甘蓝型油菜隐性上位互作核不育材料1665花药败育的细胞学研究

采用石蜡切片方法,对甘蓝型油菜隐性上位互作核不育材料1665的可育株与不育株花药进行细胞学观察.结果显示:(1)不育株花药在花粉母细胞减数分裂时期出现异常,部分花粉母细胞细胞分裂相不均等分裂或分裂异常.导致部分四分体形状异常.(2)不育株绒毡层细胞在四分体时期开始生长膨大,单核花粉时期出现液泡化和巨型化,侵占药室,使得小孢子不能正常释放或无法继续发育;部分释放出的小孢子未及时形成花粉壁,阻碍花粉继续发育.不能发育形成二核期和三核期花粉,导致花药败育.     

在常温和低温条件下离体培养的小麦花药中小孢子的早期发育

本文对小麦花药培养中雄核的早期发育作了较详细的观察。描述了小孢子发育的七种类型。前三种类型(A、A_1、A_2)小孢子第一次分裂为不等分裂,形成营养细胞和生殖细胞,营养细胞分裂形成愈伤组织、胚状体和多核花粉粒。后四种类型(B、B_1、B_2、B_3)小孢子第一次分裂为均等分裂,这样,可由小孢子直接形成愈伤组织和胚状体,它们也形成多核花粉粒。在对愈伤组织和胚状体产生的途径进行观察和分析后,发现小麦花扮植株大多数来源于均等分裂的小孢子,即为B途径发育类型。 实验中还观察到花粉发育的各种异常情况,例如,在有丝分裂不同的阶段(如前期、中期和后期)都观察到同步分裂的现象。还观察到各种类型的间期核融合(如生殖核与生殖核、生殖核与营养核以及营养核与营养核)和核内有丝分裂。通过这些方式,可以形成加倍的花粉粒和愈伤组织,由此可产生自然加倍的二倍体值株。雄核的这些行为在培养花药接种后经受低温处理(—2— 2℃或—5—0℃,48小时)的情况下,表现出明显增加的趋势。     

无丝分裂制片法

无丝分裂是一个比较复杂的变化过程。在无丝分裂早期,球形的细胞核及核仁都伸长,高尔基复合体位于伸长细胞核长轴的中线附近,并于高尔基复合体的内侧有中心体。随后,细胞核进一步伸长呈哑铃状,中央部较窄形成核颈,并在核颈部沿着细胞核长轴出现纵褶。当细胞     

玉竹雄配子的发育——着重阐明质体在生殖细胞和营养细胞中的分布和变化

玉竹(Polygonatum simizui Kitag)小孢子在分裂前,质体极性分布导致分裂后形成的生殖细胞不含质体,而营养细胞包含了小孢子中全部的质体。生殖细胞发育至成熟花粉时期,及在花粉管中分裂形成的两个精细胞中始终不含质体。虽然生殖细胞和精细胞中都存在线粒体,但细胞质中无DNA类核。玉竹雄性质体的遗传为单亲母本型。在雄配子体发育过程中,营养细胞中的质体发生明显的变化。在早期的营养细胞质中,造粉质体增殖和活跃地合成淀粉。后期,脂体增加而造粉质体消失。接近成熟时花粉富含油滴。对百合科的不同属植物质体被排除的机理及花粉中贮藏的淀粉与脂体的转变进行了讨论。     

糜子的小孢子发育和雄配子体形成

1.小孢子四分体的排列方式为左右对称形、直列式和T形。2.花粉第一次右丝分裂前夕,部分细胞质定向集中并形成细胞质索。3.有丝分裂末期出现成膜体,而后形成分开营养细胞和生殖细胞的拱形壁。4.营养核移至萌发孔,拱形壁开始消失,生殖细胞经过变形变化并进入营养细胞的细胞质。当生殖细胞完成位移并和营养核紧密贴近后,它开始分裂。5.在生殖细胞的有丝分裂过程中,其纺锤体轴的方向不止一个;细胞质分裂是产生缢缩沟。6.由     

无花粉型水稻温敏核不育系籼S的育性表现与细胞学观察

温敏核不育水稻籼S是从优质常规稻籼黄占自然突变而来的一个无花粉型光温敏核不育种质资源。在广州(23°08′N)自然条件下,一年中具有明显的“可育-不育-可育”的育性转换,5月初至10月底为稳定不育期。在人控光温条件下,低温诱导其由不育转为可育需要较长的持续时间,日均温21℃需7d以上,23.5℃需15d以上。细胞学观察表明其无花粉败育主要是由减数分裂时期的异常引起的,表现为小孢子母细胞粘连与液泡化、减数分裂受阻于前期Ⅰ的细线期、进行无丝分裂与异常的胞质分裂,始终没有正常四分体的形成,而是产生大小不同、核数不等的异常细胞,并最终解体消失。其花粉败育特点不同于以往研究过的光温敏核不育水稻,具有花粉败育时期早而败育彻底的特点。     

杜仲花粉离体萌发特征及花粉管微丝骨架分布

以干燥的杜仲成熟花粉为材料,对杜仲花粉离体萌发的适宜液体培养基配方进行了筛选,并对花粉萌发特征及花粉管微丝骨架分布规律进行了研究。结果表明:(1)适宜杜仲花粉离体萌发的液体培养基组成为200g/L蔗糖+30mg/L硼酸+10mg/L Ca(NO3)2,于26℃条件下离体培养18h的花粉萌发率可达46.29%±3.75%。(2)在适宜液体培养条件下,杜仲花粉萌发率在培养6h内急剧增长,随后趋于平稳;而花粉管在培养8h内伸长较快,之后有放缓趋势,至培养48h时,花粉管长度可达363.14±30.51μm。(3)杜仲花粉属于2胞花粉,花粉萌发过程中,营养核和生殖核的移动存在一定的时序性,通常营养核先于生殖核进入到花粉管;杜仲花粉生殖核的有丝分裂发生在花粉管中,离体培养12h可逐渐观察到有丝分裂行为。(4)花粉萌发过程,微丝骨架形成束状,与花粉管伸长方向平行排布,与较为稀疏的网状微丝阵列组成连续系统,引导细胞核的运动。     

竹节海棠叶外植体脱分化启动的细胞学观察

竹节海棠叶外植体接种于MS+6-BA1ppm+NAA0.1ppm培养基上。外植体脱分化启动过程中,表皮及叶肉细胞主要以劈裂的无丝分裂方式进行分裂:最初核延伸为纺锤形,核仁大而明显,使整个核的轮廓呈“眼”状;随着核的中部出现裂缝,核断开成为两部分,稍后,由原来的母细胞形成两个子细胞。由于核分裂前向细胞中央移动的距离及断裂时断裂面的不同,从而造成细胞团内细胞大小悬殊及分裂面严重混乱的不等分裂现象。文中对栅栏组织细胞脱分化启动后重复进行无丝分裂形成梯状细胞团的现象也进行了讨论。     

萱草幼嫩花粉原生质体培养启动细胞分裂的超微结构研究

萱草(Hemerocallis fulva L.)幼嫩花粉,即后期小孢子原生质体在培养8天时进入有丝分裂或已形成二个细胞。此外,还观察到游离核分裂、无丝分裂、微核形成等现象。这显示了花粉原生质体分裂方式的多样性。在启动分裂时发生一系列变化:如细胞核移位、大液泡消失、细胞质电子密度增加、细胞器增多、质体不含淀粉等。再生的细胞壁含许多小泡,很少纤丝,表现出现有培养条件下壁的形成能力薄弱。这是今后改进培养技术需要特别注意的问题。     

谈谈遗传学中若干基本问题

八、细胞有丝分裂与细胞离体培养 人们对细胞分裂的认识,开始时只看到它有“直接分裂”与“间接分裂”。直接分裂的例子再没有比原生动物纤毛虫的大核(营养核)的分裂为最典型的了。间接分裂后改称为有丝分裂,因为这种分裂总伴随着纺锤体的形成,而纺锤体上的微管束在光学显微镜下观察固定后的切片标本都呈显为丝线状,由此这种分裂就     

Suspension Culture of Endosperm Callus Cell and Amitosis In Vitro

The endosperm calli were induced on MS basic medium supplemented with lppm 2,4-D, 0.5ppm KT and 5% sucrose. The medium which contained lppm BAP, 0.1ppm NAA and 2% sucrose was used for cell suspension culture. In suspension cell culture, amitosis of cleavage division of nucleus have been observed after 5 days of culture. First the nuclear membrane and nucleolus disappeared. The crevice appeared in the center of the nucleus, and the nucleus divided into two daughter nuclei of similar size and each with a nucleolus. The daughter nucleus resembled an eye in shape. Following the emergence of cell wall, the two new unequal cells were produced. Such amitotic division proceeded repeatedly until the callus developed and eventually plantlet regenerated.     

Mitosis and Amitosis of Generative Cell Nuclei in Artificially Germinated Pollen Tubes in Zephyranthes candida(Lindl.)Herb.

This paper deals with the comportmem of the vegetative nucleus and its spatial association with the generative cell and sperm cells in the artificially germinated pollen tubes of Zephyranthes candida (Lindl.) Herb. before and after generative cell mitosis with the use of DNA-specific fluochrome 4′,6-diamidino-2-phenylindole (DAPI). The induction of amitosis and abnormal mitosis of generative cell nuclei by cold-pretreatment of the pollen prior to germination was studied in particular. In normal case, the generative cell, after appressing to the vegetative nucleus for certain time, underwent mitosis to form two sperms, while the vegetative nucleus became markedly elongated, diffused, and exhibited blurring of its fluorescence. After division, a pair of sperms remained shortly in close connexion with the vegetative nucleus. Then the vegetative nucleus returned to its original state. In the pollen tubes germinated from cold-pretreated pollen, amitosis of some generative cell nuclei were frequently observed. Amitosis took place via either equal or unequal division with a mode of constriction. During amitosis, the dynamic change of vegetative nucleus and its intimate association with generative cell afore described did not occur. Sperm nuclei produced from amitosis could farther undergo amitisis resulting in micronnclei. Factors affecting the amitosic rate of generative cells, such as pollen developmental stage, temperature and duration of cold-pretreatment, were studied. Besides amitosis, cold-pretreatment also induced some abnormal mitotic behavior leading to the formation of micronuclei. Based on our observations and previously reported facts in other plant materials, it is inferred that the vegetative nucleus plays an important role in normal mitosis of generative cell and development of sperms.     

An Ultrastructural Study on Triggering of Cell Division in Young Pollen Protoplast Culture of Hemerocallis fulva L.

The ultrastructural changes of young pollen protoplasts under culture condition in Hemerocallis fulva were studied. In comparison with the original pollen grains, the pollen protoplasts had been completely deprived of pollen wall, but kept the internal structure intact, including a large vacuole, a thin layer of cytoplasm and a peripherally located nucleus. After 8 days of culture a few pollen protoplasts were triggered to cell division: some of them were just undergoing mitosis with clearly visible chromosomes and spindle fibers; the others already divided into 2-celled units. The two daughter cells were equal or unequal in size but with similar distribution of organelles inside. Besides cell division, there were also free nuclear division, amitosis and formation of micronuclei indicating a diversity of division modes in pollen protoplast culture, A series of changes occurred during the process of induction of cell division, such as locomotion of the nucleus toward the central position, disappearence of the large vacuole, increase of electron density of cytoplasm, increase and activation of organelles, diminishing of starch granules in plastids, etc. However, the regeneration of surface wall was not sufficient it contained mostly vesicles with only a few microfibrits. The wall separating the two daughter cells were either complete or incomplete. The weak capability of wall formation is supposed to be one of the major obstacles which has so far restricted sustained cell divisions of young pollen protoplasts under current culture condition.     

Ultrastructural study on mitosis and cytokinesis in Scytosiphon lomentaria zygotes (Scytosiphonales,Phaeophyceae) by freeze-substitution

Summary. The ultrastructure of mitosis and cytokinesis in Scytosiphon lomentaria (Lyngbye) Link zygotes was studied by freeze fixation and substitution. During mitosis, the nuclear envelope remained mostly intact. Spindle microtubules (MTs) from the centrosome passed through the gaps of the nuclear envelope and entered the nucleoplasm. In anaphase and telophase, two daughter chromosome masses were partially surrounded with endoplasmic reticulum. After telophase, the nuclear envelope was reconstructed and two daughter nuclei formed. Then, several large vacuoles occupied the space between the daughter nuclei. MTs from the centrosomes extended toward the mid-plane between two daughter nuclei, among the vacuoles. At that time, Golgi bodies near the centrosome actively produced many vesicles. Midway between the daughter nuclei, small globular vesicles and tubular cisternae accumulated. These vesicles derived from Golgi bodies were transported from the centrosome to the future division plane. Cytokinesis then proceeded by fusion of these vesicles, but not by a furrowing of the plasma membrane. After completion of the continuity with the plasma membrane, cell wall material was deposited between the plasma membranes. The tubular cisternae were still observed at the periphery of the newly formed septum. Microfilaments could not be observed by this procedure. We conclude that cytokinesis in the brown algae proceeds by fusion of Golgi vesicles and tubular cisternae, not by a furrowing of the plasma membrane. Received September 12, 2001 Accepted November 12, 2001     

The cytoskeletal involvement in cellularization of theDrosophila melanogaster embryo

Summary The distribution and arrangement of cytoskeletal components in the early embryo ofDrosophila melanogaster were examined by thin-section electron microscopy to elucidate their involvement in the formation of the cellular blastoderm, a process called cellularization. During the final nuclear division in the cortex of the syncytial blastoderm bundles of astral microtubules were closely associated with the surface plasma membrane along the midline where a new gutter was initiated. Thus the new gutter together with the pre-formed ones compartmentalized the embryo surface to reflect underlying individual daughter nuclei. Subsequently such gutters became deeper by further invagination of the plasma membrane between adjacent nuclei to form so-called cleavage furrows. Nuclei simultaneously elongated in the direction perpendicular to the embryo surface and numerous microtubules from the centrosomes ran longitudinally between the nucleus and the cleavage furrow. Microtubules often appeared to be in close association with the nuclear envelope and the cleavage furrow membrane. The plasma membrane at the advancing tip of the furrow was always undercoated with an electron-dense layer, which could be shown to be mainly composed of 5–6 nm microfilaments. These microfilaments were decorated with H-meromyosin to be identified as actin filaments. As cleavage proceeded, each nucleus with its perikaryon became demarcated by the furrow membrane, which then extended laterally to constrict the cytoplasmic connection between each newly forming cell and the central yolk region. The cytoplasmic strand thus formed possessed a prominent circular bundle of microfilaments which were also decorated with H-meromyosin and bidirectionally arranged, similar in structure to the contractile ring in cytokinesis. These observations strongly suggest that both microtubules and actin filaments play a crucial role in cellularization ofDrosophila embryos.     

土麦冬离体萌发花粉管中生殖细胞与营养核的动态变化

主要报道了土麦冬人工培养萌发花粉管中生殖细胞与营养核的动态变化。多数花粉管中,生殖细胞与营养核贴合后,开始进行有丝分裂,贴合时,营养核略呈弥散状态。在分裂早中期,生殖细胞与营养核分开,从贴合到分开大约经历３－５ｈ,精子形成后,不与营养核连接。ＤＡＰＩ对生殖细胞的有丝分裂有抑制作用。少数花粉管中,生殖细胞核进行无丝分裂,有缢裂和劈裂两种方式。生殖细胞核发生缢裂的花粉管中,未观察到生殖细胞与营养核的贴     

Removal of cellular water prevents the reformation of the interphase nucleus

The mature snRNP (small nuclear ribonucleoprotein) particles are localized quantitatively in the interphase nucleus. Like many nuclear antigens, they distribute throughout the cytoplasm after the nuclear envelope breaks down during mitosis and then return to the newly formed daughter nuclei in early G1. Their abundance and stability and the availability of monoclonal antibodies that recognize them, make the snRNP particles a useful model system for studying the reformation of the nucleus at the completion of mitosis. A wide variety of metabolic inhibitors and alterations in normal culture conditions were investigated for their ability to interfere with the return of the snRNP particles to daughter nuclei after mitosis. None of the well-characterized cytoskeletal inhibitors, biosynthetic inhibitors, calcium antagonists, nor ionophores were effective in interfering with this return. However, the removal of cellular water by exposure of cells to hypertonic medium during mitosis blocked the reformation of the nucleus and trapped the snRNP particles in the cytoplasm. In medium of twice the normal tonicity, the function of the mitotic spindle and the cleavage furrow are inhibited, however, the cells reattach to the substratum as if returning to interphase. The chromatin stays condensed and does not form a normal interphase nucleus and the snRNP particles stay dispersed throughout the cytoplasm. This condition is reversible and after return to normal medium the nucleus reforms and the snRNP particles collect in the new nuclei. After gentle extraction of metaphase cells, about 30% of the snRNP particles are soluble, however, the remainder are associated with an insoluble remnant. These data are consistent with the notion that the snRNP particles accumulate in the nucleus due to both preferential solubility and specific binding sites in the interphase nucleus.     

禾谷镰孢菌Fusarium graminearum Schwabe分生孢子萌发过程中的核相变化及有丝分裂过程观察

通过Giemsa染色观察禾谷镰孢菌Fusarium graminearum分生孢子萌发过程中的核相变化及有丝分裂过程。观察表明,分生孢子细胞为单核,细胞核在分生孢子细胞内分裂后进入芽管,在芽管内进行多次分裂,使芽管内细胞核数目不断变化。禾谷镰孢菌有丝分裂过程可以分为4个时期,前期染色体逐渐浓缩变短,中期染色体清晰可见,后期染色单体发生分离并向相反的两极移动,末期形成新的子核。有丝分裂过程中染色体的分离同步或不同步,不同步分离中的滞后染色体形成后期桥的现象更为普遍。     

Mitosis and autospore formation in the green algaKirchneriella lunaris

Summary Asexual reproduction inKirchneriella lunaris involves autospore formation. After an initial mitosis, the curved cell cleaves to a variable extent, and then the nuclei divide again; finally the cytoplasm is partitioned into four around each nucleus. Rudimentary centrioles appear prior to the first mitosis; centriole complexes then become associated with a developing sheath of extranuclear microtubules at prophase; fenestrae appear at the poles through which both microtubules and centrioles migrate, preceding intranuclear spindle formation. The nucleus meanwhile is enveloped by a perinuclear layer of endoplasmic reticulum which is also interposed between the golgi body and nuclear envelope. Chromosome separation is accompanied by considerable spindle elongation. Finally the reforming nuclear envelope excludes both centriole complex and interzonal spindle apparatus from daughter nuclei. Cleavage is preceded by i) nuclear movement to the cell center, ii) movement of centriole complexes around daughter nuclei until they are opposite one another, and iii) the concurrent formation of a system of transverse microtubules extending across the cell. Other microtubules encircle the cell predicting the cleavage plane. A septum then appears amongst these cytokinetic microtubules, possibly derived from the plasmalemma; it extends across the cell too, through the cleaving peripheral chloroplast. Secondary mitoses follow (as above) during which this septum may be partially resorbed. Finally this septum is reformed, if necessary, and two other septa appear (as above) to quadripartition the cell. Mitotic and cytokinetic structures in this algae are briefly compared with some others.     

Mitosis in the dermatophyteMicrosporum canis as revealed by freeze substitution electron microscopy

Summary Mitosis in the dermatophyteMicrosporum canis was studied by freeze substitution and electron microscopy, and analyzed by three dimensional reconstruction from serial sections of the mitotic nuclei. The interphase nucleus has associated nucleus-associated organelle (NAO) on a portion of the outer surface of the nuclear envelope, subjacent to which there was dense intranuclear material. The NAO divided and separated on the envelope, and a spindle was formed. The spindle was composed mostly of microtubules extended between opposite NAOs. Pairing of kinetochores was observed in the spindle from an early stage of development, when chromosomes were not so condensed, and remained unchanged while chromosome condensation proceeded until metaphase. Before the completion of nuclear division, daughter nuclei were connected by a narrow spindle channel, and then the nucleolus, whose structure underwent minimal change during mitosis, was eliminated into the cytoplasm.