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Measuring Binding Kinetics of Ligands with Tethered Receptors by Fluorescence Polarization and Total Internal Reflection Fluorescence

机译:通过荧光偏振和全内反射荧光测量配体与束缚受体的结合动力学

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Binding kinetics of nuclear receptors and their specific ligands was measured using polarization anisotropy complemented with total internal reflection fluorescence. Binding affinities of tethered full length human estrogen receptor alpha (ER(alpha)) with 17beta-estradiol, diethylstilbestrol, raloxifene, 4-hydroxytamoxifen, tamoxifen, and genistein were measured to be 100 (as reference), 100, 35, 21, 8, and 1.5, respectively. They agreed with published results. For the first time, rate constants were measured, and off rates were 1.5, 1.5, 1.3, 1.6, 1.7, and 2.3 X 10~(-3) s~(-1) while on rates were 11, 10, 3.3, 2.4, 1.0, and 0.26 X 10~(5) M~(-1)s~(-1), respectively. For the antiestrogen drugs, their comparable off-rates correlated well with their equally similar potency. Eleven ginsenosides were screened as potential ligands. None were found to bind to ER(alpha), but Rb1(S) and 20(S)-Rg3 were shown to bind to peroxisome proliferator-activated receptor gamma. The latter finding corroborated strongly with the therapeutic effects of ginsenosides on diabetic mice observed in a separate study. Our method would complement surface plasmon resonance assay for small ligands in the mass range of tens to hundreds of Daltons.
机译:使用极化各向异性与全内反射荧光互补,测量核受体及其特异性配体的结合动力学。拴系的全长人雌激素受体α(ER(α))与17β-雌二醇,己二烯雌酚,雷洛昔芬,4-羟基他莫昔芬,他莫昔芬和染料木黄酮的结合亲和力经测量为100(作为参考),100、35、21、8和1.5。他们同意发表的结果。首次测量速率常数,关闭速率为1.5、1.5、1.3、1.6、1.7和2.3 X 10〜(-3)s〜(-1),打开速率为11、10、3.3、2.4 ,1.0和0.26 X 10〜(5)M〜(-1)s〜(-1)。对于抗雌激素药物,其可比的降价率与它们同样相似的效价密切相关。筛选了11种人参皂苷作为潜在的配体。没有发现与ERα结合,但是Rb1(S)和20(S)-Rg3与过氧化物酶体增殖物激活的受体γ结合。后者的发现与人参皂甙对糖尿病小鼠的治疗作用有强烈的佐证。我们的方法将对质量范围在几十到数百道尔顿之间的小配体进行表面等离子体共振分析。

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