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Novel process for the simultaneous extraction and degumming of banana fibers under solid-state cultivation

Novo processo para a extração e simultânea degomagem de fibras de banana

Abstracts

Various process parameters for the production of polygalacturonase by Streptomyces lydicus under solid-state fermentation were optimized. The optimum particle size of wheat bran for polygalacturonase production was in the range of 500-1000 µm. Initial moisture content of 70% was found to be the optimum for enzyme production. The most suitable inoculum size was 1.25 x 10(5) CFU/mL and the optimum incubation temperature was 30ºC. Addition of carbon sources resulted in 37% increase in enzyme yield (425 U/g), whereas no significant enhancement was obtained on nitrogen supplementation. Maximum enzyme yield was recorded at 72 h. When compared to the initial production medium (108.5 U/g), the enzyme yield was 3.9 fold after optimization. Solid-state fermentation was effectively employed to develop a novel process for the simultaneous extraction and degumming of banana fibers. Streptomyces lydicus was allowed to grow on wheat bran medium in which banana leaf sheath pieces were incorporated and the fiber bundles were separated after a two-step fermentative process.

Banana fiber degumming; Solid-state fermentation; Polygalacturonase; Streptomyces lydicus; Wheat bran


Vários parâmetros de processo de produção de poligalacturonase por Streptomyces lydicus por fermentação em estado sólido foram otimizados. O tamanho ótimo de partícula de farelo de trigo para a produção de poligalacturonase esteve na faixa de 500 a 1000 mm. O teor inicial de umidade de 70% foi o melhor para a produção da enzima. O inóculo inicial mais adequado foi de 1,25 x 10(5) UFC/mL e a temperatura ótima de incubação foi 30ºC. A adição de fontes de carbono resultou em aumento de 37% no rendimento da enzima (425U/g), enquanto que a suplementação com nitrogênio não melhorou o rendimento. O rendimento máximo da enzima foi obtido em 72h. A otimização resultou em um aumento de 3,9 vezes na quantidade de enzima produzida inicialmente (108,5U/g). A fermentação em estado-sólido foi eficiente para o desenvolvimento de um novo processo de extração e simultânea degomagem. Streptomyces lydicus foi cultivado em meio de farelo de trigo acrescentado de fragmentos de folhas de banana, sendo os feixes de fibras separados após um processo de fermentação em dois passos.

Degomagem de fibras de banana; fermentação em estado sólido; poligalacturonase; Streptomyces lydicus; farelo de trigo


INDUSTRIAL MICROBIOLOGY

Novel process for the simultaneous extraction and degumming of banana fibers under solid-state cultivation

Novo processo para a extração e simultânea degomagem de fibras de banana

Nicemol Jacob; Parukuttyamma Prema* * Corresponding Author. Mailing address: Biotechnology Division, National Institute for Interdisciplinary Science and Technology (CSIR), Trivandrum, 695019, India. Phone: ++91 471 25 15 325; Fax: ++91 471 24 91 712. E-mail: premar51@rediffmail.com

Biotechnology Division, National Institute for Interdisciplinary Science and Technology (CSIR), Trivandrum, India

ABSTRACT

Various process parameters for the production of polygalacturonase by Streptomyces lydicus under solid-state fermentation were optimized. The optimum particle size of wheat bran for polygalacturonase production was in the range of 500-1000 µm. Initial moisture content of 70% was found to be the optimum for enzyme production. The most suitable inoculum size was 1.25 x 105 CFU/mL and the optimum incubation temperature was 30ºC. Addition of carbon sources resulted in 37% increase in enzyme yield (425 U/g), whereas no significant enhancement was obtained on nitrogen supplementation. Maximum enzyme yield was recorded at 72 h. When compared to the initial production medium (108.5 U/g), the enzyme yield was 3.9 fold after optimization. Solid-state fermentation was effectively employed to develop a novel process for the simultaneous extraction and degumming of banana fibers. Streptomyces lydicus was allowed to grow on wheat bran medium in which banana leaf sheath pieces were incorporated and the fiber bundles were separated after a two-step fermentative process.

Key-words: Banana fiber degumming, Solid-state fermentation, Polygalacturonase, Streptomyces lydicus, Wheat bran.

RESUMO

Vários parâmetros de processo de produção de poligalacturonase por Streptomyces lydicus por fermentação em estado sólido foram otimizados. O tamanho ótimo de partícula de farelo de trigo para a produção de poligalacturonase esteve na faixa de 500 a 1000 mm. O teor inicial de umidade de 70% foi o melhor para a produção da enzima. O inóculo inicial mais adequado foi de 1,25 x 105 UFC/mL e a temperatura ótima de incubação foi 30ºC. A adição de fontes de carbono resultou em aumento de 37% no rendimento da enzima (425U/g), enquanto que a suplementação com nitrogênio não melhorou o rendimento. O rendimento máximo da enzima foi obtido em 72h. A otimização resultou em um aumento de 3,9 vezes na quantidade de enzima produzida inicialmente (108,5U/g). A fermentação em estado-sólido foi eficiente para o desenvolvimento de um novo processo de extração e simultânea degomagem. Streptomyces lydicus foi cultivado em meio de farelo de trigo acrescentado de fragmentos de folhas de banana, sendo os feixes de fibras separados após um processo de fermentação em dois passos.

Palavras-chave: Degomagem de fibras de banana, fermentação em estado sólido, poligalacturonase, Streptomyces lydicus, farelo de trigo.

INTRODUCTION

Plant fibers are schlerenchymatous cells with heavily lignified cell walls having a narrow lumen in cross section. Fiber cells are dead at maturity and serve as a support tissue (1). Natural fibers possess several advantages over synthetic fibers such as low density, appropriate stiffness and mechanical properties and also high disposability and renewability (11). Also, they are recyclable and biodegradable (2). Banana fibers can be used for various purposes such as in textile, paper or handicrafts industry. Banana paper is versatile as it is waterproof and stronger than wood-pulp paper, meaning it can be used in packaging and even as a basis for building materials. India is the first banana fruit producer in the world and the yield is 16 million tons per year. After harvesting, the pseudostem of banana is disposed as a waste material. The fiber content of the above material is 54.3% and can be effectively used as a source of natural fibers.

Banana fibers can be extracted by employing chemical, mechanical or biological methods. Chemical method causes environmental pollution, while mechanical method fails to remove the gummy material from the fiber bundle surface. Biological procedures yield more fiber bundles than the other two procedures without any harm to the environment. The extraction of banana fibers using biological natural retting has already been reported (2). After extracting the fibers, degumming is essential prior to the utilization of fibers. The removal of heavily coated, non-cellulosic gummy material from the cellulosic part of plant fibers is called degumming (16).

Pectinases have a leading role in the degumming of natural fibers by removing interlamellar pectin which acts as a cementing substance between the fibers. Solid-state fermentation (SSF) is an efficient tool for microbial enzyme production including pectinases. The yield of a desired product under SSF depends upon several factors like particle size of the substrate, initial moisture content of the medium, incubation temperature etc. and hence it is essential to optimize the levels of these factors.

The aim of the present investigation was to study the effect of process parameters and nutrient supplementation on polygalacturonase production by Streptomyces lydicus in solid-state fermentation using wheat bran and to develop a novel process for the simultaneous extraction and degumming of banana fibers utilizing polygalacturonase produced by Streptomyces lydicus.

MATERIAL AND METHODS

The microorganism

The novel strain of Streptomyces lydicus MTCC 7505 used in the present investigation was isolated from mangrove sediment (7) and was maintained on starch casein agar slants at 4ºC.

Inoculum preparation

Broth media used for the preparation of inoculum contained (g/L) (NH4)2SO4: 2; K2HPO4: 2; KH2PO4: 2; yeast extract: 3 and pectin: 5 (pH 7.0). The strain was inoculated into 100 mL of the broth in 250 mL Erlenmeyer flask and incubated for 24 h at 30ºC and 175 rpm in a rotary shaker. The inoculum contained 2.5 x 104 colony forming units (CFU) / mL.

Solid-state fermentation

Solid-state fermentation was carried out in 250 mL Erlenmeyer flasks with 10 g of wheat bran with a particle size of 500-1000 µm. The solid substrate was moistened with a solution containing (g/L) (NH4)2SO4: 4; K2HPO4: 4 and KH2 PO4: 4 (pH - 7.0), autoclaved for 45 min and inoculated with 5 mL of broth culture. The final moisture content of the flask was 50 %. Flasks were incubated for four days at 30ºC.

Optimization of process parameters

Various process parameters were optimized such as particle size of the substrate (>300, 300-500, 500-1000 and 1000-2000 µm), initial moisture content of the medium (30, 40, 50, 60, 70 and 75%), pH of the moistening solution (5.0, 6.0, 7.0, 8.0, 9.0 and 10.0), inoculum size (2.5, 5, 7.5, 10, 12.5 and 15 mL) and incubation temperature (27, 30, 33 and 36ºC). Optimization of initial moisture content was performed, maintaining the concentration of mineral salts constant, varying only the volume of distilled water so that mineral salts should not have any differential influence on growth and enzyme production. Supplementation of the growth media with 1% (w/w) of different carbon sources (glucose, galacturonic acid, sucrose, starch and pectin,), 1% (w/w) of organic nitrogen sources (yeast extract, peptone, urea and corn steep solids) and inorganic nitrogen compounds in terms of available nitrogen (0.004%, w/w) ((NH4)2HPO4, KNO3, NH4HCO3, NH4Cl and (NH4)2SO4) was also attempted. The mineral salt solution used was devoid of (NH4)2SO4, while studying the influence of nitrogen sources.

Enzyme extraction

After fermentation, the fermented material was mixed with distilled water and homogenized by keeping in a rotary shaker at 200 rpm for 1 h. Filtration was carried out through muslin cloth and the resultant filtrate was centrifuged for 20 min at 10,000 rpm and 4ºC. The supernatant was used as the enzyme source for analytical experiments.

Analytical procedures

Assay for polygalacturonase

Polygalacturonase activity was determined according to Honda et al (4). Reaction mixture containing 0.5 mL of suitably diluted enzyme was incubated with 0.5 mL of 0.5% polygalacturonic acid (SIGMA) in 100 mM McIlvaine buffer (pH 7.0) for 30 min at 50ºC. The reaction was interrupted by adding 2 mL of 100 mM borate buffer (pH 9.0) followed by 1 mL of 1% cyanoacetamide. The mixture was immersed in a boiling water bath for 10 min, cooled and read against a suitable blank at 276 nm using a spectrophotometer (Model UV PC 2401, Shimadzu Corporation, Japan). One unit (U) of polygalacturonase was defined as the amount of enzyme required to release 1 µmol of galacturonic acid from polygalacturonic acid min-1 under the assay conditions.

Estimation of biomass

Biomass estimation was carried out by determining the N-acetyl glucosamine content of the cell wall (17) and it was expressed as mg of glucosamine/g dry fermented matter.

Dry weight determination

A suitable amount of the fermented matter was dried in oven till constant weight and the dry weight of the sample was calculated.

Banana fiber degumming

Banana leaf sheath treatment was performed in 250 mL Erlenmeyer flasks and the treatment medium contained 10 g of wheat bran (500- 1000 µm) and 0.1 g of pectin, moistened by a salt solution of (g/L) K2HPO4: 4 and KH2PO4: 4 (pH-6.0). The leaf sheath pieces (30 x 10 x 2 mm) were incorporated in the above medium, autoclaved for 45 minutes and inoculated with 5 mL of broth culture. Flasks were incubated at 30ºC for three days and the wheat bran was washed off to take out the leaf sheath. The treated leaf sheath was re-fermented for another three days in fresh solid-state medium. Wheat bran was washed off and the fiber bundles were separated by hand stripping.

Fiber quality

Tensile strength of the fiber bundles was checked using Hounsfield test equipment (Model 5K-S). Diameter of the bundles was recorded with an optical microscope. Surface characteristics of the fiber bundles were analyzed with the help of scanning electron micrographs.

RESULTS

Optimization of culture parameters

Different culture parameters were optimized for the enhancement of polygalacturonase production by S. lydicus. Substrate selection was carried out earlier where wheat bran was found to be the best one (6). The optimum particle size of wheat bran for polygalacturonase production was in the range of 500-1000 µm. A decline in enzyme production was observed above and below the optimum particle size (Fig. 1). The initial moisture content is one of the most critical parameters for the successful operation of solid-state fermentation (SSF) (3). In the present investigation, 70% moisture was found to be the best for polygalacturonase production (Fig. 2). Moisture content of 80 to 90% is detrimental for the survival of actinomycetes. As evident from Figure 3, the highest enzyme activity was recorded when the pH of the moistening solution was 6.0, as compared to the control (pH 7.0). Although the optimum pH was found to be 6.0, considerable production was detected in all sets of experiments. To find out the most favourable inoculum density, inoculum size was varied from 6.25 x 104 to 3.75 x 105 CFU and the control with 1.25 x 105 CFU was the best (Fig. 4). Fig. 5 demonstrates the effect of incubation temperature on polygalacturonase production by S. lydicus and the optimum temperature was 30ºC.






Optimization of nutritional parameters

Among the various carbon additives, pectin was identified as the most favoured supplement (Fig. 6). Similar result has been reported in the case of Aspergillus japonicus where the maximum pectinolytic activity was observed in the presence of pectin (19). As illustrated in Fig. 7, none of the nitrogen supplements could augment enzyme yield.



Evaluation of fermentation time

Evaluation of fermentation time was conducted at 12 h interval, adopting the optimized conditions (Fig. 8) and the maximum enzyme activity was recorded at 72 h (425 U/g). Biomass in terms of N-acetyl glucosamine concentration showed a steep increase from 12 to 72 h and thereafter a steady state was maintained.


Banana fiber degumming

A two-step fermentative process was employed to extract the fiber bundles from fresh pseudostem of banana. The time required for the novel solid-state fermentative process was only six days. Scanning electron micrographs of the bundle was taken after biological extraction. Removal of the non-cellulosic gummy wastes was extremely good as compared to the control (fiber bundle obtained from fresh leaf sheath by hand stripping was considered as the control) (Fig. 9). Tensile strength of the biologically extracted fiber bundle was as good as the control (Table 1). Fiber bundles with the same diameter were selected for mechanical testing to avoid any false information.


DISCUSSION

Effect of culture parameters on enzyme production

SSF is an attractive tool for the production of enzymes because of its higher productivity, lower capital and operating costs, lower space requirements, simpler equipment and easier downstream processing compared to that of submerged fermentation (SmF) (14). The major factors that affect microbial synthesis of enzymes in a SSF system include selection of a suitable substrate, water content of the substrate, size of inoculum, temperature etc (12). Particle size of the substrate was found to be one among the crucial factors affecting enzyme production. The results of the present study indicating an optimum particle size of 500-1000 µm for polygalacturonase production can be correlated to the fact that the larger particle size decreases the enzyme production due to the reduction in total surface area while the smaller particle size reduces enzyme yield due to the diminution in the porosity of the medium. Initial moisture level of the medium also acts as a controlling factor for enzyme production. Low moisture level leads to reduced solubility of the nutrients of the solid substrate, lower degree of swelling and higher water tension (21) and hence, affects growth and metabolism of the organism (9). Moisture level above optimum causes decrease in the porosity, alteration in the wheat bran particle structure, gummy texture, low oxygen transfer etc (15). An extrinsic parameter, such as pH, acts synergistically with other physical parameters in addition to being a regulatory parameter in biotechnological processes (10). However, in a solid-substrate medium, the pH of the mineral salt solution does not possess a profound impact on enzyme production as the substrate itself has a pH of its own. The amount of inoculum added to the fermentation medium has significant effect on growth and enzyme production. Lower inoculum density than the optimum may not be sufficient to initiate growth and to produce the required biomass, whereas higher inoculum can cause fierce competition for nutrients (9). Incubation temperature is a key factor affecting growth and metabolism of microbes as the activity of metabolic enzymes is directly influenced by temperature of the microenvironment. S. lydicus is mesophilic in nature with a growth temperature range of 15-42ºC (7). When a mesophilic culture is concerned, very low temperature may not trigger the metabolism of the organism while very high temperature results in the denaturation of metabolic enzymes.

Effect of nutrient supplementation on enzyme production

Solid substrate not only serves as anchorage for the cells but also supplies the nutrients to the microbial cultures growing in it (13). However, some of the nutrients in the solid substrate may be available in sub optimal concentrations, or even not present in the substrate. In such cases, it would be necessary to supplement them externally (8) to enhance growth and subsequently enzyme production. In the present study, all the carbon additives except pectin and galacturonic acid could function only as nutrient supplements where as pectin and galacturonic acid acted both as nutrients as well as inducers. Both of them have been reported as inducers for polygalacturonase production (18). Normally galacturonic acid should have an inhibitory effect on enzyme production, as it is the end product of hydrolysis of pectin. But, unlike SmF, SSF system is much more resistant to catabolic repression (20). The results of nitrogen supplementation indicated that wheat bran, with 16% protein (5) in its composition, could supply the required nitrogen for the growth of the organism.

Evaluation of fermentation time

Enzyme yield has been increased considerably (3.9 fold) as compared to the initial medium (6). However, the hour of maximum enzyme production remained the same and biomass estimation led to the conclusion that the enzyme production by S. lydicus was growth associated.

Banana fiber degumming

An ecofriendly process for the simultaneous extraction and degumming of banana fibers was developed under solid state cultivation utilizing the ability of S. lydicus to produce polygalacturonase. Fiber quality is related to the length of the fiber as well as its properties (2). Length of the fiber bundle is an important factor for textile and yarn industries. In the current methodology, the required length can be achieved by varying the length of the leaf sheath pieces subjected for fermentation. The chemical composition of both biologically and mechanically extracted fibers exhibits a similar pattern (2). Hemicelluloses and pectins are the major type of gummy materials present on the outer walls of banana fiber bundles and hence the biological action does not modify the chemical composition of inner elementary fibers constitutive of the bundles, which are mainly composed of cellulose, lignin and some amount of hemicellulose (2). Biological natural retting, with an exposure time from 10 to 30 days, has been reported to obtain banana fiber bundles of different length. The tensile strength of the fiber bundles has been decreasing upon increasing biological extraction time (2) indicating the necessity of decreasing the duration of the process. The processing time required for the present method was only six days solving the above problem to a great extent. Enzyme treatment of banana leaf sheath is a good strategy compared to simultaneous fermentation as it may further reduce the duration of the treatment. The treatment of hand stripped banana fiber bundles has already been attempted with polygalacturonase obtained from S. lydicus (7). But the yield is more in biological extraction than the other strategy with hand stripping and processing (2) and so the present study was focused on biological extraction of banana fiber bundles. The present method is advantageous as compared to chemical extraction procedures as environmental pollution can be avoided. The newly developed ecofriendly methodology, which can be operated with less infrastructure and space within a short period of time, is expected to be a promising one in the field of plant fiber extraction and processing.

ACKNOWLEDGMENTS

The authors are grateful to CSIR, India for the fellowship awarded to NJ.

Submitted: April 4, 2007; Returned to authors for corrections: July 22, 2007; Approved: January 24, 2008.

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  • *
    Corresponding Author. Mailing address: Biotechnology Division, National Institute for Interdisciplinary Science and Technology (CSIR), Trivandrum, 695019, India. Phone: ++91 471 25 15 325; Fax: ++91 471 24 91 712. E-mail:
  • Publication Dates

    • Publication in this collection
      11 Apr 2008
    • Date of issue
      Mar 2008

    History

    • Accepted
      24 Jan 2008
    • Received
      04 Apr 2007
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