Kittelmann M, Klein T, Kragl U, Wandrey C, Ghisalba O
Ciba-Geigy Ltd, Pharmaceuticals Division, Basel, Switzerland.
Appl Microbiol Biotechnol. 1995 Dec;44(1-2):59-67. doi: 10.1007/BF00164481.
In an optimized sorbitol/yeast extract/mineral salt medium up to 12 U/l CMP-N-acetyl-neuraminic-acid (Neu5Ac) synthetase was produced by Escherichia coli K-235 in shake-flask culture. A colony mutant of this strain, E. coli K-235/CS1, was isolated with improved enzyme formation: in shake flasks with a yield of up to 20.8 U/l and 54 mU/mg protein in the cell extract. With this strain 26500 U CMP-Neu5Ac synthetase was produced with a high specific activity (0.128 U/mg) by fed-batch fermentation on 230-l scale. On a 10-1 scale the enzyme yield was 191 U/l culture medium. The enzyme was partially purified by precipitation with polyethyleneglycol resulting in a three- to fourfold enrichment and a recovery rate of more than 80%; most of the CTP hydrolysing enzymes were removed. The native synthetase was deactivated completely by incubation at 45 degrees C for 10 min, but could be stabilized remarkably by glycerol and different salts. The enzyme was used for the preparative synthesis of CMP-Neu5Ac with a conversion yield of 87% based on CTP.
在优化的山梨醇/酵母提取物/无机盐培养基中,大肠杆菌K - 235在摇瓶培养中可产生高达12 U/l的CMP - N - 乙酰神经氨酸(Neu5Ac)合成酶。该菌株的一个菌落突变体,即大肠杆菌K - 235/CS1,被分离出来,其酶形成能力有所提高:在摇瓶中产量高达20.8 U/l,细胞提取物中蛋白质的比活性为54 mU/mg。用该菌株通过230升规模的补料分批发酵生产出了26500 U的CMP - Neu5Ac合成酶,其比活性较高(0.128 U/mg)。在10升规模下,酶产量为191 U/l培养基。通过聚乙二醇沉淀对该酶进行了部分纯化,富集了三到四倍,回收率超过80%;大部分CTP水解酶被去除。天然合成酶在45℃孵育10分钟后完全失活,但甘油和不同的盐可使其显著稳定。该酶用于CMP - Neu5Ac的制备合成,基于CTP的转化率为87%。
