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亲和毛细管电泳辅助生物层干涉法研究人乳头瘤病毒样颗粒与层粘连蛋白 332 的相互作用。

Interaction studies between human papillomavirus virus-like particles and laminin 332 by affinity capillary electrophoresis assisted by bio-layer interferometry.

机构信息

Laboratory for the Analysis of Medicines (LAM), Center for Interdisciplinary Research on Medicines (CIRM), University of Liège, Liège, Belgium.

InBioS - Centre for Protein Engineering, Département des Sciences de La Vie, University of Liège, Liège, Belgium.

出版信息

Talanta. 2024 Apr 1;270:125602. doi: 10.1016/j.talanta.2023.125602. Epub 2023 Dec 26.

DOI:10.1016/j.talanta.2023.125602
PMID:38199121
Abstract

Human papillomavirus (HPV) interacts, in vitro, with laminin 332 (LN332), a key component of the extracellular matrix. In this study, we performed bio-layer interferometry (BLI) and affinity capillary electrophoresis (ACE) to investigate the binding properties of this interaction. Virus-like particles (VLPs), composed of the HPV16 L1 major capsid protein, were used as HPV model and LN332 as the VLPs binding partner. Using BLI, we quantitatively determined the kinetics of the interaction, via the measurement of VLP binding and release from LN332 immobilized onto the surface of aminopropylsilane biosensors. We found an averaged k of 1.74 x 10 Ms and an averaged k of 1.50 x 10 s. Furthermore, an ACE method was developed to study the interaction under physiological conditions, where the interactants are moving freely in solution, without any fluorescence labeling. Specifically, a constant amount of HPV16-VLPs was preincubated with increasing LN332 concentrations and then the samples were injected in the capillary electrophoresis instrument. A shift in the migration time of the HPV16-VLP/LN332 complexes, carrying an increasing number of LN332 molecules bound per VLP, was observed. The mobility of the complexes was found to decrease with increasing LN332 concentrations in the sample. It was used to quantify stability constant. From BLI and ACE approaches, we reported an apparent equilibrium dissociation constant in the nanomolar range (8.89 nM and 17.7 nM, respectively) for the complex between HPV16-VLPs and LN332.

摘要

人乳头瘤病毒(HPV)在体外与层粘连蛋白 332(LN332)相互作用,LN332 是细胞外基质的关键组成部分。在这项研究中,我们使用生物层干涉(BLI)和亲和毛细管电泳(ACE)来研究这种相互作用的结合特性。病毒样颗粒(VLPs)由 HPV16 L1 主要衣壳蛋白组成,用作 HPV 模型,LN332 用作 VLPs 的结合伴侣。使用 BLI,我们通过测量固定在氨丙基硅烷生物传感器表面的 LN332 上的 VLP 结合和释放来定量测定相互作用的动力学。我们发现平均 k 为 1.74 x 10^Ms,平均 k 为 1.50 x 10^s。此外,还开发了 ACE 方法来研究生理条件下的相互作用,其中相互作用的物质在溶液中自由移动,没有任何荧光标记。具体来说,将一定量的 HPV16-VLPs 与逐渐增加的 LN332 浓度预孵育,然后将样品注入毛细管电泳仪。观察到 HPV16-VLP/LN332 复合物的迁移时间发生了变化,其中每个 VLP 结合的 LN332 分子数量增加。复合物的迁移率被发现随着样品中 LN332 浓度的增加而降低。它被用于定量稳定常数。从 BLI 和 ACE 方法,我们报告了 HPV16-VLPs 和 LN332 之间复合物的表观平衡解离常数在纳摩尔范围内(分别为 8.89 nM 和 17.7 nM)。

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