玉米单染色体的分离和体外扩增

建立了玉米单染色体的分离及体外扩增的方法。取95％乙醇固定后经果胶酶和纤维酶酶解的根尖制备染色体标本,用自制的微细玻璃针在倒置显微镜下挑取目的染色体。染色体DNA经Sau3A酶切后与人工合成的Sau3A连接接头连接,经两次PCR扩增获得足以用于构建单染色体DNA文库的扩增产物。片段大小为0．3～5kb,多数为0．5～3．5kb．与前人研究方法相比,所需底物量少（只需1条染色体）,扩增片段大,为植物中小型染色体分离、体外扩增进而进行单染色体DNA文库构建奠定了基础。     

锦鸡儿属植物一些种类的染色体数目及核型研究

报道了国产10种锦鸡儿的染色体数目,并对其中9种的核型进行了研究。这9个种的核型公式分别为：荒漠锦鸡儿（Caragana roborovskyi）,2n＝16＝10m(2SAT)+6sm;川西锦鸡儿（C. erinacea）,2n=16=10m+6sm;密叶锦鸡儿（C. densa）,2n=16=10m（2SAT）+6sm;刺叶锦鸡儿（C. acanthophylla）,2n=16=12m+4sm;柄荚锦鸡儿（C. stipitata）,2n=16=10m+6sm;甘蒙锦鸡儿（C. opulens）,2n=16=12m(2SAT)+4sm;白皮锦鸡儿（C. leucophloea）,2n=32=22m(4SAT)＋10sm;北疆锦鸡儿（C. camilli-schneideri）,2n=32=20m(4SAT)+12sm;中亚锦鸡儿（C. tragacanthoides）,2n=32=20m(2SAT)+10sm+2st+2B。白毛锦鸡儿（C.licentiana）2个居群的染色体数目均为2n=32,为四倍体。研究结果表明,锦鸡儿属的核型一般比较对称,核型上的特化往往与其形态上的特化相关联,但也有例外。从倍性水平上来看,二倍体类群多是一些羽状叶的种,在分布上倾向于亚洲东部其祖先分布区,而四倍体的种类多是一些假掌状叶的类群,分布于西部干旱生境中,在形态上也表现的较为特化。这也符合锦鸡儿属的演化趋势。     

小麦体细胞再生株（R1）的染色体变异分析

本文研究了普通小麦(Triticum aestivum)、“宁麦三号”等5个基因型的体细胞再生株(R_1)减数分裂各期的染色体异常行为。结果表明:再生株 R_1代有丝分裂时表现为染色体数量上的变异,最常见的有2n-2类型,其次是2n-1类型,也有少数为2n 1和2n-4等变异类型;再生株 R_1花粉母细胞减数分裂过程中出现单价体、多价体、染色体桥、落后染色体、断片和微核等异常现象,并与各基因型细胞遗传程度上差异有关。     

黑松,马尾松及其杂种的核型比较

分析了黑松、马尾松及其杂种的核型。其核型公式：黑松为Ｋ（２ｎ）＝２４－２０ｍ（６＿（ＳＡＴ）））＋４ｓｍ;杂种为Ｋ（２ｎ）＝２４＝２３ｍ＋１ｓｍ;马尾松为Ｋ（２ｎ）＝２４－２４ｍ（４＿（ＳＡＴ））。相对长度和臂比方差分析表明,两亲本和杂种差异显著。杂种在相对长度、全组染色体总长、最长与最短染色体比、臂比平均值以及染色体类型上均处于双亲之间。这些研究结果为进一步研究该天然杂种提供必要的细胞学资料。     

东北产苍术属植物的细胞学研究

报导了中国东北产三种苍术属植物的核型资料,核型公式分别为;北苍术「Ａｔｒａｃｔｙｌｏｄｅｓ ｃｈｉｎｅｎｓｉｓ（ＤＣ．）Ｋｏｉｄｚ．」Ｋ（２ｎ）＝２４＝１２ｍ＋６ｓｍ＋６ｓｔ（４ＳＡＴ）,关苍术「Ａ．ｊａｐｏｎｉｃａ Ｋｏｉｄｚ．」（２ｎ）＝２４＝１４ｍ＋１０ｍ（２ＳＡＴ）朝鲜苍术「Ａ．ｋｏｒｅａｎａ（Ｎａｋａｉ）Ｋｉｔａｍ．」Ｋ（２ｎ）＝２４＝１０ｍ＋１４ｓｍ（２ＳＡＴ）,三者核型对称性均为２Ｂ     

小鼠生精细胞染色质与染色体构筑的扫描电镜研究(简报)

正常情况下,染色质和染色体在细胞内呈高度致密状态,在光镜和透射电镜下常呈浓染的斑块状。由于方法学上的困难,至今对染色质乃至染色体的微细结构,仍缺乏清楚的了解。特别是关于染色质如何凝缩形成染色体方面,现仍存在有争论。扫描电镜的冷冻割断技术,曾被用于对游离细胞间期核染色质的观察,并取得了较好的     

国产七种和一变种兰属植物的核型研究

对国产7种和1变种兰属植物,即邱北冬蕙兰Cymbidium qiubeiense、春兰C. goeringii、春剑 C．longibracteatum、线叶春兰C．serratum、蕙兰C.faberi、送春C.fabri var．szechuanicum、寒兰C．kanran、莎 叶兰C．cyperifolium 的核型进行了研究。具体结果如下：邱北冬蕙兰为2n=40=24m+12sm+4st;蕙兰为2n=40=30m+8sm+2st;送春为2n=40=26m+l0sm+4st;寒兰为2n=40=26m+12sm+2st;莎叶兰为2n=40=24m+12sm+4st;春兰为2n=40=24m+l0sm+4st+2t;春剑为2n=40=24m+l0sm+6st。线叶春兰为2n=40=28m+l0sm+2st。线叶春兰中偶尔发现染色体数有2n=41,43,60,80。     

串叶松香草的核型研究

串叶松香草Silphiura perfoliatum L.系菊科(Compositae)松香草属(SilphiumL.)多年生宿根草本植物,原产北美洲。1979年由中国科学院植物研究所北京植物园首次从朝鲜引进我国,1980年引种我所栽培,通过几年的试验观察表明:串叶松香草是一种高产、质优、适应性强的饲料作物,近年来,我省广泛发展和应用。据文献报     

Cytological analysis of complex-heterozygotes in populations ofOenothera grandiflora (Onagraceae) in Alabama

Genetic analysis of unusual complex-heterozygous genotypes in populations ofO. grandiflora from Alabama (USA) has shown that these strains are composed of a typicalgrandiflora (B) complex and an altered B complex (designated as B^A) which probably contains genetic elements derived from an A genotype such as the beta complex ofO. biennis group 1. Analysis of the meiotic configurations of artificial hybrids between the new strains and a series of complexes of known segmental arrangement allowed determination of the arrangements of the unknown complexes. These data are evidence for origin of the altered B complexes.     

Microfluorimetric analysis of dynamics of genomic changes in Chinese hamster fibroblasts CHL V-79 RJK with multiple drug resistance

Results of a karyological analysis of cells CHL V-79 RJK selected for their resistance to ethidium bromide (EB) causing multidrug resistance (MDR) (subline Vebr-5) were compared with data from the microfluorimetric determination of the DNA content in individual chromosomes of the karyotype. The analysis was performed at the 11th and 88th passages. Karyotyping of Vebr-5 has shown the presence of an additional genetic material (AGM) in the form of homogenously or differentially stained regions (HSR or DSR, respectively) in two chromosomes (Z1 and Z6, loci 1p29-31 and 1q26, respectively). HSR in Z6, in the site of localization of the mdr gene of the wild type had unstable length and structure, which is characteristic of the morphological markers of the amplification of genes of the mdr family. During the long cultivation of Vebr-5 in the presence of EB (88 passages), the instability of HSR (DSR) in Z6 increased. Results of a microfluorimetric analysis of Vebr-5 at the 11th passage have shown a statistically significant increase of the DNA content not only in chromosomes Z1 and Z6 marked by HSR (DSR), but also in three chromosomes (Z5, Z12, and Z13) that have no visual morphological changes. The corresponding analysis at the 88th passage has also revealed nonrandom changes in the DNA content in four more chromosomes, including an increase in Z14 and a decrease in chromosomes 8, Z7, and Z9. A decrease in the DNA content in chromosomes is considered to be the result of a partial loss of genetic material, while its increase is considered to be the result of its translocation and/or amplification. While the coefficient of the variation of the DNA content changes about 9% for large chromosomes, it amounted to about 26% for the small ones, indicating that small chromosomes to have a greater potential for instability than large chromosomes. The obtained data not only confirm, but also enlarge, the concept of the directions and character of the destabilization of the cell genetic apparatus in the process of neoplastic transformation due to MDR acquisition by these cells.