Stolt P, Stoker N G
Bacterial Molecular Genetics Unit, Department of Clinical Sciences, London School of Hygiene & Tropical Medicine, England.
J Bacteriol. 1996 Dec;178(23):6693-700. doi: 10.1128/jb.178.23.6693-6700.1996.
Plasmid pAL5000 from Mycobacterium fortuitum encodes two proteins necessary for replication: RepA (307 amino acid residues) and RepB (119 residues). A single RNA species encoding these proteins was characterized, and its 5' end was defined. The proteins were expressed as maltose-binding protein fusions in Escherichia coli. The RepB protein was shown in vitro to bind specifically to a previously defined 435-bp region of pAL5000 containing the origin of replication (ori). The precise RepB binding sites were defined by DNase I footprinting experiments. RepB binds to two motifs in the ori region: a high-affinity site within its own promoter region, implying autoregulation of its expression, and a low-affinity site further upstream, presumably the origin of replication itself. The binding to the latter motif seems to occur on one DNA strand only. The high-affinity binding site contains several palindromic sequences. Gel retardation assays were performed with the different binding sites as templates, and the binding constant to each site was estimated from protein titrations. This is the first molecular dissection of mycobacterial DNA-binding proteins and their interactions with their targets.
来自偶然分枝杆菌的质粒pAL5000编码复制所需的两种蛋白质:RepA(307个氨基酸残基)和RepB(119个残基)。对编码这些蛋白质的单一RNA种类进行了表征,并确定了其5'端。这些蛋白质在大肠杆菌中作为麦芽糖结合蛋白融合体表达。体外实验表明,RepB蛋白能特异性结合pAL5000中一个先前定义的包含复制起点(ori)的435 bp区域。通过DNase I足迹实验确定了RepB的精确结合位点。RepB与ori区域中的两个基序结合:一个在其自身启动子区域内的高亲和力位点,这意味着其表达存在自我调节,另一个在更上游的低亲和力位点,可能是复制起点本身。与后一个基序的结合似乎仅发生在一条DNA链上。高亲和力结合位点包含几个回文序列。以不同的结合位点为模板进行凝胶阻滞分析,并通过蛋白质滴定估计每个位点的结合常数。这是对分枝杆菌DNA结合蛋白及其与靶标相互作用的首次分子剖析。
