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ADAR1 expression is associated with cervical cancer progression and negatively regulates NK cell activity
Valentina Tassinari, Marta Kaciulis, Stefano Petrai, Helena Stabile, Angelina Pernazza, Martina Leopizzi, Valeria Di Maio, Francesca Belleudi, Danilo Ranieri, Vanessa Mancini, Innocenza Palaia, Federica Tanzi, Ludovica Lospinoso Severini, Silvia Ruggeri, Maria Emanuela Greco, Giovanni Bernardini, Alessandra Zingoni, Marco Cippitelli, Cristina Cerboni, Alessandra Soriani
Valentina Tassinari, Marta Kaciulis, Stefano Petrai, Helena Stabile, Angelina Pernazza, Martina Leopizzi, Valeria Di Maio, Francesca Belleudi, Danilo Ranieri, Vanessa Mancini, Innocenza Palaia, Federica Tanzi, Ludovica Lospinoso Severini, Silvia Ruggeri, Maria Emanuela Greco, Giovanni Bernardini, Alessandra Zingoni, Marco Cippitelli, Cristina Cerboni, Alessandra Soriani
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Research Article Immunology Inflammation Oncology

ADAR1 expression is associated with cervical cancer progression and negatively regulates NK cell activity

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Abstract

ADAR1 edits double-stranded RNAs (dsRNAs) by deaminating adenosines into inosines, preventing aberrant activation of innate immunity by endogenous dsRNAs, which may resemble viral structures. Several tumors exploit ADAR1 to evade immune surveillance; indeed, its deletion reduces tumor viability and reshapes infiltrating leukocytes. Here we investigated the role of ADAR1 in immune evasion mechanisms during cervical cancer (CC) progression. Patients’ biopsy samples showed higher ADAR1 expression already in premalignant lesions (squamous intraepithelial lesions [SIL]) and a substantially reduced percentage of infiltrating CD7+ innate cells in in situ and invasive carcinomas compared with normal mucosa, with CD56+ NK cells showing phenotypic alterations that may have affected their functional responses. In CC-derived cell lines (SiHa, CaSki), ADAR1 silencing reduced cell proliferation, an effect further enhanced by exogenous IFN-β administration. It also induced proinflammatory gene expression, as demonstrated by RNA-Seq analysis, and conditioned supernatants collected from these cells activated several NK cell effector functions. NK cell infiltration and activation were also confirmed in organotypic 3D tissue models of SiHa cells knocked out for ADAR1. In conclusion, ADAR1 expression increased with CC progression and was accompanied by alterations in tumor-infiltrating NK cells, but its silencing in CC-derived cell lines potentiated antitumor NK cell activities. Thus, ADAR1 inhibition may represent a therapeutic perspective for CC and possibly other malignancies.

Authors

Valentina Tassinari, Marta Kaciulis, Stefano Petrai, Helena Stabile, Angelina Pernazza, Martina Leopizzi, Valeria Di Maio, Francesca Belleudi, Danilo Ranieri, Vanessa Mancini, Innocenza Palaia, Federica Tanzi, Ludovica Lospinoso Severini, Silvia Ruggeri, Maria Emanuela Greco, Giovanni Bernardini, Alessandra Zingoni, Marco Cippitelli, Cristina Cerboni, Alessandra Soriani

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Figure 6

ADAR1 inhibition enhances NK cell functions.

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ADAR1 inhibition enhances NK cell functions.
Conditioned media (CM) from...
Conditioned media (CM) from siCtr– and siADAR1-transfected SiHa and CaSki cells were harvested after 72 hours and used in different assays. (A) CM from SiHa and CaSki cells was incubated for the indicated time points with purified NK cells isolated from healthy donors. Proliferation was measured by Incucyte Live-Cell Analysis and analyzed with Incucyte Zoom software. Proliferation index was calculated as fold change by setting Nuclight-positive NK cells at scan 0 (T0) as 1 (A.I.). Pooled data are from 3 independent experiments with NK cells from 7 different donors. (B) NK cell degranulation was evaluated by FACS using the lysosomal marker CD107a. Purified NK cells were used as effectors and treated with CM from SiHa or CaSki cells for 18 hours and then cocultured with SiHa (left panel) or K562 (middle and right panels) cells, used as targets (E/T ratio of 1:2). CD107a expression was evaluated on NK cells gated as CD56+. Pooled data are from 3 independent experiments with NK cells from 6 (target SiHa) or 7 (target K562) different donors. (C) Migration of cultured (cNK) or primary (pNK) purified NK cells was measured using a Transwell migration chamber. As chemoattractant, SiHa and CaSki CM was added to the lower compartment, and after 2–4 hours at 37°C, the migrated cells were counted using BD FACSCanto. Pooled data are from at least 2 independent experiments with 7 different donors. All data are expressed as mean ± SEM. Statistical analysis was performed by paired t test. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001.

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