Research Article
L-Serine Dehydratase Formation in Fusarium moniliforme
Department of Botany, Girls College of Education in Riyadh, P. 0. Box 27104, Riyadh 1141 7, Saudia Arabia
L-Serine dehydratase (L-serine hydro-lase, deaminating, EC 4.2.1.13) has been extensively studied in several bacteria including Aeromonas punctata[1], anaerobic bacteria[2], Arthrobacter globiformis[3], Bacillus circulans[4], Brevibacterium linens[5], Campylobacter spp.[6], Citrobacter[7] Clostridium acidiurici[8], Corynebacterium glycinophilum[9,10] Corynebacterium spp.[11], Escherichia coli[12-15], Eubacterium acidaminophilum[16], Helicobacter pylori[17] heterofermentative lactobacilli[18], homofermentative lactobacilli[19], lactobacillus murinus[20], Lactobacillus fermentum ATCC14931[21] Lactobacillus plantarum[22], Proteus vulgaris[23].
Pseudomonas cepacia[24] Salmonella typhimurium and Bacillus cereus[25], Sarcina albida[26], Staphylococcus epidermidis[27], Sterptococcus clavuligerus[28] Streptococcus faecalis[29] and Wild Rhizobia[30]. Its presence was also demonstrated in the yeast Saccharomyces cerevisia[31] and the filamentous fungi Cunninghamella elegans and Fusarium oxysporum[32,33] and Neurospora crassa[34].
Nelson[35] reported that L-serine dehydratase was produced to the extent of only 0.04 mg1 dry weight by Aeromonas punctata NRRL B-928 when grown on a chemically defined medium. Addition of 2% (w/v) L-serine to this medium increased L-serine dehydratase ten fold or more, indicating a significant inductive effect. D-serine was toxic to the organism, making weights and enzyme titers uncertain, but DL-serine induced specific activity of L-serine dehydratase at least equal to that from the L enantiomorphism.
El-Awamry et al.[32] demonstrated that FeSO4 was the best inducers for L-serine dehydratase synthesis by Cunninghamella elegans and Fusarium oxysporum. The enzyme produced during the logarithmic phase of growth of the two organisms and maximum production was obtained after 3 days incubation. The optimal pH rang for L-serine dehydratase formation in F. oxysporum was 4-5, whereas for C. elegans enzyme pH 5.0 was the optimal. L-serine dehydratase of both organisms was induced with L-serine, ammonium carbonate, some amino acids and amides, but L-serine was the best inducers. L-Serine concentration of 2.4 g L1 was the optimal for L-serine dehydratase synthesis.
The present investigation deals with the biosynthesis of L-serine dehydratase in Fusarium moniliforme under different physiological conditions. Such studied have not been reported before in f Fusarium moniliforme.
Organism: Fusarium moniliforme was obtained from Cairo Mircen, Faculty of Agriculture, Ain Shams University, Egypt.
Media and culture: The organism was grown on glucose-Czapek-Dox liquid medium with L-serine replacing NaNO3 on nitrogen equivalent basis. In addition, the medium supplement with 0.01% FeSO4 for stimulating the synthesis of L-serine dehydratase. The pH of the medium was adjusted to 5.0.
Five ml aliquots of spore suspension of Fusarium moniliforme were used to inoculate 250 ml Erlenmeyer
flasks, each containing 50 ml sterile medium. The inoculated flasks were incubated at 28 oC for 5 days, then the mycelia were harvested by filtration, washed thoroughly with distilled water and finally blotted dry with absorbent paper.
Preparation of cell-free extract: The harvested mycelia were ground with cold sand in a cold mortar and extracted with 0.05 M Tris-HCl buffer at pH 8.5. The obtained slurry was then centrifuged at 12 g for 10 min and the supernatant was used as the crude enzyme preparation.
Chemical methods: Pyruvate was estimated by the method of Friedmann and Haugen[36]. The method is based on the interaction of pyruvate with the 2, 4-dinitrophenylhydrazine reagent. The procedure can be summarized as follows: To 1 ml of the reaction mixture, 1 ml of 0.1 2, 4-dinitrophenylhydrazine in 2 N HCl was added. After 5 min, 5 ml of 2.5 N NaOH were added and the color intensity was measured spectrophotometrically at 520 nm. Protein was determined according to the method of Sutherland et al. [37].
Assay of L-serine dehydratase: L-serine dehydratase activity was routinely assayed by determining pyruvate formation from L-serine. One unit of enzyme activity is defined as the amount of protein which catalyzes the formation of one μmole pyruvate in 90 min at 30°C.
All data were statistically analyzed using Person coefficient[38].
L-Serine dehydratase activity at different stages of growth of F.moniliforme: The growth was measured by the dry weight of the mycelium and L-serine dehydratase activity in extracts of the experimental fungus were determined at different periods of incubation. Figure 1 shows that the highest specific enzyme activity was obtained at the 5th day of growth after which the enzyme activity decreased. Maximal growth was also obtained after 5th day incubation.
Effect of different pH values on L-serine dehydratase synthesis and growth of F.moniliforme: To study the effect of the original pH value of L-serine-containing medium on the intensity of growth and the activity of L-serine dehydratase in F. moniliforme, 7 pH values were chosen they rang from 2.0 to 10.
Fig. 1: | L-Serine activity at different stages of growth of F. moniliforme (●) specific activity. (◇) Dry weight |
Table 1: | Effect of different pH values on L-serine dehydratase synthesis and growth of F. moniliforme |
The final pH of the culture medium was measured after 5 days incubation |
Table 2: | Growth and L-serine dehydratase synthesis of F. moniliforme on various nitrogen source |
Each nitrogen source was added in amounts equivalent, on nitrogen basis, to the amount of nitrogen in sodium nitrate in Czapek-Dox medium |
It was found that no growth occurred at pH 2.0. It is clear that F. moniliforme could grow and synthesis L-serine dehydratase within a wide pH range (3-10). It is clear that the growth rate was more or less equal at these pH values. Maximum growth and enzyme formation were obtained at pH 5 (Table 1).
In addition, the pH values of the culture media were measured at the end of incubation. No significant change in the pH values 3, 4, 5 and 6 of these media was detected, while there was significant change in the pH values 8 and 10 of these media. The acid production by the fungus causes decrease in the pH values of the medium. These results are in close agreement to those reported for C. elegans and F. oxysporum[32].
Table 3: | Influence of different carbon sources on L-serine dehydratase synthesis and growth of F. moniliforme |
Table 4: | Effect of some metal salts on L-serine dehydratase synthesis and growth of F. moniliforme |
Each metal salts was added at concentration of 10 mg L1 |
Table 5: | Growth and synthesis of L-serine dehydratase as a function of L-serine concentration in the culture medium of F. moniliforme |
Growth and L-serine dehydratase synthesis of F. moniliforme on various nitrogen sources: Table 2 shows that F. moniliforme can grow with a great variety of nitrogen nutrients. L-Glutamic, L-glycine and ammonium chloride supported growth which was more or less equal to that of cultures grown on sodium nitrate . However, growth on Lserine was superior as nitrogen sources for sodium nitrate, while L-threonine and L-alanine supported moderate growth.
Results shown in Table 2 indicated that the synthesis of F. moniliforme Lserine dehydratase was induced by L-serine, L-glutamic, L-glycine, L-alanine, L-threonine and ammonium chloride as compared with that of nitrate-grown cultures. L-serine and L-threonine were the most potent inducers. Comparable result were obtained by Nelson[35] who found that L-serine dehydratase was produced to the extent of only 0-04 mg1 dry weight by Aeromonas punctata NRRL B-928 when grown on a chemically defined medium. Addition of 2%(w/v) L-serine to this medium increased L-serine dehydratase ten-fold or more, DL-serine induced a specific activity of L-serine dehydratase at least equal to that from the L enantiomorphism. El-Awamry et al.[32] demonstrated that Lserine dehydratase of C. elegans and F. oxysporum was induced with Lserine, ammonium carbonate, some amino acids and amides, but Lserine was the best induced.
Influence of different carbon sources on L-serine dehydratase synthesis and growth of F. moniliforme: Table 3 demonstrated that the growth of F. moniliforme was not significantly affected when glucose was replaced by starch, but significantly affected when glucose was replaced by galactose, maltose, sucrose and lactose.
Concerning the synthesis of L-serine dehydratase by F. moniliforme, it is clear from the results that maltose was the best inducer, it caused about 111%increase in specific enzyme activity. While, starch and sucrose caused 38 and 3% increased in specific enzyme activity. However, Lactose and Galactose caused 32 and 37.3% repression in enzyme formation.
Effect of some metal salts on L-serine dehydratase synthesis and growth of F. moniliforme: Table 4 shows that FeSO4 stimulated fungal growth and L-serine dehydratase formation by about 82 and 134%, respectively. CaCl2, CoCl2, CuSO4 and MnCl2 resulted a decrease in mycelial dry weight by about 53.2, 53.2 , 58.7 and 51.6%, respectively, while L-serine dehydratase formation was stimulated by CaCl2, CoCl2, CuSO4 and MnCl2 about 48, 155, 122 and 165%, respectively. This result agreed with that reported by El-Awamry et al.[32] who demonstrated that L-serine dehydratase of C. elegans and F. oxysporum was induced by metal salts and FeSO4 was the best inducer.
Growth and synthesis of L-serine dehydratase as a function of L-serine concentration in the culture medium of F. moniliforme: L-Serine was added to the basal medium as the sole source of nitrogen in concentrations ranging from 0.6 to 4.8 g L1. In Table 5 the optimum concentration of L-serine for growth was 2.4 g L1. The mount of nitrogen in this concentration is equivalent to its amount in 2 g sodium nitrate. The specific activity of L-serine dehydratase was increased with increasing L-serine concentration in the medium. Optimum concentration of L-serine for enzyme synthesis was 2.4 g L1. This result agreed with that reported for L-serine dehydratase of C. elegans and F. oxysporum[32].