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作 者:陈颖[1] 杨丽维[1] 齐欣[1] 陈晓云[1] 李明春[2] 唐柳[1] 张峻[1]
机构地区:[1]天津市林业果树研究所,天津300112 [2]南开大学微生物学系,天津300071
出 处:《食品工业科技》2012年第17期154-158,共5页Science and Technology of Food Industry
基 金:天津市应用基础及前沿技术研究计划(10JCYBJC09600;10JCYBJC05000);国家自然科学基金(21076162)
摘 要:目的:通过对前期构建的海藻糖合酶基因工程菌进行高密度发酵的研究,获得了其高密度工艺条件。方法:采用摇瓶发酵和10L自控罐高密度发酵研究了培养基、pH、发酵方式对工程菌生长及目的蛋白表达的影响,并考察了工程菌中重组质粒的遗传稳定性。结果:海藻糖合酶基因工程菌高密度发酵的培养基为2YT+0.2%葡萄糖,最适pH为7.0,发酵方式为分批补料,通过10L自控罐高密度发酵最终得到的工程菌细胞密度达到了50.78g/L,酶活达到了3.197U/mL。所构建的重组质粒在宿主中得到了稳定遗传。结论:优化了海藻糖合酶基因工程菌高密度发酵的条件,为海藻糖规模化生产奠定了基础。Object :To obtain the high dense fermentation procedure of trehalose synthase(Tres)genetic engineering bacteria previously construct. Methods: Studied the influence of medium, pH, ferment mode for incubation and induction on the growth of recombinant genetic engineering bacterial and expression of target protein in a 10L auto control biostat fermentator, and explored the genetic stability of recombinant plasmid. Result: The highdensity culture medium of trehalose synthase genetic engineering bacteria was 2YT + 0.2% glucose,the optimum pH was 7.0,the ferment mode was fed-batch.After the recombinant genetic engineering bacterial strain cultured in 10L high-density fermentation,the density of bacteria reached 50.78g/L,the enzyme activity reached 3.197U/mL.The constructed recombinant plasmid was inherited steadily in host bacteria.Conclusion :The high-density fermentation condition of trehalose synthase genetic engineering bacteria was optimized. It laid a foundation of largescale production of trehalose.
分 类 号:TS201.2[轻工技术与工程—食品科学]
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