ECSIT is a critical limiting factor for cardiac function
Linan Xu, … , David J. Grieve, Paul N. Moynagh
Linan Xu, … , David J. Grieve, Paul N. Moynagh
Published May 25, 2021
Citation Information: JCI Insight. 2021;6(12):e142801. https://doi.org/10.1172/jci.insight.142801.
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Research Article Cardiology Metabolism

ECSIT is a critical limiting factor for cardiac function

Abstract

Evolutionarily conserved signaling intermediate in Toll pathways (ECSIT) is a protein with roles in early development, activation of the transcription factor NF-κB, and production of mitochondrial reactive oxygen species (mROS) that facilitates clearance of intracellular bacteria like Salmonella. ECSIT is also an important assembly factor for mitochondrial complex I. Unlike the murine form of Ecsit (mEcsit), we demonstrate here that human ECSIT (hECSIT) is highly labile. To explore whether the instability of hECSIT affects functions previously ascribed to its murine counterpart, we created a potentially novel transgenic mouse in which the murine Ecsit gene is replaced by the human ECSIT gene. The humanized mouse has low levels of hECSIT protein, in keeping with its intrinsic instability. Whereas low-level expression of hECSIT was capable of fully compensating for mEcsit in its roles in early development and activation of the NF-κB pathway, macrophages from humanized mice showed impaired clearance of Salmonella that was associated with reduced production of mROS. Notably, severe cardiac hypertrophy was manifested in aging humanized mice, leading to premature death. The cellular and molecular basis of this phenotype was delineated by showing that low levels of human ECSIT protein led to a marked reduction in assembly and activity of mitochondrial complex I with impaired oxidative phosphorylation and reduced production of ATP. Cardiac tissue from humanized hECSIT mice also showed reduced mitochondrial fusion and more fission but impaired clearance of fragmented mitochondria. A cardiomyocyte-intrinsic role for Ecsit in mitochondrial function and cardioprotection is also demonstrated. We also show that cardiac fibrosis and damage in humans correlated with low expression of human ECSIT. In summary, our findings identify a role for ECSIT in cardioprotection, while generating a valuable experimental model to study mitochondrial dysfunction and cardiac pathophysiology.

Authors

Linan Xu, Fiachra Humphries, Nezira Delagic, Bingwei Wang, Ashling Holland, Kevin S. Edgar, Jose R. Hombrebueno, Donna Beer Stolz, Ewa Oleszycka, Aoife M. Rodgers, Nadezhda Glezeva, Kenneth McDonald, Chris J. Watson, Mark T. Ledwidge, Rebecca J. Ingram, David J. Grieve, Paul N. Moynagh

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Figure 1

Humanized ECSIT mice show intact activation of NF-κB and MAPK pathways but impaired production of mROS and clearance of S. typhimurium.

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Humanized ECSIT mice show intact activation of NF-κB and MAPK pathways b...
(A) Immunoblot analysis of ECSIT, β-actin, and total and phosphorylated (p-) forms of IκBα, JNK, ERK, and p38 MAPK in cell lysates isolated from WT and ECSIT+/+ BMDMs after LPS stimulation (100 ng/mL) for the indicated time periods. (B and C) ELISA analysis of (B) IL-6 and (C) TNF-α in cell supernatants of WT and ECSIT+/+ BMDMs after LPS stimulation (100 ng/mL) for 0 to 24 hours. (D) Immunoblot analysis of ECSIT, β-actin, and total and phosphorylated (p) forms of IκBα, JNK, ERK, and p38 MAPK in cell lysates isolated from WT and ECSIT+/+ BMDMs after challenge with heat-inactivated S. typhimurium (strain SL1344) for indicated times at an estimated multiplicity of infection (MOI) of 10. (E and F) ELISA analysis of (E) IL-6 and (F) TNF-α in cell supernatants of WT and ECSIT+/+ BMDMs after infection. (G) MitoSox (mROS) and CM-H2DCFDA (cROS) staining of WT and ECSIT+/+ BMDMs infected S. typhimurium with MFI expressed relative to uninfected WT cells. (H) CFU analysis of BMDMs from WT and ECSIT+/+ mice after 2- to 24-hour infection with S. typhimurium SL1344 at MOI of 10 and 50. (I) CFU analysis of homogenized liver and spleen tissue from WT, Ecsit+/–, and ECSIT+/+ mice after infection for 72 hours by oral gavage with S. typhimurium SL1344 (1 × 107 CFU). Data are expressed as the mean ± SD from at least 3 technical replicates, and each representation has at least 2 independent experiments (AH); unpaired 2-tailed Student’s t test, **P < 0.01. Data indicate samples from individual mice (n = 5–8) (I); 1-way ANOVA with Dunnett’s multiple comparisons test, **P < 0.01.