GENOME SIZE

采用Feulgen-显微分光光度计方法,以鸡红细胞为标准DNA（3.22pg/2C）测定了长江白鲟、达氏鲟、中华鲟、史氏鲟和北美匙吻鲟的体细胞基因组大小（DNA含量）。结果表明,上述五种鲟鱼DNA含量分别为4.11、8.26、9.07、6.07和3.96pg。长江白鲟和北美匙吻鲟均属于四倍体鱼类,分布在长江水系的中华鲟和达氏鲟两种鲟属鱼类为八倍体类型。史氏鲟初步判断为八倍体,据分析可能存在四倍体的类型。根据所得到的结果并结合已发表的DNA含量和染色体资料,分析了鲟形目鱼类在细胞遗传上的进化特点。鲟形目鱼类全为多倍体起源的鱼类,在鲟形目的两科（白鲟科和鲟科）六个属中,除鲟属外,其他五个属均为四倍体,而鲟属已发现有四倍体、八倍体、十二倍体和十六倍体。说明在细胞水平的染色体加倍与鲟形目鱼类各科、属分化没有直接联系,只在鲟形目形成的早期和鲟形目形成后的鲟属种间分化中扮演着重要角色。鲟属鱼类的染色体剧烈分化可能是造成现今鲟属种类数最多（占整个鲟形目鱼类的65%以上）的重要原因。     

高加索蜂Apis mellifera caucasica Gorb的染色体核型分析

采用常规压片法对高加索蜂单倍体雄蜂的染色体进行分析.实验结果表明高加索蜂单倍体雄蜂染色体数为n=16.根据Levan等提出的染色体划分标准得出高加索蜂:中部着丝粒染色体(m)为12条,亚中部着丝粒染色体(sm)为4条,无端部着丝粒染色体(t)和亚端部着丝粒染色体(st).染色体总臂数(NF)为32,高加索蜂雄蜂的核型公式为n=x=16=12 m+4 sm,属“1A”核型.     

宽体沙鳅的染色体核型与DNA含量分析

为了解宽体沙鳅(Sinibotia reevesae)的种质特征,以野生宽体沙鳅为材料,采用腹腔注射植物血球凝集素(PHA)和秋水仙素,肾组织细胞短期培养、常规空气干燥法制备染色体标本,并对其核型进行分析。以鸡(Gallus gallus)血细胞DNA含量(2.50 pg/2c,2c指二倍体)为标准,用流式细胞仪测定宽体沙鳅外周血细胞的DNA含量。结果表明:(1)宽体沙鳅的染色体数目为2n=96,核型组成公式为2n=36m+14sm+20st+26t,染色体总臂数NF=146;未发现与性别相关的异型染色体。(2)宽体沙鳅的DNA含量为(2.60±0.36)pg/2c。通过与其他26种鳅科鱼类核型进行比较,发现宽体沙鳅属于鳅科鱼类中的特化类群,其染色体核型经历了罗伯逊易位和染色体多倍化等过程。本研究结果可为宽体沙鳅种质资源保护和细胞遗传学研究提供基础资料。     

中国五台山多目涡虫(涡虫纲,三肠目)染色体及核型分析

利用空气干燥法对采自山西茶铺和镇海寺的五台山多目涡虫Polycelis wutaishanica Liu,1996的核型进行分析,结果表明:五台山多目涡虫体细胞有42条染色体,为2倍体,核型公式2n=2x=42 =28m 14sm,其中28条为中部着丝粒染色体, 14条为亚中部着丝粒染色体,第1对中部着丝粒染色体明显比其它染色体长。五台山多目涡虫的核型属于2C型。     

彭泽鲫染色体数目及倍性的细胞遗传学分析

对彭泽鲫(Carassius auratus variety pengze)肾细胞染色体的数目统计分析表明，彭泽鲫染色体组是由150条基本染色体和若干条小的超数染色体组成。染色体组型按着丝粒位置150条基本染色体可分为四组，每组中同源染色体的组数与已知二倍体鲫鱼的同源染色体组数一致。每个染色体小组均由三条同源染色体组成。在亚端部着丝粒染色体组(st)的第三号染色体组的三条同源染色体的短臂上均有非常明显的随体，可作为彭泽鲫是三倍体的细胞遗传学证据。彭泽鲫肾细胞的DNA相对含量是二倍体红鲫肾细胞DNA相对含量的1．55倍，与染色体实验结果一致。这些研究结果表明，彭泽鲫是一种三倍体鲫鱼，其染色体数目为3n＝150 ，核型公式为3n＝33m 51sm 33st 33t。     

施氏鲟的核型及DNA含量研究

采用体内注射小牛血清、肾组织细胞短期培养、常见空气干燥法制备了施氏鲟(Acipenser schrencki Brandt)的染色体,并进行了核型分析。施氏鲟二倍体的染色体为238±8条,其核型为78m+12sm+28st,t+120±mc,NF :328±。以外周血红细胞为样本,鸡的红细胞为对照,用美国产的FACStar Plus流式细胞仪测定了施氏鲟二倍体细胞核的DNA含量, 其DNA含量为鸡的5.06倍,绝对含量为11.73±0.68pg/N。 Abstract:Metaphase chromosome specimens of Amur Sturgeon,injected with fetalcalf serum,were prepared from short-term culture of kidney cells with air-drying technique.Its diploid chromosome number is 2n=238±8.Karyotype consists of 78m+12sm+28st,t+120±mc,NF:328±.Diploid nucleus DNA content was measured from the peripheral erythrocytes,using flow cytometer(FACStar Pus,made in USA)and erythrocytes of chick(Gallus sp)as internal standard.DNA content of the fish is 11.73±0.68pg/N and the ratio to that of chickens is 5.06.     

泉水鱼的细胞遗传学分析

以泉水鱼(Pseudogyrinocheilus prochilus)的肾为材料,采用体内注射植物血球凝集素(PHA)和秋水仙素、肾组织细胞短期培养、常规空气干燥法制备泉水鱼染色体标本,对其核型进行分析。以泉水鱼外周血细胞为样本,鸡(Gallus gallus)血细胞DNA含量(2.50 pg/2c,2c指二倍体)为标准,用流式细胞仪测定了泉水鱼的DNA含量。结果表明:(1)泉水鱼的染色体数量为2n=50,核型公式为12m+14sm+14st+10t,总臂数NF=76,未发现性别相关的异型染色体;(2)泉水鱼的DNA含量为鸡血对照的(1.05±0.04)倍,其绝对DNA含量为(2.62±0.10)pg/2c。泉水鱼的染色体数目和DNA含量显示出二倍体的特征。     

中国淡水三角涡虫(Dugesia sp)的染色体研究(Ⅰ)

利用空气干燥法对不同产地淡水三角涡虫的染色体进行了研究。核型分析表明：河南淇县鱼泉三角涡虫(Dugesia sp)和浙江杭州龙井三角涡虫(Dugesia sp)体细胞中有16条染色体,为二倍体,核型公式为2n=2x=16=16m,均为具中部着丝粒染色体;河南济源不老泉三角涡虫(Dugesia sp)有24条染色体,为三倍体,核型公式为2n=3x=24=24m,亦全部由中部着丝粒染色体组成。上述3个产地淡水三角涡虫染色体的形态较为接近。北京樱桃沟三角涡虫(Dugesia sp)的体细胞染色体数目为24,为三倍体,核型公式为2n=3x=24=22m 2sm,由中部和亚中部着丝粒染色体组成,其中第2、4号各有一条染色体属于亚中部着丝粒染色体。研究结果表明：4个产地三角涡虫的体细胞染色体数目存在较大差异,包括二倍体(2n=2x=16)和三倍体(2n=3x=24),染色体基数属于x=8类型。     

黄藤染色体核型及基因组大小分析

为探究黄藤(Daemonoropsjenkinsiana)染色体核型和基因组的大小,采用体细胞染色体常规制片法与显微摄影技术相结合的方法,对黄藤染色体进行了核型分析,同时以番茄(Lycopersicon esculentum)为内标,应用流式细胞术对黄藤叶片基因组大小、DNA含量和DNA倍性进行了测定。结果表明,黄藤茎尖是理想的染色体制片材料;黄藤的染色体数为2n=24,核型公式为K(2n)=1M+17m+5sm+1st,核型类型为2C;核型不对称系数61.20%;黄藤的DNA含量为1.57 pg,基因组大小为1 539.53 Mb,黄藤的DNA倍性为二倍体(2n)。这是首次报道黄藤的核型和基因组大小,为深入开展黄藤属及其近缘属植物的核型和基因组比较分析提供了参考依据。     

硬枝黄蝉染色体计数与核型分析

以硬枝黄蝉Allamanda neriifolia幼胚为试验材料,对其体细胞染色体进行计数与核型分析。结果表明,硬枝黄蝉幼胚细胞含9对染色体,由中部或近中部着丝粒染色体构成。核型公式为2n=2x=6sm+12m。核型不对称系数为58.95%,核型分类属于2A型。     

几种鲟鱼基因组大小、倍体的特性及鲟形目细胞进化的探讨

采用Ｆｅｕｌｇｅｎ－显微分光光度计方法,以鸡红细胞为标准ＤＮＡ（３．２２ｐｇ／２Ｃ）测定了长江白鲟、达氏鲟、中华鲟、史氏鲟和北美匙吻鲟的体细胞基因组大小（ＤＮＡ含量）。结果表明,上述五种鲟鱼ＤＮＡ含量分别为４．１１、８．２６、９．０７、６．０７和３．９６ｐｇ。长江白鲟和北美匙吻鲟均属于四倍体鱼类,分布在长江水系的中华鲟和达氏鲟两种鲟属鱼类为八倍体类型。史氏鲟初步判断为八倍体,据分析可能存在四倍体的     

广藿香毛状根多倍体诱导及其植株再生

为了提高药用植物广藿香的次生物质广藿香醇含量,采用秋水仙素人工诱导染色体加倍技术,进行了广藿香毛状根多倍体诱导及其植株再生、倍性鉴定和挥发油组分广藿香醇含量的测定。结果表明,广藿香毛状根多倍体诱导的最佳条件为0.05%秋水仙素处理36 h,其多倍体诱导率可达40%以上;经秋水仙素加倍的广藿香毛状根在MS+6-BA 0.2 mg/L+NAA 0.1 mg/L培养基中培养60 d后可获得毛状根多倍体再生植株。与对照(二倍体植株)相比,广藿香毛状根多倍体再生植株根系更发达、茎更粗、节间变短、叶片的长度、宽度和厚度均较二倍体明显增大。根尖细胞染色体压片观察证实,所获得的广藿香毛状根多倍体再生植株为四倍体,其根尖细胞染色体数约为128;同时,其叶片的气孔保卫细胞体积及其叶绿体数目均约为对照的两倍;但其气孔密度则随着倍性增加而下降,二倍体植株叶片的气孔密度约为四倍体植株叶片的1.67倍。GC-MS测定结果表明,广藿香毛状根多倍体再生植株的广藿香挥发油组分广藿香醇的含量为4.25 mg/g干重,约为二倍体植株的2.30倍。该结果证实毛状根多倍体化可提高药用植物广藿香的广藿香醇含量。     

Quantitative DNA variation between and within chromosome complements of Vigna species (Fabaceae)

Cytogenetical investigations, so far, on the organisation and evolution of the genomes of Vigna species have proved difficult due to small chromosome size, large chromosome number and uniformity in chromosome shape and size within and between the complements. In this investigation the nature and extent of DNA variation between thirteen diploid and one polyploid species have been estimated. The DNA variation between diploid species was small and species clustered around a mean value of 2.7 pg. The polyploid species had a greater DNA value of 4.95 pg. No significant variation in 2C DNA content was found between accessions of V. radiata. A comparison of the distribution of DNA among the chromosomes within complements has shown that the excess DNA acquired in evolution was distributed evenly in all chromosomes despite significant differences in chromosome size. The relative changes in chromatin area and DNA density which accompany evolutionary DNA variation was also compared.     

Chromosome numbers, nuclear DNA content, and polyploidy in Consolea (Cactaceae), an endemic cactus of the Caribbean Islands

Polyploidy, an important mechanism of plant evolution, was investigated in Consolea, an endemic Caribbean opuntioid genus represented by nine subdioecious species with very narrow distributions, including species classified as rare or threatened. Standard chromosome counting and flow cytometric analyses were used to determine chromosome numbers and ploidy of each taxon. Compared to the base number (x = 11), the mitotic and meiotic counts indicated that there are seven hexaploid (2n = 66) and two octoploid species (2n = 88); no diploids were found. Histograms of intact nuclei confirmed that all species are polyploid, with C-DNA values ranging from 4.88-9.50 pg. The variation of DNA content was significantly higher for the octoploids than for the hexaploids. Male and female sexual morphs had similar DNA content, suggesting that there are no sex chromosomes. Cytomixis between cells and microsporocytes with no chromatin were observed. This provides a mechanism whereby gametes with variable chromosome numbers are produced, influencing reproduction and promoting speciation. In conclusion, C-DNA content and chromosome number separated Consolea species into two groups, which may correspond to two phylogenetic lineages or indicate that polyploidization occurred independently, with comparable effects on C-DNA content.     

Genome evolution in the genus Sorghum (Poaceae)

BACKGROUND AND AIMS: The roles of variation in DNA content in plant evolution and adaptation remain a major biological enigma. Chromosome number and 2C DNA content were determined for 21 of the 25 species of the genus Sorghum and analysed from a phylogenetic perspective. METHODS: DNA content was determined by flow cytometry. A Sorghum phylogeny was constructed based on combined nuclear ITS and chloroplast ndhF DNA sequences. KEY RESULTS: Chromosome counts (2n = 10, 20, 30, 40) were, with few exceptions, concordant with published numbers. New chromosome numbers were obtained for S. amplum (2n = 30) and S. leiocladum (2n = 10). 2C DNA content varies 8.1-fold (1.27-10.30 pg) among the 21 Sorghum species. 2C DNA content varies 3.6-fold from 1.27 pg to 4.60 pg among the 2n = 10 species and 5.8-fold (1.52-8.79 pg) among the 2n = 20 species. The x = 5 genome size varies over an 8.8-fold range from 0.26 pg to 2.30 pg. The mean 2C DNA content of perennial species (6.20 pg) is significantly greater than the mean (2.92 pg) of the annuals. Among the 21 species studied, the mean x = 5 genome size of annuals (1.15 pg) and of perennials (1.29 pg) is not significantly different. Statistical analysis of Australian species showed: (a) mean 2C DNA content of annual (2.89 pg) and perennial (7.73 pg) species is significantly different; (b) mean x = 5 genome size of perennials (1.66 pg) is significantly greater than that of the annuals (1.09 pg); (c) the mean maximum latitude at which perennial species grow (-25.4 degrees) is significantly greater than the mean maximum latitude (-17.6) at which annual species grow. CONCLUSIONS: The DNA sequence phylogeny splits Sorghum into two lineages, one comprising the 2n = 10 species with large genomes and their polyploid relatives, and the other with the 2n = 20, 40 species with relatively small genomes. An apparent phylogenetic reduction in genome size has occurred in the 2n = 10 lineage. Genome size evolution in the genus Sorghum apparently did not involve a 'one way ticket to genomic obesity' as has been proposed for the grasses.     

Nuclear DNA content and chromosome numbers in the myxomycete Physarum polycephalum

An improved method is described for making chromosome spreads of the plasmodium of the myxomycete, Physarum polycephalum. It consists of isolating metaphase nuclei, spreading the chromosomes with hot lactic acid, and staining with acetic-orcein.Most sublines derived from the Backus Wis 1 sclerotium had about 1 pg of DNA per nucleus, and had nuclei with 50 and 75 chromosomes in both the growing and sporulating plasmodium. Mature spores contained 0.6 pg of DNA, and hatching amoebae had 20–25 chromosomes and 0.6 pg of DNA. Plasmodia of the homothallic Colonia strain had a nuclear DNA content of about 1 pg, and had 35–40 chromosomes during growth and sporulation. Polyploid plasmodial sublines were found which had 1.5 and 3 times the normal DNA content and chromosome number. The polyploid sublines had the same plasmodial protein:DNA and RNA:DNA ratios as normal cultures. DNA content of nuclei varied directly with nuclear surface area. Ploidy was determined by the parent amoebae and therefore can serve as a genetic marker.A simple technique is given for completing the life cycle of P. polycephalum axenically. Germinating spores are plated without bacteria on one-tenth strength semidefined plasmodial growth medium, containing 2% agar. Plasmodia are visible in 2–4 days.     

Isolation of tetraploid clones with high efficiency from diploid 3Y1 rat fibroblasts treated with sodium butyrate

Summary Sodium butyrate causes proliferation arrest with a G2 (4C) DNA content and induces formation of tetraploid cells upon removal of the inhibitor, in rat 3Y1 diploid fibroblasts. We isolated tetraploid clones from the butyrate-treated 3Y1 cells with high efficiency; among 21 clones randomly isolated, 5 were pure diploid, 7 were mainly tetraploid with a small contaminating diploid population, and 7 were pure tetraploid. Among the pure tetraploid clones, two showed doubled chromosome numbers with slightly broader distributions than that seen in parental 3Y1 cells. Butyrate further induced polyploid formation in the tetraploid cells thus produced, but octaploid cells that resulted could not be maintained for prolongeed, cultivation. We found no difference between the tetraploid and the (parental and parallel isolated) diploid clones in terms of colony-forming ability, proliferation rate, and sensitivity to density-dependent inhibition of proliferation. These results suggest that doubling of chromosome number by itself does not cause a change in proliferation property. The tetraploid clones had lower average saturation densities possibly due to enlargement of cell size represented by higher cellular protein content.     

Nuclear DNA content and chromosome number in some diploid and tetraploid Centaurea (Asteraceae: Cardueae) from the Dalmatia region

Given the paucity of information about genome size in the genus Centaurea, nuclear DNA content of 15 Centaurea taxa, belonging to four subgenera and six different sections, has been investigated for the first time. The sample concerns 21 populations from the Dalmatia region of Croatia. The 2C DNA content and GC percentage were assessed by flow cytometry and chromosome number was determined using standard methods. Genome size of studied Centaurea ranged from 2C=1.67 to 3.72 pg. These results were in accordance with chromosome number and especially with ploidy level that varies throughout this group; 2C DNA values ranged from 1.67 to 3.43 pg for diploid, and from 3.19 to 3.72 for polyploid taxa. No significant intraspecific variations of DNA amount were found between two subspecies of C. visiani and C. ragusina, nor between two varieties of C. gloriosa. However, some populations of C. glaberrima and C. cuspidata showed a significant difference in DNA amount. Three different basic chromosome numbers were observed in studied species (x=9, 10, and 11). The most frequent basic number was x=9. C. rupestris, C. ragusina ssp. ragusina, and C. r. ssp. lungensis possessed x=10 and C. tuberosa x=11. The species with a basic chromosome number of x=9 had a small genome size and the smallest chromosomes (on average 0.09 to 0.12 pg/chromosome) but frequently present polyploidy. Centaurea ragusina ssp. ragusina and C. r. ssp. lungensis had a mean base composition 41.3% GC.     

Chromosomal DNA content of sweet pepper determined by association of cytogenetic and cytometric tools

The nuclear DNA content of sweet pepper (Capsicum annuum L. var. annuum, 2n = 24) has been measured by flow and image cytometries but the DNA content of each chromosome of this species has not yet been regarded. DNA content of individual chromosomes has been quantified by the flow karyotyping technique, which requires a great quantity of intact metaphasic chromosomes and methods that allow the characterization of individual chromosomes; however, the obtainment of adequate number of metaphases can be difficult in some species like C. annuum. In order to estimate the DNA content of each C. annuum var. annuum cv. "New Mexican" chromosome, flow and image cytometries were associated with the cytogenetic methodology. First, the DNA amount (2C = 6.90 pg) was established by flow cytometry. Integrated optical density (IOD) values were calculated by image cytometry for each Feulgen stained metaphasic chromosome. Then, by distributing the correspondent metaphasic value (4C = 13.80 pg) proportionally to average IOD values, the following chromosomal DNA contents were obtained in pg: 0.74 (chromosome 1), 0.67 (2), 0.61 (3, 4), 0.60 (5), 0.59 (6, 7), 0.58 (8), 0.57 (9), 0.56 (10) and 0.39 (11, 12). This study reports an alternative and reproducible technique that makes quantifying the chromosomal DNA content possible.     

The expression of antibody diversity in natural and laboratory-made polyploid individuals of the clawed toad Xenopus

Antibody diversity, as measured by isoelectric focusing of dinitrophenol-specific antibodies, was compared in different polyploid species of the clawed toad Xenopus. Antibody heterogeneity increased with chromosome number and DNA content from Xenopus tropicalis (2n=20 chromosomes) to Xenopus ruwenzoriensis (2n=108 chromosomes). Laboratory allopolyploids made by hybridization between two species showing different antibody diversities and different chromosome numbers gave antibody patterns intermediate between the two parents. On the other hand, autopolyploid individuals showed no increase in antibody diversity, showing that increased polyploidy alone cannot be responsible for increased heterogeneity. In contrast to the increase in antibody diversity following polyploidization, the number of expressed major histocompatibility complex alleles, as measured by a mixed lymphocyte reaction, did not increase. This locus appeared to be diploid or in the process of rediploidization in all the Xenopus species studied. Selection has thus operated differentially on the polyploid immunoglobulin and major histocompatibility loci. It apparently preserved the additional heterogeneity acquired for immunoglobulins favoring the expression of an expanded antibody repertoire in polyploid species.