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RACK1 depletion in the ribosome induces selective translation for non-canonical autophagy.


ABSTRACT: RACK1, which was first demonstrated as a substrate of PKC? II, functions as a scaffold protein and associates with the 40S small ribosomal subunit. According to previous reports, ribosomal RACK1 was also suggested to control translation depending on the status in translating ribosome. We here show that RACK1 knockdown induces autophagy independent of upstream canonical factors such as Beclin1, Atg7 and Atg5/12 conjugates. We further report that RACK1 knockdown induces the association of mRNAs of LC3 and Bcl-xL with polysomes, indicating increased translation of these proteins. Therefore, we propose that the RACK1 depletion-induced autophagy is distinct from canonical autophagy. Finally, we confirm that cells expressing mutant RACK1 (RACK1R36D/K38E) defective in ribosome binding showed the same result as RACK1-knockdown cells. Altogether, our data clearly show that the depletion of ribosomal RACK1 alters the capacity of the ribosome to translate specific mRNAs, resulting in selective translation of mRNAs of genes for non-canonical autophagy induction.

SUBMITTER: Kim HD 

PROVIDER: S-EPMC5520723 | biostudies-literature | 2017 May

REPOSITORIES: biostudies-literature

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RACK1 depletion in the ribosome induces selective translation for non-canonical autophagy.

Kim Hag Dong HD   Kong EunBin E   Kim YongJoong Y   Chang Jin-Soo JS   Kim Joon J  

Cell death & disease 20170518 5


RACK1, which was first demonstrated as a substrate of PKCβ II, functions as a scaffold protein and associates with the 40S small ribosomal subunit. According to previous reports, ribosomal RACK1 was also suggested to control translation depending on the status in translating ribosome. We here show that RACK1 knockdown induces autophagy independent of upstream canonical factors such as Beclin1, Atg7 and Atg5/12 conjugates. We further report that RACK1 knockdown induces the association of mRNAs of  ...[more]

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