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Shiitake (lentinula edodes) production on a sterilized bagasse substrate enriched with rice bran and sugarcane molasses

Produção de shiitake (Lentinula edodes) em substrato esterilizado, elaborado à base de bagaço de cana-de-açúcar, suplementado com farelo de arroz e melaço de cana-de-açúcar

Abstracts

This investigation was performed to evaluate the biological efficiency (BE), mean mushroom weight (MMW), mean number of mushroom (MNM) and mushroom quality of Shiitake [ Lentinula edodes (Berk.) Pegler] when grown on a sterilized substrate composed by sugarcane bagasse enriched with rice bran and sugarcane molasses. The proportions of rice bran were 0, 15, 20, 25 and 30% (dry weight/dry weight of bagasse); and the concentrations of sugarcane molasses were 0, 30 and 60 g/kg (dry weight/dry weight of bagasse plus rice bran). Four flushes were obtained during the production cycle, providing 3 accumulated productions which were used for production analysis. The substrate supplemented with 25 and 30% rice bran yielded the highest BE (98.42 and 99.84%, respectively, about 230 days after spawning) and MNM and initially produced a lower MMW than the substrates supplemented with 15 and 20% rice bran. Any amount of rice bran added to the sugarcane bagasse improved mushroom quality, with the best production of marketable mushrooms obtained by the addition of 15% rice bran. The largest amount of sugarcane molasses (60 g/kg) increased BE (90.3 and 23.6%, on first and second accumulated productions, respectively) and MNM and no quantity affected mushroom quality.

Lentinula edodes; shiitake; sugarcane bagasse


Este trabalho foi conduzido com o objetivo de avaliar a eficiência biológica (EB), o peso e número médio (PMC e NMC) e a qualidade dos cogumelos de Shiitake [ Lentinula edodes (Berk.) Peger] cultivado em substrato esterilizado, elaborado à base de bagaço de cana-de-açúcar, enriquecido com farelo de arroz e melaço de cana-de-açúcar. As proporções de farelo de arroz usadas foram 0, 15, 20, 25 e 30% (peso seco/peso seco de bagaço) e as concentrações de melaço de cana-de-açúcar utilizadas foram 0, 30 e 60 g/kg(peso seco/peso seco de bagaço mais farelo de arroz). Obteve-se quatro colheitas, constituindo três produções acumuladas que foram usadas para as análises de produção. Os substratos contendo 25 e 30% de farelo de arroz produziram os maiores valores de EB (98,42 e 99,4%, respectivamente, cerca de 230 dias após a inoculação) e PMC, e inicialmente, produziram um NMC menor que os substratos contendo 15 e 20% de farelo de arroz. Qualquer quantidade de farelo de arroz adicionado ao bagaço de cana-de-açúcar melhorou a qualidade dos cogumelos e a melhor produção de cogumelos comercializáveis foi obtida com a adição de 15% de farelo de arroz. A maior quantidade de melaço de cana-de-açúcar (60 g/kg) aumentou a EB (90,3 e 23,6%, na primeira e segunda produções acumuladas, respectivamente) e PMC, e nenhuma quantidade adicionada influenciou a qualidade dos cogumelos.

Lentinula edodes; Shiitake; bagaço de cana-de-açúcar


Shiitake (lentinula edodes) production on a sterilized bagasse substrate enriched with rice bran and sugarcane molasses

Produção de shiitake (Lentinula edodes) em substrato esterilizado, elaborado à base de bagaço de cana-de-açúcar, suplementado com farelo de arroz e melaço de cana-de-açúcar

Ivan Henrique RossiI; Antonio Carlos MonteiroI* * Corresponding author. Mailing Address: Laboratório de Microbiologia, Departamento de Produção Vegetal. Faculdade de Ciências Agrárias e Veterinárias, UNESP. Via de Acesso Prof. Paulo Donato Castellane, s/n, 14884-900, Jaboticabal, SP, Brasil. Telephone: (+5516) 3209-2652/3209-2653. Fax: (+5516) 3203-4275. E-mail: montecar@fcav.unesp.br ; José Octavio MachadoI;João Luciano AndrioliI; José Carlos BarbosaII

ILaboratório de Microbiologia, Departamento de Produção Vegetal

IIDepartamento de Ciências Exatas, Faculdade de Ciências Agrárias e Veterinárias, Universidade Estadual Paulista, Jaboticabal, São Paulo, SP, Brasil

ABSTRACT

This investigation was performed to evaluate the biological efficiency (BE), mean mushroom weight (MMW), mean number of mushroom (MNM) and mushroom quality of Shiitake [ Lentinula edodes (Berk.) Pegler] when grown on a sterilized substrate composed by sugarcane bagasse enriched with rice bran and sugarcane molasses. The proportions of rice bran were 0, 15, 20, 25 and 30% (dry weight/dry weight of bagasse); and the concentrations of sugarcane molasses were 0, 30 and 60 g/kg (dry weight/dry weight of bagasse plus rice bran). Four flushes were obtained during the production cycle, providing 3 accumulated productions which were used for production analysis. The substrate supplemented with 25 and 30% rice bran yielded the highest BE (98.42 and 99.84%, respectively, about 230 days after spawning) and MNM and initially produced a lower MMW than the substrates supplemented with 15 and 20% rice bran. Any amount of rice bran added to the sugarcane bagasse improved mushroom quality, with the best production of marketable mushrooms obtained by the addition of 15% rice bran. The largest amount of sugarcane molasses (60 g/kg) increased BE (90.3 and 23.6%, on first and second accumulated productions, respectively) and MNM and no quantity affected mushroom quality.

Key words:Lentinula edodes, shiitake, sugarcane bagasse

RESUMO

Este trabalho foi conduzido com o objetivo de avaliar a eficiência biológica (EB), o peso e número médio (PMC e NMC) e a qualidade dos cogumelos de Shiitake [ Lentinula edodes (Berk.) Peger] cultivado em substrato esterilizado, elaborado à base de bagaço de cana-de-açúcar, enriquecido com farelo de arroz e melaço de cana-de-açúcar. As proporções de farelo de arroz usadas foram 0, 15, 20, 25 e 30% (peso seco/peso seco de bagaço) e as concentrações de melaço de cana-de-açúcar utilizadas foram 0, 30 e 60 g/kg(peso seco/peso seco de bagaço mais farelo de arroz). Obteve-se quatro colheitas, constituindo três produções acumuladas que foram usadas para as análises de produção. Os substratos contendo 25 e 30% de farelo de arroz produziram os maiores valores de EB (98,42 e 99,4%, respectivamente, cerca de 230 dias após a inoculação) e PMC, e inicialmente, produziram um NMC menor que os substratos contendo 15 e 20% de farelo de arroz. Qualquer quantidade de farelo de arroz adicionado ao bagaço de cana-de-açúcar melhorou a qualidade dos cogumelos e a melhor produção de cogumelos comercializáveis foi obtida com a adição de 15% de farelo de arroz. A maior quantidade de melaço de cana-de-açúcar (60 g/kg) aumentou a EB (90,3 e 23,6%, na primeira e segunda produções acumuladas, respectivamente) e PMC, e nenhuma quantidade adicionada influenciou a qualidade dos cogumelos.

Palavras-chave:Lentinula edodes, Shiitake, bagaço de cana-de-açúcar

INTRODUCTION

Over the last few years, the commercial cultivation of Shiitake, Lentinula edodes, on artificial substrates based on enriched sawdust has increased (5,15). The productivity of this system depends, among other factors, on the quality of the sawdust used as substrate (23). Sawdust is difficult to standardize because it is generally obtained from residues of different types of wood. Thus, the availability of low-cost and homogeneous substrates for production is an important factor for successful cultivation (26). Since edible mushrooms are adapted to grow on a variety of ligno-cellulosic wastes (2), it is possible to use a wide variety of unconventional materials to cultivate L. edodes.

According to Santos (22), bagasse is the residue of sugarcane submitted to several types of treatments and washes performed during sugar extraction. Sugarcane bagasse, besides being a highly available waste product in sugar and alcohol-producing areas, is rich in lignin, cellulose and hemicellulose (3). Moreover, bagasse is a homogeneous raw material in terms of chemical composition and physical and bromatologic characteristics (16), important factors for the cultivation of L. edodes. In addition, when pressed, sugarcane bagasse is porous enough to support the mycelial growth of L. edodes and also to facilitate the gas exchanges of the substrate. Nevertheless, basidiocarp production can be reduced in this material due to the shortage of nutrients, as observed by Maziero (14) and Soto-Velazco et al. (24) for Pleurotus sp culture. Thus, supplementation with nutrients is desirable. Sugarcane molasses is a subproduct rich in sugars, abundantly found in areas of high bagasse availability. Sugars can increase mushroom yield (20,25), because it is a source of energy for the metabolic activity of the mushrooms, supplying carbon, which represents almost 50% of the dry matter weight of fruiting bodies (27). Rice bran, a readily available residue in areas of rice processing, is traditionally employed to enrich the sawdust used, in the orient, for production of L. edodes mushrooms (10,12,13) and can be used to supplement sugarcane bagasse, as suggested by Oei (17) and by Eira and Minhomi (7), and as used by Iizuka (11) for the production of L. edodes mycelial extracts. The objective of the present study was to evaluate the production and quality of L. edodes mushrooms in axenic culture grown on sugarcane bagasse supplemented with different amounts of rice bran and sugarcane molasses.

MATERIALS AND METHODS

A culture of the JAB-K1 isolate grown on minimum medium (18) from basidiocarp of L. edodes (Berk.) Pegler, obtained from growers of the northeast region of São Paulo State, Brazil, was used as an inoculum for the production of the initial spawn obtained by cultivation of the fungus on a sugarcane bagasse substrate supplemented with 20% rice bran and 30 g of sugarcane molasses per kg of substrate. This initial spawn was then propagated in a substrate with the same composition to produce the spawn used in the experiment.

The sugarcane bagasse was supplemented with non-defatted rice bran, sugarcane molasses and mixtures of the two supplements, representing the variables of the experiment. The amount of water needed to correct the moisture content of the substrate to 60% (21) was calculated considering the amount of natural humidity of each component. Rice bran was mixed with bagasse before the increase in moisture content and the molasses was diluted in the water used to correct moisture. The substrate, pressed manually into a cylindrical block, was packed in two high density polyethylene bags resistant to autoclaving (13). Each experimental replicate consisted of a cylindrical block of substrate weighing 1.2 kg and measuring 15.0 cm in diameter and 15.0 to 20.0 cm in height, with a central cylindrical hole 3.0 cm in diameter running throughout the block to provide space for inoculation with approximately 4.7% of spawn (1).

The blocks were sterilized for 120 minutes at 121oC immediately after preparation and stored until the time for inoculation. The experimental treatments consisted of a 5 x 3 factorial scheme with 5 proportions of rice bran (0, 15, 20, 25 and 30%, dry weight/dry weight of bagasse) and 3 concentrations of sugarcane molasses (0, 30 and 60 g/kg, dry weight/dry weight of bagasse plus rice bran). The experiment was arranged as a completely randomized design with different numbers of replicates (a minimum of 5 and a maximum of 10 blocks per treatment), because any substrate presenting the slightest suspicion of contamination was immediately eliminated.

After spawning, the substrates were incubated at 25-28ºC in the dark in the presence of 70% humidity (1,26) until they were ready for fruiting, as indicated by complete colonization of the substrate and mycelial thickening (6,17). After 60 days (11,13), the bags were removed to expose the surface of the blocks to fluorescent light (12 h/d) for 15 days. After bag removal, a hard and thick brown coat formed on the surface of the block. During this phase, environmental humidity was raised to 90-95% in order to prevent water loss from the blocks. The blocks were then soaked in cold water (a minimum of 16 and a maximum of 26ºC) in a tank for 24 hours (19) and then placed in a fruiting room with a controlled temperature of 21 to 23ºC and relative humidity between 90 and 95%. The mushrooms were harvested over a period of 12 days starting 8 days after induction. Four flushes were obtained. Yield and quality were evaluated considering the accumulated productions of the flushes, i.e., the sum of the first two flushes represented the first accumulated production and so forth.

For the evaluation of productivity, the following parameters were used: biological efficiency (BE), calculated as the mushroom fresh weight/block dry weight ratio x 100 (21); mean number of mushrooms (MNM), corresponding to number of basidiocarps per block, and mean mushroom weight (MMW). The quality of the basidiocarps was evaluated on the basis of four size groups (larger than 7 cm, 5 to 7 cm, 3 to 5 cm, and smaller than 3 cm), and a "deformed" group. Marketable mushrooms are those measuring more than 3 cm in size, and mushrooms of highest commercial value are those measuring more than 5 cm in diameter.

After harvesting, the blocks were kept at 25 to 28ºC and 85 to 90% relative humidity during 30 days for the resting period and later fruiting induction (13). The procedure was repeated until full substrate consumption. The harvest period was of about 230 days.

RESULTS

In the first harvest, a small number of mushrooms was obtained in all treatments, a fact that prevented statistical analysis of the data. However, these results were included in the analysis of accumulated productions. In the second flush, only treatments with 0% rice bran did not produce sufficient numbers of mushrooms, however these data were also included in the analysis of accumulated production.

Substrate Productivity

Any amount of rice bran added to the sugarcane bagasse increased BE and MNM (Table 1). The largest rice bran proportions (25 and 30%) stimulated mushroom yields in the first flushes but in the subsequent stimulation was lower (15 and 20%), indicating, in this phase, the exhaustion of the substrate with largest amounts of rice bran.

The addition of 25 and 30% of rice bran led to lower MMW in the initial accumulated production (Table 1). In the subsequent accumulated productions no effect of rice bran on MMW was verified. Analysing BE, MNM and MMW jointly, the addition of 25 and 30% rice bran stimulated mushroom yield in the first two accumulated productions even though it had reduced the mean weight in the initial accumulated production (Table 1).

Any amount of molasses increased the biological efficiency and mean number of L. edodes mushrooms in the first accumulated production but in the second only an increase on BE by the addition of 60 g of molasses was observed (Table 1). The effect of the supplementation on MMW was only observed in the last accumulated production by the addition of 60 g of molasses to the substrate. MMW decreased in each accumulated production, demonstrating the exhaustion of the substrate.

Mushroom Quality

Supplementation of bagasse with 15% rice bran stimulated the production of mushrooms exceeding 7 cm in diameter, and 25 to 30% rice bran addition increased mushroom production in the 5 to 7 cm size group (Fig. 1A). Rice bran had no effect on the size group exceeding 7 cm or on the group of deformed mushrooms, but stimulated production in the size groups of 5 to 7 and 3 to 5 cm (Fig. 1B). The addition of 20 to 25% rice bran stimulated the production of mushrooms exceeding 7 cm in diameter (Fig. 1C).




In the no rice bran added treatment, the sum of the percentages of no commercial groups (deformed or less than 3 cm in diameter) reached to 40% of the harvested mushrooms, depending on the accumulated production considered. Any amount of added rice bran reduced this percentage greatly from 12 to 25%. Thus, the addition of 15% of rice bran to the sugarcane bagasse substrate stimulated the production of mushrooms of better quality.

The effect of the sugarcane molasses was observed on the 5 to 7 cm size and deformed groups in the initial accumulated production (Fig. 2A). The concentration of 60 g/kg yielded a larger number of mushrooms in the former group and a smaller number in the latter. Among the other accumulated productions (Figs. 2B and C ), only in the last it was observed effect of the 60 g/kg concentration on the group of mushrooms exceeding 7 cm in diameter. These results demonstrate that molasses, when used as a supplement in the substrate based on sugarcane bagasse, had no significant effect on the quality of L. edodes mushrooms.



DISCUSSION

The low productivity obtained in the first flush may be explained by the incubation period and the use of two plastic bags for the protection of the substrate during colonization by L. edodes. All the substrates were totally colonized by 60 days after inoculation and received the first soaking at 75 days. A time period of 60 to 90 days is necessary for incubation (11,13) but our results suggest that early fruiting was induced before maturation of the mycelium. The gas exchanges between the substrates and the environment might have been impaired by the use of two bags, so that the accumulation of CO2 during the growth of L. edodes might have increased the time needed for incubation. Several authors have pointed out the impairment of L. edodes development caused by inadequate gas exchange of the substrates (5,6). Kawai et al. (13) obtained good production with substrates placed in plastic bags with greater permeability for exchange, but Donoghue and Denison (5) observed no difference in productivity with substrates placed in plastic bags with different openings for gas exchange. On this basis, we expected the use of two plastic bags, necessary to maintain the aseptic conditions of the substrate, not to impair mushroom yield. Thus, further studies are needed to determine the time economically viable for inducing the initial production and the best methods for substrate packing for the growth and production of L. edodes on sugarcane bagasse.

The low production obtained on bagasse without rice bran clearly shows the need for supplementation in order to increase the production of L. edodes mushrooms. The higher productivity was obtained by the addition of 25 and 30% rice bran. Eira and Minhomi (7) reported that L. edodes can be cultivated axenically on bagasse supplemented with 20% rice bran and other nutrients. According to Fasidi and Kadiri (8), the increased productivity of Lentinus subnudus on a Andropogun tectorum straw substrate supplemented with 30% rice bran can be attributed to the carbohydrates, amino acids and mineral elements present in this supplement. These authors also believe that the lipids present in rice bran provide a higher mushroom yield, in agreement with Song et al. (23) who observed a gradual decrease in lipids in the substrate after the production of mushrooms. Several authors (1,4,10) have reported increase in BE quite similar to that obtained in the present study. The increase in BE obtained with increasing rice bran proportions was not linear, i.e., the increase in BE with each 5% increment in the amount of rice bran added was not proportional. The growth tendency was similar to that detected by Royse (21), who observed a 13.5% increase in BE over three flushes with each 6% amount of millet added to sawdust. In the present study, the mean increase obtained for three accumulated productions was approximately 12%.

The rice bran proportions that led to an increase in MNM and BE also caused a decrease in MMW. Similar effect was observed by Royse (21). According to Royse et al. (20) and Donoghue and Denison (6), larger and heavier mushrooms are obtained when lower BE is observed. In the present experiment, this relationship was observed only for the initial accumulated production, whereas in the second flush MMW did not differ when the four proportions of supplementation with rice bran were considered. Both MNM and BE were higher when the 25 and 30% supplements were used, suggesting that these amounts of bran stimulates the production of good quality mushrooms of good mean weight.

The addition of any amount of rice bran to sugarcane bagasse showed an improvement in mushroom quality, with the production of marketable mushrooms ranging from 75 to 88%. These results were superior to the 60 to 80% yields reported to occur by Hiromoto (9) when L. edodes is cultivated on supplemented sawdust.

The increment in productivity with addition of molasses suggests that this supplement also can be added to sugarcane bagasse for the cultivation of L. edodes. Tokimoto and Kawai (25) showed that the enlargement of the proportion of sucrose from 0.5 to 8.0% in potato-agar medium stimulated the production of L. edodes. Since 60 g/kg of substrate practically represent 5.0% sucrose, our results correspond to those obtained by these authors. Royse et al. (20) obtained a 22% increase in BE in the first flush by the addition of 0.6 to 1.2% sucrose. When they doubled the amount of sugar (2.4%) they did not observe a further increase in production. The stimulation of production observed by these authors occurred in the first induction, whereas in the present study it occurred in the second. Nevertheless, the data obtained in the two studies were similar after the second induction, since we obtained a 10% increase in BE when we added 30 g/kg molasses and a 20% increase when we added 60 g/kg molasses. This increase is explained by the fact that molasses is a source of energy and of carbon which, according to Zanetti and Ranal (27), are important for the metabolic activity of the mushrooms and represent the basis for the synthesis of various molecules that result in about 50% dry weight of fruiting bodies as carbon. We found no effect of molasses on the quality of mushrooms produced on sugarcane bagasse, similarly to observed by Royse et al. (20).

ACKNOWLEDGEMENTS

We thank FAPESP (Fundação de Amparo à Pesquisa do Estado de São Paulo, Brazil) for M. Sc. scholarship.

Submitted: January 20, 2002; Approved: December 16, 2002

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  • *
    Corresponding author. Mailing Address: Laboratório de Microbiologia, Departamento de Produção Vegetal. Faculdade de Ciências Agrárias e Veterinárias, UNESP. Via de Acesso Prof. Paulo Donato Castellane, s/n, 14884-900, Jaboticabal, SP, Brasil. Telephone: (+5516) 3209-2652/3209-2653. Fax: (+5516) 3203-4275. E-mail:
  • Publication Dates

    • Publication in this collection
      03 July 2003
    • Date of issue
      Apr 2003

    History

    • Accepted
      16 Dec 2002
    • Received
      20 Jan 2002
    Sociedade Brasileira de Microbiologia USP - ICB III - Dep. de Microbiologia, Sociedade Brasileira de Microbiologia, Av. Prof. Lineu Prestes, 2415, Cidade Universitária, 05508-900 São Paulo, SP - Brasil, Ramal USP 7979, Tel. / Fax: (55 11) 3813-9647 ou 3037-7095 - São Paulo - SP - Brazil
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