通过深层发酵生产姬松茸的菌丝体和多糖。

Mycelium and polysaccharide production of Agaricus blazei Murrill by submerged fermentation.

作者信息

Lin Jr-Hui, Yang Shang-Shyng

机构信息

Graduate Institute of Microbiology and Biochemistry, National Taiwan University, Taipei, Taiwan.

出版信息

J Microbiol Immunol Infect. 2006 Apr;39(2):98-108.

PMID:16604241

Abstract

BACKGROUND AND PURPOSE

Over the last decade, Agaricus blazei Murrill has been studied and developed as a novel functional food in Japan, Korea, China, and Taiwan. Due to the low yields, the fruiting bodies of A. blazei Murrill are relatively expensive, and a cheap and stable source of A. blazei Murrill mycelium for commercial purposes is highly desirable. Culture media and conditions were investigated with a view to reducing the cost and improving the mycelium and polysaccharide production of A. blazei Murrill by submerged fermentation.

METHODS

Thirty six isolates of A. blazei Murrill were isolated from 22 fruiting bodies produced in Taiwan, and 16 of them could be successfully cultivated on mannitol-egg yolk-polymyxin medium. The isolates were identified by species-specific polymerase chain reaction (PCR) and optimized for the culture media and conditions by submerged fermentation for mycelium and polysaccharide production. Some properties of polysaccharide extract were also investigated.

RESULTS

All of the PCR products with species-specific primers showed high identity and matched the internal transcribed spacer 1 sequences of A. blazei Murrill. The phylogenic tree of A. blazei Murrill isolates generated from random amplified polymorphic DNAs arranged all samples into 3 groups and 2 independent cases. The optimal culture media of mycelium production in submerged fermentation were 5% malt extract, 0.1% yeast extract, and 0.5% peptone at pH 6.0, while the optimal culture conditions were 200 mL medium in 500 mL Hinton flask, shaking at 90 rpm for 3 days and then shifting to 105 rpm for 5 days at 27 degrees C. Each liter of A. blazei Murrill M72 yielded 10.83 +/- 0.24 g dried mycelia weight and each liter of A. blazei Murrill M152 produced 0.251 +/- 0.004 g crude polysaccharide (3.03 +/- 0.05% of dried mycelia weight). Crude polysaccharide of A. blazei Murrill M162 contained 82.27-99.14% of total sugar and less than 1.63% of protein; it had 4 major molecular weight components (274.1, 32.7, 7.5, and 2.1 kDa, respectively), with the 2.1 kDa portion possibly a beta-(1,3)-glucan.

CONCLUSIONS

These results show that selection of media and conditions can be employed in order to improve the mycelium and polysaccharide production of A. blazei Murrill M72 or M152 by submerged fermentation. Mycelia and polysaccharide production of A. blazei Murrill with submerged fermentation is potentially feasible.

摘要

背景与目的

在过去十年间，姬松茸在日本、韩国、中国大陆及台湾地区作为一种新型功能食品得到研究与开发。由于姬松茸子实体产量较低，其价格相对昂贵，因此非常需要一种廉价且稳定的商业化姬松茸菌丝体来源。为降低成本并通过深层发酵提高姬松茸菌丝体及多糖产量，对培养基和培养条件进行了研究。

方法

从台湾产的22个姬松茸子实体中分离出36个菌株，其中16个能在甘露醇 - 蛋黄 - 多粘菌素培养基上成功培养。通过种特异性聚合酶链反应（PCR）对这些菌株进行鉴定，并通过深层发酵优化培养基和培养条件以生产菌丝体和多糖。还研究了多糖提取物的一些性质。

结果

所有用种特异性引物扩增的PCR产物均显示出高度同源性，与姬松茸的内转录间隔区1序列匹配。由随机扩增多态性DNA构建的姬松茸菌株系统发育树将所有样本分为3组和2个独立案例。深层发酵生产菌丝体的最佳培养基为5%麦芽提取物、0.1%酵母提取物和0.5%蛋白胨，pH值为6.0，最佳培养条件为在500 mL Hinton烧瓶中加入200 mL培养基，于27℃下以90 rpm振荡培养3天，然后转至105 rpm振荡培养5天。每升姬松茸M72产生10.83±0.24 g干菌丝体重量，每升姬松茸M152产生0.251±0.004 g粗多糖（占干菌丝体重量的3.03±0.05%）。姬松茸M162的粗多糖含总糖82.27 - 99.14%，蛋白质含量低于1.63%；它有4种主要分子量组分（分别为274.1、32.7、7.5和2.1 kDa），其中2.1 kDa部分可能是β-(1,3)-葡聚糖。