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PDK4 Deficiency Suppresses Hepatic Glucagon Signaling by Decreasing cAMP Levels

Authors
Park, Bo-YoonJeon, Jae-HanGo, YounghoonHam, Hye JinKim, Jeong-EunYoo, Eun KyungKwon, Woong HeeJeoung, Nam-HoJeon, Yong HyunKoo, Seung-HoiKim, Byung-GyuHe, LingPark, Keun-GyuHarris, Robert A.Lee, In-Kyu
Issue Date
Oct-2018
Publisher
AMER DIABETES ASSOC
Citation
DIABETES, v.67, no.10, pp.2054 - 2068
Indexed
SCIE
SCOPUS
Journal Title
DIABETES
Volume
67
Number
10
Start Page
2054
End Page
2068
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/72578
DOI
10.2337/db17-1529
ISSN
0012-1797
Abstract
In fasting or diabetes, gluconeogenic genes are transcriptionally activated by glucagon stimulation of the cAMP-protein kinase A (PKA)-CREB signaling pathway. Previous work showed pyruvate dehydrogenase kinase (PDK) inhibition in skeletal muscle increases pyruvate oxidation, which limits the availability of gluconeogenic substrates in the liver. However, this study found upregulation of hepatic PDK4 promoted glucagon-mediated expression of gluconeogenic genes, whereas knockdown or inhibition of hepatic PDK4 caused the opposite effect on gluconeogenic gene expression and decreased hepatic glucose production. Mechanistically, PDK4 deficiency decreased ATP levels, thus increasing phosphorylated AMPK (p-AMPK), which increased p-AMPK-sensitive phosphorylation of cyclic nucleotide phosphodiesterase 4B (p-PDE4B). This reduced cAMP levels and consequently p-CREB. Metabolic flux analysis showed that the reduction in ATP was a consequence of a diminished rate of fatty acid oxidation (FAO). However, overexpression of PDK4 increased FAO and increased ATP levels, which decreased p-AMPK and p-PDE4B and allowed greater accumulation of cAMP and p-CREB. The latter were abrogated by the FAO inhibitor etomoxir, suggesting a critical role for PDK4 in FAO stimulation and the regulation of cAMP levels. This finding strengthens the possibility of PDK4 as a target against diabetes.
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