| 摘要: |
| 以炭黑曲霉(Aspergillus carbonarius)AS3.396的高产果胶酶突变株G 5512为生产菌,在500 L发酵罐中进行深层液体发酵中试。结果表明,在发酵过程中分别进行补料和调节pH,能大幅度提高酶活性;同时进行补料和调节pH,以高酯果胶为底物时发酵液最高酶活性可达1 248.17 U/mL,以低酯果胶为底物时达2 235.75 U/mL,分别较出发菌株提高了约2倍和11倍。通过试验,还确定了从发酵液中分离提取果胶酶的最佳工艺流程:发酵酶液→超滤→酒精沉淀→真空干燥,其酶活性回收率在以高酯果胶为底物时达到89.3%,以低酯果胶为底物时为80.3%。 |
| 关键词: 果胶酶 突变菌株G5512 深层液体发酵 提取工艺 |
| DOI: |
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| 基金项目:甘肃省科技攻关项目(GZ914-2-19) |
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| Pilot tests of deep fermentation for the pectinase mutant strain G5512 and extracting technology |
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| Abstract: |
| A mutant strain G5512 with high yield of pectinase,which is suitable for the fermentation,was obtained from Aspergillus carbonarius AS 3.396 by chemical mutation using N-methy 1-N′-nitro-N-nitro-soguanidine(MNNG)and treatment with Co60 radiation.Pilot tests of deep fermentation have been carried out in a 500 liter tank by using the mutant strain G5512.The results showed that the enzyme activity of fermentation was 1 248.17 U/mL for high ester pectin and 2 235.75 U/mL for low ester pectin.The activity was three times in high ester pectin than the original strain's,and it was twelve times in low seter pectin.The optimal technological flow was obtained from collecting a pectinase of the fermentation liquor. |
| Key words: pectinase mutant strain G5512 deep fermentation extracting technology |
