Song-Yi Lee scite author profile

The inner mitochondrial membrane (IMM) proteome plays a central role in maintaining mitochondrial physiology and cellular metabolism. Various important biochemical reactions such as oxidative phosphorylation, metabolite production, and mitochondrial biogenesis are conducted by the IMM proteome, and mitochondria-targeted therapeutics have been developed for IMM proteins, which is deeply related for various human metabolic diseases including cancer and neurodegenerative diseases. However, the membrane topology of the IMM proteome remains largely unclear because of the lack of methods to evaluate it in live cells in a high-throughput manner. In this article, we reveal the in vivo topological direction of 135 IMM proteins, using an in situ-generated radical probe with genetically targeted peroxidase (APEX). Owing to the short lifetime of phenoxyl radicals generated in situ by submitochondrial targeted APEX and the impermeability of the IMM to small molecules, the solvent-exposed tyrosine residues of both the matrix and intermembrane space (IMS) sides of IMM proteins were exclusively labeled with the radical probe in live cells by Matrix-APEX and IMS-APEX, respectively and identified by mass spectrometry. From this analysis, we confirmed 58 IMM protein topologies and we could determine the topological direction of 77 IMM proteins whose topology at the IMM has not been fully characterized. We also found several IMM proteins (e.g., LETM1 and OXA1) whose topological information should be revised on the basis of our results. Overall, our identification of structural information on the mitochondrial inner-membrane proteome can provide valuable insights for the architecture and connectome of the IMM proteome in live cells.

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The structure of human EXD2 reveals a chimeric 3′ to 5′ exonuclease domain that discriminates substrates via metal coordination

Park

Lee

Jeong

et al. 2019

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EXD2 (3′-5′ exonuclease domain-containing protein 2) is an essential protein with a conserved DEDDy superfamily 3′-5′ exonuclease domain. Recent research suggests that EXD2 has two potential functions: as a component of the DNA double-strand break repair machinery and as a ribonuclease for the regulation of mitochondrial translation. Herein, electron microscope imaging analysis and proximity labeling revealed that EXD2 is anchored to the mitochondrial outer membrane through a conserved N-terminal transmembrane domain, while the C-terminal region is cytosolic. Crystal structures of the exonuclease domain in complex with Mn2+/Mg2+ revealed a domain-swapped dimer in which the central α5−α7 helices are mutually crossed over, resulting in chimeric active sites. Additionally, the C-terminal segments absent in other DnaQ family exonucleases enclose the central chimeric active sites. Combined structural and biochemical analyses demonstrated that the unusual dimeric organization stabilizes the active site, facilitates discrimination between DNA and RNA substrates based on divalent cation coordination and generates a positively charged groove that binds substrates.

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Direct Identification of Biotinylated Proteins from Proximity Labeling (Spot-BioID)

Lee

Seo

Rhee

2019

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Supra-blot: an accurate and reliable assay for detecting target proteins with a synthetic host molecule–enzyme hybrid

et al. 2020

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The Effect of Parental Attachment and Smart Phone Use on the College Life Adjustment of Freshmen

tae-eun¹,

Lee²

2014

JOFW

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Perception of Anxiety as the passion of the Enneagram Type 6 using Q methodology

Lee¹,

다르마칼리지²,

Kim³

2019

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Meta-analysis of Variables Related to Managerial Coaching Behavior

Kim¹,

Lee²

2023

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The Mediating Effect of Non-subject Activitieson the Career Adapt-Abilities of Self-Management

Lee¹,

tae-eun²

2016

Korean J. Fam. Walf.

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Song-Yi Lee

Architecture Mapping of the Inner Mitochondrial Membrane Proteome by Chemical Tools in Live Cells

The structure of human EXD2 reveals a chimeric 3′ to 5′ exonuclease domain that discriminates substrates via metal coordination

Direct Identification of Biotinylated Proteins from Proximity Labeling (Spot-BioID)

Supra-blot: an accurate and reliable assay for detecting target proteins with a synthetic host molecule–enzyme hybrid

The Effect of Parental Attachment and Smart Phone Use on the College Life Adjustment of Freshmen

Perception of Anxiety as the passion of the Enneagram Type 6 using Q methodology

Meta-analysis of Variables Related to Managerial Coaching Behavior

The Mediating Effect of Non-subject Activitieson the Career Adapt-Abilities of Self-Management

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