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阳离子卟啉对革兰氏阴性重组生物发光菌光动力灭活的机制。

Mechanisms of photodynamic inactivation of a gram-negative recombinant bioluminescent bacterium by cationic porphyrins.

机构信息

CESAM and Department of Biology, University of Aveiro, 3810-193, Aveiro, Portugal.

出版信息

Photochem Photobiol Sci. 2011 Oct;10(10):1659-69. doi: 10.1039/c1pp05097d. Epub 2011 Jul 29.

Abstract

Photodynamic therapy is a very promising approach to inactivate pathogenic microorganisms. The photodamage of cells involves reactive oxygen species (ROS) which are generated in situ by two main mechanisms (type I and/or type II). The mechanism responsible for the photoinactivation (PI) of a bioluminescent recombinant Escherichia coli, induced by three different cationic porphyrins, was identified in this work using a rapid method based on the monitoring of the metabolic activity of this bacterium. The inhibitory effect of the photodynamic process in the presence of a singlet oxygen quencher (sodium azide) or free radical scavengers (d-mannitol and l-cysteine) was evaluated by exposing bacterial suspensions with 0.5 μM Tri-Py(+)-Me-PF, 5.0 μM Tetra-Py(+)-Me or 5.0 μM Tri-SPy(+)-Me-PF to white light. Strong bacterial protection was observed with sodium azide (100 mM) for the three cationic porphyrins. However, in the presence of Tri-Py(+)-Me-PF and Tetra-Py(+)-Me and the free radical scavengers (l-cysteine and d-mannitol) the reduction on the bacterial bioluminescence was significantly higher and similar to that obtained in their absence (5.4-6.0 log reduction). In the case of Tri-SPy(+)-Me-PF two distinct behaviours were observed when l-cysteine and d-mannitol were used as free radical scavengers: while the presence of l-cysteine (100 mM) lead to a bacterial protection similar to the one observed with sodium azide, in the presence of d-mannitol only a small protection was detected. The high inhibition of the PS activity by l-cysteine is not due to its radical scavenger ability but due to the singlet oxygen quenching by the sulfanyl group (-SH). In fact, the photodecomposition of 1,3-diphenylisobenzofuran in the presence of Tri-SPy(+)-Me-PF is completely suppressed when l-cysteine is present. The results obtained in this study suggest that singlet oxygen (type II mechanism) plays a very important role over free radicals (type I mechanism) on the PI process of the bioluminescent E. coli by Tri-Py(+)-Me-PF, Tetra-Py(+)-Me and Tri-SPy(+)-Me-PF. Although the use of scavengers is an adequate and simple approach to evaluate the relative importance of the two pathways, it is important to choose scavengers which do not interfere in both PI mechanisms. Sodium azide and d-mannitol seem to be good oxygen and free radical quenchers, respectively, to study the PI mechanisms by porphyrinic photosensitizers.

摘要

光动力疗法是一种非常有前途的方法来灭活致病微生物。细胞的光损伤涉及活性氧物种(ROS),其通过两种主要机制(I 型和/或 II 型)在原位产生。本工作使用基于监测该细菌代谢活性的快速方法,鉴定了三种不同阳离子卟啉诱导的生物发光重组大肠杆菌光灭活(PI)的机制。通过用 0.5 μM Tri-Py(+)-Me-PF、5.0 μM Tetra-Py(+)-Me 或 5.0 μM Tri-SPy(+)-Me-PF 暴露细菌悬浮液,评估了在单线态氧猝灭剂(叠氮化钠)或自由基清除剂(D-甘露醇和 L-半胱氨酸)存在下光动力过程的抑制作用。对于三种阳离子卟啉,观察到叠氮化钠(100 mM)对细菌的强烈保护作用。然而,在 Tri-Py(+)-Me-PF 和 Tetra-Py(+)-Me 以及自由基清除剂(L-半胱氨酸和 D-甘露醇)存在下,细菌生物发光的降低明显更高,与不存在时的降低相似(5.4-6.0 log 降低)。在 Tri-SPy(+)-Me-PF 的情况下,当使用 L-半胱氨酸和 D-甘露醇作为自由基清除剂时,观察到两种不同的行为:虽然 L-半胱氨酸(100 mM)的存在导致类似于用叠氮化钠观察到的细菌保护,但在 D-甘露醇存在下仅检测到很小的保护。L-半胱氨酸对 PS 活性的高抑制不是由于其自由基清除能力,而是由于 -SH 基团的单线态氧猝灭。事实上,当 Tri-SPy(+)-Me-PF 存在时,1,3-二苯基异苯并呋喃的光分解完全被抑制。本研究结果表明,单线态氧(II 型机制)在 Tri-Py(+)-Me-PF、Tetra-Py(+)-Me 和 Tri-SPy(+)-Me-PF 对生物发光大肠杆菌的 PI 过程中比自由基(I 型机制)起着非常重要的作用。虽然使用清除剂是评估两种途径相对重要性的一种合适且简单的方法,但选择不干扰两种 PI 机制的清除剂很重要。叠氮化钠和 D-甘露醇似乎分别是良好的氧和自由基清除剂,用于研究卟啉类光敏剂的 PI 机制。

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