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A FRET-based screening method to detect potential inhibitors of the binding of CNNM3 to PRL2

机译:一种基于FRET的筛选方法,用于检测CNM3与PRL2结合的潜在抑制剂

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The cyclin M (CNNM) family of Mg2+ transporters is reported to promote tumour progression by binding to phosphatase of regenerating liver (PRL) proteins. Here, we established an assay for detection of the binding between the cystathionine-beta-synthase (CBS) domain of human CNNM3 (a region responsible for PRL binding) and human PRL2 using fluorescence resonance energy transfer (FRET) techniques. By fusing YPet to the C-terminus of the CNNM3 CBS domain and CyPet to the N-terminus of PRL2, we performed a FRET-based binding assay with purified proteins in multiwell plates and successfully detected the changes in fluorescence intensity derived from FRET with a reasonable Kd. We then confirmed that the addition of non-YPet-tagged CNNM3 and non-CyPet-tagged PRL proteins inhibited the changes in FRET intensity, whereas non-YPet-tagged CNNM3 with a mutation at the PRL2-binding site did not exhibit such inhibition. Furthermore, newly synthesized peptides derived from the CNNM loop region, with the PRL-binding sequences of the CNNM3 CBS domain, inhibited the interactions between CNNM3 and PRL2. Overall, these results showed that this method can be used for screening to identify inhibitors of CNNM-PRL interactions, potentially for novel anticancer therapy.
机译:据报道,Cyclin M(CNNM)的Mg2 +转运蛋白系列通过结合再生肝(PRL)蛋白质的磷酸酶来促进肿瘤进展。这里,我们建立了用于检测人CNNM3(负责PRL结合的区域的CBS)结构域与人类PRL2的胱硫胺 - β-合酶(CBS)结构域与人PRL2之间的结合的测定方法,使用荧光共振能量转移(FRET)技术。通过将YPET融合到CNNM3 CBS结构域和CYPET的C-末端至PRL2的N-末端,我们在多孔板中进行了纯化的蛋白质的基于荧光蛋白,并成功地检测到荧光强度的变化,其中合理的KD。然后,我们确认添加非YpET标记的CNNM3和非CYPET标记的PRL蛋白质抑制了FRET强度的变化,而PRL2结合位点的突变的非YPET标记的CNM3没有表现出这样的抑制作用。此外,从CNNM环形区域衍生的新合成的肽,具有CNM3 CBS结构域的PRL结合序列,抑制了CNM3和PRL2之间的相互作用。总体而言,这些结果表明,该方法可用于筛选CNNM-PRL相互作用的抑制剂,可能用于新的抗癌治疗。

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