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BOCILLIN FL a Sensitive and Commercially Available Reagent for Detection of Penicillin-Binding Proteins

机译:BOCILLIN FL用于检测青霉素结合蛋白的灵敏且可商购的试剂

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摘要

We describe a new, sensitive, rapid, and nonradioactive method involving the use of the commercially available BOCILLIN FL, a fluorescent penicillin, as a labeling reagent for the detection and study of penicillin-binding proteins (PBPs). This method allowed rapid detection of 30 ng of a purified PBP protein under UV light and of 2 to 4 ng of the protein with the aid of a FluorImager. This method also allowed rapid determination of the PBP profiles of Escherichia coli, Pseudomonas aeruginosa, and Streptococcus pneumoniae. The PBP profiles obtained are virtually identical to those reported previously with 3H-, 14C-, or 125I-labeled penicillin. Using this method enabled us to determine the 50% inhibitory concentrations of the penicillin-sensitive and -resistant PBP2x proteins of S. pneumoniae for penicillin G, thereby allowing a direct evaluation of their relative affinities for penicillin G. Finally, this method also allowed us to compare relative affinities of a PBP2x protein for different β-lactam antibiotics with the aid of fluorescence polarization technology and to monitor a PBP2x protein during purification.
机译:我们描述了一种新的,灵敏的,快速的,非放射性的方法,其中涉及使用市售的荧光青霉素BOCILLIN FL作为标记试剂来检测和研究青霉素结合蛋白(PBPs)。该方法可在Fluorlightr的帮助下在紫外光下快速检测30 ng纯化的PBP蛋白,并检测2至4 ng的蛋白。该方法还可以快速测定大肠杆菌,铜绿假单胞菌和肺炎链球菌的PBP谱。获得的PBP分布图实际上与先前使用 3 H-, 14 C-或 125 I标记的青霉素报道的相同。使用此方法使我们能够确定肺炎链球菌对青霉素G的青霉素敏感性和耐药性PBP2x蛋白的50%抑制浓度,从而可以直接评估其对青霉素G的相对亲和力。最后,该方法还使我们能够通过荧光偏振技术比较PBP2x蛋白对不同β-内酰胺抗生素的相对亲和力,并在纯化过程中监测PBP2x蛋白。

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