Glucan Binding Proteins of Oral Streptococci

口腔链球菌的葡聚糖结合蛋白

• 批准号: 6892352
• 负责人: Jeffrey A Banas
• 金额: $ 27.65万
• 依托单位: ALBANY MEDICAL COLLEGE
• 依托单位国家: 美国
• 财政年份: 1992
• 资助国家: 美国
• 起止时间: 1992-08-01 至 2008-04-30
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/6892352
• 关键词: Streptococcus mutans; binding proteins; binding sites; biofilm; cations; cell membrane; chimeric proteins; dental caries; dental plaque; enzyme activity; enzyme mechanism; glucans; hexosyltransferase; hydropathy; membrane proteins; microarray technology; microorganism culture; microorganism metabolism; molecular cloning; mutant; oral bacteria; plasmids; polymerase chain reaction; protein structure; recombinant proteins

DESCRIPTION: Streptococcus mutans possesses three distinct glucosyltransferases (GTFs) and at least three different nonenzymatic glucan binding proteins (GBPs). The precise contributions of each GTF and GBP to plaque development are unknown. Recently we showed that the loss of a glucan-binding protein (GbpA), accomplished through allelic replacement, dramatically altered the architecture of the biofilm formed by cultures of S. mutans. Based on these data we engineered strains with inactivation in genes encoding other extracellular proteins. The loss of GbpC, FruA, or P1 also resulted in changes in the biofilm architecture. To explain these observations we posit that the loss of an extracellular protein may result in specific physical and/or biochemical changes to the organism, or to its immediate environment that affect the structure of the mature biofilm formed by that organism. The Specific Aims of this application are designed to test these possibilities. Since work with the GbpA has progressed the furthest, investigations of specific GbpA properties are also included in the Aims. Aim 1) Examine the physical properties of the knockout strains including hydrophobicity, surface charge, and their interactions with cations such as calcium which are important in the development of a biofilm. Aim 2) Use a flow chamber to examine the events associated with the initial attachment of the knockout strains to the substratum and correlate the results with the structure of the mature biofilms. Aim 3) Examine how the ratio of GbpA to glucan synthesis correlates with the structure of the biofilm. Aim 4) Delete or replace the amino terminal domain (non glucan-binding domain) of GbpA and examine how this change affects the phenotypic properties of Streptococcus mutans compared to the wild-type and GbpA knockout strains. Aim 5) Express phenotypic properties of formation. Aim 6) Utilize architecture influence gene GbpA in the heterologous host Streptococcus gordonii and examine the organism in the context of sucrose-dependent adhesion and biofilm microarrays to determine how the loss of extracellular proteins and biofilm expression.

产品说明：变形链球菌具有三种不同的葡糖基转移酶（GTF）和至少三种不同的非酶葡聚糖结合蛋白（GBP）。每种GTF和GBP对斑块发展的确切贡献尚不清楚。最近，我们发现，通过等位基因替换实现的葡聚糖结合蛋白（GbpA）的丢失，显著改变了由S.变异人基于这些数据，我们设计了编码其他细胞外蛋白的基因失活的菌株。GbpC、FruA或P1的丢失也导致生物膜结构的变化。为了解释这些观察结果，我们认为细胞外蛋白的丢失可能导致生物体或其直接环境的特定物理和/或生化变化，这些变化影响由该生物体形成的成熟生物膜的结构。本应用程序的特定目标旨在测试这些可能性。由于与GbpA的合作进展最大，因此目标中还包括对GbpA特定特性的研究。目的1）检查敲除菌株的物理性质，包括疏水性、表面电荷以及它们与阳离子如钙的相互作用，这些阳离子在生物膜的形成中是重要的。目的2）使用流动室来检查与敲除菌株与基质的初始附着相关的事件，并将结果与成熟生物膜的结构相关联。目的3）检查GbpA与葡聚糖合成的比率如何与生物膜的结构相关。目的4）将GbpA的氨基端结构域（非葡聚糖结合结构域）缺失或替换，并与野生型和GbpA基因敲除菌株比较，研究这种改变对变形链球菌表型特性的影响。目的5）表达地层的表型特征。目的6）利用异源宿主格氏链球菌中的结构影响基因GbpA，在蔗糖依赖性粘附和生物膜微阵列的背景下检测该生物体，以确定胞外蛋白的丢失和生物膜的表达。