河南纺蚋多线染色体研究

目的对河南纺蚋多线染色体核型及带型进行描述,对稳定且可作为该种重要鉴别依据的结构特征加以识别,并提供表示多线染色体相对长度、着丝粒位置和重要界标的模式图。方法取成熟幼虫分离出唾液腺,经苯酚品红染色、压片后,镜检、摄影和测量,作统计学处理。结果与结论河南纺蚋多线染色体数目为3条,第Ⅰ号具中央着丝粒,第Ⅱ、Ⅲ号为亚中央着丝粒,臂比值(着丝粒位置)高度稳定;ⅠS、ⅠL、ⅡS、ⅡL、ⅢS游离端均钝圆深染,ⅢL末端疏松膨大为扇形呈颗粒状浅染;核仁组织原、巴氏环、双泡、宽深带以及浅染膨大区等主要特征性结构的位置及形态恒定一致,可作为该种的重要鉴别特征。     

嗜人按蚊的唾腺染色体

本文描述了我国疟疾媒介嗜人按蚊(Anopheles anthropophagus)的唾腺染色体图。此蚊的唾腺染色体由五个臂组成。第1号染色体为性染色体,又称X-染色体,是近端着丝粒,只有一个臂,它是各臂中最短的,此臂分为5个区;第2号染色体是中心着丝粒,左、右臂约等长,两臂共分为16个区;第3号染色体为亚中心着丝粒,右臂是各臂中最长的,左臂则是常染色体中最短的,两臂共分为18个区。     

尼罗罗非鱼染色体的C带,Ag带和减数分裂联合复合体的研究

以Sunmer法和界面铺张——硝酸银技术,对尼罗罗非鱼（Tilapia nilotica）染色体C带,Ag染带及减数分裂前期精母细胞联会复合体（SC）进行了显微和亚显微结构观察。尼罗罗非鱼的2n=44,核型可分为三个组：第一组为4对亚中着丝粒染色体;第二组为17对亚端着丝粒染色体;第三组为具1对端着丝粒的特大染色体。结构异染色质主要分布于着丝粒附近,其中Nos.6、8、15亚中着丝粒染色体短臂全部深染。带有银染核仁组织者（Ag-NORs）染色体的数目为2-6条,NORs均位于6、8、15亚中着丝粒染色体短臂。银染色可清楚地显示尼罗罗非鱼的联会复合体（SC）结构和减数分裂行为。SC组型与有丝分裂染色体的组型有较好的一致性。     

尼罗罗非鱼染色体的C带、Ag带和减数分裂联会复合体的研究

以Sumner法和界面铺张——硝酸银技术,对尼罗罗非鱼(Tilapia nilotica)染色体C带、Ag染带及减数分裂前期精母细胞联会复合体(SC)进行了显微和亚显微结构观察。 尼罗罗非鱼的2n=44,核型可分为三个组:第一组为4对亚中着丝粒染色体;第二组为17对亚端着丝粒染色体;第三组为具1对端着丝粒的特大染色体。 结构异染色质主要分布于着丝粒附近,其中Nos.6、8、15亚中着丝粒染色体短臂全部深染。带有银染核仁组织者(Ag-NORs)染色体的数目为2—6条,NORs均位于6、8、15亚中着丝粒染色体短臂。 银染色可清楚地显示尼罗罗非鱼的联会复合体(SC)结构和减数分裂行为。SC组型与有丝分裂染色体的组型有较好的一致性。     

贵州雷山产虎斑游蛇染色体组型和银带研究

贵州雷山产虎斑游蛇雌性染色体数为2 n=38+ZW。大型染色体8对,其中第1、2、3、6对为中部着丝粒染色体,第4、7、8对为端部着丝粒染色体,第5对为性染色体,Z染色体为中部着丝粒染色体,W为亚中部着丝粒染色体。银染表明核仁组织者区位于一对小型染色体及一条第4号染色体的端部。比较了贵州雷山、道真、山西太原、辽宁及日本产虎斑游蛇染色体组型的异同。     

正常人和21三体征家庭的银染核仁形成区的研究

DNA-RNA原位杂交术证明了人类18S—28S核糖体RNA基因位于5对近端着丝点染色体短臂的次缢痕处,即人类的核仁形成区(NOR)。1975年,Goodpasture和Howell等应用银氨法特异地染色核仁形成区,证实银染的位置是染色体上核糖体基因(rDNA)的位置。此后进一步证明银染物质不是rDNA,也不是rRNA,而可能是核仁     

薏苡45S和5S rDNA的染色体定位研究(简报)

通过荧光原位杂交的方法确定了45S和5S正NA序列在薏苡前中期染色体上的位置.尽管具有20条染色体的薏苡是四倍体植物,但它的基因组中只有一个45S和5S rDNA位点.根据薏苡前中期染色体的核型,确定45S rDNA序列位于薏苡第2号染色体短臂上的次级缢痕区和随体上,5S rDNA序列位于第7号染色体长臂靠近着丝粒处,5S rDNA位点到着丝粒的百分距离是29.13±1.76.     

不同地理区域鲫鱼染色体银染核仁组织者的比较研究

本文对不同地理区域的鲫鱼(Carassius auratus)—滇池高背鲫、低背鲫、方正银鲫(C.auratusgibelio)的核型及核仁组织者NORs进行了比较研究,并对高背鲫来源作些初步探讨,结果如下: 1.低背鲫Carassius auratus (back low type):2n=100,22m+30sm+48t.st,NORs=4,出现于第5—6对亚中着丝粒染色体短臂。 2.滇池高背鲫Carassius auratus(back high type):2n=156,30m+46sm+80t.st,NORs=6,出现于第5—7对亚中着丝粒染色体短臂。 3.方正银鲫C.auratus gibelio:2n=162,32m+52sm+78t.st NORs=4,出现于第5—6对亚中着粒染色体短臂。     

栽培荞麦45S和5S rDNA的染色体物理定位研究

采用双色荧光原位杂交技术,对栽培荞麦甜荞和苦荞有丝分裂中期染色体上的45S和5S rDNA基因物理位置进行了定位分析。结果表明,甜荞有4对45S rDNA位点,位于ⅠS、ⅡS、ⅢL、ⅤL(L和S代表长臂和短臂,罗马数字代表染色体序号,下同);2对5S rDNA位点,位于ⅠL、ⅣS。苦荞有5对45S rDNA位点,位于ⅠS、ⅡS、ⅢL、ⅤL、ⅦS;3对5S rDNA位点,位于ⅠL、ⅣS、ⅥS。甜荞与苦荞的45S和5S rDNA位点具有明显的差异,显示其起源上关系较远。依据中期染色体45S和5SrDNA位点信息及经典核型特征,可以准确鉴别甜荞与苦荞8对同源染色体。     

皱纹盘鲍的染色体研究

本文报道皱纹盘鲍的染色体制备方法及核型分析结果。皱纹盘鲍的2n=36,可配为18对,中央着丝点(M)的11对,即1,3,6,7,9,11,12,13,14,16,17号染色体。亚中央着丝粒(Sm)的7对,即2,4,5 8,15,18号染色体,NF=72。染色体的长度呈连续递变。其中相对长度最长的1号染色体为7.09,最短的18号染色体4.11,单倍体总长687.05。     

Cytogenetic analysis of Malpighian tubule and salivary gland polytene chromosomes of Bactrocera oleae (Dacus oleae) (Diptera: Tephritidae).

Photomaps of the Malpighian tubule and the salivary gland polytene chromosomes of Bactrocera oleae (Dacus oleae) are presented and compared with those of the fat body. Five polytene chromosomes (10 polytene arms) corresponding to the five autosomes of the mitotic nuclei, as well as a heterochromatic mass corresponding to the sex chromosomes, are observed in the nuclei of the three somatic tissues. The most prominent features of each polytene chromosome, the reverse tandem duplications, as well as the rather unusual ectopic pairing of the telomeric regions of different chromosome arms, are described. The constancy of the banding pattern based on the analysis of the three larval tissues is discussed.     

Homologous banding patterns in the polytene chromosomes from the larval salivary glands and ovarian nurse cells of Anopheles stephensi liston (Culicidae)

A comparison of the banding patterns of two homologous polytene chromosome arms from the larval salivary gland and ovarian nurse cell complement of Anopheles stephensi is presented. The homologous chromosomes from the somatic larval salivary glands and germ-line derived ovarian nurse cells have essentially the same band-interband organisation. An analysis of the ³H-uridine labelling patterns of a small chromosome segment from the two tissues indicates that germ-line polytene chromosomes are not radically different from somatic polytene chromosomes in their patterns of gene expression.     

Polytene chromosome maps of the melon fly Bactrocera cucurbitae (Diptera: Tephritidae).

Standard photographic maps of the polytene chromosomes are presented for the melon fly Bactrocera cucurbitae, a serious pest of fleshy fruits and vegetables. Five larval salivary gland polytene chromosomes (10 polytene arms) were isolated, and their characteristic features and landmarks have been recognized. Banding patterns of each of the polytene arms are presented, where variation in band intensity and puffs appear to reflect fundamental differences in chromosomes. The whole polytene genome has been typically mapped by dividing it into 100 sections and the subsections were lettered. The mitotic chromosomes of larval brain ganglia are also examined, five pairs of autosomes and an XX/XY sex chromosome pair. In addition, a heterochromatic mass corresponding to the sex chromosomes are observed in the polytene nuclei of salivary gland tissue. This investigation showed that B. cucurbitae has excellent cytological material for polytene chromosome analysis and proved to be very useful for obtaining more detailed genetic information on the pest's natural populations.     

Satellite DNA of Anopheles stephensi liston (Diptera: Culicidae)

Four satellite DNAs in the Anopheles stephensi genome have been defined on the basis of their banding properties in Hoechst 33258-CsCl density gradients. Two of these satellites, satellites I and II, are visible on neutral CsCl density gradients as a light density peak forming approximately 15% of total cellular DNA. Hoechst-CsCl density gradient profiles of DNA extracted from polytene tissues indicates that these satellites are underreplicated in larval salivary gland cells and adult female Malpighian tubules and possibly also in ovarian nurse cells. The chromosomal location of satellite I on mitotic and polytene chromosomes has been determined by in situ hybridisation. Sequences complementary to satellite I are present in approximately equal amounts on a heterochromatic arm of the X and Y chromosomes and are also present, in smaller amounts, at the centromere of chromosome 3. A quantitative analysis of the in situ hybridisation experiments indicates that sequences complementary to satellite I at these two sites differ in their replicative behaviour during polytenisation: heterosomal satellite I sequences are under-replicated relative to chromosome 3 sequences in polytene larval salivary gland and ovarian nurse cell nuclei.     

Cytogenetics of Simulium siamense Takaoka and Suzuki, 1984 (Diptera: Simuliidae) in northeastern Thailand

We analysed salivary gland polytene chromosomes of 796 larvae from 17 populations of Simulium siamense in northeastern Thailand. Seventeen floating and two fixed chromosome inversions were recorded. Three cytoforms (A, F and G) were recognised and two of them are new (F and G). Cytoform F is distinguished by a fixed inversion on the long arm of chromosome II (IIL-8) and cytoform G by fixed inversions on the long arm of chromosome II (IIL-8) and short arm of chromosome III (IIIS-2). Significant departures from Hardy–Weinberg equilibrium due to heterozygote deficiency in geographically intermediate populations and absence of shared polymorphic inversions of the cytoforms indicate separation of the gene pool. Morphometric analysis of the larvae revealed significant differences in body length (F = 5.00, p =0.007) and head capsule width (F = 4.68, p = 0.010) among cytoforms.     

Polytene chromosomes in pupal and adult blackflies (Diptera: Simuliidae)

A number of pupal and adult tissues of eight Australian blackfly species representing three genera, Austrosimulium, Cnephia and Simulium, were examined for the presence of polytene chromosomes. Banded polytene chromosomes were found in malpighian tubules, hind gut, fat body, and ovary, but only those from the malpighian tubules of female adults and pupae were of good quality. A detailed comparison of polytene chromosomes from larval salivary glands and adult malpighian tubules was made in S. ornatipes and, to a limited extent, in S. melatum. The banding patterns of chromosomes from both tissues were found to be identical with minor differences in puffing patterns in S. ornatipes and chromocenter characteristics in S. melatum. A survey of the remaining six species shows five of them to have malpighian chromosomes suitable for detailed cytological analysis. Simultaneous studies of larval, pupal and adult polytene chromosome systems offer a novel approach to the analysis of population problems in blackflies. The ability to recognise sibling species in adults also has potential practical significance in efforts to control vectors of onchocerciasis.     

Heterochromatic chromosomes and satellite DNAs of Drosophila nasutoides

Drosophila nasutoides is distinguished from other Drosophila species in that the metaphase karyotype shows a pair of very large V-shaped chromosomes. With Giemsa, a distinctive C-banding pattern is revealed along the arms of this large chromosome, indicating a largely heterochromatic nature. Furthermore, the banding patterns of the arms are symmetrical, indicating that it is an iso-chromosome. A comparison between the metaphase karyotype and polytene chromosomes suggests that the large V chromosome appears as the dot chromosome in polytene squash. One autosome has twice the arm length of typical Drosophila polytene chromosomes and arose either by centric fusion and a pericentric inversion, or by translocation connecting distal ends with a subsequent loss of one centromere. This chromosome appears to have a short arm which ectopically pairs with the proximal region of the long arm, representing a duplication of about ten bands. When the nuclear DNA is examined by neutral CsCl gradient, four satellites are observed. As much as sixty percent of the total DNA appears as satellites in the lysate of larval brains. No satellite was detectable in the lysate of salivary glands. These observations led us to suggest that the heterochromatic nature of the large V chromosome is due to the presence of all four satellites in this chromosome and that this large chromosome appears as the dot because of the under-reduplication of the satellites during polytenization.     

Effects of gamma-radiation on the organisation of polytene chromosomes ofGlyptotendipes salinus Michailova (Chironomidae,Diptera)

A series of laboratory experiments onGlyptotendipes salinus were carried out in order to assess cytogenetic effects of different doses of gamma-radiation on polytene chromosomes, isolated from salivary glands. Chrinonomid larvae (III–IV larval stage) were irradiated with doses varying from 0.05 to 1.00 Gy (5–100 rad) and were bred under laboratory conditions until the fourth larval stage. Cytogenetic slides were analyzed for an estimation of occurrence of changes in the organization of the polytene chromosomes caused by gamma-radiation. A specific heterochromatin effect was found in certain chromosomes of the investigated species after 1.00 Gy irradiation. Decondensation of the centromeric heterochromatin and increased functional activity of Balbiany ring 2 were observed in the fourth (G) chromosome. Regression of the nucleolus of the first (AB) chromosome was detected.     

Sex chromosomes and associated rDNA form a heterochromatic network in the polytene nuclei of Bactrocera oleae (Diptera: Tephritidae)

The olive fruit fly, Bactrocera oleae, has a diploid set of 2n?=?12 chromosomes including a pair of sex chromosomes, XX in females and XY in males, but polytene nuclei show only five polytene chromosomes, obviously formed by five autosome pairs. Here we examined the fate of the sex chromosomes in the polytene complements of this species using fluorescence in situ hybridization (FISH) with the X and Y chromosome-derived probes, prepared by laser microdissection of the respective chromosomes from mitotic metaphases. Specificity of the probes was verified by FISH in preparations of mitotic chromosomes. In polytene nuclei, both probes hybridized strongly to a granular heterochromatic network, indicating thus underreplication of the sex chromosomes. The X chromosome probe (in both female and male nuclei) highlighted most of the granular mass, whereas the Y chromosome probe (in male nuclei) identified a small compact body of this heterochromatic network. Additional hybridization signals of the X probe were observed in the centromeric region of polytene chromosome II and in the telomeres of six polytene arms. We also examined distribution of the major ribosomal DNA (rDNA) using FISH with an 18S rDNA probe in both mitotic and polytene chromosome complements of B. oleae. In mitotic metaphases, the probe hybridized exclusively to the sex chromosomes. The probe signals localized a discrete rDNA site at the end of the short arm of the X chromosome, whereas they appeared dispersed over the entire dot-like Y chromosome. In polytene nuclei, the rDNA was found associated with the heterochromatic network representing the sex chromosomes. Only in nuclei with preserved nucleolar structure, the probe signals were scattered in the restricted area of the nucleolus. Thus, our study clearly shows that the granular heterochromatic network of polytene nuclei in B. oleae is formed by the underreplicated sex chromosomes and associated rDNA.     

The location of 5S (ribosomal) RNA genes in Drosophila hydei

The location of the 5S ribosomal RNA cistrons in band 2-23B1,2 of the polytene (salivary gland) chromosomes of Drosophila hydei was indicated by in situ hybridization of tritiated low molecular weight RNA fractionated from total in vivo synthesized larval RNA or from in vitro synthesized salivary gland RNA and competition of the hybridization of this RNA by 5S RNA obtained from calf lens ribosomes. -- At the submicroscopic level, band 2-23B1,2 in salivary gland chromosomes shows a compact organization. The adjacent region, 23B2, is slightly puffed and displays typical RNP particles, some of which may be observed close to band 2-23B1,2.