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Exonuclease-mediated ELISA-like assay for detecting DNA-binding activity of transcription factors: measurement of activated NF-kappaB

机译:核酸外切酶介导的类似ELISA的检测转录因子DNA结合活性的方法:活化NF-κB的测定

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摘要

This paper describes an exonuclease-mediated enzyme-linked immunosorbent assay (ELISA)-like assay (EMEA) for detecting the DNA binding activity of nuclear factor kappaB (NF-kappaB). For EMEA, a special double-stranded DNA (dsDNA)-coupled plate was first prepared by immobilizing a DNA probe on an N-oxysuccinimide ester-coated plate. The immobilized DNA probe, which was internally labeled with digoxigenin (DIG)-dT contained a NF-kappaB binding consensus sequence for capturing activated NF- kappaB in analyzed samples. For measurement, the plate was first incubated with a protein sample and then treated with exonuclease III to eliminate the probes not bound by NF-kappaB. Finally, the probes protected by NF-kappaB were colorimetrically detected by an alkaline phosphatase (AP)-conjugated anti-DIG antibody. The major advantage of EMEA is that it detects NF-kappaB without the need for NF-kappaB antibodies. EMEA may provide a general approach for assays of DNA sequence-specific transcription factors for which specific antibodies are unavailable, expensive, or of insufficient quality.
机译:本文介绍了一种外切核酸酶介导的酶联免疫吸附测定(ELISA)样测定(EMEA),用于检测核因子kappaB(NF-kappaB)的DNA结合活性。对于EMEA,首先通过将DNA探针固定在涂有N-氧琥珀酰亚胺酯的板上来制备特殊的双链DNA(dsDNA)偶联板。固定有地高辛配基(DIG)-dT的固定化DNA探针包含一个NF-κB结合共有序列,用于捕获分析样品中的活化NF-κB。为了进行测量,首先将板与蛋白质样品孵育,然后用核酸外切酶III处理,以消除未与NF-κB结合的探针。最后,用碱性磷酸酶(AP)偶联的抗DIG抗体比色检测被NF-κB保护的探针。 EMEA的主要优势在于无需NF-kappaB抗体即可检测NF-kappaB。欧洲,中东和非洲(EMEA)可能提供测定DNA序列特异性转录因子的通用方法,而无法获得其特异性抗体,价格昂贵或质量不足的抗体。

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