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首页> 外文期刊>ACS Omega >Fragment Binding to β-Secretase 1 without Catalytic Aspartate Interactions Identified via Orthogonal Screening Approaches
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Fragment Binding to β-Secretase 1 without Catalytic Aspartate Interactions Identified via Orthogonal Screening Approaches

机译:片段与β-分泌酶1的结合,而没有通过正交筛选方法鉴定出催化天冬氨酸的相互作用

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摘要

An approach to identify β-secretase 1 (BACE1) fragment binders that do not interact with the catalytic aspartate dyad is presented. A ThermoFluor (thermal shift) and a fluorescence resonance energy transfer enzymatic screen on the soluble domain of BACE1, together with a surface plasmon resonance (SPR) screen on the soluble domain of BACE1 and a mutant of one catalytic Asp (D32N), were run in parallel. Fragments that were active in at least two of these assays were further confirmed using one-dimensional NMR (WaterLOGSY) and SPR binding competition studies with peptidic inhibitor OM99-2. Protein-observed NMR (two-dimensional ~(15)N heteronuclear single-quantum coherence spectroscopy) and crystallographic studies with the soluble domain of BACE1 identified a unique and novel binding mode for compound 12 , a fragment that still occupies the active site while not making any interactions with catalytic Asps. This novel approach of combining orthogonal fragment screening techniques, for both wild-type and mutant enzymes, as well as binding competition studies could be generalized to other targets to overcome undesired interaction motifs and as a hit-generation approach in highly constrained intellectual property space.
机译:提出了鉴定不与催化天门冬氨酸二联体相互作用的β-分泌酶1(BACE1)片段结合剂的方法。运行BACE1可溶性域上的ThermoFluor(热位移)和荧光共振能量转移酶促筛选,以及BACE1可溶性域上的表面等离子体共振(SPR)筛选和一个催化性Asp(D32N)突变体在平行下。使用一维NMR(WaterLOGSY)和肽抑制剂OM99-2进行SPR结合竞争研究,进一步证实了在至少两种测定中有活性的片段。蛋白质观察的NMR(二维((15)N)异核单量子相干光谱学)和BACE1可溶性结构域的晶体学研究确定了化合物 12的独特新颖结合方式,该化合物仍占据活性不会与催化性Asps发生任何相互作用的位置。这种针对野生型和突变型酶结合正交片段筛选技术的新颖方法,以及结合竞争研究,可以推广到其他目标,以克服不希望的相互作用基序,并且可以在高度受限的知识产权领域中作为命中方法。

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