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hnRNP-K is a nuclear target of TCR-activated ERK and required for T-cell late activation. | LitMetric

hnRNP-K is a nuclear target of TCR-activated ERK and required for T-cell late activation.

Int Immunol

Department of Medicine, Immunotherapy Center, Medical College of Georgia, Augusta, GA 30912-2600, USA.

Published: December 2009

AI Article Synopsis

  • Sustained ERK signaling is crucial for T-cell IL-2 production, with specific downstream targets still being researched.
  • Proteomic analysis revealed that hnRNP-K is a key ERK target necessary for this process, as it interacts with various signaling proteins and is affected by TCR stimulation.
  • Knocking down hnRNP-K expression significantly decreased IL-2 production and increased proteolysis of Vav1, suggesting that ERK signaling helps maintain T-cell activation by preventing Vav1 degradation.

Article Abstract

Sustained extracellular signal-regulated kinase (ERK)-signaling plays a critical role in T-cell-mediated IL-2 production. Although many downstream targets are known for ERK, details remain unknown about which molecules play functional roles in IL-2 production. Here, we addressed this question using proteomic analysis of nuclear proteins from TCR-activated T cells and identified hnRNP-K as one of the ERK targets essential for IL-2 production. hnRNP-K was previously shown by others to be a direct substrate of ERK and form complexes with multiple signaling proteins as well as DNA and RNA. Our data showed a clear ERK-dependent increase in one form of hnRNP-K after TCR stimulation. Small interfering RNA-mediated gene knockdown of hnRNP-K expression abrogated IL-2 production by T cells. Moreover, reduction of hnRNP-K expression caused a notable increase in proteolysis of Vav1, a binding target of hnRNP-K. Since Vav1 is an essential molecule for T-cell activation, the data suggest that ERK signaling is required for T-cell activation partly by inhibiting activation-induced proteolysis of Vav1.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2779832PMC
http://dx.doi.org/10.1093/intimm/dxp106DOI Listing

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