A novel bi-substrate fermentation (BSF) process was developed for the production of lipase from Aspergillus niger using

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ISSN: 0975-766X CODEN: IJPTFI Available Online through Research Article www.ijptonline.com UTILISATION OF SOLID WASTES FROM TANNERY FOR THE PRODUCTION OF LIPASE FROM ASPERGILLUS NIGER BY MIXED SUBSTRATE FERMENTATION PROCESS **A. Manikandan and *N.R. Kamini **Assistant Professor, School of Bio-Engineering, Department of Genetic Engineering, Bharath University, Chennai, Tamil Nadu, India. *Senior Scientist, Department of Biotechnology, Central Leather Institute of Technology, Chennai, Tamil Nadu, India. Email: manikandan.mpa@gmail.com Received on 12-07-2015 Accepted on 30-07-2015 Abstract A novel bi-substrate fermentation (BSF) process was developed for the production of lipase from Aspergillus niger using agro-industrial residues, wheat bran (WB), and beef fleshing of tannery solid waste. The study was carried out to utilization of solid waste substance from the tannery industry for the production of extracellular lipase enzyme from A. niger. Lipase enzyme was produced from tannery waste substance by using the solid state fermentation (SSF). The fungal lipase was produced from a slaughterhouse waste, and also agro-industrial residue as substrate. The high level lipase activity was at 30 ºC and 96h and the growth study indicate that addition of tannery waste substance and agro-industrial residue influence over the production of lipase enzyme. Mixed substrate fermentation was done for single substrate fermentation (SSF), bi-substrate fermentation (BSF), tri-substrate fermentation (TSF), among three fermentation systems the BSF was selected as high enzyme yields one. The optimization of different parameters like substrate concentration, inoculums range, and moisture content and characterization of fleshing was done. The lipase activity was 404.8 ± 17 U/g dry substrate (U/gds) at 30 C and 96 h and growth studies indicated that addition of WB significantly augmented the biomass and lipase production. Key Words: Beef fleshing, mixed state fermentation, Aspergillus niger, tannery industry. Introduction Enzymes are the focal point of biotechnological process since they are involved in all the aspects of biochemical conversion from the simple fermentation into conversion to the complex techniques in genetic engineering and molecular IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8823

biology. They are used as cost- effective and eco-friendly substitutes for chemical process in several industries. Enzymes have attracted attention from researchers all over the world because of the wide range of physiological, analytical and industrial applications, especially, from microorganisms, because of their broad biochemical diversity, feasibility of mass culture and ease of genetic manipulation. Hence, it is worthwhile to optimize the fermentation medium, which affects the product yield and volumetric productivity of these enzymes (Mala et al., 2007). Solid substrate fermentation (SSF) has built up credibility in recent years for the production of microbial products including enzymes through inexpensive media and it is an appropriate process for developing countries (Singhania et al., 2009). Interest in lipases has greatly increased in recent years due to their various applications in food, detergent, cosmetic, organic synthesis, and pharmaceutical industries (Treichel et al., 2010). Several reports are available on lipase production by SSF using solid substrates including wheat bran (Uvarani et al., 1998), rice bran (Rao et al., 1993) coconut oil cake (Benjamin and Pandey, 1997), gingelly oil cake (Kamini et al., 1998) and soybean meal (Han, 2003). However, reports on lipase production by SSF using mixed solid substrates (Mala et al., 2007) are very much limited and no report is available on the utilization of fleshing in different substrate combinations for the production of lipase from Aspergillus niger. Furthermore, the fermented solid material was directly evaluated for the hydrolysis of fleshing, a low cost feed stock, which is economically and industrially important for the production of fatty acid esters. Materials and Methods Screening of Lipase Producing Fungal Microorganism was done by tributyrin agar medium and Rhodamine B agar medium. Beef Fleshing and Their Characterization has been done and beef fleshing which was used in the present study was solid substance, rich in protein with a mild odour and was obtained from slaughterhouse at Chennai, India. Estimation of Protein Content was done (Kjeldhal, 1883) and extraction of lipids from Beef Fleshing using Soxhlet method has been done. After moisture analysis of beef fleshing, ash Content of Beef Fleshing has been obtained. Electrophoretic method was done for protein estimation and mixed substrate fermentation process was carried out. Inoculum and Fermentation Conditions A fungal strain of A. niger was isolated in our laboratory was used in the present study and it was maintained on Czapek Dox agar slants at 4 C. The spore suspension for inoculation was prepared by adding 2 ml of sterile distilled water to the culture slant and the spores were dislodged using an inoculation needle under aseptic conditions. A spore suspension IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8824

containing 4.3 10 8 spores/ml was used as inoculums. Lipase production was carried out in 250 ml Erlenmeyer flasks, each containing 10 g of different solid substrates either alone or in mixed combinations with two substrates, bi-substrate fermentation (BSF) or three substrates, tri-substrate fermentation (TSF), respectively, with initial moisture content adjusted to 55% with distilled water. The flasks were inoculated with 250 µl of spore suspension and the contents were mixed and incubated at 30 C for 5 days. Samples were taken at 24 h intervals and extraction of the enzyme was carried out according to Kamini et al., (1998). All the experiments were carried out in triplicates and the results were expressed as the average of triplicates. Mixed Substrate Fermentation Lipase Production by Single Substrate Fermentation: Fermentation studies were investigated by the initial moisture content was 55% and inoculum concentration 2.5% (4.3 10 8 spores/g substrate). Using optimized parameters, time course studies on lipase production were carried out for single substrate fermentation. Substrates are wheat bran, wheat raw, coconut oil cake and beef fleshing Lipase Production by BSF: Consecutive optimization studies were investigated by the initial moisture content was 55% and inoculum concentration was about 2.5% (4.3 10 8 spores/g substrate). Using optimized parameters, time course studies on lipase production were carried out for BSF. Lipase Production by TSF: TSF studies were investigated by varying the initial moisture content 60% and inoculum concentration 2.5% (4.3 10 8 spores/g substrate). Using optimized parameters, time course studies on lipase production were carried out for TSF. Optimization of BSF Parameters has been done later with effect of inoculums size on lipase production for BSF, effect of moisture content on lipase production by BSF, effect of extraction of the enzyme. Scale up of Lipase Production: Scale up of lipase production from 10 g flask level to 40 g were carried out. Substrate inoculums grown for 72 h were inoculated into 40g of mixed substrate (moisture content adjusted to 55%) in series of sterilized flasks 96 h and assayed for lipase activity at 24 h intervals. The variation of temperature and humidity during the process was monitored using a portable humidometer. Finally, trimetric determination of lipase assay was carried out (Yamada et al., 1962) IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8825

Results and Discussion Lipolytic Activity of Aspergillus niger Fig 1. Tributyrin Agar Plate Medium Fig 2. Rhodamine B Agar Plate medium Screening of fungal lipolytic activity, using tributyrin and rhodamine B agar plate for lipase production, culture was recognized as potential lipase producers. The zone of clearance in tributyrin agar plate indicate the lipolytic activity of Aspergillus niger. The view of the cultures, which showed orange-red fluorescent halos upon UV irradiation in rhodamine B agar plates. Hence, this strain was selected as potential strain for lipase production was shown in Fig.1 and Fig.2. Sodium Dodecyl Sulphate-Polyacrylamide Gel electrophoresis (SDS-PAGE) Lane 1: crude enzyme, Lane 2: ASP enzyme Lane 3: Purified enzyme (Dialysis) Fig 3. Electrophosis of Protein Sample IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8826

The purified lipase of A.niger were monomeric with molecular weight of 43 kda. An extracellular lipase isolated from the A.niger, had an apparent molecular weight. Other proteins and contamination also present in the agarose gel. The molecular weight of purified enzyme about 43kda was shown in Fig.3. Mixed Substrate Fermentation Single Substrate Fermentation: Lipase production from A. niger was carried out with the substrates WB, COC, WR and beef fleshing and the results are shown in Figure 4 and Table 1. The lipase activities were 260, 192 and 301 U/gds with WB, FL and COC, respectively, at 96 h, while a higher lipase activity of 310 U/gds was obtained with WR at 72h. Fig 4. Lipase Production by Single Substrate Fermentation Table 1. Lipase Production by Single Substrate Fermentation. Substrate 24h 48h 72h 96h 120h WB(10%) 55.3 ± 12 134 ± 19 235.8 ± 15 260.5 ±12 214.1 ± 11 FL(10%) 40.5 ± 17 93.8 ± 13 147.4 ± 18 192.9 ± 17 163 ±14 COC (10%) 60.1 ± 19 192.3 ± 18 281.7 ± 11 301.4 ± 18 258.6 ± 18 WR (10%) 85.5 ± 12 179 ± 17 310.1 ± 16 293.1 ± 18 278.5 ± 16 Bi-substrate Fermentation Accordingly, BSF was carried out by addition of fleshing to WB in different ratio (Table 4.3). Maximal lipase activities of 404 and 345 U/gds were obtained with combinations of FL: WB (1:1) and WB: FL (1:3), respectively, at 96 h. The enzyme yields obtained with other combinations were also higher than individual substrates was shown in Figure 5 and Table 2. IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8827

Fig 5. Lipase Production by BSF Table 2. Lipase Production by BSF Substrate Combination 24h 48h 72h 96h 120h WB(7.5)+FL(2.5) 48.2 ± 12 156.5 ± 16 294.8 ± 12 308.7 ± 18 291.8 ±12 WB(5)+FL(5) 68.1 ± 15 198.7 ± 10 352.3 ± 18 404.8 ± 17 363.5 ±11 WB(2.5)+FL(7.5) 62.4 ± 19 168.6 ± 18 323.5 ± 15 345.3 ± 15 315.2 ±18 Tri-substrate Fermentation In order to enhance the lipase production, TSF experiments were carried out using FL, COC, WB and WR, since maximum lipase activity was obtained with a combination of 5 g of FL and 5 g of WB in BSF (Table 4.3). In TSF, an optimal lipase activity of 422 U/gds was obtained using a mixture of WB, 5 g; COC, 2.5 g and WR, 2.5 g, which was comparatively higher than other combinations of TSF was shown in Figure 6 and Table 3. The initial moisture content and inoculum concentration were found to be the critical factors for lipase production. Accordingly, a maximum yield of 422 U/gds was obtained at 96 h with an initial moisture content of 60% and an inoculum concentration of 2.5%. Fig 6. Lipase Production by TSF IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8828

Table 3. Lipase Production by TSF Substrate Combination 24h 48h 72h 96h 120h WB(5)+WR(2.5)+COC(2.5) 72.1 ±11 180.8 ±16 312.2 ±14 422.7 ±11 389.4 ±18 WB(5)+WR(2.5)+FL(2.5) 51.3 ±15 135.1 ±13 289.7 ±13 335.6 ±17 320.2 ±11 WB(5)+FL(2.5)+COC(2.5) 60.8 ±10 156.7 ±12 295.3 ±11 381.4 ±15 338.1 ±15 FL(5)+WR(2.5)+COC(2.5) 44.5 ±18 128.6±12 258.4 ±17 321.9 ±13 302.1 ±19 Summary Lipase production by mixed substrate fermentation lipase production from A. niger was carried out with the substrates WB, COC, WR and beef fleshing. The lipase activities were 260, 192 and 301 U/gds with WB, FL and COC, respectively, at 96 h, while a higher lipase activity of 310 U/gds was obtained with WR at 72 h. The reported activities with our strain were higher, when compared to the activities of various microorganisms including A. niger and Penicillium candidum with WB (Rivera-Munoz et al., 1991) and Candida rugosa with COC (Benjamin and Pandey, 1997) as substrates. In general, mixed solid substrates are viable substrates for SSF processes. Accordingly, BSF was carried out by addition of COC and WR to WB independently. Maximal lipase activities of 459.1 ± 16 and 362.2 ± 18 U/gds were obtained with combinations of COC: WB (1:3) and WR: WB (1:1), respectively, at 96 h. The enzyme yields obtained with other combinations were also higher than individual substrates, since the nutrients and trace elements present in the BSF enables the organisms to yield more protein favorably by influencing its biochemical pathways for lipase production (Cordova et al., 1998). WR has been used as a substrate for the production of antibiotics like Neomycin (Adinarayana et al., 2003a), Cephalosporin C (Adinarayana et al., 2003b) and Cephamycin C (Kota and Sridhar, 1999) and the present work will serve as a baseline for the production of enzymes using WR as substrate either alone or in mixed combinations with other substrates. Conclusion By modification of various agro-products, a new BSF was developed, which could enhance the growth and production of lipase from A. niger. The lipase production has been scaled up from 10g to 40 kg level and the production of lipase from A. niger is a growth associated process. Having established that A. niger lipase could be effectively used as an additive in detergent formulation, it is of utmost relevance to produce the enzyme in an economically feasible medium. IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8829

The direct use of the fermented substrate for fleshing hydrolysis potentially reduces the cost of biocatalysts with lipases, which will be of great importance in the production of relatively low-value products, such as fatty acid esters. References 1. Adinarayana, K., Ellaiah, P., Srinivasulu, B., Devi, R.B. and Adinarayana, G. 2003a. Response surface methodological approach to optimize the nutritional parameters for neomycin production by Streptomyces marinensis under solid state fermentation, Process Biochem. Vol. 38, pp.1565 1572. 2. Adinarayana, K., Prabhakar, T., Srinivasulu, V., Rao, M.A., Lakshmi, P.J. and Ellaiah, P. 2003b. Optimization of process parameters for cephalosporin C production under solid state fermentation from Acremonium chrysogenum. Process Biochem., Vol. 39, 171 177. 3. Benjamin S and Pandey A. (1997). Coconut cake- a potent substrate for the production of lipase by Candida rugosa in solid-state fermentation. Acta Biotechnol. 17, 241-251. 4. Cordova, J., Nemmaoui, M., Ismaili-Alaoui, M., Morin, A., Roussos, S., Raimbault, M. and Benjilali, B. 1998. Lipase production by solid state fermentation of olive cake and sugarcane bagasse. J. Mol. Catal. B: Enzym., Vol. 5, pp.75 78. 5. Han, B., R.R Beumer, F.M. Rombouts and M. J.R. Nout, 2003. Microbiological safety and quality of commercial sufu- a Chinese fermented soya food. Food Control, 12: 541-547. 6. Kamini NR, Mala JGS, Puvanakrishnan P. (1998). Lipase production from Aspergillus niger by solid-state fermentation using gingelly oil cake. Proc. Biochem. 33, 505-511. 7. Kjeldahl, J. 1883.A new method for the determination of nitrogen in organic matter. Zeitschreft fur Analytische Chemie. 22: 366. 8. Kota, K.P., Sridhar, P. 1999. Solid state cultivation of Streptomyces clavuligerus for cephamycin C production, Process Biochem., Vol. 34, pp. 325 328. 9. Mala, J.G.S., Edwinoliver, N.G., Kamini, N.R., Puvanakrishnan, R. 2007. Mixed substrate solid state fermentation for production and extraction of lipase from Aspergillus niger MTCC 2594, J. Gen. Appl. Microbiol., Vol. 53, pp. 247 253. IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8830

10. Rao PV, Jayaraman K and Lakshmanan CM (1993) Production of lipase by Candida rugosa in solid state fermentation. 1: determination of significant process variables. Proc. Biochem. 28, 385-389. 11. Rivera-Munoz, G., Tinoco-Valencia, J.R., Sanchez, S., Farres, A. 1991. Production of microbial lipases in a solid state fermentation system, Biotechnol. Lett., Vol. 13, pp.277 280. 12. Singhania, R. R; Patel, A. K., Soccol, C. R.; Pandey, A. 2009. Recents advances in solid-state fermentation. Biochemical Engineering Journal, Amsterdam, v. 44, n. 1, p. 13-18. 13. Treichel H, Oliveira D, Mazutti, MA, Luccio, M, Oliveira JV (2010).A review on microbial lipases production. Food Bioprocess Tech. 3 (2): 182-196. 14. Uvarani G, Jaganathan L, Shridas P and Boopathy R (1998) Purification and characterization of lipase from Rhizomucor miehei. J. Sci. Ind. Res. 57, 607-610. 15. Yamada, K., U. Ota, and H. Machinda. 1962. Studies on the production of lipase by microorganism. Quantitative determination of lipase. Agricultural and Biological Chemistry. 26: 63-69. Corresponding Author: **A. Manikandan, Email: manikandan.mpa@gmail.com IJPT Sep-2015 Vol. 7 Issue No.2 8823-8831 Page 8831