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首页> 外文期刊>Current Protocols in Chemical Biology >Metabolic Incorporation of N-Acetyl Muramic Acid Probes into Bacterial Peptidoglycan
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Metabolic Incorporation of N-Acetyl Muramic Acid Probes into Bacterial Peptidoglycan

机译:将N-乙酰象酸探针的代谢掺入细菌肽肽

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Bacterial cells utilize small carbohydrate building blocks to construct peptidoglycan (PG), a highly conserved mesh-like polymer that serves as a protective coat for the cell. PG production has long been a target for antibiotics, and its breakdown isa source for human immune recognition. A key component of bacterial PG, N-acetyl muramic acid (NAM), is a vital element in many synthetically derived immunostimulatory compounds. However, the exact molecular details of these structures and how they are generated remain unknown due to a lack of chemical probes surrounding the NAM core. A robust synthetic strategy to generate bioorthogonally tagged NAM carbohydrate units is implemented. These molecules serve as precursors for PG biosynthesis and recycling. Escherichia coli cells are metabolically engineered to incorporate the bioorthogonal NAM probes into their PG network. The probes are subsequently modified using copper-catalyzed azide-alkyne cycloaddition to install fiuorophores directly into the bacterial PG, as confirmed by super-resolution microscopy and high-resolution mass spectrometry. Here, synthetic notes for key elements of this process to generate the sugar probes as well as streamlined user-friendly metabolic labeling strategies for both microbiology and immunological applications are described.
机译:细菌细胞利用小碳水化合物构建块来构建肽聚糖(PG),一种高度保守的网状聚合物,其用作细胞的保护涂层。 PG产量长期以来一直是抗生素的目标,其崩溃ISA为人类免疫识别来源。细菌PG,N-乙酰蛋白酸(NAM)的关键组分是许多合成衍生的免疫刺激化合物中的重要元素。然而,由于围绕Nam核心的缺乏化学探针,这些结构的确切分子细节以及它们的产生仍然未知。实施了生成生物正交标记的NAM碳水化合物单元的稳健的合成策略。这些分子用作PG生物合成和再循环的前体。对大肠杆菌细胞进行代谢工程化以将生物正交nam探针掺入它们的PG网络中。随后使用铜催化的叠氮化物 - 炔烃环编辑改性探针,以将FIOOROOCHORE直接安装到细菌PG中,如通过超分辨率显微镜和高分辨率质谱所证实。这里,描述了该方法的关键要素的合成票据,以产生糖探针以及用于微生物学和免疫应用的简化的用户友好的代谢标记策略。

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