Bioscience Journal  |  2021  |  vol. 37, e37021  |  ISSN 1981-3163 
 

1 

 

 
 

Roheena ABDULLAH1 , Ammara AKHTAR1 , Kinza NISAR1 , Afshan KALEEM1 ,  

Mehwish IQTEDAR1 , Tehreema IFTIKHAR2 , Faiza SALEEM1 , Farheen ASLAM1  
 
1 Department of Biotechnology, Lahore College for Women University, Lahore, Pakistan. 
2 Department of Botany, Government College University, Lahore, Pakistan. 

 
Corresponding author: 
Roheena Abdullah 
Email: roheena_abdullah@yahoo.com 
 
How to cite: ABDULLAH, R., et al. Process optimization for enhanced production of cellulases form locally isolated fungal strain by submerged 
fermentation. Bioscience Journal. 2021, 37, e37021. https://doi.org/10.14393/BJ-v37n0a2021-53815 

 
Abstract 
Cellulase has myriad applications in various sectors like pharmaceuticals, textile, detergents, animal feed 
and bioethanol production, etc. The current study focuses on the isolation, screening and optimization of 
fungal strain through one factor at a time technique for enhanced cellulase production.  In current study 
sixteen different fungal cultures were isolated and the culture which quantitatively exhibits higher titers of 
cellulase activity was identified both morphologically and molecularly by 18S rDNA and designated as 
Aspergillus niger ABT11. Different parameters like fermentation medium, volume, temperature, pH and 
nutritional components were optimized. The highest CMCase and FPase activities  was achieved in 100ml of 
M5 medium in the presence of 1% lactose and sodium nitrate at 30 oC, pH5 after 72 hours. The result 
revealed A. niger can be a potential candidate for scale up studies. 
 
Keywords: Aspergillus niger. Cellulase. CMCase. FPase. Molecular Characterization. 
 
1. Introduction 

Cellulose is an insoluble crystalline polysaccharide of repeating units of glucose that is linked through 
β-1, 4-glucosidic bonds. The group of cellulases possess the ability of completely hydrolyse the cellulose and 
needed three main components i.e. Endoglucanases, Exoglucanases and β-glucosidases. Endoglucanases act 
on the amorphous region of cellulose while Exoglucanase acts on crystalline region, resulting in the 
production of cellobiose units which are further attacked by β-glucosidase and ultimately production of 
glucose (Oliveira et al. 2019). Cellulases has multifarious applications in different sectors like textile, 
pharmaceuticals, detergents and animal feed , food and paper etc. (Bhat 2000).    

The chief skeletal constituent of plant cell wall is cellulose, which is found along with hemicelluloses, 
pectin and lignin. Cellulases can be obtained from microorganisms, including fungi and bacteria. However,  
filamentous fungi are preferred over bacteria because of their ability to penetrate deep in cellulosic 
substrates by using their  hyphal extensions and thus showing their enzyme systems in confined cavities 
within the cellulosic particles as compared to bacteria that cannot penetrate deep in to the substrate (Lynd  
et al. 2002). In addition to this fungal cellulases has the capability to act  on both amorphous and crystalline 
structures of cellulose in contrast to bacteria (Damisa  et al. 2011). Most commonly used fungal species for 
the production of cellulases are Aspergillus niger, Penicillium dupontii, Fusarium oxysporum and Trichoderma 
viride etc. (Hussain et al. 2012).  

PROCESS OPTIMIZATION FOR ENHANCED PRODUCTION OF 
CELLULASES FORM LOCALLY ISOLATED FUNGAL STRAIN BY 

SUBMERGED FERMENTATION 

https://orcid.org/0000-0003-3932-6297
https://orcid.org/0000-0002-3497-5004
https://orcid.org/0000-0003-0424-4320
https://orcid.org/0000-0002-3972-0051
https://orcid.org/0000-0002-2350-3431
https://orcid.org/0000-0001-5369-0859
https://orcid.org/0000-0001-7697-7377
https://orcid.org/0000-0003-4380-2401


Bioscience Journal  |  2021  |  vol. 37, e37021  |  https://doi.org/10.14393/BJ-v37n0a2021-53815 

 

 
2 

Process optimization for enhanced production of cellulases form locally isolated fungal strain by submerged fermentation 

Presently the production of cellulase has extensively been studied, but the relatively high productivity 
costs have hindered the frequent use of enzyme for industrial applications. So there is a dire need to improve 
the economics of cellulase production either by reducing the productivity cost or enhancing the enzyme 
activities.  The production cost is basically associated with the enzyme productivity of microbial strain as well 
as the type of fermentation media used (Akula and Golla 2018). Keeping in view the above consideration the 
current work focused on the process optimization for enhanced cellulase production by locally isolated 
fungal strain. 
 
2. Material and Methods 

Isolation of cellulolytic fungi 
Different fungal strains having cellulolytic potential were isolated from different natural sources such 

as the compost and different soil samples were collected from different areas of Punjab, Pakistan. The 
isolation of fungi  was carried out using serial dilution method (Reddy et al. 2014). The primary screening 
was performed on the basis of the zone of cellulose hydrolysis (Kim  et al. 2006), while secondary screening 
was performed via submerged fermentation. The strain showed highest cellulolytic potential was identified 
both morphologically and molecularly. 
 
Molecular characterization 

Molecular characterization was carried out according to Nisar et al. (2020). 
 
Pretreatment of substrate 

The small pieces of sugar cane bagasse were sun dried and after this treated with sodium hydroxide 
(4%) by dipping in the solution for 24 hours. The sample was then washed with water and dried in oven for 
3-4 h at 60°C (Haq et al. 2006).  
 
Fermentation 

The sterilized fermentation medium (100ml) was prepared in 250 ml Erlenmeyer flasks was 
inoculated with 1ml of conidial inoculum. All the flasks were incubated at 30⁰C for 72 hours in a shaking 
incubator with 160 rpm agitation speed. Later, the fermented broth was centrifuged for 15-20 min at 6000 
× g. The clear supernatant was used for the determination of CMCase and FPase activity (da Silva et al. 2016). 
 
Evaluation of different fermentation media used for cellulase production 

Following media (g/l) was evaluated to produce cellulases: 
M1:  3 sugar cane bagasse; 1.4 (NH4)2SO4; 0.3 urea; 2.0 KH2PO4; 0.3 CaCl2;0.3 MgSO4.7H2O; 0.75 

tryptone; 0.005 FeSO4.7H2O; 0.0014 ZnSO4; 0.0016 MnSO4.3H2O; 2 Tween-80 (Tao  et al. 2010). 
M2: 1.0 KH2PO4; KCl 0.5; (NH4)2SO4 0.5; MgSO4.7H2O 0.2; L-asparginine 0.5; CaCl2 0.1; yeast extract 

0.5; 10 Wheat bran (Haq  et al. 2005). 
M3: Urea 0.3; 1.4 (NH4)2SO4; KH2PO4 2.0; 0.4 CaCl2·2H2O; 0.3 MgSO4·4H2O; 1.0 peptone; 0.005 

FeSO4·7H2O; 0.0016 MnSO4·4H2O; 0.0014 ZnSO4·7H2O; 0.002 CoCl2·6H2O; 2.0 Tween 80; 10 Whatman No.1 
(Karnchanatat  et al. 2008). 

M4:  50 Wheat bran, ammonium nitrate 8 (Padmavathi  et al. 2012). 
M5: 2g Wheat straw, 50 ml of Mandel and Sternberg’s mineral medium containing (g/l): 1.4 

(NH4)2SO4; 2.0 KH2PO4; 0.3 CaCl2; 0.0003 MgSO4. 7H2O; 0.005 FeSO4.7 H2O; 0.0016 MnSO4. H2O; 0.0014 
ZnSO4.7H2O; 0.002 CoCl2 (Singh et al. 2009). 

M6: KH2PO4 2.0; MgSO4.7H2O 0.3; CaCl2.2H2O 0.3; (NH4)2SO4 1.4; FeSO4.7H2O 0.005; MnSO4. H2O 
0.0016; ZnSO4.7 H2O 0.0014; CoCl2.6H2O 0.002; peptone 1.0; Tween 80 1.0; 10 CMC  (Karnchanatat  et al. 
2008). 
 
Assay of FPase and CMCase   

FPase and CMCase assay was performed following the Gao et al. (2008). For the determination of 
FPase 50 mg of Whatman filter paper (1×6 cm) along with 0.5ml of supernatant and 0.5ml of 0.1M citrate 
buffer (pH, 5.0) was incubated at 60°C for half an hour. Blank was also run side by side. After incubation the 



Bioscience Journal  |  2021  |  vol. 37, e37021  |  https://doi.org/10.14393/BJ-v37n0a2021-53815 

 
 

 
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ABDULLAH, R., et al. 

reducing sugar was measured by DNS method (Miller 1959). The absorbance was noted at 546nm using 
spectrophotometer. For the determination of CMCase above mentioned procedure was followed except 
Whatman filter paper strip was replaced by 0.5ml of CMCase (1%) prepared in citrate buffer (0.1 M; pH5). 

One unit of FPase and CMCase activity was defined as the“ quantity of enzyme requisite to release 1 
µmol of reducing sugars from appropriate substrate  under standard assay conditions” (Chellapandi and Jani 
2008). 
 
Determination of total protein and dry cell mass 

Dry cell mass was determined by following the method of Irfan et al. (2011) and Total protein was 
estimated by Bradford et al. (1976). The    Bovine serum albumin was used as a standard. 
 
Statistical analysis 

All the experimental data was analyzed statistically using SPSS (17.0).   
 
Bioinformatics analysis 

Sequence was analyzed using BLAST and phylogenetic tree was constructed through MEGA 7 (Kumar 
et al. 2018). 
 
3. Results and Discussion 

Due to increasing demand of cellulases and consequently higher productivity it becomes essential to 
give more attention to explore the hyper productive microbial strain and process optimization strategies. In 
the current study sixteen different fungal strains were screened for the desire enzyme production (data not 
shown). The fungi possessing the highest cellulolytic ability was identified both on morphological and 
molecular basis (18S rDNA) by using universal primers ITS-1(F): TCCGTAGGTGAACCTGCGG and ITS-4 (R): 
TCCTCCGCTTATTGATATGC and found to be Aspergillus niger. The Blast analysis clearly indicates the isolate 
belong to Aspergillus genus and show 99% similarity with Aspergillus niger (Figure 1). This strain was 
designated as Aspergillus niger ABT11. The production of cellulases through fermentation is multivariable 
process and depends upon the genetic nature of organism, medium composition and physicochemical 
properties. All these factors dramatically affect the enzyme productivity. In this study six different media 
were tested (Figure 2) and M5 medium found to the best medium the reason could be that it contains wheat 
straw which serve as a carbon source for the growth of fungi and subsequently for the enzyme production. 
In addition to this it also contains low lignin contents. Our findings agree with the Gori and Malana (2010) 
who stated wheat straw as a best substrate for cellulase production. 
 

 
Figure 1. Phylogenetic relationship of Aspergillus niger and related filamentous fungi  

based on their ITS sequences. 
 
 
 
 



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Process optimization for enhanced production of cellulases form locally isolated fungal strain by submerged fermentation 

 
Figure 2. Effect of media on the cellulase production. 

 
The time of fermentation greatly influences the product formation. In this investigation fermentation 

is carried out up to 120h (Figure 3A). The enzyme activity was increased with the rise in the fermentation 
time till 72hours. After this a gradual decrease occurs in the activity of the enzyme and drastic reduction was 
observed at 120h. The reason could be the exhaustion of nutrients or production of toxic substance may 
occur which retard the growth of organism and subsequently CMCase and FPase production (Malik et al.  
2010). Our studies were contradictory to Karthikeyan et al. (2010) who investigated 120h was an optimum 
fermentation period for the production of cellulase. However, our studies were similar to Gori and Malana 
(2010) who reported 72h as a best incubation time for cellulase production. 

A critical feature in fungal enzyme production is the optimal temperature that stimulates catalytic 
site optimum saturation, whereas higher temperature ultimately denatures the enzyme (Geoffry et al. 2018). 
The influence of varying the range of incubation temperature from 25-45°C was recorded (Figure 3B). The 
maximal CMCase and FPase activities was noted at 30°C further  rise in temperature results decrease in the 
enzyme activity. Higher temperature during enzyme production inhibits the growth of fungi and cause 
denaturation of protein and consequently low enzyme yield (Yoon et al. 2014). The current results disagree 
with El-Hadi et al. (2014) who reported 37°C for cellulase production. The influence of varying media volume 
(25 - 200 ml) on the cellulase production was investigated (Figure 3C). The highest production of CMCase 
(6.52 U/ml) and FPase (6.62 U/ml) was achieved in 100ml.  Further increase in volume caused the enzyme 
production to decrease. The reason lies in the fact that in the shake flask supply of oxygen is related to the 
volume of the medium when the volume of medium increase or decrease above the optimal level the growth 
of fungi and corresponding yield of the enzymes was reduced accordingly (Carlile et al. 2001). 

The pH of medium has a strong influence on fungal growth, metabolism and enzymatic processes. It 
also affects the transport of different compounds through cell membrane. Effect of pH variations on the 
production of cellulase was evaluated (Figure 3D). The varying pH ranging from 3-10 was screened. The pH 
5 proved to be best and gave maximal CMCase (7.42 U/ml) and FPase (7.65 U/ml) productivity.  Any change 
more or less than the optimal state result in the less production of enzyme. The optimal pH is needed to 
retain three dimension shape of the enzyme active site. The variation in pH causes loss in shape of enzyme 
because of changes in ionic bonding of enzyme (Mmango-Kaseke et al. 2016). Akula and Golla (2018) 
reported pH 5 for optimal cellulase production which was comparable to our finding. 

Different carbon sources like sucrose, glucose, fructose, maltose, lactose, xylose were screened for 
the production of cellulase (Figure 4A). Lactose at 1% concentration gave the maximal production of CMCase 
and FPase (13.64 U/ml; 13.51 U/ml) respectively (Figure 4B). However, glucose inhibits the synthesis of 
cellulase.  Many workers reported that lactose act as a strong inducer to produce cellulase (Akula and Golla 
2016; EL-Hadi et al. 2014). The impact of using varying types of nitrogen sources including both organic and 



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ABDULLAH, R., et al. 

inorganic i.e. ammonium sulphate, ammonium chloride, ammonium nitrate, meat extract, yeast extract, 
peptone, sodium nitrate and urea were evaluated (Figure 4C). Among all the above used nitrogen sources 
sodium nitrate gave highest activity of CMCase (13.95 U/ml) and FPase (13.82 U/ml). All other nitrogen 
sources exhibited less enzyme production (Figure 4D). So, different NaNO3 concentrations (0.5 to 2%) were 
screened. The highest CMCase (14.86 IU/ml) and FPase (14.66 U/ml) activity was achieved at 1%. Our studies 
are comparable to Abd-Elrsoul and Bakhiet (2018) who also reported sodium nitrate as a best nitrogen 
source, but contrary to Pothiraj and Eyini (2007) who reported that optimal cellulase production can be 
achieved from organic nitrogen sources, such as a yeast extract and peptone. 
 

 
Figure 3. Influence of different parameters on cellulase production. A – time of incubation;  

B – temperature; C – volume; D – pH. 
 

 
Figure 4. Influence of nutritional factors on cellulase production. A – carbon sources; B – concentration of 

lactose; C – nitrogen sources; D – sodium nitrate concentration. 



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Process optimization for enhanced production of cellulases form locally isolated fungal strain by submerged fermentation 

4. Conclusions 

The indigenously isolated Aspergillus niger ABT11 after optimization of cultural conditions exhibited 
the highest cellulase producing potential.  The result indicates Aspergillus niger ABT1I can be promising 
candidate for economic production of cellulases by using wheat straw as a substrate for large scale 
production. 
 
Authors' Contributions: ABDULLAH, R.: conception and design, acquisition of data, analysis and interpretation of data, and drafting the article; 
AKHTAR, A.: acquisition of data; NISAR, K.: acquisition of data, and drafting the article; KALEEM, A.: conception and design, acquisition of data, 
analysis and interpretation of data, and drafting the article; IQTEDAR, M.: conception and design, acquisition of data, analysis and interpretation 
of data and drafting the article; IFTIKHAR, T.: drafting the article; SALEEM, F.: conception and design, acquisition of data, analysis and 
interpretation of data and drafting the article; ASLAM, F.: conception and design, acquisition of data, analysis and interpretation of data and 
drafting the article. All authors have read and approved the final version of the manuscript. 
 
Conflicts of Interest: The authors declare no conflicts of interest. 
 
Ethics Approval: Not applicable. 
 
Acknowledgments: Not applicable. 
 
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Received: 16 April 2020| Accepted: 18 October 2020| Published: 12 May 2021 

 

 

  

This is an Open Access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, 
distribution, and reproduction in any medium, provided the original work is properly cited. 

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