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相关概念视频

Translocation of Proteins into the Mitochondria01:19

Translocation of Proteins into the Mitochondria

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Mitochondrial precursors are translocated to the internal subcompartments via independent mechanisms involving distinct protein machineries called translocases.
Sorting of outer membrane proteins:
Mitochondrial outer membrane proteins are of two types: the transmembrane, beta-barrel porins, and the membrane-anchored, alpha-helical proteins. Beta-barrel porin precursors are translocated by the TOM complex and inserted into the outer mitochondrial membrane by the SAM complex. In contrast,...
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Mitochondrial Precursor Proteins01:39

Mitochondrial Precursor Proteins

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Mitochondrial precursors are partially unfolded or loosely folded polypeptide chains. Newly synthesized precursors are inhibited from spontaneously folding into their native conformation by the cytosolic chaperones, heat shock proteins 70 (Hsp70), and mitochondrial import stimulation factors (MSFs). Precursors bound to MSFs are guided to the TOM70-TOM37 receptors, while precursors bound to Hsp70  chaperones are targetted to TOM20-TOM22 receptor complexes.
Most of the mitochondrial...
2.6K
Mitochondrial Protein Sorting01:39

Mitochondrial Protein Sorting

4.4K
Mitochondria are double-membrane organelles of the eukaryotes involved in cellular metabolism, signaling, ATP synthesis, and programmed cell death.  Each of these processes requires specific proteins and enzymes that must be correctly sorted to the right mitochondrial subcompartment for the proper functioning of the organelle.
Most of these mitochondrial proteins are encoded by the nucleus and imported to the mitochondria as unfolded or loosely folded precursors. Mitochondrial precursors...
4.4K
Porin Insertion in the Outer Mitochondrial Membrane01:12

Porin Insertion in the Outer Mitochondrial Membrane

3.3K
Porins are beta-barrel proteins translocated to the mitochondrial outer membrane through the TOM complex into the intermembrane space. Porin precursors bind TIM chaperones within the intermembrane space and are guided to the Sorting and Assembly Machinery complex or SAM complex on the outer mitochondrial membrane.
Three models describe the assembly of porins by the SAM complex and their insertion into the outer membrane. Model 1 suggests that porins are assembled outside the SAM channel as the...
3.3K
ATP Synthase: Mechanism01:48

ATP Synthase: Mechanism

15.1K
In animals, the mitochondrial F1F0 ATP synthase is the key protein that synthesizes ATP molecules through a complex catalytic mechanism. While the nuclear genome encodes the majority of ATP synthase subunits, the mitochondrial genome encodes some of the enzyme's most critical components. The formation of this multi-subunit enzyme is a complex multi-step process regulated at the level of transcription, translation, and assembly. Defects in one or more of these steps can result in decreased...
15.1K
Energy to Drive Translocation01:37

Energy to Drive Translocation

2.1K
Mitochondrial protein import is powered by two distinct energy sources: ATP hydrolysis and electrochemical potential across the inner membrane. Newly synthesized precursors are bound by cytosolic chaperones of the Hsp70 family, which guide them to the import receptors on the mitochondrial surface. Utilizing the energy of ATP hydrolysis, Hsp70 chaperones transfer these precursors to the TOM receptors on the mitochondrial outer membrane.
Generally, polypeptides are unfolded by two distinct...
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相关实验视频

Updated: Sep 10, 2025

Reconstitution of Msp1 Extraction Activity with Fully Purified Components
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对于线粒体特异性功能障碍的空间时间可追溯类自组件.

Xia Wu1,2, Hao Zhang1, Mingxuan Li1

  • 1State Key Laboratory of Geomicrobiology and Environmental Changes, Faculty of Materials Science and Chemistry, China University of Geosciences, Wuhan 430074, China.

Analytical chemistry
|August 19, 2025
PubMed
概括
此摘要是机器生成的。

我们开发了T-FFVLK,一种光探头,用于跟踪活细胞中的线粒体功能障碍. 这种探测器自组装成线粒体内的破坏性结构,使细胞下成像和疾病治疗潜力成为可能.

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Immunodetection of Outer Membrane Proteins by Flow Cytometry of Isolated Mitochondria
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Immunodetection of Outer Membrane Proteins by Flow Cytometry of Isolated Mitochondria

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Synthesis and Characterization of 1,2-Dithiolane Modified Self-Assembling Peptides
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Synthesis and Characterization of 1,2-Dithiolane Modified Self-Assembling Peptides

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相关实验视频

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Reconstitution of Msp1 Extraction Activity with Fully Purified Components
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Reconstitution of Msp1 Extraction Activity with Fully Purified Components

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Immunodetection of Outer Membrane Proteins by Flow Cytometry of Isolated Mitochondria
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Synthesis and Characterization of 1,2-Dithiolane Modified Self-Assembling Peptides
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科学领域:

  • 生物技术是生物技术.
  • 细胞生物学 细胞生物学
  • 分子成像学分子成像学

背景情况:

  • 的自我组装是创建影响细胞命运的功能性剂的关键策略.
  • 通过复杂的细胞内环境中的体自我组装来实现精确的有机细胞定位和功能性干扰仍然存在挑战.

研究的目的:

  • 开发一种光体探针,用于空间时空可追溯的有机体定位和功能干扰.
  • 使用自组装系统可视化和报告线粒体功能障碍.

主要方法:

  • 开发T-FFVLK,一种光体探针,将一种向线粒体的分子与一种自我组装的体结合在一起.
  • 追踪探测器的细胞入口,隔间定位和自组装动态.
  • 评估探针诱导的线粒体形态和功能变化,包括微管损伤和细胞循环停止.

主要成果:

  • T-FFVLK成功地准线粒体,形成破坏性的自我组装结构,并报告线粒体功能障碍.
  • 探针促进了 lysosomal 逃逸,并在线粒体定位时呈现出增加的光.
  • 线粒体丰富发生在6小时内,在12小时内观察到功能变化,导致细胞循环停止.

结论:

  • T-FFVLK作为一种有价值的工具,可以实时观察活细胞中的线粒体功能障碍.
  • 该探测器显示了细胞下成像应用的巨大潜力.
  • 这种自我组装的系统为未来针对线粒体的疾病治疗策略提供了希望.