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细胞外产物作为荧光假单胞菌生物膜形成和脱离的介质

Extracellular products as mediators of the formation and detachment of Pseudomonas fluorescens biofilms.

作者信息

Allison D G, Ruiz B, SanJose C, Jaspe A, Gilbert P

机构信息

School of Pharmacy and Pharmaceutical Sciences, University of Manchester, UK.

出版信息

FEMS Microbiol Lett. 1998 Oct 15;167(2):179-84. doi: 10.1111/j.1574-6968.1998.tb13225.x.

DOI:10.1111/j.1574-6968.1998.tb13225.x
PMID:9867469
Abstract

Pseudomonas fluorescens B52 produces substantial biofilms at the air/liquid/solid interface of glass coverslips clamped vertically and partly submerged in liquid medium at 21 degrees C. Biofilm formation was maximal ca. 20-50 h after inoculation of the liquid medium and as indicated by environmental scanning electron microscopy (ESEM), contained large numbers of bacterial cells that were embedded within an extensive exopolymeric matrix. Incubation beyond 50 h led to reductions in biofilm which ESEM related primarily to losses of exopolymer. Both biofilm formation and the subsequent decline in exopolymer deposition was more rapid, and occurred to greater extents, when supernatants from two-day old cultures of B52 were used as the initial growth media. The addition of N-acyl-hexanoyl homoserine lactone to fresh growth medium had a similar effect upon biofilm formation as using spent culture medium. Homoserine lactones could not be demonstrated in spent culture supernatants by an Agrobacterium tumefaciens bioassay. An exopolysaccharide lyase was detected in spend culture media taken from dense biofilm cultures whose action was specifically directed towards biofilm exopolysaccharide. Results suggest that (i) cell-cell signals such as homoserine lactones are associated with the formation of P. fluorescens biofilms, (ii) the enzymic degradation of exopolymers has a specific role in the detachment of cells under starvation conditions, and (iii) whilst short chain (C6) exogenous homoserines can trigger such response in P. fluorescens, its own signal substance is likely to possess a longer (> C8) fatty acyl chain.

摘要

荧光假单胞菌B52在垂直夹紧并部分浸没于21℃液体培养基中的玻璃盖玻片的气/液/固界面处产生大量生物膜。生物膜形成在接种液体培养基后约20 - 50小时达到最大,环境扫描电子显微镜(ESEM)显示,生物膜包含大量嵌入广泛胞外聚合物基质中的细菌细胞。培养超过50小时会导致生物膜减少,ESEM显示这主要与胞外聚合物的损失有关。当使用B52两天龄培养物的上清液作为初始生长培养基时,生物膜形成以及随后胞外聚合物沉积的下降更快,且程度更大。向新鲜生长培养基中添加N - 己酰高丝氨酸内酯对生物膜形成的影响与使用陈旧培养基类似。通过根癌土壤杆菌生物测定法在陈旧培养上清液中未检测到高丝氨酸内酯。在取自密集生物膜培养物的陈旧培养基中检测到一种胞外多糖裂解酶,其作用专门针对生物膜胞外多糖。结果表明:(i)诸如高丝氨酸内酯之类的细胞间信号与荧光假单胞菌生物膜的形成有关;(ii)胞外聚合物的酶促降解在饥饿条件下细胞脱离中具有特定作用;(iii)虽然短链(C6)外源高丝氨酸可在荧光假单胞菌中触发此类反应,但其自身的信号物质可能具有更长(> C8)的脂肪酰链。

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