A simple chromosomal marker can reliably distinguishes <Emphasis Type="Italic">Poncirus</Emphasis> from <Emphasis Type="Italic">Citrus</Emphasis> species

Several chromosome types have been recognized in Citrus and related genera by chromomycin A₃ (CMA) banding patterns and fluorescent in situ hybridization (FISH). They can be used to characterize cultivars and species or as markers in hybridization and backcrossing experiments. In the present work, characterization of six cultivars of P. trifoliata (“Barnes”, “Fawcett”, “Flying Dragon”, “Pomeroy”, “Rubidoux”, “USDA”) and one P. trifoliata × C. limonia hybrid was performed by sequential analyses of CMA banding and FISH using 5S and 45S rDNA as probes. All six cultivars showed a similar CMA⁺ banding pattern with the karyotype formula 4B + 8D + 6F. The capital letters indicate chromosomal types: B, a chromosome with one telomeric and one proximal band; D, with only one telomeric band; F, without bands. In situ hybridization labeling was also similar among cultivars. Three chromosome pairs displayed a closely linked set of 5S and 45S rDNA sites, two of them co-located with the proximal band of the B type chromosomes (B/5S-45S) and the third one co-located with the terminal band of a D pair (D/5S-45S). The B/5S-45S chromosome has never been found in any citrus accessions investigated so far. Therefore, this B chromosome can be used as a marker to recognize the intergeneric Poncirus × Citrus hybrids. The intergeneric hybrid analyzed here displayed the karyotype formula 4B + 8D + 6F, with two chromosome types B/5S-45S and two D/5S-45S. The karyotype formula and the presence of two B/5S-45S chromosomes clearly indicate that the plant investigated is a symmetric hybrid. It also demonstrates the suitability of karyotype analyses to differentiate zygotic embryos or somatic cell fusions involving trifoliate orange germplasm. During the submission of this paper, we analyzed 25 other citrus cultivars with the same methodology and we found that the chromosome marker reported here can indeed distinguish Poncirus trifoliata from grapefruits, pummelos, and one variegated access of Citrus, besides the previously reported access of limes, limons, citrons, and sweet-oranges. However, among 14 mandarin cultivars, two of them displayed a single B/5S-45S chromosome, whereas in Citrus hystrix D.C., a far related species belonging to the Papeda subgenus, this chromosome type was found in homozygosis. Since these two mandarin cultivars are probably of hybrid origin, we assume that for almost all commercial cultivars and species of the subgenus Citrus this B type chromosome is a useful genetic marker.     

黄芩的花粉母细胞减数分裂及核型分析

采用压片法,对黄芩花粉母细胞减数分裂及核型进行了研究。结果表明:黄芩的大多数花粉母细胞减数分裂中染色体的行为正常,在终变期同源染色体配对后可形成9个二价体,后期Ⅰ染色体以9∶9的方式向细胞两极分离,其减数分裂为同时型;在少数花粉母细胞减数分裂中观察到落后染色体、染色体桥等异常行为;其花粉粒育性为76.49%。黄芩的染色体数目为2n=2X=18,核型公式为K(2n)=2X=18=16m+2 sm,染色体相对长度组成为2n=1 s+4M1+3M2+1L,其核型为"1A"型。     

秤锤树的核型研究及其减数分裂过程的观察

观察研究了秤锤树有丝分裂和减数分裂的细胞学特征。秤锤树核型为2n=2x=24=4m 7sm(2SAT) 1st,属于较为原始的2A型。有丝分裂间期核为复杂染色中心型,前期出现B染色体,中期染色体中等大小。减数分裂中期具12对正常的二价体,但后期I和后期Ⅱ均有染色体异常现象发生。统计断片、落后染色体和染色体桥出现的比例与花粉粒败育性比例比较一致,表明秤锤树的小孢子在发生和发育过程中较高频率的败育现象可能存存一常的细胞学原因．     

安徽黄精属的细胞分类学研究

本文首次报道黄精属ＰｏｌｙｇｏｎａｔｕｍＭｉｌｌ我国三种特有植物的染色体数目和核型,结果如下：安徽黄精Ｐ．ａｎｈｕｉｅｎｓｅ发现两个细胞型：（１）２ｎ＝２４＝４ｍ＋６ｓｍ＋１４ｓｔ;（２）２ｎ＝２０＝４ｍ十６ｓｍ＋１０ｓｔ;　　黄精Ｐ．ｌａｎｇｙａｅｎｓｙ２ｎ＝１８＝６ｍ＋８ｓｍ＋４ｔ;距药黄精Ｐ．ｆｒａｎｃｈｅｔｉｉ有三个细胞型：（１）２ｎ＝２２＝８ｍ＋８ｓｍ（２ｓｃ）＋６ｓｔ;（２）２ｎ＝２０＝２ｍ＋１４ｓｍ＋４ｓｔ;（３）２ｎ＝１８＝４ｍ＋８ｓｍ＋４ｓｔ＋２Ｔ,全部属３Ｂ核型。黄精属植物安徽共有１０种,本文对９种黄精的染色体数目、核型进行了比较研究,发现它们可划分成三个类群,与中国植物志（第十五卷）的形态分类基本相符。     

风毛菊属6种植物的核型分析

采用常规压片技术对分布于横断山区菊科(Compositae)风毛菊属(Saussurea DC.)的6种植物进行染色体数目和核型分析。结果表明:尖苞雪莲（S.polycolea var.acutisquama）核型公式为:2n=2x=32=20m+12sm,属2B型;球花雪莲核（S.globosa）型公式为:2n=2x=34=16m+18sm,属2B型;重齿风毛菊(S.katochaete)核型公式为:2n=2x=32=8m+18sm+6st,属3B型;柱茎风毛菊(S.columnaris)核型公式为:2n=2x=32=24m+8sm,属2B型;禾叶风毛菊(S.graminea)核型公式为:2n=2x=28=8m+18sm+2st,属3B型;长毛风毛菊(S.hieracioides)核型公式为:2n=2x=32=12m+16sm+4st,属2B型。6个种染色体中均未发现随体。其中尖苞雪莲和柱茎风毛菊染色体为首次报道。     

4个洋水仙品种的核型分析

采用常规压片技术对4个洋水仙品种的体细胞染色体数目和核型进行了分析。结果显示:4个品种的染色体组成复杂多样,其核型公式依次为‘哈韦拉’2n=2x=14=8sm+6st;‘面对面’2n=3x=24=2m+15sm+7st;‘快活’2n=3x=24=3m+13sm+8st;‘花唱片’2n=4x=28=8m+16sm+4st,其核型不对称系数依次为75.19%、72.73%、74.25%和71.03%,核型类型分别为3B、3B、3B和3A。从4个洋水仙品种来源等方面的资料分析了这些品种倍性及其可能的育种价值,其中‘哈韦拉’为二倍体种间杂种,‘面对面’和‘快活’为异源三倍体;‘花唱片’为四倍体。     

风毛菊属5种植物的核型分析

采用常规压片法,对风毛菊属(Saussurea)5种植物的染色体数目和核型类型进行分析。结果表明:大耳叶风毛菊(S.macrota)核型公式为2n=2x=26=10m+12sm+4st,属2A型;长梗风毛菊(S.dolichopoda)核型公式为2n=2x=26=14m+8sm+4st,属2A型;川陕风毛菊(S.licentiana)核型公式为2n=2x=28=12m+16sm,属2B型;杨叶风毛菊(S.populifolia)核型公式为2n=2x=28=6m+18sm+4st,属2B型;尾叶风毛菊(S.caudata)核型公式为2n=2x=30=14m+14sm+2st,属2A型。这5种风毛菊属植物中,除大耳叶风毛菊染色体数目和核型类型与前人报道的一致外,其余4种植物的染色体数目和核型类型均为首次报道,并在川陕风毛菊中发现1对B染色体。     

角堇与大花三色堇染色体核型分析

以2份角堇与4份大花三色堇自交系为试验材料,采用染色体常规压片方法,观察和分析了它们的细胞染色体数目、相对长度、平均臂比等核型指标,以明确两种植物细胞学特点,为分类以及育种提供理论依据。结果表明:(1)2份角堇自交系染色体数目均为2n=2x=26,染色体基数为x=13,染色体核型公式分别为2n=2x=26=8m+12sm+6st、2n=2x=26=4m+16sm+6st,核型不对称系数为67.20%~70.10%,核型分类均属于3B。(2)4份大花三色堇自交系均为四倍体,其中2份(EYO-1-2-1-4、DSRFY-1-1-2)染色体数目为44,核型公式为2n=4x=44=4m+16sm+6st、2n=4x=44=16m+24sm+4st;2份(G10-1-3-1-4、XXL-YB-1-1-1-1)染色体数目为48,核型公式分别为2n=4x=48=8m+20sm+20st、2n=4x=48=4m+36sm+8st,核型不对称系数为66.74%~71.77%,核型分类属于2B、3B。     

All meiotic chromosomes and both centrosomes at spindle pole in the zygotes discarded as two polar bodies in clam Corbicula leana: unusual polar body formation observed by antitubulin immunofluorescence

To understand the unusual polar body formation in the androgenetic clam, Corbicula leana, whole-mount eggs stained with monoclonal antibodies against α-tubulin, γ-tubulin, and 4’-6’-diamidino-2-phenylindole were examined. The meiotic spindle was located at the peripheral region of the egg at metaphase I, and its axis was parallel to the egg surface. After segregation of chromosomes at anaphase I, cytoplasmic bulges formed at both meiotic spindle pole sites. Centrosomes were located at the apical portion of the each bulge. From the apical portion of the bulge a bundle of astral microtubules radiated toward the bulge base in late anaphase resembling a half spindle. Maternal chromosomes and both centrosomes were all distributed in two ”first polar bodies” and were eventually discarded. After the polar body formation only one male pronucleus existed in the egg cytoplasm. The present study showed that the anaphase microtubules originating from a single aster can induce the polar body formation without overlapping of microtubules from the opposing aster. Received: 29 September 1999 / Accepted: 24 November 1999     

The ribosome cycle,nucleoli, and cytoplasmic nucleoloids in the meiocytes ofLilium

Summary During the meiotic prophase in pollen mother cells ofLilium species the ribosome population of the cytoplasm diminishes to a minimum reached during the diplotene-diakinesis interval. This fall is associated with a drop in the ribonuclease-extractable RNA present in whole, fixed cells. A rise in RNA and in number of observable ribosomes follows during the meiotic mitoses and in the very early life of the spores. Bodies with the characteristics of nucleoli—here termed nucleoloids—are released into the cytoplasm at anaphase I and anaphase II, and it is suggested that these may represent the main mechanism through which the ribosome population of the cytoplasm is restored after the prophase elimination.     

广东四个墨兰品种的核型研究

研究了广东四个墨兰品种金嘴墨兰、银边墨兰、企剑黑墨和企剑白墨的染色体数目和核型。结果表明,企剑黑墨和企剑白墨的染色体数目为2n=40,为二倍体,核型公式分别为：2n=2x=40=30m＋10sm和2n=2x=40=2M＋36m＋2st;金嘴墨兰和银边睾兰的染色体数目为2n=41,为非整倍体。4个墨兰品种的染色体结构主要由中部着丝粒染色体组成,除银边墨兰为1B型外,其它均为2B型。     

3个彩色马蹄莲引进品种的核型分析

利用普通压片法对3个引进彩色马蹄莲(Zantedeschia hybrid)品种的染色体数与核型进行了分析。结果表明:所试验品种染色体数均为2n=32。染色体形态比较一致,多是由中部(m)以及近中部(sm)着丝粒染色体组成。其中,‘Allure’为2n=2x=32=14m(2SAT)+2sm,‘Cupdio’的核型公式为2n=2x=32=14m+2sm,Odessa的核型公式为2x=32=1M+15m(1SAT)。3个品种核型不对称系数分别为56.72%,56.25%和56.38%,核型分类显示其均为1A型。     

6个香雪兰品种的染色体核型及聚类分析

以香雪兰（Freesia hybrida）6个品种的根尖为研究材料进行核型分析以揭示其核型特征,进一步通过聚类分析品种间的相似性并探讨可能的亲缘关系。结果表明：香雪兰6个品种均为四倍体,染色体数目都为44。6个品种的核型公式不同：‘Gold River’为2n=4x=44=33m+11sm,‘White River’为2n=4x=44=1M+34m+9sm,‘Castor’为2n=4x=44=35m+9sm,‘上农红台阁’为2n=4x=44=32m+12sm,‘Pink Passion’为2n=4x=44=38m+6sm,‘Red River’为2n=4x=44=37m+7sm。核型参数因品种而异,其中,‘Castor’在相对长度范围和臂比范围上均为最广,‘上农红台阁’核不对称系数最大。6个品种核型不对称系数为57.00%~60.07%,核型类型均为2B,进化程度中等,处于由对称至不对称的过渡阶段,其核型进化的趋势大致为：‘Pink Passion’→‘Red River’→‘Gold River’→‘White River’→‘Castor’→‘上农红台阁’。聚类结果显示,遗传距离为15时可将所有品种分为两类,第一类包含‘Gold River’‘上农红台阁’和‘Castor’; 第二类包含‘Pink Passion’‘Red River’和‘White River’,其核型参数的差异可作为香雪兰品种分类和鉴定的辅助依据,为其细胞学研究和育种实践提供理论参考。     

Continuous cultures of tomato and citron roots in vitro

Summary Initial trials with tomato-root cultures disclosed the desirability of employing a gently agitated liquid medium containing iron in the chelated form. For the normal cultivars “Ace” and “Tropic”, subcultures were best achieved by utilizing sectors that possessed one or more newly emerged laterals. Continuous cultures of a nonlateral-forming tomato mutant, “Diageotropica”, and of citron were accomplished by subculturing tips of the elongating primary roots. The tomato roots were cultured in White's medium with the Fe₂(SO₄)₃ replaced by 0.03 mM NaFeEDTA. Sustained growth of citron-root tips necessitated the use of a medium containing Murashige and Skoog salts, 7.5% sucrose, 100 mg per I each of citric acid and thiamine HCl, and 5000 mg per li-inositol. The success with citron-root cultures was extendable to all cultivars ofC. medica L., but not to otherCitrus species relatives. Both citron and “Diageotropica” root cultures manifested undiminished elongation through repeated subcultures; but neither produced laterals in response to any cultural treatments. Research was supported in part by National Science Foundation Grant OIP75-10390 and Elvenia J. Slosson Fellowship in Ornamental Horticulture.     

ASK1, a SKP1 homolog, is required for nuclear reorganization, presynaptic homolog juxtaposition and the proper distribution of cohesin during meiosis in Arabidopsis

Nuclear reorganization and juxtaposition of homologous chromosomes at late leptotene/early zygotene are essential steps before chromosome synapsis at pachytene. We report the results of detailed studies, which demonstrate that nuclear reorganization and homolog juxtapositioning processes are defective in a null mutant, ask1-1. Our results from 4, 6-diamino-2-phenylindole (DAPI)-stained spreads showed that the “synizetic knot”, which is typically found in wild type (WT) meiosis during late leptotene and zygotene, was missing in the ask1-1 mutant. Furthermore, ask1-1 meiocytes exhibited only limited homolog juxtaposition at centromere regions at early zygotene. Immunodetection of the cohesin protein SYN1 identified ask1 defects in cohesin distribution from zygotene to anaphase I. Analysis of meiotic chromosomes in ask1-1 and syn1 single mutants, as well as an ask1-1 syn1 double mutant indicate that ASK1 is required for normal SYN1 distribution during meiotic prophase I and suggest that ask1 associated defects may be primarily related to SYN1 mislocalization.     

Desynaptische Mutanten mit Unterschieden im Univalentenverhalten

After application of neutrons on dry seeds ofPisum sativum three recessive mutants were isolated showing irregularities in the course of meiosis. A cytogenetical analysis showed that at metaphase I, a varying number of univalents are formed, most likely as a result of reduced chiasma frequencies. At anaphase I, some univalents divide precociously in mutant 2982 but none do so in mutants 2989 and 2552. As a consequence, most cells of 2989 and 2552 built up more than two spindles at anaphase II, whereas the majority of cells in 2982 form two spindles. This situation is reflected in the frequency distribution of gones per PMC at tetrad stage. The discussion deals with the possible causes of univalent formation at meiotic prophase and the variability of univalent behaviour at anaphase I.     

Genetic diversity and relationship of clonal tea (<Emphasis Type="Italic">Camellia sinensis</Emphasis>) cultivars in China as revealed by SSR markers

Tea plant [Camellia sinensis (L.) O.Kuntze)] is one of the most popular non-alcoholic beverage crops in the world today. In recent years, many clonal tea cultivars have been developed and widely planted to replace the diverse traditional tea populations. In this article, we study the relationships between classifications based on simple sequence repeat (SSR) markers and on morphological traits for 185 tea plant cultivars. Results show that the genetic diversity index (H) is between 0.229 and 0.803, and the mean value is 0.543; the observed heterozygosity (H _o) ranges from 0.103 to 0.683, with an average of 0.340, while the genetic identity varies from 0.267 to 0.984. Based on tea-making properties, the genetic diversity in the “black-green tea” group is much higher than in the “Oolong tea” group. Based on morphological traits, cluster analysis classifies the 185 cultivars into three groups, “group I,” “group II” and “group III.” Most cultivars are related based on the geographical origin and their genetic backgrounds.     

中国蜘蛛抱蛋属的细胞分类学研究Ⅱ

报道了 11种蜘蛛抱蛋属植物的染色体数目和核型。结果如下 :伞柱蜘蛛抱蛋 ** ,2 n=36 =2 0 m+6 sm(2 sat) +10 st,属 2 C型 ;辐花蜘蛛抱蛋 ** ,2 n=38=2 2 m+6 sm(2 sat) +10 st,属 2 C型 ;棒蕊蜘蛛抱蛋 **,2 n =36 =18m +8sm (2 sat) +10 st,属 2 C型 ;柳江蜘蛛抱蛋 **,2 n=38=2 0 m +6 sm(2 sat) +12 st,属 2 C型 ;小花蜘蛛抱蛋 ,2 n=38=16 m +4sm +8st (2 sat) +10 t,属 3C型 ;线叶蜘蛛抱蛋 ** ,2 n=36 =2 0 m(2 sat) +16 st,属 2 C型 ;罗甸蜘蛛抱蛋 ,2 n=38=16 m+6 sm(2 sat) +16 st,属 2 C型 ;四川蜘蛛抱蛋 ,2 n=38=2 4 m +4sm+10 st (2 sat) ,属 2 C型 ;广东蜘蛛抱蛋 ,2 n=36 =18m +2 sm(2 sat) +16 st,属 2 C型 ;洞生蜘蛛抱蛋 **,2 n=36 =18m +2 sm(2 sat) +14st+2 t,属 2 C型 ;大花蜘蛛抱蛋 ,2 n=36 =16 m+6 sm(2 sat) +14st,属 3C型。其中棒蕊蜘蛛抱蛋、柳江蜘蛛抱蛋、线叶蜘蛛抱蛋和洞生蜘蛛抱蛋的染色体数目和核型以及广东蜘蛛抱蛋的核型均为首次报道。     

凤仙花近缘种间核型分析与叶表皮微形态研究

为探究凤仙花近缘种植物的细胞学和微形态学方面的亲缘关系,该文选取荔波凤仙花(Impatiens liboensis)及近缘种赤水凤仙花(I.chishuiensis)和管茎凤仙花(I.tubulosa)的根尖和叶表皮为实验材料,采用体细胞染色体常规压片法和叶表皮光学显微镜观察法对凤仙花近缘种植物进行染色体及叶表皮特征研...     

Black rat (Rattus rattus) genomic variability characterized by chromosome painting

Black rats are of outstanding interest in parasitology and infective disease analysis. We used chromosome paints from both the mouse(Mus musculus) and the Norway rat(Rattus norvegicus) to characterize the genome of two Black rat subspecies from Italy. Both subspecies have two large metacentrics (n. 1, 4) not present in the Norway rat (2n = 42).Rattus rattus rattus has a diploid number of 2n = 38, whileRattus rattus frugivorous has two small metacentric “supernumerary” or B chromosomes for a diploid number of 2n = 38 + 2B. The 21 mouse paints gave 38 signals on theR. r. rattus karyotype and 39 signals in theR. r. frugivorous karyotype. The two metacentrics, not present inR. norvegicus, were hybridized by mouse 16/1/17 and mouse 4/10/15. These chromosomes are homologous to: RRA1 = RNO 5/7, and RRA4 = RNO 9/11 and not “4/7” and “11/12” as previously reported. Furthermore, the synteny of Chr 13 of theR. r. frugivorous withR. norvegicus Chr 16 and mouse Chrs 8/14 is not complete, because there is a small pericentromeric insertion of RNO Chr 18 (mouse Chr 18). If we consider only the two metacentrics, RRA1 and RRA4, the principal differences betweenR. norvegicus andR. rattus, then we can propose the derived synteny of 124 genes in the black rat. A comparison of the Z index between rats and mice shows an acceleration of genomic evolution among genus, species, and subspecies. The chromosomal differences betweenR. r. rattus xR. r. frugivorous suggest that they may be classified as different species because hybrids would produce 50% unbalanced gametes.