Worrall A F, Connolly B A
Department of Biochemistry, University of Southampton, United Kingdom.
J Biol Chem. 1990 Dec 15;265(35):21889-95.
A gene coding for bovine pancreatic DNase I has been constructed from synthetic oligonucleotides. This gene has been cloned into a plasmid vector pDOC55 designed to allow very tight control of expression of potentially lethal proteins. Induction of protein synthesis from the gene yielded a peptide of molecular weight of approximately 31,000, consistent with DNase I. The yield of this protein from the pDOC55 construct (pAW5) was approximately 150 micrograms/liter of cell culture. Attempts to clone the gene into a less tightly controlled expression vector based on the tac-promoter (pKK223-3) were unsuccessful, presumably due to the expected lethality of the product. Mutagenesis of the gene to replace the active site histidine (His-134) in the protein with glutamine yielded a gene readily clonable into both expression systems. Yields of the mutagenized protein were approximately 6 micrograms/liter from a pDOC55 system and 20 mg/liter from a pKK223-3 system. The activity of the proteins were assayed using the Kunitz procedure and their cleavage selectivities by digestion of the Escherichia coli tyr T promoter. The recombinant native enzyme had both the same specific activity and DNA cleavage selectivity as the protein isolated from bovine pancreas using these two assays. The H134Q mutant had a specific activity of about 0.001% of the native protein but had an unaltered DNA cleavage selectivity.
已通过合成寡核苷酸构建了编码牛胰脱氧核糖核酸酶I的基因。该基因已被克隆到质粒载体pDOC55中,该载体设计用于非常严格地控制潜在致死性蛋白质的表达。从该基因诱导蛋白质合成产生了一种分子量约为31,000的肽,与脱氧核糖核酸酶I一致。从pDOC55构建体(pAW5)中获得的这种蛋白质的产量约为150微克/升细胞培养物。尝试将该基因克隆到基于tac启动子的控制较松的表达载体(pKK223-3)中未成功,推测是由于产物预期的致死性。将该基因进行诱变,用谷氨酰胺取代蛋白质中的活性位点组氨酸(His-134),得到了一个易于克隆到两种表达系统中的基因。诱变蛋白的产量在pDOC55系统中约为6微克/升,在pKK223-3系统中约为20毫克/升。使用Kunitz方法测定蛋白质的活性,并通过消化大肠杆菌tyr T启动子来测定其切割选择性。使用这两种测定方法,重组天然酶与从牛胰腺中分离的蛋白质具有相同的比活性和DNA切割选择性。H134Q突变体的比活性约为天然蛋白质的0.001%,但DNA切割选择性未改变。
