitution of Chunky broiler chickens, and these were compared with the Hy-Line and WL-GM (Garber) line of White Leghorn, the GSP line of Fayoumi, the BM-C line of Black Minorca (egg-chickens), and an outgroup of wild-origin Japanese quail. A high genetic difference (five haplotypes) was observed at the cytochrome b region in the Chunky broiler in contrast to the high homologies observed among the other chicken breeds (egg-purpose). Chunky broilers can be distinguished from the other breeds (White Leghorn, Fayoumi, and Black Minorca) at positions 552 and 779. The molecular phylogenetic tree exhibited genetic differences within Chunky broilers, and between Chunky broilers and the other three chicken breeds. As a result, some chicken strains or breeds apparently different from the other egg-chickens may have contributed to the Chunky broiler formation. Artificial selection may be one of the biggest factors causing nucleotide diversity in the chicken breeds.     

我国部分地方鸡种肤色伴性遗传初步观察

对泰和鸡、仙居鸡、固始鸡、北京油鸡、萧山鸡、狼山鸡（Ｎ系）进行肤色伴性遗传观察,结果表明：泰和鸡常染色体上含有１对黑色素基因ＰＰ,仙居鸡、萧山鸡、北京油鸡性染色体上含有Ｉｄ抑制色素基因,狼山鸡、固始鸡、泰和鸡性染色体上含有ｉｄ基因,泰和鸡♂与含有Ｉｄ基因鸡种（仙居鸡、萧山鸡、北京油鸡）♀杂交,Ｆ１代肤色能自别雌雄,公鸡为黄皮肤,母鸡为黑皮肤。     

浙江省地方鸡种的遗传多样性研究

测定了浙江省5个地方鸡种及来航鸡（对照）线粒体D－环区的部分序列（539bp）,构建了鸡种的分子系统树。在所测序列中共有24个变异位点,变异率为4．45％。结果显示,浙江省地方鸡种分为两支,有两个母系来源,一支为仙居鸡,它和外来品种来航鸡关系较近,有共同的母系祖先。另一支为灵昆鸡、白银耳鸡、乌骨鸡和萧山鸡,它们有着共同的母系祖先,其中灵昆鸡,白银耳鸡、乌骨鸡较近,萧山鸡与此3种鸡关系较远。     

Endothermic heart rate response in broiler and White Leghorn chicks (Gallus gallus domesticus) during the first two days of post-hatch life

The embryonic modal value of heart rate (MHR) differs between broiler and White Leghorn chickens, but the initial development of cholinergic chronotropic control of embryonic heart rate (HR) does not. Thus, we hypothesized that hatchling MHR should also differ between broiler and White Leghorn strains, while the development of a physiological regulation, such as the endothermic HR response, should not be different between hatchlings of the two strains. To test this, we measured the response of HR and cloaca temperature (Tb) to alteration of ambient temperature (Ta); i.e., 35 degrees C-25 degrees C-35 degrees C, in four groups of hatchlings on Days 0 and 1 post-hatch. Fertile eggs of both strains with similar mass were incubated simultaneously in the same incubator. Eggs of broiler chickens hatched approximately 7 h earlier than White Leghorn chicken eggs. Chick mass at hatching was identical in both strains, but diverged during 2 days after hatching. Tb measured at the initial Ta of 35 degrees C was identical in both strains. MHR at the same Ta was approximately 30 bpm lower in broiler chicks than in White Leghorn chicks, but the difference was reversed to that observed in the embryos. The endothermic HR response was advanced by approximately 1 day in broiler chicks compared with White Leghorn chicks. As a result, eggs of similar mass in both strains produced chicks with similar mass and Tb at hatching, but during 2 days of post-hatch life their masses diverged and regulation of the endothermic HR response developed earlier in broiler than in White Leghorn hatchlings. This physiological heterochrony between strains is most likely due to genetic selection for fast growth in broiler chickens.     

Gene duplication of endothelin 3 is closely correlated with the hyperpigmentation of the internal organs (Fibromelanosis) in silky chickens

During early development in vertebrates, pluripotent cells are generated from the neural crest and migrate according to their presumptive fate. In birds and mammals, one of the progeny cells, melanoblasts, generally migrate through a dorsolateral route of the trunk region and differentiate to melanocytes. However, Silky is an exceptional chicken in which numerous melanoblasts travel via a ventral pathway and disperse into internal organs. Finally, these ectopic melanocytes induce heavy dermal and visceral melanization known as Fibromelanosis (Fm). To identify the genetic basis of this phenotype, we confirmed the mode of inheritance of Fm as autosomal dominant and then performed linkage analysis with microsatellite markers and sequence-tagged site markers. Using 85 backcross progeny from crossing Black Minorca chickens (BM-C) with F(1) individuals between White Silky (WS) and BM-C Fm was located on 10.2-11.7 Mb of chicken chromosome 20. In addition, we noticed a DNA marker that all Silky chickens and the F(1) individuals showed heterozygous genotyping patterns, suggesting gene duplication in the Fm region. By quantitative real-time PCR assay, Silky line-specific gene duplication was detected as an ~130-kb interval. It contained five genes including endothelin 3 (EDN3), which encoded a potent mitogen for melanoblasts/melanocytes. EDN3 with another three of these duplicated genes in Silky chickens expressed almost twofold of those in BM-C. Present results strongly suggest that the increase of the expression levels resulting from the gene duplication in the Fm region is the trigger of hypermelanization in internal organs of Silky chickens.     

Genome‐wide association study reveals novel variants for growth and egg traits in Dongxiang blue‐shelled and White Leghorn chickens

This study was designed to investigate the genetic basis of growth and egg traits in Dongxiang blue‐shelled chickens and White Leghorn chickens. In this study, we employed a reduced representation sequencing approach called genotyping by genome reducing and sequencing to detect genome‐wide SNPs in 252 Dongxiang blue‐shelled chickens and 252 White Leghorn chickens. The Dongxiang blue‐shelled chicken breed has many specific traits and is characterized by blue‐shelled eggs, black plumage, black skin, black bone and black organs. The White Leghorn chicken is an egg‐type breed with high productivity. As multibreed genome‐wide association studies (GWASs) can improve precision due to less linkage disequilibrium across breeds, a multibreed GWAS was performed with 156 575 SNPs to identify the associated variants underlying growth and egg traits within the two chicken breeds. The analysis revealed 32 SNPs exhibiting a significant genome‐wide association with growth and egg traits. Some of the significant SNPs are located in genes that are known to impact growth and egg traits, but nearly half of the significant SNPs are located in genes with unclear functions in chickens. To our knowledge, this is the first multibreed genome‐wide report for the genetics of growth and egg traits in the Dongxiang blue‐shelled and White Leghorn chickens.     

Parallel Evolution of Polydactyly Traits in Chinese and European Chickens

Polydactyly is one of the most common hereditary congenital limb malformations in chickens and other vertebrates. The zone of polarizing activity regulatory sequence (ZRS) is critical for the development of polydactyly. The causative mutation of polydactyly in the Silkie chicken has been mapped to the ZRS; however, the causative mutations of other chicken breeds are yet to be established. To understand whether the same mutation decides the polydactyly phenotype in other chicken breeds, we detected the single-nucleotide polymorphism in 26 different chicken breeds, specifically, 24 Chinese indigenous breeds and 2 European breeds. The mutation was found to have fully penetrated chickens with polydactyly in China, indicating that it is causative for polydactyly in Chinese indigenous chickens. In comparison, the mutation showed no association with polydactyly in Houdan chickens, which originate from France, Europe. Based on the different morphology of polydactyly in Chinese and European breeds, we assumed that the trait might be attributable to different genetic foundations. Therefore, we subsequently performed genome-wide association analysis (GWAS) to locate the region associated with polydactyly. As a result, a ~0.39 Mb genomic region on GGA2p was identified. The region contains six candidate genes, with the causative mutation found in Chinese indigenous breeds also being located in this region. Our results demonstrate that polydactyly in chickens from China and Europe is caused by two independent mutation events that are closely located in the chicken genome.     

应用微卫星标记分析中国地方鸡种的遗传变异

利用 8个微卫星位点对中国 9个地方鸡种和 1个引进品种进行了遗传检测。计算出了各品种的平均杂合度、平均多态信息含量 (PIC)及品种间的遗传距离 ,并进行了系统聚类。结果表明 :8个微卫星位点上共检测到了5 4个等位基因 ,每个位点上平均为 6 .75个。各位点平均多态信息含量为 0 .5 0 71～ 0 .74 34,均表现出了高度多态性。各群体平均杂合度较高 ,为 0 .5 5 6 4～ 0 .7135 ,说明我国地方鸡种有着较丰富的遗传多样性。地方鸡种间的遗传距离相对较远 ,10个鸡种共分为三大类。研究结果对我国鸡种资源的评估、保存和预测杂种优势具有一定的指导意义     

Genetic relationships between Japanese native and commercial breeds using 70 chicken autosomal SNP genotypes by the DigiTag2 assay

Recently, single nucleotide polymorphisms (SNPs) have been used to identify genes or genomic regions responsible for economic traits, including genetic diseases in domestic animals, and to examine genetic diversity of populations. In this study, we genotyped 70 chicken autosomal SNPs using DigiTag2 assay to understand the genetic structure of the Japanese native chicken breeds Satsumadori and Ingie, and the relationship of these breeds with other established breeds, Rhode Island Red (RIR), commercial broiler and layer. Five breeds, each consisting of approximately 20 chickens, were subjected to the assay, revealing the following: Average expected heterozygosities of broiler, Satsumadori, RIR, layer and Ingie were 0.265, 0.254, 0.244, 0.179 and 0.176, respectively. Phylogenetic analysis using the concatenated 70 autosomal SNP genotypes distinguished all chickens and formed clusters of chickens belonging to the respective breeds. In addition, the 2-D scatter plot of the first two principal components was consistent with the phylogenic tree. Taken together with the pairwise F(st) distances, broiler and RIR were closely positioned near each other, while Ingie was positioned far from the other breeds. Structure analysis revealed that the probable number of genetic clusters (K) was six and four with maximum likelihood and ΔK values, respectively. The clustering with maximum likelihood revealed that, in addition to the clustering of the other five breeds, the Satsumadori was subdivided into two genetic clusters. The clustering with ΔK value indicated that the broiler and Rhode Island Red were assigned to the same genetic cluster.     

利用微卫星标记分析四川8个地方鸡品种遗传多样性

通过选用30个多态性较好的微卫星标记,检测了四川省8个地方鸡品种：峨嵋黑鸡、泸宁鸡、旧院黑鸡、米易鸡、石棉草科鸡、凉山崖鹰鸡、兴文乌骨鸡、沐川乌骨鸡的遗传多样性。利用等位基因频率计算出各群体的平均遗传杂合度（H）、多态信息含量（PIC）和群体间的DA遗传距离。结果表明：30个微卫星位点中有24个微卫星位点在8个鸡群体中的多态信息含量均为高度多态,可作为有效的遗传标记用于各鸡品种的遗传多样性和系统发生关系的分析。各鸡种的杂合度都较高,平均杂合度范围是0.629~0.681,最高的是泸宁鸡（0.681）,最低的是旧院黑鸡（0.629）。据分析可能是由于交通闭塞,形成了家禽品种的多种多型,而且杂合度的高低与PIC值的大小体现了较高的一致性。对DA遗传距离的计算表明：用UPGMA法进行聚类分析,结果8个鸡品种被聚为3类：Ⅰ类：峨嵋黑鸡、米易鸡、泸宁鸡、旧院黑鸡聚为一类。米易鸡、泸宁鸡先聚在一起,然后又与峨嵋黑鸡在较近的距离聚在一起,然后再与旧院黑鸡聚在一起;Ⅱ类：石棉草科鸡、兴文乌骨鸡、沐川乌骨鸡聚为一类。兴文乌骨鸡、沐川乌骨鸡在较近的距离聚在一起,然后又与石棉草科鸡在较近的距离聚在一起;Ⅲ类：凉山崖鹰鸡独自聚为一类。这与几个鸡品种的来源、分化、选育历史及地理分布是一致的。