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212 
Bioscience Journal  Original Article 

Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

PRODUCTION AND CHARACTERIZATION OF A THERMOSTABLE Β-
GLUCOSIDASE FROM Myceliophthora heterothallica 

 
PRODUÇÃO E CARACTERIZAÇÃO DE UMA Β-GLICOSIDASE TERMOESTÁVEL 

DE Myceliophthora heterothallica 
 

Maria Eduarda da Mata MARTINS1; Eduardo da Silva MARTINS2;  
Heytor Lemos MARTINS3 

1. Tecnóloga em Alimentos, Universidade do Estado de Minas Gerais, Frutal, MG, Brasil. 2. Professor, Doutor, Laboratório de 
Microbiologia, Departamento de Ciências Exatas e da Terra, Universidade do Estado de Minas Gerais, Frutal, MG, Brasil. 3. Mestrando 

em Ciências Ambientais, Universidade do Estado de Minas Gerais, Frutal, MG, Brasil. 
 

ABSTRACT: The conversion of biomass from agro-industrial residues into bioproducts is of great 
interest, especially to Brazil, where bioenergy has a huge potential for development. Enzymes involved in 
biodegradation of lignocellulosic biomass are those of the cellulase system, of which β-glucosidase is a 
constituent. The production and characterization of β-glucosidase by the thermophilic fungus Myceliophthora 
heterothallica by solid-state cultivation on different agro-industrial residues (sugarcane bagasse, sugarcane 
straw, wheat bran and a mixture of these three materials (1:1:1 w/w) was evaluated. Solid-state cultivation were 
conducted in 250 mL Erlenmeyer flasks, with 5 g of each substrate. Different culture parameters, such as 
supplementary nutrient solution to the substrate, supplementary nutrient solution pH, initial substrate moisture 
and fungus incubation temperature, were evaluated to establish conditions of higher enzyme production by the 
fungus  The greatest production of enzymes occurred in a mixture of wheat bran, sugarcane bagasse and straw 
bagasse (1:1:1). The activity of β-glucosidase was greater under the following conditions: nutrient solution 
composed of NH4NO3, MgSO4.7H2O and (NH4)2SO4 (0.1%), at pH 4.5 or 6.0, fungus incubation at 40°C or 
45°C, initial moisture of substrate at 80%. Enzyme presented optimum pH at pH 5.0 and good pH stability. 
Best temperature was 65°C and enzyme showed 100% stability for 1h, up to 60°C. The use of agro-industrial 
residues provided good production of β-glucosidase by fungus, with enzyme having the characteristics 
desirable from the industrial application. 

 
KEYWORDS: β-glucosidase. Fungus. Myceliophthora heterothallica. Solid-state cultivation. 

 
INTRODUCTION 
 

Solid-state cultivation (SSC) is an 
increasingly employed process to obtain microbial 
products for agricultural residues as substrates for 
microbial growth, with value aggregation (GAO et 
al., 2008; ASGHER et al., 2016). The application of 
residues to bioprocesses has become important from 
the environmental point of view since it reduces 
problems related to their inadequate management 
and consequent environmental damages. In addition, 
the materials´ low cost and high availability make 
them excellent alternative substrates for obtaining 
microbial products used in industrial processes 
(PANDEY et al., 2000). 

One of the most prominent sectors in Brazil, 
especially in the states of São Paulo and Minas 
Gerais, is the sugar-energy sector, due to the 
establishment and expansion of sugarcane plants in 
several municipalities (OLIVEIRA; MENDES, 
2014). Since there is a great generation of sugar 
cane residues, such as straw and bagasse, the latter 
are potential substrates to obtain bioproducts. 

Further, besides the use of biomass residues 
from sugarcane to generate electricity, industries 
produce second-generation ethanol with microbial 
enzymes derived from the residue, reported by 
scientific studies. However, obtaining fermentable 
sugars through the degradation of these materials 
may also enhance the production of several other 
industrial products, such as biosurfactants, flavoring 
agents, organic acids and others (SANTOS et al., 
2012). 

One of the most important groups of 
enzymes in the lignocellulosic biomass degradation 
is cellulases, an enzymatic complex whose enzymes 
act synergistically in the transformation of cellulose 
into monomers and glucose dimers. They are 
generally subdivided into three classes: endo-1,4-β-
D-glucanases or endoglucanases (which break the 
glycosidic bonds of cellulose chains and create new 
terminals); exo-1,4-β-D-glucanases or 
cellobiohydrolases (responsible for terminal action 
leading to cellobiosis) and 1,4-β-D-glucosidases 
(which hydrolyze cellobiose to glucose) (YOON et 
al., 2014). 

Received: 01/04/19 
Accepted: 10/10/19 



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Production and characterization…   MARTINS, M. E. M.; MARTINS, E. S.; MARTINS, H. L. 

Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

β-Glucosidases increase the overall yield of 
fermentable sugars and reduce the inhibitory effect 
of cellobiose in other cellulolytic enzymes. 
Consequently, they continue the enzymatic 
hydrolysis process (RANI et al., 2014). These 
enzymes have several applications in industrial 
processes, including the conversion of glycosides 
from isoflavones to aglycones, which have 
antioxidant activities, and are more easily absorbed 
by the human intestine, providing such health 
benefits as the prevention of certain types of cancer 
and as risk-reduction factors against cardiovascular 
diseases, osteoporosis, menopausal symptoms and 
diabetes. In wine production, the addition of 
microbial β-glucosidase in vinification processes 
enhances the release of volatile terpenes 
(deglycosylated by the enzyme action) and 
contributes towards the wine´s aromatic 
composition (SINGHANIA et al., 2013; SANTOS 
et al., 2016). 

Thermophilic microorganisms have been 
studied to produce generally thermostable enzymes 
(MARTINS et al., 2013). Enzymatic mixtures used 
for the degradation of polysaccharides derived from 
biomass (cellulose, hemicellulose, pectin) are 
commonly produced by mesophilic fungal strains 
belonging to the genera Trichoderma and 
Aspergillus (VAN DEN BRINK; DE VRIES, 2011). 
However, thermophilic microorganisms are reported 
to contain enzymes which are more resistant to 
denaturation and proteolysis (KUMAR; 
NUSSINOV, 2001). 

Enzyme thermal stability allow the 
saccharification of biomass polysaccharides at high 
temperatures and, consequently, decrease in reaction 
time, increase in greater mass transfer and the 
composition of substrate viscosity, which optimizes 
the processes in which they act, with decrease of 
costs. Thus, the alternative is the study of other 
microorganisms that produce thermostable enzymes 
that degrade plant biomass (BERKA et al., 2011; 
VAN DEN BRINK et al., 2013). 

Myceliophthora is a genus composed of 
mesophilic and thermophilic fungi, which includes 
10 species. M. thermophila, M. heterothallica, M. 
hinnulea and M. fergusii were described as 
thermophilic and regarded as industrially interesting 
enzyme producers due to their high activity and 
thermostability rates (MAIJALA et al., 2012). 
Current study evaluated β-glucosidase production 
by thermophilic fungus Myceliophthora 
heterothallica in solid-state cultivation using agro-
industrial residues as substrates, to determine the 
effect of different fermentative parameters on 
enzyme production, and to characterize the enzyme 

in relation with optimal pH and temperature of 
performance and the stability to these factors. 

 
MATERIAL AND METHODS 
 
Microorganism 

The thermophilic fungus Myceliophthora 
heterothallica F.2.1.4. was isolated from sugarcane 
bagasse compost provided by the Laboratory of 
Applied Biochemistry and Microbiology of the 
Universidade Estadual Paulista (UNESP), Brazil, 
and maintained in the Laboratory of Microbiology 
of the Universidade do Estado de Minas Gerais 
(UEMG), Brazil. The fungus was activated on Agar 
Malt medium (Acumedia) and incubated at 45°C for 
5 days. Culture medium composed of oatmeal 
(Quaker) 3% and bacteriological Agar 2%, pH 
adjusted to 5.5, was kept under the same conditions 
of temperature and culture time for periodic peaks 
and conservation of pure culture. 

 
Enzyme production  

For each solid-state cultivation (SSC) 
culture, a pre-inoculum of the fungus was placed in 
a 250 mL Erlenmeyer flask containing 100 mL of a 
medium composed of oat flour (Quaker) 3% and 
Agar (2%), pH adjusted for 5.5 with HCl. The 
fungus was inoculated onto the surface of this 
medium, by streaking, and incubated at 45°C until 
complete growth. The microorganism was then 
suspended with 150 ml distilled water and 
inoculated into each Erlenmeyer. 

The fungus was cultivated in 5.0 g of the 
following substrates: sugarcane bagasse, sugarcane 
straw, wheat bran and a mixture of these three 
materials (1:1:1 w/w) (namely MIX). Bagasse and 
sugarcane straw were retrieved from sugarcane 
plants in the municipality of Frutal MG Brazil. 
Wheat bran was purchased on the local market. 
Substrates were washed, dried at 60°C and sieved in 
a 10 mesh. 

Solid-state cultivation cultures were 
conducted in 250 mL Erlenmeyer flasks, with 5 g of 
each substrate. In cultures for the evaluation of the 
influence of time on enzyme production, initially 
sterilized distilled water was used for hydration of 
the medium at pH 5.0 and the fungus was cultured 
at 45°C. Samples were taken every 24 hours, up to 
240 hours (10 days). Further, 40 mL (wheat bran) 
and 80 mL (bagasse, cane straw and three-substrate 
mix) of distilled water were added to each sample. 
The mixture was homogenized manually and 
subsequently shaken (50 rpm), for 20 minutes. The 
material was then filtered on a nylon cloth disc, 
centrifuged at 10000 xg for 15 min, at 5°C, and the 



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Production and characterization…   MARTINS, M. E. M.; MARTINS, E. S.; MARTINS, H. L. 

Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

supernatant was used for the determination of 
enzymatic activities. 

 
Cultivation parameters 

Different culture parameters, such as 
supplementary nutrient solution to the substrate, 
supplementary nutrient solution pH, initial substrate 
moisture and fungus incubation temperature, were 
evaluated to establish conditions of higher enzyme 
production by the fungus. 

The following nutrient solutions were used 
on the substrate to assess the effect of substrate 
supplementation on enzyme production:  
1- Distilled water 0.1% (control);  
2- NH4NO3 (0.1%);  
3- (NH4)2SO4;  
4- NH4NO3, MgSO4.7H2O and (NH4)2SO4 (0.1%);  
5- Yeast extract (0.1%), so that the initial moisture 

is at 80%. The pH rates of each solution were 
evaluated from 4.0 to 6.0 (with a variation of 0.5 
in 0.5), at a 5x5 factorial plan. 

So that the effect of the substrate´s initial 
moisture could be evaluated, volumes of the nutrient 
solution (chosen in the previous stage) were added 
to the inoculum so that initial moisture contents 
were 60%, 65%, 70%, 75% and 80%. Fermentation 
temperatures evaluated were 40°C, 45°C, 50°C and 
55°C, at a 5x5 factorial plan. 

 
β-glucosidase characterization  

The effect of pH on the enzyme activity was 
evaluated at pH range between 3.0 and 10.0 using 
0.1 M buffers: pH 3: sodium citrate; pH 3–5.5: 
sodium acetate; pH 6.0-6.5: MES; pH 7.0–7.5: 
HEPES; pH 8.0–10.0: glycine. Temperature effect 
was assayed by incubating the reaction mixture at a 
temperature ranging between 35 and 80°C, in 
optimal pH. Further, the effect of pH on enzyme 
stability was analyzed by incubating the crude 
enzyme solution in various buffers with pH ranging 
between 3.0 and 10.0, during 24h, at 25°C, followed 
by the determination of 𝛽-glucosidase residual 
activity, under optimum conditions of pH and 
temperature. Thermal stability was determined by 
incubating the crude enzyme between 40 and 80°C, 
for 60 min, followed by the determination of β-
glucosidase residual activity, under optimum pH 
and temperature conditions. 

Effect of glucose on β-glucosidase activity 
was determined by adding glucose at different 
concentrations (0–50mM) in the reaction mixture, 
under optimum pH and temperature conditions. 

 
 
 

Enzymatic assay and statistical analysis of data 
β-D-Glucosidase activity was assessed in a 

mixture of 50 mm sodium acetate buffer, pH 5.0, 
450 𝜇L of 4 mM L−1 p-nitrophenyl-β-D-
glucopyranoside (pNP-Glc) as substrate, and 50 𝜇L 
of the enzyme solution incubated for 10 min, at 
60°C. Reaction ceased by adding 2 mL of 2 M 
Na2CO3 and absorbance read at 410 nm. One unit of 
β-glucosidase (U) was defined as the amount of 
enzyme that releases 1 𝜇mole of nitrophenol/min in 
reaction conditions (PALMA-FERNANDEZ et al., 
2002). 

Analysis of variance of the experiments was 
carried out with data obtained from the different 
treatments applied. Scott-Knott test was applied at 
5% significance. 

 
RESULTS AND DISCUSSION 

 
Production of β-glucosidase by M. heterothallica 
on different substrates 

The highest production rate of initial β-
glucosidase occurred in the substrate formed by the 
mixture of wheat bran, sugarcane bagasse and straw 
(1:1:1 w/w), with initial rates (30.5 U g-1) (Figure 
1). Rates were high when compared to results in the 
literature, since no variation of cultivation 
parameters had yet been made for its production. As 
observed, prior to defining cultivation parameters 
that could increase β-glucosidase production, the 
activity rate obtained was close to some reports in 
the literature for fungal β-glucosidases, such as 40.4 
U g-1 obtained by A. fumigatus cultivated at 45°C  in 
wheat bran (MORETTI et al., 2012), 41.8 U g-1 

obtained by Thermomucor indicae-seudaticae N31 
cultivated at 45°C  in soybean meal (PEREIRA et 
al., 2015) and 30.5 U g-1 obtained by A. fumigatus 
cultivated at 45°C  in sugarcane bagasse (DE 
OLIVEIRA RODRIGUES et al., 2017). 

β-glucosidase activity was detected as from 
2 days of culture, with peaks of activity on the 4th 
and 7th day, indicating that there may also be 
isoforms of the enzyme in the enzymatic extract. 
The peak of enzymatic activity occurred in 7 days, 
with rate presenting statistical difference when 
compared to the others. In the case of wheat bran, 
the activity was detected as from day 1 of 
cultivation, with peaks on the 6th and 8th day of 
culture. In sugarcane straw, it showed a peak 
between 2 and 5 days, and another between 7 and 10 
days. In sugarcane bagasse, the enzymatic activity 
was also lower than that found in the other 
substrates (Figure 1). 

 



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Production and characterization…   MARTINS, M. E. M.; MARTINS, E. S.; MARTINS, H. L. 

Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

Results indicate that, in addition to 
complementing the wheat bran with carbon source 
and energy, sugarcane bagasse and straw may 
contribute towards a greater fungus growth (visual 
data, not quantified in the experiments). This may 

be due to the fact that the mixture provided a greater 
contact surface of the fungus to the substrates (SHI 
et al., 2009), particularly wheat bran which, in an 
isolated way, becomes more compacted and 
increases the enzymes production. 

 

 
Figure 1. Production of β-glucosidase by M. heterothallica, on different substrates and culture times. 

*Condition in which theres statistical difference in the Scott-Knott test (<0.05).  
 
Effect of culture parameters on β-glucosidase 
production by M. heterothallica 

When the effect of different supplemental 
nutrient solutions to the substrate (MIX) on the β-
glucosidase production was evaluated, it has been 
observed that the substrate supplementation 
increased enzyme production, when compared to 
control (water only). Statistical analysis of BG 
activity data with the different nutrient solutions 
revealed that the conditions in which there was a 

significant statistical difference comprised the 
supplementation of the substrate with the solution 
composed of NH4NO3, MgSO4.7H2O and 
(NH4)2SO4 (0.1%), at pH 4.5 and 6.0 (Figure 2). 
When compared to initial rates in control, the 
supplementation with the solution increased by 
almost 3 times the maximum β-glucosidase activity 
rate obtained by the fungus (Figure 2). The above 
demonstrated the importance of evaluating this 
factor for enzyme production.   

 

 
Figure 2. Production of β-glucosidase by M. heterothallica in substrate composed by wheat bran, sugarcane 

bagasse and sugarcane straw (1:1:1), supplemented with different nutrient solutions at different pH 
values, in 4 days of cultivation. 1- Distilled water (control); 2- NH4NO3 (0.1%); 3- (NH4)2SO4 
(0.1%); 4- NH4NO3, MgSO4.7H2O and (NH4)2SO4 (0.1%); 5- yeast extract (0.1%).    
*Conditions in which there was statistical difference in the Scott-Knott test (<0.05). 

 
As a rule, when studying 

complementary source of nutrients to the 
substrate, nitrogen sources are mainly 
evaluated. Gottschalk et al. (2013) reported that 
inorganic nitrogen sources are generally more 

easily assimilated by fungi than organic ones, 
even though they point out that this depends on 
fungal lineage, the nature of the element and its 
concentration. Ahmed et al. (2017) cited that 
most research works on the microbial β-



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Production and characterization…   MARTINS, M. E. M.; MARTINS, E. S.; MARTINS, H. L. 

Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

glucosidase production do not focus on the 
optimization of supplementary nitrogen sources 
to the carbon sources in the fermentation. The 
authors also reinforce the need to study the 
mechanisms by which nitrogen sources 
influence the expression of these enzymes. 
These observations corroborate the importance 
of the evaluation of different supplementary 
sources of nutrients on β-glucosidase 
production. 

In the case of the substrate´s initial pH, 
different species require different pH rates for 
optimal β-glucosidase production. However, as 
in the case of temperature, most β-glucosidases 
research fails to report pH optimization for its 
production. A random pH rate is used in which 
these species grow optimally (AHMED et al., 
2017). This information reinforces the study of 
these variables in current analysis. Throughout 
the microbial culture, in solid-state 
fermentation, pH rate is not controlled because 
of the process´s heterogeneity (GARCIA et al., 

2015). According to Pandey et al. (2000), the 
difficulty of monitoring and controlling 
parameters in solid-state fermentation is 
perhaps the main disadvantage of the process, 
and pH variations during the fermentation 
process may occur due to the metabolic activity 
of the microorganisms. They may be increased 
or decreased according to the by-products 
released or the nutrients consumed during the 
process. 

Under the best conditions established in 
previous experiments, the effect of the initial 
moisture of the substrate (MIX) and the 
incubation temperature of the fungus on β-
glucosidase production was determined. 
Incubation of the fungus at 40ºC or 45ºC, with 
initial substrate moisture at 80%, provided the 
highest activity of the enzyme, with significant 
statistical difference. Higher moisture rates 
(85%) decreased enzymatic activity at all 
incubation temperatures (Figure 3). 

 

 
Figure 3. Production of β-glucosidase by M. heterothallica in substrate composed by wheat bran, sugarcane 

bagasse and sugarcane straw (1:1:1), supplemented with NH4NO3, MgSO4.7H2O and (NH4)2SO4 
(0.1%), at pH 4.5, in 4 days of cultivation, at different conditions of moisture and fungus incubation 
temperature.  
*Conditions in which there was statistical difference in the Scott-Knott test (<0.05). 

 
Regarding to substrate moisture, when the 

moisture content is below the required level, the 
nutrients´ solubility is limited and hinders their 
effective absorption by the fungi. On the other hand, 
when it is raised, the substrate particles are 
surrounded by a thick layer of water, tending to 
stick together and limiting gas exchanges. Thus, it is 
essential to establish the adequate level of moisture 
for microbial growth and obtain its products 
(YOON et al., 2004; SANTOS et al., 2016). 

Cultivation temperature for the production 
of β-glucosidases varies from species to species. In 
most cases, it coincides with the optimal 

temperature of growth of the microorganism. On the 
other hand, the ideal temperature for enzyme 
production does not always correspond to the 
temperature of the microorganism´s natural habitat 
(AHMED et al., 2017). Consequently, several 
microorganisms produce the enzyme at 
temperatures other than its optimum growth, as 
occurred in current assay with M. heterothallica 
fungus, where optimum growth temperature was 
between 45°C and 50°C, although the highest 
enzymatic activity rate was detected when the 
cultivation occurred at 40°C. Elyas et al. (2010) 
reported that the optimal growth temperature of 



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Production and characterization…   MARTINS, M. E. M.; MARTINS, E. S.; MARTINS, H. L. 

Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

Aspergillus AS58 fungal strain was 30°C, whereas 
the highest activity rate of its β-glucosidase was 
detected at 35°C. 

High or very low temperatures may 
decrease the microorganism´s growth and thus the 
formation of the product. Low thermal conductivity 
of the agro-industrial residues used in solid-state 
cultivation processes may hinder the dissipation of 
the metabolic heat generated by microbial growth 
(PANDEY et al., 2003). Thus, the analysis of 
culture temperature is highly relevant for delineating 
a bioprocess to produce enzymes (SANTOS et al., 
2016). 

 
Biochemical characterization of β-glucosidase 

β-glucosidase produced has a better 
performance at pH rates between 4.0 and 5.5, with 
activities very close to each other at this pH range, 
with a peak at pH 5.0 when incubated at 60°C 

(Figure 4). No enzymatic activity occurred at pH 
rates above 7.5. Thus, data indicate that the fungus 
produces a β-glucosidase that may be applied in 
processes that require higher acidic pH rates. Acid 
cellulase is more adequate to degrade feedstock 
cellulose in the bioconversion industry, where 
biomass undergoes acid pre-treatment. The ability to 
work in an acidic pH environment is also a 
requirement for enzymes used in the textile industry 
in the finishing step where they act on cellulolytic 
fibers (SHARMA et al., 2016).  

With respect to stability when exposed for 
24h in the absence of substrate in buffers with 
different pH rates, it has been observed that the 
enzyme maintains more than 80% of its activity 
within a wide pH range (3.5 to 9.5). At optimum pH 
(5.0), it maintained 88.1% of its activity, after 24h 
(Figure 4). 

 

 
Figure 4. Biochemical characterization of β-glucosidase produced by M. heterothallica.  

■- optimum pH; --pH stability for 24h, a 25ºC.  
 

According to Baffi et al. (2011), most 
microbial β-glucosidases present optimum pH 
between 4.0 and 6.0. Garcia et al. (2015) reported 
that optimal pH of β-glucosidase produced by 
Lichtheimia ramosa ranged between 5.0 and 6.0, 
with peak at pH 5.5. With regard to pH stability, the 
enzyme also showed high stability (over 90%) over 
a wide pH range (between 3.0 and 10.0), similar to 
results in current assay. Santa-Rosa et al. (2018) 
reported that β-glucosidase from Penicillium sp. 
presented a higher activity at pH rates between 5.0 
and 7.0, with optimum activity at pH 6.0.  

In the case of optimum temperature for β-
glucosidase activity, an increase in enzyme activity 
was observed up to 65°C, at which temperature 
(75.4 U g-1) was detected. Activity decreases as 
from this temperature, especially after 75°C (Figure 
5). In the case of the enzyme´s thermostability, 
results showed that β-glucosidase presented 100.0% 
and 48.6% stability when respectively exposed at 
60ºC and 65ºC. Activity declined in temperatures 

above 65ºC. Enzyme was not detected when 
exposed at 70°C, for 1 h (Figure 5). Pereira et al. 
(2015) reported that β-glucosidase from 
Myceliophthora thermophila presented optimum 
activity at 70°C and the enzyme maintained more 
than 93% of its original activity when incubated at 
55°C.  

Optimal β-glucosidase temperature of 
fungus M. heterothallica lies within the optimum 
temperature range of these enzymes produced by 
different fungi. Results demonstrate that enzyme has 
a significant thermostability when compared to 
enzymes of several microorganisms reported in the 
literature. Many commercial β-glucosidases of fungi 
are stable for a short time at high temperatures, 
denaturing at higher temperatures or time of 
exposure (LIU et al., 2012). Although enzymes from 
different organisms vary greatly in properties and 
functions, cost-effective production, high hydrolytic 
efficiency and great tolerance to unfavorable 
conditions are prerequisites of an industrial 



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http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

biocatalyst in various applications. Of particular 
interest, β-glucosidases from thermophilic fungi are 
more favorable due to the high-temperature activity 

and good thermostability (PEI et al., 2011; 
MALLEK-FAKHFAKH et al., 2016).  

 
 

 
Figure 5. Biochemical characterization of β-glucosidase produced by M. heterothallica.  

■- optimum temperature; -- temperature stability for 1h.  
 

Thermostability study showed that β-
glucosidase from M. heterothallica is highly 
thermostable as it retained above 90% of its original 

activity after 120 min of incubation up to 60°C. At 
65°C, enzyme half-life was approximately 1h. 
(Figure 6).  

 

 
Figure 6. Effect of different temperatures on β-glucosidase stability.  

 
Pereira et al. (2015) reported the production 

of a β-glucosidase of the thermophilic fungus 
Thermoascus aurantiacus, which showed maximum 
activity within 70°C and 75°C range. It maintained 
75% stability when incubated for 1h at temperatures 
between 55°C and 75°C. Garcia et al. (2015) 
reported a β-glucosidase of the mesophilic fungus 
Lichtheimia ramosa, which presented optimum 
temperature of 65°C, maintaining 98% and 40% of 
its activity when exposed for 1h at 55°C and 60°C, 
respectively. Santa-Rosa et al. (2018) reported the 
production of a β-glucosidase of Penicillium sp., 
with an optimal temperature of 60°C, maintaining 
95.7% of its activity when incubated for 1h. 

The high thermostability of β-glucosidase of 
M. heterothallica presented in the present work is 
desirable in industrial processes that require 
cellulolytic enzymes that maintain activity under 
high temperatures. 

Glucose in the reaction medium caused a 
decrease in β-glucosidase activity with increasing 
glucose concentration. Residual activity of the 
enzyme at concentrations 5, 10, 15, and 20mM was 
66.3%, 54.6%, 43.0%, and 29.3%, respectively. It 
actually decreased progressively, maintaining 4.0% 
of activity with glucose at 40mM (Fig 7). In order to 
verify whether the inhibition of the enzyme was 
competitive or not, a test was performed in which 
the substrate concentration was increased from 



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Production and characterization…   MARTINS, M. E. M.; MARTINS, E. S.; MARTINS, H. L. 

Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

4mM to 10mM. Since enzymatic activity returned to 
the level as when the reaction medium had no 

glucose (100% of original activity), inhibition 
proved to be competitive. 

 

 
Figure 7: Effect of glucose on β-glucosidase activity by M. heterothallica. 
 

Since most microbial β-glucosidases are 
inhibited by glucose, it becomes a major limitation 
for the use of these enzymes in industrial processes 
(LEITE et al., 2008).  High glucose concentrations 
may directly or indirectly interfere with the binding 
of the substrate to the activated site and reduce the 
reaction rate (SINGHANIA et al., 2013). Inhibition 
of β-glucosidase produced by M. heterothallica was 
completely reversed when the substrate 
concentration increased but maintained the same 
glucose concentration. Results demonstrated that 
enzyme interaction with the inhibitor was 
competitive. Competitive inhibition may be reversed 
by increasing the concentration of the substrate. The 
reversibility of glucose inhibition of β-glucosidase 
in current study confirmed the potential of the 
enzyme in applications requiring saccharification 
processes. 

CONCLUSIONS 
 

The use of agro-industrial residues as 
substrate provided good β-glucosidase production 
by M. heterothallica, with the enzyme having the 
desirable characteristics from industrial application, 
such as good thermostability and stability over a 
wide pH range.  

The high thermostability of β-glucosidase of 
M. heterothallica presented in the present work is 
desirable in industrial processes that require 
cellulolytic enzymes that maintain activity under 
high temperatures. 

 
ACKNOWLEDGMENTS  
 

The authors wish to thank Programa 
PIBIC/UEMG for financial support. 

 
 

RESUMO: A conversão da biomassa vegetal proveniente de resíduos agroindustriais em bioprodutos é 
de grande interesse, principalmente para o Brasil, onde a agroenergia possui grande potencial de 
desenvolvimento. Enzimas envolvidas na biodegradação da biomassa lignocelulósica fazem parte do grupo das 
celulases, no qual a 𝛽-glucosidase é um constituinte. O presente estudo avaliou a produção e caracterização de 
uma β-glicosidase pelo fungo termofílico Myceliophthora heterothallica por cultivo em estado sólido de 
diferentes resíduos agroindustriais (bagaço de cana-de-açúcar, palha de cana-de-açúcar, farelo de trigo e em 
uma mistura dos três materiais (1:1: 1 p/p). O cultivo em estado sólido foi realizado em frascos Erlenmeyer de 
250 mL, contendo 5 g de cada substrato. Diferentes parâmetros de cultivo, como solução nutriente suplementar 
ao substrato, pH da solução nutriente suplementar, umidade inicial do substrato e temperatura de incubação do 
fungo foram avaliados, visando estabelecer condições para maior produção da enzima pelo fungo. A maior 
produção da enzima ocorreu na mistura de farelo de trigo, e bagaço e palha de cana-de-açúcar (1:1:1). A 
atividade da β-glicosidase foi maior nas seguintes condições: solução nutriente composta por NH4NO3, 
MgSO4.7H2O e (NH4)2SO4 (0,1%) com pH 4,5 e 6,0, temperatura de incubação do fungo a 40°C e 45°C, com 
umidade inicial do substrato em 80%. A enzima apresentou pH ótimo de 5,0, e boa estabilidade ao pH. A 
temperatura ótima foi de 65°C, e a enzima apresentou 100% de estabilidade por 1h, até 60°C. A utilização de 



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Biosci. J., Uberlândia, v. 36, n. 1, p. 212-222, Jan./Feb. 2020 
http://dx.doi.org/10.14393/BJ-v36n1a2020-47758 

resíduos agroindustriais proporcionou boa produção de β-glicosidase pelo fungo, com a enzima apresentando 
características desejáveis para aplicação industrial.   

 
PALAVRAS-CHAVE: Enzimas celulolíticas. Fungo. Myceliophthora heterothallica. Cultivo em 

estado sólido.  
 

 
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