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IOSR Journal of Pharmacy and Biological Sciences (IOSR-JPBS)
e-ISSN: 2278-3008, p-ISSN:2319-7676. Volume 6, Issue 5 (May. – Jun. 2013), PP 15-19
www.iosrjournals.org
www.iosrjournals.org 15 | Page
Optimization of Cultural Parameters for Cellulase Enzyme
Production from Fungi Species Isolated From Degradation Corn
Cob
Bamigboye, O. O.
Department of Biology Emmanuel Alayande College of Education, Oyo.
Abstract: Cellulalytic fungi synthesize cellulose enzyme for biodegradation of cellulose. This depends on
various condition which include the source f isolation. This study was designed to determine the optimum
condition necessary for cellulose production by fungi.
Cellulose activities at different temperatures, pH and nitrogen sources by Rhizopus oryzae Aspergillus
niger; A. flams, P. expansum and A. oryzae in liquid medium was studied and cellulose enzyme assay carried
out by dinitrosalicylic acid method.
All the fungal isolates have their highest cellulose activity at 400
c except Penicillium expansum whose
highest value of 1.28mg/ml was obtained at 320
c. Cellulase produced 6m was found to be highest in all the
isolate at pH 4.0 exception P expansum which occur at pH 5.5 (1.21mg/ml). The highest value e1.45mg/ml was
obtained in A niger. Highest cellulose activity for A. niger, A. oryzae & P. expansum occurred in peptone.
The study shows the need to determine the best physiological condition that allow for the optimal
cellulose activity of fungal isolate. This will enhance their enzyme production.
Key Word: Cellulase, fungi, pH, Nitrogen, temperature
I. Introduction
Cellulases a cosorfulm of free enzymes which comprises of enchoglucanase (β 1-4-D glucan-4-
glucanolydrolase EC 3.2.1.4, carboxymethyl cellulalse, EC) Exoglucanase (β -1,4-D glucan-4-glucahydrolase
EC allobiohydrolase, CBH) and cellobiases (β-d-glucoside glucohydrolase, EC 3.2.1.21, β-I, 4-D-glucosidase)
which are found in many of the 57 glycosyl hydrolase families. (Siddigui et al. 2000) cellulose is the enzyme
that hydrolyzes the β-1-4 glycosidic bonds I enzyme.
Fungi are the most prominent cellulose producing microorganism (Immanuel et al 2007). Although a
large number of microorganisms are capable of degrading cellulose, only a few of these produce significant
quantities of cell free enzyme capable of completely hydrolyzing crystalline cellulose (Kooniinok, 2005). The
need to optimize the cultural condition for igmnt maximum production of the enzyme is therefore essential.
II. Materials and Method
All chemicals used were reagent grade obtained from May & Baker and Sigma – Aldrich chemical
company India. The fungi, Aspergillus niger, Rhizopus oryzae, Aspergilus oryzae, Penicillum expansum and
Aspergillus flavus used in this study were isolated from degrading corn cob on Potato Dextrose agar and yeast
extract agar. Pure cultures obtained were identified by conventional test and maintained on PDA slants.
The five fungal isolates were separately grown and tested for production of cellulose in submerged
culture in a chemically defined medium composed of KHzP0µ (1gl-1
) MgS047Hz0 (0.5gl-1
) yeast extract (1gl-1
)
Ccl2 2H20 Co.14gl-1
) carboxymethyl cellulose 10g and thiavaine 0.0025gl-1
). The cultures were grown at 270
c
for 28 days, culture broth was sampled at different days during growth to determine enzyme productivity by
carboxymethyl hydrolysis.
Enzyme assay
Cellulose activity was assayed by the determination of reducing sugar released from carboxymethyl
cellulose (CMC). After growth had been allowed to proceed for the required length of time at the required
temperature, the cultures were filtered through sintered glass crucibles and the cellulolytic activity of the
filterates was determined using the method of Reese and Mandels (1963). The assay medium was 0.55%
caroxymethyl cellulose (CMC) in 0.55m acetate buffer (pH 5.5) and 9ml of this were incubated with 1ml of the
fungus filterate for 1 hour at 370
c. Filterates of the uninoculated control was also obtained and similarly
assayed. To estimate the amount of reducing sugars released, 1ml of dinitrosalicylic acid (DNSA) reagent was
added to 1ml of the filterate – CMC reaction mixture and the absorbance was determined at 540mm using an SP
600 spectrophotometer.
The absorbance of standard aqueous solution of D-glucose at various concentrations (0-10mg per ml)
Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated
www.iosrjournals.org 16 | Page
was determined and used to construct a graph of percentage absorbance as related to mg of glucose per ml. The
amount of reducing sugar produced by 1ml of bacteria filterate from the CMC assay medium was calculated
form this graph. Cellulolytic activity of the filterates was then expressed in term of the amount of total reducing
sugars (RS) per ml.
Effect of Temperature on Cellulase Activity
Bottles of the chemically defined medium were inoculated and incubated at 28, 32 and 400
C. These
were subsequently filtered and cellulose activity of the filtrate were determined at 0, 4, 7, 14, 21 and 28 days.
Effect pH on Celulase Activity
Some bottles of the chemically defined medium were inoculated and incubated at 270
C. Prior to
inoculation the pH of the media was adjusted to pH 4.0, 5.5 and 7. The samples were filtered at 0,4, 7, 14, 21
and 28 days and cellulose activity at the afferent pH was determined.
Effect of Nitrogen Source on Cellulase Activity
The organisms were cultivated in the chemically defined media containing 1% carboxymethyl cellulose
and supplemented with different Nitrogen sources of 1% (w/v). The nitrogen sources used include yeast extract,
peptone, urea, (NH4)2 SO4 and NaNO2. These were incubated at 270
C and cellulose activity of the filtrate were
determined at 0, 4, 7, 14, 21 and 28 days in the different Nitrogen sources.
III. Result and Discussion
Cellulose activity under different physiological conditions by Rhozopus oryzae, Aspergillus niger, A
flavus, Penicillum expansum and A. oryzae was studied.
All the fungal isolates showed cellulase activity, fungi of the geura Aspergillus and Penicillium have
been reported as good cellulase producers (Milala et al., 2005, Hoffinem ad Wood, 1985, Abo State et al.,
2010).
The result of cellulase activity at different temperatures by the fungal isolates is shown in figure 1.
Cellulase activity was found to be highest in 400
c in A niger with a value of 1.32mg/ml. Rhizopus oryzae at
320
c in day 14. All the fungal isolates had their highest reducing sugar production at 400
C except Penicillum
expansum with the highest value of 1.28mg/ml on day 14. This agreed with Immaneul et al., (2007) who
reported the optimum temperature for cellulase enzyme production by A. niger & A. fungatus at 400
C.
The optimum pH for A niger, A flavus and Rhizopus oryzae was pH 4.0 as shown in figure 2 while P
expansum and Aspergillus oryzae was at pH 5.5. Akiba et al., (1995) reported that cellulase production was
high at pH 4 and 4.5 by A. niger optimum activity for A. niger, A oryzae and P expansum occurred in peptone
as seen in Figure 3a
& b. This correlates with the result of Guatam et al., (2011) who reported that peptone
enhanced the production of cellulase by A niger on solid municipal waste residue.
Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated
www.iosrjournals.org 17 | Page
Fig.6: Effect of temperature on the cellulase production by fungal isolates
Cellulase activity at 32o
C
Cellulase activity at 40o
C
Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated
www.iosrjournals.org 18 | Page
Fig.7: Effect of pH on the cellulase production by fungal isolates
Fig.8a: Effect of different nitrogen sources on cellulase production by fungal isolates
Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated
www.iosrjournals.org 19 | Page
Fig.8b:Effect of different nitrogen sources on cellulase production by fungi isolates
References
[1]. Abo-State, M.A.M., Hammad, A.E., Selin M. and Gannam R.B. 2010. Enhanced production of cellulases by Aspergillus sp on
agricultural wastes by solid state fermentation. American – Eurasian Journal of Agricultural & Environmental Science. 402 – 410.
[2]. Akiba, S., Kimura, K. and Kumugal, H. 1995. Purification and characterization of protein resistant cellulase from Aspergillus niger.
Journal of Fermentation Bioengineering 79: 125 – 130
[3]. Gautam, S.P., Bundela, R.S., Pandey, A.K., Khan, J. Awashi, M.K. and Sarsaiya, S. 2011. Optimization for the production of
cellulose enzyme from municipal solid waste residue by two novel cellulolytic Fungi Biotechnology Research Tnternational 2011: 8.
[4]. Hoffman, R. M and Wood, T.M. 1985. Isolation and partial characterization of a mutant Penicillium for the saccharification of straw.
Biotechnology. Bioengineering 27: 81-85.
[5]. Immanuel, G., Akila Bhagavath, C. M. Iyapppa Raj, P., Essakking, P. and Palavessam A. 2007. Production and partial purification
of cellulase by Aspergillus niger and A. fumigatus fermented in coir waste and saw dust. Internet Journal for Microbiology 3:1 – 17.
[6]. Koomnok, C. 2005. Selection of cellulose producing thermophilic fungi. 31st
congress on Science and Technology of Thailand.
[7]. Milala, M.A., Shugaba, A., Gidado, A., Ene, A.C. and Wafar, J.A. 2005. Studies on the use of aricultural wastes for cellulase
enzyme production by Aspergillus niger. Research Journal of Agriculture and biological Sciences 1. 4: 323-325.
[8]. Nishida, Y., Suzuki K.I., Kumayai, Y., Tanaka, H., Inove, A. and Ojima, T. 2007. Isolation and primary structure of a cellulose from
the Japanese sea urchin. Strongylocentrotus nudus. Biochime. 1-10.
[9]. Siddigni, K.S., Saqib, A.A.N., Rashid, M.H. and Rajoka M.I. (2000). Carboxyl group modification significantly altered the kinetic of
purified carboxymethylcellulase from Aspergillus niger. Enzyme and Microbial Technology Vol 27, No 7, Pp 467 – 474.

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Optimization of Cultural Parameters for Cellulase Enzyme Production from Fungi Species Isolated From Degradation Corn Cob

  • 1. IOSR Journal of Pharmacy and Biological Sciences (IOSR-JPBS) e-ISSN: 2278-3008, p-ISSN:2319-7676. Volume 6, Issue 5 (May. – Jun. 2013), PP 15-19 www.iosrjournals.org www.iosrjournals.org 15 | Page Optimization of Cultural Parameters for Cellulase Enzyme Production from Fungi Species Isolated From Degradation Corn Cob Bamigboye, O. O. Department of Biology Emmanuel Alayande College of Education, Oyo. Abstract: Cellulalytic fungi synthesize cellulose enzyme for biodegradation of cellulose. This depends on various condition which include the source f isolation. This study was designed to determine the optimum condition necessary for cellulose production by fungi. Cellulose activities at different temperatures, pH and nitrogen sources by Rhizopus oryzae Aspergillus niger; A. flams, P. expansum and A. oryzae in liquid medium was studied and cellulose enzyme assay carried out by dinitrosalicylic acid method. All the fungal isolates have their highest cellulose activity at 400 c except Penicillium expansum whose highest value of 1.28mg/ml was obtained at 320 c. Cellulase produced 6m was found to be highest in all the isolate at pH 4.0 exception P expansum which occur at pH 5.5 (1.21mg/ml). The highest value e1.45mg/ml was obtained in A niger. Highest cellulose activity for A. niger, A. oryzae & P. expansum occurred in peptone. The study shows the need to determine the best physiological condition that allow for the optimal cellulose activity of fungal isolate. This will enhance their enzyme production. Key Word: Cellulase, fungi, pH, Nitrogen, temperature I. Introduction Cellulases a cosorfulm of free enzymes which comprises of enchoglucanase (β 1-4-D glucan-4- glucanolydrolase EC 3.2.1.4, carboxymethyl cellulalse, EC) Exoglucanase (β -1,4-D glucan-4-glucahydrolase EC allobiohydrolase, CBH) and cellobiases (β-d-glucoside glucohydrolase, EC 3.2.1.21, β-I, 4-D-glucosidase) which are found in many of the 57 glycosyl hydrolase families. (Siddigui et al. 2000) cellulose is the enzyme that hydrolyzes the β-1-4 glycosidic bonds I enzyme. Fungi are the most prominent cellulose producing microorganism (Immanuel et al 2007). Although a large number of microorganisms are capable of degrading cellulose, only a few of these produce significant quantities of cell free enzyme capable of completely hydrolyzing crystalline cellulose (Kooniinok, 2005). The need to optimize the cultural condition for igmnt maximum production of the enzyme is therefore essential. II. Materials and Method All chemicals used were reagent grade obtained from May & Baker and Sigma – Aldrich chemical company India. The fungi, Aspergillus niger, Rhizopus oryzae, Aspergilus oryzae, Penicillum expansum and Aspergillus flavus used in this study were isolated from degrading corn cob on Potato Dextrose agar and yeast extract agar. Pure cultures obtained were identified by conventional test and maintained on PDA slants. The five fungal isolates were separately grown and tested for production of cellulose in submerged culture in a chemically defined medium composed of KHzP0µ (1gl-1 ) MgS047Hz0 (0.5gl-1 ) yeast extract (1gl-1 ) Ccl2 2H20 Co.14gl-1 ) carboxymethyl cellulose 10g and thiavaine 0.0025gl-1 ). The cultures were grown at 270 c for 28 days, culture broth was sampled at different days during growth to determine enzyme productivity by carboxymethyl hydrolysis. Enzyme assay Cellulose activity was assayed by the determination of reducing sugar released from carboxymethyl cellulose (CMC). After growth had been allowed to proceed for the required length of time at the required temperature, the cultures were filtered through sintered glass crucibles and the cellulolytic activity of the filterates was determined using the method of Reese and Mandels (1963). The assay medium was 0.55% caroxymethyl cellulose (CMC) in 0.55m acetate buffer (pH 5.5) and 9ml of this were incubated with 1ml of the fungus filterate for 1 hour at 370 c. Filterates of the uninoculated control was also obtained and similarly assayed. To estimate the amount of reducing sugars released, 1ml of dinitrosalicylic acid (DNSA) reagent was added to 1ml of the filterate – CMC reaction mixture and the absorbance was determined at 540mm using an SP 600 spectrophotometer. The absorbance of standard aqueous solution of D-glucose at various concentrations (0-10mg per ml)
  • 2. Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated www.iosrjournals.org 16 | Page was determined and used to construct a graph of percentage absorbance as related to mg of glucose per ml. The amount of reducing sugar produced by 1ml of bacteria filterate from the CMC assay medium was calculated form this graph. Cellulolytic activity of the filterates was then expressed in term of the amount of total reducing sugars (RS) per ml. Effect of Temperature on Cellulase Activity Bottles of the chemically defined medium were inoculated and incubated at 28, 32 and 400 C. These were subsequently filtered and cellulose activity of the filtrate were determined at 0, 4, 7, 14, 21 and 28 days. Effect pH on Celulase Activity Some bottles of the chemically defined medium were inoculated and incubated at 270 C. Prior to inoculation the pH of the media was adjusted to pH 4.0, 5.5 and 7. The samples were filtered at 0,4, 7, 14, 21 and 28 days and cellulose activity at the afferent pH was determined. Effect of Nitrogen Source on Cellulase Activity The organisms were cultivated in the chemically defined media containing 1% carboxymethyl cellulose and supplemented with different Nitrogen sources of 1% (w/v). The nitrogen sources used include yeast extract, peptone, urea, (NH4)2 SO4 and NaNO2. These were incubated at 270 C and cellulose activity of the filtrate were determined at 0, 4, 7, 14, 21 and 28 days in the different Nitrogen sources. III. Result and Discussion Cellulose activity under different physiological conditions by Rhozopus oryzae, Aspergillus niger, A flavus, Penicillum expansum and A. oryzae was studied. All the fungal isolates showed cellulase activity, fungi of the geura Aspergillus and Penicillium have been reported as good cellulase producers (Milala et al., 2005, Hoffinem ad Wood, 1985, Abo State et al., 2010). The result of cellulase activity at different temperatures by the fungal isolates is shown in figure 1. Cellulase activity was found to be highest in 400 c in A niger with a value of 1.32mg/ml. Rhizopus oryzae at 320 c in day 14. All the fungal isolates had their highest reducing sugar production at 400 C except Penicillum expansum with the highest value of 1.28mg/ml on day 14. This agreed with Immaneul et al., (2007) who reported the optimum temperature for cellulase enzyme production by A. niger & A. fungatus at 400 C. The optimum pH for A niger, A flavus and Rhizopus oryzae was pH 4.0 as shown in figure 2 while P expansum and Aspergillus oryzae was at pH 5.5. Akiba et al., (1995) reported that cellulase production was high at pH 4 and 4.5 by A. niger optimum activity for A. niger, A oryzae and P expansum occurred in peptone as seen in Figure 3a & b. This correlates with the result of Guatam et al., (2011) who reported that peptone enhanced the production of cellulase by A niger on solid municipal waste residue.
  • 3. Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated www.iosrjournals.org 17 | Page Fig.6: Effect of temperature on the cellulase production by fungal isolates Cellulase activity at 32o C Cellulase activity at 40o C
  • 4. Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated www.iosrjournals.org 18 | Page Fig.7: Effect of pH on the cellulase production by fungal isolates Fig.8a: Effect of different nitrogen sources on cellulase production by fungal isolates
  • 5. Optimization Of Cultural Parameters For Cellulase Enzyme Production From Fungi Species Isolated www.iosrjournals.org 19 | Page Fig.8b:Effect of different nitrogen sources on cellulase production by fungi isolates References [1]. Abo-State, M.A.M., Hammad, A.E., Selin M. and Gannam R.B. 2010. Enhanced production of cellulases by Aspergillus sp on agricultural wastes by solid state fermentation. American – Eurasian Journal of Agricultural & Environmental Science. 402 – 410. [2]. Akiba, S., Kimura, K. and Kumugal, H. 1995. Purification and characterization of protein resistant cellulase from Aspergillus niger. Journal of Fermentation Bioengineering 79: 125 – 130 [3]. Gautam, S.P., Bundela, R.S., Pandey, A.K., Khan, J. Awashi, M.K. and Sarsaiya, S. 2011. Optimization for the production of cellulose enzyme from municipal solid waste residue by two novel cellulolytic Fungi Biotechnology Research Tnternational 2011: 8. [4]. Hoffman, R. M and Wood, T.M. 1985. Isolation and partial characterization of a mutant Penicillium for the saccharification of straw. Biotechnology. Bioengineering 27: 81-85. [5]. Immanuel, G., Akila Bhagavath, C. M. Iyapppa Raj, P., Essakking, P. and Palavessam A. 2007. Production and partial purification of cellulase by Aspergillus niger and A. fumigatus fermented in coir waste and saw dust. Internet Journal for Microbiology 3:1 – 17. [6]. Koomnok, C. 2005. Selection of cellulose producing thermophilic fungi. 31st congress on Science and Technology of Thailand. [7]. Milala, M.A., Shugaba, A., Gidado, A., Ene, A.C. and Wafar, J.A. 2005. Studies on the use of aricultural wastes for cellulase enzyme production by Aspergillus niger. Research Journal of Agriculture and biological Sciences 1. 4: 323-325. [8]. Nishida, Y., Suzuki K.I., Kumayai, Y., Tanaka, H., Inove, A. and Ojima, T. 2007. Isolation and primary structure of a cellulose from the Japanese sea urchin. Strongylocentrotus nudus. Biochime. 1-10. [9]. Siddigni, K.S., Saqib, A.A.N., Rashid, M.H. and Rajoka M.I. (2000). Carboxyl group modification significantly altered the kinetic of purified carboxymethylcellulase from Aspergillus niger. Enzyme and Microbial Technology Vol 27, No 7, Pp 467 – 474.