Characteristics of a β-1,4-D endoglucanase from Trichoderma virens wholly applied in a palm-fruit husk-based diet for poultry layers

Odeniyi, Olubusola A.; Onilude, Anthony A.; Ayodele, Maria A.

doi:10.1590/S1517-83822012000400031

Abstract

The characteristics of an endoglucanase produced by a Trichoderma virens strain T9 newly isolated from a palm-fruit husk dump site, its physiological characteristics and enzyme production were studied. Whole cells of the depolymerizing-enzyme producing T. virens were applied to palm-fruit husk and bird performance characteristics when employed as poultry diet additive were considered. Endoglucanase activity in submerged fermentation was 1.6 nkat. Optimum activity was recorded at pH 6.0 and 55ºC. The enzyme retained 50% residual glucanase activity at 70ºC for 10 minutes. 1.0% Tween-80 and SDS yielded endoglucanase activity 2.15 times higher than the control. Activity wasboosted by 20mM Ca2+ (115.0%); 10mM K+ (106.5%); and was totally inhibited by 1mM Hg2+. The addition of T. virens -fermented palm-fruit husk with other layer feed components on the bird characteristics showed that change in bird weight between the control and test birds were not significantly different (p>0.05) but differed in terms of daily feed ingested (p<0.05). The feed to weight-gain ratio was best with the unmodified palm-fruit husk based diet (8.59). There was no significant difference in the egg weights from modified palm-fruit husk based diet and control (p>0.05). The shell thickness (0.64mm) and yolk content (23.61%) were highest in the microbially-modified husk diet. The alternative to maize based diets proffered by the application of T. virens -modified palm-fruit husk in poultry nutrition in terms of bird weight and feed to weight-gain ratio affords the poultry farmer an economic advantage and allows for a greater utilization of the maize in human diets.

Trichoderma virens; endoglucanase; physiology; poultry layer feed

INDUSTRIAL MICROBIOLOGY

Characteristics of a β-1,4-D endoglucanase from Trichoderma virens wholly applied in a palm-fruit husk-based diet for poultry layers

Olubusola A. OdeniyiI, ^* * Corresponding Author. Mailing address: Microbial Physiology and Biochemistry Research, Department of Microbiology, University of Ibadan, Ibadan, Nigeria.; Tel.: +234-8025198741.; E-mail: busolaodeniyi@gmail.com ; Anthony A. Onilude^I; Maria A. Ayodele^II

^IMicrobial Physiology and Biochemistry Research, Department of Microbiology, University of Ibadan, Ibadan, Nigeria

^IIGermplasm Health Unit, International Institute of Tropical Agriculture, Ibadan, Nigeria

ABSTRACT

The characteristics of an endoglucanase produced by a Trichoderma virens strain T9 newly isolated from a palm-fruit husk dump site, its physiological characteristics and enzyme production were studied. Whole cells of the depolymerizing-enzyme producing T. virens were applied to palm-fruit husk and bird performance characteristics when employed as poultry diet additive were considered. Endoglucanase activity in submerged fermentation was 1.6 nkat. Optimum activity was recorded at pH 6.0 and 55ºC. The enzyme retained 50% residual glucanase activity at 70ºC for 10 minutes. 1.0% Tween-80 and SDS yielded endoglucanase activity 2.15 times higher than the control. Activity wasboosted by 20mM Ca²⁺ (115.0%); 10mM K⁺ (106.5%); and was totally inhibited by 1mM Hg²⁺. The addition of T. virens -fermented palm-fruit husk with other layer feed components on the bird characteristics showed that change in bird weight between the control and test birds were not significantly different (p>0.05) but differed in terms of daily feed ingested (p<0.05). The feed to weight-gain ratio was best with the unmodified palm-fruit husk based diet (8.59). There was no significant difference in the egg weights from modified palm-fruit husk based diet and control (p>0.05). The shell thickness (0.64mm) and yolk content (23.61%) were highest in the microbially-modified husk diet.

The alternative to maize based diets proffered by the application of T. virens -modified palm-fruit husk in poultry nutrition in terms of bird weight and feed to weight-gain ratio affords the poultry farmer an economic advantage and allows for a greater utilization of the maize in human diets.

Key words: Trichoderma virens, endoglucanase, physiology, poultry layer feed

INTRODUCTION

Plant matter represents a major source of renewable organic matter (9, 19). Their composition makes them of veritable biotechnological value (12). In the tropics and around the world, a lot of plant materials are generated all the year round through forestry and agro-industrial practices and thus constitute pollution problems. These problems are generally solved in developing countries through the burning of biomass especially to create space for a new planting season. However, these agricultural 'wastes' can be potentially converted to value-added renewable bio-products such as fuels, chemicals, improved animal feeds, and cheap energy sources for fermentation (9). Even though the composition of plant matter is basically crystalline with insoluble cellulose fibrils and surrounding amorphous regions of hexoses and pentoses (22, 23), interactions of many bacteria and fungi with them are quite complex.

Microbial degradation of plant structural polysaccharides requires an array of microbial enzymes which work synergistically to achieve effective hydrolysis (2, 3). Microorganisms are known to produce these enzymes (8, 13) for cellulose hydrolysis. Types of microbial cellulases enlisting different modes of action (3), have been documented to include endoglucanases (carboxymethylcellulases) which hydrolyse the amorphous regions of the plant cellulose structure; exoglucanases (cellobiohydrolases) which progressively cleave units of cellobiose from the crystalline or amorphous ends of the cellulose structure while β-glucosidases (cellobiases) hydrolyse soluble cellooligosaccharides into glucose units. Many Trichoderma species have been described to possess cellulose-degrading capacities (14, 20, 25, 29).

Palm fruit abounds in the western part of Africa and has been the traditional source of oil, especially for cooking. Palm-fruit husk is a readily accessible fibrous substrate obtained after oil extraction from the fruits. This by-product, termed 'Oguso' in the western part of Nigeria, finds application only during massive cooking where it aids the effective combustion of fire wood. Therefore palm oil producers dry up the husk and sell for such purposes only. The alternative use of this husk, in conjunction with T. virens, especially in enzyme production and animal nutrition towards ensuring food security is considered in this work.

MATERIALS AND METHODS

Microorganism and culture conditions

The Trichoderma virens isolate was obtained from a natural palm-fruit husk dump site within Ibadan metropolis, Nigeria, and cultivated on Potato Dextrose agar (Sigma) at 27± 2ºC. The isolate was identified based on morphological characteristics and DNA sequencing as T. virens strain isolate PFH (palm fruit husk) T9. Five day-old cultures were used to inoculate sterilized palm-fruit husk of mesh size 5mm² in a solid substrate experimental set-up. The Trichoderma virens isolate was used as an enzyme preparation consisting of whole cells (7, 17).

Enzyme production and characterisation

Screening for the production of endo-1,4-β glucanase was effected using a medium described by Yeoh et al. (27). A 3mm disc of 5-day old T. virens culture was centrally located on an agar plate containing 1.0% cellulose and 4.5% w/vCzapek Dox agar. Plates were flooded after 3 days with hydrochloric acid and iodide mixture {(1ml 0.1M HCl) and (5ml of 1%w/vI₂ and 2% w/v KI)} and the zone of clearing to the fungal diameter recorded. Enzyme production was carried out using submerged fermentation at 27ºC with orbital shaking at 125 rpm on a rotary Orbit shaker bath, (Lab-line instruments, Illinois, USA).This involved cultivating two 3 mm plugs of T. virens in 50 mL of culture medium made up of 1% Carboxymethylcellulose (CMC), 0.14% (NH₄)₂SO₄, 0.6% K₂HPO₄, 0.20% KH₂PO₄ and 0.01% MgSO₄7H₂O, pH 6.0 in a 250 mL Erlenmeyer flask.The mycelium was harvested after 4 days of growth from the culture liquid by centrifugation at 2795Xg using Hermle^® centrifuge (Germany). The supernatantwas used as crude enzyme for all practical purposes.

Partial purification of Enzyme

The concentrated extracellular enzyme extract was subjected to ammonium sulphate precipitation, dialysis and column chromatography. Ammonium sulphate was added up to 80% saturation; the solution was kept overnight at 4.0 ºC and centrifuged at 13000Xg for 20 minutes. The enzyme solution was dialysed against 0.1M citrate phosphate buffer (pH 6.0) and loaded onto a BioRad^® AG 1-X4 resin previously equilibrated with 0.1M citrate phosphate buffer. The column was washed with the same buffer at a flow rate of 36mlh^-1. Three millilitre fractions were collected and those exhibiting enzyme activity were pooled.

Total protein and Enzyme assays

Soluble protein in culture filtrate was measured bythe method of Lowry et al., (1951) using bovine serum albumin as standard. The activity of the Endo-1,4-β glucanase extract was determined by the method of Robson and Chambliss (21) and the reducing sugar formed was measured as glucose by the dinitrosalicylic acid procedure of Miller et al. (15). One unit of enzyme activity is expressed as the amount which corresponds to the release of 1 nano mole equivalent of glucose per second under the stated conditions.

Characterisation of T. virens Degrading Activity

The pH effect on cellulolytic activity of the isolate T. virens was conducted in 0.1M citrate phosphate assay buffers of pH 4.0 to 9.0. The same Endo-1, 4-β glucanase assay was carried out at various temperatures (27, 40, 50, 60, 70, 80, 90 and 100ºC) and time intervals of 5, 10, 15, 30 and 60 minutes. The effect of metal salts on enzyme activity was carried out by pre-incubating the enzyme in metal salt solutions of calcium, cobalt (20 mM), potassium, lithium (10 mM) and mercury (1 mM Hg2+) for 60 minutes and the residual activities determined. To analyse the effect of different surfactants on enzyme activity, 1ml of 0.05, 0.1, 0.1, 1.0 and 5.0% of polyoxyethylene sorbitanmono-oleate (Tween 80), polyethylene glycol p-isooctylphenylether (Triton X-100) and Sodium Dodecyl Sulphate (SDS) was incubated with 1mL enzyme then assayed using the standard procedure as described above.

Feeding experiment

Birds: Thirty-six, 26 weeks-old point-of-lay ISA brown birds were purchased from a commercial poultry farm in Ibadan, Nigeria. The birds were distributed into three treatments of 12 birds each, the choice of treatment depending on the feed type and microbial addition. Each treatment was arranged into replicates of 6 birds. They were identified with individual leg rings and randomly assigned with 2 birds per cage. The experiment spanned four weeks.

Fermentation of palm-fruit husk: Multiples of a mixture of 5g of palm-fruit husk with a mineral solution (MS) mixture of 10 ml of 1% (NH₄)₂SO₄ and 0.02% MgSO₄ (at a total of 67% of moisture) were autoclaved. Each flask was inoculated by transferring 3mm agar plug excisedfrom the margin of a 5-day-old T. virens culture and incubated for 48 hours in a solid substrate fermentation system. The fermented and non-fermented husk substrates were each mixed in a mash with other poultry layer feed components as shown in Table 2 to make bird feed.

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Feed: Birds were fed a basal diet in which the maize component was entirely substituted for with palm-fruit husk with or without the addition of T. virens strain isolate PFH T9. The normal feed diet and other feed components were obtained commercially from Amo-Byng^® Feed, Awe, Oyo State. Palm-fruit husk was obtained after the traditional extraction of oil from the fruit. All birds were allowed free access to feed and water. The analytical composition (26) of both the microbial and non-microbially modified palm-fruit husk diet and control diet is as stated in Table 1.

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Monitoring of Birds' performance Characteristics: Feed consumption and increase in body weight were monitored throughout the duration of the experiment with an electronic weighing balance. The egg characteristics considered included weight, yolk and shell characteristics. The experimental data were analysed using an ANOVA test with p<0.05 considered significant. To determine significant differences between treatment groups for substrate, and microbial additive effects, a t-test was done using Graph-pad Prism 4.0 software.

RESULTS

Screening for ability of T. virens isolate to produce endo-1,4-β glucanase revealed a ratio of cleared zone to fungal diameter of 5.8. Enzyme assay showed an endo-1,4-β glucanase activity of 1.6n kat. With increasing pH, the endo-1,4-β glucanase activity increased gradually between 4.0 and 5.0, then sharply at 6.0 (Figure 1). Beyond this range, enzymatic activities gradually decreased as the pH approached a neutral then alkali range. Conversely, the growth rate rapidly decreased beyond pH 4.0. The highest thermal stability exhibited by this enzyme spanned 27ºC to 40ºC throughout the incubation periods applied and at 50ºC up to 10 minutes (Figure 2). Beyond this time, enzymatic activities reduced to 46.7% after 60 minutes. At 60ºC, percentage residual activity was higher at 5 and 10 minutes (73.3%) then reduced at 15 minutes (63%). After this, as temperature increased, values consistently reduced. A residual glucanase activity of 50% was realized at 70ºC and 10 minutes. The least response to changes (23.3%) was demonstrated at 90ºC for 5 minutes. Complete inactivation was recorded beyond this temperature and time regime.

Cobalt ion repressed the activities of the endo-1,4-β glucanase (37.5%) while Hg²⁺ totally inhibited it (Figure 3). K⁺ and Ca²⁺ raised activity by 6.5% and 15% respectively. Tween-80 and SDS at 1.0% concentration gave the highest endo-1,4-β glucanase activity (3.4nkat), followed by values at 0.5% (Figure 4). Triton X-100 yielded its best endo-1,4-β glucanase activity at 0.5% concentration. A purification factor of 6.57 with 369.03% yield was achieved with the endo-1,4-β glucanase showing a specific activity of 3.99nkat/mg protein (Table 2).

The highest daily feed was consumed by the control diet birds (Table 3), while the least was by the birds maintained on the plain husk diet (130.6g). There was no significant difference (p>0.05) in daily bird weight gain, however, increase in bird weight was numerically highest for the birds maintained on the control feed (15.14g/day). The least feed/gain ratio was recorded from the husk diet without fungal inclusions. From Table 4, egg production and egg weight were significantly different (P< 0.05) and numerically higher from the control diet. The least was from the husk diet without fungal inclusions. The albumen content was highest (67.51%) from the control diet. The highest values recorded for the dry shell weight, wet shell weight and the shell thickness were from the microbially-modified palm-fruit husk-based diet (Table 5). This was followed by that from the control experiment and least from the husk diet without fungal additions. The dry shell weight was not significantly different when subjected to a one way ANOVA analysis. The results from the analysis of wet eggshell weight recorded the same pattern documented for the dry shell weight. There were significant differences in the shell thicknesses from the 3 tests (p< 0.05). The highest quantity of yolk was recorded from the birds maintained on the diet of husk and T. virens (Table 6). The least was from the control diets. Egg cholesterol /50ml egg weight was least with the un-modified husk diet fed on layers. That of the control birds was higher (216.3mg/50ml) and the highest quantity of egg cholesterol was recorded in birds fed the microbially-modified experimental diet. By ANOVA, there was no significant difference in the yolk values, while there was for the egg cholesterol results. Non-parametric results showed a significant difference (p< 0.05), in the yolk quantities between the husk diet with T. virens and the control diet.

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DISCUSSION AND CONCLUSION

The genus Trichoderma has been known as a high producer of cellulases many of which have been characterized (18). The effect of H⁺ concentration in reaction mixtures on enzymatic activities work in conjunction with other factors within the reaction mixture such as the ionization state of the enzyme, the enzyme-substrate complex and the molecular weights of the enzymes (6, 29). It was interesting to note that while fungal growth was most supported at pH 4.0 and reduced as the pH range increased, the endo-1,4-β glucanase recorded an activity peak at pH 6.0 and had activity throughout all the pH ranges applied. This shows that the T. virens endo-1,4-β glucanase has a broad range of pH activity, is pH tolerant and so may be employed in various industrial processes at all these ranges. Fungi are known to express enzymatic activities across a wide pH range and some retain activity through all.

Stability to temperature change is an important characteristic in enzymology and assists in the choice of the enzyme selected for industrial purposes especially those involving a high temperature step. Nagieb et al. (16), described a T. reesei cellulase with temperature stability up to 45ºC, a gradual loss to 60ºC beyond which a rapid loss of activity occurred. The T. virens endoglucanase studied in this work was similar in that at 60ºC and beyond no activity was recorded after 60 minutes and a sharp activity loss was consistently observed as incubation time increased. Temperature and pH were found to be important parameters which influenced enzyme activity. All these enzymatic responses would probably come into play in the successive colonization and the sequential degradation of structural plant polysaccharides (10, 24).

Metal ions possess either an inhibitory or stimulatory effect on microbial enzymes. On the endo-1,4-β glucanase tested, the activation was most elicited by calcium and potassium ions. The activity of this enzyme cannot be said to be conclusively dependent on the presence of cations since two other divalent ions inhibited enzymatic activities. While some hydrolytic enzymes would require the involvement of divalent cations (5), others, like the activities of a Meloidogyne incognita reported by Bera-Maillert et al. (4) do not. All the surfactants used augmented the activities of the endo-1,4-β glucanase enzyme. Surfactant enhancement was most exhibited through the addition of 1.0% SDS at all the concentrations enlisted. This was followed by that of Tween 80 and least by Triton-X-100. The endo-1,4-β glucanase activities were improved by more than 43.75% of the control enzyme through the inclusion of surfactants to the reaction mixture. The reduction in surface tension, created by the addition of the different surfactants allowed more active sites on the CMC substrate for the endo-1,4-β glucanase to bind to and as such improved the amount of reducing sugars generated. The endo-1,4-β glucanase specific activity and yield decreased at the ammonium sulphate step. Both increased, slightly and very sharply respectively at the column chromatography relative to the crude.

Animal experiment showed that feed consumption was best with the conventional feed and there was a significant difference between the quantity consumed by the test and control groups. Amongst the husk samples, feed consumption was numerically close and statistically insignificant. The slightly higher numerical value shows that the inclusion of the fungus assisted the layer birds in ingesting more feed quantities than they might have. The feed to gain ratio, however, showed the least feed quantity needed to record a 1g increase in weight was from the unmodified palm-fruit husk modified diet. Interestingly, almost 10g of feed intake was required to elicit a 1g increase in body weight of the control birds maintained on the conventional diets. Increases in bird weights were not significantly different among test groups and also within the test and control groups. There was no significant effect of husk addition or microbial inclusions upon the bird weight gains studied. However, there was a highly significant difference of husk inclusion upon the quantity of feed ingested between the test and control bird responses. Non-parametric results of egg production and egg weight showed that best values were recorded from the control diet and there were no significant differences in husk treatments with and without microorganism (p>0.05). There was, however, between the test and control experiments. Between the palm-fruit husk diets and the control, the results of the shell thickness showed there was a significant difference in favour of birds maintained on T. virens- modified diet. Microbial inclusions provided the highest eggshell thickness. The weights recorded for the eggshells in their wet and dried states did not demonstrate a significant statistical difference. The highest shell weight was obtained from the microbially-modified husk-fed layers. Microbial inclusion would obviously be beneficial from the values presented especially in terms of improving the final quality of the eggs sold to the consumers. A thick egg shell and weight would discourage easy breaking and cause more profit to be made by the farmer. Yolk parameters also showed that microbial inclusions afforded higher quantities of yolk. This is of great importance in human nutrition since the yolk is the most nutritive component of the poultry egg. The need to ensure food security and make enough maize substrate available for human nutrition instead of the constant competition between man and animals for the same nutritive substrate has caused research to focus on the effects of incorporating different concentrations of palm-kernel fibre into poultry diets. Ahmad (1) reported the recycling of products of palm-oil mill effluent into fertilizers and animal feed in order to maximize available resources and preserve the environment.

To the best of our knowledge, this is the first report on the complete incorporation of T. virens with the external husk component of oil-palm fruit into a poultry layer diet totally devoid of maize substrate. Since there was no significant difference in the bird weight values, and the feed to gain ratio were better with husk diets, the two husk treatments may be employed as substitutes for or partially incorporated into maize based diets in poultry layer nutrition. The husk diets might also generate 'earlier satiety' in birds such that excess maize is not ingested as a result of the compulsive pecking habits of the birds.

ACKNOWLEDGEMENTS

The authors are grateful to the authorities of the International Institute of Tropical Agriculture, Ibadan, Nigeria for the use of research facilities in the Germplasm Health Unit Laboratory. All national guidelines regarding the treatment, care and use of animals were strictly adhered to.

Submitted: May 22, 2010

Returned to authors for corrections: January 26, 2012

Approved: June 07, 2012.

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*

Corresponding Author. Mailing address: Microbial Physiology and Biochemistry Research, Department of Microbiology, University of Ibadan, Ibadan, Nigeria.; Tel.: +234-8025198741.; E-mail:

busolaodeniyi@gmail.com

Publication Dates

Publication in this collection
19 Feb 2013
Date of issue
Dec 2012

History

Received
22 May 2010
Accepted
07 June 2012
Reviewed
26 Jan 2012

This work is licensed under a Creative Commons Attribution-NonCommercial 4.0 International License.

[1] 1. Ahmad, F. (2001). Sustainable agriculture system in Malaysia. Paper presented at the Regional Workshop on Integrated Plant Nutrition System (IPNS), Development in Rural Poverty Alleviation, United Nations Conference Complex, Bangkok, Thailand. P.18-20

[2] 2. Baker, J.O.; Adney, W.S.; Thomas, S.R.; Nieves R.A.; Chou Y.C.; Vinzant T.B.; Tucker M.P.; Laymon R.A.; Himmel M.E. (1995). Synergism between purified bacterial and fungal cellulases. In Saddler J. N., Himmel M. E.(eds.). Enzymatic degradation of insoluble carbohydrates American Chemical Society Symposium Series 618. American Chemical Society, Washington, D.C., p. 113 - 141

[3] 3. Beguin, P.; Aubert, J.P. (1994). The biological degradation of cellulose. FEMS Microbiol. Rev., 13, 25 - 58.

[4] 4. Bera-Maillert, C.; Arthaud, l.; Abad, P.; Rosso, M. N. (2000a). Biochemical characterization of M1-ENG1, a family 5 endoglucanase secreted by root knot nematode Meloidogyne incognita Eur. J. Biochem., 267, 3255-3263.

[5] 5. Bera-Maillet, C.; Broussolle, V.; Pristas, P.; Giardeau, J.P.; Guidet, G.; Forano, E.(2000b). Characterization of endoglucanases EGB and EGC from Fibrobacter succinogenes, Bio. Biophys. Acta, 1476, 191-202.

[6] 6. Dixon, M.; Webb, E.C. (1971). Enzymes Longman group Ltd. London. 67-188.

[7] 7. Food Chemical Codex National Academy of Sciences Food and Nutrition Board, (1981). Food Chemicals Codex 3rd Ed. Washington, DC: National Academy Press.

[8] 8. Gilkes, N.R.; Langsford, M.T.; Wakarchuk, W.W.; Kilburn D.G.; Miller R.C.; Warren R.A.J.(1984). The cellulase system of Cellulomunas finni J. Gen. Microbiol. 130, 1367-1376.

[9] 9. Howard, R.L.; Abotsi, E.; Jansen van Rensburg, E.L.; Howard, S. (2003). Lignocellulose biotechnology: issues of bioconversion and enzyme production. Afr. J. Biotechnol, 2, 602-619.

[10] 10. Li, X.; Gao, P. (1997). CMC-liquefying enzyme, a low molecular mass initial cellulose-decomposing cellulase responsible for fragmentation from Streptomyces sp. LX J. Appl.Microbiol. 83, 59-66.

[11] 11. Lowry, O.H.; Rosebrough, N.J.; Farr, A.L.; Randall, R.J. (1951). Protein measurement with the Folin Phenol reagent. J. Biol. Chem. 193, 265 - 275.

[12] 12. Malherbe, S.; Cloete, T.E. (2003). Lignocellulose biodegradation: fundamentals and applications: A review. Environ. Sci. Biotechnol. 1,105-114.

[13] 13. Mansfield, S.D.; Saddler, J.N.; Gubitz, G.M. (1998). Characterization of endoglucanases from the brown rot fungi Gloeophyllum sepiarium and Gloeophyllum trabeum Enz. Microbiol. Technol. 23, 133 - 140.

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Characteristics of a β-1,4-D endoglucanase from Trichoderma virens wholly applied in a palm-fruit husk-based diet for poultry layers

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