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A Rational Designed PslG With Normal Biofilm Hydrolysis and Enhanced Resistance to Trypsin-Like Protease Digestion

机译:一种理性设计的PSLG,具有正常的生物膜水解,增强胰蛋白酶样蛋白酶消化的抗性

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摘要

A glycosyl hydrolase produced by Pseudomonas aeruginosa, PslG, has become a promising candidate for biofilm treatment because of its ability to inhibit and disperse biofilms by disrupting exopolysaccharide matrix at nanomolar concentrations. However, as a protein, PslG used for treatment may be degraded by the ubiquitous proteases (of which trypsin-like serine proteases are a major group) secreted by human cells. This would lead to an insufficient effective concentration of PslG. Here, based on the result of liquid chromatography–tandem mass spectrometry (LC-MS/MS) and structural analysis, we generate a PslG mutant (K286A/K433S) with greatly enhanced trypsin resistance. This measure raises IC50 (the concentration of trypsin that can degrade 50% of protein in 30 min at 37°C) from 0.028 mg mL–1 of the wild-type PslG to 0.283 mg mL–1 of PslGK286A/K433S. In addition, biofilm inhibition assay shows that PslGK286A/K433S is much more efficient than wild-type PslG in the presence of trypsin. This indicates that PslGK286A/K433S is a better biofilm inhibitor than wild-type PslG in clinical use where trypsin-like proteases widely exist.
机译:由Pseudomonas铜绿假单胞菌PSLG产生的糖基水解酶已成为生物膜处理的有希望的候选者,因为它通过在纳米摩尔浓度下破坏外渗基质来抑制和分散生物膜的能力。然而,作为蛋白质,用于处理的PSLg可以通过人细胞分泌的普遍蛋白酶(胰蛋白酶样丝氨酸蛋白酶是主要群体)降解。这将导致PSLG的有效浓度不足。这里,基于液相色谱 - 串联质谱(LC-MS / MS)和结构分析的结果,我们产生具有极大提高胰蛋白酶抗性的PSLG突变体(K286A / K433S)。该措施提高了IC50(胰蛋白酶的浓度,可以在37℃下在30分钟内降解50%的蛋白质)从野生型PSLG的0.028mg ml-1至0.283mg ml-1的pslgk286a / k433s。此外,生物膜抑制测定表明,在胰蛋白酶存在下,PSLGK286A / K433S比野生型PSLG更有效。这表明PSLGK286A / K433s是比野生型PSLG在临床用途中的更好的生物膜抑制剂,其中胰蛋白酶样蛋白酶广泛存在。

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