Targeting pleckstrin-2/Akt signaling reduces proliferation in myeloproliferative neoplasm models
Xu Han, Yang Mei, Rama K. Mishra, Honghao Bi, Atul D. Jain, Gary E. Schiltz, Baobing Zhao, Madina Sukhanova, Pan Wang, Arabela A. Grigorescu, Patricia C. Weber, John J. Piwinski, Miguel A. Prado, Joao A. Paulo, Len Stephens, Karen E. Anderson, Charles S. Abrams, Jing Yang, Peng Ji
Xu Han, Yang Mei, Rama K. Mishra, Honghao Bi, Atul D. Jain, Gary E. Schiltz, Baobing Zhao, Madina Sukhanova, Pan Wang, Arabela A. Grigorescu, Patricia C. Weber, John J. Piwinski, Miguel A. Prado, Joao A. Paulo, Len Stephens, Karen E. Anderson, Charles S. Abrams, Jing Yang, Peng Ji
View: Text | PDF
Research Article Hematology Oncology

Targeting pleckstrin-2/Akt signaling reduces proliferation in myeloproliferative neoplasm models

Abstract

Myeloproliferative neoplasms (MPNs) are characterized by the activated JAK2/STAT pathway. Pleckstrin-2 (Plek2) is a downstream target of the JAK2/STAT5 pathway and is overexpressed in patients with MPNs. We previously revealed that Plek2 plays critical roles in the pathogenesis of JAK2-mutated MPNs. The nonessential roles of Plek2 under physiologic conditions make it an ideal target for MPN therapy. Here, we identified first-in-class Plek2 inhibitors through an in silico high-throughput screening approach and cell-based assays, followed by the synthesis of analogs. Plek2-specific small-molecule inhibitors showed potent inhibitory effects on cell proliferation. Mechanistically, Plek2 interacts with and enhances the activity of Akt through the recruitment of downstream effector proteins. The Plek2-signaling complex also includes Hsp72, which protects Akt from degradation. These functions were blocked by Plek2 inhibitors via their direct binding to the Plek2 dishevelled, Egl-10 and pleckstrin (DEP) domain. The role of Plek2 in activating Akt signaling was further confirmed in vivo using a hematopoietic-specific Pten-knockout mouse model. We next tested Plek2 inhibitors alone or in combination with an Akt inhibitor in various MPN mouse models, which showed significant therapeutic efficacies similar to that seen with the genetic depletion of Plek2. The Plek2 inhibitor was also effective in reducing proliferation of CD34-positive cells from MPN patients. Our studies reveal a Plek2/Akt complex that drives cell proliferation and can be targeted by a class of antiproliferative compounds for MPN therapy.

Authors

Xu Han, Yang Mei, Rama K. Mishra, Honghao Bi, Atul D. Jain, Gary E. Schiltz, Baobing Zhao, Madina Sukhanova, Pan Wang, Arabela A. Grigorescu, Patricia C. Weber, John J. Piwinski, Miguel A. Prado, Joao A. Paulo, Len Stephens, Karen E. Anderson, Charles S. Abrams, Jing Yang, Peng Ji

×

Figure 3

Plek2 activates Akt and protects Akt through Hsp72.

Options: View larger image (or click on image) Download as PowerPoint
Plek2 activates Akt and protects Akt through Hsp72. (A) IP of anti-HA wi...
(A) IP of anti-HA with cell lysate from 293T cells transfected with HA-Plek2, followed by Western blot assays of indicated proteins. (B) Western blotting assays of indicated proteins from Cos-7 cells transfected with HA-Plek2. (C) Quantitative PCR analysis of AKT from Cos-7 cells transfected with HA-Plek2. (D) Western blotting assays of indicated proteins from HEL cells transfected with Flag-Plek2. (E) GST pull-down assay using GST or GST-Plek2 with a recombinant Akt. Akt was detected by a Western blotting assay. GST and GST-Plek2 were revealed using Coomassie stain. (F) Same as E, except GST-Plek2 DEP was used. (G) GST pull-down assay of GST or GST-Plek2 incubated with cell lysis from 293T cells. Indicated proteins were detected by Western blotting. (H) Bead-conjugated streptavidin pull-down of 293T cells transfected with BirA-Plek2 and incubated with biotin (50 μM). A Western blotting assay of the indicated proteins was performed after SDS-PAGE. (I) Western blotting analyses of the indicated proteins in 293T cells transfected with GFP fusion Hsp72 and HA-GST-Akt. (J) IP of Flag tag with cell lysate from 293T cells transfected with Flag-Plek2 followed by a Western blotting assay of indicated proteins.