Growth-phase-dependent expression of the lipolytic system of Acinetobacter calcoaceticus BD413: cloning of a gene encoding one of the esterases.

R G Kok, V M Christoffels, B Vosman, K J Hellingwerf
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引用次数: 93

Abstract

Acinetobacter calcoaceticus BD413, when grown in batch culture in nutrient broth, produces both extracellular lipase activity and cell-bound esterase activity during and after the transition between exponential growth and the stationary phase. From a library of A. calcoaceticus DNA in Escherichia coli, plasmids were isolated that enabled E. coli to grow on media with tributyrin as the sole carbon source. Assays with model substrates classified the product of the cloned gene as an esterase. Via deletion analysis, the esterase gene was mapped on a 1.8 kbp chromosomal DNA fragment. This fragment was sequenced and found to contain one open reading frame, termed estA, which encodes a protein of 40.0 kDa. The amino acid sequence of this protein shows homology to a number of lipolytic enzymes, most notably to esterases. Deletion of estA only partially abolished cell-bound esterase activity in A. calcoaceticus, indicating that BD413 forms at least two esterases. Both esterases show the same temporal regulation of expression. beta-Galactosidase activity was measured in strains in which a promoterless lacZ gene was inserted into estA. Induction of lacZ expression in these strains also occurred at the end of exponential growth in batch cultures, indicating that production of the esterase is regulated at the genetic level.

钙酸不动杆菌BD413脂溶系统生长相依赖性表达:一个酯酶编码基因的克隆。
钙酸不动杆菌BD413在营养液中分批培养时,在指数生长期和固定生长期过渡期间和之后,产生细胞外脂肪酶活性和细胞结合酯酶活性。从大肠杆菌的钙酸杆菌DNA文库中分离出质粒,使大肠杆菌能够在以三丁酸甘油酯为唯一碳源的培养基上生长。用模型底物测定克隆基因的产物为酯酶。通过缺失分析,酯酶基因被定位在1.8 kbp的染色体DNA片段上。对该片段进行测序,发现它包含一个开放阅读框,称为estA,它编码一个40.0 kDa的蛋白质。该蛋白的氨基酸序列与许多脂溶酶,尤其是酯酶具有同源性。在A. calcoaceticus中,estA的缺失仅部分地消除了细胞结合酯酶的活性,这表明BD413至少形成了两种酯酶。两种酯酶表现出相同的时间表达调控。在无启动子lacZ基因插入estA的菌株中测量β -半乳糖苷酶活性。在这些菌株中,lacZ表达的诱导也发生在批量培养的指数生长结束时,表明酯酶的产生在遗传水平上受到调节。
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