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液泡积累和共定位不是细胞质可溶性蛋白发生选择性自噬的适当标准。

Vacuolar accumulation and colocalization is not a proper criterion for cytoplasmic soluble proteins undergoing selective autophagy.

机构信息

MOE Key Laboratory of Laser Life Science & Guangdong Provincial Key Laboratory of Laser Life Science, College of Biophotonics, South China Normal University, Guangzhou, China.

Guangzhou Key Laboratory of Spectral Analysis and Functional Probes, College of Biophotonics, South China Normal University, Guangzhou, China.

出版信息

Plant Signal Behav. 2021 Oct 3;16(10):1932319. doi: 10.1080/15592324.2021.1932319. Epub 2021 Jun 27.

Abstract

Autophagy is an important cytoprotective process that mediates degradation of dysfunctional or unnecessary cellular components. In the process of autophagy, a double-membrane organelle termed the autophagosome is formed to sequestrate portions of cytoplasm and subsequently delivered into lysosome or vacuole for degradation. The accumulation of autophagic bodies in the vacuoles after treatment with concanamycin A (ConcA) is a widely used protocol for monitoring the occurrence of autophagy in plants. Here, it was found that the cytoplasmic soluble GFP was accumulated in vacuoles upon ConcA treatment. Importantly, the GFP signal showed good colocalization with the autophagic marker mCherry-ATG8f in vacuoles based on two commonly used methods, the Pearson-Spearman correlation colocalization analysis and the plot profile analysis. Further results showed that the free GFP did not interact with ATG8s. Thus, analysis of accumulation and colocalization only in vacuoles is not a trustworthy way to judge whether degradation of cytoplasmic protein is dependent on the selective autophagy pathway in plants. In this short perspective, we propose several primary steps to distinguish that the cytoplasmic proteins are degraded by selective or bulk autophagy, hoping they could contribute to identify and clarify the selective autophagic cargos and receptors in plants.

摘要

自噬是一种重要的细胞保护过程,介导细胞内功能失调或不必要的成分的降解。在自噬过程中,形成一个双层膜细胞器,称为自噬体,以隔离细胞质的部分,并随后递送至溶酶体或液泡中进行降解。在用康纳霉素 A (ConcA)处理后,自噬体在液泡中的积累是一种广泛用于监测植物自噬发生的常用方法。在这里,发现细胞质可溶性 GFP 在 ConcA 处理时积累在液泡中。重要的是,根据两种常用的方法,即 Pearson-Spearman 相关共定位分析和绘图轮廓分析,GFP 信号与液泡中的自噬标记 mCherry-ATG8f 显示出良好的共定位。进一步的结果表明,游离 GFP 不与 ATG8s 相互作用。因此,仅在液泡中分析积累和共定位并不是判断细胞质蛋白降解是否依赖于植物选择性自噬途径的可靠方法。在这篇短评中,我们提出了几个初步步骤来区分细胞质蛋白是通过选择性自噬还是批量自噬降解的,希望它们有助于识别和阐明植物中的选择性自噬货物和受体。

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