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892 
Bioscience Journal  Original Article 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 
http://dx.doi.org/10.14393/BJ-v35n3a2019-42070 

EVALUATION OF Lysinibacillus SP, ISOLATED FROM Coptotermes 

curvignathus GUT, FOR THE DELIGNIFICATION OF OIL PALM RESIDUES 
 

AVALIAÇÃO DE Lysinibacillus SP, ISOLADO A PARTIR DO INTESTINO DE 
Coptotermes curvignathus, PARA A DESLIGNIFICAÇÃO DE RESÍDUOS DE ÓLEO 

DE PALMA (DENDÊ) 
 

Fadilah AYERONFE1; Angzzas KASSIM1*; Patricia HUNG2; Hafiz ZAINULABIDIN3; 

Nadiah ISHAK1; Sharfina SYARIFAH1; Ashuvila ARIPIN1 
1. Department of Chemical Engineering Technology, Faculty of Engineering Technology, Universiti Tun Hussein Onn Malaysia, 

86400, Johor, Malaysia; 2. Department of Crop Science, Faculty of Agriculture and Food Sciences, Universiti Putra Malaysia 97008, 
Sarawak, Malaysia; 3. Faculty of Mechanical and Manufacturing Engineering, Universiti Tun Hussein Onn Malaysia, 86400, Johor, 

Malaysia; oluwatosinfadu@gmail.com, angzzas@uthm.edu.my, patricia@upm.edu.my, nadiah.ishak89@gmail.com, 
sharfina.sms.20@gmail.com, ashuvila_2329@yahoo.com 

 

ABSTRACT. The application of ligninolytic bacteria and enzymes is a green pre-treatment alternative 
in the production of paper and biofuel from oil palm residues. In this study we investigated the ability of 
Lysinibacillus pakistanensis isolated from termite gut in degrading the lignin component of oil palm residues. 
The residues were biotreated with the bacterial strain in an aerated submerged fermentation system for 7 days at 
30 , pH 7 and compared with untreated control. Enzyme activities were determined using specific substrates. 
Peak lignin peroxidase (377.6 U/L), manganese peroxidase (218.19 U/L), and laccase (405.4 U/L) activity were 
recorded after 4,4, and 5 days of incubation respectively, using oil palm leaf as substrates. Lignin loss of 4.5%, 
5.7% and 6.6% in oil palm leaf, oil palm trunk and empty fruit bunch respectively was achieved after treatment 
with the microorganism. SEM images revealed structural changes in the cell wall of the residues. Pre-treatment 
with this bacterial strain has promising prospects of improving the efficiency of the pulping process in an 
environmentally safe manner. 

 
KEYWORDS: Biodelignification. Oil palm. Pulping. Lignin. Enzymes. 

 
INTRODUCTION 

 
The pulp and paper industry is one of the 

high demand sectors, resulting from the accelerating 
demands for paper-based products. Despite the 
increasing deployment of paperless communication 
with the advent of information technology, world 
paper consumption is continually increasing rather 
than decreasing as expected (SZABO et al., 2009). 
The removal of lignin is one of the key processes in 
paper production as it imparts stiffness on 
mechanical pulp fibres and yellow coloration on 
newsprints (PALIWAL et al., 2012). Moreover, the 
efficient hydrolysis of cellulose either for pulp or 
biofuel production is contingent upon degradation of 
lignin. Conventional methods of dissolving lignin in 
wood involve the use of chemicals and bleaching 
agents (LIEW et al., 2011; AYERONFE et al., 
2018). These processes do not only require high 
inputs of energy but also produce highly toxic 
effluents which are not environmental friendly 
(SUMATHI; HUNG, 2006).  The continuous 
increase in demand for paper products and growing 
environmental concerns necessitate the need to look 

towards technological improvement in the 
conventional pulping methods. 

To this effect, research on the use of 
microbial enzymes as a pre-treatment method has 
gained interest.  Pre-treatments of wood pulp with 
ligninolytic enzymes might provide milder and 
cleaner processes of delignification with no 
substantial loss to cellulose. This will not only save 
cost and energy, but will also improve the fibre 
bonding and the quality of paper produced (LIEW et 
al., 2011; FERRAZ, 2008).  

The ligninolytic capabilities of fungi have 
been explored over the years (CRISTINA et al., 
2013, OBRUCA et al., 2012; TANAKA et al. 
2012). However, long weeks of incubation and 
ligninase enzymes expression in fungi being a 
secondary metabolism have limited its commercial 
deployment (BUGG et al., 2008). Fungi lack of 
stability under practical conditions also underscores 
the need to explore bacterial ligninolytic potential. 
Exploring the diversity in lignin-degrading 
environments; such as soils in forestry locations and 
also in wood digesting insects, may also reveal 
novel enzymatic activities for lignin degradation 
(TAYLOR et al., 2012). 

Received: 01/05/18 
Accepted: 05/12/18 



893 

Evaluation of lysinibacillus sp…  AYERONFE; F. et al. 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 

Few reports exist on degradation of lignin 
by some termites species gut flora (GEIB et al. 
2008; Ke et al., 2011). GEIB et al. (2008) 
demonstrated the depolymerisation, demethylation 
and ring hydroxylation of lignin by gut microflora 
of Zootermopsis angusticollis and Anoplophora 
glabripennis. Sunil et al. (2016) investigated the 
lignin degrading ability of Trabulsiella sp, which 
was reported to have degraded up to 60% of 
guaiacylglycerol-β-guaiacyl ether (GGE). Lignin 
degrading capabilities of gut flora of of 
Rhynchophorus Ferrugineus have also been 
reported (KASSIM et al., 2016). There are also 
reports of aromatic degradation capabilities of 
bacteria isolated from termite guts. An aromatic-
degrading strain of Burkholderia and Citrobacter  
has been isolated from the gut C. formosanus 
(HARAZONO et al., 2003). A strain of 
Rhodococcus erythropolis capable of degrading 
polychlorinated biphenyl was isolated from 
Reticulitermes speratus (CHUNG et al., 1994). 
These reports put forward the practicability of 
termite symbiotic systems as screening sources for 
biocatalysts of industrial interest. However, the 
integration of enzymes secreted by termites gut 
microflora in pulping process has not been explored 
commercially, as much effort have been focused on 
lignin degradation by fungi (SINGHAL et al., 2015; 
SINGH et al., 2013)].  

Oil palm is an economical perennial crop 
widely cultivated in West Africa and Southeast 
Asia. In Malaysia, Oil palm plantation increased 
from 2.3 million in 1994 to about 3.87 million ha in 
2004 and to approximately 4.85 million ha in 2010 
(MPOB 2011). As a consequence, the palm oil 
production has recorded a rocketing upswing over 
the years, from about 7.8 million tons in 1995 to 
about 15 million tonnes in 2005 and to 18.8 million 
tonnes in 2012 (MPOB 2012).  

The explosive growth of the oil palm 
plantation has generated massive amounts of waste 
which are, at present, not efficiently utilized, 
thereby creating obstacles in replanting operations 
and colossal environmental concerns. The 
exploration of these oil palm residues in the 
production of value added products will not only 
help alleviate the disposal and environmental 
problems associated with it, but as well add value to 
the creation of rural agricultural-based economy. 
This study therefore, aimed to explore the green 
delignification of oil palm residues using bacteria 
isolated from termite’s gut. 
 
MATERIAL AND METHODS 

 

Microorganism 

Pure cultures of bacterial isolates from 
Coptotermes curvignathus gut was obtained from 
the Department of Crop Science, University Putra 
Malaysia, Sarawak. The isolate was re-streaked on 
LB agar plate for 24hrs and used for further 
analysis. Stock cultures were kept in 25% glycerol 
stock. 
 

Screening for lignin degrading potential of the 

isolate 

The lignin degrading capacity of the isolate 
was assayed for based on its ability to grow on 
Mineral salt media (MSM) supplemented with kraft 
lignin as sole carbon source, as well as its  ability to 
decolorise commercialized dyes. MSM-Lignin agar 
was prepared according to Bandounas et al. (2011). 
200 mL M9 Salt solution (64 g Na2HP04.7H20, 15 g 
KHPO4.7H20, 2.5 g NaCl, 5.0 g NH4Cl, 1 L ddH20), 
100 µ L 1M CaCl, 2 mL 1M MgSO4, 5 g of lignin 
powder, 15 g of agar powder, 800 ml of ddH2O and 
autoclaved at 120 ⁰C for 20 minutes. MSM-lignin 
agar plates were observed for colonies formation 
after incubation for 7 days at 37 ºC. Un-inoculated 
MSM-lignin plates served as controls. 

The isolates which showed good growth on 
MSM-Lignin agar were further screened using 
indicator dyes (methylene blue and azure B) as 
described by (Bandounas et al., 2011), colonies on 
MSM-Lignin agar were streaked on LB agar plates 
supplemented with 2g/l and 2g/l methylene blue and 
azure B respectively. The plates were incubated at 
37ºC for 72hrs and observed for zone of clearance.  
 

Identification of lignin degrading 

microorganisms  
The Microbial genomic DNA of the isolate 

was extracted from the pure using DNeasy Qiagen 
Kit according to manufacturer’s instruction. The 
16S rRNA gene amplification and sequencing were 
carried out by First Base Laboratory, Malaysia. The 
primers 27F (5’-AGAGTTTGATCMTGGCTCAG-
3’) and 1495R (5’-GGTTACCTTGTTACGACTT-
3’) were used for the amplification of the 16S rRNA 
gene. The PCR reactions were carried out at 95°C 
for 5 min, 30 cycles of 94°C for 40s, 55°C for 40s, 
72°C for 80s and a final extension of 7 min at 72°C, 
The PCR products were analysed on 0.8% (w/v) 
agarose gel and sequenced. All sequences were 
blasted using BLAST 
(http://blast.ncbi.nlm.nih.gov/blast/Blast.cgi) against 
the NCBI 16S ribosomal RNA sequences (Bacteria 
only) Database, excluding uncultured Bacteria 
bacterium (taxid: 77133). Sequence data were 
aligned with software package MEGA and the 



894 

Evaluation of lysinibacillus sp…  AYERONFE; F. et al. 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 

Phylogenetic tree was constructed using the 
neighbour-joining method. 

 

Biodegradation experiment 
The degradation experiment was conducted 

in an aerated submerged fermentation system 
(OBRUCA et al., 2012). To evaluate the lignin 
degrading capacity of the isolate, the isolate was 
cultured for a period of 7 days in LB medium 
containing 2g (oven dried weight) of the different 
oil palm residues (oil palm leaf (OPL), empty fruit 
bunch (EFB) and oil palm trunk (OPT)) as sole 
substrates. The residues were washed and 
autoclaved to get rid of contaminants prior to 
inoculation with the bacterial strain. Cultures were 
incubated at 30ºC at 120 rpm for 7 days in an 
incubator shaker. The control and cultured samples 
were centrifuged at 5000 rpm for 20 min to remove 
biomass and suspended solids. The supernatants 
containing the crude enzymes extract were used to 
determine the activity of ligninolytic enzymes. 
 

Ligninolytic enzymes assay 

Lignin peroxidase, LiP activity was 
measured by monitoring the oxidation of veratryl 
alcohol to veratryl aldehyde in the presence of H2O2, 
this was determined by the increase in absorbance at 
310nm. (ɛ310 = 9300 M-1 cm-1) in 100 mM citrate 
buffer (pH 3.0) at 30 oC. Manganese peroxidase, 
MnP activity was assayed spectrophotometrically 
with phenol red (ɛ610 = 22000 M-1 cm-1) as 
substrate in 50 mM sodium lactate at (pH 5.0) 30oC 
(OBRUCA et al., 2012). Laccase activity was 
measured using 2, 2-azinobis (3-
ethylbenzthiazoline-6- sulphonic acid) (ABTS) in 
0.1M acetate buffer (pH4.5) at 30 oC. Oxidation of 
ABTS was determined by the increase in A420 
(ɛ420 = 36,000 M-1 cm-1) (CHEN et al., 2012). The 
enzyme activity was expressed in international units 
(U), defined as the amount of enzyme required to 
convert 1 μmole of substrate to product per minute. 
Determination of lignin loss 

The lignin content of the control and 
biotreated biomass was determined prior to and after 
degradation experiment by treatment with cold 
sulphuric acid according to T222om-02 test.  
Percentage lignin loss was calculated as follows 
(Tappi Test T222om-02): 

 

     
Scanning electron microscopy 

At the end of the degradation experiment, 
the cultured samples were centrifuged to extract the 

delignified residues. The residues were washed and 
dried. The dried residues were sputter-coated with 
gold-palladium alloy to increase conductivity. 
Morphological changes in the samples, resulting 
from lignin degradation, were then observed under a 
scanning electron microscope (Carl Zeiss EVO LS 
10). 
 

Statistical analysis 
Data obtained were subjected to analysis of 

variance (ANOVA, p<0.05) using appropriate 
statistical software (Minitab). This test was used to 
determine the differences between the mean of the 
samples. The significance of the results was 
determined using p-value (p˂0.05). The results 
indicate the mean of three replicates, whereas the 
error bars in graphs denote standard error. 
 

RESULTS AND DISCUSSION 

 

Screening and identification of lignin degrading 

bacteria 
The bacterial strain was selected based on 

the ability to grow on mineral salt medium 
supplemented with kraft lignin as sole carbon 
source, as well as the ability to decolorise industrial 
dyes evident by the formation of zone of clearance 
around the plates. The selected bacterial isolate was 
identified based on 16S rRNA sequencing and was 
found to exhibit maximum homology with 
Lysinibacillus pakistanensis. The identification of 
Lysinibacillus sp from termite gut bacteria has not 
been reported neither has the ligninolytic potential 
of this genus been reported. However, Lysinbacillus 
spp were found to be present in dye contaminated 
soil (ANJANEYA et al., 2011; Liang et al. 2009). 
Saratale et al. (2003) isolated Lysinibacillus sp. 
RGS from dyes contaminated soil, capable of 
decolorising sulfonated dyes and textile effluents.  
Chaudhari et al. (2013) also reported the 
decolourization of reactive Orange M2R dye and 
chromate reduction by Lysinibacillus sp. KMK-A. 
These reports lend credence to the insinuation of a 
possible link between aromatic degradation and 
lignin metabolism, which is tenable given that much 
of the aromatic material found in the soil are lignin 
derivatives. 
 

Enzymes Assay 
The production of ligninolytic enzymes 

during degradation of oil palm residues by 
Lysinibacillus sp is being reported for the first time. 
The result indicates that Lysinibacillus sp can 
produce the three different ligninolytic enzymes 



895 

Evaluation of lysinibacillus sp…  AYERONFE; F. et al. 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 

(Lignin peroxidase, Manganese and laccase (Figure 1).  

0

50

100

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1 2 3 4 5 6 7

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ro
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oil palm leaf

empty fruit bunch

oil palm trunk

 
(a) 

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(b) 

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oil palm leaf

empty fruit bunch

oil palm trunk

 
(c) 

Figure 1. Lignin peroxidase (a), Laccase (b), and Manganese peroxidase (c) activity profile during the 
degradation of oil palm residues by Lysinibacillus sp. Results are mean of three independent 
samples with standard error 

 
However maximal production of lignin 

peroxidase varies with the substrates used. This 
variation could be attributed to the differences in the 
chemical compositions of the substrates. 
Ligninolytic enzymes production was higher using 
OPL as substrate than observed using EFB and 
OPT. The high lignin content of OPL (29.58%), 

compared to EFB (20.35%) and OPT could be a 
stimulant of ligninolytic enzymes production. This 
is consistent with a previous study on the production 
of ligninolytic enzymes by Pleurotus eryngii on 
agro-industrial wastes (AKPINAR; UREK 2014). It 
was reported that higher lignin contents in apricot 
wastes significantly stimulated the lignin 



896 

Evaluation of lysinibacillus sp…  AYERONFE; F. et al. 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 

metabolism when compared to pomegranate wastes. 
Laccase and lignin peroxidase were the 
predominating enzymes observed during pre-
treatment with the bacterial strain.  Lacasse activity 
was undetected after a day of incubation. 

However, activity steadily increases in the 
following 3 days of incubation, reaching maximal 
(405.4 U/L, 375.56 U/L, 376.66 U/L) in medium 
supplemented with oil palm leaf, empty fruit bunch 
and oil palm trunk respectively, after 5 days of 
incubation (Figure 1). Laccase activity thereafter 
declined. Decline in activity could result from the 
build-up of lignin degradation derivatives which 
may exhibit inhibitory effects on enzyme 
production. This is consistent with the results 
obtained during the degradation of kraft lignin by 
Pandoraea sp. B-6 isolated from bamboo chips. It 
was reported that laccase activity was maintained at 
a low level in the initial 2 days of incubation, peak 
activity (1120.6 U/L) was recorded after 5 days of 
incubation (Shi et al., 2013). The peak laccase 
activity after 5 days of incubation also correlates 
with peak growth/beginning of cell death in the 
isolates (data not shown). It could be that laccase 
enzymes mainly functions when the exponential 
growth of phase is almost over. A similar 
conclusion was reached in a previous study (Shi et 
al., 2013). Maximal lignin peroxidase activity was 
recorded between 4-6 days of incubation. A similar 
finding was reported during kraft lignin metabolism 
by bacterial strains isolated from oil palm plantation 
soils (HASHIMAH et al., 2013). Lignin peroxidase 
was highest (377.6 U/L) using with oil palm leaf as 
substrates, as compared to 372.92 U/L and 324. 
16U/L recorded using oil palm trunk and empty fruit 
bunch respectively. However, in contrast to decline 
in LiP activity observed during degradation of oil 
palm leaf, activity increases steadily throughout the 
degradation experiments using oil palm trunk and 
empty fruit bunch as substrates. MnP activity 
increases significantly in the initial 3-4 days of 
incubation, which was immediately followed by a 
marked decline. Interestingly, activity steadily 
increases in the following days of incubation. 
Decline in activity and a sudden rise in activity 
could be explained by the breakdown of inhibitory 
compounds to yield products that can be 
metabolised by the isolate. Maximal MnP activity 
observed in the initial 3 and 4 days also shows that 
manganese peroxidase production is crucial in lignin 
metabolism by Lysinibacillus sp. 
 

Determination of Lignin Loss 
Lignin losses in oil palm leaf, empty fruit 

bunch and oil palm trunk bio-treated with 

Lysinibacillus sp were 4.5%, 6.6% and 5.7% 
respectively. The loss in lignin content after 
degradation experiment could be attributed to the 
action of the ligninolytic enzymes which have also 
been implicated in previously reported lignin 
degradation experiments (KAMSANI et al., 2016; 
NTOUGIAS et al., 2015). There is a significant 
difference in the percentages of lignin loss recorded 
for each residue after treatment with Lysinibacillus 
sp. This could be due to the structural differences of 
the lignin component of each residue, as well as the 
degree of susceptibility of each residue to microbial 
degradation (SKYBA et al., 2013).  Colonization of 
wood by microorganism facilitates the softening of 
lignin thereby reducing the input of energy and 
chemicals required in subsequent pulping process. 
The higher the lignin loss, the more easily fibres 
will bleach with the utilization of few chemicals. 
This will ultimately improve the pulp production 
economics (FERRAZ et al., 2008; LIEW et al., 
2011). 

Percentage lignin loss during lignin 
degradation by white rot fungi on spruce wood 
shavings ranged from 2.5% - 7.2% (FACKLER et 
al., 2006). However, it took 2 weeks of incubation 
to achieve such extent of degradation in the fungi 
studied. Interestingly, only 7 days of incubation was 
sufficient to record comparable results in the 
bacterial strains involved in this study. Lignin 
metabolism being a primary metabolism rather than 
secondary as reported in fungi is propitious for 
potential biotechnological applications. Lignin loss 
of 4% was also reported during of biopulping of 
wood chips with Phlebia brevispora after 30 days 
incubation (FONSECA et al., 2014). Singh et al. 
(2010) reported a 9.35% reduction in lignin content 
of oil palm trunk after 4 weeks of treatment with 
white-rot fungus Trametes versicolor. 14.5% wheat 
straw-lignin was also degraded by Pleurotus eryngii 
(SKYBA et al., 2013). Nevertheless, production 
parameters were optimized to enhance lignin 
metabolism. Higher degradation could also be 
achieved by the selected bacterial strains in this 
study with longer incubation periods if production 
parameters were optimized. 

It is intriguing that maximum enzyme 
production was observed using oil palm leaf as 
substrates. However, higher lignin degradation was 
recorded in empty fruit bunch. This could result due 
to the low lignin content of empty fruit bunch 
thereby making it easily degraded than others.  

The structure of lignin, which is determined 
by the composition of monolignols, varies between 
and within species (SKYBA et al., 2013). The 
susceptibility of wood to degradation is largely 



897 

Evaluation of lysinibacillus sp…  AYERONFE; F. et al. 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 

dependent on the composition, as well as 
distribution of lignin in the different cell layers 
(SKYBA et al., 2013). Moreover, the level of 
enzymes activity sometimes does not correlate with 
the degree of lignin loss, which is consistent with 
previous reports (FACKLER et al., 2006; 
KNEZEVIC et al., 2013). In some cases, the 
reduction in the lignin content by the fungal species 
correlated with the enzymes expression pattern 
during lignin degradation by white rot fungi on 
spruce wood shavings (FACKLER et al., 2006). 
However, it was concluded that the cumulative total 
peroxidase activity of the fungal cultures after 14 
days with the decrease of the lignin content within 
the same time showed a very low correlation 
(FACKLER et al., 2006). Percentage lignin loss in 
Ceriporiopsis subvermispora correlated with 
increased peroxidase activity after 8 days of 
cultivation. However, delignification increases 
despite decreased peroxidase activity in the 
following days of cultivation. Treatment with 
Phlebia brevispora resulted in higher reduction in 
lignin content (6.2%), as compared to that with 
Dichomitus squalens BS1000.73 (4.4%) even 
though peroxidase activity in cultures of the latter 
was 19 fold higher than that observed in the cultures 
of the former. Knezevic et al. (2013) also reported 
that significant lignin breakdown seemed to occur in 
later stages of wheat straw fermentation, even 
though the peak of enzyme activity was reached 
much earlier. Apparently, the rate of lignin 
breakdown is not necessarily correlated with the 
level of enzyme activity. 
 

Scanning electron microscopy 

To gain insight into the structural changes 
in the cell wall of the residues, the treated and 
untreated samples were observed using a scanning 
electron microscope (Carl Zeiss EVO LS 10) 
(Figure 2). 

The surface morphology of the untreated 
samples (Fig. 2) appeared more compact and 
unaltered as opposed the rough and fractured 
surfaces of the treated samples. This modification 
could be attributed to the loss of lignin in the treated 
samples. Similar observations have been reported in 
previous studies (SINGHAL  et al., 2015; SINGH et 
al., 2013). Interestingly, such structural changes are 
crucial in pulping processes as less chemicals and 
energy will be required in subsequent chemical and 
mechanical pulping process respectively. Formation 
of pits on the surface of bagasse fibres was reported 
in the biopulping of bagasse by Cryptococcus 
albidus (SINGHAL  et al., 2015). Alteration in the 
cell wall of sugarcane bagasse as a result of acidic 

treatments has also been reported (MORAES 
ROCHA et al., 2011) 

 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 



898 

Evaluation of lysinibacillus sp…  AYERONFE; F. et al. 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 

 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 

(a)       (b) 
 

 
 

 

 

 

 

 

 

 

 

 

(c)        (d) 

 

 

 

 

 

 

 

 

 

 

 

(e)        (f) 

Figure 2. SEM micrographs of (a) control OPL; (b) biotreated OPL; (c) control EFB; (d) biotreated EFB; (e) 
control OPT; and (f) biotreated OPT 

 

 



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Evaluation of lysinibacillus sp…  AYERONFE; F. et al. 

Biosci. J., Uberlândia, v. 35, n. 3, p. 892-902, May/June. 2019 

CONCLUSIONS 
 
The application of ligninolytic bacteria and 

enzymes is a green pre-treatment alternative in the 
production of paper and biofuel from oil palm 
residues.  

In this study we investigated the ability of 
Lysinibacillus sp isolated from termite gut in 
degrading the lignin component of oil palm 
residues. All three ligninolytic enzymes were 
expressed by the organism. However, the level of 
production of the ligninolytic enzymes, LiP, MnP 
and Lac varies with the different carbon sources. 
This could be attributed to the nature and 
components of the different residues. Although, 
highest enzyme activity was recorded using oil palm 
leaf as substrate, the highest lignin loss was 
observed in empty fruit bunch, suggesting that the 
level of enzyme activities does not necessarily 

correlate with the extent of lignin degradation. 
Interestingly, these observations propose the 
utilization of these residues not only in paper 
production, but also as substrates in the cost-
effective production of ligininolytic enzymes for 
industrial applications. However, optimization of 
production parameters such as pH, temperature, 
presence of inducers, is necessary in order to 
enhance the degradation efficiency of the bacterial 
strain. 
 

ACKNOWLEDGEMENT 

 

This research was financially supported by 
Ministry of Science Technology and Innovation 
(SO27) and Fundamental Research Grant Scheme 
(1549). The authors like to thank technicians at the 
Department of Crop Science laboratory, Universiti 
Putra Malaysia. We are thankful for their support. 

 
 

RESUMO: A aplicação de bactérias e enzimas ligninolíticas é uma alternativa verde  de pré-tratamento 
na produção de papel e biocombustível a partir de resíduos de óleo de palma. Neste estudo, investigamos a 
capacidade de Lysinibacillus pakistanensis isolado do intestino de cupins na degradação do componente de 
lignina dos resíduos de dendê. Os resíduos foram biotratados com a estirpe bacteriana num sistema de 
fermentação submersa arejado durante 7 dias a 30ºC, pH 7 e comparados com controle não tratado. As 
atividades enzimáticas foram determinadas usando substratos específicos. Pico de lignina peroxidase (377,6 
U/L), peroxidase de manganês (218,19 U/L) e atividade de lacase (405,4 U/L) foram registradas após 4,4 e 5 
dias de incubação, respectivamente, utilizando como substratos a folha da palmeira de dendê. A perda de 
lignina de 4,5%, 5,7% e 6,6% na folha da palmeira, no tronco do dendezeiro e cacho de frutas vazio, 
respectivamente, foi alcançada após o tratamento com o microorganismo. Imagens de MEV revelaram 
alterações estruturais na parede celular dos resíduos. O pré-tratamento com esta cepa bacteriana tem 
perspectivas promissoras de melhorar a eficiência do processo de polpação de maneira ambientalmente segura. 
 

PALAVRAS-CHAVE: Biodelignificação. Óleo de palma. Polpação. Lignina. Enzimas. 
 
 
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