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大肠杆菌在两阶段恒化器中持续、高水平生产和分泌质粒编码蛋白。

Continuous, high level production and excretion of a plasmid-encoded protein by Escherichia coli in a two-stage chemostat.

作者信息

Fu J, Wilson D B, Shuler M L

机构信息

School of Chemical Engineering, Cornell University, Ithaca, NY 14853, USA.

出版信息

Biotechnol Bioeng. 1993 Apr 25;41(10):937-46. doi: 10.1002/bit.260411004.

Abstract

The stable continuous overproduction of a plasmidencoded protein, beta-lactamase, for at least 50 days by Escherichia coli K-12, RB791(pKN), with release into the culture medium has been demonstrated in two-stage chemostats. The second-stage culture was continuously induced with 0.1 mM IPTG. Continuous expression of beta-lactamase could not be sustained with this strain in a single-stage chemostat because of cell death and selection for lac(-1) cells. Beta-lactamase production in the second stage was sensitive to the second-stage dilution rate and the distribution of the limiting substrate (i.e., glucose) between the first and second stages. The fraction of viable, excreting cells and the average copy number in the induced culture was measurably higher under those conditions of dilution rate and substrate distribution which yielded high beta-lactamase levels. The best operating conditions found at 20 degrees C were a first-stage dilution rate of 0.12 h(-1), a second-stage dilution rate of 0.03 h(-1), and equal glucose feed supplied to each stage. Enzymatically active beta-lactamase was produced at a level of 25% of total cellular protein with 90% excretion yielding 300 mg beta-lactamase/L that was 50% pure at an OD(600) < 6.

摘要

已在两级恒化器中证明,大肠杆菌K-12、RB791(pKN)能稳定持续过量生产质粒编码的蛋白质β-内酰胺酶至少50天,并释放到培养基中。第二阶段培养物用0.1 mM异丙基-β-D-硫代半乳糖苷(IPTG)持续诱导。由于细胞死亡和对lac(-1)细胞的选择,该菌株在单级恒化器中无法维持β-内酰胺酶的持续表达。第二阶段β-内酰胺酶的产生对第二阶段的稀释率以及第一阶段和第二阶段之间限制性底物(即葡萄糖)的分配敏感。在产生高β-内酰胺酶水平的稀释率和底物分配条件下,诱导培养物中活的、分泌细胞的比例和平均拷贝数明显更高。在20℃下发现的最佳操作条件是第一阶段稀释率为0.12 h(-1),第二阶段稀释率为0.03 h(-1),且向每个阶段供应等量的葡萄糖进料。产生的具有酶活性的β-内酰胺酶水平为总细胞蛋白的25%,排泄率为90%,产生300 mgβ-内酰胺酶/L,在OD(600) < 6时纯度为50%。

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