原创力文档不动杆菌bd189对赭曲霉毒素a的脱毒分析-analysis on detoxification of ochratoxin a by acinetobacter bd 189.docxVIP
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不动杆菌bd189对赭曲霉毒素a的脱毒分析-analysis on detoxification of ochratoxin a by acinetobacter bd 189
IV
IV
provide biological proof of the detoxifying capability of Strain BD189. After 24 h of incubation with OTA, the viable bacteria of Strain BD189 exhibited strong detoxifying capability (removed more than 80% of OTA) while the heat-inactivated bacteria could not remove OTA. In addition, HPLC detected the presence of the degradation product Ochratoxin α (OTα) after the viable bacteria incubated with OTA. This indicated that the detoxification mechanism of OTA by Acinetobacter sp. BD189 was a biodegradation process rather than a cell-wall adsorption. The results of micronucleus assay showed that the pretreatment of Strain BD189 with OTA could cause a substantial decrease of micronucleus formation induced by OTA in HepG2 cells. This indicated that Strain BD189 could degrade OTA and really decreased the biological toxicity of OTA.
The third part was to investigate the detoxifying characteristics of Acinetobacter sp. BD189 and the properties of its OTA-degrading enzyme. The time curve of OTA degradation by Strain BD189 was accordant with the characteristics of enzymatic reaction. OTA degradation rate reached highest
between 30 and 40℃ while it was much lower at 10、20and 50 ℃. When the
effect of pH was examined, maximum degradation was observed at pH 6.5 and pH 7.5 while it was much lower at acidic and alkaline conditions. Moreover, the higher the concentration of bacteria was, the more OTA was
PAGE
PAGE VI
degraded. The results showed that the OTA-degrading enzyme of Strain BD189 was an endoenzyme, and its optimum temperature and pH for
degrading activity were 30℃ and pH8.0, respectively. The metal-ion chelator
EDTA could inhibit the degrading activity of the enzyme while the Carboxypeptidase Inhibitor could not. This suggested that the enzyme was a metalloenzyme and had different properties compared to carboxypeptidase A, which was another enzyme that could degrade OTA to OTα.
Conclusively, Acinetobacter sp. BD189 had significantly detoxifying capability
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