Exine-Detached Pollen of Nicotiana tabacum as an Electroporation Target for Gene Transfer

In developing alternative systems for plant transformation the authors investigated the use of male gametophyte as the foreign gene receptor. However, delivery of foreign DNA into pollen is difficult because of the existence of a thick exine, therefore a new experimental system was developed using exine-detached pollen (EDP) of Nicotiana tabacum as an electroporation target which was also compared with germinating pollen (GP) and pollen grains (P). A transient GUS expression assay was conducted to analyze the effects of different electroporation conditions and promoter activity. The pollen-specific promoter Zml3 from Zea mays mediated high level of GUS gene expression but CaMV 35S only had very low activity in both EDP and GP. The optimal field strength for gene transfer was obtained at 750 V/cm for EDP and 1250 V/cm for GP when the time constant of pulse was 13 ms. The GUS activity in EDP had a 5-fold increase as compared with GP and P respectively. The level of GUS gene expression was slightly increased when adding 10 % PEG into the electroporation buffer. This result indicates that pollen deprived of exine responds much better to foreign gene transfer than the previously used intact pollen grains and may be a better vector to introduce, via pollen tube, genes into the egg cell and offsprings.     

Expression of a foreign gene in electroporated pollen grains of tobacco

Summary The incorporation of genetically engineered DNA into pollen and subsequent fertilization of eggs by the transformed pollen would be a convenient method for producing genetically engineered seed. This method of pollen transformation would circumvent the need for other types of gene transfer methods such as the use of Agrobacterium tumefaciens, which has a limited host range and thus a limited capability for genetically engineering plants. It would also avoid the problems associated with the regeneration of some plants from tissue, cell, or protoplast culture after receiving foreign DNA. To this end, the genetically engineered plasmid DNA vector pBI221 containing the gene encoding -glucuronidase (GUS) was introduced by electroporation into germinating pollen grains of tobacco (Nicotiana gossei L.). Transient expression of the GUS gene was demonstrated by the presence of GUS activity in fluorometric assays of pollen extracts 24 h after the introduction of pBI221 via electroporation. Intact pBI221 was detected by Southern blotting procedures as a distinct DNA band in pollen extracts 1 h after electroporation. In addition, pBI221 was detected as a diffuse band of higher molecular weight DNA 24 h after electroporation, suggesting that some of the pBI221 was incorporated into the genome of the pollen.     

烟草脱外壁花粉的电激基因转移

以 β-葡糖苷酸酶 GUS 基因作为报告基因 ,通过瞬间表达的检测 ,比较了烟草 Nicotianatabacum L . 脱外壁花粉、未萌发与萌发花粉的电激导入效果 ,探讨了不同电激条件及启动子对外源基因瞬间表达的影响 .结果表明 :当脉冲时间常数为 13 ms时 ,导致脱外壁花粉和萌发花粉生活力下降约50 %的电场强度分别为 750 V/ cm和 12 50 V/ cm,在此条件下电激 ,二者的导入效果最好 .脱外壁花粉的GUS基因表达水平约为萌发花粉的 5倍、花粉粒的 30倍 .玉米花粉特异启动子 Zm13- 2 60 能启动 GUS基因在脱外壁花粉和萌发花粉中高效表达 ,而 Ca MV 35S的启动活性很低     

Treatment of maize pollen to reduce nuclease activity

Recently it has been reported that maize (Zea mays L.) pollen can be stored up to several hours in a hypertonic aqueous medium at 0°C without losing its germinability (Broglia and Brunori 1994). We found that both release and activity of pollen nucleases are diminished in a cold hypertonic aqueous medium. Nucleases can be washed off while preserving germination ability and thus preserving the possibility of passive uptake of exogeneous DNA into germinating pollen grains. Alternatively, active DNA transfer into non-germinating pollen grains in the storage medium itself may be facilitated, due to the very reduced nuclease activity in this medium.     

Advances in Pollen Mediated Genetic Transformation

植物遗传转化技术是植物科学基础理论与应用研究的有力武器,已成为植物遗传改良的重要途径之一。但是、目前遗传转化所采用的受体系统,大都需要体外培养和植株再生过程,才能获得转基因植株。其中、基因型限制和遗传变异是该技术不可逾越的两大障碍。花粉管通道法可省去转化体的离体培养,不过、多数植物受花器结构的限制而难以经花柱注射ＤＮＡ,只能向子房注射,并不是真正的“花粉管通道”。又由于此法外源基因的导入发生在授粉之后,因此该方法亦不属于花粉遗传转化。利用小孢子胚胎发生体系进行遗传转化与利用花粉作为外源ＤＮＡ的媒介,继而、通过授粉受精获得转基因种子,是目前花粉遗传转化的两个重要方面和活跃的研究方向。前者仍需要离体再生系统,后者则可以利用植物自身的再生机制,本文称之为花粉介导法（ｐｏｌｅｎ－ｍｅｄｉａｔｅｄｔｒａｎｓｆｏｒｍａｔｉｏｎ）。该方法通过自然的胚胎发育过程获得转基因子代,避免了组织培养过程中的遗传变异和转基因植株的嵌合现象。可望成为简便快速的植物遗传转化体系。目前对花粉介导的遗传转化进行专门评述的文献较少,本文对该领域的研究分三个层次进行了综述。一、外源基因转化方法小孢子或由小孢子形成的胚状体是很有潜力的遗传转化受体     

Rapid optimization of electroporation conditions for plant cells,protoplasts, and pollen

The optimization of electroporation conditions for maximal uptake of DNA during direct gene transfer experiments is critical to achieve high levels of gene expression in transformed plant cells. Two stains, trypan blue and fluorescein diacetate, have been applied to optimize electroporation conditions for three plant cell types, using different square wave and exponential wave electroporation devices. The different cell types included protoplasts from tobacco, a stable mixotrophic suspension cell culture from soybean with intact cell walls, and germinating pollen from alfalfa and tobacco. Successful electroporation of each of these cell types was obtained, even in the presence of an intact cell wall when conditions were optimized for the electroporation pulse. The optimal field strength for each of these cells differs, protoplasts having the lowest optimal pulse field strength, followed by suspension cells and finally germinating pollen requiring the strongest electroporation pulse. A rapid procedure is described for optimizing electroporation parameters using different types of cells from different plant sources.     

Calcium uptake from the stigma by germinating pollen in Primula officinalis L. and Ruscus aculeatus L.

Summary The flow of calcium ions from the stigma to germinating pollen was studied by autoradiography in Primula officinalis (dry stigma) and Ruscus aculeatus (wet stigma). ⁴⁵Ca²⁺ ions were observed to be taken up by the pistils from an agar medium and then transported intracellularly to both the stigmal cells and the stigmal exudate. The ⁴⁵Ca²⁺ present in the stigma was taken up by the germinating pollen grains.     

Storage in an Organic Solvent as a Means for Preserving Viability of Pollen Grains

Pollen grains of Lilium auratum, Lilium longiflorum, Camellia sasanqua and Impatiens balsamina were soaked in various kinds of organic solvents such as acetone, benzene, petroleum benzine, benzyl alcohol, butanol, ethanol, methanol, isopropanol, diethyl ether, petroleum ether and choroform, and stored at 4-6 C for 24 hr. All pollen grains except in benzyl alcohol showed evidence of viability, and grains which had been stored in acetone, benzene, petroleum benzine, diethyl ether, petroleum ether and chloroform produced longer pollen tubes than grains of fresh pollen, especially Camellia sasanqua, whose pollen grew tubes 3 times as long as those of a control. Lilium auratum pollen grains had retained their viability after 80 days in acetone, benzene, petroleum benzine, diethyl ether and petroleum ether, and generative nuclei in pollen thus stored divided to form 2 sperm nuclei in artificial culture.     

Transfection of a DNA/protein complex into nuclei of mammalian cells using polyoma capsids and electroporation

We used empty capsids ofpolyoma virus to transfer DNA fragments and DNA/protein complexes into human cells. We encapsulated labeled and unlabeled single stranded DNA fragments by viral capsids. A complex of DNA with a DNA binding protein, recA, will also be taken up by the capsids, whereas the free protein is not incorporated. We further compared this gentle biological method of DNA transfection with a well-established physical method, electroporation. Electroporation also allows the transfer of DNA as well as protein into cells, although there is no proof that a DNA/protein complex can survive the procedure functionally. Whereas the viability of capsid transfected cells is unaffected (100%), electroporation reduces the viability to 90–95%. On the other hand, the amount of DNA found in the nucleus of electroporated cells is higher than for cells treated with loaded viral capsids.     

High level of GUS gene expression driven by pollen-specific promoters in electroporated lily pollen protoplasts

Gene constructs that contained the -glucuronidase (GUS) gene under the control of a pollen-specific Zm13 promoter from maize and a LAT52 promoter from tomato were introduced by electroporation into pollen protoplasts isolated from bicellular pollen grains of Lilium longiflorum. After 20 h in culture, the pollen protoplasts exhibited the apparent expression of GUS in a fluorometric assay. The GUS activity induced under the control of the Zm13 promoter was over 10 000 times higher than activity in the control (with no DNA or without electroporation). By contrast, the GUS gene was nearly silent in the lily microspore protoplasts and generative cell protoplasts. The GUS activity driven by the Zm13 and LAT52 promoters was also detected by a cytochemical assay. The frequency of blue-staining pollen protoplasts was about 70% in the case of the Zm13 promoter. The efficiency of gene transfer by electroporation was much higher than by particle bombardment. This protoplast-specific electroporation system is suitable for rapid and reliable examination of pollen-specific promoters, being as good as the particle bombardment system.     

Protection of pollen germination from adverse temperatures: a possible role for proline

Abstract After germination, pollen grains of Lilium longiflorum became very sensitive to short periods of heat stress as shown by the greatly reduced germination percentages upon subsequent incubation at the optimal temperature. Addition of proline to the incubation medium made pollen more resistant to heat. It was demonstrated that in a short time a large amount of proline was taken up by the cell. Germination and metabolic functions were completely or partially protected from heat damage by proline treatment. As well, it was shown that proline treatment at least partially protected pollen grains from cold stress. These results suggest that the high proline concentrations found in pollen of many species may confer resistance to germinating pollen grains at unfavourable temperatures thereby enhancing the chances of successful fertilization.     

Effects of exogenous phytohormones on intracellular pH of Petunia hybrida pollen grains

The effects of exogenous phytohormones (IAA, ABA, and GA₃) on the intracellular (cytoplasmic) pH (pH_c) in ungerminating and germinating petunia (Petunia hybrida L.) pollen grains were studied. The pH_c values were measured with fluorescein diacetate. In ungerminating pollen grains, all phytohormones reduced pH_c relatively rapidly; after 10–15 min, initial value was restored. In germinating pollen grains, IAA and ABA induced a relatively rapid cytosol alkalization, which was not reversed during experiment. GA₃ acidified the cytosol, i.e., exerted the effect similar to that in ungerminating pollen grains. Sodium orthovanadate suppressed completely the hormone-induced pH_c shift toward alkaline values in germinating pollen grains, whereas this inhibitor did not affect pH_c in the absence of phytohormones. Sodium orthovanadate also slowed the recovery of pH_c after hormone-induced cytoplasm acidification in ungerminating pollen grains, reduced pH_c in control ungerminating grains, and weakened substantially the effects of all phytohormones on these pollen grains. On the basis of these results, we suggested that physiological activities of phytohormones in this system were mediated by pH_c modulation, namely, a transient disturbance in the cytosolic pH homeostasis, which could trigger further phytohormone-induced cell responses. We concluded that a hormone-induced cytoplasm alkalization in pollen grains was mediated by the activity of their plasma membrane H⁺-ATPase and that this proton pump was involved in the control of pH_c in both germinating and ungerminating pollen grains.     

Unreduced diploid nuclei in Cupressus dupreziana A. Camus pollen

Size and DNA content of pollen of Cupressus dupreziana A. Camus, a highly endangered Mediterranean conifer, were assessed by cytomorphological observations and flow cytometric analyses and then compared to C. sempervirens L. pollen. Mature C. dupreziana pollen was composed of two uninucleated types of pollen grains differing in size. Around 35% of the grains exhibited a size similar to C. sempervirens pollen, while 65% exhibited a larger diameter. However only one peak of fluorescence was detected by flow cytometry. DNA content of C. dupreziana pollen was twice the DNA content of C. sempervirens pollen. Comparison of DNA contents of mature and germinating pollen revealed that mature pollen of both species were arrested in the G2 phase. Comparison with the DNA content of somatic tissue (2C) provided evidence for the production of unreduced pollen in C. dupreziana. This unexpected feature in gymnosperms is discussed in terms of reproductive strategy of this species. Received: 11 December 1999 / Accepted: 22 December 1999     

Dry matter disappearance and gelatinization of grains as influenced by processing and conditioning

Four ruminally cannulated steers (average body weight 430 kg) were used in a 4 × 4 split plot. Latin square design, in situ experiment to evaluate grain processing methods and effects of grain conditioner on dry matter (DM) disappearance (DMI) and degree of gelatinization of four grains. Effects of grinding or steam flaking, with and without the addition of a commercial grain conditioner, on DMD of corn (Zea mays), barley (Hordeum vulgare), wheat (Triticum vulgare) and sorghum (Sorghum vulgare) were measured at incubation times of 0, 6, 12, 24, 36 and 48 h. Degree of gelatinization of grains was determined by polarized light microscopy as loss of birefringence.

Ground grams had greater DMD than flaked grains at 0 h (sorghum, P < 0.05), 24 h (wheat, P < 0.01), 24 h (barley, P < 0.05) and 36 h (wheat, P < 0.01); however, steam flaking increased DMD at 36 h (corn, sorghum, P < 0.01) and 48 h (sorghum, P < 0.01) compared with grinding. In situ DMD was greater (P < 0.05) for ground, ground + conditioned and steam-flaked barley than for steam-flaked + conditioned barley at 24 h. Ground wheat had the greatest (P < 0.10) DMD among ground grains at 12 and 24 h; likewise, ground + conditioned wheat had the greatest (P < 0.10) DMD among ground + conditioned grains. A trend for increased DMD of wheat was observed across time, and among processing and conditioning methods, compared with other grains. Degree of gelatinization was greater for steam-flaked than for ground grains. Corn, wheat and barley reached gelatinization at lower temperatures than sorghum. These data suggest that effects of processing and conditioning varied among grains and within grains across time. Use of a commercial grain conditioner did not consistently alter DMD of grains.     

An Improved Cellophane Method for in Vitro Germination of Recalcitrant Pollen

The cellophane technique of La Cour and Faberge has been improved by the use of a booklet of filter paper. The booklet consists of seven squares of filter paper stapled together; the cellophane on which the pollen is germinated is placed between the two top leaves of the booklet and the whole soaked in a sucrose-based nutrient medium for 15 min. This arrangement keeps the cellophane flat as it absorbs medium. The top leaf of the booklet is then removed, the pollen dusted on it and the completed preparation closed in a plastic-wrapped Petri dish. The lower leaves of the booklet keep the cellophane moist for up to 24 hr. Proportions of pollen grains germinating are at least as high as in the hanging drop method; pollen of species that germinate poorly or not all in hanging drops do well in this technique. Because the pollen tubes adhere tightly to the cellophane, staining, observation, and studies of various sorts are facilitated.     

Introduction of impermeable molecules into pollen grains by electroporation

Summary Electroporation was used to introduce plasma membrane impermeable molecules into the cytoplasm of pollen grains ofLilium longiflorum. Ungerminated pollen grains were exposed to the fluorescent dye quin2 or FITC-labelled dextrans and electroporated with exponentially decaying voltage pulses of 250 to 2000 V/cm and time constants of 0.01 to 10 s. The number of electroporated pollen grains increased with the strength and duration of the voltage pulses, and with the osmolarity of the external medium. Optimal results were obtained with pulses of 1000 V/cm and 10 s time constant, and with 900 mM mannitol in the electroporation buffer. The size of the pores produced in the plasma membrane by electroporation allowed uptake of 40 kDa dextran but not 70 kDa dextran. The rate of germination of pollen grains was low immediately after electroporation, but increased with time in pollen growth medium. The conditions of electroporation reported here may be used to load genetic material into pollen grains for the production of transgenic plants.Abbreviations PGM pollen growth medium - FDA fluorescein diacetate - FITC fluorescein isothiocyanate     

Pollen recognition and rejection during the sporophytic self-incompatibility response: Brassica and beyond

Many hermaphrodite flowering plants avoid self-fertilization through genetic systems of self-incompatibility (SI). SI allows a plant to recognize and to reject self or self-related pollen, thereby preserving its ovules for outcrossing. Genes situated at the S-locus encode the ‘male’ (pollen) and ‘female’ (pistil) recognition determinants of SI. In sporophytic SI (SSI) the male determinant is expressed in the diploid anther, therefore haploid pollen grains behave with a diploid S phenotype. In Brassica, the male and the female determinants of SSI have been identified as a peptide ligand and its cognate receptor, respectively, and recent studies have identified downstream signalling molecules involved in pollen rejection. It now needs to be established whether the Brassica mechanism is universal in species with SSI, or unique to the Brassicaceae.     

海南凤仙花不同海拔种群的传粉生物学

凤仙花属(Impatiens)植物具有极为广泛的多样性和类型各异的特化传粉者, 被誉为“双子叶的兰花”, 受到众多传粉生物学家的关注。本文以海南特有种海南凤仙花(Impatiens hainanensis)为研究对象, 对3个不同海拔梯度的种群进行了开花生物学特性和开花物候、花器官结构、花粉活力和柱头活性、传粉者种类和访花行为及繁育系统的比较研究。结果表明: 单花花期4.10 ± 0.46 d, 雄性期和雌性期分别约为3.15 ± 0.24 d和0.95 ± 0.36 d; 种群开花峰期在8月初, 高海拔种群的花期高峰相对滞后。低、中海拔种群花粉活力呈现先升高后下降的趋势, 以开花第2 d花粉活力最高; 高海拔种群花粉活力随开花时间推移逐渐下降; 柱头活性随开花时间的推移而增强, 高海拔种群开花各天次均较低、中海拔种群低。主要传粉昆虫为黄黑无垫蜂(Amegilla leptocoma)和绿条无垫蜂(A. zonata), 低、中海拔种群以黄黑无垫蜂为主, 高海拔种群以绿条无垫蜂为主。未观察到自动自花授粉和无融合生殖现象, 人工授粉能明显增加坐果率(75-90%), 自然坐果率在高海拔种群相对较低(40-60%), 说明存在较强的传粉者限制。海南凤仙花的保护需要同时关注其有效传粉者的保护, 促进有效传粉昆虫在不同海拔种群之间的往来, 保证种群间的花粉流与种子流, 维持海南凤仙花的种群遗传多样性与有效种群大小。     

Responses of tobacco pollen to high humidity and heat stress: viability and germinability in vitro and in vivo

Summary Responses of pollen grains of Nicotiana tabacum to high humidity (95% RH, 4 h) and temperature (38°/45° C, 4 h) stresses were investigated. Pollen grains were subjected to only RH or only temperature, or to both of these stresses. Their viability was assessed on the basis of the fluorochromatic reaction (FCR) test, and vigour was assessed on the basis of the time taken for in vitro germination as well as on the emergence of pollen tubes through the cut end of semi-vivo implanted styles. None of the stress conditions affected pollen viability and high RH or high temperature stress did not individually affect pollen vigour. However, pollen vigour was markedly affected when both the stresses were given together. Pollen grains subjected to high RH at 38° C took a longer time to germinate in vitro and the pollen tubes emerged later from the cut end of the semi-vivo styles; division of the generative cell was also delayed. Pollen grains subjected to high RH at 45° C failed to germinate in vitro, but did germinate on the stigma. Many pollen tubes subjected to this treatment showed abnormalities, and the growth of pollen tubes in the pistil was much slower than that observed in other treatments. Pollen samples subjected to all of the stress conditions were able to induce fruit and seed set. The implications of these results on the relationship between the FCR test and viability, and between viability and vigour, especially in stressed pollen, are discussed.