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SIMULTANEOUS PRODUCTION OF BIOSURFACTANTS AND LIPASES FROM Aspergillus niger AND OPTIMIZATION BY RESPONSE SURFACE METHODOLOGY AND DESIRABILITY FUNCTIONS

Abstract

Microbial conversion for the synthesis of high added-value compounds, such as biosurfactants and lipases, is one of the most promising fields within the biotechnology industry, given its current development. In this study the simultaneous production of biosurfactants and lipases by Aspergillus niger in a submerged bioprocess was analyzed. Full Factorial Design (23) was conducted to assess the influence of the malt extract (g·L-1; 25, 50, 75) and soybean oil concentrations (% v/v; 0.0, 1.25, 2.5) and agitation rates (rpm; 0.0, 100, 200) on biosurfactant and lipase production. Higher levels of the factors favored microbial growth, while their lower levels favored the production of biosurfactants and lipases. The variables were optimized through the response surface methodology and desirability functions, obtaining simultaneous maximized values of 0.48 g·L-1 (biomass); 42.03% (EAw/o);2.17 UE (EAw/o) and 3.28 U (LA). This indicates the possibility of combined biosurfactant and lipase production.

Keywords
Filamentous fungus; Biosurfactants; Lipases; Optimization

INTRODUCTION

Advances in the production of microbial compounds have opened up new possibilities for more extensive industrial scale-up applications (Vannelli et al., 2007Vannelli, T., Qi W.W., Sweigard J., Gatenby A.A. and Sariaslani S.F. Production of p-hydroxycinnamic acid from glucose in Saccharomyces cerevisiae and Escherichia coli by expression of heterologous genes from plants and fungi, Metabolic Engineering, 9, p.142-151 (2007).). The potential of synthesis of the biocompounds produced by fungi is already known, and biosurfactants and lipolytic enzymes may be mentioned (Roveda et al., 2010Roveda, M., Hemkemeier, M. and Colla, L.M. Avaliação da produção de lipases por diferentes cepas de microrganismos isolados de efluentes de laticínios por fermentação submersa, Ciência e Tecnologia de Alimentos, 30, p.126-131 (2010).; Araujo et al., 2013Araujo, L.V., Freire, D.M.G. and Nitschke, M., Biossurfactantes: Propriedades Anticorrosivas, Antibiofilmes e antimicrobianas, Química Nova, 36, No. 6, p. 848-858 (2013).).

Biosurfactants are surface-active compounds produced by living beings on microbial cell surfaces or extracellularly excreted. These compounds contain hydrophobic and hydrophilic moieties that make them good agents for emulsification (Paramaporn et al., 2010Paramaporn, C., Phonnok, S., Durand, A., Marie, E. and Thanomsub, B.W., Bioproduction and Anticancer Activity of Biosurfactant Produced by the Dematiaceous Fungus Exophiala dermatitidis SK80, Journal of Microbiology and Biotehcnology, 20, p.1664-1671 (2010).; Morita et al., 2012Morita, T., Fukuoka, T., Imura, T. and Kitamoto, D., Formation of the two novel glycolipid biosurfactants, mannosylribitol lipid and mannosylarabitol lipid, by Pseudozyma parantarctica JCM 11752T, Applied Microbiology and Biotechnology, 96, p.931 (2012).; Sarafin et al., 2014Sarafin, Y., Donio, M.B.S., Velmurugan, S., Michaelbabu, M. and Citarasu, T., Kocuria marina BS-15 a biosurfactant producing halophilic bacteria isolated from solar salt works in India, Saudi Journal of Biological Sciences, 21, p.511 (2014).). They possess significant anti-biological and anti-microbial activities, low toxicity, low irritancy, and good compatibility with human skin, making them favorable for pharmaceutical and cosmetic formulations. The emulsification properties allow their use in food additives (emulsifiers) and their surface active properties are very promising for oil tank cleaning, decontamination of polluted areas, microbial-enhanced oil recovery, industrial cleaning, and soil remediation (Paramaporn et al., 2010Paramaporn, C., Phonnok, S., Durand, A., Marie, E. and Thanomsub, B.W., Bioproduction and Anticancer Activity of Biosurfactant Produced by the Dematiaceous Fungus Exophiala dermatitidis SK80, Journal of Microbiology and Biotehcnology, 20, p.1664-1671 (2010).; Bhardwaj et al., 2013Bhardwaj, G., Cameotra, S.S. and Chopra, H.K., Biosurfactants from Fungi: A Review, Petroleum & Environmental Biotechnology, 4, p.1-6 (2013).; Souza et al., 2014Souza, E.C., Vessoni-Penna, T.C. and Oliveira, R.P.S., Biosurfactant-enhanced hydrocarbon bioremediation: An overview, International Biodeterioration & Biodegradation, 89, p.88-94 (2014).).

Lipases (EC 3.1.1.3) are enzymes that can catalyze partial hydrolysis reactions or total triglycerides decomposition into free fatty acids, mono- and diglycerides, and also acting in esterification, transesterification and interesterification in low water environments (Reinehr et al., 2014Reinehr, C.O., Rizzardi, J., Silva, M.F., Oliveira, D., Treichel, H. and Colla, L.M., Production of lipases with Aspergillus niger and Aspergillus fumigatus through solid state fermentation: evaluation of substrate specificity and use in esterification and alcoholysis reactions, Química Nova, 37, p.454-460 (2014).). Lipolytic enzymes have been explored and used for novel biotechnological applications such as detergent, food, pharmaceutical and cosmetics production, chemical synthesis and in waste treatment (Carvalho et al., 2003Carvalho, P.O., Campos, P.R.B., Noffs, M. D'A., Oliveira, J. G., Shimizu, M.T. and Silva, D.M. Application of microbial lipases to concentrate polyunsaturated fatty acids, Química Nova, 26, p.75-80 (2003).; Colla et al., 2010Colla, L.M., Rizzardi, J., Pinto, M.H., Reinehr, C.O., Bertolin, T.E., and Costa, J.A.V. Simultaneous production of lipases and biosurfactants by submerged and solid-state bioprocesses, Bioresource Technology, 101, p.8308-8313 (2010).; Colla et al., 2012Colla, L.M., Reinehr, C.O. and Costa, J.A.V. Applications and production of microbial lipases, Revista CIATEC, 4, p.1-14 (2012).; Kumar et al., 2012Kumar, S., Mathur, A., Singh, V., Nandy, S., Khare, S. K. and Negi, S., Bioremediation of waste cooking oil using a novel lipase produced by Penicillium chrysogenum SNP5 grown in solid medium containing waste grease, Bioresource Technology, 120, p.300-304 (2012).).

The fungal production of these compounds depends on its physiology, as well as on the substrate formulation and process parameters. Complex substrates, such as malt extract, sugarcane molasses, corn steep liquor, vegetable oils, animal fat and oil derivatives are used for the biosynthesis of enzymes and biosurfactants (Di Luccio et al., 2004Di Luccio, M., Capra, F., Ribeiro, N.P., Vargas, G.D.L.P., Freire, D.M.G. and Oliveira, D., Effect of temperature, moisture, and carbono supplementation on lipase production by solid-state fermentation of soy cake by Penicillium simplicissimum, Applied Biochemistry and Biotechnology, 113-116, p.173-180 (2004).; Paramaporn et al., 2010Paramaporn, C., Phonnok, S., Durand, A., Marie, E. and Thanomsub, B.W., Bioproduction and Anticancer Activity of Biosurfactant Produced by the Dematiaceous Fungus Exophiala dermatitidis SK80, Journal of Microbiology and Biotehcnology, 20, p.1664-1671 (2010).; Bharali et al., 2011Bharali, P., Das, S., Konwar, B. K. and Thakur, A. J., Crude biosurfactant from thermophilic Alcaligenes faecalis: Feasibility in petro-spill bioremediation, International Biodeterioration & Biodegradation, 65, p.682-690 (2011).; Gudiña et al., 2015Gudiña, E. J., Rodrigues, A. I., Alves, E., Domingues, M. R., Teixeira, J. A. and Rodrigues, L. R., Bioconversion of agro-industrial by-products in rhamnolipids toward applications in enhanced oil recovery and bioremediation, Bioresource Technology, 177, p.87-93 (2015).; Bonugli-Santos et al., 2015Bonugli-Santos, R. C., dos Santos Vasconcelos, M. R., Passarini, M. R. Z., Vieira, G. A. L., Lopes, V. C. P., Mainardi, P. H., dos Santos, J. A., de Azevedo Duarte, L., Otero, I. V. R., da Silva Yoshida, A. M., Feitosa, V. A., Pessoa Jr, A. and Sette, L. D., Marine-derived fungi: diversity of enzymes and biotechnological applications, Frontiers in Microbiology, 6, p.1-15, (2015).).

Due to the great influence of culture conditions on the production of enzymes and biosurfactants, the use of experimental design and statistical analysis is a successfully applied methodology (Bonugli-Santos et al., 2015Bonugli-Santos, R. C., dos Santos Vasconcelos, M. R., Passarini, M. R. Z., Vieira, G. A. L., Lopes, V. C. P., Mainardi, P. H., dos Santos, J. A., de Azevedo Duarte, L., Otero, I. V. R., da Silva Yoshida, A. M., Feitosa, V. A., Pessoa Jr, A. and Sette, L. D., Marine-derived fungi: diversity of enzymes and biotechnological applications, Frontiers in Microbiology, 6, p.1-15, (2015).). This methodology provides an efficient approach for the determination of the most important process parameters such as temperature, pH, aeration and substrate selection, which in turn can lead to process optimization. These parameters are best controlled in processes which involve submerged cultivation (Submerged Bioprocess - SmgB) due to the great homogeneity of the culture medium (Colla et al., 2010Colla, L.M., Rizzardi, J., Pinto, M.H., Reinehr, C.O., Bertolin, T.E., and Costa, J.A.V. Simultaneous production of lipases and biosurfactants by submerged and solid-state bioprocesses, Bioresource Technology, 101, p.8308-8313 (2010).; Colla et al., 2016Colla, L.M., Primaz, A.L., Benedetti, S., Loss, R.A., Lima, M., Reinehr, C.O., Bertolin, T.E. and Costa, J.A.V. Surface response methodology for the optimization of lipase production under submerged fermentation by filamentous fungi, Brazilian Journal of Microbiology, 47, p.461-467 (2016).). Aeration of growing microbial culture can be ensured by inserting air into the culture medium and by agitation, resulting in an increased interface between gas and liquid capable of reducing the size of the air bubbles, making oxygen more easily accessible to the cells (Bakri et al., 2011Bakri, Y., Mekaeel, A. and Koreih, A., Influence of agitation speeds and aeration rates on the Xylanase activity of Aspergillus niger SS7, Brazilian Archives of Biology and Technology, 54, p.659-664 (2011).). However, the intensity of agitation should remain within a narrow range to keep the damage effect in the system at a minimum level (Kozma et al., 2006Kozma, L., Nyeste, L. and Szentirmai, A., Optimization problems of fermentor aeration-agitation system, Hungarian Journal, 34, p.35-39, (2006).).

Filamentous fungi are largely used for industrial lipase production. However, few fungi are already known as biosurfactant producers. Aspergillus fumigatus, Aspergillus niger, Candida bombicola, Candida rugosa, Pseudozyma sp. Penicillium sp. and Yarrowia lipolytica are fungi normally used for the production of biosurfactants and lipolytic enzymes (Fontes et al., 2008Fontes, G.C., Amaral, P.F., F.A. and Coelho, M.A.Z., Produção de biossurfactante por Levedura, Química Nova, 31, p.2091-2099 (2008).; Fukuoka et al., 2008Fukuoka, T., Kawamura, M., Morita, T., Imura, T., Sakai, H., Abe, M. and Kitamoto, D., A basidiomycetous yeast, Pseudozyma crassa, produces novel diastereomers of conventional mannosylerythritol lipids as glycolipid biosurfactants, Carbohydrate Research, 343, p.2947-2955 (2008).; Castiglioni et al., 2009Castiglioni, G.L., Bertolin, T.E. and Costa, J.A.V. Solid-state biosurfactant production by Aspergillus funigatus using agricultural residues as substrate, Química Nova, 32, p.292-295 (2009).; Kannahi and Sherley 2012Kannahi, M. and Sherley, M., Biosurfactant production by Pseudomonas putida and Aspergillus niger from oil contaminated site, International Journal of Chemical and Pharmaceutical Sciences, 3, p.37-42 (2012).; Kumar et al., 2012Kumar, S., Mathur, A., Singh, V., Nandy, S., Khare, S. K. and Negi, S., Bioremediation of waste cooking oil using a novel lipase produced by Penicillium chrysogenum SNP5 grown in solid medium containing waste grease, Bioresource Technology, 120, p.300-304 (2012).; Bhardwaj et al., 2013Bhardwaj, G., Cameotra, S.S. and Chopra, H.K., Biosurfactants from Fungi: A Review, Petroleum & Environmental Biotechnology, 4, p.1-6 (2013).; Santos et al., 2013Santos, D.K.F., Rufino, R.D., Luna, J.M., Santos, V.A., Salgueiro, A.A. and Sarubbo, L.A., Synthesis and evaluation of biosurfactant produced by Candida lipolytica using animal fat and corn steep liquor, Journal of Petroleum Science and Engineering, 105, p.43-50 (2013).; Reinehr et al., 2014Reinehr, C.O., Rizzardi, J., Silva, M.F., Oliveira, D., Treichel, H. and Colla, L.M., Production of lipases with Aspergillus niger and Aspergillus fumigatus through solid state fermentation: evaluation of substrate specificity and use in esterification and alcoholysis reactions, Química Nova, 37, p.454-460 (2014).). Aspergillus niger is a well-known lipase producer with suitable properties for industrial applications (Mahadik et al., 2002Mahadik, N.D. Puntambekar, U.S. Bastawde, K.B. Khire, J.M. and Gokhale, D.V., Production of acidic lipase by Aspergillus niger in solid-state fermentation, Process Biochemistry, 38, p. 715-721 (2002).; Basheer et al., 2011Basheer, S.M., Chellappan, S., Beena, P.S., Sukumaran, R.K., Elyas, K.K. and Chandrasekaran, M., Lipase from marine Aspergillus awamori BTMFW032: Production, partial purification and application in oil effluent treatment, New Biotechnology, 28, p.627-638 (2011).). It is also reported as a biosurfactant producer (Hussain et al., 2014Hussain, E., Baig, M. A. and Butt, G. Y., Evaluation of Different Carbon Sources in Production of Biosurfactant by Mycoflora of Southern Punjab Pakistan, European Academic Research, 2, p.2086-2092 (2014).). Therefore, this study aims to verify the impact of different factors (malt extract, agitation and soybean oil) on the simultaneous production of biosurfactants and lipases by Aspergillus niger in a submerged bioprocess, optimizing this process through the use of the response surface methodology (RSM) and desirability functions.

MATERIALS AND METHODS

Microorganism

The fungal strain Aspergillus niger isolated from an oil sample of a vegetable oil refining company located in Gaspar, SC - Brazil, was identified and previously selected as both a biosurfactant producer and a secretor of lipases (Sperb et al., 2015Sperb, J.G.C., Costa, T.M., Vaz, D.A., Valle, J.A.B., Valle, R.C.S.C. and Tavares, L.B.B., Avaliação qualitative da produção de lipases e biossurfactantes por fungos isolados de resíduos oleosos, Engevista, 17, No.3, p.385-397 (2015).). The fungus was maintained at 4 ºC in Petri dishes containing potato dextrose agar (PDA) and transferred to new dishes every two months.

Culture medium and experimental apparatus

The culture medium was prepared with malt extract (Kasvi®) and soybean oil (Soya®), according to the concentrations indicated in the experimental design (Table 1). In all assays, a saline solution containing KH2PO4 (2 g·L-1), MgSO4 (1 g·L-1), MnSO4 (0.01 g·L-1), FeSO4. 7 H2O (0.63 mg·L-1), and ZnSO4 (0.62 mg·L-1) was added.

Table 1
Factorial design matrix for ME, AG, SO and experimental values obtained for biomass, EAw/o, EAw/o and LA assays.

The experiments were carried out in 250 mL Erlenmeyer flasks with 100 mL of the culture medium in a rotary shaker at 25 ºC and agitation rates as specified in the experimental design (Table 1). The inoculation was accomplished using circular areas of 20 mm diameter containing mycelium grown in Petri dishes. According to preliminary laboratorial studies the best incubation period for this experiment was seven days. After fermentation, the mycelial biomass was separated by filtration through a vacuum filter and the cell free broth was assayed for biosurfactant and lipase activities.

Biomass quantification

Biomass quantification in the culture medium of SmgB was determined by the dry mass technique. After fermentation, the mycelial biomass was separated by vacuum filtration using membranes with 0.8 µm pores. This biomass was dried at 50 ºC until constant mass. The resulting values were converted to grams per liter of culture medium.

Determination of emulsifying activity

The water in oil (w/o) emulsifying activity (EAw/o) was determined by the method recommended by Paraszkiewicz (2002)Paraszkiewicz, K., Kanwal, A. and Dlugónski, J., Emulsifier production by steroid transforming filamentous fungus Curvalaria lunata Growth and product characterization, Journal of Biotechnology, 92, p.287-294 (2002). using 2 mL of soybean oil and 3.5 mL of cell free broth. The mixture was vortexed at 7000 rpm for 2 min. After 24 hours, the height of the emulsified phase was verified, using a caliper rule, comparing it to the total liquid height. The EAw/o was determined according Eq. 1.

(1) EA w / O = H e H t . 100

EAw/o is the emulsifying activity water-in-oil (%); He is the height of the emulsified phase (mm); Ht is the total height of the medium (mm).

Oil-in-water (o/w) emulsifying activity (EAw/o) was determined by the method of Johnson et al., (1992)Von, J., Singh, M., Saini, V.S., Adhikari, D.K., Sista, V. and Yadav, N. K., Bioemulsifier production by an oleaginous yeast Rhodotorula glutinis IIP-30. Biotechnology Letters 14, p. 487-49 (1992)., using 2 mL of soybean oil and 3.5 mL of the cell free broth. The mixture was vortexed at 7000 rpm for 2 min. After 60 min, the absorbance of the emulsified phase was read in a spectrophotometer (Shimadzu UV-1650) at 610 nm. The emulsifying activity was obtained by Eq. 2. Water was used as the blank medium.

(2) EA O / w = Abs sample Abs blank

EAw/o is the emulsifying activity oil-in-water (units of emulsification, UE); Abssample is the absorbance of the sample (ABS); Absblank is the absorbance of the blank medium (ABS).

One unit of emulsification (UE) was defined as the amount of absorbance read in this assay.

Lipase activity

Lipase activity was analyzed in crude extracts, using a modified titrimetric method as described by Pastore et al., (2003)Pastore, G.M., Costa, V.S.R. and Koblitz, M.G.B., Purificação parcial e caracterização bioquímica de lipase extracelular produzida por nova linhagem de Rhizopus sp, Ciência e Tecnologia de Alimentos, 23, No. 2, p. 135-140 (2003).. The method is based on the titration with NaOH of the fatty acids released from the hydrolysis of olive oil, previously emulsified with xanthan gum, by the action of the lipase present in the cell free broth. Reaction mixture containing 5 mL of the emulsion (1% of xanthan gum (w/v) and 25% of olive oil (v/v)), 2 mL of phosphate buffer (pH 7) and 1 mL of culture medium was incubated at 37 ºC during 15 min. Reaction was stopped by adding 15 mL of (1:1) acetone:ethanol solution and the amount of the fatty acids was quantified through the titration assay with a solution of 0.05M NaOH until achieving pH 7. The lipase activity was determined according to Eq. 3:

(3) LA = V NaOH · Cm NaOH t . V sample

where LA is the lipase activity (µmol· mL-1·min-1); VNaOH is the volume of NaOH used for titration (mL); CmNaOH is the molar concentration of NaOH (µmol·mL-1); t is the time (min); Vsample is the volume of sample used (mL).

One unit (U) of lipase activity was defined as the amount of enzyme which releases 1 µmol·mL-1·min-1 of fatty acids under the assay conditions.

Experimental design

A full factorial design (23) with 1 center point and 2 replicates was used to identify the factors that have significant impacts on biomass, biosurfactant and lipase production in SmgB. A set of 9 experiments was used to determine the relative effect of different malt extract (ME) and soybean oil (SO) concentrations and agitation rates (AG) in 2 levels, high (+1) and low (-1). In Table 1 the real values used and their levels are shown, as well as the experimental values obtained for Biomass, EAw/o, EAw/o and LA assays.

The experimental values were fitted to the multivariate model, given by Eq. 4, through the least squares method. Surface response graphs were built by using these regression equations.

(4) Y = β 0 + j = 1 k β j x j + i < j β ij x i x j + β ijk x i x j x k + ɛ

where Y is the predicted response; β0, βj, ... βn are the regression coefficients; xi, xj, xk are the real values of the independent variables; ϵ is the associated error of the model.

Model curvature analysis for each response surface was generated, according to Eq. 5. The curvature analysis is based on the sum of the curvature squares.

(5) SS curv = n f n c y ¯ f y ¯ c 2 n f + n c

where SScurv is the summation of the curvature squares; nf is the number of experiments carried on the main factorial matrix; nc is the number of experiments carried out on center points; yf is the mean value obtained in the main factorial matrix; yc is the mean value obtained on the center points.

The regression coefficients of the multivariate model, curvature analysis, response surface graphs and all statistical analysis were performed with a 95 % significance level, using the software Statistica® 7.0 (Statsoft).

Optimization of the responses

The optimization method of non-linear programming desirability functions, described by Derringer and Suich (1980)Derringer, G., Suich, R., Simultaneous Optimization of Several Response Variables, Journal of Quality Technology, 12, n.4, p. 214-219 (1980)., was used to obtain the best responses under the factorial design of this study. The one-sided transformations were used, as stated in equations 6 (for maximization) and 7 (for minimization) below:

(6) d max = 0 if Y < L Y L T L S if L Y T 1 if Y > T
(7) d min = 0 if Y > H H Y H T t if T Y H 1 if T < Y

where dmax is the one-sided desirability value for maximization; dmin is the one-sided desirability value for minimization; Y is the predicted response; L is the lowest response value obtained in this study; H is the highest response value obtained in this study; T is the target for the response; s and t are exponential values defined by user's criteria.

The process optimization criteria were the maximization of EAw/o, EAw/o and LA values (Desirability for max values = 1 and min. values = 0) while minimizing biomass quantities (Desirability for max values = 0 and min. values = 1). Unitary values were used in the exponents s and t, as linear desirability functions were preferred.

The overall desirability is calculated by the geometric mean of all individual desirability values, according to Eq. 8. The optimization routine consists of changing the factor values (according to the factorial matrix) until the maximum overall desirability value is achieved.

(8) D = d Biomass · d EA w / O · d EA O / w · d LA 1 / 4

where D is the overall desirability; dBiomass is the desirability for Biomass; dEAw/O is the desirability for the EAw/o; dEAO/w is the desirability for the EAo/w; dLA is the desirability for the LA.

The criteria for choosing the minimization of biomass and the maximization of the remaining responses were due to the consideration that the products are of extracellular nature. Therefore, the least biomass produced in the process represents the least purification costs and less residue formation.

The optimization routine as well as the drawing of desirability contour plots were performed in Statistica® 7.0 software (Statsoft), by the use of the Response Desirability Profile tool. The optimization study considered the whole response surfaces, described by the regression model in Eq. 4.

RESULTS AND DISCUSSION

The effects and relationships among the factors ME, AG and SO in the production of biomass, biosurfactants and lipases for Aspergillus niger were determined according to the design of experiments. Biomass concentration, biosurfactant and lipase production for each assay with the experimental responses are presented in Table 1.

The full factorial design led to the following regression equations (9 - 12), where the numbers with an asterisk are not significant at the 95% level. Null values of the regression coefficients were omitted in this article. The fit of the regression equations, as well as the adjusted determination coefficients (adj. R2) can be visualized in Fig. 1.

(9) Biomass = 0 . 050 + 0 . 017 ME + 0 . 001 AG + 1 . 374 SO 0 . 007 ME . SO 0 . 003 AG . SO
(10) EA w / O = 44 . 631 0 . 104 ME 0 . 125 AG 5 . 984 SO + 0 . 001 ME . AG + 0 . 007 ME . SO + 0 . 026 AG . SO
(11) EA O / w = 2 . 140 + 0 . 001 ME + 0 . 006 AG 0 . 019 SO 0 . 001 ME . SO 0 . 002 AG . SO
(12) LA = 2 . 972 + 0 . 012 ME 0 . 0183 AG 0 . 200 SO 0 . 003 ME . SO + 0 . 004 AG . SO

Figure 1
Representation of the Predicted values x Observed values: Biomass (A) adj. R2 = 0.96; EAw/o (B) adj. R2 = 0.65; EAw/o (C) adj. R2 = 0.78; LA (D) adj. R2 = 0.81.

Regression models showed a good degree of adjustment with ane overall adjusted R2 of 0.80. The lowest adjusted R2 was 0.65 for the EAw/o response. However, the model is considered suitable for representation of the results.

Analysis of the regression coefficients and their significance (95% level) showed that all main factors impact positively on biomass production, with SO being the major contributor to its growth. This indicates that the fungus Aspergillus niger is capable of using the lipids from soybean oil for its development.

The biosurfactant production was monitored using as parameters the emulsifying activities EAw/o and EAw/o. It is also known that emulsification activities from Aspergillus strains strongly correlate with the production of biosurfactants (Castiglioni et al., 2009Castiglioni, G.L., Bertolin, T.E. and Costa, J.A.V. Solid-state biosurfactant production by Aspergillus funigatus using agricultural residues as substrate, Química Nova, 32, p.292-295 (2009).; Ishaq et al., 2015Ishaq, U., Akram, M. S., Iqbal, Z., Rafiq, M., Akrem, A., Nadeem, M., Shafi, F., Shafiq, Z., Mahmood, S., Baig, M.A. Production and characterization of novel self-assembling biosurfactants from Aspergillus flavus, Journal of Applied Microbiology, 119, p.1035-1045 (2015).). The response of EAw/o was impacted negatively by the factors AG and SO, while ME was not significant (at the level of 5%). The interaction values ME.AG and AG.SO were positive and significant but their absolute values compared to the ones of the main factors. The interaction factor of ME.SO was not significant. The response EAw/o was impacted positively by ME and AG; however, their absolute values were low. SO was not significant for this emulsification activity. The effect of interaction of ME and SO for EAw/o was significant and impacted negatively on this response. The remaining interaction factors were either to low or not significant.

According to Table 1, it was verified that low SO is favorable for obtaining EAw/o Aspergillus niger. Furthermore, lower AG increases both EAw/o and EAw/o values. Fatty acids and maltose are both substrates which can be used by Aspergillus niger as carbon and energy sources (Lu et al., 2010Lu, X., Sun, J., Nimtz, M., Wissing, J., Zeng, A.P. and Rinas, U., The intra- and extracellular proteome of Aspergillus niger growing on defined medium with xylose or maltose as carbon substrate, Microbial Cell Factories, 9, p. 1-13 (2010); Papanikolaou et al., 2011Papanikolaou, S., Dimou, A., Fakas, S., Diamantopoulou, P., Philippoussis, A., Galiotou-Panayotou, M. and Aggelis, G., Biotechnological conversion of waste cooking olive oil into lipid-rich biomass using Aspergillus and Penicillium strains, Applied Microbiology, 110, p.1138-1150 (2011)). It can be clearly seen (Table 1) that the addition of soybean oil into the culture medium stimulated the biomass production (assays 5, 6, 7, 8 and 9). Similar values for biomass were observed by Colla et al., (2010)Colla, L.M., Rizzardi, J., Pinto, M.H., Reinehr, C.O., Bertolin, T.E., and Costa, J.A.V. Simultaneous production of lipases and biosurfactants by submerged and solid-state bioprocesses, Bioresource Technology, 101, p.8308-8313 (2010). with Aspergillus spp. in the presence of soybean oil, achieving maximum values of 4.49 g·L-1. A wide range of oils have been reported as substrates used in culture media. Sarkar and Laha (2013)Sarkar, D. and Laha, S., Optimization of extracellular lipase enzyme production from Aspergillus niger by submerged and solid-state Fermentation process, International Journal of Pharmacy and Biological Sciences, 4, p.978-985 (2013). observed biomass concentrations (derived from 20 mL of the medium) of 13.8 mg·mL-1, 15.2 mg·mL-1 and 13.1 mg·mL-1 for sunflower oil, olive oil and coconut oil respectively. Higher values (13.3 g·L-1) of biomass were obtained by Papanikolaou et al., (2011) for Aspergillus niger LFMB 1 with waste cooking olive oil in 168 hours. The maximum biomass concentration (4.10 g·L-1) in this study was obtained in the assay that had the higher values (+1) of ME, AG and SO.

Lipidic carbon sources (as vegetable oils) are cited as essential inducers for obtaining significant biosurfactant and lipase amounts (Dutra et al., 2008Dutra, J. C. V., Terzi, S. C., Bevilaqua, J. V., Damaso, M. C. T., Couri, S., Langone, M. A. P. and Senna, L. F. Lipase Production in Solid-State Fermentation Monitoring Biomass Growth of Aspergillus niger Using Digital Image Processing, Applied Biochemistry and Biotechnology, 147, p.63-75 (2008).; Saharan et al., 2011Saharan, B. S., Sahu, R. K., Sharma, D., A Review on Biosurfactants: Fermentation, Current Developments and Perspectives. Genetic Engineering and Biotechnology Journal, 11, p.1-14 (2011).). However, the mechanism that regulates biosynthesis widely varies for different microorganisms (Dalmau et al., 2000Dalmau, E., Montesinos, J. L., Lotti, M. and Casas, C., Effect of different carbon sources on lipase production by Candida rugosa, Enzyme and Microbial Technology, 26, p.657-663 (2000).). In this study the lipase production was independent of the addition of lipids to the culture medium, achieving its maximum value of 3.89 U (Table 1) in the assay with the high level (+1) of ME and low levels (-1) of AG and SO. Colla et al. (2010)Colla, L.M., Rizzardi, J., Pinto, M.H., Reinehr, C.O., Bertolin, T.E., and Costa, J.A.V. Simultaneous production of lipases and biosurfactants by submerged and solid-state bioprocesses, Bioresource Technology, 101, p.8308-8313 (2010). in their study obtained a maximum lipolytic activity of 4.52 U using soybean oil as a supplementary carbon source for Aspergillus spp. Sarkar and Laha (2013)Sarkar, D. and Laha, S., Optimization of extracellular lipase enzyme production from Aspergillus niger by submerged and solid-state Fermentation process, International Journal of Pharmacy and Biological Sciences, 4, p.978-985 (2013). obtained higher lipase production values when using glucose and olive oil as substrates and reduced lipolytic activity values were observed when using glucose as the sole carbon source. Higher soybean oil concentrations impacted negatively lipase production by Aspergillus niger and Aspergillus flavus according to Colla et al. (2016)Colla, L.M., Primaz, A.L., Benedetti, S., Loss, R.A., Lima, M., Reinehr, C.O., Bertolin, T.E. and Costa, J.A.V. Surface response methodology for the optimization of lipase production under submerged fermentation by filamentous fungi, Brazilian Journal of Microbiology, 47, p.461-467 (2016)..

Low ME levels and the absence of soybean oil favored emulsification activities, with EAw/o value of 42.03% and EAw/o value of 2.59 UE. Biosurfactant molecules are mainly formed as microbial secondary metabolites and play critical roles in the survival of their producing microorganisms by facilitating nutrient transport, interfering in microbe-host interactions and quorum sensing mechanisms or by acting as biocide agents (Gudiña et al., 2013Gudiña, E. J., Rangarajan, V., Sen, R. and Rodrigues, L. R., Potential therapeutic applications of biosurfactants, Trends in Pharmacological Sciences, 34, p.667-675 (2013).). Carbon source restriction may have been favorable for the activation of microbial secondary metabolism, which resulted in little fungal biomass formation: 0.48 and 0.83 g·L-1 in assays 1 and 3, respectively. An EAw/o value of 42.67% and an EAw/o value of 2.95 UE were obtained by Colla et al., (2010)Colla, L.M., Rizzardi, J., Pinto, M.H., Reinehr, C.O., Bertolin, T.E., and Costa, J.A.V. Simultaneous production of lipases and biosurfactants by submerged and solid-state bioprocesses, Bioresource Technology, 101, p.8308-8313 (2010). by using Aspergillus spp. Santos et al., (2013)Santos, D.K.F., Rufino, R.D., Luna, J.M., Santos, V.A., Salgueiro, A.A. and Sarubbo, L.A., Synthesis and evaluation of biosurfactant produced by Candida lipolytica using animal fat and corn steep liquor, Journal of Petroleum Science and Engineering, 105, p.43-50 (2013). studied the production of biosurfactants by Yarrowia lipolytica, achieving the best EAw/o results of 47% in a cell-free broth, having corn steep liquor (2.5%) and animal fat (5%) as substrates and soybean oil as the nonpolar phase of the emulsification test. In this study, it was verified that higher (+1) SO values resulted in lower emulsifying activities.

It is possible to verify that, agitation played a significant role in all of the acquired responses. Agitation ensures the supply of nutrients, especially oxygen, facilitating mass transfer phenomena. However, high agitation rates lead to high energy dissipation rates connected with high shear stress, which may result in fragmentation and damage of cells and mycelial networks (Kelly et al., 2004Kelly, S., Grimm, L. H., Hengstler, J., Schultheis, E., Krull, R. and Hempel, D. C., Agitation effects on submerged growth and product formation of Aspergillus niger, Bioprocess and Biosystems Engineering, 26, p.315-323 (2004).; Bakri et al., 2011Bakri, Y., Mekaeel, A. and Koreih, A., Influence of agitation speeds and aeration rates on the Xylanase activity of Aspergillus niger SS7, Brazilian Archives of Biology and Technology, 54, p.659-664 (2011).). The impact of colony morphology on the production of metabolites has been discussed by the academia, but there are many contrasting results (Ibrahim et al., 2015Ibrahim, D., Weloosamy, H., Lim, S., Effect of agitation speed on the morphology of Aspergillus niger HFD5A-1 hyphae and its pectinase production in submerged fermentation, World Journal of Biological Chemistry, 6, no. 3, p. 265-271 (2015).; Quintanilla et al., 2015Quintanilla, D., Hagemann, T., Hansen, K., Gernaey, K. V., Fungal Morphology in Industrial Enzyme Production - Modeling and Monitoring, Advances in Biochemical Engineering/Technology, 149, p.29-54 (2015).). Visual impacts were observed in the fungal colony in this study. In the static process (AG, level -1) the colony grew as a biofilm on top of the liquid substrate solution and under agitation there was the formation of pelletized colonies. No clear relationship between the morphology of fungal colonies and the studied responses was noted.

The significance analysis of the curvature of the models was carried out, and the assays of EAw/o and EAw/o showed significant values while biomass and lipase activity had no significant values for this analysis. The plotting of response surface curves for EAw/o and EAw/o, Fig. 2 and 3 respectively, show the interaction between the factors malt extract (ME), agitation (AG) and soybean oil (SO). The variables not represented on each plot are fixed at their lower levels (-). Through this analysis it is possible to verify the nearness to critical values of EAw/o and EAw/o, under the conditions of this study.

Figure 2
Response Surface curves of EAw/o production from Aspergillus niger showing interaction between: AG and ME (A); SO and ME (B); SO and AG (C).

In Fig. 2 and 3 it is verified that the critical values are found in the region with the lower response values, indicating the presence of a point of minimum productivity. Considering that, among the objectives of this work is the simultaneous maximization of the EAw/o and EAw/o responses, and the maximal response regions lie far from the critical points, the first order model is suitable for the optimization routine.

Figure 3
Response Surface curves of EAw/o production from Aspergillus niger showing interaction between: AG and ME (A); SO and ME (B); SO and AG (C).

The optimization step using the desirability functions was conducted and the results obtained by this procedure are demonstrated on the contour plots of Fig. 4.

Figure 4
Desirability contour plot from Aspergillus niger showing interactions between: AG and ME (A); SO and ME (B); SO and AG (C).

The surfaces generated by the desirability functions allow one to verify the points where the answers are closest to those values defined as objectives. Fig. 4 shows the strong interactions between the factors ME and SO and ME and AG, which generated two regions (Fig. 4A and 4B) of maximum desirability, one of them in the higher (+1) and the other in lower (-1) values of ME, but with the values of SO and AG always at their lower levels (-1). This trend is confirmed in Fig. 4C where there is only one region of maximum desirability, found in the region of the lowest values of SO and AG. This corroborates earlier analysis that accounted for a region of minimum EAw/o and EAw/o with all factors at their highest levels.

The optimized desirability function value was 0.85, which is a very good desirability value, at the lower levels of all factors. The values of the responses, under optimized conditions, are 0.48 g·L-1 of Biomass; EAw/o of 42.03%; EAw/o of 2.17 UE and LA of 3.28 U.

CONCLUSIONS

Submerged cultures of filamentous fungi are widely used to produce commercial biocompounds. Simultaneously obtaining compounds in a singular bioprocess would result in higher process efficiencies. Hence, the possibility of simultaneous production of biosurfactant and lipase was assayed in this study by using Aspergillus niger, cultivated in SmgB, varying malt extract (ME) and soybean oil (SO) concentrations and agitation rates (AG). It was found that higher SO led to poor emulsification and lipase activities and greater biomass growth, the same occurs for AG. Limited access to substrate was a very important factor that affected the production of biosurfactants and lipases positively, in contrast with biomass production, which is affected positively by substrate availability in the medium. Further studies are needed in order to verify the mechanism used by the fungus in this process of converting soybean oil into fungal biomass.

The application of the design of experiments, response surface and desirability function methodologies proved to be valuable and important tools in the comprehension, development and optimization of bioprocesses. Due to their application it was possible to verify the impacts caused by the factors (ME, AG and SO), their interaction values and the best response values to a given condition (desirability), in an objective and practical way. Therefore, according to this study factorial matrix, the lowest values of the factors should be used for optimum biosurfactant and lipase production. Due to the diversity of biomolecules synthesized by microorganisms, characterization studies and identification of the molecules produced will be necessary.

ACKNOWLEDGEMENTS

The authors are thankful to the Coordination for the Improvement of Higher Education Personnel (CAPES) for financial support and L.B.B. Tavares is fellowship holder of the National Council for Scientific and Technological Development (CNPq).

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Publication Dates

  • Publication in this collection
    Jul-Sep 2018

History

  • Received
    27 June 2016
  • Reviewed
    09 July 2017
  • Accepted
    22 Aug 2017
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