Your search keyword '"Carannante V"' showing total 18 results

1. Livello di digitalizzazione della filiera turistica in Toscana

Author

Carannante, V., Coli, E., D’Acunto, D., Deri, M. G., Fantoni, G., Lemmi, E., Marchi, V., and Raschi, A

Subjects

digitalizzazione, turismo, industria 4.0

Published

2021

2. Single cell resolution analysis of ultrasound-produced multi-cellular tumor spheroids

Author

Olofsson, Karl, Carannante, V., Frisk, Thomas, Kushiro, K., Takai, M., Lundquist, A., Önfelt, Björn, Wiklund, Martin, Olofsson, Karl, Carannante, V., Frisk, Thomas, Kushiro, K., Takai, M., Lundquist, A., Önfelt, Björn, and Wiklund, Martin

Abstract

We have previously presented an ultrasonic standing wave (USW) 3D culture platform enabling parallel production, staining and processing of 100 uniformly sized multi-cellular tumor spheroids (MCTS) [1]. Here, we use the system for single cell resolution analysis of A498 renal carcinoma MCTS by off-chip fluorescence-activated cell sorting (FACS) and on-chip automatic image analysis methods based on 3D confocal microscopy images., QC 20230328

Published

2020

3. Acoustic formation of multicellular tumor spheroids enabling on-chip functional and structural imaging

Author

Olofsson, K., Carannante, V., Ohlin, Mathias, Frisk, T., Kushiro, K., Takai, M., Lundqvist, A., Önfelt, B., Wiklund, M., Olofsson, K., Carannante, V., Ohlin, Mathias, Frisk, T., Kushiro, K., Takai, M., Lundqvist, A., Önfelt, B., and Wiklund, M.

Abstract

Understanding the complex 3D tumor microenvironment is important in cancer research. This microenvironment can be modelled in vitro by culturing multicellular tumor spheroids (MCTS). Key challenges when using MCTS in applications such as high-throughput drug screening are overcoming imaging and analytical issues encountered during functional and structural investigations. To address these challenges, we use an ultrasonic standing wave (USW) based MCTS culture platform for parallel formation, staining and imaging of 100 whole MCTS. A protein repellent amphiphilic polymer coating enables flexible production of high quality and unanchored MCTS. This enables high-content multimode analysis based on flow cytometry and in situ optical microscopy. We use HepG2 hepatocellular carcinoma, A498 and ACHN renal carcinoma, and LUTC-2 thyroid carcinoma cell lines to demonstrate (i) the importance of the ultrasound-coating combination, (ii) bright field image based automatic characterization of MTCS, (iii) detailed deep tissue confocal imaging of whole MCTS mounted in a refractive index matching solution, and (iv) single cell functional analysis through flow cytometry of single cell suspensions of disintegrated MTCS. The USW MCTS culture platform is customizable and holds great potential for detailed multimode MCTS analysis in a high-content manner.

Published

2018

4. Acoustic formation of multicellular tumor spheroids enabling on-chip functional and structural imaging

Author

Olofsson, K., primary, Carannante, V., additional, Ohlin, M., additional, Frisk, T., additional, Kushiro, K., additional, Takai, M., additional, Lundqvist, A., additional, Önfelt, B., additional, and Wiklund, M., additional

Published

2018

5. Unanchored micro-tumors in an ultrasonic actuated multi-well microplate with protein repellent coating

Author

Olofsson, K., Carannante, V., Frisk, T., Kushiro, K., Takai, M., Önfelt, B., Wiklund, Martin, Olofsson, K., Carannante, V., Frisk, T., Kushiro, K., Takai, M., Önfelt, B., and Wiklund, Martin

Abstract

In this paper we demonstrate an improved tissue engineering method producing 100 three-dimensional (3D) HepG2 cell structures in parallel based on a combination of ultrasonic actuation and polymer coating in a multi-well microplate. By the use of a polymer coating in the plates, the method creates non-adherent tumor models of controlled size and shape which introduces both a more flexible 3D culture system as well as improved quality of the 3D tumor relative to previous studies [1]., Conference code: 126047; Export Date: 22 May 2017; Conference Paper. QC 20170607

Published

2016

6. IL-15, TIM-3 and NK cells subsets predict responsiveness to anti-CTLA-4 treatment in melanoma patients

Author

Domenico Mallardo, Elina Staaf, Antonio M. Grimaldi, Cinzia Garofalo, Rolf Kiessling, Sofia Johansson, Costanza Maria Cristiani, Paolo A. Ascierto, Elio Gulletta, Mariaelena Capone, Valentina Carannante, A. Anichini, Rosa Sottile, Eleonora Palella, Francesco Colucci, Yago Pico de Coaña, Klas Kärre, Gabriele Madonna, Gennaro Ciliberto, Ennio Carbone, Rossana Tallerico, Paolo Frumento, Ester Simeone, Maria Wolodarski, Colucci, Francesco [0000-0001-5193-6376], Apollo - University of Cambridge Repository, Tallerico, R, Cristiani, Cm, Staaf, E, Garofalo, C, Sottile, R, Capone, M, De Coana, Yp, Madonna, G, Palella, E, Wolodarski, M, Carannante, V, Mallardo, D, Simeone, E, Grimaldi, Am, Johansson, S, Frumento, P, Gulletta, E, Anichini, A, Colucci, F, Ciliberto, G, Kiessling, R, Kaerre, K, Ascierto, Pa, and Carbone, E

Subjects

lcsh:Immunologic diseases. Allergy, 0301 basic medicine, T cell, TIM-3, Immunology, NK cells, Biology, Anti-CTLA-4, lcsh:RC254-282, 03 medical and health sciences, Interleukin 21, 0302 clinical medicine, PD-1, medicine, melanoma, Immunology and Allergy, Original Research, Janus kinase 3, Melanoma, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, medicine.disease, Immune checkpoint, Blockade, 030104 developmental biology, medicine.anatomical_structure, Oncology, IL-15, Interleukin 15, 030220 oncology & carcinogenesis, Interleukin 12, lcsh:RC581-607

Abstract

Despite the success of immune checkpoint blockade in melanoma, the majority of patients do not respond. We hypothesized that the T and NK cell subset frequencies and expression levels of their receptors may predict responses and clinical outcome of anti-CTLA-4 treatment. We thus characterized the NK and T cell phenotype, as well as serum levels of several cytokines in 67 melanoma patients recruited in Italy and Sweden, using samples drawn prior to and during treatment. Survival correlated with low expression of the inhibitory receptor TIM-3 on circulating T and NK cells prior to and during treatment and with the increased frequency of mature circulating NK cells (defined as CD3(-)CD56(dim) CD16(+)) during treatment. Survival also correlated with low levels of IL-15 in the serum. Functional experiments in vitro demonstrated that sustained exposure to IL-15 enhanced the expression of PD-1 and TIM-3 on both T and NK cells, indicating a causative link between high IL-15 levels and enhanced expression of TIM-3 on these cells. Receptor blockade of TIM-3 improved NK cell-mediated elimination of melanoma metastasis cell lines in vitro. These observations may lead to the development of novel biomarkers to predict patient response to checkpoint blockade treatment. They also suggest that induction of additional checkpoints is a possibility that needs to be considered when treating melanoma patients with IL-15.

Published

2017

7. A thermoplastic chip for 2D and 3D correlative assays combining screening and high-resolution imaging of immune cell responses.

Author

van Ooijen H, Verron Q, Zhang H, Sandoz PA, Frisk TW, Carannante V, Olofsson K, Wagner AK, Sandström N, and Önfelt B

Subjects

Humans, Cell Culture Techniques methods, Cell Culture Techniques instrumentation, Tumor Microenvironment immunology, Single-Cell Analysis methods, Single-Cell Analysis instrumentation, Cell Line, Tumor, Imaging, Three-Dimensional methods, Cell Culture Techniques, Three Dimensional methods, Cell Culture Techniques, Three Dimensional instrumentation, Spheroids, Cellular immunology, Killer Cells, Natural immunology

Abstract

We present an easy-to-use, disposable, thermoplastic microwell chip designed to support screening and high-resolution imaging of single-cell behavior in two- and three-dimensional (2D and 3D) cell cultures. We show that the chip has excellent optical properties and provide simple protocols for efficient long-term cell culture of suspension and adherent cells, the latter grown either as monolayers or as hundreds of single, uniformly sized spheroids. We then demonstrate the applicability of the system for single-cell analysis by correlating the dynamic cytotoxic response of single immune cells grown under different metabolic conditions to their intracellular cytolytic load at the end of the assay. Additionally, we illustrate highly multiplex cytotoxicity screening of tumor spheroids in the chip, comparing the effect of environment cues characteristic of the tumor microenvironment on natural killer (NK)-cell-induced killing. Following the functional screening, we perform high-resolution 3D immunofluorescent imaging of infiltrating NK cells within the spheroid volumes., Competing Interests: Declaration of interests B.Ö. is a shareholder of Vycellix. B.Ö. and N.S. are investigating possibilities to make the chip available through commercialization., (Copyright © 2025 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2025

8. In vitro models to study natural killer cell dynamics in the tumor microenvironment.

Author

Carannante V, Wiklund M, and Önfelt B

Subjects

Humans, Killer Cells, Natural, Cell Culture Techniques, Immunotherapy, Tumor Microenvironment, Neoplasms therapy

Abstract

Immunotherapy is revolutionizing cancer therapy. The rapid development of new immunotherapeutic strategies to treat solid tumors is posing new challenges for preclinical research, demanding novel in vitro methods to test treatments. Such methods should meet specific requirements, such as enabling the evaluation of immune cell responses like cytotoxicity or cytokine release, and infiltration into the tumor microenvironment using cancer models representative of the original disease. They should allow high-throughput and high-content analysis, to evaluate the efficacy of treatments and understand immune-evasion processes to facilitate development of new therapeutic targets. Ideally, they should be suitable for personalized immunotherapy testing, providing information for patient stratification. Consequently, the application of in vitro 3-dimensional (3D) cell culture models, such as tumor spheroids and organoids, is rapidly expanding in the immunotherapeutic field, coupled with the development of novel imaging-based techniques and -omic analysis. In this paper, we review the recent advances in the development of in vitro 3D platforms applied to natural killer (NK) cell-based cancer immunotherapy studies, highlighting the benefits and limitations of the current methods, and discuss new concepts and future directions of the field., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2023 Carannante, Wiklund and Önfelt.)

Published

2023

9. Generation of tumor spheroids in microwells to study NK cell cytotoxicity, infiltration and phenotype.

Author

Carannante V, Sandström N, Olofsson K, Van Ooijen H, Hell B, Wiklund M, and Önfelt B

Subjects

Humans, Cell Culture Techniques methods, Phenotype, Killer Cells, Natural, Spheroids, Cellular, Neoplasms

Abstract

The development of new immunotherapeutic drugs and combinatorial strategies requires the implementation of novel methods to test their efficacy in vitro. Here, we present a series of miniaturized in vitro assays to assess immune cell cytotoxic activity, infiltration, and phenotype in renal carcinoma spheroids with the use of a recently developed multichambered microwell chip. We provide protocols for tumor spheroid formation, NK cell culture, fluorescence labelling and imaging of live or fixed cells directly in the chip together with data analysis., (Copyright © 2023 Elsevier Inc. All rights reserved.)

Published

2023

10. Targeting myeloid suppressive cells revives cytotoxic anti-tumor responses in pancreatic cancer.

Author

Sarhan D, Eisinger S, He F, Bergsland M, Pelicano C, Driescher C, Westberg K, Benitez II, Humoud R, Palano G, Li S, Carannante V, Muhr J, Önfelt B, Schlisio S, Ravetch JV, Heuchel R, Löhr MJ, and Karlsson MCI

Abstract

Immunotherapy for cancer that aims to promote T cell anti-tumor activity has changed current clinical practice, where some previously lethal cancers have now become treatable. However, clinical trials with low response rates have been disappointing for pancreatic ductal adenocarcinoma (PDAC). One suggested explanation is the accumulation of dominantly immunosuppressive tumor-associated macrophages and myeloid-derived suppressor cells in the tumor microenvironment (TME). Using retrospectively collected tumor specimens and transcriptomic data from PDAC, we demonstrate that expression of the scavenger receptor MARCO correlates with poor prognosis and a lymphocyte-excluding tumor phenotype. PDAC cell lines produce IL-10 and induce high expression of MARCO in myeloid cells, and this was further enhanced during hypoxic conditions. These myeloid cells suppressed effector T and natural killer (NK) cells and blocked NK cell tumor infiltration and tumor killing in a PDAC 3D-spheroid model. Anti-human MARCO (anti-hMARCO) antibody targeting triggered the repolarization of tumor-associated macrophages and activated the inflammasome machinery, resulting in IL-18 production. This in turn enhanced T cell and NK cell functions. The targeting of MARCO thus remodels the TME and represents a rational approach to make immunotherapy more efficient in PDAC patients., Competing Interests: The authors have no financial or other competing interests., (© 2022 The Authors.)

Published

2022

11. Miniaturized and multiplexed high-content screening of drug and immune sensitivity in a multichambered microwell chip.

Author

Sandström N, Carannante V, Olofsson K, Sandoz PA, Moussaud-Lamodière EL, Seashore-Ludlow B, Van Ooijen H, Verron Q, Frisk T, Takai M, Wiklund M, Östling P, and Önfelt B

Subjects

Humans, Cell Culture Techniques, Spheroids, Cellular, Carcinoma, Non-Small-Cell Lung, Lung Neoplasms, Antineoplastic Agents

Abstract

Here, we present a methodology based on multiplexed fluorescence screening of two- or three-dimensional cell cultures in a newly designed multichambered microwell chip, allowing direct assessment of drug or immune cell cytotoxic efficacy. We establish a framework for cell culture, formation of tumor spheroids, fluorescence labeling, and imaging of fixed or live cells at various magnifications directly in the chip together with data analysis and interpretation. The methodology is demonstrated by drug cytotoxicity screening using ovarian and non-small cell lung cancer cells and by cellular cytotoxicity screening targeting tumor spheroids of renal carcinoma and ovarian carcinoma with natural killer cells from healthy donors. The miniaturized format allowing long-term cell culture, efficient screening, and high-quality imaging of small sample volumes makes this methodology promising for individualized cytotoxicity tests for precision medicine., Competing Interests: B.Ö. is a consultant, has ownership in Vycellix, and receives research funding from Affimed., (© 2022 The Authors.)

Published

2022

12. A 2B adenosine receptor antagonists rescue lymphocyte activity in adenosine-producing patient-derived cancer models.

Author

Tay AHM, Prieto-Díaz R, Neo S, Tong L, Chen X, Carannante V, Önfelt B, Hartman J, Haglund F, Majellaro M, Azuaje J, Garcia-Mera X, Brea JM, Loza MI, Jespers W, Gutierrez-de-Teran H, Sotelo E, and Lundqvist A

Subjects

Adenosine pharmacology, Humans, Lymphocytes metabolism, Receptor, Adenosine A2B genetics, Receptor, Adenosine A2B metabolism, Neoplasms drug therapy, Purinergic P1 Receptor Antagonists

Abstract

Background: Adenosine is a metabolite that suppresses antitumor immune response of T and NK cells via extracellular binding to the two subtypes of adenosine-2 receptors, A 2 ARs. While blockade of the A 2A ARs subtype effectively rescues lymphocyte activity, with four A 2A AR antagonists currently in anticancer clinical trials, less is known for the therapeutic potential of the other A 2B AR blockade within cancer immunotherapy. Recent studies suggest the formation of A 2A AR/A 2B AR dimers in tissues that coexpress the two receptor subtypes, where the A 2B AR plays a dominant role, suggesting it as a promising target for cancer immunotherapy., Methods: We report the synthesis and functional evaluation of five potent A 2B AR antagonists and a dual A 2A AR/A 2B AR antagonist. The compounds were designed using previous pharmacological data assisted by modeling studies. Synthesis was developed using multicomponent approaches. Flow cytometry was used to evaluate the phenotype of T and NK cells on A 2B AR antagonist treatment. Functional activity of T and NK cells was tested in patient-derived tumor spheroid models., Results: We provide data for six novel small molecules: five A 2B AR selective antagonists and a dual A 2A AR/A 2B AR antagonist. The growth of patient-derived breast cancer spheroids is prevented when treated with A 2B AR antagonists. To elucidate if this depends on increased lymphocyte activity, immune cells proliferation, and cytokine production, lymphocyte infiltration was evaluated and compared with the potent A 2A AR antagonist AZD-4635. We find that A 2B AR antagonists rescue T and NK cell proliferation, IFNγ and perforin production, and increase tumor infiltrating lymphocytes infiltration into tumor spheroids without altering the expression of adhesion molecules., Conclusions: Our results demonstrate that A 2B AR is a promising target in immunotherapy, identifying ISAM-R56A as the most potent candidate for A 2B AR blockade. Inhibition of A 2B AR signaling restores T cell function and proliferation. Furthermore, A 2B AR and dual A 2A AR/A 2B AR antagonists showed similar or better results than A 2A AR antagonist AZD-4635 reinforcing the idea of dominant role of the A 2B AR in the regulation of the immune system., Competing Interests: Competing interests: None declared, (© Author(s) (or their employer(s)) 2022. Re-use permitted under CC BY. Published by BMJ.)

Published

2022

13. Single cell organization and cell cycle characterization of DNA stained multicellular tumor spheroids.

Author

Olofsson K, Carannante V, Takai M, Önfelt B, and Wiklund M

Subjects

Carcinoma, Renal Cell metabolism, Cell Culture Techniques methods, Cell Line, Tumor, Cell Nucleus metabolism, DNA metabolism, Humans, Microscopy, Confocal methods, Sonication methods, Spheroids, Cellular cytology, Tumor Cells, Cultured, Cell Cycle, Spheroids, Cellular metabolism

Abstract

Multicellular tumor spheroids (MCTSs) can serve as in vitro models for solid tumors and have become widely used in basic cancer research and drug screening applications. The major challenges when studying MCTSs by optical microscopy are imaging and analysis due to light scattering within the 3-dimensional structure. Herein, we used an ultrasound-based MCTS culture platform, where A498 renal carcinoma MCTSs were cultured, DAPI stained, optically cleared and imaged, to connect nuclear segmentation to biological information at the single cell level. We show that DNA-content analysis can be used to classify the cell cycle state as a function of position within the MCTSs. We also used nuclear volumetric characterization to show that cells were more densely organized and perpendicularly aligned to the MCTS radius in MCTSs cultured for 96 h compared to 24 h. The method presented herein can in principle be used with any stochiometric DNA staining protocol and nuclear segmentation strategy. Since it is based on a single counter stain a large part of the fluorescence spectrum is free for other probes, allowing measurements that correlate cell cycle state and nuclear organization with e.g., protein expression or drug distribution within MCTSs., (© 2021. The Author(s).)

Published

2021

14. Ultrasound-Based Scaffold-Free Core-Shell Multicellular Tumor Spheroid Formation.

Author

Olofsson K, Carannante V, Takai M, Önfelt B, and Wiklund M

Abstract

In cancer research and drug screening, multicellular tumor spheroids (MCTSs) are a popular model to bridge the gap between in vitro and in vivo. However, the current techniques to culture mixed co-culture MCTSs do not mimic the structural architecture and cellular spatial distribution in solid tumors. In this study we present an acoustic trapping-based core-shell MCTSs culture method using sequential seeding of the core and shell cells into microwells coated with a protein repellent coating. Scaffold-free core-shell ovarian cancer OVCAR-8 cell line MCTSs were cultured, stained, cleared and confocally imaged on-chip. Image analysis techniques were used to quantify the shell thickness (23.2 ± 1.8 µm) and shell coverage percentage (91.2 ± 2.8%). We also show that the shell thickness was evenly distributed over the MCTS cores with the exception of being slightly thinner close to the microwell bottom. This scaffold-free core-shell MCTSs formation technique and the analysis tools presented herein could be used as an internal migration assay within the MCTS or to form core-shell MCTS co-cultures to study therapy response or the interaction between tumor and stromal cells.

Published

2021

15. Soluble and Exosome-Bound α-Galactosylceramide Mediate Preferential Proliferation of Educated NK Cells with Increased Anti-Tumor Capacity.

Author

Wagner AK, Gehrmann U, Hiltbrunner S, Carannante V, Luu TT, Näslund TI, Brauner H, Kadri N, Kärre K, and Gabrielsson S

Abstract

Natural killer (NK) cells can kill target cells via the recognition of stress molecules and down-regulation of major histocompatibility complex class I (MHC-I). Some NK cells are educated to recognize and kill cells that have lost their MHC-I expression, e.g., tumor or virus-infected cells. A desired property of cancer immunotherapy is, therefore, to activate educated NK cells during anti-tumor responses in vivo. We here analyze NK cell responses to α-galactosylceramide (αGC), a potent activator of invariant NKT (iNKT) cells, or to exosomes loaded with αGC. In mouse strains which express different MHC-I alleles using an extended NK cell flow cytometry panel, we show that αGC induces a biased NK cell proliferation of educated NK cells. Importantly, iNKT cell-induced activation of NK cells selectively increased in vivo missing self-responses, leading to more effective rejection of tumor cells. Exosomes from antigen-presenting cells are attractive anti-cancer therapy tools as they may induce both innate and adaptive immune responses, thereby addressing the hurdle of tumor heterogeneity. Adding αGC to antigen-loaded dendritic-cell-derived exosomes also led to an increase in missing self-responses in addition to boosted T and B cell responses. This study manifests αGC as an attractive adjuvant in cancer immunotherapy, as it increases the functional capacity of educated NK cells and enhances the innate, missing self-based antitumor response.

Published

2021

16. High-Resolution Imaging of Tumor Spheroids and Organoids Enabled by Expansion Microscopy.

Author

Edwards SJ, Carannante V, Kuhnigk K, Ring H, Tararuk T, Hallböök F, Blom H, Önfelt B, and Brismar H

Abstract

Three-dimensional cell cultures are able to better mimic the physiology and cellular environments found in tissues in vivo compared to cells grown in two dimensions. In order to study the structure and function of cells in 3-D cultures, light microscopy is frequently used. The preparation of 3-D cell cultures for light microscopy is often destructive, including physical sectioning of the samples, which can result in the loss of 3-D information. In order to probe the structure of 3-D cell cultures at high resolution, we have explored the use of expansion microscopy and compared it to a simple immersion clearing protocol. We provide a practical method for the study of spheroids, organoids and tumor-infiltrating immune cells at high resolution without the loss of spatial organization. Expanded samples are highly transparent, enabling high-resolution imaging over extended volumes by significantly reducing light scatter and absorption. In addition, the hydrogel-like nature of expanded samples enables homogenous antibody labeling of dense epitopes throughout the sample volume. The improved labeling and image quality achieved in expanded samples revealed details in the center of the organoid which were previously only observable following serial sectioning. In comparison to chemically cleared spheroids, the improved signal-to-background ratio of expanded samples greatly improved subsequent methods for image segmentation and analysis., (Copyright © 2020 Edwards, Carannante, Kuhnigk, Ring, Tararuk, Hallböök, Blom, Önfelt and Brismar.)

Published

2020

17. Laboratory cryo x-ray microscopy for 3D cell imaging.

Author

Fogelqvist E, Kördel M, Carannante V, Önfelt B, and Hertz HM

Subjects

Cytoplasmic Vesicles ultrastructure, HEK293 Cells, Humans, Cryoelectron Microscopy methods, Electron Probe Microanalysis methods, Imaging, Three-Dimensional methods

Abstract

Water-window x-ray microscopy allows two- and three-dimensional (2D and 3D) imaging of intact unstained cells in their cryofixed near-native state with unique contrast and high resolution. Present operational biological water-window microscopes are based at synchrotron facilities, which limits their accessibility and integration with complementary methods. Laboratory-source microscopes have had difficulty addressing relevant biological tasks with proper resolution and contrast due to long exposure times and limited up-time. Here we report on laboratory cryo x-ray microscopy with the exposure time, contrast, and reliability to allow for routine high-spatial resolution 3D imaging of intact cells and cell-cell interactions. Stabilization of the laser-plasma source combined with new optics and sample preparation provide high-resolution cell imaging, both in 2D with ten-second exposures and in 3D with twenty-minute tomography. Examples include monitoring of the distribution of carbon-dense vesicles in starving HEK293T cells and imaging the interaction between natural killer cells and target cells.

Published

2017

18. IL-15, TIM-3 and NK cells subsets predict responsiveness to anti-CTLA-4 treatment in melanoma patients.

Author

Tallerico R, Cristiani CM, Staaf E, Garofalo C, Sottile R, Capone M, Pico de Coaña Y, Madonna G, Palella E, Wolodarski M, Carannante V, Mallardo D, Simeone E, Grimaldi AM, Johansson S, Frumento P, Gulletta E, Anichini A, Colucci F, Ciliberto G, Kiessling R, Kärre K, Ascierto PA, and Carbone E

Abstract

Despite the success of immune checkpoint blockade in melanoma, the majority of patients do not respond. We hypothesized that the T and NK cell subset frequencies and expression levels of their receptors may predict responses and clinical outcome of anti-CTLA-4 treatment. We thus characterized the NK and T cell phenotype, as well as serum levels of several cytokines in 67 melanoma patients recruited in Italy and Sweden, using samples drawn prior to and during treatment. Survival correlated with low expression of the inhibitory receptor TIM-3 on circulating T and NK cells prior to and during treatment and with the increased frequency of mature circulating NK cells (defined as CD3 - CD56 dim CD16 + ) during treatment. Survival also correlated with low levels of IL-15 in the serum. Functional experiments in vitro demonstrated that sustained exposure to IL-15 enhanced the expression of PD-1 and TIM-3 on both T and NK cells, indicating a causative link between high IL-15 levels and enhanced expression of TIM-3 on these cells. Receptor blockade of TIM-3 improved NK cell-mediated elimination of melanoma metastasis cell lines in vitro . These observations may lead to the development of novel biomarkers to predict patient response to checkpoint blockade treatment. They also suggest that induction of additional checkpoints is a possibility that needs to be considered when treating melanoma patients with IL-15.

Published

2016