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交互式计算和实验方法提高了基于周质结合蛋白的尼古丁生物传感器在生物流体中测量的灵敏度。

Interactive computational and experimental approaches improve the sensitivity of periplasmic binding protein-based nicotine biosensors for measurements in biofluids.

作者信息

Haloi Nandan, Huang Shan, Nichols Aaron L, Fine Eve J, Friesenhahn Nicholas J, Marotta Christopher B, Dougherty Dennis A, Lindahl Erik, Howard Rebecca J, Mayo Stephen L, Lester Henry A

机构信息

Department of Applied Physics, Science for Life Laboratory, KTH Royal Institute of Technology, 10044 Stockholm, Sweden.

Division of Biology and Biological Engineering, California Institute of Technology, Pasadena CA 91125 USA.

出版信息

bioRxiv. 2024 Jan 18:2023.01.16.524298. doi: 10.1101/2023.01.16.524298.

DOI:10.1101/2023.01.16.524298
PMID:36712031
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9882114/
Abstract

We developed fluorescent protein sensors for nicotine with improved sensitivity. For iNicSnFR12 at pH 7.4, the proportionality constant for vs [nicotine] (δ-slope, 2.7 μM) is 6.1-fold higher than the previously reported iNicSnFR3a. The activated state of iNicSnFR12 has a fluorescence quantum yield of at least 0.6. We measured similar dose-response relations for the nicotine-induced absorbance increase and fluorescence increase, suggesting that the absorbance increase leads to the fluorescence increase via the previously described nicotine-induced conformational change, the "candle snuffer" mechanism. Molecular dynamics (MD) simulations identified a binding pose for nicotine, previously indeterminate from experimental data. MD simulations also showed that Helix 4 of the periplasmic binding protein (PBP) domain appears tilted in iNicSnFR12 relative to iNicSnFR3a, likely altering allosteric network(s) that link the ligand binding site to the fluorophore. In thermal melt experiments, nicotine stabilized the PBP of the tested iNicSnFR variants. iNicSnFR12 resolved nicotine in diluted mouse and human serum at 100 nM, the peak [nicotine] that occurs during smoking or vaping, and possibly at the decreasing levels during intervals between sessions. NicSnFR12 was also partially activated by unidentified endogenous ligand(s) in biofluids. Improved iNicSnFR12 variants could become the molecular sensors in continuous nicotine monitors for animal and human biofluids.

摘要

我们开发了对尼古丁具有更高灵敏度的荧光蛋白传感器。对于pH 7.4条件下的iNicSnFR12,其与[尼古丁]的比例常数(δ斜率,2.7 μM)比之前报道的iNicSnFR3a高6.1倍。iNicSnFR12的激活态荧光量子产率至少为0.6。我们测量了尼古丁诱导的吸光度增加和荧光增加之间类似的剂量反应关系,这表明吸光度增加是通过之前描述的尼古丁诱导的构象变化(“烛剪”机制)导致荧光增加的。分子动力学(MD)模拟确定了尼古丁的结合姿势,这在之前的实验数据中是不确定的。MD模拟还表明,周质结合蛋白(PBP)结构域的螺旋4在iNicSnFR12中相对于iNicSnFR3a似乎发生了倾斜,这可能改变了将配体结合位点与荧光团连接起来的变构网络。在热熔实验中,尼古丁使测试的iNicSnFR变体的PBP稳定。iNicSnFR12能够分辨稀释的小鼠和人血清中100 nM的尼古丁,这是吸烟或吸电子烟时出现的尼古丁峰值浓度,也可能是两次吸烟间隔期间逐渐降低的浓度。NicSnFR12还被生物流体中未鉴定的内源性配体部分激活。经过改进的iNicSnFR12变体可能会成为用于动物和人类生物流体的连续尼古丁监测仪中的分子传感器。

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本文引用的文献

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β2 nAChR Activation on VTA DA Neurons Is Sufficient for Nicotine Reinforcement in Rats.VTA 神经元上β2 nAChR 的激活足以增强尼古丁在大鼠中的强化作用。
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