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1.
The Tibetan gazelle (Procapra picticaudata) is a threatened species and distributed on the Qinghai-Tibet Plateau of China (Qinghai Province, Tibet Autonomous Region and the adjacent Gansu Province, Sichuan Province, and Xinjiang Uigur Autonomous Region). Small peripheral populations of Tibetan gazelle were once found in northern Sikkim and Ladakh, but now these are close to extinction. To describe the evolutionary history and to assess the genetic diversity within this monotypic species and population structure among different geographic locations in China, we sequenced mitochondrial DNA from the control region (CR) and cytochrome (cyt) b gene for 46 individuals from 12 geographic localities in Qinghai, Tibet, Xinjiang, Gansu, and Sichuan. A total of 25 CR haplotypes and 16 cyt b haplotypes were identified from these gazelle samples. CR haplotype diversity (0.98+/-0.01) and nucleotide diversity (0.08+/-0.009) were both high. Phylogenetic trees indicate that the Tibetan gazelle in China can be divided into three main clades: Tibet, Sichuan (SCH) and Qinghai-Arjin Shan-Kekexili (QH-ARJ-KKXL). Analysis of molecular variance (AMOVA) and network analysis consistently support this geographic structure in both datasets. Significant differentiation between populations argues for the presence of management units (MUs). Such differentiation may reflect a geographic separation resulting from the uplift of the Qinghai-Tibet Plateau during the Late Pliocene and Pleistocene. Mismatch distribution analysis implies that Tibetan gazelle has undergone complex population changes. We suggest that the present population structure has resulted from habitat fragmentation during the recent glacial period on the Qinghai-Tibet Plateau and population expansion from glacial refugia after the glacial period. It is likely that the present populations of Tibetan gazelle exhibit a pattern reminiscent of several bottlenecks and expansions in the recent past. 相似文献
2.
测定了福建东张水库18尾陆封型香鱼的ND4-tRNASer基因533 bp序列,发现2个可变位点和2个简约信息位点,共检测到4种单倍型。基于Kimura 2-parameter模型的遗传距离在0.001 9~0.003 9之间,在NJ系统树上无明显谱系结构;单倍型多样性(Hd)和核苷酸多样性(Pi)分别为0.627和0.001 37,平均核苷酸差异数为0.732,远低于两侧洄游型日本香鱼指名亚种(Hd为0.793,Pi为0.002 94),与被列为IUCN濒危物种名录的日本琉球香鱼亚种(Hd=0.519,Pi=0.001 11)相当。东张水库香鱼遗传多样性如此贫乏到底是历史原因还是近期陆封的结果,仍需进一步研究。目前亟待采取有效措施保护东张水库陆封香鱼。 相似文献
3.
为了探究我国灰鹅品种的遗传多样性和系统进化,运用DNA测序技术测定了我国13个灰鹅品种mtDNAD-loop区521bp序列。结果表明:这13个灰鹅品种521bpD-loop区序列的T、C、A和G碱基含量分别为23.8%、29.0%、32.3%和15.0%;平均单倍型多样度和核苷酸多样度分别为0.19245和0.00036;13个灰鹅种间变异大于种内变异,且均未出现群体扩张现象;共享单倍型和系统进化树分析表明,伊犁鹅起源于灰雁(Anser anser),其余12个灰鹅品种起源于鸿雁(A.cygnoides)。 相似文献
4.
基于线粒体控制区序列对光裸方格星虫(Sipunculus nudus Linnaeus,1766)的2个养殖群体(营盘YP、竹林ZL)和4个野生群体(防城港FC、钦州QZ、大冠沙DG和越南海防YN)的91个个体进行遗传差异分析,研究光裸方格星虫养殖和野生群体的遗传变异情况。结果显示:获得的514 bp DNA序列中,野生与养殖群体的多态性位点数分别为82和60,均显示出对AT的偏倚性。共定义85个单倍型,共享单倍型4个,其中共享单倍型Hap5为原始单倍型,营盘群体均为独享单倍型。各群体的单倍型多样性(Hd)相同,野生群体的平均核苷酸多样性(Pi)(0.01531)略高于养殖群体(0.01514),6个群体的遗传多样性水平依次为YN > YP > QZ > FC > ZL > DG。各群体间的遗传分化并不显著(P>0.05),光裸方格星虫的遗传变异主要来自群体内个体间(99.08%),同时未发现明显的地理谱系结构。研究表明,光裸方格星虫野生群体的遗传多样性水平总体略高于养殖群体;滩涂底播养殖方式较池塘养殖更利于维持光裸方格星虫遗传多样性;各群体间不存在显著的遗传分化,养殖群体正逐渐积累遗传变异,但尚未足够以形成其独立的遗传结构。 相似文献
5.
A. I. Baranova D. V. Panchenko M. V. Kholodova K. F. Tirronen P. I. Danilov 《Biology Bulletin》2016,43(6):567-572
Based on the results of the analysis of nucleotide sequence polymorphism in the hypervariable fragment (left domain) of the mtDNA control region (D loop), the genetic diversity of wild reindeer from the eastern part of the Kola Peninsula (Murmansk oblast, Terskii region) was studied. Low values of the genetic diversity indices for Eurasian wild reindeer were detected. The effect of domestic reindeer breeding on the development of genetic diversity of the wild reindeer population in the studied region (indicating a low degree of hybridization of domesticated and wild reindeer) was estimated. 相似文献
6.
Genetic Diversity and Systematic Evolution of Chinese Domestic Ducks Along the Yangtze-Huai River 总被引:1,自引:0,他引:1
To investigate the population structure and systematic evolution of the domestic duck in China, we sequenced the 667 bp mitochondrial DNA (mtDNA) D-loop control region of 106 ducks from nine breeds along the Yangtze-Huai River. Of the total analyzed sites, 34 (5.1%) were polymorphic due to transitions, transversions, insertions, and deletions. Nucleotide content was 25.6% A, 33.3% C, 15.2% G, and 25.9% T. In total, 31 haplotypes were identified in the target region; of these, the major haplotype was A7, and nine haplotypes were shared by the tested ducks. The haplotype diversity (Hd) and average nucleotide diversity (Pi) were 0.798% and 0.28%, respectively. Hd was highest in the Jingjiang shelduck, followed by the Youxian and Enshi shelducks, and it was lowest in the Wendeng black duck. Nucleotide diversity (Dxy) among the nine breeds ranged from 0.139 to 0.433%, and the Kimura 2-parameter distances were 0.0013-0.0044. Molecular variance indicated that a very high proportion of the insignificant genetic variance was attributable to variations within breeds. Phylogenetic analysis of 31 haplotypes revealed only one distinct maternal lineage in the tested ducks, and no evidence was found of a contribution of the Anas zonorhyncha group B haplotype to the maternal origin of Chinese domestic duck breeds along the Yangtze-Huai. 相似文献
7.
中国部分猪种SLA-DQB外显子2遗传多样性 总被引:14,自引:0,他引:14
运用PCR-SSCP和克隆测序对中国部分猪种的SLA-DQB基因外显子2的多态性分析表明:有功能的DQB基因有68个新等位基因,假基因(SLA-DXB)等位基因有5个。各等位基因的数量分布极其不平衡,而且许多品种都表现出共享等位基因。9个主要等位基因中, C08广泛分布在中国猪种的6大地方类型11个品种及云南和四川野猪中,它为中国猪种特有的共享等位基因,占总数的55.10%。在单一的个体中拥有5条以上序列,说明SLA-DQB基因座在某些品种中拷贝数为3个。SLA-DQB外显子2的等位基因核苷酸和氨基酸多态变异位点分别高达81个和49个,等位基因多样度(H=0.889)以及核苷酸多样度(Pi =0.047)都很高,总体表现为β折叠区的Pi值均高于α螺旋区。综合分析表明华南型、西南型猪H和Pi均较高,高原型的藏猪最低。类群内遗传距离排序与Pi值高低排序一样,可见各地方类型中核苷酸替换的差异正比于核苷酸多样度。类群间遗传距离比较,江海型与华北型间的距离最大,而华中型和高原型间的遗传距离最小。 相似文献
8.
目前青藏高原高海拔地区古DNA研究匮乏。拉托唐古墓地位于青藏高原西南高海拔区域,本文对该墓地出土距今约700年的人骨进行古DNA提取,捕获了高质量线粒体全基因组数据,结合东亚线粒体基因组数据库,运用遗传统计方法开展分析。研究结果表明,距今3000年以内青藏高原西南部人群的遗传历史具有连续性,距今700年左右的拉托唐古墓地居民与距今3150-1250年的古代尼泊尔居民以及现代中国西藏居民母系遗传关系较近,且他们都具有共同的M9a1a1c1b1a单倍群。对M9a1a1c1b1a单倍群的深入研究发现,距今10930-5150年期间青藏高原可能发生了人口扩张事件。以上结果为我们了解古代青藏高原高海拔地区人群遗传历史提供了重要信息。 相似文献
9.
P. A. Sorokin N. V. Soldatova V. S. Lukarevskiy M. V. Kholodova 《Biology Bulletin》2011,38(6):585-590
Polymorphism of the nucleotide sequence of a hypervariable fragment of the D-loop (985 bp) of mtDNA in 76 Goitered gazelles
of subspecies Gazella subgutturosa subgutturosa from Uzbekistan, Turkmenistan, and Azerbaijan was studied. The genetic similarity of gazelles from Turkmenistan and Uzbekistan
has been identified. The population of gazelles from Shirvanskaya steppe reserve (Azerbaijan) is unique and strictly isolated
from other groups studied. A high haplotypic (H = 0.9649 ± 0.0091) and relatively low nucleotide diversity (π = 0.0212 ± 0.0105)
were noted for all investigated groups of gazelle based on this mtDNA fragment, which is probably related to ecological peculiarities
of the species and the history of formation of regional populations. 相似文献
10.
【目的】Wolbachia 是一种广泛存在于节肢动物中的胞内共生细菌,影响寄主的生物学特性。花蓟马 Frankliniella intonsa (Trybom)是重要的害虫,对农作物及园林植物造成危害。本研究旨在明确 Wolbachia 在花蓟马中的感染情况,并分析其与寄主线粒体DNA多样性的关系。【方法】采集中国境内26个花蓟马自然种群,运用多位点序列分型技术(multilocus sequence typing, MLST)对其体内 Wolbachia 感染率及株系进行分析;利用线粒体 COI 分子标记研究花蓟马的遗传分化及遗传多样性;通过比较感染和未感染 Wolbachia 个体 COI 数据,探究 Wolbachia 多样性与寄主线粒体DNA多样性之间的关系。【结果】花蓟马中 Wolbachia 的感染率为0%~60%,共检测到5种 Wolbachia 株系(wFint1,wFint2,wFint3,wFint4及wFint5),均属于B大组且形成一个单系群。Wolbachia感染情况与这些花蓟马种群(除CC, GZ, TA和TY, N<5)的线粒体DNA多样性相关,表现为不感染 Wolbachia 的种群中线粒体DNA单倍型多样性(Hd)与核苷酸多样性(Pi)均高于感染 Wolbachia 的种群,且 Wolbachia 感染率与 Hd 呈显著负相关( P <0.05)。AMOVA分析表明花蓟马线粒体DNA遗传分化与Wolbachia 感染情况有关。【结论】 Wolbachia 可能在侵染花蓟马种群后出现遗传分化;Wolbachia 感染与寄主线粒体DNA多样性有关。 相似文献
11.
中国部分家养山羊mtDNA D环区遗传多样性与进化 总被引:1,自引:0,他引:1
对我国10个家养山羊品种140只个体的mtDNA D-loop区进行测序分析, 测得结果: 整个D-loop区为 1 211~1 213 bp, 共检测到84种单倍型, 171个多态位点。其中核苷酸多样性(Nucleotide diversity, Pi)为: 0.02063 ± 0.00225, 单倍型多样性(Haplotype gene diversity, Hd)为: 0.988 ± 0.003, 平均核苷酸差异数(Average number of nucleotide differences) k为: 24.896。表明我国家养山羊品种遗传多样性丰富。通过构建NJ网络进化树, 得出中国家养山羊主要分为两大支系, 并且其中一支与角骨羊(Capra aegagrus)聚在一起, 而旋角野山羊(Capra fal-coneri)单独聚为一支, 说明角骨羊对中国家养山羊贡献较大。 相似文献
12.
Population variation of human mtDNA control region sequences detected by enzymatic amplification and sequence-specific oligonucleotide probes. 总被引:29,自引:6,他引:23 
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下载免费PDF全文 M Stoneking D Hedgecock R G Higuchi L Vigilant H A Erlich 《American journal of human genetics》1991,48(2):370-382
A method for detecting sequence variation of hypervariable segments of the mtDNA control region was developed. The technique uses hybridization of sequence-specific oligonucleotide (SSO) probes to DNA sequences that have been amplified by PCR. The nucleotide sequences of the two hypervariable segments of the mtDNA control region from 52 individuals were determined; these sequences were then used to define nine regions suitable for SSO typing. A total of 23 SSO probes were used to detect sequence variants at these nine regions in 525 individuals from five ethnic groups (African, Asian, Caucasian, Japanese, and Mexican). The SSO typing revealed an enormous amount of variability, with 274 mtDNA types observed among these 525 individuals and with diversity values, for each population, exceeding .95. For each of the nine mtDNA regions significant differences in the frequencies of sequence variants were observed between these five populations. The mtDNA SSO-typing system was successfully applied to a case involving individual identification of skeletal remains; the probability of a random match was approximately 0.7%. The potential useful applications of this mtDNA SSO-typing system thus include the analysis of individual identity as well as population genetic studies. 相似文献
13.
挖掘本土天敌资源是害虫生物防治的有效手段。桨角蚜小蜂Eretmocerus spp.是烟粉虱Bemisia tabaci重要的寄生性天敌之一,明确桨角蚜小蜂本地种类及遗传分化关系,对本土天敌资源挖掘具有重要意义。本研究在天津5个地区采集了13个地理、寄主的桨角蚜小蜂种群,利用线粒体mtDNA COI基因片段作为分子标记,进一步通过MEGAX、DnaSP 5.10等软件进行遗传分化分析。结果表明,本研究所采种群中包含2种桨角蚜小蜂,其中测得蒙氏桨角蚜小蜂Eretmocerus mundus mtDNACOI基因序列20条(755 bq),未命名桨角蚜小蜂Eretmocerus sp. WTT-2016 mtDNA COI基因序列20条(739 bq)。两种桨角蚜小蜂的遗传多样性均较低,其中蒙氏桨角蚜小蜂Hd=0.368,Pi=0.00557,K=4.205;未命名桨角蚜小蜂Hd=0.616,Pi=0.00106,K=0.784。错配分析表明,蒙氏桨角蚜小蜂在天津种群较稳定,近年来未出现扩张现象。 相似文献
14.
草鱼野生与选育群体线粒体DNA控制区D-loop遗传变异分析 总被引:4,自引:0,他引:4
为探究经过2个选育世代后选育群体遗传多样性和遗传结构的变化, 研究对4个野生群体(邗江、九江、石首和吴江)和2个选育世代(F1和F2)进行了线粒体DNA控制区(D-loop)序列的遗传变异分析。实验结果表明, 4个野生群体在单倍型数目(H)、单倍型多样性(Hd)、核苷酸多样性(π)、平均核苷酸差异数(K)水平上均高于2个选育世代, 在2个选育世代内表现为F1代群体的核苷酸多样性(π)和平均核苷酸差异数(K)大于F2代群体, 但单倍型多样性(Hd)小于F2代群体; 单倍型分析结果表明, 6个群体间无共享单倍型, 4个野生群体间共发现2种共享单倍型(Hap1和Hap3), 石首群体和2个选育世代共享1种单倍型(Hap15); 遗传分化指数(Fst)分析结果表明, 邗江、九江、吴江3个野生群体和2个选育世代间存在较大的遗传分化(Fst范围为0.41475—0.55128), 石首群体与F1代群体之间存在较小的遗传分化, 与F2代群体之间存在中等水平的遗传分化, 同时F1代群体与F2代群体之间存在较小的遗传分化; 基于6个群体276个个体构建的邻接(Neighbor-Joining, NJ)进化树和基于27种单倍型构建的单倍型网络图也得到了相似的结论, 即邗江、九江、吴江3个野生群体和2个选育世代间的亲缘关系较远, 石首群体和2个选育世代两两之间的亲缘关系较近。以上结果表明, 经过2个世代的选择育种, 选育群体的遗传结构已发生了变化, 并且随着选育的进行, 选育世代的遗传多样性下降的较为明显, 这警示着我们在今后的育种工作中应适当改变现有的选育方案, 并实时监测选育群体的遗传多样性, 以便为今后进一步的选育工作打下坚实的基础。 相似文献
15.
小口白甲鱼都柳江种群mtDNA D环的序列变异及遗传多样性 总被引:1,自引:0,他引:1
采用PCR结合DNA测序技术,测定分析了易危鱼类小口白甲鱼(Onychostoma lini)都柳江种群36个个体mtDNA D环约470bp序列的变异及遗传多样性。结果表明,在36个个体中,该序列的长度为469~475bp,其碱基组成为A+T的平均含量(68.4%)高于G+C(31.6%)。共检测到25个多态位点,其中转换19个、颠换6个。核苷酸多样性(π)为0.00575,平均核苷酸差异数(K)为2.695。36个个体分属5个单倍型,单倍型多样度(Hd)为0.260,单倍型间的平均遗传距离(P)为0.026。5个单倍型构建的UPGMA系统树聚为2个分支。目前小口白甲鱼都柳江种群mtDNA D环序列存在着较丰富的变异和遗传多样性。 相似文献
16.
为从分子水平上探究西藏牦牛类群的遗传多样性、亲缘关系,本研究测定了日多牦牛、类乌齐牦牛、丁青牦牛、错那牦牛、隆子牦牛、仲巴牦牛、聂荣牦牛、申札牦牛等8 个西藏牦牛类群共328 头牦牛mtDNAD-loop区序列,分析其多态性,构建系统进化树。结果表明:本次测定的西藏牦牛mtDNA D-loop 区序列长度为
887 - 895 bp,共检测到135 个变异位点,其中单态突变位点52 个,简约信息位点83 个。在328 个个体中共检测出91 种单倍型,平均单倍型多样性(Hd)、平均核苷酸多样性(π)分别为0. 884、0.010 27,显示西藏牦牛具有丰富的遗传多样性。8 个类群间平均遗传距离为0.011;日多牦牛与错那牦牛间遗传距离最小(0. 006);类乌
齐牦牛与隆子牦牛间遗传距离最大(0.015)。系统进化分析显示西藏牦牛可分为两大类,错那牦牛是较纯的牦牛类群,其它牦牛类群在进化过程中出现相互交流的情况。 相似文献
17.
基于非损伤性取样,利用mtDNA和微卫星DNA遗传标记,对来自青藏高原三江源国家级自然保护区、羌塘国家级自然保护区和甘肃党河南山地区等地的277 份疑似雪豹粪便样品进行了物种鉴定、个体识别和遗传多样性研究。结果显示:在190份成功扩增的mtDNA cyt b基因片段中,确定有89份属于雪豹;微卫星分析确定其属于48个不同的个体。在48个雪豹mtDNA cyt b基因片段中,共检测出13个多态性位点,定义了9个单倍型,单倍型多态性为0.776,核苷酸多态性为 1.50%, 9个单倍型的遗传距离为 0.009-0.058。研究表明在研究区域均存在雪豹分布,并具有一定的遗传多态性,地理距离分布较远的羌塘国家级自然保护区和甘肃党河南山地区的雪豹样品具有一定的遗传差异。 相似文献
18.
胡黄连为特产中国-喜马拉雅特有高山植物,作为常用中、藏药材,受到灭绝性采挖,作为濒危和二级保护植物亟待科学的保护。该研究以云南和西藏7个野生居群91个个体为材料,基于 cpDNA trnL-F 非编码序列测序分析胡黄连的遗传多样性和遗传结构,分析显著进化单元,确立优先保护居群并提出科学的保护策略。结果表明:胡黄连 trnL-F 序列长度为871~876 bp,根据序列的核苷酸变异共鉴定出5个单倍型,西藏占有2个单倍型,云南占有3个单倍型,西藏和云南2个地区的所有单倍型均不共享。胡黄连具有较低的单倍型多样性(Hd =0.43419)和核苷酸多样性(Dij =0.00466)。种群间分化度(Fst =0.864520)和基因流(Nm =0.04)、居群间的遗传分化水平(GST =0.916)、AMOVA 分析(0.78%的遗传变异发生在居群内,60.97%的遗传变异发生在地区内居群间,38.25%的遗传变异发生在地区间)均表明,胡黄连居群间存在明显遗传分化。多数一致性树将胡黄连划分为3个进化分支(Ⅰ、Ⅱ、Ⅲ),这3个分支均与地理相关,分支Ⅰ分布于横断山区的4个居群,分支Ⅱ是分布于东喜马拉雅的一个居群,分支Ⅲ是分布于喜马拉雅中段的2个居群。3个分支分属于3个“进化显著单元(ESU)”。这3个 ESU 中白马雪山、茨中、定日、波密、聂拉木五个居群都需要保护,建议现阶段应优先保护的居群是云南白马雪山和西藏波密居群,以就地保护为主。 相似文献
19.
本研究基于7个叶绿体DNA片段(cpDNA)和2个核DNA片段(ITS和PZ8)的测序数据,对龙血树柴胡(Bupleurum dracaenoides Huan C.Wang,Z.R.He&H.Sun)8个居群的153个样本进行了遗传多样性和分布式样研究。cpDNA片段分析结果显示:龙血树柴胡在物种水平具有较高的遗传多样性(Hd=0.862;Pi=0.00567),但居群内遗传多样性低,遗传变异主要存在于居群间,遗传分化显著(Fst=0.959);而核DNA片段ITS和PZ8的数据分析结果显示,其遗传多样性较低(Hd=0.532,Pi =0.00121和Hd=0.349,Pi=0.00060),遗传变异主要存在于居群内,居群间仅存在一定程度的遗传分化。中性检验和失配分布分析结果发现龙血树柴胡没有经历过近期种群扩张事件,8个居群的153个样本从遗传成份上可被分为两组。研究结果将为龙血树柴胡的资源保护和发掘提供参考。 相似文献
20.
Sixteen sequences of the hypervariable segment I (HVS-I, 16039-16398) in mtDNA control region from ancient Tuoba Xianbei remains excavated from Qilang Mountain Cemetery were analyzed. In which, 13 haplotypes were found by 25 polymorphic sites. The haplotype diversity and nucleotide diversity were 0.98 and 0.0189, respectively, and the mean of nucleotide number differences was 6.25. Haplogroup analysis indicates these remains mainly belong to haplogroup C (31.25%) and D (43.75%). According to the published data were considered, we can suggest that the Tuoba Xianbei presented a close genetic affinity to Oroqen, Outer Mongolian and Ewenki populations, especially Oroqen. 相似文献