在体外化脓性CF痰液中添加细菌海藻酸裂解酶可导致海藻酸盐的破坏和痰液粘弹性的改变

R.J. Mrsny, B.A. Lazazzera, A.L. Daugherty, N.L. Schiller, T.W. Patapoff
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引用次数: 40

摘要

摘要:藻酸盐是一种存在于囊性纤维化(CF)患者化脓性气道分泌物中的大分子外多糖。这种聚合物是由一些与CF复发性肺部感染特征相关的机会性病原体产生的,已被认为会增加化脓性CF气道分泌物的粘弹性。我们研究了一种针对这种外多糖的酶的使用,一种从细菌来源获得的海藻酸裂解酶,破坏其聚合性质,并在体外影响CF痰流变学特性的变化。住院CF患者的痰中含有80-200 μg / ml海藻酸盐,内源性海藻酸解酶活性不可测。用由铜绿假单胞菌黏液菌株制备的外源性海藻酸裂解酶处理导致一小部分测试样品中海藻酸盐的破坏和痰粘弹性的降低。用重组人脱氧核糖核酸酶I对这些样品进行类似处理,以切割化脓痰中的DNA,并使用从痰中提取的海藻酸盐作为海藻酸解酶实验底物,这表明外源海藻酸解酶不能破坏海藻酸痰,不是由于底物不可接近或底物无反应。在使用海藻酸盐作为底物的研究中,通过金属离子分析确定了海藻酸盐裂解酶抗性痰样品中Ca2+和Zn2+的浓度,发现它们抑制酶的活性。在一些样品中,最初对裂解酶活性有抗性的痰样品中高浓度的Ca2+和Zn2+可以通过透析显着降低,并且这些样品对裂解酶具有敏感性。其他痰样本在透析后没有显示Ca2+和Zn2+浓度降低,这些样本仍然是赖氨酸酶不敏感的。总之,这些结果表明,化脓性CF痰中存在的细菌藻酸盐可能相当稳定,内源性藻酸盐裂解酶的活性似乎有限,体外添加外源性藻酸盐裂解酶可导致藻酸盐的破坏,并改变一些化脓性CF痰样品的粘弹性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Addition of a Bacterial Alginate Lyase to Purulent CF Sputum In Vitro Can Result in the Disruption of Alginate and Modification of Sputum Viscoelasticity

Summary: Alginate is a large molecular weight exopolysaccharide present in the purulent airway secretions of cystic fibrosis (CF) patients. This polymer, produced by some of the opportunistic pathogens associated with the recurrent lung infections characteristic of CF, has been suggested to effect an increase in the viscoelastic properties of purulent CF airway secretions. We have investigated the use of an enzyme targeted at this exopolysaccharide, an alginate lyase obtained from a bacterial source, to disrupt its polymeric nature and effect a change in the rheological properties of CF sputum in vitro. Expectorated sputum samples obtained from hospitalized CF patients were found to contain 80-200 μg alginate per ml sputum with no measurable endogenous alginate lyase activity. Treatment with exogenous alginate lyase prepared from a mucoid strain of Pseudomonas aeruginosa resulted in the disruption of alginate and a decrease in sputum viscoelasticity in a small percentage of the samples tested. Similar treatment of these samples with recombinant human deoxyribonuclease I to cleave DNA present in purulent sputum and the use of alginate extracted from sputum as an alginate lyase assay substrate suggested that the inability of the exogenous alginate lyase to disrupt sputum alginate was not due to substrate inaccessibility or an unresponsive substrate. Concentrations of Ca2+ and Zn2+ in alginate lyase-resistant sputum samples, determined by metal ion analysis, were found to inhibit enzyme activity in studies using seaweed alginate as a substrate. High concentrations of Ca2+ and Zn2+ in sputum samples initially resistant to lyase activity could be reduced significantly in some samples by dialysis and these same samples acquired sensitivity to the lyase. Other sputum samples did not show reduced concentrations of Ca2+ and Zn2+ following dialysis and these samples remained lyase-insensitive. Together, these results suggest that bacterial alginate present within purulent CF sputum may be quite stable, that endogenous alginate lyase activities appear to be limited and that the in vitro addition of exogenous alginate lyase can lead to the disruption of alginate and a change in the viscoelastic properties of some purulent CF sputum samples.

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