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脱氧雪腐镰刀菌烯醇(呕吐毒素)的微生物转化

Microbial transformation of deoxynivalenol (vomitoxin).

作者信息

He P, Young L G, Forsberg C

机构信息

Department of Animal and Poultry Science, University of Guelph, Ontario, Canada.

出版信息

Appl Environ Microbiol. 1992 Dec;58(12):3857-63. doi: 10.1128/aem.58.12.3857-3863.1992.

Abstract

Microbial inocula from rumen fluid, soil, and contents of the large intestines of chickens (CLIC) and of swine (SLIC) were tested for their ability to transform deoxynivalenol (vomitoxin) in vitro. Microorganisms in (CLIC) completely transformed pure vomitoxin, and this activity was retained through six serial subcultures. No alteration of the toxin by incubation with SLIC was detected, whereas 35% of the vomitoxin was metabolized in the original culture of rumen fluid and 50% was metabolized by the soil sample, though metabolism was decreased in subsequent subcultures of either sample. A single metabolite was isolated and identified as deepoxy vomitoxin. The increase in concentration of deepoxy vomitoxin in the culture medium corresponded with the decrease in vomitoxin concentration. The vomitoxin transformation rate was not affected by either the ratio of CLIC to vomitoxin (5 to 0.2 g of CLIC per mg of vomitoxin) or the initial concentration of vomitoxin (14 to 1,400 ppm) in the medium. Biotransformation of vomitoxin was completely inhibited when the pH in the medium was lowered to 5.20. Sodium azide at a 0.1% (wt/vol) concentration in the medium blocked the transformation of vomitoxin, suggesting that the deepoxidation of vomitoxin is an energy-dependent process. About 50% of the vomitoxin in moldy corn in culture medium was transformed by microorganisms from CLIC. The vomitoxin transformation rate in moldy corn was not affected when the concentration of CLIC changed from 0.2 to 0.8 g/ml of medium. Vomitoxin in the moldy corn was not transformed when CLIC were added to corn without culture medium.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

对来自瘤胃液、土壤以及鸡(CLIC)和猪(SLIC)大肠内容物的微生物接种物进行了体外转化脱氧雪腐镰刀菌烯醇(呕吐毒素)能力的测试。CLIC中的微生物能完全转化纯呕吐毒素,且该活性在六次连续传代培养中得以保留。未检测到SLIC对毒素有改变作用,而瘤胃液原始培养物中35%的呕吐毒素被代谢,土壤样品代谢了50%的呕吐毒素,不过这两个样品后续传代培养时代谢作用均有所下降。分离出一种单一代谢物并鉴定为脱环氧呕吐毒素。培养基中脱环氧呕吐毒素浓度的增加与呕吐毒素浓度的降低相对应。呕吐毒素的转化率不受CLIC与呕吐毒素比例(每毫克呕吐毒素对应5至0.2克CLIC)或培养基中呕吐毒素初始浓度(14至1400 ppm)的影响。当培养基pH降至5.20时,呕吐毒素的生物转化被完全抑制。培养基中0.1%(重量/体积)浓度的叠氮化钠可阻断呕吐毒素的转化,这表明呕吐毒素的脱环氧化是一个能量依赖过程。培养基中发霉玉米里约50%的呕吐毒素被CLIC中的微生物转化。当CLIC浓度从0.2克/毫升培养基变为0.8克/毫升培养基时,发霉玉米中呕吐毒素的转化率不受影响。当向未添加培养基的玉米中添加CLIC时,发霉玉米中的呕吐毒素未被转化。(摘要截选至250词)

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