A STUDY OF LIGHT INTENSITY,PERIODICITY, AND WAVELENGTH ON ZOOSPORE PRODUCTION BY PROTOSIPHON BOTRYOIDES KLEBS12

When mature Protosiphon cells were placed in darkness, zoospore production was more extensive and was completed in a shorter time at a temperature of 27 C than at 22 or 15 C. Cool-white fluorescent (Sylvania) light inhibited the process measurably at a radiation intensity of 0.6±10³ ergsjcm²-sec; inhibition was 96% complete at 14±10³ ergs/cm²-sec. For mature cells previously grown under repeated 12-12 hr light-dark cycles, a dark period of approximately 2 hr at 22 C allowed cell division to proceed to a stage such that reillumination did not inhibit continued development of zoospores. Monochromatic light from 402 to approximately -494 nm, as compared to darkness, inhibited zoospore formation; maximal inhibition was at 432-461 nm. In contrast, monochromatic light from 522 to 726 nm stimulated zoospore formation relative to darkness. Synchronous zoospore production was obtained using the following regimes: (A) 12 hr cool-white alternated with 12 hr yellow, (B) 12 hr cool-white alternated with 12 hr blue. Under regime A synchronous zoospore release (following synchronous production) occurred near the end of the yellow irradiation period, while under regime B it occurred near the end of the cool-white irradiation period. The significance of this in terms of photoprocesses and possible photoreceptors is discussed.     

OBSERVATIONS ON CELL DEVELOPMENT IN CHLAMYDOMONAS SEGNIS (CHLOROPHYCEAE) AT LOW AND HIGH CARBON DIOXIDE TENSION1

Some cell cycle events were compared in Chlamydomonas segnis Ettl during its development in synchronous cultures (12:12 LD) supplied with air and air enriched with 5% CO₂. In cultures bubbled with air, growth resulted in production of 2 relatively small zoospores. In cultures provided with 5% CO₂, 4 large zoospores were formed but not released in darkness unless the cultures were bubbled with CO₂-free air and/or exposed to light. Respiration in zoospores was inhibited by high CO₂ tension. In cultures maintained under continuous illumination for one cell cycle, provision of 5% CO₂ led to enhanced growth, a relatively long S-phase and a 4 h delay of the second cell division. In such cultures, the DNA content of parental cells (12 h L) was insufficient to support two cell divisions. The RNA/DNA ratio of the resulting zoospores was 10 compared to 4 in air cultures. These results provided evidence that the delay of the second cell division was a consequence of the delay in DNA production.     

In vitro production of zoospores by the mosquito pathogen Lagenidium giganteum (Oomycetes: Lagenidiales) on solid media

Reliable, large-scale production of Lagenidium giganteum zoospores was obtained on solid media. The fungus was grown for 7 days in a liquid medium of wheat germ, hemp seed, yeast extract, and glucose, then placed onto hemp-seed agar. Zoosporogenesis was induced on agar by immersing the fungal cultures into water. Zoospore production began 10 hr postimmersion, peaked at 18 hr, and ceased by 36 hr. A single, 10-cm Petri dish of fungus on hemp-seed agar produced 1.7?3.8 × 10⁷ zoospores during the 26 hr of zoosporogenesis. Optimal zoospore production occurred with 4- to 7-day-old cultures; cultures older than 10 days produced few zoospores. The temperature range for zoosporogenesis was 15–35°C. The extent of zoosporogenesis was directly related to the volume of water used to induce zoospore formation and inversely proportional to agar thickness. Bioassay of zoospores against second instar Culex quinquefasciatus larvae yielded an LD₅₀ of 400 zoospores/ml.     

EFFECT OF NITROGEN,SULFUR AND OTHER FACTORS ON ZOOSPORE PRODUCTION BY PROTOSIPHON BOTRYOIDES

O'Kelley , J. C., and T. R. Deason . (U. Alabama, University.) Effect of nitrogen, sulfur and other factors on zoospore production by Protosiphon botryoides. Amer. Jour. Bot. 49(7): 771–777. Illus. 1962.—Nutrient-medium pH, osmotic pressure, staling products, and mineral depletion were studied in relation to zoospore production by Protosiphon botryoides in liquid media. In an intermediate range (pH 5.1–7.7), pH has little or no influence specifically on zoospore production. Although distilled water is an unsuitable medium for zoospore production, if a balanced nutrient medium is supplied, osmotic pressure is without pronounced influence over a wide range. Staling products in old cultures exert a minor inhibitory effect. Deficiencies of nitrate, sulfate, or calcium in liquid media can decrease drastically zoospore production or release, and nitrate or calcium depletion appears to be mainly responsible for loss of the capacity of Protosiphon to produce and release zoospores in aged liquid cultures.     

Citric acid production from glucose. I. Growth and excretion kinetics in a stirred fermentor

The growth and citric acid production kinetics of Saccharomycopsis lipolytica on glucose are investigated in an aerated stirred fermentor. Cellular growth first proceeds exponentially until exhaustion of ammonia in the fermentation medium. Cells then continue to grow at a reduced rate with a concomitant decrease in intracellular nitrogen content. Citric and isocitric acid production starts at the end of the growth phase. During about 80 hr excretion proceeds at a constant rate of 0.7 g/liter/hr for citric acid and 0.1 g/liter/hr for isocitric acid. The final citric and isocitric acid concentrations are 95 and 10g/liter, respectively. During acid excretion cellular respiration accounts for 60 and 35% of consumed oxygen and glucose. Both acid and CO₂ production rates follow a Michaelis–Menten-type dependence on oxygen concentration with Michaelis–Menten constants of 0.9 and 0.15 mg/liter for acid and CO₂ productions, respectively.     

LIGHT,TEMPERATURE AND PHOTOPERIOD AS FACTORS CONTROLLING REPRODUCTION IN ULOTHRIX ZONATA (ULVOPHYCEAE)1

In many lakes in the northern United States and Canada the filamentous green alga Ulothrix zonata (Weber and Mohr) Kütz grows abundantly in early spring in shallow waters. Asexual reproduction occurs by formation of quadriflagellate zoospores which disrupt, the integrity of the cells upon release causing the filament to disintegrate. Study of the effects of 100 different combinations of irradiance, temperature and photoperiod revealed that zoospore formation is favored by high temperatures near 20°C, high light levels of 520 μE·m^?2·s^?1 and photoperiods of either short day (8:16 h light-dark) or long day cycles (16:8 h light-dark). Zoospore formation is minimal under conditions of low temperature (5°C), low irradiance (32.5 μE·m^?2·s^?1) and neutral day-lengths (12:12 h light-dark). These observations explain the decline in U. zonata biomass when water temperatures rise above 10° C. The combined effect of rising water temperatures and increasing daylengths causes progressively more filaments to switch from vegetable growth to zoospore production resulting in an increasing loss of biomass.     

Zoospore production in selected xanthophycean algae

The effects of incubation time and deficiencies of calcium and nitrate on zoospore production were investigated in Botrydiopsis arhiza Borzi, B. intercedens Vischer et Pascher, Bumilleriopsis peterseniana Vischer, Pseudobumilleriopsis pyrenoidosa Deason et Bold, and Ophiocytium maius Naegeli. Release of zoospores occurred after the transfer of stationary phase, vegetative cells into fresh Bold's basal medium. Maximum yields of zoospores were produced on the second day after transfer, 0·5–1·0 h after the start of the light period of a 12–12 h light-dark cycle. Lack of calcium or nitrate reduced the yield of zoospores in each taxon. Only O. maius produced large numbers of motile cells in nitrate-free medium.     

CHARACTERIZATION OF BLEACHING IN CHLORELLA INDUCED BY SUBOPTIMAL GROWTH TEMPERATURES1

Incubation of cultures of a high-temperature strain of chlorella at 10 C stopped growth and bleached all chlorophyll in the cells in 24 hr. Optimal conditions of light (3.0 mw/cm²), gas (1% CO₂-in-air), and inorganic medium for maximal growth at 39 C were maintained in the transfer from 39 to 12, 10, or 5 C. The bleaching process at 10 C is characterized by a lag period for the first few hours followed by a linear decrease in chlorophyll content of cultures. The amounts of time required to bleach half of the chlorophyll initially present (effective half-times) at 10 C were 14 hr for chlorophyll a and 17 hr for chlorophyll b. Effective half-times of bleaching for total chlorophyll were 47 hr at 12 C and 6 hr at 5 C. Addition of glucose to inorganic medium delayed but did not prevent bleaching. Use of argon gas instead, of 1% CO₂-in-air prevented cells from bleaching in both inorganic and glucose media, and indicated an oxygen requirement for bleaching. Incubation of 6 additional strains of Chlorella at 10 C resulted in responses ranging from bleaching to no growth to growth.     

Cellulase and protein production from mixed cultures of Trichoderma viride and a yeast

Fermentations with mixed cultures of the cellulolytic fungus Trichoderma viride and the yeast Saccharomyces cerevisiae or Candida utiliswere examined. The fermentations were carried out in an aerated 5 liter fermentor with NaOH treated barley straw as the cellulose source (2–4%). Yeast was inoculated 24–32 hr after the fungus and the growth of the two organisms was followed through the production of CO₂ and cell protein. In comparison with fermentations with T. viridealone, the production time for maximum yields of cellulases and cell protein was reduced by several days, depending on the straw concentrations. The protein content of the growth product was 21–22% and the amino acid composition of the product resembled that of T. viride alone.     

THE EFFECT OF ESTRADIOL ON THE CELL KINETICS IN THE UTERINE AND CERVICAL EPITHELIUM OF NEONATAL MICE

The effect of estradiol-17β on the length of the various phases of the cell cycle was studied in the neonatal mouse uterine, and cervical epithelium. A double labelling method was used, and in addition labelled mitoses were counted. In the uterus proper, estradiol shortens the length of the total cell cycle, T_c, from 17-9 hr to 15-7 hr, and the duration of S phase, T_s, from 6–7 to 5-1 hr 6 hr after estradiol treatment. 12 hr after estradiol treatment, T_c is shortened to 7-4 hr and T_s to 4–5 hr. The shortening of T_c at 12 hr is mainly due to an effect on T_G1, which is shortened from 8–55 hr in untreated animals to 1–8 hr in estradiol treated animals. The T_c of cervix epithelium cells in untreated animals was found to be 21-8 hr. After treating the mice for 6 hr with estradiol the T_c was now increased to 47 hr and further to 61 -2 hr following 12 hr treatment with the hormone. T_s increases from 8-3 hr to 15-2 hr following 6 hr estradiol treatment, and to 15-4 hr after 12 hr treatment. The effect is most pronounced in T_G1, which is lengthened from 10–95 hr in untreated animals to 28-1 hr and 43 hr, respectively, in animals treated for either 6 or 12 hr with estradiol.     

Impact of low‐intensity pulsed ultrasound on the growth of Schizochytrium sp. for omega‐3 production

Schizochytrium sp. is a microalga that is known for its high content of oils or lipids. It has a high percentage of polyunsaturated fatty acids in the accumulated oil, especially docosahexaenoic acid (DHA). DHA is an important additive for the human diet. Large‐scale production of Schizochytrium sp. can serve as an alternative source of DHA for humans as well as for fish feed, decreasing the burden on aqua systems. Therefore, research on improving the productivity of Schizochytrium attracts a lot of attention. We studied the potential of using low‐intensity pulsed ultrasound (LIPUS) in the growth cycle of Schizochytrium sp. in shake flasks. Different intensities and treatment durations were tested. A positive effect of LIPUS on biomass accumulation was observed in the Schizochytrium sp. culture. Specifically, LIPUS stimulation at the ultrasound intensity of 400 mW/cm² with 20 min per treatment 10 times a day with equal intervals of 2.4 h between the treatments was found to enhance the growth of Schizochytrium biomass most effectively (by up to 20%). Due to the nature of cell division in Schizochytrium sp. which occurs via zoospore formation, LIPUS stimulation was inefficient if applied continuously during all 5 days of the growth cycle. Using microscopy, we studied the interval between zoospore formation in the culture and selected the optimal LIPUS application days (Days 0–1 and Days 4–5 of the 5‐day growth cycle). Microscopic images have also shown that LIPUS stimulation enhances zoospore formation in Schizochytrium sp., leading to more active cell division in the culture. This study shows that LIPUS can serve as an additional tool for cost‐efficiency improvement in the large‐scale production of Schizochytrium as a sustainable and environmentally friendly source of omega‐3 (DHA).     

Effects of Carbon Dioxide on Coccidian Oocysts from 6 Host Species*

SYNOPSIS Activation of sporozoites in oocysts of Eimeria acervulina (chicken), E. intricata (sheep), and E. scabra (swine) occurred after pretreatment in aqueous 0.02 M cysteine hydrochloride under an atmosphere of CO₂, followed by incubation in a trypsin-bile mixture. Sporozoites of E. stiedae (rabbit), E. bilamellata (squirrel), and Isospora canis (dog) became activated when incubated in trypsin and bile with or without prior CO₂-pretreatment of oocysts; however, when CO₂-pretreatment was used, activation of these species in trypsin and bile was greatly enhanced. For E. acervulina, 12% of the oocysts were activated after 4 hr CO₂-pretreatment and 10 hr incubation in trypsin and bile at 43 C; higher temperatures or longer pretreatment times did not cause greater activation. Eimeria intricata oocysts became activated after 1 hr pretreatment and 10 hr incubation in trypsin and bile at 37, 39 or 41 C, respectively. The highest activation (31%) occurred after 20 hr pretreatment and 10 hr incubation in trypsin and bile at 41 C. Ninety percent of E. scabra oocysts contained active sporozoites after 1 hr CO₂-pretreatment and 10 hr incubation in trypsin and bile at 37 C. At 39 or 41 C, 100% activation occurred with this species after similar pretreatment and treatment periods. With E. bilamellata, 64% activation occurred in nonpretreated oocysts incubated 10 hr in trypsin and bile at 41 C, whereas 100% activation occurred if oocysts were pretreated with CO₂ for 1 hr before treatment with trypsin and bile. Thirty-one, 35, and 36% of CO₂-pretreated E. stiedae oocysts were activated after 1 hr incubation in trypsin and bile at 37, 39 or 41 C, respectively, whereas 1, 2, and 20% activation occurred in nonpretreated oocysts incubated at the same temperatures. Sporozoites in 99-100% of I. canis oocysts were activated after 10 hr treatment in trypsin and bile with or without 1 hr CO₂-pretreatment at 23, 37, 39 or 41 C.     

Effect of different CO2 concentrations on biomass,pigment content,and lipid production of the marine diatom Thalassiosira pseudonana

The marine diatom Thalassiosira pseudonana grown under air (0.04% CO₂) and 1 and 5% CO₂ concentrations was evaluated to determine its potential for CO₂ mitigation coupled with biodiesel production. Results indicated that the diatom cultures grown at 1 and 5% CO₂ showed higher growth rates (1.14 and 1.29 div day⁻¹, respectively) and biomass productivities (44 and 48 mg_AFDWL⁻¹ day⁻¹) than air grown cultures (with 1.13 div day⁻¹ and 26 mg_AFDWL⁻¹ day⁻¹). The increase of CO₂ resulted in higher cell volume and pigment content per cell of T. pseudonana. Interestingly, lipid content doubled when air was enriched with 1–5% CO₂. Moreover, the analysis of the fatty acid composition of T. pseudonana revealed the predominance of monounsaturated acids (palmitoleic-16:1 and oleic-18:1) and a decrease of the saturated myristic acid-14:0 and polyunsaturated fatty acids under high CO₂ levels. These results suggested that T. pseudonana seems to be an ideal candidate for biodiesel production using flue gases.

     

PHOTOSYNTHESIS AND RESPIRATION OF ARCEUTHOBIUM TSUGENSE (LORANTHACEAE)

Dark respiration rates of the aerial shoots of Arceuthobium tsugense, obtained by manometric and IRGA techniques, show production of CO₂ to range between 155–300 μl CO₂ g^-1hr^-1 with evidence of seasonal variation. Experiments with ¹⁴CO₂ indicate that the aerial shoots are capable of some photosynthetic CO₂ fixation, with 10–15 % of the available ¹⁴C incorporated by the plant tissue in one hr. Biochemical characterization of the products of photosynthesis reveals that 80–90 % of the incorporated ¹⁴C is ethanol soluble. Ten percent of the ethanol soluble fraction is lipoidal in nature, the rest is H₂O soluble. IRGA experiments indicate an apparent photosynthetic CO₂ fixation capacity of 80–90 μl CO₂ g^-1hr^-1, or 25–30% of the amount of CO₂ produced by respiration. The significance of these findings is discussed with respect to nutrition of the parasite and effects upon the host.     

Changes in the CO2 Concentrating Mechanism During the Cell Cycle in Dunaliella tertiolecta

Synchronised cells of Dunaliella tertiolecta were used to investigate the expression of the CO₂ concentrating mechanism over the cell cycle during growth in either ambient air (low Ci cells) or air enriched with 5% CO₂ (high Ci cells). The cultures were analysed for extracellular carbonic anhydrase activity, affinity of photosynthesis for inorganic carbon (Ci) and the ability to accumulate Ci. In high Ci cells, carbonic anhydrase activity changed between 2 ? 4 units mg^?1 Chi during the light-dark rhythm showing no clear periodicity. Similarly, the apparent affinity for Ci remained rather constant over the cell cycle. This was judged from the Ci concentrations required for half maximum rate of photosynthesis (K_1/2(Ci)) of 72 ? 80μM. In the same cells the accumulation ratio of internal Ci versus external Ci ranged between 5 and 9.5 without a clear rhythm. In contrast, these parameters showed distinct periodical changes in synchronised low Ci cells. Carbonic anhydrase activity changed from 10 to 350 units mg^?1 Chl with maximum and minimum activities occurring in the middle and at the end of the light period, respectively. The K_1/2(Ci) values showed similar periodicity ranging between 13 ? 36μM. In addition the accumulation ratio increased up to 30 in the middle of illumination and decreased to its lowest level of 12 at the end of the light period. These results indicate the presence of a common step in regulating the induction of the measured parameters and that light is not an absolute requirement for the induction of the CO₂ concentrating mechanism in synchronous low CO₂ grown cells of Dunaliella tertiolecta.     

Biomethanation: Anaerobic fermentation of CO2, H2 and CO to methane

Studies to examine the microbial fermentation of coal gasification products (CO₂, H₂ and CO) to methane have been done with a mixed culture of anaerobic bacteria selected from an anaerobic sewage digestor. The specific rate of methane production at 37°C reached 25 mmol/g cell hr. The stoichiometry for methane production was 4 mmol H₂/mol CO₂. Cell recycle was used to increase the cell concentration from 2.5 to 8.3 g/liter; the volumetric rate of methane production ran from 1.3 to 4 liter/liter hr. The biogasification was also examined at elevated pressure (450 psi) and temperature to facilitate interfacing with a coal gasifier. At 60°C, the specific rate of methane production reached 50 mmol/g cell hr. Carbon monoxide utilization by the mixed culture of anaerobes and by a Rhodopseudomonas species was examined. Both cultures are able to carry out the shift conversion of CO and water to CO₂ and hydrogen.     

The effect of CO2 ventilation on kinetics and yields of cell-mass and ethanol in batch cultures ofZymomonas mobilis

Summary The effect of CO₂ removal by continuous sparging of N₂ in batch cultures ofZymomonas mobilis (ATCC10988) was examined. N₂ sparging considerably reduces lag times in batch cultures, possibly because of continuous removal of CO₂ from the culture media. Ventilation of CO₂ from culture media results in an increase of about 15% in the average specific growth rate and about 12% in the cell-mass yield with no noticeable trend in the average specific glucose uptake and ethanol production rates. The overall ethanol yield on glucose, however, decreases slightly by 5%. Analysis of ventilated experiments show that the CO₂ production is directly coupled with the ethanol formation but not necessarily with the cell-mass production, indicating a decoupling of growth from ethanol production. Further, comparison of ventilated and non-ventilated experiments rules out the possibility of CO₂ accumulation in the culture media as a factor responsible for increasing growth inhibition and decoupling of growth from ethanol fermentation at increasing initial glucose concentrations in batch cultures.     

Studies on synchronously dividing cultures of Euglena gracilis Klebs (strain Z). 3. Circadian components of cell division

Euglena gracilis Klebs (Z) was grown axenically and autotrophically in four-liter serum bottles at 25°C on an aerated, continuously stirred, inorganic salt medium. Four fluorescent illumination regimes were employed: (1) continuous bright light of 3500 lux (LL_b); (2) continuous dim light of 800 lux (LL_d); (3) a L_bD: 14, 10 (3500 lux) light-dark cycle; and (4) a L_dD: 14, 10 (800 lux) light-dark cycle. Cell number was automatically monitored throughout all experiments. In LL_b the generation time (G.T.) of the population was about 12 hours, whereas in LL_d following LL_b it was approximately five days; exponential growth occurred in either case. In L_bD: 14, 10 synchronous growth occurred with a doubling of cell number every cycle of 24 hours. In L_dD: 14, 10, however, although rhythmic cell division took place every 24 hours, the average increase in cell number during the division burst which occurred in each dark period was only 13.4%, so that the G.T. of the culture was about five days, as was the case for LL_d. In the constant conditions of temperature and continuous dim light (LL_d), following synchronous growth in L_bD: 14, 10, small (17.0%) rhythmic division bursts lasting 14.5 hours continued to occur for at least ten days, with a period of 24.2 hours. The overall G.T. of the culture was about five days. These data demonstrating the circadian, endogenous nature of rhythmic cell division under certain conditions of continuous dim illumination were discussed in relation to the synchronous division observed in temperature and light-dark cycles.     

Diurnal changes in malate-decarboxylation activity in the leaves of a CAM plant, Bryophyllum daigremontianum

Bryophyllum diagremontianum plants grown under light-dark regimeswere exposed to one more cycle of the regime or to continuousdarkness for 24 hr. Photosynthetic O₂ evolution by leaf segmentsfrom these plants was investigated in the presence of 15 mMNaHCO₃ (CO₂-dependent O₂ evolution) or in the absence of CO₂(malate-dependent O₂ evolution). The malate-dependent O₂ evolutionserved as an index of the activity of malate decarboxylation.Malate content was respectively 67, 64 and 85 µmoles/g.fwin leaves measured at 7 hr 30 min in light and 6 hr 26 min inthe dark from plants under the light-dark regime (light 12 hr/dark12 hr) and those measured at 6 hr 26 min in the dark from plantsunder the continuous dark regime. The malate- and CO₂-dependentphotosynthetic O₂ evolutions in the same leaves were 9.7 and22, 0.2 and 17, and 16 and 26 µmoles/g.fw.hr, respectively.Thus, the diurnal change in capacity for malate-dependent O₂evolution was relieved by continuous dark treatment. These results suggest that the diurnal change in malate decarboxylationin this crassulacean acid metabolism plant does not occur byan endogenous rhythm. This further indicates lack of an endogenousrhythm for the influx-efflux of malate across the vacuole andin malate decarboxylation enzyme activity. (Received August 1, 1979; )     

Increased heterocyst frequency by patN disruption in Anabaena leads to enhanced photobiological hydrogen production at high light intensity and high cell density

The effects of increasing the heterocyst-to-vegetative cell ratio on the nitrogenase-based photobiological hydrogen production by the filamentous heterocyst-forming cyanobacterium Anabaena sp. PCC 7120 were studied. Using the uptake hydrogenase-disrupted mutant (ΔHup) as the parent, a deletion-insertion mutant (PN1) was created in patN, known to be involved in heterocyst pattern formation and leading to multiple singular heterocysts (MSH) in Nostoc punctiforme strain ATCC 29133. The PN1 strain showed heterocyst differentiation but failed to grow in medium free of combined-nitrogen; however, a spontaneous mutant (PN22) was obtained on prolonged incubation of PN1 liquid cultures and was able to grow robustly on N₂. The disruption of patN was confirmed in both PN1 and PN22 by PCR and whole genome resequencing. Under combined-nitrogen limitation, the percentage of heterocysts to total cells in the PN22 filaments was 13–15 and 16–18% under air and 1% CO₂-enriched air, respectively, in contrast to the parent ΔHup which formed 6.5–11 and 9.7–13% heterocysts in these conditions. The PN22 strain exhibited a MSH phenotype, normal diazotrophic growth, and higher H₂ productivity at high cell concentrations, and was less susceptible to photoinhibition by strong light than the parent ΔHup strain, resulting in greater light energy utilization efficiency in H₂ production on a per unit area basis under high light conditions. The increase in MSH frequency shown here appears to be a viable strategy for enhancing H₂ productivity by outdoor cultures of cyanobacteria in high-light environments.