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首页> 外文期刊>Magnetic Resonance in Chemistry: MRC >H-1-NMR relaxometric studies of interaction between apoptosis specific MRI paramagnetic contrast agents and micellar models of apoptotic cells
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H-1-NMR relaxometric studies of interaction between apoptosis specific MRI paramagnetic contrast agents and micellar models of apoptotic cells

机译:H-1-NMR弛豫法研究凋亡特异性MRI顺磁性对比剂与凋亡细胞胶束模型之间的相互作用

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摘要

H-1-NMR was previously used to analyze the interaction between peptides (E3 and R826) selected by phage display to target apoptotic cells and phospholipidic models of these cells. In order to avoid the use of apoptotic cells and to obtain a fast evaluation of the efficiency of the potential MRI contrast agents obtained by grafting these peptides and their scramble analogs on a paramagnetic gadolinium complex, their proton relaxometric behavior was investigated in the presence of micelles mimicking healthy and apoptotic cells. Their preferential interaction with 1,2-dipalmitoyl-sn-glycero-3-phospho-L-serine micelles mimicking apoptotic cells as compared with 1,2-dipalmitoyl-sn-glycero-3-phosphocholine micelles modeling healthy cells was shown by nuclear magnetic relaxation dispersion profiles and the enhancement of the transverse proton relaxation rates at 60 MHz. The association constant values confirm the stronger interaction of the selected conjugated peptides (K-a Gd-PMN-E3(gadolinium 2,2',2 '',2'''-[((4-carboxy)pyridine-2,6-diyl)bis(methylenenitrilo)]-tetrakis acetate) grafted with E3 peptide): 2.43 10(4) M-1; K-a Gd-DTPA-R826(gadolinium ((1-p-isothiocyanatobenzyl)-diethylenetriaminepentaacetate) grafted with R826 peptide): 2.91 10(4) M-1) as compared with their conjugated scrambles (K-a Gd-PMN-E3sc(gadolinium 2,2',2 '',2'''-[((4-carboxy)pyridine-2,6-diyl)bis(methylenenitrilo)]-tetrakis acetate) grafted with E3 scramble peptide): 0.18 10(4) M-1; K-a Gd-DTPA-R826sc(gadolinium ((1-p-isothiocyanatobenzyl)-diethylenetriaminepentaacetate) grafted with R826 scramble peptide): 0.32 10(4) M-1) even if the conjugation of E3 and R826 seems to decrease their interaction. Copyright (C) 2015 John Wiley & Sons, Ltd.
机译:以前曾使用H-1-NMR分析通过噬菌体展示选择的靶向细胞凋亡的肽和这些细胞的磷脂模型之间的肽(E3和R826)之间的相互作用。为了避免使用凋亡细胞并快速评估通过将这些肽及其加扰类似物嫁接到顺磁性ado络合物上而获得的潜在MRI造影剂的效率,在存在胶束的情况下研究了它们的质子弛豫行为模拟健康和凋亡细胞。通过模拟核细胞,与模拟健康细胞的1,2-二棕榈酰-sn-甘油-3-磷酸胆碱胶束相比,它们与模拟细胞凋亡细胞的1,2-二棕榈酰-sn-甘油-3-磷酸-L-丝氨酸胶束优先相互作用。弛豫色散分布和60 MHz时横向质子弛豫速率的增强。缔合常数值证实了选定的共轭肽(Ka Gd-PMN-E3(ga 2,2',2'',2'''-[((4-羧基)吡啶-2,6-二基)接枝有E3肽的双(亚甲基腈)-乙酸四酯):2.43 10(4)M-1; Ka Gd-DTPA-R826(用R826肽接枝的ga((1-对-异硫氰酸苄基)-二亚乙基三胺五乙酸酯):2.91 10(4)M-1)与共轭杂物(Ka Gd-PMN-E3sc(ga 2 ,3',2'',2'''-[((4-羧基)吡啶-2,6-二基)双(亚甲基腈)]-乙酸四酯)接枝E3加扰肽):0.18 10(4)M -1; K-a Gd-DTPA-R826sc(ga((1-对-异硫氰酸苄基)-二亚乙基三胺五乙酸酯)嫁接到R826加扰肽):0.32 10(4)M-1),即使E3和R826的结合似乎减少了它们的相互作用。版权所有(C)2015 John Wiley&Sons,Ltd.

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