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藻酸盐及其O-乙酰化在铜绿假单胞菌微菌落和生物膜形成中的作用。

Role of alginate and its O acetylation in formation of Pseudomonas aeruginosa microcolonies and biofilms.

作者信息

Nivens D E, Ohman D E, Williams J, Franklin M J

机构信息

Center for Environmental Biotechnology, University of Tennessee, Knoxville, Tennessee, 37996, USA.

出版信息

J Bacteriol. 2001 Feb;183(3):1047-57. doi: 10.1128/JB.183.3.1047-1057.2001.

Abstract

Attenuated total reflection/Fourier transform-infrared spectrometry (ATR/FT-IR) and scanning confocal laser microscopy (SCLM) were used to study the role of alginate and alginate structure in the attachment and growth of Pseudomonas aeruginosa on surfaces. Developing biofilms of the mucoid (alginate-producing) cystic fibrosis pulmonary isolate FRD1, as well as mucoid and nonmucoid mutant strains, were monitored by ATR/FT-IR for 44 and 88 h as IR absorbance bands in the region of 2,000 to 1,000 cm(-1). All strains produced biofilms that absorbed IR radiation near 1,650 cm(-1) (amide I), 1,550 cm(-1) (amide II), 1,240 cm(-1) (P==O stretching, C---O---C stretching, and/or amide III vibrations), 1,100 to 1,000 cm(-1) (C---OH and P---O stretching) 1,450 cm(-1), and 1,400 cm(-1). The FRD1 biofilms produced spectra with an increase in relative absorbance at 1,060 cm(-1) (C---OH stretching of alginate) and 1,250 cm(-1) (C---O stretching of the O-acetyl group in alginate), as compared to biofilms of nonmucoid mutant strains. Dehydration of an 88-h FRD1 biofilm revealed other IR bands that were also found in the spectrum of purified FRD1 alginate. These results provide evidence that alginate was present within the FRD1 biofilms and at greater relative concentrations at depths exceeding 1 micrometer, the analysis range for the ATR/FT-IR technique. After 88 h, biofilms of the nonmucoid strains produced amide II absorbances that were six to eight times as intense as those of the mucoid FRD1 parent strain. However, the cell densities in biofilms were similar, suggesting that FRD1 formed biofilms with most cells at depths that exceeded the analysis range of the ATR/FT-IR technique. SCLM analysis confirmed this result, demonstrating that nonmucoid strains formed densely packed biofilms that were generally less than 6 micrometer in depth. In contrast, FRD1 produced microcolonies that were approximately 40 micrometer in depth. An algJ mutant strain that produced alginate lacking O-acetyl groups gave an amide II signal approximately fivefold weaker than that of FRD1 and produced small microcolonies. After 44 h, the algJ mutant switched to the nonmucoid phenotype and formed uniform biofilms, similar to biofilms produced by the nonmucoid strains. These results demonstrate that alginate, although not required for P. aeruginosa biofilm development, plays a role in the biofilm structure and may act as intercellular material, required for formation of thicker three-dimensional biofilms. The results also demonstrate the importance of alginate O acetylation in P. aeruginosa biofilm architecture.

摘要

衰减全反射/傅里叶变换红外光谱法(ATR/FT-IR)和扫描共聚焦激光显微镜(SCLM)被用于研究藻酸盐及其结构在铜绿假单胞菌在表面附着和生长中的作用。通过ATR/FT-IR监测黏液型(产藻酸盐)囊性纤维化肺部分离株FRD1以及黏液型和非黏液型突变株形成生物膜的过程,持续44小时和88小时,监测2000至1000 cm⁻¹区域的红外吸收带。所有菌株产生的生物膜在1650 cm⁻¹(酰胺I)、1550 cm⁻¹(酰胺II)、1240 cm⁻¹(P==O伸缩、C---O---C伸缩和/或酰胺III振动)、1100至1000 cm⁻¹(C---OH和P---O伸缩)、1450 cm⁻¹和1400 cm⁻¹处吸收红外辐射。与非黏液型突变株的生物膜相比,FRD1生物膜产生的光谱在1060 cm⁻¹(藻酸盐的C---OH伸缩)和1250 cm⁻¹(藻酸盐中O-乙酰基的C---O伸缩)处相对吸光度增加。88小时的FRD1生物膜脱水后显示出其他红外带,这些带也在纯化的FRD1藻酸盐光谱中发现。这些结果证明藻酸盐存在于FRD1生物膜中,且在超过1微米深度处相对浓度更高,这是ATR/FT-IR技术的分析范围。88小时后,非黏液型菌株生物膜产生的酰胺II吸光度是黏液型FRD1亲本菌株的六至八倍。然而,生物膜中的细胞密度相似,这表明FRD1形成的生物膜中大多数细胞位于超过ATR/FT-IR技术分析范围的深度。SCLM分析证实了这一结果,表明非黏液型菌株形成紧密堆积的生物膜,深度一般小于6微米。相比之下,FRD1产生的微菌落深度约为40微米。产生缺乏O-乙酰基藻酸盐的algJ突变株产生的酰胺II信号比FRD1弱约五倍,并产生小的微菌落。44小时后,algJ突变株转变为非黏液型表型并形成均匀的生物膜,类似于非黏液型菌株产生

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Bacterial alginate biosynthesis--recent progress and future prospects.细菌藻酸盐生物合成——最新进展与未来展望。
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