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Regulation and genetic enhancement of beta-amylase production in Clostridium thermosulfurogenes.

机译:热硫梭菌中β-淀粉酶生产的调控和遗传增强。

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摘要

We studied the general mechanism for regulation of beta-amylase synthesis in Clostridium thermosulfurogenes. beta-Amylase was expressed at high levels only when the organism was grown on maltose or other carbohydrates containing maltose units. Three kinds of mutants altered in beta-amylase production were isolated by using nitrosoguanidine treatment, enrichment on 2-deoxyglucose, and selection of colonies with large clear zones on iodine-stained starch-glucose agar plates. beta-Amylase was produced only when maltose was added to cells growing on sucrose in wild-type and catabolite repression-resistant mutant strains, but the differential rate of enzyme synthesis in constitutive mutants was constant regardless of the presence of maltose. In carbon-limited chemostats of wild-type and catabolite repression-resistant mutant stains, beta-amylase was expressed on maltose but not on glucose or sucrose. beta-Amylase synthesis was immediately repressed by the addition of glucose. Therefore, we concluded that beta-amylase synthesis in C. thermosulfurogenes was inducible and subject to catabolite repression. The addition of cAMP did not eliminate the repressive effect of glucose. The mutants were generally characterized in terms of beta-amylase production, growth properties, fermentation product formation, and alterations in glucose isomerase and glucoamylase activities. A hyperproductive mutant produced eightfold more beta-amylase on starch medium than the wild type and more rapidly fermented starch to ethanol.
机译:我们研究了热硫梭菌中调节β-淀粉酶合成的一般机制。仅当生物体在麦芽糖或其他含有麦芽糖单元的碳水化合物上生长时,β-淀粉酶才能高水平表达。通过使用亚硝基胍处理,在2-脱氧葡萄糖上富集并选择碘染色的淀粉-葡萄糖琼脂平板上具有大透明区的菌落,来分离出三种改变了β-淀粉酶产量的突变体。仅在将麦芽糖添加到野生型和抗分解代谢物抗性突变体菌株中的蔗糖上生长的细胞中时,才产生β-淀粉酶,但无论是否存在麦芽糖,组成型突变体中酶合成的差异速率都是恒定的。在野生型和抗分解代谢物的碳限制的化学稳定剂突变体染色中,β-淀粉酶在麦芽糖上表达,但在葡萄糖或蔗糖上不表达。加入葡萄糖后,β-淀粉酶的合成立即受到抑制。因此,我们得出的结论是,在热硫脲梭菌中β-淀粉酶的合成是可诱导的,并受到分解代谢物的抑制。添加cAMP并不能消除葡萄糖的抑制作用。通常根据β-淀粉酶的产生,生长特性,发酵产物的形成以及葡萄糖异构酶和葡糖淀粉酶活性的改变来表征突变体。一个高产的突变体在淀粉培养基上产生的β-淀粉酶比野生型多八倍,并且将淀粉发酵更快地转化为乙醇。

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