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A Pectin-Methylesterase-lnhibitor-Based Molecular Probe for in Situ Detection of Plant Pectin Methylesterase Activity

机译:基于果胶-甲酯酶抑制剂的分子探针用于植物果胶甲酯酶活性的原位检测

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In the quest of obtaining a molecular probe for in situ detection of pectin methylesterase (PME), the PME inhibitor (PMEI) was biotinylated and the biotinylated PMEI (bPMEl) was extensively characterized. Reaction conditions for single labeling of the purified PMEI with retention of its inhibitory capacity were identified. High-performance size-exclusion chromatography (HPSEC) analysis revealed that the bPMEl retained its ability to form a complex with plant PME and that it gained the capacity to strongly bind an avidin species. By means of dot-blot binding assays, the ability of the probe to recognize native and high-temperature or high-pressure denatured plant PMEs, coated on an absorptive surface, was investigated and compared to the binding characteristics of recently reported anti-PME monoclonal antibodies. Contrary to the antibodies, bPMEl only detected active PME molecules. Subsequently, both types of probes were used for PME localization in tissue-printing experiments. bPMEl proved its versatility by staining prints of carrot root, broccoli stem, and tomato fruit. Applying the tissue-printing technique on carrot roots after thermal treatment demonstrated the complementarity of bPMEl and anti-PME antibodies, with the former selectively detecting the remaining active PME and the latter staining both native and inactivated PME molecules.
机译:为了获得用于原位检测果胶甲基酯酶(PME)的分子探针,对PME抑制剂(PMEI)进行了生物素化,并对生物素化的PMEI(bPME1)进行了广泛表征。鉴定了单标记纯化PMEI并保留其抑制能力的反应条件。高性能尺寸排阻色谱法(HPSEC)分析显示,bPMEl保留了与植物PME形成复合物的能力,并且具有牢固结合亲和素物种的能力。通过点印迹结合试验,研究了探针识别包覆在吸收性表面上的天然和高温或高压变性植物PME的能力,并将其与最近报道的抗PME单克隆抗体的结合特性进行了比较。抗体。与抗体相反,bPMEl仅检测到活性PME分子。随后,两种类型的探针都用于组织印刷实验中的PME定位。 bPMEl通过对胡萝卜根,西兰花茎和番茄果实的印迹进行染色,证明了其多功能性。热处理后在胡萝卜根上应用组织印刷技术证明了bPMEl和抗PME抗体的互补性,前者选择性检测剩余的活性PME,而后者则染色天然和灭活的PME分子。

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