Staining Germinating Pollen and Pollen Tubes

Germinating pollen on stigmas and pollen tubes in styles of Antirrhinum, Brassica, Oenothera, Raphanus, Rosa, solatium and Tagetes spp. were prepared for examination as follows: The styles were fixed in ethyl alcohol-acetic acid 3:1 for 1 hr, and hydrolyzed at 60°C for 5 to 60 min (depending on the species) in 45% acetic acid. The stigma with its attached strand(s) of stigmatoid tissue was then dissected out under a stereoscopic microscope, placed in a few drops of a staining solution made by dissolving 150 mg of safranin O and 20 mg of aniline blue in 25 ml of hot 45% acetic acid. After 5-15 min in this stain, the tissue was placed in a fresh drop of stain on a microscope slide and gently squashed under a cover glass. Because of a gradual precipitation of the aniline blue component, the stain had to be filtered regularly before use. However, a staining solution could be kept at room temperature for several weeks.     

Haustorial Pollen Tubes in Fuchsia boliviana

Persistent pollen tubes have been observed in Fuchsia boliviana.It is proposed that after fertilization the pollen tube becomesan important channel conveying food materials from the surroundingtissues to the embryo. Fuchsia, pollen tubes, callosic channel, Onagraceae     

Keto Acids in Pollen and Pollen Tubes of Sesbania aegyptica

Pollen and pollen tubes of Sesbania aegyptica Pers. contain α-ketoglutaric acid, oxaloacetic acid and pyruvic acid. Changes in the keto acids have been correlated with their corresponding amino acids during different phases of germination. It is suggested that keto acids were readily turned over during the elongation of pollen tubes.     

Fullerene-Based Symmetry in Hibiscus rosa-sinensis Pollen

The fullerene molecule belongs to the so-called super materials. The compound is interesting due to its spherical configuration where atoms occupy positions forming a mechanically stable structure. We first demonstrate that pollen of Hibiscus rosa-sinensis has a strong symmetry regarding the distribution of its spines over the spherical grain. These spines form spherical hexagons and pentagons. The distance between atoms in fullerene is explained applying principles of flat, spherical, and spatial geometry, based on Euclid’s “Elements” book, as well as logic algorithms. Measurements of the pollen grain take into account that the true spine lengths, and consequently the real distances between them, are measured to the periphery of each grain. Algorithms are developed to recover the spatial effects lost in 2D photos. There is a clear correspondence between the position of atoms in the fullerene molecule and the position of spines in the pollen grain. In the fullerene the separation gives the idea of equal length bonds which implies perfectly distributed electron clouds while in the pollen grain we suggest that the spines being equally spaced carry an electrical charge originating in forces involved in the pollination process.     

Haustorial Role of Pollen Tubes

In angiosperms, the pollen tube is siphonogamous and its mainfunction is to carry the male gametes for double fertilization.In some taxa, as in Cucurbitaceae, the tube branches after enteringthe ovule, prior to fertilization. The tube may even swell andform a bulla. During post-fertilization development of the ovule,a portion of the tube may persist in the micropyle, or in theembryo sac, or in both, sometimes even in the micropyle of themature seed. Haustorial function has been presumed in a numberof taxa. In Grevillea, following fertilization, the pollen tube branchesat the micropyle, and the branches grow intercellularly intothe ovarian tissue where further branching occurs. A haustorialrole of the pollen tube is presumed from circumstantial evidence.In gymnosperms (for example, Cycas, Zamia and Ginkgo) the pollentube is nonsiphonogamous, arises from the distal (upper) poleof pollen grain, and grows laterally in the apical region ofthe nucellus. The tube branches in Cycas and Ginkgo but remainsunbranched in Zamia. These pollen tube branches are enucleate,and are not concerned with the transport of male gametes forfertilization. However, the haustorial role has been well documented.In Podocarpus, the pollen tube is siphonogamous and arises fromthe proximal (lower) pole of pollen grain. After traversingthe nucellus, the tube forms a bulla at the point of contactwith the female gametophyte, and several branches originatefrom the bulla. The pollen tube branches grow along the innersurface of the nucellus and the outer surface of the femalegametophyte. The haustorial role of the pollen tube branchesis uncertain. Procedures for convincingly demonstrating thehaustorial role of pollen tubes are discussed. Angiosperms, gymnosperms, pollen tube, bulla, fertilization, haustorial role     

Electrotropism of Nicotiana Pollen Tubes

Electrotropism of tobacco pollen tubes towards the anode wasanalysed. The threshold and saturation values for the electrotropismwere less than 50 mV mm^–1 and 200 mV mm^–1, respectively.The tropic response gradually increased with increasing durationto exposure, but no further increase in the tropic responsewas observed when exposure of the electric field was terminated.Pollen tubes growing towards the cathode had a tendency to burstin a strong electric field. These results suggest that an externallyapplied electric field acts as a motive force for electrotropismbut not as a trigger and that endogenous currents play a rolein tip growth of pollen tubes. Possible mechanisms responsiblefor the electrotropism of pollen tubes are discussed. (Received July 9, 1993; Accepted September 18, 1993)     

Cytoskeleton in Pollen and Pollen Tubes of Ginkgo biloba L.

The distribution of F-actin and microtubules was investigated in pollen and pollen tubes of Ginkgo biloba L. using a confocal laser scanning microscope after fluorescence and immunofluorescence labeling. A dense F-actin network was found in hydrated Ginkgo pollen. When Ginkgo pollen was germinating,F-actin mesh was found under the plasma membrane from which the pollen tube would emerge. After pollen germination, F-actin bundles were distributed axially in long pollen tubes of G. biloba. Thick F-actin bundles and network were found in the tip of the Ginkgo pollen tube, which is opposite to the results reported for the pollen tubes of some angiosperms and conifers. In addition, a few circular F-actin bundles were found in Ginkgo pollen tubes. Using immunofluorescence labeling, a dense microtubule network was found in hydrated Ginkgo pollen under confocal microscope. In the Ginkgo pollen tube, the microtubules were distributed along the longitudinal axis and extended to the tip. These results suggest that the cytoskeleton may have an essential role in the germination of Ginkgo pollen and tube growth.     

Fluorescence Microscopy in the Study of Pollen Grains and Pollen Tubes

Fresh pollen gains were either crushed directly in a 0.01% solution of acridine orange (0.1 M phosphate-citrate buffer, pH 5.2-5.4) or they were germinated previously in 5-25% sucrose solution (glass-distilled water of pH 5.0-6.0 with 100 ppm H₃BO₃) inside moist incubating chambers at 24-30° C. Observations and records were made by using ultraviolet or blue-violet light with suitably coupled exciter and barrier filters. When the pollen grains, tube walls or cytoplasm interfered with observation of a particular cell content, the same was either pressed or dissected out of the gain or the tube. The vegetative, generative or sperm cells as well as other protoplasmic contents, such as plastid-like bodies, lipid granules and mitochondria could be differentiated.     

Fertilizing Pollen Tubes Parasitise Ovary Wall in Grevillea

Tissue-invasive pollen tube branching occurs in an Australianshrub, Grevillea banksii R.Br. (Proteaceae). Parenchyma andphloem of the ovary wall are soon infiltrated after fertilization,by intercellular branches and the lumina of xylem elements areentered. Ovular tissues are not affected. Grevillea banksii, pollen, haustoria, ovary wall     

A Method for Staining Pollen Tubes in Pistil

A quadruple staining procedure has been developed for staining pollen tubes in pistil. The staining mixture is made by adding the following in the order given: lactic acid, 80 ml; 1% aqueous malachite green, 4 ml; 1% aqueous acid fuchsia, 6 ml; 1% aqueous aniline blue, 4 ml; 1 % orange G in 50% alcohol, 2 ml; and chloral hydrate, 5 g. Pistils are fixed for 6 hr in modified Carnoy's fluid (absolute alcohol:chloroform:glacial acetic acid 6:4:1), hydrated in descending alcohols, transferred to stain and held there for 24 hr at 45±2 C They were then transferred to a clearing and softening fluid containing 78 ml lactic acid, 10 g phenol, 10 g chloral hydrate and 2 ml 1% orange G. The pistils were held there for 24 hr at 45±2 C, hydrolyzed in the clearing and softening fluid at 58±1 C for SO min, then stored in lactic acid for later use or immediately mounted in a drop of medium containing equal parts of lactic acid and glycerol for examination. Pollen tubes are stained dark blue to bluish red and stylar tissue light green to light greenish blue. This stain permits pollen tubes to be traced even up to their entry into the micropyle.     

应用水稻花粉离体萌发体系观察花粉管内微丝分布

采用非固定、DMSO渗透和异硫氰酸标记的鬼笔环肽（FITC—Ph）染色方法,观察水稻花粉离体萌发过程中花粉管内肌动蛋白微丝的形态和分布。结果表明：（1）水稻花粉水合2min后即可萌发,花粉管生长速度在600～1500μm／h之间。（2）水合而未萌发的花粉粒中,大量较短的梭形微丝束构成微丝网络结构,萌发过程中花粉粒内的梭形微丝束松解,部分微丝转移至萌发的花粉管内沿花粉管纵轴呈束状结构;随着花粉管的伸长,微丝束主要分布在花粉管中前端,但在花粉管顶端区域始终未见明显的微丝束。（3）水合后不能正常萌发的花粉粒内肌动蛋白微丝呈弥散不规则分布,在相同萌发时间生长迟缓的花粉管中,微丝束较少,且主要位于花粉管近萌发孔的部位。表明微丝骨架的形态和分布影响水稻花粉管的萌发和生长。     

Culture of Pollen Tubes for Chromosomal Analysis at the Pollen Tube Division

It is possible to grow pollen tubes routinely for cytological analysis of nuclei at the pollen tube division. Pollen has been grown successfully after temperature, pressure, gas, moisture, and radiation treatments. The technic for growing Tradescantia pollen is described, but any method is satisfactory which ensures that: (a) the pollen is kept dry before sowing, (b) a minimum of time elapses between sowing pollen on culture medium and placing in a moist growing box, and (c) the growing pollen tubes are not allowed to dry out. Pollen of other species can be grown by the same methods.     

An Ultrastructural Study on Pollen Protoplasts and Pollen Tubes Germinated From Them in Gladiolus gandavensis

Large quantities of protoplasts were isolated enzymatically from the mature pollen grains in Gladiolus gandavensis. Regeneration of cell wall and germination of pollen tubes were performed during culture of purified pollen protoplasts in Ks medium supplemented with 32% sucrose, 0.1 mg/1 2,4-D, 1 mg/1 NAA and 0.2 mg/1 6-BA, with a germination rate up to 47.7%. The materials were fixed gently with gradually increasing concentration of glutaraldehyde, followed by osmium, then preembedded in a thin layer of agar and surveyed under an inverted microscope so as to select desired specimens for subsequent procedure. Small agar blocks containing specimens were dehydrated through ethanal-propylene oxide series, embedded in Araldite and ultratomed. Electron microscopic observations show that the pollen protoplasts are surrounded by a smooth plasma membrane and with ultrastructurally intact cytoplasm, a vegetative nucleus and a generative cell. After 8h of culture, wall regeneration commences resulting in a multilayered, fibrillar wall structure which is different from the intine. No exine is formed. Numerous vesicles participate actively in the wall formation. The wall is uneven in thickness around its periphery; a thickened area somewhat resembling to germ furrow is formed, from which pollen tube emerges. The tubes contain abundant plastids, mitochondria and dictyosomes. Vesicles are released out of the plasma membrane and involved in tube wall formation. After 18h of culture, the vegetative nucleus and generative cell have migrated into the tube. Technical points of preparing pollen protoplast specimens for ultastructural studies and the fearnres of wall regeneration in pollen protoplast culture are discussed.     

Finite-Element Analysis of Geometrical Factors in Micro-Indentation of Pollen Tubes

Micro-indentation is a new experimental approach to assess physical cellular properties. Here we attempt to quantify the contribution of geometrical parameters to a cylindrical plant cell’s resistance to lateral deformation. This information is important to correctly interpret data obtained from experiments using the device, such as the local cellular stiffness in pollen tubes. We built a simple finite-element model of the micro-indentation interacting partners – micro-indenter, cell (pollen tube), and underlying substratum, that allowed us to manipulate geometric variables, such as geometry of the cell, cell radius, thickness of the cell wall and radius of the indenting stylus. Performing indentation experiments on this theoretical model demonstrates that all four parameters influence stiffness measurement and can therefore not be neglected in the interpretation of micro-indentation data.     

百合花粉管中的胞吞/胞吐作用观察分析

应用细胞膜染料FM 4-64结合Zeiss 5 live快速扫描型共聚焦显微镜观察了百合花粉管中的吞排作用.结果显示,培养基中加入FM4-64后,染料迅速进入到花粉管中,并在花粉管顶端形成一个锥形的区域;锥形区域表现出周期性变化,并且与花粉管脉冲生长呈负相关,即锥形区形成期花粉管生长缓慢,而锥形区消退期花粉管生长迅速;在锥形区域的消退期,花粉管顶端,尤其是最顶端快速向前延伸,而在锥形区域的形成期,花粉管最顶端的延伸速度显著下降,但亚顶端区域仍基本维持原有的生长速度.研究发现,花粉管的最顶端既是内吞作用也是胞吐作用的主要场所,但胞吞作用仅局限于花粉管的最顶端,而胞吐作用发生在包括亚顶端在内的整个花粉管顶端;胞吞和胞吐作用在花粉管最顶端交替发生,可能是花粉管脉冲生长的一个非常重要的原因.     

Cytochemical Analysis of Callose Localization in Lilium longiflorum Pollen Tubes

Callose, a ß, 1–3 glucan as a component of plantcells has received sporadic attention. Here, we report an attemptto determine whether aniline blue and lacmoid are indeed specificfor visualizing callose. We also re-evaluate, based on a checkfor stain specificity, the localization of callose in elongatingLilium longiflorum, cv. ‘Ace’ pollen tubes. Specificityof these stains was checked by chemical and enzymatic extractionprocedures which solubilize proteins and polysaccharides. Resultsherein question the generally accepted validity of the fluorescent-anilineblue method for detecting callose. Lacmoid either possessesan affinity for both callose and protein or for callose as aglycoprotein. As for callose localization, the walls of thenon-growing region of the lily pollen tube contain callose,probably as a glycoprotein. Presence of the callosicglycoproteinin the wall of the growing tube-tip is dependent on tube length.Callose plugs exhibiting an affinity for aniline blue or lacmoidwere never seen. Phase-contrast microscopy revealed non-stainablewall ingrowths in fixed-tubes and free-moving cytoplasmic masseswithin living tubes.