链霉菌属菌株FRI-5中IM-2结合蛋白的纯化与特性分析
Purification and characterization of the IM-2-binding protein from Streptomyces sp. strain FRI-5.
作者信息
Ruengjitchatchawalya M, Nihira T, Yamada Y
机构信息
Department of Biotechnology, Faculty of Engineering, Osaka University, Japan.
出版信息
J Bacteriol. 1995 Feb;177(3):551-7. doi: 10.1128/jb.177.3.551-557.1995.
IM-2 [(2R,3R,1'R)-2-(1'-hydroxybutyl)-3-(hydroxymethyl)butanolide] of Streptomyces sp. strain FRI-5 is one of the butyrolactone autoregulators of Streptomyces species and triggers production of blue pigment as well as the nucleoside antibiotics showdomycin and minimycin. A tritium-labeled IM-2 analogue, 2,3-trans-2(1'-beta-hydroxy-[4',5'-3H]pentyl)-3-(hydroxymethyl)butano lide ([3H]IM-2-C5; 40 Ci/mmol), was synthesized for a competitive binding assay, and an IM-2-specific binding protein was found to be present in the crude cell extract of Streptomyces sp. strain FRI-5. During cultivation for 24 h, the specific IM-2-binding activity increased rapidly, reached a plateau at 10 to 14 h, and declined sharply thereafter, showing only 6% activity after 24 h of cultivation. A Scatchard plot of the binding data demonstrated that the dissociation constant (Kd) for [3H]IM-2-C5 was 1.3 nM, while the Kd for a 3H-labeled virginiae butanolide (VB) analogue, 2-(1'-alpha-hydroxy-[6',7'-3H]heptyl)-3-(hydroxymethyl)butanolide ([3H]VB-C7), another butyrolactone autoregulator possessing the opposite configuration at C-1' was 35 nM. Furthermore, at a 15-fold molar excess, the effectiveness of several autoregulators as nonlabeled competitive ligands against [3H]IM-2-C5 was IM-2 type > VB-C type >> A-factor type, indicating that the binding protein in Streptomyces sp. strain FRI-5 is highly specific toward IM-2. Ultracentrifugation showed that the IM-2-binding protein is present almost exclusively in the 100,000 x g supernatant fraction, indicating that the binding protein is a cytoplasmic soluble protein. The binding protein was purified by ammonium sulfate precipitation, DEAE-Sephacel chromatography, Sephacryl S-100 HR gel filtration, DEAE-5PW high-performance liquid chromatography (HPLC), and phenyl-5PW HPLC. The apparent Mr of the native IM-2-binding protein as determined by molecular sieve HPLC was about 60,000 in the presence of 0.5, 0.3, or 0.1 M KCl, while by sodium dodecyl sulfate-polyacrylamide gel electrophoresis it was about 27,000, suggesting that the native binding protein is present in the form of a dimer.
链霉菌属菌株FRI-5产生的IM-2[(2R,3R,1'R)-2-(1'-羟基丁基)-3-(羟甲基)丁内酯]是链霉菌属的丁内酯自调控因子之一,可触发蓝色色素以及核苷抗生素秀多霉素和小霉素的产生。为进行竞争性结合试验,合成了一种氚标记的IM-2类似物,2,3-反式-2(1'-β-羟基-[4' ,5'-3H]戊基)-3-(羟甲基)丁内酯([3H]IM-2-C5;40 Ci/mmol),并发现链霉菌属菌株FRI-5的粗细胞提取物中存在一种IM-2特异性结合蛋白。在培养24小时期间,IM-2特异性结合活性迅速增加,在10至14小时达到平台期,此后急剧下降,培养24小时后仅显示6%的活性。结合数据的Scatchard图表明,[3H]IM-2-C5的解离常数(Kd)为1.3 nM,而一种3H标记的弗吉尼亚丁内酯(VB)类似物,2-(1'-α-羟基-[6',7'-3H]庚基)-3-(羟甲基)丁内酯([3H]VB-C7),另一种在C-1'具有相反构型的丁内酯自调控因子的Kd为35 nM。此外,在15倍摩尔过量的情况下,几种自调控因子作为未标记的竞争性配体对[3H]IM-2-C5的有效性为IM-2型>VB-C型>>A因子型,表明链霉菌属菌株FRI-5中的结合蛋白对IM-2具有高度特异性。超速离心表明,IM-2结合蛋白几乎完全存在于100,000×g上清液组分中,表明该结合蛋白是一种细胞质可溶性蛋白。通过硫酸铵沉淀、DEAE-葡聚糖凝胶层析、Sephacryl S-100 HR凝胶过滤、DEAE-5PW高效液相色谱(HPLC)和苯基-5PW HPLC对结合蛋白进行了纯化。在0.5、0.3或0.1 M KCl存在下,通过分子筛HPLC测定的天然IM-2结合蛋白的表观Mr约为60,000,而通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳测定约为27,000,表明天然结合蛋白以二聚体形式存在。
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