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Mechanism and uses of a membrane peptide that targets tumors and other acidic tissues in vivo

机译:体内靶向肿瘤和其他酸性组织的膜肽的机制和用途

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The pH-selective insertion and folding of a membrane peptide, pHLIP [pH (low) insertion peptide], can be used to target acidic tissue in vivo, including acidic foci in tumors, kidneys, and inflammatory sites. In a mouse breast adenocarcinoma model, fluorescently labeled pHLIP finds solid acidic tumors with high accuracy and accumulates in them even at a very early stage of tumor development. The fluorescence signal is stable for > 4 days and is approximately five times higher in tumors than in healthy counterpart tissue. In a rat antigen-induced arthritis model, pHLIP preferentially accumulates in inflammatory foci. pHLIP also maps the renal cortical interstitium; however, kidney accumulation can be reduced significantly by providing mice with bicarbonate-containing drinking water. The peptide has three states: soluble in water, bound to the surface of a membrane, and inserted across the membrane as an α-helix. At physiological pH, the equilibrium is toward water, which explains its low affinity for cells in healthy tissue; at acidic pH, titration of Asp residues shifts the equilibrium toward membrane insertion and tissue accumulation. The replacement of two key Asp residues located in the transmembrane part of pHLIP by Lys or Asn led to the loss of pH-sensitive insertion into membranes of liposomes, red blood cells, and cancer cells in vivo, as well as to the loss of specific accumulation in tumors. pHLIP nanotechnology introduces a new method of detecting, targeting, and possibly treating acidic diseased tissue by using the selective insertion and folding of membrane peptides.
机译:膜肽的pH选择性插入和折叠pHLIP [pH(低)插入肽]可用于靶向体内酸性组织,包括肿瘤,肾脏和炎症部位的酸性病灶。在小鼠乳腺腺癌模型中,荧光标记的pHLIP可以高度准确地发现固体酸性肿瘤,甚至在肿瘤发展的非常早期就可以在其中积聚。荧光信号在超过4天的时间内保持稳定,并且在肿瘤中的荧光信号比在健康的对应组织中高大约五倍。在大鼠抗原诱导的关节炎模型中,pHLIP优先在炎症灶中积累。 pHLIP还可以绘制肾皮质间质的图。但是,通过为小鼠提供含碳酸氢盐的饮用水可以大大减少肾脏的蓄积。该肽具有三种状态:可溶于水,与膜表面结合并以α-螺旋的形式插入整个膜。在生理pH值下,平衡趋向于水,这说明了其对健康组织中细胞的低亲和力。在酸性pH下,Asp残留的滴定使平衡朝着膜插入和组织积累的方向移动。用Lys或Asn替代位于pHLIP跨膜部分的两个关键Asp残基导致体内对脂质体,红细胞和癌细胞膜的pH敏感插入的丧失,以及特异性抗体的丧失在肿瘤中积累。 pHLIP纳米技术通过选择性插入和折叠膜肽,引入了一种检测,靶向和治疗酸性病变组织的新方法。

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