Unraveling the nature of physicochemical and biological processes underlying vesicular exocytotic release events through modeling of amperometric current spikes.

Q3 Biochemistry, Genetics and Molecular Biology
QRB Discovery Pub Date : 2025-07-24 eCollection Date: 2025-01-01 DOI:10.1017/qrd.2025.10010
Alexander Oleinick, Irina Svir, Christian Amatore
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引用次数: 0

Abstract

This work offers a comprehensive approach to understanding the phenomena underlying vesicular exocytosis, a process involved in vital functions of living organisms such as neuronal and neuroendocrine signaling. The kinetics of release of most neuromediators that modulate these functions in various ways can be efficiently monitored using single-cell amperometry (SCA). Indeed, SCA at ultramicro- or nanoelectrodes provides the necessary temporal, flux, and nanoscale resolution to accurately report on the shape and intensity of single exocytotic spikes. Rather than characterizing amperometric spikes using standard descriptive parameters (e.g., amplitude and half-width), however, this study summarizes a modeling approach based on the underlying biology and physical chemistry of single exocytotic events. This approach provides deeper insights into intravesicular phenomena that control vesicular release dynamics. The ensuing model's intrinsic parsimony makes it computationally efficient and friendly, enabling the processing of large amperometric traces to gain statistically significant insights.

Abstract Image

Abstract Image

Abstract Image

通过模拟安培电流峰值,揭示囊泡胞吐释放事件背后的物理化学和生物过程的本质。
这项工作提供了一种全面的方法来理解泡性胞吐现象,这是一个涉及生物体重要功能的过程,如神经元和神经内分泌信号。大多数神经介质的释放动力学,以各种方式调节这些功能可以有效地监测使用单细胞电流计(SCA)。事实上,在超微或纳米电极上的SCA提供了必要的时间、通量和纳米级分辨率,以准确报告单个胞外突峰的形状和强度。然而,本研究不是使用标准描述性参数(例如振幅和半宽度)来表征安培峰值,而是总结了一种基于单个胞吐事件的潜在生物学和物理化学的建模方法。这种方法为控制囊泡释放动力学的囊内现象提供了更深入的见解。随后的模型固有的简约性使其计算效率和友好性,使处理大的安培轨迹能够获得统计上显著的见解。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
QRB Discovery
QRB Discovery Biochemistry, Genetics and Molecular Biology-Biophysics
CiteScore
3.60
自引率
0.00%
发文量
18
审稿时长
12 weeks
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