虫草蝙蝠蛾的有丝分裂染色体特性

本文首次报道虫草蝙蝠蛾（鳞翅目，蝙蝠蛾科，蝙蛾属）的有丝分裂染色体核型。应用醋酸分离和热干燥技术，研究了云南的两种虫草蝙蝠蛾Hepialus zhayuensis Chu er Wang Hepialus sp.的有丝分裂染色体，　他们的染色体数目为2n=64。在有丝分裂的早中期染色体上清晰地呈现出散漫着丝粒。然而，分裂中期和较晚的中期阶段，每条染色体裁都具有显著的初级着丝粒（即主缢痕）。他们的雄性中期核型都有一对典型的异型性染色体，X染色体着色稍淡，且都具中或亚中着丝粒；Y染色体比X染色体长，染色很深。 在胸性的分裂间期细胞中，观察到异固缩性染色质体，此异固缩体是Y染色体。     

中国云南果蝇属暗果蝇种组的核型分化

观察了新近发现于我国云南的果蝇属暗果蝇种组(Drosophila obscura species group)种类D．luguensis、D．dianensis和D．limingi的有丝分裂中期核型,并将3个种的核型与各自的近缘种类进行了比较。D．luguensis具2n=12条染色体,包括3对中央着丝粒(V形)染色体、2对近端着丝粒(棒状)染色体以及1对微小(点状)染色体。其中X和Y染色体均为中央着丝粒染色体。D．dianensis和D．limingi具2n=10条染色体,包括1对大的V形常染色体,1对小的V形常染色体,2对J形(亚中着丝粒型)常染色体和1对点状染色体。其中X染色体为J形,Y染色体为短棒状。基于核型比较的结果以及D．sinobscura亚组地理分布的资料,结合种间系统发育关系研究结果,认为D．luguensis可能保留了该亚组祖先种类的核型。D．sinobscum的核型(2n=12：2V,1J,2R,1D)可能由一个pre-“sinobscura-hubeiensis”谱系的一个分支通过臂间倒位演化而来,而D．hubeiensis的核型(2n=10：4V,1D)可能由该谱系的另一分支通过着丝粒融合(2对近端着丝粒常染色体的融合)而形成。推测在D．dianensis和近缘欧洲种D．subsilvestris(2n=12：3V,2R,1D)间、D．limingi和东亚近缘种D．tsukubaensis(2n=12：3V,2R,1D)间的物种分化过程中,可能有相似的染色体变异类型发生。     

蝙蝠科七种蝙蝠的核型

报道了贵州7 种蝙蝠科蝙蝠的核型。伏翼和印度伏翼的染色体数为2n = 26 , 常染色体都由10 对双臂染色体和2 对微小点状染色体组成, N.F = 44 , 性染色体是大小悬殊的端着丝粒染色体; 两者核型的主要区别在于前者的No.3 是中着丝粒染色体, 后者为亚中着丝粒染色体; 大鼠耳辐(四川亚种) 、水鼠耳蝠和西南鼠耳蝠的染色体数都是2n = 44 , 常染色体都由4 对中着丝粒染色体和17 对端着丝粒染色体组成, N.F = 50 , 其中大鼠耳蝠(四川亚种) 和水鼠耳蝠核型非常相似, 西南鼠耳蝠与前二者有一定区别; 山蝠(福建亚种) 是2n = 36 , 常染色体包括7 对中着丝粒染色体、1 对亚中着丝粒染色体和9 对端着丝粒染色体, N.F = 50 ; 南蝠2n = 50 , 常染色体由24 对端着丝粒染色体组成, N.F = 48 , X染色体是最大的中着丝粒染色体。     

近亲幽灵蛛的核型分析（蜘蛛目：幽灵蛛科）

报告近亲幽灵蛛的核型分析,包括:染色体数目、形态结构和性染色体组成。实验材料采自石家庄郊区的校园中,细胞学数据主要来自对肝胎细胞有丝分裂中期的观察。实验结果表明:近亲幽灵蛛的染色体数目是:雄体细胞为25条,雌体细胞为26条。性别决定机制属XO系统,X染色体是核型中最长的1条(对),也是唯一1条(对)典型的业中部着丝粒染色体,这在我们过去的实验中尚属第一次发现。对近亲幽灵蛛的C-带标本分析表明:所有染色体都有明显的着丝粒带,只是X染色体及1~＃常染色体的着丝粒带为淡染带。4~＃常染色体长臂中部有一宽染深带。极具识别特点。5~＃常染色体中的1条具一般着丝粒带,另1条全部深染,表明它富含结构异染色质。此外,其常染色体1~＃、3~＃、4~＃、8~＃、11~＃、12~＃和X染色体上,除有着丝粒带外,在长臂末端均出现端粒带(T带),其产生机制有待进一步研究。在染色体G-显带标本中,获得了较清晰的带纹。     

用C-带和涂染技术检测棕色田鼠Y染色体

采用染色体C 带技术和小鼠整条Y染色体特异探针检测棕色田鼠的Y染色体 ,结果如下 :棕色田鼠雄性个体C 带中期分裂相中 ,X性染色体是亚中部着丝粒染色体 ,在着丝粒处存在着强烈的C阳性带 ,而且在短臂的中间也有一条C阳性带 ,但是没有发现深染的Y染色体。用小鼠整条Y染色体特异探针涂染棕色田鼠的骨髓细胞中期分裂相和间期核 ,以小鼠骨髓细胞中期分裂相和间期核作为对照。涂染结果表明 :棕色田鼠骨髓细胞中期分裂相和间期核涂染信号检出率分别为 0 - 2 %和 3% - 5 % ,两者均呈阴性反应 ,而对照都呈阳性反应。根据实验结果 ,作者认为在棕色田鼠的Y染色体上及整个基因组DNA中不存在小鼠整条Y染色体特异DNA的同源序列 ,其Y染色体上可能没有决定雄性性别的重要基因     

小鼠的克隆着丝粒(SFA)DNA的鉴定

着丝粒是真核染色体上的重要细胞器,是真核染色体作为基因载体行使其遗传功能的关键结构.着丝粒DNA首先是从酵母中分离克隆并被用以构建酵母人工染色体.鉴于真核有丝分裂机制研究和构建高等动物人工染色体研究的需要,从分离和检定过的小鼠着丝粒DNA库中筛选出了6#着丝粒DNA(SFADNA),并用荧光原位杂交法(FISH)对其进行了在染色体上的定位检定.用缺口平移法和PCR法分别标记了SFA DNA和SFA DNA中的小鼠寡份卫星DNA作为探针,分别与小鼠腹水癌细胞和小鼠L929细胞进行原位杂交;并用荧光抗体显示杂交信号的位置.结果,SFA DNA在两种细胞的中期染色体上的杂交信号都位于亚末端的初级缢痕处,表现为单一粗大的斑块.寡份卫星DNA在两种细胞的中期染色体上的杂交信号亦都位于亚末端的初级缢痕处,但极大多数的斑点均表现为成对的细小斑点.初级缢痕正是染色体着丝粒所在的特征性部位.故以上结果说明定位于该部位的克隆的6#SFA DNA,和其中的小鼠寡份卫星DNA都来源于小鼠着丝粒DNA.     

着丝粒结构与功能研究的新进展

着丝粒是真核生物染色体的显著特征。在细胞有丝分裂和减数分裂中, 着丝粒作为保证染色体正常分裂并分离到子细胞的结构和功能元件, 参与了同源染色体配对、姐妹染色单体黏合、分离及分裂后期启动的调控等。本文对近年来着丝粒结构和功能研究的新进展进行了概述。     

着丝粒结构与功能研究的新进展

着丝粒是真核生物染色体的显著特征。在细胞有丝分裂和减数分裂中,着丝粒作为保证染色体正常分裂并分离到子细胞的结构和功能元件,参与了同源染色体配对、姐妹染色单体黏合、分离及分裂后期启动的调控等。本文对近年来着丝粒结构和功能研究的新进展进行了概述。     

小鼠富集着丝粒DNA在小鼠减数分裂粗线期染色体上的原位杂交

本工作用Hoechst 33258及着丝粒特异抗体间接免疫荧光法显示的小鼠粗线期染色体主缢痕区,与以小鼠富集着丝粒(SFA)DNA为探针在粗线期染色体上的原位杂交主缢痕区作了比较。发现SFA DNA探针不仅杂交于全部常染色体联会复合体上的着丝粒区,并且杂交于着丝粒周围的异染色质区;而且,也杂交于X,Y染色体的着丝粒区。由此结论:此富集SFA DNA中含有全套常染色体及X,Y染色体的SFA DNA。     

大鼠高重复序列Rat(Hind Ⅲ)-1的染色体定位研究

以分离、纯化的370bp大小的Rat(HindⅢ)-1高重复序列为探针,用Biotin-Ⅱ-dUTP进行缺口翻译标记;与Wistar大鼠骨髓间期细胞和中期染色体进行原位杂交;用生物索化的碱性磷酸酶检测杂交结果。大鼠核型中除X,Y,1,2,12和20号染色体外,其余染色体着丝粒处均有杂交颗粒,以10,5,7,11,13号染色体所占比例较多。间期细胞核中亦可见到排列不规则的杂交颗粒。核杂交效率高于染色体杂交效率。Rat(HindⅢ)-1可能是Wistar大鼠特有的、普遍分布于染色体着丝粒处的一类高重复序列。     

小花蝽属两种核型的研究(半翅目: 花蝽科)

本文利用姬姆萨染色空气干燥压片方法,对花蝽科小花蝽属中国2种小花蝽的性细胞核型进行了研究.研究结果表明该2种小花蝽的2倍体均具有24条染色体和X-Y性别机制,但2种间在染色体行为特征方面具有差别,主要表现在细胞减数分裂的晚终变期和中期常染色体以及性染色体的排列形状与位置等方面,该特征可以用于种间的细胞分类.     

CYTOLOGICAL STUDIES OF PATERCULUS ELATUS (YANG) (HEMIPTERA:PENTATOMIDAE)

Abstract The karyotype of a Chinese pentatomid species Paterculus elatus (Yang) was studied in male germ cells prepared on air-dried slides stained with Giemsa. Karyotype analyses using specific software were made and model karyotype chart was presented. P. elatus (Yang ) has 16 chromosomes on mitosis metaphase plate and a X-Y sex chromosomal mechanism. The cytogenetic analysis has revealed the presence of a pair of m-chromosomes and a supernumerary chromosome.     

两种突颜蝗的染色体C带核型研究

采用染色体C分带技术初次对癞蝗科Pamphagidae中国特有的突颜蝗属Eotmethis B.-Bienko 2个种,即天祝突颜蝗E. tientsuensis (Chang)和景泰突颜蝗E.jintaiensis Xi et Zheng的精原细胞有丝分裂中期和初级精母细胞减数分裂中期（中期I）染色体C带核型进行了比较研究。结果表明: 2种突颜蝗的染色体基数、着丝粒位置及染色体分组形式相同,且与前人的研究结果基本吻合,反映了癞蝗科昆虫核型的稳定性。同时,2种突颜蝗染色体相对长度值较为接近;结构异染色质总含量没有明显差异;并且两者无论在精原细胞有丝分裂中期还是减数分裂中期I细胞,其3号、4号和X染色体上都显现深着色较大块的着丝粒C带, 9号染色体上都出现大块深着色的端部C带,2号染色体上都发生清晰的近中部居间C带,以上反映了2个种在系统发生上的亲缘关系。另外,2种突颜蝗在C带带型上的差异,在1号、7号、8号染色体上有不同程度的反映,尤其是对应的7号、8号染色体上着丝粒C带块的大小和强弱有明显变化。     

卷蝽Paterculus elatus(Yang)的细胞学研究(半翅目:蝽科)(英文)

本文研究了中国蝽科昆虫──卷蝽 Ｐａｔｅｒｃｕｌｕｓ ｅｌａｔｕｓ（Ｙａｎｇ）的核型并采用核型分析软件对第一次减数分裂终变期的染色体进行了该型分析。结果表明：卷蝽的２ｎ＝１６,具有ＸＹ性别决定机制,具有一对ｍ－染色体,在有些细胞中出现一个超量染色体。     

Genetic and cytogenetic analysis of the fruit fly Rhagoletis cerasi (Diptera: Tephritidae).

The European cherry fruit fly, Rhagoletis cerasi, is a major agricultural pest for which biological, genetic, and cytogenetic information is limited. We report here a cytogenetic analysis of 4 natural Greek populations of R. cerasi, all of them infected with the endosymbiotic bacterium Wolbachia pipientis. The mitotic karyotype and detailed photographic maps of the salivary gland polytene chromosomes of this pest species are presented here. The mitotic metaphase complement consists of 6 pairs of chromosomes, including one pair of heteromorphic sex chromosomes, with the male being the heterogametic sex. The analysis of the salivary gland polytene complement has shown a total of 5 long chromosomes (10 polytene arms) that correspond to the 5 autosomes of the mitotic nuclei and a heterochromatic mass corresponding to the sex chromosomes. The most prominent landmarks of each polytene chromosome, the "weak points", and the unusual asynapsis of homologous pairs of polytene chromosomes at certain regions of the polytene elements are also presented and discussed.     

Codling moth cytogenetics: karyotype, chromosomal location of rDNA, and molecular differentiation of sex chromosomes.

We performed a detailed karyotype analysis in the codling moth, Cydia pomonella (L.) (Lepidoptera: Tortricidae), the key pest of pome fruit in the temperate regions of the world. The codling moth karyotype consisted of 2n = 56 chromosomes of a holokinetic type. The chromosomes were classified into 5 groups according to their sizes: extra large (3 pairs), large (3 pairs), medium (15 pairs), small (5 pairs), and dot-like (2 pairs). In pachytene nuclei of both sexes, a curious NOR (nucleolar organizer region) bivalent was observed. It carried 2 nucleoli, each associated with one end of the bivalent. FISH with an 18S ribosomal DNA probe confirmed the presence of 2 clusters of rRNA genes at the opposite ends of the bivalent. In accordance with this finding, 2 homologous NOR chromosomes were identified in mitotic metaphase, each showing hybridization signals at both ends. In highly polyploid somatic nuclei, females showed a large heterochromatin body, the so-called sex chromatin or W chromatin. The heterochromatin body was absent in male nuclei, indicating a WZ/ZZ (female/male) sex chromosome system. In keeping with the sex chromatin status, pachytene oocytes showed a sex chromosome bivalent (WZ) that was easily discernible by its heterochromatic W thread. To study molecular differentiation of the sex chromosomes, we employed genomic in situ hybridization (GISH) and comparative genomic hybridization (CGH). GISH detected the W chromosome by strong binding of the Cy3-labelled, female-derived DNA probe. With CGH, both the Cy3-labelled female-derived probe and Fluor-X labelled male-derived probe evenly bound to the W chromosome. This suggested that the W chromosome is predominantly composed of repetitive DNA sequences occurring scattered in other chromosomes but accumulated in the W chromosome. The demonstrated ways of W chromosome identification will facilitate the development of genetic sexing strains desirable for pest control using the sterile insect technique.     

Karyotype variation in Drosophila birchii

Drosophila birchii, a member of the melanogaster species group of the subgenus Sophophora, is common in the tropical rain forests of the Australia-New Guinea areas. Chromosome squashes are easily prepared from the larval ganglion cells and the sex chromosomes are readily recognizable. The species exhibits a remarkable karyotype variation. The metaphase plate figures, in general, show two pairs of V's, one pair of dots and one pair of sex chromosomes. Variations in metaphase chromosome morphology are found in the X (with four types), the Y (with three types) and chromosome IV (with two types). Chromosomal interchanges between X- and Y-chromosomes Type I are postulated to be involved in the differentiation of sex chromosome morphology while the modification of chromosome IV seems likely to be a result of the acquisition of extra heterochromatin. These chromosome types form seven distinct metaphase plate figures, all encountered in wild populations, thus giving D. birchii the most variable karyotype in the genus Drosophila.     

Comparing the karyotype of the European domestic goose and the Asian goose on the basis of the karyotype of their interspecific cross-breed, using the RBG chromosome staining technique

The aim of the research was to compare the karyotypes of two goose species: the European domestic goose and the Asian goose on the basis of the karyotype of their interspecific cross-breed, using the RBG chromosome staining technique. The karyotype standard for Anseriformes has not been determined yet. The RBG technique is considered as one of the standard methods for analysing chromosomes. It is a dynamic method. The R bands appear during the cell growth cycle in the early S phase. The formation of the characteristic band configuration for each chromosome facilitates chromosome segregation and analysis. The mitotic chromosomes for experiments were obtained from an in vitro blood lymphocyte culture and stained according to the RBG technique. The first eight largest autosome pairs and the ZW sex chromosomes were analysed. No differences were found between the band patterns of the analysed chromosomes, except for the fourth autosome pair.     

C-heterochromatin and extra (B) chromosome distribution in six species of the Nabis (Heteroptera, Nabidae) with the modal male karyotype 2n = 16 + XY

The basic male karyotype of the six Nabis species (Heteroptera, Nabidae) is confirmed as being 2n=16+XY. The chromosomes are holokinetic while male meiosis is achiasmatic. The sex chromosomes undergo postreduction and in second metaphase show distance pairing, registered in all nabid species examined so far. Using C-banding technique for the first time in the family Nabidae, the heterochromatin was revealed on chromosomes of six species. The species showed different amount and distribution of C-heterochromatin. Only in Nabis (Dolichonabis) limbatus did the C-bands distribution make possible the identification of every chromosome pair in the karyotype. In other species, C-bands were found in some of the autosomes and the X, localized either interstitially or at telomeres. Only the Y usually showed relative stability ofthe C-banding pattern. In four of six species, extra (B) chromosomes were observed and their behaviour in meiosis described.     

Karyotype of mitotic metaphase and meiotic diakinesis in non-heading Chinese cabbage

Non-heading Chinese cabbage [Brassica rapa L. ssp. chinensis (L.) Hanelt] is one of the most popular leafy vegetables. Despite the economic importance of non-heading Chinese cabbage, little attention has been given to its cytogenetic profile. This study reveals the karyotype of non-heading Chinese cabbage. Fluorescence in situ hybridization (FISH) with 45S and 5S rDNA probes was performed on mitotic metaphase complementary regions. We located 45S rDNA on the centromeric or adjacent region of chromosomes A1 and A2, with the largest on the satellite of chromosome A5. Meanwhile, 5S rDNA co-localized with 45S rDNA on chromosomes A2 and A5, and on the telomeric region of chromosome A10. We performed DAPI fluorescence banding on the same metaphase chromosomes to identify homologous chromosomes. The DAPI fluorescence pattern was observed mainly on the centromeric heterochromatin regions of each chromosome. However, the lengths of chromosomes A2 and A6 were completely stained, except for their telomeric regions. Meiotic diakinesis chromosomes as new substrates in FISH-developed karyotype were revealed for the first time. The karyotype of non-heading Chinese cabbage reveals that it contains eight submetacentric chromosomes, one subtelocentric chromosome (bearing satellite), and one telocentric chromosome. Diakinetic chromosome pairing can overcome the difficulty of unlabeled chromosome identification. This study provided valuable information for cytogenetic research and molecular breeding of non-heading Chinese cabbage by using the combination of FISH and DAPI fluorescence patterns on mitotic and meiotic chromosomes.