Low ÃŽ- Irradiation Doses on Saccharomyces Cerevisiae

Low - prick Doses on genus Saccharomyces CerevisiaeRESULTS OF LOW - IRRADIATION DOSES ON SACCHAROMYCES CEREVISIAE FERMETATION PROCESSLetiia OPREAN1, Dan CHICEA2, Enik GASPAR, Ecaterina LENGYELAbstract Four different strains of Saccharomyces cerevisiae yeast try ons were irradiated using a 90Sr atomic source. The results of this ongoing cogitation reveal that the sm alone irradiation doses employ in the work reported here puzzle measurable changes in the fermentation parameters and in the lipid and phospholipid levels.Key words Saccharomyces cerevisiae, small doses, fermentation.1. INTRODUCTIONYeasts be a growth form of eukaryotic microorganisms classified in the kingdom Fungi. Approximately 1500 species of yeasts have been described, most of which reproduce asexually by budding, although in a few cases by binary fission. Yeasts are unicellular, although some species with yeast forms may become multicellular through the formation of a string of connected budding cells known as pseudohyphae, or trustworthy hyphae as seen in most moulds. Industrial yeasts are of special interest for microbiology and biotechnology because they have a big content of lipids and phospholipids that are currently used in naturist products preparation.Nowadays, comprehensive research is being done with respect to the methods of obtaining lipids and phospholipids from lipid biocomponents, in order to identify new methods for obtaining liposomal substances, needed by the pharmaceutical, cosmetic and medical industry. At present, egg lecithin is being used instead but the use of this source has several drawbacks, such as for example the fact that it oxidizes easily. Eukaryotes (yeasts, fungi, algae) are the main microorganisms that produce lipids and phospholipids. Of great interest to microbiology and biotechnology are the researches conducted in the field of phospholipids synthesis, of obtaining phospholipids from microorganisms and of optimizing culture media for their cultivati on.During the last decades, ionizing radiations have been investigated to determine their mould on life history organisms. Radionuclides are released into the environment from various sources nuclear accidents, as planned discharges from the nuclear power industry, disposal of radioactive waste, medical use, nuclear weapons development or recycling. Ionizing radiations are able to cause toxically and genetic effects on organisms, because radionuclides do accumulate in biotic and abiotic components of the environment 1. Nuclear radiation can stimulate morphogenetic changes apparent in the early development stages 2, 3. Nuclear radiation can directly disturb metabolic processes, such as photosynthesis, growth, plant respiration, active transport as well as ionic balance and enzyme synthesis 4. The literature reveals that low doses of ionizing radiations can stimulate cell proliferation 5, 6. In this study, we investigated the low doses of beta radiation influence on the four Saccha romyces cerevisia string section, mainly the influence on the fermentation process.The details of the samples irradiation and fermentation analysis are presented in sections 2 and 3.2. savour IRRADIATIONThe samples were irradiated one at a time in an irradiation sleeping room that was build for this purpose. The hole in the upper part fits a methamphetamine tube than can be easily inserted and paraphraseed. The tube is used to place the sample in the proximity of the beta irradiation source. The schematic of the irradiation chamber is presented in Fig.1. The dose debit through the glass tube, in the very location where the yest samples were placed one by one, was measurable using a RFT KD27012 dosimeter with an ion chamber.Fig. 1 The beta-irradiation chamberThe - source was 90Sr and decays by the turning away (1)having E=546 keV, with a branching ratio of 100% 7. The daughter nucleus, 90Y, is unstable as well. It decays by the scheme (2)with the energies, branching ratios a nd half-lives presented in Table 1.Table 1The energies, branching ratios and half-lives of the 90Y 7.E (keV)I (%)Half-life, hours93.830.000001464.00519.390.011564.00642.770.00183.192280.199.988564.00Four strings of Saccharomyces cerevisiae yeast samples were used. The first string, labeled SCP, was spaced from Turkish yeast having the stigmatize Pakmaya. The second string was labeled SCO and was separated from yeast having the trademark Dr.Oetker. The third string, labeled SCSL, was separated from French yeast having the trademark Saff Levure. The fourth string, labeled SCH, was separated from Dutch yeast having the trademark Hollandia.Two sample of each string were prepared, having a suffix 1, for the pick up, nonirradiated samples and 2 for the irradiated samples. The yeast sample type, irradiation time and irradiation dosis are presented in Table 2Table 2The sample type, irradiation time and irradiation dosisNr.SampleIrradiation time (h)Irradiation Dosis, (Gray)1SCP1002SCP251 23SCO1004SCO25125SCSF1006SCSF25127SCH1008SCH25123. Fermentation detailsBoth the control and the irradiated samples were cultivated in Malt Agar. Malt Agar is used for isolating and cultivating yeasts and molds from food and for cultivating yeast and mold stock cultures 8, 9. Malt Agar contains malt extract which provides the carbon, protein and nutrient sources required for the growth of microorganisms. Agar is the solidifying agent. The acidic pH of Malt Agar allows for optimal growth of molds and yeasts while restricting bacterial growth.The ogdoad samples described above were subject to a fermentation process conducted in identical conditions, in an ECONOMY 20 fermenter. The temperature was maintained constant at 28C. The acidity was maintained at pH=5.8. The maltasic military action (which is defined as catalysis of the hydrolysis of maltose by an alpha-D-glucosidase-type action) and the CO2 emission were monitored for 96 hours 10. The results of the fermentation activity, mea sured as CO2 emission and the maltasic activity measured at 24 hours interval are presented in Table 3. The CO2 emission at 24 hours interval is presented in Fig. 2 and the maltasic activity in Fig. 3.Table 3Results of the fermentation activityNr.crt.Yeast stringCO2-24hmaltasic activity24 hCO2-48hmaltasic activity48 hCO2-72hmaltasic activity72 hCO2-96hmaltasic activity96 h1SCP10.57801.58101.38000.37602SCP20.812201.612401.512000.512003SCO10.78401.38501.18300.28204SCO20.912801.712901.512800.412505SCSL10.67601.47801.27500.37506SCSL20.711901.512101.311600.311807SCH10.78601.49201.19000.48508SCH20.812301.612401.412200.21220Fig. 2 The CO2 emission for the four Saccharomyces cerevisiae yeast stringsExamining Table 1, Fig. 2 and 3 we notice that the fermentation process produced by the irradiated samples (batch having the suffix 2) is more intense, which is proved by the increased CO2 emission and by the increased maltasic activity.4. Conclusions and discussionsOne of the efficient procedur es to select high productivity yeasts is irradiating the samples with nuclear radiation. To our knowledge, results of irradiation on yeast have not been reported yet and the literature is poor in yeast irradiation 11.Examining the results we can conclude that for all four Saccharomyces cerevisiae yeast strings the low 12 Gray irradiation dosis had a stimulating effect in respect of the fermentation process. The SCO and SCH strings had the higher stimulation effect.Fig. 3 The maltasic activity for the four Saccharomyces cerevisiae yeast stringsWe believe that the differences are produced by the yeast genome changes produced by irradiation.The results of this ongoing study revealed that the small irradiation doses used in the work reported here produce measurable improvement in the fermentation parameters. Special care must be taken in evaluating the side effects of the irradiationREFERENCESV.I. Kryukov, V.I. Shishkin, S.F. Sokolenko, Radiacionnaja biologija. Radioekologija, 36 , 209, (1996).I.W. Mericle, R.P. Mericle, Radiat. Botany, 7, 449, (1967).D. Chicea, M. Racuciu, Romanian Journal of Physics 52, 5-6, 589, (2007).V.A. Sidorov, Naukova dumka, Kiev, (1990).Conter, D. Dupouy, H. Planel, Int J Radiat Blot, 43, 421, (1983).F. Croute, J.P. Soleilhavoup, S. Vidal, S. Dupouy, H. Planel, Rad.Res., 92, 560, (1982).LBNL Isotopes Project Nuclear Data Dissemination understructure Page. Retrieved March 11, 2002, from http//ie.lbl.gov/toi.htmlEwing, Davis and Reavis, Public Health Lab. 15, 153, (1957).MacFaddin, Media for isolation-cultivation-identification-maintenance of medical bacteria, vol. 1, Williams Wilkins, Baltimore, (1985).H. Kuriyama, W. Mahakarnchanakul, S. Matsui, H. Kobayashi, Biotechnol. Lett., 15 (2), 189, (1993).J. Kiefer, M. Ebert, Biophysik., 6, 3, 271, (1970).