IRS1- Insuliinireseptorisubstanssi 1.
Lisätietoa:
IRS1 säätyy mm. Kelch proteiinien KLHL9, KLHL13, adaptorien ja CUL3
E-3-ubikitiiniligaasiekompleksin avulla ja kulkeutuu proteosomaaliseen
hajoitukseen ubikitinoituna.
Mutta ATG16L1 autofagiatekijä taas vähentää KLHL9 ja KLHL13 substraattiadaptoreita ja täten pääsee IRS1 toimimaan ja tehostamaan insuliinisignalointia.
Deficiency of the autophagy gene ATG16L1 induces insulin resistance through KLHL9/KLHL13/CUL3-mediated IRS1 degradation
Abstract
Connections between deficient autophagy and insulin resistance have emerged, however, the mechanism through which reduced
autophagy impairs insulin-signaling remains unknown. We examined mouse embryonic fibroblasts lacking Atg16l1
(ATG16L1 KO mouse embryonic fibroblasts (MEFs)), an essential autophagy
gene, and observed deficient insulin and insulin-like
growth factor-1 signaling. ATG16L1 KO MEFs
displayed reduced protein content of insulin receptor substrate-1
(IRS1), pivotal
to insulin signaling, whereas IRS1myc
overexpression recovered downstream insulin signaling. Endogenous IRS1
protein content
and insulin signaling were restored in ATG16L1 KO
mouse embryonic fibroblasts (MEF) upon proteasome inhibition. Through
proximity-dependent
biotin identification (BioID) and
co-immunoprecipitation, we found that Kelch-like proteins KLHL9 and
KLHL13, which together
form an E3 ubiquitin (Ub) ligase complex with
cullin 3 (CUL3), are novel IRS1 interactors. Expression of Klhl9 and Klhl13 was elevated in ATG16L1 KO MEFs and siRNA-mediated knockdown of Klhl9, Klhl13, or Cul3 recovered IRS1 expression. Moreover, Klhl13 and Cul3 knockdown increased insulin signaling. Notably, adipose tissue of high-fat fed mice displayed lower Atg16l1 mRNA expression and IRS1 protein content, and adipose tissue KLHL13 and CUL3 expression positively correlated to body mass index in humans. We propose that ATG16L1 deficiency evokes insulin resistance
through induction of Klhl9 and Klhl13, which, in complex with Cul3, promote proteasomal IRS1 degradation.
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