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Role of succinate in airway epithelial cell regulation following traumatic lung injury
Madathilparambil V. Suresh, Sinan Aktay, George Yalamanchili, Sumeet Solanki, Dily Thazhath Sathyarajan, Manikanta Swamy Arnipalli, Subramaniam Pennathur, Krishnan Raghavendran
Madathilparambil V. Suresh, Sinan Aktay, George Yalamanchili, Sumeet Solanki, Dily Thazhath Sathyarajan, Manikanta Swamy Arnipalli, Subramaniam Pennathur, Krishnan Raghavendran
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Research Article Inflammation Pulmonology

Role of succinate in airway epithelial cell regulation following traumatic lung injury

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Abstract

Lung contusion and gastric aspiration (LC and GA) are major risk factors for developing acute respiratory distress following trauma. Hypoxia from lung injury is mainly regulated by hypoxia-inducible factor 1α (HIF-1α). Published data from our group indicate that HIF-1α regulation in airway epithelial cells (AEC) drives the acute inflammatory response following LC and GA. Metabolomic profiling and metabolic flux of Type II AEC following LC revealed marked increases in glycolytic and TCA intermediates in vivo and in vitro that were HIF-1α dependent. GLUT-1/4 expression was also increased in HIF-1α+/+ mice, suggesting that increased glucose entry may contribute to increased intermediates. Importantly, lactate incubation in vitro on Type II cells did not significantly increase the inflammatory byproduct IL-1β. Contrastingly, succinate had a direct proinflammatory effect on human small AEC by IL-1β generation in vitro. This effect was reversed by dimethylmalonate, suggesting an important role for succinate dehydrogenase in mediating HIF-1α effects. We confirmed the presence of the only known receptor for succinate binding, SUCNR1, on Type II AEC. These results support the hypothesis that succinate drives HIF-1α–mediated airway inflammation following LC. This is the first report to our knowledge of direct proinflammatory activation of succinate in nonimmune cells such as Type II AEC in direct lung injury models.

Authors

Madathilparambil V. Suresh, Sinan Aktay, George Yalamanchili, Sumeet Solanki, Dily Thazhath Sathyarajan, Manikanta Swamy Arnipalli, Subramaniam Pennathur, Krishnan Raghavendran

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Figure 11

The absence of HIF-1α resulted in elevated SDH activity following LC and GA.

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The absence of HIF-1α resulted in elevated SDH activity following LC and...
HIF-1α+/+ and HIF-1α–/– mice were subjected to LC or GA (n = 6). (A–C) We employed qPCR to identify the presence of the SDHB gene expression (A) and Western blots by protein level (B and C) following GA. (D–F) We also measured the SDHB gene (D) and the protein expression through capillary Western blots after LC (E and F). The data for GAPDH, as shown in Figure 10B and B after GA and Figure 10E and E after LC, are identical due to the use of a single Western blot and the same samples before and after treatment with GA/LC. (G and H) The level of SDH activity was tested in HIF-1α+/+ and HIF-1α–/– mice (n = 3) that were exposed to acid aspiration (G) and LC (H). After analyzing the data, we used the unpaired t test with Welch’s correction to determine its statistical significance. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001.

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