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膜片钳技术在研究线粒体膜生物物理学中的应用。

Patch-clamp technique to study mitochondrial membrane biophysics.

机构信息

Department of Physiology, School of Medicine, University of Maryland, Baltimore, Baltimore, MD, USA.

出版信息

J Gen Physiol. 2023 Aug 7;155(8). doi: 10.1085/jgp.202313347. Epub 2023 Jun 22.

DOI:10.1085/jgp.202313347
PMID:37347216
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10287547/
Abstract

Mitochondria are double-membrane organelles crucial for oxidative phosphorylation, enabling efficient ATP synthesis by eukaryotic cells. Both of the membranes, the highly selective inner mitochondrial membrane (IMM) and a relatively porous outer membrane (OMM), harbor a number of integral membrane proteins that help in the transport of biological molecules. These transporters are especially enriched in the IMM, where they help maintain transmembrane gradients for H+, K+, Ca2+, PO43-, and metabolites like ADP/ATP, citrate, etc. Impaired activity of these transporters can affect the efficiency of energy-transducing processes and can alter cellular redox state, leading to activation of cell-death pathways or metabolic syndromes in vivo. Although several methodologies are available to study ion flux through membrane proteins, the patch-clamp technique remains the gold standard for quantitatively analyzing electrogenic ion exchange across membranes. Direct patch-clamp recordings of mitoplasts (mitochondria devoid of outer membrane) in different modes, such as whole-mitoplast or excised-patch mode, allow researchers the opportunity to study the biophysics of mitochondrial transporters in the native membrane, in real time, in isolation from other fluxes or confounding factors due to changes in ion gradients, pH, or mitochondrial potential (ΔΨ). Here, we summarize the use of patch clamp to investigate several membrane proteins of mitochondria. We demonstrate how this technique can be reliably applied to record whole-mitoplast Ca2+ currents mediated via mitochondrial calcium uniporter or H+ currents mediated by uncoupling protein 1 and discuss critical considerations while recording currents from these small vesicles of the IMM (mitoplast diameter = 2-5 µm).

摘要

线粒体是双层膜细胞器,对氧化磷酸化至关重要,使真核细胞能够有效地合成 ATP。这两层膜,高度选择性的内线粒体膜(IMM)和相对多孔的外线粒体膜(OMM),都含有许多整合膜蛋白,这些蛋白有助于生物分子的运输。这些转运蛋白在 IMM 中特别丰富,在那里它们有助于维持 H+、K+、Ca2+、PO43- 和代谢物(如 ADP/ATP、柠檬酸等)的跨膜梯度。这些转运蛋白的活性受损会影响能量转换过程的效率,并改变细胞的氧化还原状态,导致细胞死亡途径或体内代谢综合征的激活。尽管有几种方法可用于研究膜蛋白的离子通量,但膜片钳技术仍然是定量分析跨膜电致离子交换的金标准。通过不同模式(如完整线粒体或分离的膜片模式)对 mitoplast(不含外膜的线粒体)进行直接膜片钳记录,使研究人员有机会在天然膜中实时、孤立地研究线粒体转运蛋白的生物物理学特性,不受离子梯度、pH 值或线粒体膜电位(ΔΨ)变化引起的其他通量或混杂因素的影响。在这里,我们总结了使用膜片钳技术研究几种线粒体膜蛋白的方法。我们展示了如何可靠地应用该技术来记录通过线粒体钙单向转运体介导的完整 mitoplast Ca2+电流或通过解偶联蛋白 1 介导的 H+电流,并讨论了在记录这些 IMM 小囊泡(mitoplast 直径=2-5 µm)的电流时的关键考虑因素。

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本文引用的文献

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The mitochondrial permeability transition pore in Ca homeostasis.钙离子稳态中的线粒体通透性转换孔
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