Li Y H, Chen Y Y, Burne R A
Center for Oral Biology and Department of Microbiology and Immunology, University of Rochester School of Medicine and Dentistry, Rochester, NY 14642, USA.
Environ Microbiol. 2000 Apr;2(2):169-77. doi: 10.1046/j.1462-2920.2000.00088.x.
The metabolism of urea by urease enzymes of oral bacteria profoundly influences oral biofilm pH homeostasis and oral microbial ecology. The purpose of this study was to gain insight into the regulation of expression of the low pH-inducible urease genes in populations of Streptococcus salivarius growing in vitro in biofilms and to explore whether urease regulation or the levels of urease expression in biofilm cells differed significantly from planktonic cells. Two strains of S. salivarius harbouring urease promoter fusions to a chloramphenicol acetyltransferase (cat) gene were used: PurelCAT, containing a fusion to the full-length, pH-sensitive promoter; or Pureldelta100CAT, a constitutively derepressed deletion derivative of the urease gene promoter. The strains were grown in a Rototorque biofilm reactor in a tryptone-yeast extract-sucrose medium with or without pH control. Both CAT and urease activities in biofilms were measured at 'quasi-steady state' and after a 25mM glucose pulse. The results showed that CAT expression in PurelCAT was repressed at relatively neutral pH values, and that expression could be induced by acidic pH after carbohydrate challenge. Biofilms of PurelCAT grown at low pH, without buffering, had about 20-fold higher CAT levels, and only a modest further induction could be elicited with carbohydrate pulsing. The levels of CAT in biofilms of PurelCAT grown in buffered medium were slightly higher than those reported for planktonic cells cultured at pH 7.0, and the levels of CAT in Purel-CAT growing at low pH or after induction were similar to those reported for fully induced planktonic cells. CAT activity in Pureldelta100CAT was constitutively high, regardless of growth conditions. Interestingly, urease activity detected in biofilms of the parent strain, S. salivarius 57.1, could be as much as 130-fold higher than that reported for fluid chemostat cultures grown under similar conditions. The higher level of urease activity in biofilms was probably caused by the accumulation of the stable urease enzyme within biofilm cells, low pH microenvironments and the growth phase of populations of cells in the biofilm. The ability of S. salivarius biofilm cells to upregulate urease expression in response to pH gradients and to accumulate greater quantities of urease enzyme when growing in biofilms may have a significant impact on oral biofilm pH homeostasis and microbial ecology in vivo. Additionally, S. salivarius carrying the pH-sensitive urease gene promoter fused to an appropriate reporter gene may be a useful biological probe for sensing biofilm pH in situ.
口腔细菌的脲酶对尿素的代谢深刻影响口腔生物膜的pH稳态和口腔微生物生态。本研究的目的是深入了解唾液链球菌群体在体外生物膜中生长时低pH诱导型脲酶基因表达的调控,并探讨生物膜细胞中脲酶的调控或表达水平与浮游细胞是否存在显著差异。使用了两株携带脲酶启动子与氯霉素乙酰转移酶(cat)基因融合的唾液链球菌:PurelCAT,包含与全长、pH敏感启动子的融合;或Pureldelta100CAT,脲酶基因启动子的组成型去阻遏缺失衍生物。这些菌株在Rototorque生物膜反应器中,于胰蛋白胨-酵母提取物-蔗糖培养基中生长,有无pH控制。在“准稳态”和25mM葡萄糖脉冲后测量生物膜中的CAT和脲酶活性。结果表明,PurelCAT中的CAT表达在相对中性的pH值下受到抑制,并且在碳水化合物刺激后酸性pH可诱导表达。在无缓冲的低pH条件下生长的PurelCAT生物膜,其CAT水平高出约20倍,并仅通过碳水化合物脉冲可引起适度的进一步诱导。在缓冲培养基中生长的PurelCAT生物膜中的CAT水平略高于在pH 7.0培养的浮游细胞所报道的水平,并且在低pH或诱导后生长的Purel-CAT中的CAT水平与完全诱导的浮游细胞所报道的水平相似。Pureldelta100CAT中的CAT活性无论生长条件如何均持续较高。有趣的是,在亲本菌株唾液链球菌57.1的生物膜中检测到的脲酶活性可能比在类似条件下生长的液体恒化器培养物所报道的活性高出多达130倍。生物膜中较高水平的脲酶活性可能是由于稳定的脲酶在生物膜细胞内积累、低pH微环境以及生物膜中细胞群体的生长阶段所致。唾液链球菌生物膜细胞响应pH梯度上调脲酶表达以及在生物膜中生长时积累更多脲酶的能力可能对体内口腔生物膜pH稳态和微生物生态产生重大影响。此外,携带与适当报告基因融合的pH敏感脲酶基因启动子的唾液链球菌可能是用于原位检测生物膜pH的有用生物探针。
