Dinaciclib induces immunogenic cell death and enhances anti-PD1–mediated tumor suppression
Dewan Md Sakib Hossain, Sarah Javaid, Mingmei Cai, Chunsheng Zhang, Anandi Sawant, Marlene Hinton, Manjiri Sathe, Jeff Grein, Wendy Blumenschein, Elaine M. Pinheiro, Alissa Chackerian
Dewan Md Sakib Hossain, Sarah Javaid, Mingmei Cai, Chunsheng Zhang, Anandi Sawant, Marlene Hinton, Manjiri Sathe, Jeff Grein, Wendy Blumenschein, Elaine M. Pinheiro, Alissa Chackerian
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Research Article Oncology

Dinaciclib induces immunogenic cell death and enhances anti-PD1–mediated tumor suppression

Abstract

Blockade of the checkpoint inhibitor programmed death 1 (PD1) has demonstrated remarkable success in the clinic for the treatment of cancer; however, a majority of tumors are resistant to anti-PD1 monotherapy. Numerous ongoing clinical combination therapy studies will likely reveal additional therapeutics that complement anti-PD1 blockade. Recent studies found that immunogenic cell death (ICD) improves T cell responses against different tumors, thus indicating that ICD may further augment antitumor immunity elicited by anti-PD1. Here, we observed antitumor activity following combinatorial therapy with anti-PD1 Ab and the cyclin-dependent kinase inhibitor dinaciclib in immunocompetent mouse tumor models. Dinaciclib induced a type I IFN gene signature within the tumor, leading us to hypothesize that dinaciclib potentiates the effects of anti-PD1 by eliciting ICD. Indeed, tumor cells treated with dinaciclib showed the hallmarks of ICD including surface calreticulin expression and release of high mobility group box 1 (HMGB1) and ATP. Mice treated with both anti-PD1 and dinaciclib showed increased T cell infiltration and DC activation within the tumor, indicating that this combination improves the overall quality of the immune response generated. These findings identify a potential mechanism for the observed benefit of combining dinaciclib and anti-PD1, in which dinaciclib induces ICD, thereby converting the tumor cell into an endogenous vaccine and boosting the effects of anti-PD1.

Authors

Dewan Md Sakib Hossain, Sarah Javaid, Mingmei Cai, Chunsheng Zhang, Anandi Sawant, Marlene Hinton, Manjiri Sathe, Jeff Grein, Wendy Blumenschein, Elaine M. Pinheiro, Alissa Chackerian

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Figure 5

Dinaciclib-treated tumor cells enhance DC function.

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Dinaciclib-treated tumor cells enhance DC function. DiO-labeled CT26 cel...
DiO-labeled CT26 cells were treated with the indicated concentrations of dinaciclib for 24 hours and then cocultured with BMDCs for an additional 24 hours. (A) The percentage of CD11c+ DCs with engulfed tumor cells was assessed by flow cytometry, as was the expression of (B) MHCII, (C) CD86, and (D) CD80 on CD11c+ DCs after coculture. (E) Secretion of IL-1β into the coculture supernatant was determined by MSD assay. Data represent the mean value ± SEM of 3 to 4 replicates from 1 representative experiment. ***P < 0.001, **P < 0.01, and *P < 0.05, for comparisons between individual dinaciclib dose groups and the untreated group (0 μM). Statistical data obtained via 1-way ANOVA with Bonferroni post-test.