p66Shc Mediates SUMO2-induced Endothelial Dysfunction

  1. Jitendra Kumar
  2. Shravan K. Uppulapu
  3. Sujata Kumari
  4. Kanika Sharma
  5. William Paradee
  6. Ravi Prakash Yadav
  7. Vikas Kumar
  8. Santosh Kumar

  • Curated by eLife

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    eLife Assessment

    This study offers valuable insights into the role of post-translational modifiers, specifically SUMO2ylation at K81 in p66Shc, and its impact on endothelial function through reactive oxygen species. A series of compelling experiments demonstrated that lysine 81 of p66Shc is the site of SUMO2 conjugation, which is crucial for mitochondrial localization and essential for S36 phosphorylation, leading to specific pathological effects. The combination of cell overexpression and animal studies provides solid data supporting this mechanistic link.

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Abstract

Background

Sumoylation is a post-translational modification that can regulate different physiological functions. Increased sumoylation, specifically conjugation of SUMO2/3 (small ubiquitin-like modifier 2/3), is detrimental to vascular health. However, the molecular mechanism mediating this effect is poorly understood.

Methods

We used cell-based assays and mass spectrometry to show that p66Shc is a direct target of SUMO2 and SUMO2 regulates p66Shc function via lysine-81 modification. To determine the effects of SUMO2-p66ShcK81 on vascular function, we generated p66ShcK81R knockin mice and crossbred to LDLr -/- mice to induce hyperlipidemia. Next, to determine p66ShcK81-SUMO2ylation-induced changes in endothelial cell signaling, we performed mass spectrometry followed by Ingenuity Pathway Analysis.

Results

Our data reveal that p66Shc mediates the effects of SUMO2 on endothelial cells. Mass spectrometry identified that SUMO2 modified lysine-81 in the unique collagen homology-2 domain of p66Shc. SUMO2ylation of p66Shc increased phosphorylation at serine-36, causing it to translocate to the mitochondria, a step critical for oxidative function of p66Shc. Notably, sumoylation-deficient p66Shc (p66ShcK81R) was resistant to SUMO2-induced p66ShcS36 phosphorylation and mitochondrial translocation. P66ShcK81R knockin mice were resistant to endothelial dysfunction induced by SUMO2ylation and hyperlipidemia. Ingenuity Pathway Analysis revealed multiple signaling pathways regulated by p66ShcK81-SUMO2ylation in endothelial cells, highlighting Rho-GTPase as a major pathway affected by SUMO2-p66ShcK81.

Conclusions

Collectively, our work reveals SUMO2-p66Shc signaling as a fundamental regulator of vascular endothelial function. We discovered that p66ShcK81 is an upstream modification regulating p66Shc signaling and mediates hyperlipidemia-induced endothelial dysfunction and oxidative stress.

Article activity feed

  1. eLife

    eLife Assessment

    This study offers valuable insights into the role of post-translational modifiers, specifically SUMO2ylation at K81 in p66Shc, and its impact on endothelial function through reactive oxygen species. A series of compelling experiments demonstrated that lysine 81 of p66Shc is the site of SUMO2 conjugation, which is crucial for mitochondrial localization and essential for S36 phosphorylation, leading to specific pathological effects. The combination of cell overexpression and animal studies provides solid data supporting this mechanistic link.

  2. eLife

    Reviewer #1 (Public review):

    Summary:

    The authors describe a role of sumoylation at K81 in p66Shc which affects endothelial dysfunction. This explores a new mechanism for understanding the role of PTMs in cellular processes.

    Strengths:

    The experiments are well planned and the results are well represented.
    Vascular tonality experiments were carried out nicely, given the amount of time and effort one needs to put in to get clean results from these experiments.

    Weaknesses:

    (1) The production of ROS has been measured in a very superficial way.
    The term "ROS" confers a plethora of chemical species which exerts different physiological effects on different cells and situations.
    Mitochondria through one of the source , but not the only source of ROS production. Only measuring ROS with mitosox do not reflect the cellular condition of ROS in a specific condition. I would suggest authors consider doing IF of oxidative stress specific markers , carbonyl group and also, maybe, Amplex red for determining average oxidative stress and ros production in the cells.
    (2) 8-OHG signal seems very confusing in Figure 7E. 8-ohg is supposed to be mainly in the nucleus and to some extent in mitochondria. The signal is very diffused in the images. I would suggest a higher magnification and better resolution images for 8-ohg. Also, the VWF signal is pretty weak whereas it should be strong given the staining is in aorta. Authors should redo the experiments.
    (3) PCA analysis is quite not clear. Why is there a convergence among the plots? Authors should explain. Also, I would suggest that the authors do the analysis done in Figure 8B again with R based packages. IPA, though being user-friendly, mostly does not yield meaningful results and the statistics carried out is not accurate. Authors should redo the analysis in R or Python whichever is suitable for them.
    (4) The MS analysis part seems pretty vague in methods. Please rewrite.

  3. eLife

    Reviewer #2 (Public review):

    Summary:

    The article builds on the earlier work that both p66Shc and SUMOylation are essential nitric oxide (NO) based development of endothelial vasculature (PMID: 10580504; 28760777 and 35187108). The current manuscript brings forward a finding of how SUMO2ylation of p66Shc mediated ROS production which is essential for endothelial cells. They further identify that lysine 81 of p66Shc is the residue which is conjugated to SUMO2 and is crucial for mitochondrial localization. They further show that K81 SUMO2ylation is essential for S36 phosphorylation.

    Strengths:

    Convincingly shows that p66Shc is SUMO2ylated on lysine 81 in cells and also shows that the phosphorylation (serine 36) reduces upon loss of this critical SUMOylation site.

    Weaknesses:

    All the experiments performed here are in overexpression background therefore, it would be crucial to show that p66Shc is SUMO2ylated at physiological levels.

  4. eLife

    Reviewer #3 (Public review):

    Summary:

    The authors set out to determine how SUMO2 impairs endothelial function through direct modification of the protein p66Shc. p66Shc is known to promote reactive oxygen species production, and here the authors demonstrate that SUMO2 modifies p66Shc at lysine-81, resulting in increased phosphorylation, mitochondrial translocation. These are prosed to mediate the detrimental effects of SUMO2 in a mouse model of hyperlipidemia.

    Strengths:

    A major strength of this work is the multi-pronged approach combining biochemical assays, proteomic analyses, and a genetically modified mouse model expressing a SUMOylation resistant mutant of p66Shc. These experiments comprehensively illustrate that lysine-81 SUMOylation of p66Shc is necessary for the observed endothelial dysfunction in hyperlipidemic conditions.

    Weaknesses:

    One notable weakness is that the link between the observed cellular changes and the ultimate in vivo phenotype remains only partially explored. While the authors successfully show that p66ShcK81R knockin mice are protected from endothelial dysfunction in a hyperlipidemic context, additional experiments characterizing the broader tissue-specific roles, or examining further endothelial assays in vivo, would strengthen the mechanistic conclusions. It would also be beneficial to see more direct evaluations of p66Shc subcellular localization in the protective knockin mice to complement the proteomic findings.

    Despite these gaps, the data broadly support the authors' main conclusions. The authors lay out a plausible mechanistic pathway for how hyperlipidemia and increased global SUMOylation can converge on the oxidative stress pathway to provoke vascular dysfunction.

    The likely impact of this work on the field is noteworthy. Beyond clarifying how a single post-translational modification event can influence the pathophysiology of endothelial cells, the study provides a model for investigating broader roles of SUMO2 in other cardiovascular conditions and highlights the importance of identifying additional SUMOylation sites and their downstream impact.

    In conclusion, by demonstrating the direct SUMOylation of p66Shc at lysine-81 and linking that modification to endothelial dysfunction in a hyperlipidemic mouse model, this paper offers valuable insights into how broadly acting post-translational modifiers can evoke specific pathological effects.

  5. eLife

    Author response:

    Public Reviews:

    Reviewer #1 (Public review):

    (1) The production of ROS has been measured in a very superficial way.

    The term "ROS" confers a plethora of chemical species which exerts different physiological effects on different cells and situations.

    Mitochondria through one of the source, but not the only source of ROS production. Only measuring ROS with mitosox do not reflect the cellular condition of ROS in a specific condition. I would suggest authors consider doing IF of oxidative stress specific markers , carbonyl group and also, maybe, Amplex red for determining average oxidative stress and ros production in the cells.

    We agree with the reviewer that a detailed analysis of ROS production and its markers would strengthen the manuscript. Accordingly, we will perform the Amplex Red assay for Figure 1.

    (2) 8-OHG signal seems very confusing in Figure 7E. 8-ohg is supposed to be mainly in the nucleus and to some extent in mitochondria. The signal is very diffused in the images. I would suggest a higher magnification and better resolution images for 8-ohg. Also, the VWF signal is pretty weak whereas it should be strong given the staining is in aorta. Authors should redo the experiments.

    The reviewer’s comment is correct regarding the expected signal. We will repeat the assays. However, we would like to note that the flat morphology of the endothelial cell monolayer on the aortic surface may limit the visualization of subcellular signal differentiation when transversely sectioned.

    (3) PCA analysis is quite not clear. Why is there a convergence among the plots? Authors should explain. Also, I would suggest that the authors do the analysis done in Figure 8B again with R based packages. IPA, though being user-friendly, mostly does not yield meaningful results and the statistics carried out is not accurate. Authors should redo the analysis in R or Python whichever is suitable for them.

    Thank you for your valuable feedback. We acknowledge the concern regarding the PCA analysis and the convergence observed in the plots. In the revised manuscript, we will revise our interpretation to clarify this observation.

    Additionally, we appreciate your suggestion to use R-based packages for pathway analysis. We will make efforts to regenerate the analysis presented in Figure 8B using R to enhance the statistical robustness and reproducibility of our results.

    (4) The MS analysis part seems pretty vague in methods. Please rewrite.

    We will revise the methods section to improve the legibility.

    Reviewer #2 (Public review):

    All the experiments performed here are in overexpression background therefore, it would be crucial to show that p66Shc is SUMO2ylated at physiological levels.

    To address this concern, we will attempt to assess p66Shc-SUMO2 levels under physiological conditions. However, we would like to highlight a technical limitation: the currently available antibodies do not distinguish p66Shc from other isoforms, nor SUMO2 from SUMO3. Therefore, enriching for the endogenous p66Shc-SUMO2 adduct will require novel tools and techniques, which we are actively exploring.

    Reviewer #3 (Public review):

    One notable weakness is that the link between the observed cellular changes and the ultimate in vivo phenotype remains only partially explored. While the authors successfully show that p66ShcK81R knockin mice are protected from endothelial dysfunction in a hyperlipidemic context, additional experiments characterizing the broader tissue-specific roles, or examining further endothelial assays in vivo, would strengthen the mechanistic conclusions. It would also be beneficial to see more direct evaluations of p66Shc subcellular localization in the protective knockin mice to complement the proteomic findings.

    That is an excellent suggestion. We will determine the tissue specific distribution of endogenous p66ShcK81R.

    Despite these gaps, the data broadly support the authors' main conclusions. The authors lay out a plausible mechanistic pathway for how hyperlipidemia and increased global SUMOylation can converge on the oxidative stress pathway to provoke vascular dysfunction.

    The likely impact of this work on the field is noteworthy. Beyond clarifying how a single post-translational modification event can influence the pathophysiology of endothelial cells, the study provides a model for investigating broader roles of SUMO2 in other cardiovascular conditions and highlights the importance of identifying additional SUMOylation sites and their downstream impact.

    In conclusion, by demonstrating the direct SUMOylation of p66Shc at lysine-81 and linking that modification to endothelial dysfunction in a hyperlipidemic mouse model, this paper offers valuable insights into how broadly acting post-translational modifiers can evoke specific pathological effects.

  6. Version published to 10.1101/2024.01.24.577109v3 on bioRxiv
  7. Version published to 10.1101/2024.01.24.577109v2 on bioRxiv
  8. Version published to 10.1101/2024.01.24.577109v1 on bioRxiv