DIFFERENTIATION OF MITOCHONDRIAL DNA POLYMORPHISMS IN POPULATIONS OF FIVE JAPANESE ABIES SPECIES

Mitochondrial DNA polymorphism of 40 populations of five Abies species was investigated using PCR-amplified coxI and coxIII gene probes. Using four combinations of probe and restriction enzyme, we detected three major haplotypes and 15 total haplotypes. We also found varied levels of gene diversity for the different species: 0.741, 0.604, 0.039, 0.000, and 0.292 for A. firma, A. homolepis, A. veitchii, A. mariesii, and A. sachalinensis, respectively. The marginal and southern populations of A. firma and A. homolepis have unique haplotypes, especially the Kyushu, Shikoku, and Kii Peninsula populations, which inhabit areas coinciding with probable refugia of the last glacial period and possess high levels of mtDNA genetic diversity. The haplotypes in some populations suggested mtDNA capture also occurred between species through introgression/hybridization. The strong mtDNA population differentiation in Abies is most likely due to the maternal inheritance of mitochondria and restricted seed dispersal. A phenetic tree based on the genetic similarity of the mtDNA suggests that some species are polyphyletic. Based on mtDNA variation, the five Abies species could be divided roughly into three groups: (1) A. firma and A. homolepis, (2) A. veitchii and A. sachalinensis, and (3) A. mariesii. However, we found that all these Abies species, except A. mariesii, are genetically very closely related according to an analysis of their cpDNA sequences. This showed that the chloroplast rbcL gene differed by only one base substitutions among the four species. We believe that the mtDNA variation and cpDNA similarity clearly reflect relationships among, and the dissemination processes affecting these Abies species since the last glacial period.     

MITOCHONDRIAL DNA AND MORPHOLOGICAL DIFFERENTIATION OF ALBINARIA POPULATIONS (GASTROPODA: CLAUSILIIDAE)

Albinaria, despite its restricted geographical distribution,exhibits an extreme degree of differentiation. The use of conventionalor numerical taxonomy has not facilitated the understandingof evolution of the genus. Twelve populations belonging to fourspecies were studied with a combined approach using mitochondrialDNA (mtDNA) and qualitative morphological data. The completemtDNA genome of A. coerulea from Amorgos island was cloned andused in mtDNA restriction site analysis of the other populations.Maximum parsimony cladistic analysis of nine populations providedtrees sharing the same basic topology. Certain restriction sitesand morphological characters appear to be species specific,while incongruity is observed at the intraspecific level. Sequencedivergence and the paleogeographic history of the area wereused for construction of an evolutionary scenario and a roughestimation of the Albinaria mtDNA clock. (Received 7 February 1994; accepted 20 July 1994)     

MITOCHONDRIAL BIOGENESIS DURING DIFFERENTIATION OF ARTEMIA SALINA CYSTS

Mitochondria isolated from cysts of Artemia salina (brine shrimp) were found to be devoid of cristae and to possess a low respiratory capability. Hydration of the cysts induces marked biochemical and morphological changes in the mitochondria. Their biogenesis proceeds in two stages. The first stage is completed within 1 h and is characterized by a rapid increase in the respiratory capability of the mitochondria, their cytochrome oxidase, cytochrome b, cytochrome c and perhaps some morphological changes. In the second stage there is an increase in the protein-synthesizing capacity of the mitochondria as well as striking changes in mitochondrial morphology leading to the formation of cristae.     

MITOCHONDRIAL DNA AND PROTEIN DIFFERENTIATION BETWEEN HYBRIDIZING CYTOTYPES OF THE WHITE-FOOTED MOUSE,PEROMYSCUS LEUCOPUS

Restriction-enzyme analysis of mitochondrial DNA and protein electrophoresis were used to document patterns of gene flow across a hybrid zone between chromosomal races of Peromyscus leucopus. Chromosomal markers (three inversions) are such that individuals can be classified as potential F₁'s, backcrosses, or parental types. Allozymic characterization of the hybrid zone is congruent with the chromosomal data (Stangl, 1986) and indicates an assymetrical distribution of markers, with the northeastern markers being distributed at a higher frequency into southwestern populations. Restriction patterns of mtDNA suggest that the two cytotypes may have had different evolutionary histories, and the distribution of haplotypes is concordant with other genetic markers used to identify the hybrid zone. Concordant changes in chromosomes, allozymes, and mtDNA suggest that the most viable hypothesis for the origin of the zone is secondary contact. A unique aspect of this study is that the same individuals were used for protein electrophoresis, mtDNA analysis, and chromosomal analysis. Thus, patterns of genetic variation can be interpreted free of any historical bias associated with samples collected at different times.     

GENETIC SUBDIVISIONS AMONG SMALL CANIDS: MITOCHONDRIAL DNA DIFFERENTIATION OF SWIFT,KIT, AND ARCTIC FOXES

Gene flow can effectively suppress genetic divergence among widely separated populations in highly mobile species. However, the same may not be true of species that typically disperse over shorter distances. Using mtDNA restriction-site and sequence analyses, we evaluate the extent of divergence among populations of two small relatively sedentary North American canids, the kit and swift foxes (genus Vulpes). We determine the significance of genetic differentiation among populations separated by distance and those separated by discrete topographic barriers. Our results show the among-population component of genetic variation in kit and swift foxes is large and similar to that of small rodents with limited dispersal ability. In addition, we found two distinct groupings of genotypes, separated by the Rocky Mountains, corresponding to the traditional division between kit and swift fox populations. Previous workers have characterized these morphologically similar populations either as separate species or subspecies. Our mtDNA data also suggest that kit and swift fox populations hybridize over a limited geographic area. However, the sequence divergence between kit and swift foxes is similar to that between these taxa and the arctic fox (Alopex lagopus), a morphologically distinct species commonly placed in a separate genus. This result presents a dilemma for species concepts, and we conclude that kit and swift foxes should be recognized as separate species.     

线粒体DNA和人类进化

线粒体ＤＮＡ（ｍｔＤＮＡ）由于自身比较独特的遗传特性（母系遗传、缺乏重组和进化速率高）而被广泛地应用于人类群体的起源和演化研究。通过对其全序列的限制性酶切和Ｄ－环高变区序列数据的分析,ｍｔＤＮＡ较好地阐明了人类学中诸如现代人类起源、人群过去动态的估计以及单个人群的区域性微分化和人口历史学等问题。综述了近年来世界各人群ｍｔＤＮＡ的研究进展、研究方法的改进、ｍｔＤＮＡ与核基因标记结果的异同、ｍｔＤＮＡ     

THE EFFECT OF ETHIDIUM BROMIDE ON MITOCHONDRIAL DNA SYNTHESIS AND MITOCHONDRIAL DNA STRUCTURE IN HELA CELLS

The synthesis of mitochondrial DNA (mDNA) in HeLa cells is selectively inhibited by relatively low concentrations of ethidium bromide. After exposure of cells to strongly inhibitory concentrations of the drug, the apparent superhelix density of mDNA is rapidly increased, as judged by its buoyant density in CsCl in the presence of ethidium bromide. Mitochondrial DNA synthesized in the presence of partially inhibitory concentrations of ethidium bromide is also altered in its buoyant density in the presence of the dye, but is more heterogeneous in this respect. However, the change in buoyant density of newly synthesized mDNA may be explained by changes in structure other than a change in superhelix density, as indicated by its increased resistance to digestion by pancreatic DNase.     

贵州四个山羊品种mtDNA多态性及起源分化

采用１５种限制性内切酶,研究贵州省４个山羊品种共９３只个体的线粒体ＤＮＡ多态性。其中ＢｏｍＨＩ、ＨｉｎｄⅢ和ＳａｌⅠ３种酶的酶切类型存在多态。共检测到１８种限制性态型,归结为３种ｍｔＤＮＡ单倍型。单倍型Ⅰ、Ⅱ在贵州山羊４个品种分布频率较高,分别为７７．４２％和２１．５０％,单倍型Ⅲ分布频率较低（１．０８％）;品种间亲缘关系聚类分析表明白山羊和黑山羊亲缘关系最近,其次为黔林羊,而与小香羊的亲缘关系最     

线粒体DNA聚合酶的起源与演化

随着新的DNA聚合酶A家族成员的加入,家族内部的系统发育关系需要重新检查,来自大肠杆菌DNA聚合酶I(DNA Pol I)和它的细菌、噬菌体和真核细胞同源物被用来重建这个家族的系统发育史.分析显示:在真核生物演化的不同阶段,线粒体DNA聚合酶基因可能通过水平基因转移方式起源于不同类群的生物.原始真核生物线粒体DNA聚合酶基因可能来源于细菌,植物线粒体DNA聚合酶基因可能从质粒获得,而真菌和动物线粒体DNA聚合酶基因可能起源于T3/T7相关噬菌体.     

MITOCHONDRIAL DNA REPLICATION IN SEA URCHIN OOCYTES

Mitochondrial DNA (mtDNA) replicative intermediates from Strongylocentrotus purpuratus oocytes were isolated by ethidium bromide-CsCl density gradient centrifugation and examined by electron microscopy after formamide spreading. In some experiments, the mtDNA was radioactively labeled by exposing isolated oocytes to [³H]thymidine. Oocyte mtDNA replication appears to follow the displacement loop model outlined in mouse L cells. There are differences in detail. The frequency of D-loop DNA is much lower in oocytes, suggesting that the relative holding time at the D-loop stage is shorter. Duplex synthesis on the displaced strand occurs early and with multiple initiations. The frequency of totally duplex replicative forms, or Cairns' forms, is the highest reported for mtDNA. The differences may be related to the fact that oocyte mtDNA replication occurs in the absence of cell division and need not be coordinated with a cell cycle. Molecules with expanded D loops banded in the intermediate region between the lower and upper bands in an ethidium bromide-CsCl gradient, supporting the notion that displacement replication proceeds on a closed circular template which is subject to nicking-closing cycles. In mature sea urchin eggs, replicative forms are absent and virtually all the mtDNA is stored as clean circular duplexes. Some novel structural variants of superhelical circular DNA (molecules with denaturation loops and double branch-migrated replicative forms) are reported.     

EVOLUTION AND MITOCHONDRIAL DNA IN NEUROSPORA CRASSA

We studied mitochondrial DNA variability in 19 natural Neurospora crassa isolates and one wild-type isolate to examine evolution of these fungi and their mitochondrial DNA (mtDNA). We combined restriction endonuclease analysis of natural isolate mtDNA with DNA-DNA hybridization to cloned EcoR I fragments of a wild-type genome to discriminate between length mutations and site changes due to nucleotide substitution. Most variability was due to length mutations (insertions and deletions); genome size could vary 25% between pairs of isolates. Length-mutation distribution was not random, nor simply explained by the presence of coding versus noncoding regions. Restriction-site changes were few; the estimated amount of nucleotide substitution per nucleotide between the most divergent pair of isolates was 0.78%. Evolutionary relationships among isolates based on both types of mutations were compatible, and suggest that geographically distinct populations of mitochondrial DNA exist in the biological species, N. crassa. In contrast, no such correlation was shown by the previously determined distribution of nuclear heterokaryon incompatibility genes in the same isolates (Mylyk, 1975, 1976).     

MITOCHONDRIAL DNA PHYLOGENIES FOR THE DROSOPHILA OBSCURA GROUP

Species belonging to the obscura group of the genus Drosophila have long held a central position in evolutionary studies, especially in experimental population genetics. Despite the considerable amount of accumulated knowledge, many of the phylogenetic relationships of the species in the group remain unclear. Here we present DNA sequence data for the mitochondrial gene cytochrome oxidase I (COI) for 13 species native to both the Old and New Worlds. We combine these data with seven other mitochondrial gene sequences from previous studies, for a total of over 3 kb per species. Strongly supported conclusions include: (1) the two North American subgroups, pseudoobscura and affinis, are each monophyletic; and (2) among Eurasian species two unambiguous clades are identified, one containing D. tristis, D. ambigua, and D. obscura and the other containing D. guanche, D. subobscura, and D. madeirensis. Constructing firm hypotheses connecting these four major clades is problematic with all datasets. Major ambiguities are the number of invasions giving rise to the North American obscura species and the relationships among the Eurasian species. The inadequacy of the mtDNA data to resolve these ambiguities does not reside in lack of changes; the transversions-only parsimony tree has 283 informative characters. Rather, the problems are likely intrinsic to the history of the group: while radiating in temperate Eurasia, North America was colonized once or twice, followed by one or two radiations in the New World.     

鱼类线粒体DNA的遗传与进化

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褐家鼠线粒体DNA遗传多态性的研究

通过碱变性法提取线粒体ＤＮＡ,用地高辛标记的探针Ｓｏｕｔｈｅｒｎ杂交限制性酶切多态性（ＲＦＬＰ）分析,研究中国家鼠Ｒａｔｔｕｓｎｏｒｖｅｇｉｃｕｓ遗传多态性。采用ＡｐａⅠ、ＡｖａⅠ、ＢａｎＨＩ、ＢｃｌⅠ、ＢｇｌⅠ、ＣｌａⅠ、ＥｃｏＲⅠ、ＥｃｏＲⅤ、ｈｉｎｄⅢ、ＰｖａⅡ、ＳｃａⅠ和ＸｂａⅠ等１２种限制性内切酶分析来自我国８个地区２６只褐家鼠的线粒体ＤＮＡ,共检出２０种限制性态型和１１种ｍｔＤＮＡ单倍     

两种邻域分布石鸡间的线粒体DNA渗透

采用聚合酶链式反应(PCR)和mtDNA细胞色素b基因314 bp核苷酸序列测定等方法,证明在大石鸡与山石鸡的异域种群之间存在广泛的差异.然而采自六盘山地区与山石鸡相邻分布的大石鸡种群的样本中却存在山石鸡的mtDNA基因型,这种基因型与其它大石鸡个体的基因型有4.4%核苷酸差异.在与山石鸡相邻分布的大石鸡种群中有25%的个体具有山石鸡的mtDNA基因型,而采自六盘山接触地带以西约200 km处兰州市郊的大石鸡标本中则没有发现这种基因型.此发现支持山石鸡和大石鸡之间存在或曾经有过杂交的假设.作者还提出了一种限制性内切酶分析方法,可以快速地检测这种mtDNA基因型.在此之前还没有过关于山石鸡和大石鸡之间基因流动的报道.     

鸮形目8种鸟类线粒体DNA多态性研究

采用14种限制性内切酶,对鸮形目8种鸟类(Tyto alba、T.capensis、Otus bakkamoena、O.scops、Asio otus、A.flammeus、Strix aluco、Glaucidium cuculoides)线粒体DNA进行限制性片段长度多态分析, 结果表明:不同种间存在基因组长度多态性,短耳鸮为23.35 kb,长耳鸮为19.78 kb,斑头鸺鹠为18.62 kb,红角鸮为17.65 kb.鸮形目种间具有较高的遗传变异,其中仓鸮和草鸮的平均遗传距离为1.0%,长耳鸮和短耳鸮平均为10.8%,红角鸮和领角鸮平均为13.1%,灰林鸮和斑头鸺鹠为12.3%,其中红角鸮与斑头鸺鹠的平均遗传距离最大为17.5%.鸮形目鸟类线粒体DNA的进化速率为每百万年变化2.0%～2.2%,提示鸮形目两个科间在距今2 800～3 000万年前分歧开来,同时,鸱鸮科各种间的分歧时间在距今2 000～2 500万年前,即处于中新世中期.     

四种犬科（Canidae）动物线粒体DNA分子进化

以９种限制性内切酶分析家犬,狼,赤狐,貉共７只动物的一粒体ＤＮＡ限制性片段长度多态性（ｍｔＤＮＡＲＦＬＰ）,通过双酶解法构建各种动物的限制性内切酶图谱,用ＵＰＧ法,ＮＪ法和简略法分析这些动物之间的遗传关系。结果表明,１．犬的个体差异小,而赤弧的个体间遗传分化程度非常高;２．犬和狼的亲缘关系很近,应是同一种动物;３．在属间关系中,犬属与狐属的关系较接近,貉属是一个较早分化的独立分支。     

EXPERIMENTAL EVIDENCE FOR MITOCHONDRIAL DNA INTROGRESSION BETWEEN DROSOPHILA SPECIES

Differential introgression of mitochondrial genomes has been used to explain the occurrence in some species of individuals bearing mtDNA from a related species. This situation has been observed for Drosophila mauritiana (endemic to Mauritius) where a high proportion of individuals (88%) carries an mtDNA also found in D. simulans populations from Madagascar and Réunion. Using these two species, experiments were carried out to test for differential mtDNA introgression. A single virgin female from one species (initial frequency 0.03) was introduced into a population of the other. D. simulans mtDNA can, within three generations, almost entirely displace (frequency up to 0.80) D. mauritiana mtDNA. Hybrid male sterility probably curtails to a large degree parallel introgression of nuclear genes. The progress of cytoplasmic introgression is dependent on the degree of inbreeding of the recipient D. mauritiana strains. In reciprocal experiments, introgression was much less likely: few D. mauritiana migrant females are inseminated and their mtDNA frequency always remains very low. The results of these experiments support the hypothesis that a selective advantage of hybrids (probably at the nuclear level) has promoted mtDNA transfer from D. simulans Madagascar or Reunion populations into D. mauritiana through introgressive hybridization.     

NUCLEAR GENE DOSAGE EFFECTS ON MITOCHONDRIAL MASS AND DNA

In order to assess the effect of nuclear gene dosage on the regulation of mitochondria we have studied serial sections of a set of isogenic haploid and diploid cells of Saccharomyces cerevisiae, growing exponentially in the absence of catabolite repression, and determined the amount of mitochondrial DNA per cell. Mitochondria accounted for 14% of the cytoplasmic and 12% of the total cellular volume in all cells examined regardless of their ploidy or their apparent stage in the cell cycle. The mean number of mitochondria per cell was 22 in the diploid and 10 in the haploids. The volume distribution appeared unimodal and identical in haploids and diploids. The mitochondrial DNA accounted for 12.6 ± 1.2% and 13.5 ± 1.3% of the total cellular DNA in the diploid and haploid populations, respectively. These values correspond to 3.6 x 10^-15 g, 2.2 x 10⁹ daltons, or 44 genomes (50 x 10⁶ daltons each) per haploid and twice that per diploid cell. On this basis, the average mitochondrion in these cells contains four mitochondrial genomes in both the haploid and the diploid.