Spore germination

The germination of dormant spores of Bacillus species is the first crucial step in the return of spores to vegetative growth, and is induced by nutrients and a variety of non-nutrient agents. Nutrient germinants bind to receptors in the spore's inner membrane and this interaction triggers the release of the spore core's huge depot of dipicolinic acid and cations, and replacement of these components by water. These latter events trigger the hydrolysis of the spore's peptidoglycan cortex by either of two redundant enzymes in B. subtilis, and completion of cortex hydrolysis and subsequent germ cell wall expansion allows full spore core hydration and resumption of spore metabolism and macromolecular synthesis.     

Maize embryo germination

The cell-cycle progression of germinating embryos of maize (Zea mays L.) was studied from 0 to 72 h after the start of imbibition using DNA flow cytometry on isolated nuclei, and analyses of thymidine kinase activity, histone biosynthesis and levels of proliferating cell nulcear antigen (PCNA). At the start of germination, 75% of the cells were in G1, but this population had decreased to 25% by 72 h. The concomitant increase of cells in S-phase did not occur continuously, but stepwise, indicating that during germination most of the cells enter S-phase as a partially synchronized population. Within the initial 60 h of embryo germination the cells passed through one S-phase; the start and duration of this period of replicative DNA synthesis was further substantiated by the analysis of S-phase-associated events, the biosynthesis of core histones and the enzyme activity of thymidine kinase, which both began to increase at about 12 h after the start of differentiation. Thymidine kinase fluctuated periodically during germination with a transient maximum at 30 h and a second peak at 72 h; histone biosynthesis was not detectable until 12 h after the start of germination. The levels of PCNA protein closely resembled the pattern of thymidine kinase during germination. Together with the cytometric data this allows a clear assignment of cell cycle events to different times of embryo differentiation.Abbreviation PCNA proliferating-cell nuclear antigen Dedicated to Prof. Walter Larcher on the occasion of his 65th birthdayThe authors wish to thank Prof. G. Mikuz (Department of Pathology, University of Innsbruck, Austria) and Prof. G. Stöffler (Department of Microbiology, University of Innsbruck, Austria) for their interest and support. The technical assistance of Mrs. R. Gantschnig is gratefully acknowledged. E.I. Georgieva was recipient of short-term fellowships from the Austrian Academy of Sciences, the Austrian Forschungsgemeinschaft and the Austrian Akademischer Austauschdienst. G. López-Rodas was recipient of a postdoctoral fellowship from the Programa sectorial de Formación de Profesorado y Personal investigador del Ministerio de Educación y Ciencia (Spain). This work was supported in part by Grant SO6011 (to P.L.) from the Austrian Fonds zur Förderung der wissenschaftlichen Forschung and the Dr. Legerlotz-Foundation.     

Seed germination in Gactaceae

The mode of germination of representatives of 89 genera of the Cactaceae, 4 genera of Portulacaceae and 1 genus of Phytolaccaceae was studied. Most of the species of the Cactaceae germinate by means of a seed lid (operculum). In the Cactaceae studied 11 kinds of germination could be distinguished, 3 of which were with, and 8 without, operculum formation.
Opercula are restricted in their occurrence to the subfamilies Cactoideae (Cereoideae) and Pereskioideae and are not found in the subfamily Opuntioideae. Within the subfamily Cactoideae operculum formation was found to occur in all tribes and in all investigated subtribes. Opercula were also found in two genera of the related family of the Portulacaceae. In the Phytolaccaceae no operculum formation was observed.     

Mycoheterotrophic germination of Pyrola asarifolia dust seeds reveals convergences with germination in orchids

Dust seeds that germinate by obtaining nutrients from symbiotic fungi have evolved independently in orchids and 11 other plant lineages. The fungi involved in this 'mycoheterotrophic' germination have been identified in some orchids and non-photosynthetic Ericaceae, and proved identical to mycorrhizal fungi of adult plants. We investigated a third lineage, the Pyroleae, chlorophyllous Ericaceae species whose partial mycoheterotrophy at adulthood has recently attracted much attention. We observed experimental Pyrola asarifolia germination at four Japanese sites and investigated the germination pattern and symbiotic fungi, which we compared to mycorrhizal fungi of adult plants. Adult P. asarifolia, like other Pyroleae, associated with diverse fungal species that were a subset of those mycorrhizal on surrounding trees. Conversely, seedlings specifically associated with a lineage of Sebacinales clade B (endophytic Basidiomycetes) revealed an intriguing evolutionary convergence with orchids, some of which also germinate with Sebacinales clade B. Congruently, seedlings clustered spatially together, but not with adults. This unexpected transition in specificity and ecology of partners could support the developmental transition from full to partial mycoheterotrophy, but probably challenges survival and distribution during development. We discuss the physiological and ecological traits that predisposed to the repeated recruitment of Sebacinales clade B for dust seed germination.     

Studies on germination of chrysanthemum pollen I. Effect of sugars on germination

1. 1. The percentage of chrysanthemum pollen stained with Nitroblue tetrazolium ranged from 60 to 90 %, indicating the presenceof active succinate dehydrogenase in the pollen.
2. 2. Exogenousapplication of oligosaccharides such as sucrose,lactose andraffinose at concentration of 20 to 35 % favoredgerminationof chrysanthemum pollen. However, the germinationrate was notelevated higher than 10 % in most of the chrysanthemumcultivars.
3. 3. Sugar content of chrysanthemum pollen was less than 10%of the fresh weight. The sugar was composed of glucose, fructoseand sucrose, the amount of sucrose being about four times asmuch as that of glucose or fructose.
4. 4. The ß-fructofuranosidaseactivity of chrysanthemumpollen was very high. These and relevantresults suggest thatthe poor germination of chrysanthemum pollenis due neitherto abortion nor to the deficiency of specialsugars in the pollen.

(Received November 14, 1967; )     

Control of the germination of secondary dormant cocklebur seeds by various germination stimulants

The responsiveness of non-dormant, upper cocklebur (Xanthiumpennsylvanicum Wallr.) seeds to various germination stimulants,such as CO₂ C₂H₄ CS(NH₂)₂, BA and enriched O₂, decreased withincreasing periods of water imbibition and was completely lostin the state of secondary dormancy. Unlike CO₂ BA and CS(NH₂)₂however, C₂H₂ and enriched O₂ effectively prevented the developmentof secondary dormancy, and their combination was the most effectivefor stimulating the germination of seeds which had undergoneimbibition for a long time. CS(NH₂)₂ and BA were effective,not by themselves but either under anaerobiosis or elevatedO₂ tension. Growth of the axial and cotyledonary segments excisedfrom aged seeds remained responsive to these germination stimulantsand could be further stimulated by exogenous C₂H₂. With imbibitionat a lower temperature, the seeds maintained high germinationin response to various stimulants and a high rate of C₂H₂ andCO₂ production during a long period of water imbibition. Theseresults are discussed in terms of the two possible causes forthe loss of responsiveness or induction of the secondary dormancy. (Received June 27, 1978; )     

Inhibition of microsporidian spore germination

Microsporidia are obligate intracellular parasites that are increasingly recognized as significant causes of disease in AIDS patients. Gordon Leitch, Govinda Visvesvara and Qing He here describe the deployment of the microsporidian spore infection apparatus, the polar filament, and show how this may be a useful site for chemotherapeutic interdiction of the infections caused by these parasites.     

Pre-harvest germination in male-sterile wheats

F¹ hybrid grain borne on cytoplasmic male-sterile (A line) parents germinated (sprouted) before maturity but grain set on male-fertile analogues (B lines) of the A lines did not. Sprouting may involve varied with the pollinator and with the A lines although their ranking order varied between experiments. Unsprouted grain harvested from A lines subsequently germinated more rapidly than that from the B lines.     

Aids to seed germination studies

Summary Two aids to seed germination studies are described. The first, a closed unit, enables rapid and effective surface sterilisation of small fragile seeds to be carried out. The second, for use in field situations, facilitates a given number of seeds being placed under natural conditions. The design of the apparatus causes minimal interference with the microclimate and prevents seed loss by natural vectors and seed input from indigenous species adjacent to experimental areas.     

Metabolic control of seed germination

We have used proteomics to better characterize germination and early seedling vigor in sugarbeet. Our strategy includes (1) construction of proteome reference maps for dry and germinating seeds of a high-vigor reference seed lot; (2) investigation of the specific tissue accumulation of proteins (root, cotyledon, perisperm); (3) investigation of changes in protein expression profiles detected in the reference seed lot subjected to different vigor-modifying treatments, e.g. aging and/or priming. More than 1 000 sugarbeet seed proteins have been identified by LC/MS-MS mass spectrometry (albumins, globulins and glutelins have been analyzed separately). Due to the conservation of protein sequences and the quality of MS sequencing (more than 10 000 peptide sequences have been obtained), the success rate of protein identification was on the average of 80%. This is to our knowledge the best detailed proteome analysis ever carried out in seeds. The data allowed us to build a detailed metabolic chart of the sugarbeet seed, generating new insights into the molecular mechanisms determining the development of a new seedling. Also, the proteome of a seed-storage tissue as the perisperm is described for the first time.     

Spore germination in Dictyostelium discoideum

Mutant spores of Dictyostelium discoideum, strain SG-10, differ from wild type spores in their ability to spontaneously germinate, to be activated with 5% dimethyl Sulfoxide (DMSO), and to be deactivated with 0.2 M sucrose. Both heat-activated wild type and mutant spores began to swell after a lag of 60–75 min at ambient temperature. Suspension of heat activated spores in 5% DMSO resulted in blockage of spore swelling and a concomitant severe inhibition of respiration; removal of 5% DMSO allowed resumption of respiration and the spores began to swell after a lag of only 15 min. It was concluded that 5% DMSO allowed the early reactions (M) to proceed but blocked the later reactions (R) of post-activation lag.Treatment of one day old spores with 20% DMSO solution for 30–120 min quantitatively activated the population. The post-activation lag time was directly dependent on the time of 20% DMSO treatment. Spores activated with 20% DMSO treatment could be deactivated by incubation at 0°C; the spores most quickly deactivated at 0°C were those within 10 min of swelling. Mitochondrial transport inhibitors such as azide and cyanide caused deactivation in an analogous manner. It is hypothesized that spores proceed to the second portion of the lag phase called (R) before the environment determines if dormancy is reimposed or if germination will proceed. The sensitive strain (SG-10) showed a greater degree of damage than the wild type after supraoptimal treatment with 40% DMSO. The spores became more resistant with age to the damaging action of 40% DMSO. All the observed effects of DMSO treatment were compatible with our multistate model of activation which suggests that the early portion of the lag phase (M) may involve a relative uncoupling of oxidative phosphorylation while the later portion (R) may require tight coupling.     

Phytochrome regulation of seed germination

Seed germination of many plant species is influenced by light. Of the various photoreceptor systems, phytochrome plays an especially important role in seed germination. The existence of at least five phytochrome genes has led to the proposal that different members of the family have different roles in the photoregulation of seed germination. Physiological analysis of seed germination ofArabidopsis thaliana (L.) Heynh. with phytochrome-deficient mutants showed for the first time that phytochrome A and phytochrome B modulate the timing of seed germination in distinct actions. Phytochrome A photo-irreversibly triggers the photoinduction of seed germination after irradiation with extremely low fluence light in a wide range of wavelengths, from UV-A, to visible, to far-red. In contrast, phytochrome B mediates the well-characterized photoreversible reaction, responding to red and far-red light of fluences four orders of magnitude higher than those to which PhyA responds. Wild plants, such asA. thaliana, survive under ground as dormant seeds for long periods, and the timing of seed germination is crucial for optimizing growth and reproduction. It therefore seems reasonable for plants to possess at least two different physiological systems for sensing the light environment over a wide spectral range with exquisite sensitivity of different phytochromes. This redundancy seems to enhance plant survival in a fluctuating environment.     

Photocontrol of fungal spore germination

Germination of Puccinia graminis f. sp. tritici uredospores is inhibited by continuous irradiation. Prehydration of spores enhances both dark germination and photoinhibition. Simultaneous irradiation with ineffective red (653 nanometers) and inhibitory far red light (720 nanometers) results in partial nullification of the inhibition brought about by far red light alone. This result would be consistent with the involveent of a photoreversible pigment system similar to phytochrome, operating via the high irradiance reaction.     

Thermoperiodism in cocklebur seed germination

Germination potential in nondormant, upper cocklebur (Xanthium pensylvanicum Wallr.) seeds, which were incapable of germinating under constant temperatures below 25 C in air, was increased by exposure to diurnally alternating temperatures. The cocklebur seeds failed to respond to the temperature fluctuations in the beginning of water imbibition, and their responsiveness appeared only after aerobic presoaking for a limited period or after anaerobic pretreatment for 1 to 3 days.

Maximal germination was obtained after exposure to a thermoperiodic regime of 8 hours at 23 C and 16 hours at 8 C. A process occurring during the high temperature phase was aerobic and had to precede the inductive low temperature phase, its effect increasing with temperature. Critical minimum length of the inductive low temperature phase changed with the duration of a preceding anaerobiosis, for instance about 4 hours after 1 day anaerobiosis, but about 2 hours after 2 days. Percentage of subsequent germination was in proportion to the number of thermoperiodic cycles. A process of the inductive low temperature phase was not perturbed by inserting a brief higher temperature period into its phase; indeed, such insertion rather increased germination potential when performed in the earlier parts of the inductive low temperature phase. The effect of the low temperature survived for 13 to 17 hours during the higher temperature period.