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1. Evaluation of sted super-resolution image quality by image correlation spectroscopy (QuICS)

Author

Elena Cerutti, Morgana D’Amico, Isotta Cainero, Gaetano Ivan Dellino, Mario Faretta, Giuseppe Vicidomini, Pier Giuseppe Pelicci, Paolo Bianchini, Alberto Diaspro, and Luca Lanzanò

Subjects
Medicine, Science
Abstract

Abstract Quantifying the imaging performances in an unbiased way is of outmost importance in super-resolution microscopy. Here, we describe an algorithm based on image correlation spectroscopy (ICS) that can be used to assess the quality of super-resolution images. The algorithm is based on the calculation of an autocorrelation function and provides three different parameters: the width of the autocorrelation function, related to the spatial resolution; the brightness, related to the image contrast; the relative noise variance, related to the signal-to-noise ratio of the image. We use this algorithm to evaluate the quality of stimulated emission depletion (STED) images of DNA replication foci in U937 cells acquired under different imaging conditions. Increasing the STED depletion power improves the resolution but may reduce the image contrast. Increasing the number of line averages improves the signal-to-noise ratio but facilitates the onset of photobleaching and subsequent reduction of the image contrast. Finally, we evaluate the performances of two different separation of photons by lifetime tuning (SPLIT) approaches: the method of tunable STED depletion power and the commercially available Leica Tau-STED. We find that SPLIT provides an efficient way to improve the resolution and contrast in STED microscopy.

Published
2021
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4. Light-sheet confined super-resolution using two-photon photoactivation.

Author

Francesca Cella Zanacchi, Zeno Lavagnino, Mario Faretta, Laura Furia, and Alberto Diaspro

Subjects
Medicine, Science
Abstract

Light-sheet microscopy is a useful tool for performing biological investigations of thick samples and it has recently been demonstrated that it can also act as a suitable architecture for super-resolution imaging of thick biological samples by means of individual molecule localization. However, imaging in depth is still limited since it suffers from a reduction in image quality caused by scattering effects. This paper sets out to investigate the advantages of non-linear photoactivation implemented in a selective plane illumination configuration when imaging scattering samples. In particular, two-photon excitation is proven to improve imaging capabilities in terms of imaging depth and is expected to reduce light-sample interactions and sample photo-damage. Here, two-photon photoactivation is coupled to individual molecule localization methods based on light-sheet illumination (IML-SPIM), allowing super-resolution imaging of nuclear pH2AX in NB4 cells.

Published
2013
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5. Antibodies validated for routinely processed tissues stain frozen sections unpredictably

Author

Mario Faretta, Giorgio Cattoretti, Maddalena Maria Bolognesi, Francesca Maria Bosisio, Francesco Mascadri, Laura Furia, Bolognesi, M, Mascadri, F, Furia, L, Faretta, M, Bosisio, F, and Cattoretti, G

Subjects
0301 basic medicine, Biochemistry & Molecular Biology, Pathology, medicine.medical_specialty, Tissue Fixation, Biology, Stain, Biochemical Research Methods, General Biochemistry, Genetics and Molecular Biology, Epitope, Fixatives, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Formaldehyde, medicine, Frozen Sections, antigen retrieval, antibody validation, Coloring Agents, paratope, mazze di tamburo, epitope, Frozen section procedure, Paraffin Embedding, Science & Technology, fixatives, Antibodies, Monoclonal, Reproducibility of Results, Antibody validation • antigen retrieval • epitope • fixatives • frozen sections • paratope, 030104 developmental biology, Antigen retrieval, chemistry, frozen sections, 030220 oncology & carcinogenesis, biology.protein, Paratope, Tissue staining, Antibody, Life Sciences & Biomedicine, Biotechnology
Abstract

Background: Antibody validation for tissue staining is required for reproducibility; criteria to ensure validity have been published recently. The majority of these recommendations imply the use of routinely processed (formalin-fixed, paraffin-embedded) tissue. Materials & methods: We applied to lightly fixed frozen sections a panel of 126 antibodies validated for formalin-fixed, paraffin-embedded tissue with extended criteria. Results: Less than 30% of the antibodies performed as expected with all fixations. 35% preferred one fixation over another, 13% gave nonspecific staining and 23% did not stain at all. Conclusion: Individual antibody variability of the paratope's fitness for the fixed antigen may be the cause. Revalidation of established antibody panels is required when they are applied to sections whose fixation and processing are different from the tissue where they were initially validated. ispartof: BIOTECHNIQUES vol:70 issue:3 pages:137-148 ispartof: location:England status: published

Published
2021
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6. Evaluation of sted super-resolution image quality by image correlation spectroscopy (QuICS)

Author

Gaetano Ivan Dellino, Elena Cerutti, Luca Lanzano, Isotta Cainero, Mario Faretta, Pier Giuseppe Pelicci, Paolo Bianchini, Morgana D'Amico, Alberto Diaspro, and Giuseppe Vicidomini

Subjects
Physics, Digital image correlation, Multidisciplinary, business.industry, Image quality, Science, media_common.quotation_subject, Autocorrelation, Resolution (electron density), STED microscopy, Noise (electronics), Article, Confocal microscopy, Optics, Medicine, Contrast (vision), Super-resolution microscopy, business, Image resolution, Biological fluorescence, media_common
Abstract

Quantifying the imaging performances in an unbiased way is of outmost importance in super-resolution microscopy. Here, we describe an algorithm based on image correlation spectroscopy (ICS) that can be used to assess the quality of super-resolution images. The algorithm is based on the calculation of an autocorrelation function and provides three different parameters: the width of the autocorrelation function, related to the spatial resolution; the brightness, related to the image contrast; the relative noise variance, related to the signal-to-noise ratio of the image. We use this algorithm to evaluate the quality of stimulated emission depletion (STED) images of DNA replication foci in U937 cells acquired under different imaging conditions. Increasing the STED depletion power improves the resolution but may reduce the image contrast. Increasing the number of line averages improves the signal-to-noise ratio but facilitates the onset of photobleaching and subsequent reduction of the image contrast. Finally, we evaluate the performances of two different separation of photons by lifetime tuning (SPLIT) approaches: the method of tunable STED depletion power and the commercially available Leica Tau-STED. We find that SPLIT provides an efficient way to improve the resolution and contrast in STED microscopy.

Published
2021

7. The Adaptive and Innate Immune Cell Landscape of Uterine Leiomyosarcomas

Author

Francesca Maria Bosisio, Giorgio Cattoretti, R. Mancari, Silvestro Carinelli, Marco Manzoni, Maddalena Maria Bolognesi, Asier Antoranz, Mario Faretta, Manzoni, M, Bolognesi, M, Antoranz, A, Mancari, R, Carinelli, S, Faretta, M, Bosisio, F, and Cattoretti, G

Subjects
Adult, Leiomyosarcoma, Cell type, B7 Antigens, T-Lymphocytes, Cell, Programmed Cell Death 1 Receptor, lcsh:Medicine, Biology, Adaptive Immunity, Article, B7-H1 Antigen, Monocytes, High dimensional, immunity, sarcoma, 03 medical and health sciences, 0302 clinical medicine, Immune system, medicine, Biomarkers, Tumor, Humans, lcsh:Science, Lung cancer, Author Correction, Hepatitis A Virus Cellular Receptor 2, 030304 developmental biology, Aged, 0303 health sciences, Multidisciplinary, Innate immune system, Melanoma, lcsh:R, Middle Aged, medicine.disease, Acquired immune system, Immunity, Innate, 3. Good health, medicine.anatomical_structure, Oncology, 030220 oncology & carcinogenesis, Uterine Neoplasms, Cancer research, Tumour immunology, lcsh:Q, Female, Sarcoma, Single-Cell Analysis
Abstract

Reactivation of the anti-tumor response has shown substantial progress in aggressive tumors such as melanoma and lung cancer. Data on less common histotypes are scanty. Immune checkpoint inhibitor therapy has been applied to few cases of uterine leiomyosarcomas, of which the immune cell composition was not examined in detail. We analyzed the inflammatory infiltrate of 21 such cases in high-dimensional, single cell phenotyping on routinely processed tissue. T-lymphoid cells displayed a composite phenotype common to all tumors, suggestive of antigen-exposure, acute and chronic exhaustion. To the contrary, myelomonocytic cells had case-specific individual combinations of phenotypes and subsets. We identified five distinct monocyte-macrophage cell types, some not described before, bearing immunosuppressive molecules (TIM3, B7H3, VISTA, PD1, PDL1). Detailed in situ analysis of routinely processed tissue yields comprehensive information about the immune status of sarcomas. The method employed provides equivalent information to extractive single-cell technology, with spatial contexture and a modest investment. ispartof: SCIENTIFIC REPORTS vol:10 issue:1 ispartof: location:England status: published

Published
2020

10. Nanoscale distribution of nuclear sites analyzed by superresolution STED-ICCS

Author

Paolo Bianchini, Gaetano Ivan Dellino, Enrico Gratton, Maria J. Sarmento, Isotta Cainero, Luca Lanzano, Michele Oneto, Mario Faretta, Lorenzo Scipioni, P G Pelicci, Alberto Diaspro, Laura Furia, and Simone Pelicci

Subjects
Physics, medicine.anatomical_structure, Microscopy, STED microscopy, medicine, Biophysics, Colocalization, Stimulated emission, Dual color, Nanoscopic scale, Nucleus, Superresolution
Abstract

Deciphering the spatiotemporal coordination between nuclear functions is important to understand its role in the maintenance of human genome. In this context, superresolution microscopy has gained considerable interest as it can be used to probe the spatial organization of functional sites in intact single cell nuclei in the 20-250 nm range. Among the methods that quantify colocalization from multicolor images, image cross-correlation spectroscopy (ICCS) offers several advantages, namely it does not require a pre-segmentation of the image into objects and can be used to detect dynamic interactions. However, the combination of ICCS with super-resolution microscopy has not been explored yet.Here we combine dual color stimulated emission depletion (STED) nanoscopy with ICCS (STED-ICCS) to quantify the nanoscale distribution of functional nuclear sites. We show that STED-ICCS provides not only a value of colocalized fraction but also the characteristic distances associated to correlated nuclear sites. As a validation, we quantify the nanoscale spatial distribution of three different pairs of functional nuclear sites in MCF10A cells. As expected, transcription foci and a transcriptionally repressive histone marker (H3K9me3) are not correlated. Conversely, nascent DNA replication foci and the Proliferating cell nuclear antigen (PCNA) protein have a high level of proximity and are correlated at a nanometer distance which is close to the limit of our experimental approach. Finally, transcription foci are found at a distance of 130 nm from replication foci, indicating a spatial segregation at the nanoscale. Overall, our data demonstrate that STED-ICCS can be a powerful tool for the analysis of nanoscale distribution of functional sites in the nucleus.Statement of significanceSeveral methods are available to quantify the proximity of two labeled molecules from dual color images. Among them, image cross-correlation spectroscopy (ICCS) is attractive as it does not require a pre-segmentation of the image into objects and can be used to detect dynamic interactions. Here, we combine for the first time ICCS with superresolution stimulated emission depletion (STED) microscopy (STED-ICCS) to quantify the spatial distribution of functional sites in the nucleus. Our results show that STED-ICCS, in addition to quantifying the colocalized fraction, detects characteristic nanometer distances associated to correlated nuclear sites. This work shows that STED-ICCS can be a powerful tool to quantify the nanoscale distribution of functional sites in the nucleus.

Published
2019
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11. Nanoscale Distribution of Nuclear Sites by Super-Resolved Image Cross-Correlation Spectroscopy

Author

Pier Giuseppe Pelicci, Enrico Gratton, Maria J. Sarmento, Luca Lanzano, Gaetano Ivan Dellino, Simone Pelicci, Lorenzo Scipioni, Alberto Diaspro, Paolo Bianchini, Michele Oneto, Laura Furia, Isotta Cainero, and Mario Faretta

Subjects
Biophysics, Color, 03 medical and health sciences, 0302 clinical medicine, Transcription (biology), Microscopy, medicine, Humans, Nanotechnology, 030304 developmental biology, Physics, Cell Nucleus, 0303 health sciences, biology, Spectrum Analysis, STED microscopy, Colocalization, Articles, Proliferating cell nuclear antigen, Histone, medicine.anatomical_structure, biology.protein, MCF-7 Cells, Human genome, Nucleus, 030217 neurology & neurosurgery
Abstract

Deciphering the spatiotemporal coordination between nuclear functions is important to understand its role in the maintenance of human genome. In this context, super-resolution microscopy has gained considerable interest because it can be used to probe the spatial organization of functional sites in intact single-cell nuclei in the 20-250 nm range. Among the methods that quantify colocalization from multicolor images, image cross-correlation spectroscopy (ICCS) offers several advantages, namely it does not require a presegmentation of the image into objects and can be used to detect dynamic interactions. However, the combination of ICCS with super-resolution microscopy has not been explored yet. Here, we combine dual-color stimulated emission depletion (STED) nanoscopy with ICCS (STED-ICCS) to quantify the nanoscale distribution of functional nuclear sites. We show that super-resolved ICCS provides not only a value of the colocalized fraction but also the characteristic distances associated to correlated nuclear sites. As a validation, we quantify the nanoscale spatial distribution of three different pairs of functional nuclear sites in MCF10A cells. As expected, transcription foci and a transcriptionally repressive histone marker (H3K9me3) are not correlated. Conversely, nascent DNA replication foci and the proliferating cell nuclear antigen(PCNA) protein have a high level of proximity and are correlated at a nanometer distance scale that is close to the limit of our experimental approach. Finally, transcription foci are found at a distance of 130 nm from replication foci, indicating a spatial segregation at the nanoscale. Overall, our data demonstrate that STED-ICCS can be a powerful tool for the analysis of the nanoscale distribution of functional sites in the nucleus.

Published
2019

12. RNAi screens identify CHD4 as an essential gene in breast cancer growth

Author

Laura Riva, Giancarlo Pruneri, Lorenzo Fornasari, Luisa Lanfrancone, Alessandro Carugo, Carolina D'Alesio, Carmen Criscitiello, Simona Punzi, Angelo Cicalese, Mario Faretta, Daniela Bossi, Pier Giuseppe Pelicci, Giuseppe Curigliano, and Laura Furia

Subjects
0301 basic medicine, Oncology, Time Factors, Mice, SCID, medicine.disease_cause, 0302 clinical medicine, Cellular Oncology, Mice, Inbred NOD, Gene Regulatory Networks, RNAi screen, Cell cycle, in vivo murine and human models, 3. Good health, Tumor Burden, Gene Expression Regulation, Neoplastic, Phenotype, 030220 oncology & carcinogenesis, Female, RNA Interference, Breast carcinoma, Research Paper, Mi-2 Nucleosome Remodeling and Deacetylase Complex, Signal Transduction, Cyclin-Dependent Kinase Inhibitor p21, medicine.medical_specialty, Breast Neoplasms, 03 medical and health sciences, Breast cancer, breast cancer, Internal medicine, Cell Line, Tumor, medicine, Animals, Humans, Genetic Predisposition to Disease, Epigenetics, Cell Proliferation, Gene Library, epigenetic targets, business.industry, DNA Helicases, Cancer, Computational Biology, Cell Cycle Checkpoints, medicine.disease, CHD4, 030104 developmental biology, Immunology, Cancer cell, Carcinogenesis, business, Neoplasm Transplantation
Abstract

// Carolina D’Alesio 1, * , Simona Punzi 1, * , Angelo Cicalese 1 , Lorenzo Fornasari 1 , Laura Furia 1 , Laura Riva 2 , Alessandro Carugo 1, 3 , Giuseppe Curigliano 4 , Carmen Criscitiello 4 , Giancarlo Pruneri 5, 6 , Pier Giuseppe Pelicci 1, 7 , Mario Faretta 1 , Daniela Bossi 1 , Luisa Lanfrancone 1 1 Department of Experimental Oncology, European Institute of Oncology, Milan 20141, Italy 2 Center for Genomic Science of IIT@SEMM, Fondazione Istituto Italiano di Tecnologia, Milan 20139, Italy 3 Department of Molecular and Cellular Oncology, UT MD Anderson Cancer Center, Houston, TX 77030, USA 4 Division of Experimental Therapeutics, European Institute of Oncology, Milan 20141, Italy 5 School of Medicine, University of Milan, Milan 20122, Italy 6 Biobank for Translational Medicine Unit, Department of Pathology, European Institute of Oncology, Milan 20141, Italy 7 Department of Oncology, University of Milan, Milan 20139, Italy * These authors have contributed equally to this work Correspondence to: Luisa Lanfrancone, email: luisa.lanfrancone@ieo.eu Keywords: RNAi screen, epigenetic targets, breast cancer, CHD4, in vivo murine and human models Received: July 22, 2016 Accepted: September 29, 2016 Published: October 13, 2016 ABSTRACT Epigenetic regulation plays an essential role in tumor development and epigenetic modifiers are considered optimal potential druggable candidates. In order to identify new breast cancer vulnerabilities and improve therapeutic chances for patients, we performed in vivo and in vitro shRNA screens in a human breast cancer cell model (MCF10DCIS.com cell line) using epigenetic libraries. Among the genes identified in our screening, we deeply investigated the role of Chromodomain Helicase DNA binding Protein 4 ( CHD4 ) in breast cancer tumorigenesis. CHD4 silencing significantly reduced tumor growth in vivo and proliferation in vitro of MCF10DCIS.com cells. Similarly, in vivo breast cancer growth was decreased in a spontaneous mouse model of breast carcinoma (MMTV-NeuT system) and in metastatic patient-derived xenograft models. Conversely, no reduction in proliferative ability of non-transformed mammary epithelial cells (MCF10A) was detected. Moreover, we showed that CHD4 depletion arrests proliferation by inducing a G0/G1 block of cell cycle associated with up-regulation of CDKN1A (p21). These results highlight the relevance of genetic screens in the identification of tumor frailties and the role of CHD4 as a potential pharmacological target to inhibit breast cancer growth.

Published
2016

13. The landscape of S100B+ and HLA-DR+ dendritic cell subsets in tonsils at the single cell level via high-parameter mapping

Author

Giorgio Cattoretti, Francesca Maria Bosisio, Carlo Parravicini, Denis Schapiro, Ann M. Haberman, Maddalena Maria Bolognesi, Tagliabue R, Marco Manzoni, and Mario Faretta

Subjects
medicine.anatomical_structure, Tonsil, Cell, medicine, HLA-DR, Dendritic cell, IRF8, Biology, medicine.disease_cause, Phenotype, Autoimmunity, IRF4, Cell biology
Abstract

SUMMARYDendritic cells (DC) (classic, plasmacytoid, inflammatory) are an intense focus of interest because of their role in inflammation, autoimmunity, vaccination and cancer. We present a tissue-based classification of human DC subsets in tonsils with a high-parameter (>40 markers) immunofluorescent approach, cell type-specific image segmentation and the use of bioinformatics platforms. Through this deep phenotypic and spatial examination, classic cDC1, cDC2, pDC subsets have been further refined and a novel subset of DC co-expressing IRF4 and IRF8 identified. Based on unique tissue locations within the tonsil, and close interactions with T cells (cDC1) or B cells (cDC2), DC subsets can be further subdivided by correlative phenotypic changes associated with these interactions. In addition, monocytes and macrophages expressing HLA-DR or S100AB are identified and localized in the tissue. This study thus provides a whole tissue in situ catalog of human DC subsets and their cellular interactions within spatially defined niches.

Published
2018
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14. A Liquid Tunable Microscope as a New Paradigm in Optical Microscopy to Paint 4D Chromatin Organisation in the Cell Nucleus

Author

Melody Di Bona, Luca Pesce, Isotta Cainero, Francesca Cella Zanacchi, Simone Pelicci, Aymeric Le Gratiet, Luca Lanzano, Giuseppe Vicidomini, Alberto Diaspro, Paolo Bianchini, Mario Faretta, Paola Barboro, and Michele Oneto

Subjects
Cell nucleus, Materials science, Microscope, medicine.anatomical_structure, Optical microscope, law, Biophysics, medicine, Chromatin organisation, law.invention
Published
2018

15. The Combination of the PARP Inhibitor Rucaparib and 5FU Is an Effective Strategy for Treating Acute Leukemias

Author

Giovanni Martinelli, Andrea Ghelli Luserna di Rorà, Klaus-Michael Debatin, Francesco Bertolini, Chiara Ronchini, Lüder Hinrich Meyer, P G Pelicci, Mario Faretta, Ilaria Iacobucci, Stefania Orecchioni, Maria Vittoria Verga Falzacappa, Falzacappa, Maria Vittoria Verga, Ronchini, Chiara, Faretta, Mario, Iacobucci, Ilaria, Ghelli Luserna Di Rorà, Andrea, Martinelli, Giovanni, Meyer, Lüder Hinrich, Debatin, Klaus-Michael, Orecchioni, Stefania, Bertolini, Francesco, and Pelicci, Pier Giuseppe

Subjects
DNA Replication, Male, Antimetabolites, Antineoplastic, Cancer Research, Xenograft Model Antitumor Assay, Indoles, DNA Repair, Cell Survival, DNA repair, DNA damage, Poly ADP ribose polymerase, Apoptosis, Poly(ADP-ribose) Polymerase Inhibitors, Pharmacology, Poly(ADP-ribose) Polymerase Inhibitor, Mice, chemistry.chemical_compound, Cell Line, Tumor, Animals, Humans, Medicine, Neoplasm, Rucaparib, Leukemia, Animal, business.industry, Medicine (all), Apoptosi, Myeloid leukemia, Drug Synergism, medicine.disease, Xenograft Model Antitumor Assays, Disease Models, Animal, Oncology, chemistry, Indole, Drug Resistance, Neoplasm, PARP inhibitor, Female, Fluorouracil, business, Human, DNA Damage
Abstract

The existing treatments to cure acute leukemias seem to be nonspecific and suboptimal for most patients, drawing attention to the need of new therapeutic strategies. In the last decade the anticancer potential of poly ADP-ribose polymerase (PARP) inhibitors became apparent and now several PARP inhibitors are being developed to treat various malignancies. So far, the usage of PARP inhibitors has been mainly focused on the treatment of solid tumors and not too much about their efficacy on leukemias is known. In this study we test, for the first time on leukemic cells, a combined therapy that associates the conventional chemotherapeutic agent fluorouracil (5FU), used as a source of DNA damage, and a PARP inhibitor, rucaparib. We demonstrate the efficacy and the specificity of this combined therapy in killing both acute myeloid leukemia and acute lymphoid leukemia cells in vitro and in vivo. We clearly show that the inhibition of DNA repair induced by rucaparib is synthetic lethal with the DNA damage caused by 5FU in leukemic cells. Therefore, we propose a new therapeutic strategy able to enhance the cytotoxic effect of DNA-damaging agents in leukemia cells via inhibiting the repair of damaged DNA. Mol Cancer Ther; 14(4); 889–98. ©2015 AACR.

Published
2015
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16. Multiplex staining by sequential immunostaining and antibody removal on routine tissue sections

Author

Francesca Maria Bosisio, Stefano Zannella, Giorgio Cattoretti, Maddalena Maria Bolognesi, Mario Faretta, Carla Rossana Scalia, Marco Manzoni, Bolognesi, M, Manzoni, M, Scalia, C, Zannella, S, Bosisio, F, Faretta, M, and Cattoretti, G

Subjects
High-Throughput Screening Assay, 0301 basic medicine, Pathology, Tissue Fixation, Antibodie, Placenta, Protein Renaturation, Rabbit, Kidney, Mice, 0302 clinical medicine, Pregnancy, Multiplex, Fluorescent Antibody Technique, Indirect, Skin, epitope, 0303 health sciences, medicine.diagnostic_test, biology, Chemistry, Goats, Articles, Immunohistochemistry, Primary and secondary antibodies, 3. Good health, Antigen, 030220 oncology & carcinogenesis, Goat, Female, Rabbits, Anatomy, Human, medicine.medical_specialty, Histology, Immunofluorescence, Stain, Antibodies, 03 medical and health sciences, antibody removal, medicine, Animals, Humans, Antigens, immunofluorescence, Image analysis, 030304 developmental biology, Tissue Embedding, Animal, High-Throughput Screening Assays, Staining, multiplex, Autofluorescence, 030104 developmental biology, biology.protein, Immunostaining, Biomedical engineering
Abstract

Multiplexing (mplx), labeling for multiple immunostains the very same cell or tissue section in situ, has raised considerable interest. The methods proposed include the use of labelled primary antibodies, spectral separation of fluorochromes, bleaching of the fluorophores or chromogens, blocking of previous antibody layers, all in various combinations. The major obstacles to the diffusion of this technique are high costs in custom antibodies and instruments, low throughput, scarcity of specialized skills or facilities.We have validated a method based on common primary and secondary antibodies and diffusely available fluorescent image scanners. It entails rounds of four-color indirect immunofluorescence, image acquisition and removal (stripping) of the antibodies, before another stain is applied. The images are digitally registered and the autofluorescence is subtracted. Removal of antibodies is accomplished by disulphide cleavage and a detergent or by a chaotropic salt treatment, this latter followed by antigen refolding. More than thirty different antibody stains can be applied to one single section from routinely fixed and embedded tissue. This method requires a modest investment in hardware and materials and uses freeware image analysis software. Mplx on routine tissue sections is a high throughput tool for in situ characterization of neoplastic, reactive, inflammatory and normal cells.

Published
2017
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17. Molecular investigation of coexistent chronic myeloid leukaemia and peripheral T-cell lymphoma - a case report

Author

Simona Sammassimo, Alicja M. Gruszka, Angelica Calleri, Giuliana Gregato, Francesco Bertolini, Giancarlo Pruneri, Rita De Molfetta, Laura Cannella, Mario Faretta, Giovanna Andreola, Cristina Rabascio, and Myriam Alcalay

Subjects
Male, Population, Fusion Proteins, bcr-abl, Antineoplastic Agents, Bioinformatics, Article, hemic and lymphatic diseases, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, Medicine, Humans, Adverse effect, education, Protein Kinase Inhibitors, Myeloproliferative neoplasm, In Situ Hybridization, Fluorescence, education.field_of_study, Multidisciplinary, business.industry, Myeloid leukemia, Lymphoma, T-Cell, Peripheral, Middle Aged, medicine.disease, Peripheral T-cell lymphoma, Lymphoma, Imatinib mesylate, Cancer research, Imatinib Mesylate, business, Tyrosine kinase
Abstract

Chronic myeloid leukemia (CML) is a myeloproliferative neoplasm underlain by the formation of BCR-ABL1 – an aberrant tyrosine kinase – in the leukaemic blasts. Long-term survival rates in CML prior to the advent of tyrosine kinase inhibitors (TKIs) were dismal, albeit the incidence of secondary malignancies was higher than that of age-matched population. Current figures confirm the safety of TKIs with conflicting data concerning the increased risk of secondary tumours. We postulate that care has to be taken when distinguishing between coexisting, secondary-to-treatment and second in sequence, but independent tumourigenic events, in order to achieve an unbiased picture of the adverse effects of novel treatments. To illustrate this point, we present a case of a patient in which CML and peripheral T-cell lymphoma (PTCL) coexisted, although the clinical presentation of the latter followed the achievement of major molecular response of CML to TKIs.

Published
2015

18. New method to detect histone acetylation levels by flow cytometry

Author

Marco Ballarini, Simona Ronzoni, Pier Giuseppe Pelicci, Mario Faretta, and Saverio Minucci

Subjects
Histology, medicine.drug_class, Biology, Pathology and Forensic Medicine, Histones, Cell Line, Tumor, Histone H2A, Biomarkers, Tumor, medicine, Humans, Analysis of Variance, Histone deacetylase 5, Blood Cells, Leukemia, Histone deacetylase 2, HDAC11, Histone deacetylase inhibitor, Acetylation, Cell Biology, Flow Cytometry, Molecular biology, Histone Deacetylase Inhibitors, Trichostatin A, Histone, Acute Disease, biology.protein, Histone deacetylase, medicine.drug
Abstract

Background Reversible histone acetylation affects chromatin structural organization, thus regulating gene expression and other nuclear events. Levels of histone acetylation are tightly modulated in normal cells, and alterations of their regulating mechanisms have been shown to be involved in tumorigenesis. Methods We developed a new flow cytometric technique for detection of histone acetylation, based on a specific monoclonal antibody that recognizes acetylated histone tails. Bivariate analysis for histone acetylation levels and DNA were performed to study modulation of chromatin organization during the cell cycle and after induction of histone hyperacetylation by the histone deacetylase (HDAC) inhibitor trichostatin A (TSA). Histone acetylation and transcription levels were monitored during differentiation induced by retinoic acid alone or in combination with TSA. Blood samples from patients were analyzed with the described protocol to monitor the effects of HDAC inhibitors in vivo and validate the developed protocol for clinical usage. Results Flow cytometric detection of acetylation status can successfully detect modifications induced by HDAC inhibitor treatment in vivo as demonstrated by analysis of various blood samples from patients treated with valproic acid. Changes in acetylation levels during the cell cycle demonstrated a reproducible increase in histone acetylation during the replication phase that was subsequently decreased at the G2M entrance, thus paralleling the behavior of DNA replication and transcriptional activity. Conclusions Multiparameter analysis of histone acetylation and expression of molecular markers, DNA ploidy, and/or cell cycle kinetics can provide a quick and statistically reliable tool for the diagnosis and evaluation of treatment efficacy in clinical trials using HDAC inhibitors. © 2005 Wiley-Liss, Inc.

Published
2005
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19. Kinetic Heterogeneity of an Experimental Tumour Revealed by BrdUrd Incorporation and Mathematical Modelling

Author

Carmela Sinisgalli, Alessandro Bertuzzi, Mario Faretta, G. Starace, Giorgio Valoti, Paolo Ubezio, and Alberto Gandolfi

Subjects
Cell division, Citofluorimetria, General Mathematics, Immunology, Population, Cell, Mice, Nude, Biology, Models, Biological, General Biochemistry, Genetics and Molecular Biology, Flow cytometry, Mice, chemistry.chemical_compound, In vivo, Tumor Cells, Cultured, Econometrics, medicine, Animals, Humans, Doubling time, education, Tumori sperimentali, General Environmental Science, Ovarian Neoplasms, Pharmacology, education.field_of_study, DNA-BrdUrd, medicine.diagnostic_test, General Neuroscience, Carcinoma, Cell Cycle, DNA, Neoplasm, Cell cycle, Flow Cytometry, Stima di parametri, Modelli matematici, Kinetics, medicine.anatomical_structure, Bromodeoxyuridine, Computational Theory and Mathematics, chemistry, Biophysics, Female, General Agricultural and Biological Sciences, Cell Division
Abstract

In the present paper we propose a method of analysis of the cell kinetic characteristics of in vivo experimental tumours, that uses DNA-BrdUrd flow cytometry data at various times after the bromodeoxyuridine (BrdUrd) injection and mathematical modelling. The model of the cell population takes into account the cell-cell heterogeneity of the progression rate across cell cycle phases within the tumour, and assumes a strict correlation between the durations of S and G2M phases. The model also allows for a nonconstant DNA synthesis rate across S phase. In addition, the measurement process is modelled, considering the possibility of nonimpulsive labelling and providing a representation of the time course of the bivariate DNA-BrdUrd fluorescence distribution. Sequential DNA-BrdUrd distributions were obtained in vivo from a human ovarian carcinoma transplanted in mice and, for comparison, in vitro from a cell line of the same origin. From these data, that included the fractional density and the mean BrdUrd-fluorescence of BrdUrd-positive cells as a function of the DNA-fluorescence, kinetic parameters such as the potential doubling time (Tpot) and the mean and variance of the transit times in S and G2M phases, were estimated. This study revealed the presence of a substantial heterogeneity in S and G2M phases within the in vivo cell population and of a lower heterogeneity in the in vitro population. Moreover, our analysis suggests a nonnegligible effect of the BrdUrd pharmacokinetics in the in vivo cell labelling.

Published
2002
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20. High-resolution cytometry for high-content cell cycle analysis

Author

Laura Furia, Pier Giuseppe Pelicci, and Mario Faretta

Subjects
Microscopy, Histology, medicine.diagnostic_test, Computer science, Real-time computing, Cell Cycle, High resolution, Nanotechnology, General Medicine, Automated microscopy, Biochemistry, Flow cytometry, Medical Laboratory Technology, Automation, High-content screening, Content (measure theory), medicine, Image Processing, Computer-Assisted, Image Cytometry, Animals, Humans, Cytometry
Abstract

One of the major limitations of flow cytometry (FCM) is the absence of an intracellular view. Automated microscopy and image analysis, together with technological developments, led to new approaches in cytometry that bypass the above limitation, introducing high resolution, high content, and large statistical sampling. However, few attempts have been made, until now, to translate the wide repertoire of FCM assays into high-content image screening. This unit describes the implementation of an acquisition and analysis protocol for evaluation of the cell cycle by automated microscopy. The approach grants the possibility to perform simultaneous analysis of a high number of different parameters. A large part of this unit is devoted to the description of hardware features that can optimize the recorded information together with the acquisition and analysis procedures employed to produce good-quality data. Curr. Protoc. Cytom. 70:7.41.1-7.41.15. © 2014 by John Wiley & Sons, Inc. Keywords: image cytometry; cell cycle; S phase; high-content analysis; high resolution; automated microscopy; wide-field microscopy

Published
2014

21. Mode of action of thiocoraline, a natural marine compound with anti-tumour activity

Author

Daniele Bergamaschi, M. Bonfanti, Jose Jimeno, Mario Faretta, S Ronzoni, Maurizio D'Incalci, Eugenio Erba, Glynn Faircloth, C V Catapano, and Stefano Taverna

Subjects
Cancer Research, Time Factors, Cell division, DNA polymerase, DNA-Directed DNA Polymerase, thiocoraline, natural compound, chemistry.chemical_compound, Inhibitory Concentration 50, Depsipeptides, medicine, Tumor Cells, Cultured, Humans, Tumor Stem Cell Assay, Genetics, Antibiotics, Antineoplastic, biology, Cell Cycle, DNA replication, Regular Article, DNA polymerase α, DNA, Cell cycle, Flow Cytometry, Molecular biology, Anti-Bacterial Agents, Oncology, chemistry, Mechanism of action, Bromodeoxyuridine, Cell culture, biology.protein, medicine.symptom, Peptides, Cell Division
Abstract

Thiocoraline, a new anticancer agent derived from the marine actinomycete Micromonospora marina, was found to induce profound perturbations of the cell cycle. On both LoVo and SW620 human colon cancer cell lines, thiocoraline caused an arrest in G1 phase of the cell cycle and a decrease in the rate of S phase progression towards G2/M phases, as assessed by using bromodeoxyuridine/DNA biparametric flow cytometric analysis. Thiocoraline does not inhibit DNA-topoisomerase II enzymes in vitro, nor does it induce DNA breakage in cells exposed to effective drug concentrations. The cell cycle effects observed after exposure to thiocoraline appear related to the inhibition of DNA replication. By using a primer extension assay it was found that thiocoraline inhibited DNA elongation by DNA polymerase α at concentrations that inhibited cell cycle progression and clonogenicity. These studies indicate that the new anticancer drug thiocoraline probably acts by inhibiting DNA polymerase α activity. © 1999 Cancer Research Campaign

Published
1999

22. DNA damage in stem cells activates p21, inhibits p53, and induces symmetric self-renewing divisions

Author

Pier Giuseppe Pelicci, Alessandra Insinga, Luisa Albano, Simona Ronzoni, Andrea Viale, Angelo Cicalese, Mario Faretta, Laura Furia, and Barbara Gallo

Subjects
Senescence, Cyclin-Dependent Kinase Inhibitor p21, Mice, 129 Strain, DNA Repair, DNA damage, DNA repair, Stem cell theory of aging, Apoptosis, Biology, medicine.disease_cause, Mice, Mammary Glands, Animal, medicine, Animals, Mice, Knockout, Multidisciplinary, Cell Cycle Checkpoints, Cell cycle, Biological Sciences, Hematopoietic Stem Cells, Cell biology, Up-Regulation, Mice, Inbred C57BL, Adult Stem Cells, Cancer research, Female, Stem cell, Tumor Suppressor Protein p53, Carcinogenesis, Cell Division, Adult stem cell, DNA Damage
Abstract

DNA damage leads to a halt in proliferation owing to apoptosis or senescence, which prevents transmission of DNA alterations. This cellular response depends on the tumor suppressor p53 and functions as a powerful barrier to tumor development. Adult stem cells are resistant to DNA damage-induced apoptosis or senescence, however, and how they execute this response and suppress tumorigenesis is unknown. We show that irradiation of hematopoietic and mammary stem cells up-regulates the cell cycle inhibitor p21, a known target of p53, which prevents p53 activation and inhibits p53 basal activity, impeding apoptosis and leading to cell cycle entry and symmetric self-renewing divisions. p21 also activates DNA repair, limiting DNA damage accumulation and self-renewal exhaustion. Stem cells with moderate DNA damage and diminished self-renewal persist after irradiation, however. These findings suggest that stem cells have evolved a unique, p21-dependent response to DNA damage that leads to their immediate expansion and limits their long-term survival.

Published
2013

23. Methyltransferase recruitment and DNA hypermethylation of target promoters by an oncogenic transcription factor

Author

Saverio Minucci, Mirco Fanelli, Francesco Fazi, Tony Kouzarides, Mario Faretta, François Fuks, Pier Giuseppe Pelicci, Luciano Di Croce, Veronica A. Raker, Francesco Lo Coco, Clara Nervi, and Massimo Corsaro

Subjects
Methyltransferase, Oncogene Proteins, Fusion, Receptors, Retinoic Acid, Retinoic Acid, Gene Expression, medicine.disease_cause, Cell Transformation, DNA Methyltransferase 3A, Leukemia, Promyelocytic, Acute, Receptors, Tumor Cells, Cultured, DNA (Cytosine-5-)-Methyltransferases, Cloning, Molecular, Promoter Regions, Genetic, Promyelocytic, Oncogene Proteins, DNA methylation, Multidisciplinary, Leukemia, Cultured, Cell Differentiation, Methylation, Exons, Neoplasm Proteins, Tumor Cells, Zinc, Cell Transformation, Neoplastic, Azacitidine, DNA (Cytosine-5-)-Methyltransferase 1, Recombinant Fusion Proteins, Tretinoin, Biology, Acute, Decitabine, Histone Deacetylases, Cell Line, Promoter Regions, Genetic, APL, PML/RAR, medicine, Gene silencing, Humans, Epigenetics, Gene Silencing, Fusion, Transcription factor, Cell Nucleus, Neoplastic, Binding Sites, Molecular, Promoter, CpG Islands, DNA (Cytosine-5-)-Methyltransferase, Mutation, Transcription Factors, DNA Methylation, Cancer research, Carcinogenesis, Settore MED/15 - Malattie del Sangue, Cloning
Abstract

DNA methylation of tumor suppressor genes is a frequent mechanism of transcriptional silencing in cancer. The molecular mechanisms underlying the specificity of methylation are unknown. We report here that the leukemia-promoting PML-RAR fusion protein induces gene hypermethylation and silencing by recruiting DNA methyltransferases to target promoters and that hypermethylation contributes to its leukemogenic potential. Retinoic acid treatment induces promoter demethylation, gene reexpression, and reversion of the transformed phenotype. These results establish a mechanistic link between genetic and epigenetic changes during transformation and suggest that hypermethylation contributes to the early steps of carcinogenesis.

Published
2002

24. Cell cycle effects of gemcitabine

Author

Federica Viale, Paolo Cappella, Daniela Tomasoni, Monica Lupi, Fabio Banzato, Francesco Montalenti, Paolo Ubezio, Maurizio D'Incalci, Mario Faretta, Cappella, P, Tomasoni, D, Faretta, M, Lupi, M, Montalenti, F, Viale, F, Banzato, F, D'Incalci, M, and Ubezio, P

Subjects
DNA Replication, Cancer Research, medicine.medical_specialty, Antimetabolites, Antineoplastic, Cell Survival, Pharmacology, Biology, chemotherapy, Deoxycytidine, S Phase, chemistry.chemical_compound, Internal medicine, medicine, Tumor Cells, Cultured, Humans, Cytotoxicity, Cisplatin, Ovarian Neoplasms, DNA synthesis, Dose-Response Relationship, Drug, Cell growth, flow cytometry, gemcitabine, apoptosis, DNA, Neoplasm, Cell cycle, Gemcitabine, Endocrinology, cell proliferation, Oncology, chemistry, Apoptosis, Female, cell cycle, Growth inhibition, medicine.drug
Abstract

Gemcitabine (2',2'-difluoro-2'-deoxycytidine, or dFdC) is a promising anticancer agent with demonstrated clinical activity in solid tumours currently undergoing clinical trials. Despite extensive studies on the biochemical mechanism of action, cell cycle perturbations induced by dFdC have not yet been thoroughly investigated, apart from the expected inhibition of DNA synthesis. The aim of our study was to clarify whether cell population kinetics is a vital factor in the cytotoxicity of dFdC in single or repeated treatments and in the dFdC-cisplatin combination. Ovarian cancer cells growing in vitro were treated with dFdC for 1 hr in a range of concentrations from 10 nM to 10 microM. Cell kinetics was investigated by DNA-bromodeoxyuridine flow cytometry, using different experimental protocols to measure either the time course of DNA-synthesis inhibition or the fate of cells in G(1), S or G(2)M at the time of dFdC treatment or 24 hr later. A modified sulforhodamine B test was used to assess the growth inhibition caused by dFdC given alone or with cisplatin. Although dFdC promptly inhibited DNA synthesis, cytotoxicity on proliferating cells was not specific for cells initially in the S phase. DNA synthesis was restored after a G(1) block of variable, dose-dependent length, but recycling cells were intercepted at the subsequent checkpoints, resulting in delays in the G(2)M and G(1) phases. The activity of repeated treatment with dFdC + dFdC or dFdC + cisplatin was highly dependent on the interval length between them. These results suggest that the kinetics of cell recycling from a first dFdC treatment strongly affects the outcome of a second treatment with either dFdC itself or cisplatin.

Published
2001

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