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Phage-displayed peptides as biosensor reagents.

机译:噬菌体显示的肽作为生物传感器试剂。

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This study investigated the potential to utilize phage-displayed peptides as reagents in sensor applications. A library of random 12-mers displayed on phage was panned against staphylococcal enterotoxin B (SEB), a causative agent of food poisoning. Nine SEB binding phage clones were isolated, all of which share the consensus sequence Trp His Lys at their amino terminus. Binding of several of these phage was shown to be inhibited when they were assayed in a competitive enzyme-linked immunosorbent assay (ELISA) format with synthesized peptide corresponding to the peptide-encoding region of one of the clones. Whole phage were labeled with the dye Cy5, and incorporated into fluoroimmunoassays. Labeled phage were able to detect SEB down to a concentration of 1.4 ng/well in a fluorescence-based immunoassay. When incorporated into an automated fluorescence-based sensing assay, Cy5-labeled phage bound to probes coated with SEB generated a robust signal of about 10,000 pA, vs a signal of 1,000 pA using a control fiber coated with streptavidin. These results demonstrate the potential for development of phage-based sensor reagents.
机译:本研究研究了在传感器应用中使用噬菌体展示的肽作为试剂的可能性。在噬菌体中显示出在噬菌体上显示的随机12-MERS库,对葡萄球菌肠毒素B(SEB),一种食物中毒的致病剂。九种SEB结合噬菌体克隆被隔离,所有这些都在其氨基末端分享了他的Lys的共有序列。当在竞争性酶联免疫吸附测定(ELISA)形式中测定它们的竞争性酶联免疫测定(ELISA)形式中,抑制了几种这些噬菌体的结合,其具有与其中一种克隆的编码区域对应的合成肽。用染料Cy5标记整个噬菌体,并掺入氟莫纳腺组中。标记的噬菌体能够在荧光的免疫测定中检测到1.4ng /孔的浓度为1.4ng /孔。当掺入自动荧光的感测测定中时,Cy5标记的噬菌体与涂有SEB的探针,产生约10,000Pa的鲁棒信号,使用涂有链霉抗生物素蛋白的对照纤维的1,000Pa的信号。这些结果证明了基于噬菌体的传感器试剂的发育的可能性。

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