Bioscience Journal  |  2021  |  vol. 37, e37023  |  ISSN 1981-3163 
 

1 

 

 
 

Mehwish IQTEDAR1 , Sidra RIAZ1 , Saima Shehzad MIRZA2 , Mahwish AFTAB1 ,  

Afshan KALEEM1 , Roheena ABDULLAH1 , Ayesha AEIHTESHAM3 ,  

Farheen ASLAM3 , Myra WASIM3  
 
1 Department of Biotechnology, Lahore College for Women University, Lahore, Pakistan. 
2 Microbiology Laboratory, Punjab Bioenergy Institute, University of Agriculture, Faisalabad, Pakistan. 
3 Department of Zoology, Quid e Azam campus, University of the Punjab, Lahore. 

 
Corresponding author: 
Mehwish Iqtedar 
Email: miqtedar@gmail.com 
 
How to cite: IQTEDAR, M., et al. Bioethanol production from urban cellulosic waste employing Alcaligenes faecalis HI-1 isolated from gut of 
termite Heterotermes indicola. Bioscience Journal. 2021, 37, e37023. https://doi.org/10.14393/BJ-v37n0a2021-53598 

 
Abstract 
This study assessed the potential of termite gut inhabiting bacteria towards bioconversion of cellulosic waste 
into biofuel. Total seven bacterial isolates from the gut of Heterotermes indicola were isolated. Among all 
the isolates, HI-1 produced the largest zone upon primary screening.  Untreated paper had more cellulose 
content (73.03%) than acid (0.5%) treated paper that was used as a lignocellulosic substrate for 
saccharification. Among all the isolates tested, glucose yield (1.08mg/mL) was high for HI-1 isolate. Several 
factors were considered for optimizing augmented glucose yield (8.57mg/mL) and growth (8.07×108cfu/mL), 
such as temperature 37°C, pH 4.5, 5% (w/v) substrate concentration, 6 % bacterial inoculum size, agitation 
150 rpm with PEG 0.25 % and Ca2+ ions 0.002 g/L. Overall 8-fold increase in glucose yield was achieved. 
Enzyme activity of HI-1 showed higher endoglucanase 0.29 ± 0.01 (U/mL/min) and exoglucanase 0.15±0.01 
(U/mL/min) activity under optimum conditions, mentioned above. temperature 37°C, pH 4.5, substrate 
concentration 5%, inoculum size 6%, surfactants PEG 0.01%, ions Ca2+(0.002g/L) and agitation (120 rpm). 
Simultaneous saccharification and fermentation (SSF) of hydrolyzed office paper yielded 5.43mg/mL 
bioethanol. According to 16S rRNA sequence homology, the bacterial isolate H1 was identified as Alcaligenes 
faecalis. Bioethanol production from office paper untreated waste proved an effective strategy. Bacteria 
having natural tendency towards cellulosic waste consumption are promising for bioconversion of cellulosic 
waste to valuable products. 
 
Keywords: Bioethanol. Cellulolytic Bacteria. Office Paper. Termite Gut. 
 
1. Introduction 

Fossil fuel depletion causes increase in oil prices and petroleum products that led to a sharp interest 
in finding alternative energy sources. Biofuels can substitute fossil fuels and confer several advantages, ie., 
produced from renewable sources, lessens greenhouse gas emissions, and cost effective (Wyman 1994). In 
previous years, cellulases from cellulolytic bacteria have been applied in biofuel production due to their 
unique saccharolytic properties (Chang and Yao 2011). Cellulose, being an abundant biopolymer on earth, is 
the best resource for renewable energy (Rezaei et al. 2008). Bioethanol generated from cellulose in the form 
of agro-industrial waste has an improved eco-balance, as it does not compete with the food production, 
while on the other hand, it is readily accessible at low cost (Zhou et al. 2007). Paper materials are the largest 

BIOETHANOL PRODUCTION FROM URBAN CELLULOSIC 
WASTE EMPLOYING Alcaligenes faecalis HI-1 ISOLATED 

FROM GUT OF TERMITE Heterotermes indicola 

https://orcid.org/0000-0002-2350-3431
https://orcid.org/0000-0002-4673-9797
https://orcid.org/0000-0002-3287-9879
https://orcid.org/0000-0003-0131-328X
https://orcid.org/0000-0002-3972-0051
https://orcid.org/0000-0003-3932-6297
https://orcid.org/0000-0003-0533-6366
https://orcid.org/0000-0003-4380-2401
https://orcid.org/0000-0001-7720-2581


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Bioethanol production from urban cellulosic waste employing Alcaligenes faecalis HI-1 isolated from gut of termite Heterotermes indicola 

municipal solid waste product (Muttamara et al. 1994). Therefore, it is necessary to find ways for the 
conversion of wastepaper and its products into consumable value (Van Wyk 2003). Cellulose is the main 
synthesizing unit of paper which can enzymatically be transformed into sugar molecules that can later be 
fermented into ethanol.  

The guts of some insects like termites, beetles, leaf cutting ants and wood feeding roaches are highly 
adapted to diverse microflora and are considered highly competent natural bioreactors. Microtermes obesi, 
Microtermes mycophagous, Odontotermes obesus, Eremotermes paradoxalis and Microtermes unicolor are 
the most documented termite species from ecosystems of Pakistan (Ahmed et al. 2004). The microflora of 
the termite gut has a considerable impact on the degradation of cellulose from complex biopolymers like 
wood and other materials containing cellulose and hemicelluloses (Varma et al. 1994). Several facultative 
anaerobes have been isolated from the gut of different species of termites including Clostridium nzayombii 
and Homoacetogens termitida (Kane et al. 1991). Cellulolytic species of bacteria from certain phyla such as 
Thermotogea, Spirochaetes, Proteobacteria, Firmicutes, Actinobacteria, Bacteroids and Fibrobacteres have 
been reported from termite gut (Bergquist et al. 1999).  

To digest cellulose, cellulolytic microorganisms produce cellulases, an extracellular complex of 
multienzymes or as single polypeptides having multiple cellulosic domains. Cellulases have gained much 
attention because of their diversity and practical applications in pharmaceutical, fiber, textile industries, 
laundry detergents and in fermentation of biomass for biofuel production. To overcome the global energy 
crisis, the present study aimed to develop a new approach to investigate the potential of cellulolytic bacteria 
isolated from termite gut and employed to eco-friendly conversion of highly cellulosic urban waste (office 
paper) into reducible sugars that can later be fermented into bioethanol. 
 
2. Material and Methods 

Isolation of cellulolytic bacteria from termite gut 

Termites collected from different localities of Lahore were identified and their guts were removed 
according to Akhtar (1974). For isolation of cellulolytic bacteria, Carboxymethyl cellulose (CMC) media 
having 7 pH was used (Kasan et al. 2008). 
 
Primary screening of cellulase producing bacteria 

Congo red assay was performed to determine the cellulolytic activity of the isolates (Upadhaya et al. 
2012). Streaked plates of CMC media were incubated at 37°C for 48 hours. Colonies were flooded with Congo 
red stain (0.1%) for up to 20 min, later the stain was removed by flushing the plates with 1M NaCl. Diameters 
of clear zones around the colonies were measured.  
 
Pretreatment and proximate analysis of substrate 

Waste office paper was used as a cellulosic substrate, they were shred into small pieces (5 to 10mm) 
and were exposed to different pretreatments to analyze the % cellulose, moisture, dust, and lignin content 
as reported previously (Wayman et al. 1992). Pre-treatment was done by two methods, where in one 
method paper was exposed to steam in the presence of dilute sulphuric acid (0.5%) to remove lignin and 
hemicelluloses while the other was only steam treatment (Anwar et al. 2012). 
 
Secondary screening 

S-I media comprising (g/L) Peptone 5.0, Yeast extract 5.0, (NH4)2SO4 1.0, KH2PO4 1.0, MgSO4.7H2O 
0.3, KCl 0.5 and 1% substrate (office paper) having pH 7.  The media was inoculated with 1mL (108) of 
bacterial culture and incubated at 37°C for 5 days. Cell biomass was measured by spectrophotometric 
method at 600 nm, while reducing sugar was measured according to Miller (1959). 
 
 
 



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IQTEDAR, M., et al. 

Optimization 

Isolate having high cellulolytic activity was subjected to one factor optimization at different 
conditions such as temperature 37°C, 40°C and 55°C, pH 4.5, 7.0 and 8.5, substrate concentration 1, 5 and 
10%, inoculums size 2, 6 and 10%, and agitation 150rpm for 72 hours. Effects of surfactants such as SDS (0.25 
%), EDTA (0.25%), Triton X-100 (0.25%) and PEG (0.25%) on bacterial growth and reducing sugar yield were 
observed. Effects of metal ions such as FeSO4.7H2O (0.004g/L), ZnSO4.7H2O (0.003g/L) and CaCl2.2H2O 
(0.002g/L) were also studied on bacterial growth and cellulolytic activity. Media used for optimization was 
S-I. 
 
Enzyme activity: CMCase assay 

For CMCase assay 100µL of crude enzyme was mixed with 900µL of 1% CMC (1g of CMC dissolved in 
20mM of phosphate buffer having pH 7.0) kept at 50°C for 30 minutes. After incubation, the reaction was 
stopped by adding 1mL 3, 5-Dinitrosalicylic acid solution and kept in boiling water for 5 minutes and then 
cooled at room temperature. Reducing sugar was measured as reported previously (Miller 1959). Endo-β-1, 
4-glucanase activity was defined in one unit as; “amount of enzyme that can hydrolyze CMC and liberate 1µL 
glucose per minute at 50°C”. 

CMCase activity (IU/mL/min) = Absorbance × Standard Factor/ Incubation time. 
 
Enzyme activity: FPase assay 

For FPase assay, 1mL of culture aliquot was centrifuged at 10,000rpm for 10 minutes and then mixed 
with 50mg strip of Whatman filter paper (1×6cm), immersed in 1mL of 0.05M sodium phosphate buffer at 
pH 5.0 and incubated at 50°C for 60 minutes (Mandels et al., 1976). After incubation, 1mL of DNS solution 
was added and boiled for about 5 minutes and later cooled to room temperature. The reducing sugar was 
measured by DNS method (Miller 1959). The activity of exoglucanase in one unit was described as “enzyme 
amount that can release 1μmole reducing sugar in one min from filter paper”. 

FPase activity (IU/mL/min) = Absorbance × Standard Factor/ Incubation time. 
 
Simultaneous saccharification and fermentation (SSF) 

The yeast (Saccharomyces cerevisae) inoculum of 24 hours (106) was prepared in YPD media 
containing 1% yeast extract, 2% peptone and 5% glucose (Anwar et al. 2012). Simultaneous saccharification 
and fermentation was carried out in 250mL flasks that contained 100mL S-I medium. Media was aseptically 
inoculated with 5% yeast suspension (Saccharomyces cerevisae). Anaerobic conditions were established by 
fitting a rubber cork over each flask and one end of capillary was inserted into it whereas the outer tip was 
dipped in Ca(OH)2.  SSF experiments were performed under optimum conditions temperature 37°C, pH 4.5, 
substrate concentration 5%, inoculum size 6%, surfactants PEG 0.01%, ions Ca2+(0.002g/L) and agitation (120 
rpm) for a period of 3 days. The ethanol produced during SSF was estimated by HPLC.  
 
Ethanol estimation by HPLC 

The aliquots of fermented products were analyzed by HPLC (Shimadzu Corporation Koyoto, Japan) 
for estimation of ethanol yield. The samples were quantified by using the column CLC-NH2. The mobile phase 
used was acetonitrile and water (75:25, v/v) at 1mL/min. The injection volume was 10µL and column 
temperature was maintained at room temperature. 
 
Molecular identification 

Based on 16S rDNA sequence, identification of bacterial isolate H-SC1 was done through First Base 
Company (Singapore) using sequencing primers 785F 5' (GGA TTA GAT ACC CTG CTA) 3' and 907R 5' (CCG 
TCA ATT CMT TTR AGT TT) 3'. PCR primers used were 27F 5' (AGA GTT TGA TCM TGG CTC AG) 3' and 1492R 
5' (TAC GGY TAC CTT GTT ACG ACT T) 3'. The phylogenetic relationship was checked based on homology 
sequence by Neighbor joining method (Saitou and Nei 1987; Sambrook and Russell 2001). 



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Bioethanol production from urban cellulosic waste employing Alcaligenes faecalis HI-1 isolated from gut of termite Heterotermes indicola 

Statistical analysis 

All experiments were performed in triplicates. Data was analyzed using software SPSS 16.0. Duncan’s 
Multiple Range test was performed on the data to calculate significance difference (p≤0.05) between values 
obtained at different conditions. Intergroup differences in proximate analysis and secondary screening were 
calculated by applying t-test with significance at p≤0.05. 
 
3. Results and Discussion 

The present study was undertaken to investigate the potential of cellulolytic bacteria isolated from 
the gut of termites in bioconversion of highly cellulosic urban waste, and office paper into reducible sugars 
that was later fermented to bioethanol. Termite specie collected for this study was identified as 
Heterotermes indicola. Seven bacterial strains were isolated from H. indicola. Alcaligenes faecalis HI-1 from 
the current study was identified as facultative anaerobe. Other facultative anaerobes Bacillus cereus (Thayer 
1976; Ramin et al. 2009), Cellulomonas (Wenzel et al. 2002), Cellulomonas pachnodae (Bakalidou et al. 2002), 
Enterobacter aerogenes and Acinetobacter (Ramin et al. 2009) had been reported from guts of termites and 
were capable of lignocellulosic degradation. Alcaligenes has been reported from hind-gut of other termite 
specie such as Reticulitermes hesperus (Thayer 1976) and Odontotermes obesus (Devi et al. 2006) and 
identified as facultative wood digesting bacteria, however it is not previously reported from Heterotermes 
indicola. 
 
Primary screening 

In the primary screening all bacterial isolates produced clear zones against Congo red reagent which 
confirmed their cellulolytic nature (Figure 1A). 
 
Proximate analysis 

In the present study an important urban cellulosic waste, an office paper, has been considered a 
cheap substrate for bioethanol production (Coman et al. 2012). Utilization of office paper waste is beneficial 
in two ways as, on one side waste is managed and on the other side a useful product i.e., biofuel is produced. 
Different studies have been conducted on the bioconversion of wastepaper to bioethanol. Proximate 
analysis of pretreated and control samples revealed that cellulose and lignin content of untreated office 
paper were 73% higher as compared to pretreated office paper (67%). Whereas moisture and ash content 
were significantly (p≤0.05) higher in pretreated office paper (Table 1). There might be a possibility that 
sulfuric acid not only dissolved lignin but also affected cellulose content thereby producing undesirable 
products. In this context, it can be concluded that in case of wastepaper, pretreatment is not necessary for 
efficient bioconversion to bioethanol (Zhu et al. 2011).  
 
Table 1. Proximate analysis of untreated and pretreated (0.5% H2SO4) office paper. 

Substrate condition % Moisture % Ash % Cellulose % Lignin  

Untreated  5.18±0.02 2.33±0.01 73.03±0.04* 18.02±0.03* 
Pretreated  7.0±0.02* 2.52±0.02* 67.04±0.05 13±0.05 

Data has been analyzed by applying t-test with significance at p≤0.05 represented by *. 

 
Secondary screening 

All the isolates produced significantly higher (p≤0.05) glucose by utilizing untreated office paper as 
compared to pretreated office paper (Figure 1A). The highest glucose producing bacterial isolate was 
Alcaligenes faecalis HI-1 that produced 1.07±0.04 (mg/mL) of glucose with significantly (p≤0.05) higher cell 
biomass up to 2.60×108±0.004 (cells/mL) (Figure 1B). Previous studies focused only on the enzymatic 
conversion of wastepaper to sugar monomers (Van Wyk 2003). Whereas in the current study cellulolytic 
bacteria from the termite gut was used to convert cellulose waste to generate glucose monomers. 
 



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Figure 1. A – halozones formed by cellulolytic bacteria HI-1 in Congo red media; B – growth (108 cells/mL) 

and glucose yield (mg/mL) by cellulolytic bacterial isolates obtained from termite gut during secondary 
screening using office paper at different conditions. 

 
Optimization 

Enhanced cellulase activity relies heavily on various physicochemical factors and the current study 
focused on standardizing the physical and biochemical conditions for maximum enzyme activity and 
enhanced glucose concentration.  
 
Temperature 

Incubation temperature has considerable effect on the growth, survival and metabolism of 
microorganisms and their activities. Glucose release and bacterial growth were the two parameters studied 
during optimization using untreated office paper (Figure 2A). It was found that Alcaligenes faecalis HI-1 had 
significantly (p≤ 0.05) higher growth (3.33×108 ±0.02 cells/mL) with enhanced glucose yield (2.36±0.02 
mg/mL) at temperature 37 °C after 48 hours of incubation. As Alcaligenes faecalis HI-1 showed both 
increased cellulase activity and cell biomass with respect to glucose production at 37ºC, indicating that 
bacteria had efficiently utilized the substrate (office paper) by producing enzymes that efficiently converted 
the cellulose of substrate into glucose. Bacillus subtilis, Pseudomonas fluorescence, Bacillus 
sp., Cellulomonas and Micrococcus sp. have been reported to exhibit maximum growth and cellulase activity 
at temperature range from 37- 40°C (Immanuel et al. 2006). 
 
pH 

In the current study Alcaligenes faecalis HI-1 showed highest cell biomass and maximum glucose yield 
(mg/mL) at pH 4.5 with a fold increase in glucose yield. Increase in bacterial biomass was 3.86×108±0.02 
(cells/mL) and glucose yield was 3.43 ± 0.01 (mg/mL) after 48 hours of incubation (Figure 2B). pH had a 
profound effect on microorganisms and their activities. The change in the pH might have affected ionic 
bonding of the enzymes that may affect functional structure of the enzymes which degrade cellulose 
(Mussatto et al. 2008). Maximum activity of cellulolytic enzymes was reported between pH 4.2 to 5.8, 
whereas pH 4.8 has been considered optimal for the stability of cellulase enzymes (Pardo and Forchiassin 
1999). 
 
Substrate concentration 

Optimum concentration of substrate for Alcaligenes faecalis HI-1 was 5% that liberated glucose up 
to 5.02±0.03 (mg/mL) after 48 hours of incubation (Figure 2C). High degree of glucose yield obtained from 
hydrolysis of paper materials is also reported by other authors but at low substrate concentration (Wayman 
et al. 1992; Solange et al. 2008). 



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Bioethanol production from urban cellulosic waste employing Alcaligenes faecalis HI-1 isolated from gut of termite Heterotermes indicola 

 
Figure 2. Cell biomass and glucose production by Alcaligenes faecalis HI-1 under different physic-organic 

conditions. A – temperature; B – pH; C – substrate concentration; D – inoculum. Superscripts shows 
significant difference at p ≤ 0.05. 

 
Inoculum concentration 

Glucose yield increased further to 5.86±0.03 (mg/mL) by increasing the inoculum concentration to 
6%. Alcaligenes faecalis HI-1 showed 17% increase in glucose content with increased cell biomass at 6% 
inoculum in saccharification medium of office paper (Figure 2D). There is currently no work available in which 
Alcaligenes faecalis HI-1 bacterial inoculum is optimized for production of glucose during saccharification. 
Currently, a different approach is undertaken in which cellulose degradation potential of cellulolytic bacteria 
isolated from the termite gut was studied by utilizing office wastepaper.  
 
Agitation 

A significant increase in glucose yield (6.76±0.04mg/mL) was obtained with 48 hours of agitation 
(120rpm) (Figure 3A). Sufficient oxygen is necessary for the cells for efficient activity. 
 
Surfactants 

Among the surfactants used, a significant (p≤0.05) decrease in cell biomass as well as glucose 
production was observed with SDS, EDTA and Triton X100, while PEG (0.1%) enhanced the glucose yield to 
7.88±0.06 (mg/mL) after 24 hours (Figures 3B and 3C). PEG, because of its hydrophobic nature can modify 
the structure of substrate and therefore enhances the availability of cellulose for the enzyme activity. PEG 
adsorbs on the surface of lignin and repels the enzymes for unproductive binding (Sipos et al. 2010).  
 
Metal ionsm 

Addition of metal ions to the culture showed that Ca2+ ions increased the cell biomass to 
8.07×108±0.07(cells/mL) along with increasing the glucose yield (8.57±0.08mg/mL) to 8-fold after 24 hours 
of incubation (Figure 3D). Addition of Ca2+ ions (0.002g/L) to the media enhances cellulase production was 
also inferred by Shankar and Isaiarasu (2011).  
 



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IQTEDAR, M., et al. 

 
Figure 3. Cell biomass and glucose production by Alcaligenes faecalis HI-1 under different physic-organic 
conditions. A – agitation (120rpm); B – surfactants SDS (0.25 %), EDTA (0.25%), Triton X-100 (0.25%) and 

PEG (0.25%); C – optimizing different concentrations of PEG; D – metal ions FeSO4.7H2O (0.004g/L), 
ZnSO4.7H2O (0.003g/L) and CaCl2.2H2O (0.002g/L). Superscripts shows significant difference at p ≤ 0.05. 

 
Enzyme assays 

Alcaligenes faecalis HI-1 showed higher CMCase (endoglucanase) 0.29±0.01 (U/mL/min) and FPase 
(exoglucanase) 0.15±0.01 (U/mL/min) activity at 4.5 pH and at 37°C after 72 hours of incubation in the 
presence of PEG (0.1%) and calcium chloride (0.002g/L) (Figures 4A and 4B). Other authors have reported 
increase in CMCase and FPase productivity under similar conditions with pH range of 4.2 to 5.8 (Pardo and 
Forchiassin 1999; Abo-State el al. 2013). Whereas pH 4.8 has been considered optimal for stability of 
cellulase enzymes (Pardo and Forchiassin 1999). 

 
Simultaneous saccharification and fermentation (SSF) 

Fermentation was carried out for the saccharified substrate obtained from Alcaligenes faecalis HI-1 
under optimum conditions. Fermentation conditions were: 5% substrate concentration, 6% inoculums size, 
pH 4.5, 5% inoculum of S. cerevisae, agitation at 150rpm at 37˚C for a period of 3 days. Although temperature 
was not optimum for the yeast, it showed the metabolic activity. The ethanol yield obtained by 
saccharification of office wastepaper by cellulolytic strain Alcaligenes faecalis HI-1 was 5.43mg/mL (Figure 
5).  Bioethanol reported by enzymatic saccharification of wastepaper has been reported in another study by 
Ballesteros et al (2002). However, in these studies direct saccharification was done by using commercial 
enzymes. In the present study, the application of cellulolytic bacteria for cellulase production instead of 
using cellulase enzymes was a novel and cost-effective approach. By further refining the process the batch 
culture can be upgraded to continuous culture for continuous productivity of biofuel. 
 

 
 

 



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Bioethanol production from urban cellulosic waste employing Alcaligenes faecalis HI-1 isolated from gut of termite Heterotermes indicola 

 
Figure 4. A – CMCase and FPase activity (U/mL/min) of Alcaligenes faecalis HI-1 during 24 to 96 hrs of 

incubation under optimum conditions temperature 37°C, pH 4.5, substrate concentration 5%, inoculum 
size 6%, surfactants PEG 0.01%, ions Ca2+(0.002g/L) and agitation (120 rpm); B – synergistic increase in 

glucose yield with growth of Alcaligenes faecalis HI-1 under optimum conditions temperature 37°C, pH 4.5, 
substrate concentration 5%, inoculum size 6%, surfactants PEG 0.01%, ions Ca2+(0.002g/L) and agitation 

(120 rpm).  
 

 
Figure 5. HPLC analysis. A – peak showing retention time of standard ethanol; B – ethanol yield after 

fermentation of saccharified waste office paper by Alcaligenes faecalis H1-1. 
 
16S rRNA gene sequence analysis 

The amplified 16SrDNA sequence have 99% homology with specie Alcaligenes faecalis, so the isolate 
was designated as Alcaligenes faecalis HI-1. 
 
4. Conclusions 

The current study was a novel approach to produce bioethanol from office wastepaper by utilizing 
cellulolytic bacteria from the termite’s gut. New habitats must be searched for novel cellulolytic bacteria 
which can ultimately lead to novel enzymes with efficient activity. The data gathered in the present study 
revealed that cellulolytic bacteria Alcaligenes faecalis HI-1 isolated from gut of Heterotermes indicola was 
competent enough to breakdown the cellulosic content of office waste paper into glucose which can be 
fermented into bioethanol by Saccharomyces cerevisae. The office waste paper has the potential to be 
converted into bioethanol without any pretreatment and is relatively cost effective. This study provided 
ecofriendly bioethanol from cheap urban cellulosic waste (office paper) which can replace gasoline products 



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IQTEDAR, M., et al. 

and overcome the global energy crisis. In addition to bioethanol production, this study is also beneficial with 
respect to bioremediation of urban wastes where such bacteria can be employed for generating compost 
from urban waste. 

 
Authors' Contributions: IQTEDAR, M.: conception and design, acquisition of data; RIAZ, S.: conception and design, acquisition of data; MIRZA, 
S.S.: acquisition of data; AFTAB, M.: acquisition of data; KALEEM, A.: analysis and interpretation of data; ABDULLAH, R.: analysis and 
interpretation of data; AEIHTESHAM, A.: acquisition of data; ASLAM, F.: drafting the article; WASIM, M.: 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: Authors acknowledge the cooperation and guidance provide by the entomologist Prof. Dr. Muhammad Saeed Akhtar 
(Zoology Department, University of the Punjab, Lahore) in collection and identification of the termites. 
 

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Received: 06 April 2020 | Accepted: 12 October 2020 | Published: 12 May 2021 

 

 

  

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distribution, and reproduction in any medium, provided the original work is properly cited. 

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