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Homogeneous Assay for Target Engagement Utilizing Bioluminescent Thermal Shift

机译:用于利用生物发光热移的目标接合的同质测定

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Protein thermal shift assays (TSAs) provide a means for characterizing target engagement through ligand-induced thermal stabilization. Although these assays are widely utilized for screening libraries and validating hits in drug discovery programs, they can impose encumbering operational requirements, such as the availability of purified proteins or selective antibodies. Appending the target protein with a small luciferase (NanoLuc) allows coupling of thermal denaturation with luminescent output, providing a rapid and sensitive means for assessing target engagement in compositionally complex environments such as permeabilized cells. The intrinsic thermal stability of NanoLuc is greater than mammalian proteins, and our results indicate that the appended luciferase does not alter thermal denaturation of the target protein. We have successfully applied the NanoLuc luciferase thermal shift assay (NaLTSA) to several clinically relevant protein families, including kinases, bromodomains, and histone deacetylases. We have also demonstrated the suitability of this assay method for library screening and compound profiling.
机译:蛋白质热移测定(TSAs)提供了一种通过配体诱导的热稳定性表征靶接合的装置。尽管这些测定被广泛用于筛查文库并验证药物发现程序中的命中,但它们可以施加抵押操作要求,例如纯化的蛋白质或选择性抗体的可用性。用小荧光素酶(Nanoluc)施加靶蛋白允许用发光输出耦合热变性,提供快速和敏感的方法,用于评估组成复杂环境的靶接合,例如透化细胞。纳米的内在热稳定性大于哺乳动物蛋白质,我们的结果表明所附的荧光素酶不会改变靶蛋白的热变性。我们已成功地将纳米荧光素酶热移测定(NALTSA)应用于几个临床相关的蛋白质家族,包括激酶,溴染色剂和组蛋白脱乙酰酶。我们还证明了该测定方法对图书馆筛查和化合物分析的适用性。

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