Abstract
Beta-glucan,
 one of the major cell wall components of Saccharomyces cerevisiae (S. 
cerevisiae), has been found to enhance immune functions.
 At present 
study, we developed an optimal procedure to extract and purify 
beta-glucan. At first, yeast cells were grown in sabouraud dextrose agar
 and then cultured in yeast extract-peptone-glucose (YPG) broth. After 
incubation, cells were harvested, washed and disrupted by means of 
sonication method. The obtained cell walls were used to prepare 
alkali-soluble beta-glucan (glucan-S1). In this regard, 2% sodium 
hydroxide (NaOH) and 3% acetic acid were used in alkaline-acid 
extraction, respectively.
 This preparation contained 2.4% protein. In 
the next step, DEAE sephacel chromatography was used to remove remaining
 proteins (glucan-S2). Subsequently this preparation was applied into 
concanavalin-A sepharose column to remove manann. Finally, beta-glucan 
free of mannoprotein complexes was prepared (glucan-S3).
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