Systematic In‐Depth Proteomic Analysis of Mitochondria‐Associated Endoplasmic Reticulum Membranes in Mouse and Human Testes

Wang, Xiaoli; Wen, Yujiao; Dong, Juan; Cao, Congcong; Yuan, Shuiqiao

doi:10.1002/pmic.201700478

Cited by 40 publications

(51 citation statements)

References 53 publications

(54 reference statements)

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“…When the full length of MFN2 was ectopically co-expressed with MIWI, TDRKH, and DDX4 in HEK293T cells, MFN2 was pulled down by MIWI, TDRKH, and DDX4, indicating MFN2’s ability to interact with MIWI, TDRKH and DDX4 proteins (Figure.4F-G). Importantly, our previous studies have shown that all of these interacting proteins are within the MAM structures of mouse and human testes (Wang et al, 2018), suggesting MFN2 may function with the Nuage-associated proteins in maintaining MAM structure integrity.…”

Section: Resultsmentioning

confidence: 96%

“…Alteration of MAMs increasingly was reported in several human diseases, highlighted by neurodegenerative diseases(Paillusson et al, 2016). Our previous work has demonstrated an abundance of MAMs in mouse and human testes and identified a large portion of MAM proteins in testes (Wang et al, 2018), which suggests that MAM proteins may have critical functions in spermatogenesis.…”

Section: Introductionmentioning

confidence: 92%

“…Mitofusins (MFN1/2), the homologs of Fzo in yeast and Drosophila, are the critical regulators of mitochondrial fusion in mammalian cells and enriched in MAMs (Hales and Fuller, 1997; Santel and Fuller, 2001; Wang et al, 2018). Loss of either Mfn1 or Mfn2 in mice leads to embryonic lethality, and cultured cells obtained from the mutant mouse embryos display overtly fragmented mitochondria (Chen et al, 2003).…”

Section: Introductionmentioning

confidence: 99%

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Mitofusin2 cooperates with Nuage-associated proteins and involves mRNA translational machinery in controlling mRNA fates during spermatogenesis

Wang

Zhang

et al. 2020

Preprint

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Mitochondria play a critical role in spermatogenesis and regulated by several mitochondrial fusion proteins. Its interaction with other organelles forms several unique structures, including mitochondria-associated ER membrane (MAM) and a specific type of Nuage close to mitochondria. However, the importance of mitochondria functions and mitochondrial fusion proteins in its associated-structure formation and mRNA translation during spermatogenesis remain unclear. Here, we show that Mitofusin 2 (MFN2), a mitochondrial fusion GTPase protein, cooperates with Nuage-associated proteins, including MIWI, DDX4, TDRKH and GASZ and involves translational machinery to control the fates of gamete-specific mRNAs in spermatogenesis. Conditional mutation of Mfn2 in postnatal germ cells results in male sterility due to germ cell developmental defects characterized by disruption of mitochondrial morphology, abnormal MAMs structure, aberrant mRNA translational processes, and anomalous splicing events. Moreover, MFN2 interacts with MFN1, another mitochondrial fusion protein with high-sequence similar to MFN2, in testes to facilitate spermatogenesis. Mutation of Mfn1 and Mfn2 simultaneously in testes causes very severe infertile phenotypes. Importantly, we further show that MFN2 is enriched in polysome fractions in testes and interacts with MSY2, a germ cell-specific DNA/RNA-binding protein, and eukaryotic elongation factor 1 alpha (eEF1A) to control gamete-specific mRNA translational delay during spermatogenesis. Collectively, our findings demonstrate that MFN2 works with Nuage-associated proteins and involves translational secession to regulate gamete-specific mRNA fates. Our data reveal a novel molecular link among Mitofusins, Nuage-associated proteins, and mRNA translational processes in controlling male germ cell development.

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Section: Resultsmentioning

confidence: 96%

Section: Introductionmentioning

confidence: 92%

Section: Introductionmentioning

confidence: 99%

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Mitofusin2 cooperates with Nuage-associated proteins and involves mRNA translational machinery in controlling mRNA fates during spermatogenesis

Wang

Zhang

et al. 2020

Preprint

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“…We compared our split-TurboID proteomes to previous ER-mitochondria contact proteomes obtained by other methods. The four comparison datasets were: (1) a MAM preparation from human tissue (35), (2) a study combining MAM isolation and proximity labeling (36), (3) our previous study using APEX labeling on the OMM and ERM separately, followed by dataset intersection (9), and (4) the Contact-ID-generated ER-mitochondria proteome (21). Figure 5B shows that specificity, as measured by the fraction of proteins with prior OMM or ERM annotation, is similar for all of the proximity labeling-based studies, but much poorer for the MAM dataset, which contains contaminants from many other organelles.…”

Section: Split-turboid Mediated Proteomic Mapping Of Er-mitochondria mentioning

confidence: 99%

“…Known ERM and OMM proteins (as annotated by GOCC) are labeled blue and red, respectively; ERM and OMM dual-annotated proteins are colored purple, and all other proteins are shown in black. Cutoffs used to filter the mass (35). (C) Markov clustering of split-TurboID proteome using protein-protein interaction scores from the STRING database (33).…”

Section: Figure 4 Proteomic Mapping Of Er-mitochondria Contacts In Hmentioning

confidence: 99%

Split-TurboID enables contact-dependent proximity labeling in cells

Cho

Branon

Rajeev

et al. 2020

Preprint

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Proximity labeling (PL) catalyzed by promiscuous enzymes such as TurboID have enabled the proteomic analysis of subcellular regions difficult or impossible to access by conventional fractionation-based approaches. Yet some cellular regions, such as organelle contact sites, remain out of reach for current PL methods. To address this limitation, we split the enzyme TurboID into two inactive fragments that recombine when driven together by a protein-protein interaction or membrane-membrane apposition. At endoplasmic reticulum (ER)-mitochondria contact sites, reconstituted TurboID catalyzed spatially-restricted biotinylation, enabling the enrichment and identification of >100 endogenous proteins, including many not previously linked to ER-mitochondria contacts. We validated eight novel candidates by biochemical fractionation and overexpression imaging. Overall, split-TurboID is a versatile tool for conditional and spatially-specific proximity labeling in cells.

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Functional diversity of apolipoprotein E: from subcellular localization to mitochondrial function

Rueter¹,

Rimbach²,

Huebbe³

2022

Cell. Mol. Life Sci.

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Human apolipoprotein E (APOE), originally known for its role in lipid metabolism, is polymorphic with three major allele forms, namely, APOEε2, APOEε3, and APOEε4, leading to three different human APOE isoforms. The ε4 allele is a genetic risk factor for Alzheimer’s disease (AD); therefore, the vast majority of APOE research focuses on its role in AD pathology. However, there is increasing evidence for other functions of APOE through the involvement in other biological processes such as transcriptional regulation, mitochondrial metabolism, immune response, and responsiveness to dietary factors. Therefore, the aim of this review is to provide an overview of the potential novel functions of APOE and their characterization. The detection of APOE in various cell organelles points to previously unrecognized roles in mitochondria and others, although it is actually considered a secretory protein. Furthermore, numerous interactions of APOE with other proteins have been detected, providing indications for new metabolic pathways involving APOE. The present review summarizes the current evidence on APOE beyond its original role in lipid metabolism, to change the perspective and encourage novel approaches to future research on APOE and its isoform-dependent role in the cellular metabolism.

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Systematic In‐Depth Proteomic Analysis of Mitochondria‐Associated Endoplasmic Reticulum Membranes in Mouse and Human Testes

Cited by 40 publications

References 53 publications

Mitofusin2 cooperates with Nuage-associated proteins and involves mRNA translational machinery in controlling mRNA fates during spermatogenesis

Mitofusin2 cooperates with Nuage-associated proteins and involves mRNA translational machinery in controlling mRNA fates during spermatogenesis

Split-TurboID enables contact-dependent proximity labeling in cells

Functional diversity of apolipoprotein E: from subcellular localization to mitochondrial function

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