共查询到20条相似文献,搜索用时 109 毫秒
1.
2.
白花紫露草(Tradescantia fluminensis),属于鸭跖草科,是一种观赏叶子的盆景植物,俗名也叫吊兰。我们发现它是生物教学中可供多种实验的好材料。如细胞质环流、质壁分离及复原、细胞核和核仁及叶绿体等的观察。同时,它容易栽培,繁殖快,一年四季均可生长,加之某些部位不含叶绿体而便于观察。细胞质环流的观察取雄蕊毛或表皮毛3—5条,放在滴有清水的载片上,加盖片后,先低倍后高倍镜观察,效果十分理想。质壁分离的观察环流实验完成后,在盖片的一侧滴蔗糖溶液,另一侧用吸水纸吸引,不久将会出现质壁分离现象。细胞核和核仁的观察叶表皮细胞活体观察或染 相似文献
3.
4.
5.
6.
采用体外渗透和显微注射的方法。将植物微管特效解聚剂甲基氨草磷(APM)引入紫露草雄蕊毛细胞后,发现原来沿着胞质束运动的胞质颗粒运动速度渐慢,进而胞质束消失,颗粒运动停止。显微注射后,还发现APM可通过胞间通道由被注射的细胞向两侧细胞扩散,从而也导致两侧细胞胞质束消失,颗粒运动停止。APM对胞质环流的抑制作用是可逆的。结果表明微管可能是胞质束的重要组份之一,植物胞质环流与微管的聚合与解聚状态有密切关系。 相似文献
7.
苦草属植物体外部形态相似,叶线行或带形,野外难以直接鉴定到种,而雄花雄蕊数目、果实和种子的显微结构是苦草属(Vallisneria)植物物种的鉴别性特征之一。苦草属物种的雄花小,仅有1.5 mm,人工解剖雄花观察方法难以实现雄花雄蕊数目的识别;本研究采用雄株雄佛焰苞水培预培养技术获取自然开放的雄花并利用解剖学显微镜对3种苦草属植物雄花、果实和种子进行了解剖观察和研究。显微结构观察表明,苦草(V. natans)雄蕊1枚,果实圆柱形,表面光滑,种子无翅,具纵条纹;刺苦草(V. spinulosa)雄蕊2枚,果实三棱形,棱上具刺,种子具翅;密刺苦草(V. denseserrulata)雄蕊2枚,果实三棱圆柱形,表面光滑,种子无翅。依据文献,密刺苦草、刺苦草、长梗苦草(V. longipedunculata)和安徽苦草(V. anhuiensis)是安徽苦草属新分布记录种,其中长梗苦草和安徽苦草是分布于安徽的新种。 相似文献
8.
花药壁及其中绒毡层的结构与功能 总被引:4,自引:0,他引:4
花药壁及其中绒毡层的结构与功能牛佳田(黑龙江省佳木斯师范专科学校154007)被子植物的花药壁是指雄蕊花药中药室外面由抱子体性质的几层细胞所组成的壁结构。分化至完全的花药壁从外至内依次是表皮、药室内壁(成熟后分成纤维层和唇细胞)、中层、绒毡层。花药壁... 相似文献
9.
两种纤毛虫营养细胞和休眠细胞蛋白组成的比较分析 总被引:1,自引:0,他引:1
应用生化抽提和SDS-PAGE方法显示,膜状急纤虫(Tachysoma pellionella)的营养细胞含38条蛋白谱带,休眠细胞含29条蛋白谱带,两者共有谱带为26条,特有谱带各为12条和3条,相似度为77.6%;休眠细胞的包囊壁含22条蛋白谱带,细胞脱包囊后残留的包囊壁含15条蛋白谱带,两者共有谱带为14条,特有谱带各为8条和1条,相似度为76%。包囊游仆虫(Euplotes encysticus)的营养细胞和休眠细胞均含23条蛋白谱带,两者共有谱带为19条,特有谱带各为4条,相似度为82.6%;休眠细胞的包囊壁和细胞脱包囊后残留的包囊壁均含20条蛋白谱带,两者共有谱带为19条,特有谱带均为1条,相似度为95%。结果表明,两种纤毛虫的营养细胞向休眠细胞转化过程中,细胞结构的主要蛋白质成分发生了明显变化,这些变化与细胞在不同生理状态下结构的分化及其生命活动特征相关。形成“毛基体吸收型包囊”的急纤虫与形成“毛基体非吸收型包囊”的游仆虫相比较,前者营养期和休眠期细胞蛋白组成有更明显的差异,这可能与其细胞结构更大程度的脱分化有关;根据纤毛虫休眠细胞的包囊壁和细胞脱包囊后残留的包囊壁两者蛋白组成的差异推测,前者包囊壁可能含有与休眠细胞生命活动相联系的“活性”成分。 相似文献
10.
采用“外类群对比准则”(OutgroupComparisonCriteria,Carcarft1983)的性状分析方法,对我国特有植物四棱草属Sohnabelia及其近缘属筋骨草属Ajuga,香科科属Teucrium(唇形科)和莸属Caryopteria大青属Clerdendron(马鞭草科)等5属6种主要植物比较研究,首次发现在这些植物叶片上,具有一种新的毛状体,其形状呈箭形,故定名为箭形毛(Arrow—shaped—hair),在扫描电子显微镜下观察是由头部、柄部和基部组成,在光学显微镜下,确认这类毛状体属于多细胞单列毛,由细胞变形而成形。此外,尚有长柔毛(Shag-hair),盾状毛(Peltate—hair)和鳞片毛(Scales—hair)等四种类型。从以上毛状体的微形态特征及其演化规律,作者认为四棱草属和近缘属在唇形科与马鞭草科系统演化框架里,可能是处于中间过渡类型。 相似文献
11.
Under both separate and combined influence of 232nd-nitrate and potassium nitrate a study was made of the yield of somatic mutation frequencies, the level of morphologically abnormal cells and the loss of reproduction integrity in the stamen hairs of Tradescantia (clone 02). All investigated concentrations of 232nd-nitrate and potassium nitrate exerted statistically significant genotoxic effects and increased the level of morphological cell abnormalities in the stamen hairs of Tradescantia. Also, 0.36 mg/l 232nd and 0.51 mg/l KNO3 concentrations cause a statistically significant loss of reproduction integrity in the stamen hair. The combined action of 232nd-nitrate and potassium nitrate in all investigated concentrations and parameters causes a statistically significant effect. 相似文献
12.
Mutant sectors in stamen hairs of Clone 02 Tradescantia are designated as "multiple sectors" when two or more occupy the same hair, separated by non-mutant cells. Statistical analyses show that most multiple sectors do not arise as chance associations of independent events: when the frequency of stamens with two or more sectors is lowest, the probability that the sectors will be located in the same, rather than in different, hairs is highest. Ontogenetically, the ratio of sector pairs in different hairs to pairs in the same hair is highest in that period of response to acute irradiation prior to the appearance of entire-hair sectors; thereafter, the ratio subsides, approaching that of spontaneous mutation and indicating that the initiating event takes place early in hair development. Most mononemic chromosome models will not account for the production of multiple mutant and non-mutant sectors, dispersed along a linear structure such as a stamen hair, following a single mutational event. Consideration is given to two models (one mononemic, and the other dinemic) which will readily provide the possibilities for either the immediate segregation of mutant and non-mutant cells, or for the perpetuation in daughter nuclei of a "heterozygous" chromosome capable of segregation at some later mitosis. The dinemic model is preferred because it affords operation of the mutation mechanism (including breakage and deletion) at either the DNA molecule or subunit level. 相似文献
13.
H P Leenhouts M J Sijsma A Cebulska-Wasilewska K H Chadwick 《International journal of radiation biology and related studies in physics, chemistry, and medicine》1986,49(1):109-119
The induction of somatic mutations in the stamen hair cells of Tradescantia KU 9 has been used to investigate the effects of combined exposure to 1,2-dibromoethane (DBE) and X-rays. At low radiation doses a synergistic interaction has been found between the two agents for both DBE exposure followed by acute X-rays and chronic simultaneous exposures. The synergism is discussed in terms of an interaction of single strand lesions in the DNA. It is concluded that although this type of interaction should not be too important for radiological protection, it could be of significance in evaluating the effects of chemicals at low exposure rates. 相似文献
14.
Fluorescently-labeled fimbrin decorates a dynamic actin filament network in live plant cells 总被引:8,自引:0,他引:8
Recently it has been established, through a detailed biochemical analysis, that recombinant Arabidopsis thaliana fimbrin 1 (AtFim1) is a member of the fimbrin/plastin family of actin filament bundling or cross-linking proteins [D.R. Kovar et al. (2000) Plant J 24:625-636]. To determine whether AtFim1 can function as an F-actin-binding protein in the complex environment of the plant cell cytoplasm, we created a fluorescent protein analog and introduced it by microinjection into live Tradescantia virginiana L. stamen hair cells. AtFim1 derivatized with Oregon Green 488 had biochemical properties similar to unlabeled fimbrin, including the Kd value for binding to plant F-actin and the ability to cross-link filaments into higher-order structures. Fluorescent-fimbrin decorated an array of fine actin filaments in the cortical cytoplasm of stamen hair cells, which were shown with time-course studies to be highly dynamic. These data establish AtFim1 as a bona fide member of the fimbrin/plastin family, and represent the first use of a plant actin-binding protein as a powerful cytological tool for tracking the spatial and temporal redistribution of actin filaments in individual cells. 相似文献
15.
The cell plate is the new cell wall, with bordering plasma membrane, that is formed between two daughter cells in plants, and it is formed by fusion of vesicles (approximately 60 nm). To start to determine physical properties of cell plate forming vesicles for their transport through the phragmoplast, and fusion with each other, we microinjected fluorescent synthetic lipid vesicles that were made of 1,2-dioleoyl-sn-glycero-3-[phospho-rac-(1-glycerol)] (DOPG) into Tradescantia virginiana stamen hair cells. During interphase, the 60-nm wide DOPG vesicles moved inside the cytoplasm comparably to organelles. During cytokinesis, they were transported through the phragmoplast and accumulated in the cell plate region together with the endogenous vesicles, even inside the central cell plate region. Because at this stage microtubules are virtually absent from that region, while actin filaments are present, actin filaments may have a role in the transport of vesicles toward the cell plate. Unlike the endogenous vesicles, the synthetic DOPG vesicles did not fuse with the developing cell plate. Instead, they redistributed into the cytoplasm of the daughter cells upon completion of cytokinesis. Because the redistribution of the vesicles occurs when actin filaments disappear from the phragmoplast, actin filaments may be involved in keeping the vesicles inside the developing cell plate region. 相似文献
16.
Electron micrographs of staminate hair cells of Tradescantia reflexa indicate that early prophase chromosomes are composed of a number of helically arranged chromonemata. Favorable preparations reveal as many as 64 identifiable subsidiary strands, assumedly arranged as intertwined pairs to form a hierarchy of pairs of pairs. The helices of the smallest discernible units have a diameter of about 125 A, with highly electron-scattering material disposed peripherally around a less dense "core." The wall of this peripheral ring has a thickness of about 40 A, and apparently represents another pair of coiled threads surrounding a 40 A central axis. The implications of the findings are discussed briefly. 相似文献
17.
We have taken soil samples from two sites in Prague, the capital of the Czech Republic, that are heavily polluted by motor vehicles. As a negative control, soil samples from a recreational site in Prague with no motor vehicle traffic were used. Soil samples from these sites were extracted with water or 5% dimethylsulphoxide (DMSO) for 24 h and cuttings of Tradescantia clone 4430 were immersed for 12 h at 25 degrees C in the extraction solutions. As a positive control Tradescantia plants have been treated with the promutagenic arylamine o-phenylenediamine at the same treatment conditions. None of the tested soil extractions significantly increased the frequency of somatic mutations in the stamen hair assay. By contrast, a 5% DMSO soil extract from one of the tested sites (entrance of the Letná tunnel) significantly increased the frequency of micronuclei (MNC) in the pollen mother tetrad cells. A repetition of the treatment 14 days later also resulted in an increase in the frequency of MNC, however the increase was not statistically significant. This study was conducted for the International Programme on Plant Bioassays. 相似文献
18.
Inositol 1,4,5 trisphosphate [Ins(1,4,5)P3] is produced from the hydrolysis of phosphatidylinositol 4,5 bisphosphate, and as part of a second-messenger signal transduction mechanism, induces release of Ca2+ from internal stores in both plant and animal systems. It is less well established how the active Ins(1,4,5)P3 is inactivated. Studies in animal cells have demonstrated two separate metabolic pathways. Ins(1,4,5)P3 can be hydrolyzed by a 5-phosphatase or phosphorylated by a 3-kinase, resulting in the formation of Ins(1,4)P2 and Ins(1,3,4,5)P4, respectively, neither of which is able to mobilize intracellular Ca2+. Plant cell extracts have been reported to have hydrolytic and kinase activities that produce Ins(1,4)P2, and Ins(4,5)P2 and Ins(1,4,5,6)P4 from Ins(1,4,5)P3. These results offer little insight into the enzyme activities in the intact plant cell since the observed activities might be confined to intracellular compartments that have little if any impact on the signaling events within the cytosol that require Ins(1,4,5)P3. To resolve the mechanism of Ins(1,4,5)P3 inactivation, we microinjected stamen hair cells of Tradescantia virginiana L. with nonhydrolysable analogs of Ins(1,4,5)P3 that have been previously shown to cause Ca2+ release from intracellular stores. Our results indicate a sustained cytosolic [Ca2+] increase when cells were injected with the 5-phosphatase-insensitive 5-monophosphorothioate derivative of Ins(1,4,5)P3, in contrast to a brief transient when injected with the 3-kinase-insensitive 3-fluoro-3-deoxy Ins(1,4,5)P3 analog. We conclude that the 5-phosphatase pathway is the preferred pathway for Ins(1,4,5)P3 inactivation in the stamen hair cells of Tradescantia. 相似文献
19.
Tests have shown plant bioassays to be excellent for mutagenicity studies. Most studies with plant bioassays, however, have been carried out either in the laboratory, or if, in situ, as monitors of atmospheric contaminants. The primary purpose of this study was to assess the utility of in situ plant mutagenicity bioassays in monitoring water contaminants. The assay systems tested were the Tradescantia stamen hair and micronucleus assays for the detection of gene mutations and chromosomal aberrations respectively, and the Vicia faba bioassay system which detects chromosomal aberrations in root tips. The assays were used to test the effluent from a pulp and paper mill located on the north shore of Lake Superior. Assays were performed in a creek containing raw effluent and in the bay of Lake Superior into which the creek emptied. All in situ treatments were carried out for 24 h. The effluent from the creek was heavy with pulp and debris which coated the plant cuttings and the Vicia faba seedlings and may have restricted the uptake from the effluent. In the creek, at test sites 11.5 km from the source, the effluent was toxic to the Vicia faba roots as evidenced by a reduction in the mitotic index. The data for the Tradescantia stamen hair assay in the creek were equivocal. The cuttings from the creek test sites and the air and water control sites appeared to have undergone a physiological delay. Within a day or two after the return to the laboratory, that is 6-8 days after testing, flowering almost ceased and did not fully resume until about day 35. This reduction in flowering was particularly severe with the cuttings from the effluent and air control sites, making it very difficult to interpret the results. In contrast, the Tradescantia micronucleus and Vicia faba chromosomal aberration data were unequivocal; each produced positive responses at both test sites relative to the air and water controls. The results obtained for the bay sites with all 3 assays were in agreement. In that section of the bay visibly contaminated by the creek effluent, increases in stamen hair mutants, micronuclei, and chromosome aberrations were measured. In general, there was a considerable reduction in the number of mutant events observed for the water samples brought back from the test sites and tested in the laboratory.(ABSTRACT TRUNCATED AT 400 WORDS) 相似文献
20.
Anaphase in dividing guard mother cells of Allium cepa and stamen hair cells of Tradescantia virginiana consists almost entirely of chromosome-to-pole motion, or anaphase A. Little or no separation of the poles (anaphase B) occurs. Anaphase is reversibly blocked at any point by azide or dinitrophenol, with chromosome motion ceasing 1-10 min after application of the drugs. Motion can be stopped and restarted several times in the same cell. Prometaphase, metaphase, and cytoplasmic streaming are also arrested. Carbonyl cyanide m-chlorophenyl hydrazone also stops anaphase, but its effects are not reversible. Whereas the spindle collapses in the presence of colchicine, the chromosomes seem to "freeze" in place when cells are exposed to respiratory inhibitors. Electron microscope examination of dividing guard mother cells fixed during azide and dinitrophenol treatment reveals that spindle microtubules are still present. Our results show that chromosome-to-pole motion in these cells is sensitive to proton ionophores and electron transport inhibitors. They therefore disagree with recent reports that anaphase A does not require a continuous supply of energy. It is possible, however, that anaphase does not directly use ATP but instead depends on the energy of chemical and/or electrical gradients generated by cellular membranes. 相似文献