The next‐generation BET inhibitor, PLX51107, delays melanoma growth in a CD8‐mediated manner

Erkes, Dan A.; Field, Conroy O.; Capparelli, Claudia; Tiago, Manoela; Purwin, Timothy J.; Chervoneva, Inna; Berger, Adam C.; Hartsough, Edward J.; Villanueva, Jessie; Aplin, Andrew E.

doi:10.1111/pcmr.12788

Cited by 22 publications

(27 citation statements)

References 47 publications

(106 reference statements)

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“…BRDT inhibitors, including PLX51107 and INCB054329, have been demonstrated to suppress the progression of lung cancer cells, bladder cancer cells and intestinal cancer cells ( 24 , 25 ). The present study first analyzed the function of PLX51107 and INCB054329 on various RCC cell lines.…”

Section: Resultsmentioning

confidence: 99%

BRDT is a novel regulator of eIF4EBP1 in renal cell carcinoma

et al. 2020

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Among all types of kidney diseases, renal cell carcinoma (RCC) has the highest mortality, recurrence and metastasis rates, which results in high numbers of tumor-associated mortalities in China. Identifying a novel therapeutic target has attracted increasing attention. Bromodomain and extraterminal domain (BET) proteins have the ability to read the epigenome, leading to regulation of gene transcription. As an important member of the BET family, bromodomain testis-specific protein (BRDT) has been well studied; however, the mechanism underlying BRDT in the regulation of RCC has not been fully investigated. Eukaryotic translation initiation factor 4E-binding protein 1 (eIF4EBP1) is a binding partner of eIF4E that is involved in affecting the progression of various cancer types via regulating gene transcription. To identify novel regulators of eIF4EBP1, an immunoprecipitation assay and mass spectrometry analysis was performed in RCC cells. It was revealed that eIF4EBP1 interacted with BRDT, a novel interacting protein. In addition, the present study further demonstrated that BRDT inhibitors PLX51107 and INCB054329 blocked the progression of RCC cells, along with suppressing eIF4EBP1 and c-myc expression. Small interfering (si) RNAs were used to knock down BRDT expression, which suppressed RCC cell proliferation and eIF4EBP1 protein expression. In addition, overexpression of eIF4EBP1 partially abolished the inhibited growth function of PLX51107 but knocking down eIF4EBP1 improved the inhibitory effects of PLX51107. Furthermore, treatment with PLX51107 or knockdown of BRDT expression decreased c-myc expression at both the mRNA and protein levels, and attenuated its promoter activity, as determined by luciferase reporter assays. PLX51107 also significantly altered the interaction between the c-myc promoter with eIF4EBP1 and significantly attenuated the increase of RCC tumors, accompanied by decreased c-myc mRNA and protein levels in vivo . Taken together, these data suggested that blocking of BRDT by PLX51107, INCB054329 or BRDT knockdown suppressed the growth of RCC via decreasing eIF4EBP1, thereby leading to decreased c-myc transcription levels. Considering the regulatory function of BET proteins in gene transcription, the present study suggested that there is a novel mechanism underlying eIF4EBP1 regulation by BRDT, and subsequently decreased c-myc in RCC, and further identified a new approach by regulating eIF4EBP1 or c-myc for enhancing BRDT-targeting RCC therapy.

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Section: Resultsmentioning

confidence: 99%

BRDT is a novel regulator of eIF4EBP1 in renal cell carcinoma

et al. 2020

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“…Time course studies established that PLX51107 was present at ~1–2 µg/ml, and PLX3397 was present at ~20–60 µg/ml in the blood plasma of treated mice (Figure A). PLX51107 significantly increased CD8+ T cells in D4M3.A tumors during treatment, as previously demonstrated (Erkes et al, ), but did not alter the influx of CD8+ T cells in YUMM1.7 tumors (Figure B). We previously showed that expression of PD‐L1, a therapeutic target of BETi (Zhu et al, ), was decreased by PLX51107 treatment in D4M3.A tumors (Erkes et al, ), suggesting that BET inhibition is achieved in vivo .…”

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confidence: 98%

“…To analyze tumor‐infiltrating lymphocytes by flow cytometry, tumors were dissected and processed into single‐cell suspensions. Cells were stained with a fixable live/dead stain followed by surface antibody staining, as previously described (Erkes et al, ). Cells were surface stained with the following antibodies clones from Biolegend: CD45.2 (104), CD11c (N418), CD11b (M1/70), CD103 (2E7), F4/80 (BM8), CD3 (17A2), CD19 (6D5), CD206 (C068C2) I‐A/I‐E (M5/114.15.1), CD8α (53–6.7), and CSF‐1R (AFS98).…”

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confidence: 99%

“…After intradermal cell implantation, tumors were grown to ~50 mm 3 , and then, mice were fed either control or PLX51107‐laced chow. D4M3.A tumors displayed robust tumor growth delay with PLX51107 treatment, as previously described (Erkes et al, ) in contrast, YUMM1.7 tumors exhibited only modest growth delay (Figure a). Accordingly, PLX51107 prolonged animal survival by ~20 days, and only ~5 days in mice bearing D4M3.A and YUMM1.7 tumors, respectively (Figure b).…”

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“…We note that PLX3397 inhibits other tyrosine kinases besides CSF‐1R, such as cKIT, FLT3, and PDGFR‐ß, that may also contribute to the regulation of melanoma growth (Cannarile et al, ). PLX51107 can inhibit cancer cell growth in vitro; however, in vivo we observe additional effects on the tumor immune microenvironment (Erkes et al, ). Further investigation is required to thoroughly understand the effects of PLX51107 on diverse immune cell types within the tumor.…”

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PLX3397 inhibits the accumulation of intra‐tumoral macrophages and improves bromodomain and extra‐terminal inhibitor efficacy in melanoma

Erkes

Rosenbaum

Field

et al. 2019

Pigment Cell Melanoma Res

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Bromodomain and extra‐terminal inhibitors (BETi) delay tumor growth, in part, through tumor cell intrinsic alterations and initiation of anti‐tumor CD8+ T‐cell responses. By contrast, BETi effects on pro‐tumoral immune responses remain unclear. Here, we show that the next‐generation BETi, PLX51107, delayed tumor growth to differing degrees in Braf V600E melanoma syngeneic mouse models. These differential responses were associated with the influx of tumor‐associated macrophages during BETi treatment. Tumors that were poorly responsive to PLX51107 showed increased influx of colony‐stimulating factor‐1 receptor (CSF‐1R)‐positive tumor‐associated macrophages. We depleted CSF‐1R+ tumor‐associated macrophages with the CSF‐1R inhibitor, PLX3397, in combination with PLX51107. Treatment with PLX3397 enhanced the efficacy of PLX51107 in poorly responsive Braf V600E syngeneic melanomas in vivo. These findings suggest that tumor‐associated macrophage accumulation limits BETi efficacy and that co‐treatment with PLX3397 can improve response to PLX51107, offering a potential novel combination therapy for metastatic melanoma patients.

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Nanoparticle‐Mediated Tumor Microenvironment Remodeling Favors the Communication with the Immune Cells for Tumor Killing

Lucena‐Sánchez,

Hicke,

Clara‐Trujillo

et al. 2024

Advanced Therapeutics

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Melanoma is one of the most common types of skin cancer with a bad prognosis and limited treatment options, especially in advanced stages. Recently, immunotherapy has changed the landscape of oncology. Cancer cells can activate various mechanisms to suppress immune responses, such as the immunological checkpoint PD‐1/PD‐L1, whose blockage reactivates immune‐killing of melanoma cells. Moreover, exposure to inhibitory cytokines such as TGF‐β induces T regulatory cell differentiation, which promotes cancer immunosuppression. Current advances in this area have provided exciting outcomes in the clinical treatment of melanoma, however, there are still limitations, and a combination of several treatments is usually needed. Based on the above, inhibition of the TGF‐ β production and the PD‐1/PD‐L1 checkpoint might be a feasible strategy to increase T cell infiltration and cytotoxicity and thus overcome tumor immune escape. In this work, mesoporous silica nanoparticles (MSNs) loaded with a PD‐L1 inhibitor (JQ1) and capped with polyethyleneimine (PEI) and a siRNA targeting TGF‐β (TGF‐β siRNA) are reported. An efficient PD‐L1 downregulation and TGF‐β silencing are achieved using the nanoparticles, along with the promotion of cancer death in pre‐treated cells. This system demonstrates to be a specific and innovative therapeutic approach for the treatment of melanoma.This article is protected by copyright. All rights reserved

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The next‐generation BET inhibitor, PLX51107, delays melanoma growth in a CD8‐mediated manner

Cited by 22 publications

References 47 publications

BRDT is a novel regulator of eIF4EBP1 in renal cell carcinoma

BRDT is a novel regulator of eIF4EBP1 in renal cell carcinoma

PLX3397 inhibits the accumulation of intra‐tumoral macrophages and improves bromodomain and extra‐terminal inhibitor efficacy in melanoma

Nanoparticle‐Mediated Tumor Microenvironment Remodeling Favors the Communication with the Immune Cells for Tumor Killing

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