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2. The activity of a mammalian proline-rich peptide against Gram-negative bacteria, including drug-resistant strains, relies on a nonmembranolytic mode of action

Author

Ciociola T, Giovati L, Giovannelli A, Conti S, Castagnola M, and Vitali A

Subjects
Antimicrobial peptide, proline-rich peptides, drug-resistant bacteria, confocal microscopy, scanning electron microscopy, Galleria mellonella model., Infectious and parasitic diseases, RC109-216
Abstract

Tecla Ciociola,1 Laura Giovati,1 Angela Giovannelli,2 Stefania Conti,1 Massimo Castagnola,2,3 Alberto Vitali3 1Department of Medicine and Surgery, University of Parma, Parma, 2Institute of Biochemistry and Clinical Biochemistry, Catholic University, Rome, 3Institute for the Chemistry of Molecular Recognition, C.N.R., c/o Institute of Biochemistry and Clinical Biochemistry, Catholic University, Rome, Italy Background: A peptide of 2,733 Da named SP-E, previously isolated from pig saliva and already described for its antifungal activity and absence of toxicity against mammalian cells, is characterized by a high content of proline residues (70% of entire sequence), that confer structural features probably related to peptide activity. Purpose: The aim of this study was to evaluate the activity of SP-E against Gram-negative bacteria, including drug-resistant clinical isolates. Methods: SP-E and shorter fragments of the same peptide were tested in vitro against the selected bacteria by colony forming unit assays. Scanning electron microscopy and confocal microscopy were also applied. SP-E potential therapeutic activity was evaluated in vivo in a Galleria mellonella model of bacterial infection. Results: SP-E proved to be active against the tested bacteria with EC50 values in the micromolar range. Though maintaining antibacterial properties, the shorter peptides showed lower activity in respect to the parental molecule. Kinetics of killing action and nonmembranolytic internalization within Escherichia coli and Pseudomonas aeruginosa cells strongly suggested a cytosolic mechanism of action involving one or more intracellular molecular targets. A single injection of SP-E exerted a therapeutic effect in G. mellonella larvae infected with P. aeruginosa. Conclusion: The biological properties of SP-E strongly back this peptide as a new promising multitasking antimicrobial molecule. Keywords: antimicrobial peptide, proline-rich peptides, drug-resistant bacteria, confocal microscopy, scanning electron microscopy, Galleria mellonella model

Published
2018

3. L1CAM EXPRESSION IDENTIFIES DIFFERENT COLORECTAL TUMOR SUBGROUPS

Author

Cau, F., primary, Gerosa, C., additional, Ziranu, G., additional, Pretta, A., additional, Murru, R., additional, Fraschini, M., additional, Piras, M., additional, Eyken, P.V., additional, La Nasa, G., additional, Castagnola, M., additional, Coghe, F., additional, Orrù, G., additional, Zorcolo, L., additional, Fanni, D., additional, Scartozzi, M., additional, and Faa, G., additional

Published
2023
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4. Combined Salivary Proteome Profiling and Machine Learning Analysis Provides Insight into Molecular Signature for Autoimmune Liver Diseases Classification

Author

Guadalupi, G., Contini, C., Iavarone, Federica, Castagnola, Massimo, Messana, Irene, Faa, G., Onali, Sebastiano, Chessa, L., Vitorino, R., Amado, F., Diaz, G., Manconi, B., Cabras, T., Olianas, A., Iavarone F. (ORCID:0000-0002-2074-5531), Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), Onali S., Guadalupi, G., Contini, C., Iavarone, Federica, Castagnola, Massimo, Messana, Irene, Faa, G., Onali, Sebastiano, Chessa, L., Vitorino, R., Amado, F., Diaz, G., Manconi, B., Cabras, T., Olianas, A., Iavarone F. (ORCID:0000-0002-2074-5531), Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), and Onali S.

Abstract

Autoimmune hepatitis (AIH) and primary biliary cholangitis (PBC) are autoimmune liver diseases that target the liver and have a wide spectrum of presentation. A global overview of quantitative variations on the salivary proteome in presence of these two pathologies is investigated in this study. The acid-insoluble salivary fraction of AIH and PBC patients, and healthy controls (HCs), was analyzed using a gel-based bottom-up proteomic approach combined with a robust machine learning statistical analysis of the dataset. The abundance of Arginase, Junction plakoglobin, Desmoplakin, Hexokinase-3 and Desmocollin-1 decreased, while that of BPI fold-containing family A member 2 increased in AIHp compared to HCs; the abundance of Gelsolin, CD14, Tumor-associated calcium signal transducer 2, Clusterin, Heterogeneous nuclear ribonucleoproteins A2/B1, Cofilin-1 and BPI fold-containing family B member 2 increased in PBCp compared to HCs. The abundance of Hornerin decreased in both AIHp and PBCp with respect to HCs and provided an area under the ROC curve of 0.939. Machine learning analysis confirmed the feasibility of the salivary proteome to discriminate groups of subjects based on AIH or PBC occurrence as previously suggested by our group. The topology-based functional enrichment analysis performed on these potential salivary biomarkers highlights an enrichment of terms mostly related to the immune system, but also with a strong involvement in liver fibrosis process and with antimicrobial activity.

Published
2023

5. Top-Down Proteomics Detection of Potential Salivary Biomarkers for Autoimmune Liver Diseases Classification

Author

Olianas, A., Guadalupi, G., Cabras, T., Contini, C., Serrao, S., Iavarone, Federica, Castagnola, Massimo, Messana, Irene, Onali, Sebastiano, Chessa, L., Diaz, G., Manconi, B., Iavarone F. (ORCID:0000-0002-2074-5531), Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), Onali S., Olianas, A., Guadalupi, G., Cabras, T., Contini, C., Serrao, S., Iavarone, Federica, Castagnola, Massimo, Messana, Irene, Onali, Sebastiano, Chessa, L., Diaz, G., Manconi, B., Iavarone F. (ORCID:0000-0002-2074-5531), Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), and Onali S.

Abstract

(1) Autoimmune hepatitis (AIH) and primary biliary cholangitis (PBC) are autoimmune liver diseases characterized by chronic hepatic inflammation and progressive liver fibrosis. The possible use of saliva as a diagnostic tool has been explored in several oral and systemic diseases. The use of proteomics for personalized medicine is a rapidly emerging field. (2) Salivary proteomic data of 36 healthy controls (HCs), 36 AIH and 36 PBC patients, obtained by liquid chromatography/mass spectrometry top-down pipeline, were analyzed by multiple Mann-Whitney test, Kendall correlation, Random Forest (RF) analysis and Linear Discriminant Analysis (LDA); (3) Mann-Whitney tests provided indications on the panel of differentially expressed salivary proteins and peptides, namely cystatin A, statherin, histatin 3, histatin 5 and histatin 6, which were elevated in AIH patients with respect to both HCs and PBC patients, while S100A12, S100A9 short, cystatin S1, S2, SN and C showed varied levels in PBC with respect to HCs and/or AIH patients. RF analysis evidenced a panel of salivary proteins/peptides able to classify with good accuracy PBC vs. HCs (83.3%), AIH vs. HCs (79.9%) and PBC vs. AIH (80.2%); (4) RF appears to be an attractive machine-learning tool suited for classification of AIH and PBC based on their different salivary proteomic profiles.

Published
2023

6. Estimation of postmortem interval using top-down HPLC–MS analysis of peptide fragments in vitreous humour: A pilot study

Author

Boroumand, M., Grassi, V. M., Castagnola, F., De-Giorgio, F., D'Aloja, E., Vetrugno, Giuseppe, Pascali, Vincenzo Lorenzo, Vincenzoni, F., Iavarone, Federica, Faa, G., Castagnola, Massimo, Vetrugno G. (ORCID:0000-0003-0181-2855), Pascali V. L. (ORCID:0000-0001-6520-5224), Iavarone F. (ORCID:0000-0002-2074-5531), Castagnola M. (ORCID:0000-0002-0959-7259), Boroumand, M., Grassi, V. M., Castagnola, F., De-Giorgio, F., D'Aloja, E., Vetrugno, Giuseppe, Pascali, Vincenzo Lorenzo, Vincenzoni, F., Iavarone, Federica, Faa, G., Castagnola, Massimo, Vetrugno G. (ORCID:0000-0003-0181-2855), Pascali V. L. (ORCID:0000-0001-6520-5224), Iavarone F. (ORCID:0000-0002-2074-5531), and Castagnola M. (ORCID:0000-0002-0959-7259)

Abstract

This study reports the detection of a set of 35 peptide fragments and 7 intact proteins in the vitreous humour using a top-down proteomic platform based on high-resolution HPLC-MS and MS/MS analysis. The concentrations of thymosin b4 (R = 0.932) and two peptide fragments (i.e., vimentin fragment (Fr.) 443-465 (R = 0.998) and polyubiquitin Fr. 1-73 (R = 0.968)) were observed to have very strong linear correlations with postmortem intervals. Data are available via ProteomeXchange with identifier PXD037095. These preliminary results suggest that some biochemical molecular events are linearly related to the postmortem interval and that the concentrations of these peptides and fragments can be clinically useful in establishing the time of death if measured within the first 160 h postmortem. (c) 2022 Elsevier B.V. All rights reserved.

Published
2023

7. The Post-Translational Modifications of Human Salivary Peptides and Proteins Evidenced by Top-Down Platforms

Author

Messana, Irene, Manconi, B., Cabras, T., Boroumand, M., Sanna, M. T., Iavarone, Federica, Olianas, A., Desiderio, Claudia, Rossetti, Diana Valeria, Vincenzoni, F., Contini, C., Guadalupi, G., Fiorita, Antonella, Faa, G., Castagnola, Massimo, Messana I. (ORCID:0000-0002-1436-6105), Iavarone F. (ORCID:0000-0002-2074-5531), Desiderio C., Rossetti D. V., Fiorita A., Castagnola M. (ORCID:0000-0002-0959-7259), Messana, Irene, Manconi, B., Cabras, T., Boroumand, M., Sanna, M. T., Iavarone, Federica, Olianas, A., Desiderio, Claudia, Rossetti, Diana Valeria, Vincenzoni, F., Contini, C., Guadalupi, G., Fiorita, Antonella, Faa, G., Castagnola, Massimo, Messana I. (ORCID:0000-0002-1436-6105), Iavarone F. (ORCID:0000-0002-2074-5531), Desiderio C., Rossetti D. V., Fiorita A., and Castagnola M. (ORCID:0000-0002-0959-7259)

Abstract

In this review, we extensively describe the main post-translational modifications that give rise to the multiple proteoforms characterized to date in the human salivary proteome and their potential role. Most of the data reported were obtained by our group in over twenty-five years of research carried out on human saliva mainly by applying a top-down strategy. In the beginning, we describe the products generated by proteolytic cleavages, which can occur before and after secretion. In this section, the most relevant families of salivary proteins are also described. Next, we report the current information concerning the human salivary phospho-proteome and the limited news available on sulfo-proteomes. Three sections are dedicated to the description of glycation and enzymatic glycosylation. Citrullination and N- and C-terminal post-translational modifications (PTMs) and miscellaneous other modifications are described in the last two sections. Results highlighting the variation in the level of some proteoforms in local or systemic pathologies are also reviewed throughout the sections of the manuscript to underline the impact and relevance of this information for the development of new diagnostic biomarkers useful in clinical practice.

Published
2023

8. A top-down proteomic approach reveals a salivary protein profile able to classify Parkinson's disease with respect to Alzheimer's disease patients and to healthy controls

Author

Contini, C., Fadda, L., Lai, Giampaolo, Masala, C., Olianas, A., Castagnola, Massimo, Messana, Irene, Iavarone, Federica, Bizzarro, Alessandra, Masullo, Carlo, Solla, P., Defazio, G., Manconi, B., Diaz, G., Cabras, T., Lai G., Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), Iavarone F. (ORCID:0000-0002-2074-5531), Bizzarro A., Masullo C. (ORCID:0000-0001-7798-3410), Contini, C., Fadda, L., Lai, Giampaolo, Masala, C., Olianas, A., Castagnola, Massimo, Messana, Irene, Iavarone, Federica, Bizzarro, Alessandra, Masullo, Carlo, Solla, P., Defazio, G., Manconi, B., Diaz, G., Cabras, T., Lai G., Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), Iavarone F. (ORCID:0000-0002-2074-5531), Bizzarro A., and Masullo C. (ORCID:0000-0001-7798-3410)

Abstract

Parkinson's disease (PD) is a complex neurodegenerative disease with motor and non-motor symptoms. Diagnosis is complicated by lack of reliable biomarkers. To individuate peptides and/or proteins with diagnostic potential for early diagnosis, severity and discrimination from similar pathologies, the salivary proteome in 36 PD patients was investigated in comparison with 36 healthy controls (HC) and 35 Alzheimer's disease (AD) patients. A top-down platform based on HPLC-ESI-IT-MS allowed characterizing and quantifying intact peptides, small proteins and their PTMs (overall 51). The three groups showed significantly different protein profiles, PD showed the highest levels of cystatin SA and antileukoproteinase and the lowest of cystatin SN and some statherin proteoforms. HC exhibited the lowest abundance of thymosin & beta;4, short S100A9, cystatin A, and dimeric cystatin B. AD patients showed the highest abundance of & alpha;-defensins and short oxidized S100A9. Moreover, different proteoforms of the same protein, as S-cysteinylated and S-glutathionylated cystatin B, showed opposite trends in the two pathological groups. Statherin, cystatins SA and SN classified accurately PD from HC and AD subjects. & alpha;-defensins, histatin 1, oxidized S100A9, and P-B fragments were the best classifying factors between PD and AD patients. Interestingly statherin and thymosin & beta;4 correlated with defective olfactory functions in PD patients. All these outcomes highlighted implications of specific proteoforms involved in the innate-immune response and inflammation regulation at oral and systemic level, suggesting a possible panel of molecular and clinical markers suitable to recognize subjects affected by PD.

Published
2023

10. Altered mitochondrial function in cells carrying a premutation or unmethylated full mutation of the FMR1 gene

Author

Nobile, V., Palumbo, F., Lanni, S., Ghisio, V., Vitali, A., Castagnola, M., Marzano, V., Maulucci, G., De Angelis, C., De Spirito, M., Pacini, L., D'Andrea, L., Ragno, R., Stazi, G., Valente, S., Mai, A., Chiurazzi, P., Genuardi, M., Neri, G., Tabolacci, E., Nobile V., Castagnola M. (ORCID:0000-0002-0959-7259), Marzano V., Maulucci G. (ORCID:0000-0002-2154-319X), De Angelis C., De Spirito M. (ORCID:0000-0003-4260-5107), D'Andrea L., Chiurazzi P. (ORCID:0000-0001-5104-1521), Genuardi M. (ORCID:0000-0002-7410-8351), Tabolacci E. (ORCID:0000-0002-4707-2242), Nobile, V., Palumbo, F., Lanni, S., Ghisio, V., Vitali, A., Castagnola, M., Marzano, V., Maulucci, G., De Angelis, C., De Spirito, M., Pacini, L., D'Andrea, L., Ragno, R., Stazi, G., Valente, S., Mai, A., Chiurazzi, P., Genuardi, M., Neri, G., Tabolacci, E., Nobile V., Castagnola M. (ORCID:0000-0002-0959-7259), Marzano V., Maulucci G. (ORCID:0000-0002-2154-319X), De Angelis C., De Spirito M. (ORCID:0000-0003-4260-5107), D'Andrea L., Chiurazzi P. (ORCID:0000-0001-5104-1521), Genuardi M. (ORCID:0000-0002-7410-8351), and Tabolacci E. (ORCID:0000-0002-4707-2242)

Abstract

Fragile X-related disorders are due to a dynamic mutation of the CGG repeat at the 5′ UTR of the FMR1 gene, coding for the RNA-binding protein FMRP. As the CGG sequence expands from premutation (PM, 56-200 CGGs) to full mutation (> 200 CGGs), FMRP synthesis decreases until it is practically abolished in fragile X syndrome (FXS) patients, mainly due to FMR1 methylation. Cells from rare individuals with no intellectual disability and carriers of an unmethylated full mutation (UFM) produce slightly elevated levels of FMR1-mRNA and relatively low levels of FMRP, like in PM carriers. With the aim of clarifying how UFM cells differ from CTRL and FXS cells, a comparative proteomic approach was undertaken, from which emerged an overexpression of SOD2 in UFM cells, also confirmed in PM but not in FXS. The SOD2-mRNA bound to FMRP in UFM more than in the other cell types. The high SOD2 levels in UFM and PM cells correlated with lower levels of superoxide and reactive oxygen species (ROS), and with morphological anomalies and depolarization of the mitochondrial membrane detected through confocal microscopy. The same effect was observed in CTRL and FXS after treatment with MC2791, causing SOD2 overexpression. These mitochondrial phenotypes reverted after knock-down with siRNA against SOD2-mRNA and FMR1-mRNA in UFM and PM. Overall, these data suggest that in PM and UFM carriers, which have high levels of FMR1 transcription and may develop FXTAS, SOD2 overexpression helps to maintain low levels of both superoxide and ROS with signs of mitochondrial degradation.

Published
2020

11. The human carotid atherosclerotic plaque: an observational review of histological scoring systems.

Author

GEROSA, C., CERRONE, G., SURI, J. S., AIMOLA, V., CAU, F., CONI, P., PIRAS, M., CAU, R., BALESTRIERI, A., SCANO, A., ORRÙ, G., VAN EYKEN, P., LA NASA, G., COGHE, F., CASTAGNOLA, M., GIBO, Y., FANNI, D., and SABA, L.

Abstract

OBJECTIVE: The atherosclerotic plaque is a complex dynamic pathological lesion of the arterial wall, characterized by multiple elementary lesions of different diagnostic and prognostic significance. Fibrous cap thickness, lipid necrotic core dimension, inflammation, intra-plaque hemorrhage (IPH), plaque neovascularization and endothelial dysfunction (erosions) are generally considered the most relevant morphological details of plaque morphology. In this review, the most relevant features able to discriminate between stable and vulnerable plaques at histological level are discussed. SUBJECTS AND METHODS: Retrospectively, we have evaluated the laboratory results from one hundred old histological samples from patients treated with carotid endarterectomy. These results were analyzed to assess elementary lesions that characterize stable and unstable plaques. RESULTS: A thin fibrous cap (<65 micron), loss of smooth muscle cells, collagen depletion, a large lipid-rich necrotic core, infiltrating macrophages, IPH and intra-plaque vascularization are identified as the most important risk factors associated with plaque rupture. CONCLUSIONS: Immunohistochemistry for smooth muscle actin (smooth muscle cell marker) and for CD68 (marker of monocytes/macrophages) and glycophorin (marker of red blood cells) are suggested as useful tools for an in deep characterization of any carotid plaque and for distinguishing plaque phenotypes at histology. Since patients with a carotid vulnerable plaque are at higher risk of developing vulnerable plaques in other arteries as well, the definition of the vulnerability index is underlined, in order to stratify patients at higher risk for undergoing cardiovascular events. [ABSTRACT FROM AUTHOR]

Published
2023

13. Molecular pathways triggered by COVID-19 in different organs: ACE2 receptor-expressing cells under attack? A review

Author

Saba L., Gerosa C., Fanni D., Marongiu F., Nasa G. L. A., Caocci G., Barcellona D., Balestrieri A., Coghe F., Orru G., Coni P., Piras M., Ledda F., Suri J. S., Ronchi A., D'Andrea F., Cau R., Castagnola M., Faa G., Saba, L., Gerosa, C., Fanni, D., Marongiu, F., Nasa, G. L. A., Caocci, G., Barcellona, D., Balestrieri, A., Coghe, F., Orru, G., Coni, P., Piras, M., Ledda, F., Suri, J. S., Ronchi, A., D'Andrea, F., Cau, R., Castagnola, M., and Faa, G.

Subjects
Liver Cirrhosis, COVID -19, Molecular pathway, Fibrosi, Liver Cirrhosi, Myocarditi, ACE2, Capillary Permeability, Renin-Angiotensin System, SARS- COV-2, Atrial Fibrillation, Humans, Cytokine, Blood Coagulation, Cardiomyopathie, SARS-CoV-2, Angiotensin II, Receptors, Coronaviru, COVID-19, Thrombosis, Fibroblasts, Virus Internalization, Fibrosis, Systemic Inflammatory Response Syndrome, Myocarditis, Thrombosi, Fibroblast, Cytokines, Angiotensin-Converting Enzyme 2, Endothelium, Vascular, Angiotensin I, Cardiomyopathies, Cytokine Release Syndrome, Human, Receptors, Coronavirus
Abstract

OBJECTIVE: In human pathology, SARS-CoV-2 utilizes multiple molecular pathways to determine structural and biochemical changes within the different organs and cell types. The clinical picture of patients with COVID-19 is characterized by a very large spectrum. The reason for this variability has not been clarified yet, causing the inability to make a prognosis on the evolution of the disease. MATERIALS AND METHODS: PubMed search was performed focusing on the role of ACE 2 receptors in allowing the viral entry into cells, the role of ACE 2 downregulation in triggering the tissue pathology or in accelerating previous disease states, the role of increased levels of Angiotensin II in determining endothelial dysfunction and the enhanced vascular permeability, the role of the dysregulation of the renin angiotensin system in COVID-19 and the role of cytokine storm. RESULTS: The pathological changes induced by SARS-CoV-2 infection in the different organs, the correlations between the single cell types targeted by the virus in the different human organs and the clinical consequences, COVID-19 chronic pathologies in liver fibrosis, cardiac fibrosis and atrial arrhythmias, glomerulosclerosis and pulmonary fibrosis, due to the systemic fibroblast activation induced by angiotensin II are discussed. CONCLUSIONS: The main pathways involved showed different pathological changes in multiple tissues and the different clinical presentations. Even if ACE2 is the main receptor of SARS-CoV-2 and the main entry point into cells for the virus, ACE2 expression does not always explain the observed marked inter-individual variability in clinical presentation and outcome, evidencing the complexity of this disorder. The proper interpretation of the growing data available might allow to better classifying COVID-19 in human pathology.

Published
2020

15. Liver changes in Wilson's disease: the full spectrum. A report of 127 biopsies from 43 patients

Author

Fanni, D., Guido, M., Gerosa, C., Vallascas, V., Moi, M., Coni, P., Vallebona, E., van Eyken, P., Barcellona, D., Scano, A., Orru, G., Pampaloni, P., Castagnola, M., and Faa, G.

Subjects
Adult, Male, Steatosis, Adolescent, Histopathology, Infant, Ballooning, Fibrosis, Liver, Wilson disease, Middle Aged, Young Adult, Hepatolenticular Degeneration, Child, Preschool, Humans, Female, Child
Abstract

Wilson's Disease (WD) is an autosomal recessive copper overload. Several mutations of the copper pump named ATP7B have been involved. WD is difficult to diagnose mainly because of its heterogeneity of presentation. The histologic spectrum is wide and not specific, ranging from very mild changes to severe disease. The histological picture of WD may overlap different conditions, including ALD, NAFLD, viral hepatitis or autoimmune liver disease.We describe our experience on WD based on a single-center series of liver biopsies. One-hundred twenty-seven liver samples from 43 Sardinian WD patients were reviewed. The most reported pattern was steatohepatitis, accounting 82/127 biopsies (64.6%), followed by hepatitis in 25 biopsies (19.7%), and steatosis in 20 biopsies (15.7%).As for the elementary lesions, inflammation, steatosis, glycogenated nuclei and ballooning were the most frequent, being found in 107, 102, 90 and 86 biopsies out of the 127. Notably, all these lesions showed a predominant periportal location. There was no significant difference in the diagnostic pattern or in each elementary lesion between the biopsies performed at presentation and those performed during the follow-up. Lipogranuloma (significantly more numerous in the follow-up biopsies) and fibrosis (likewise significantly progressed in follow-up biopsies) were the only exceptions.Our data confirm the variability of the histological pattern in WD. However, the preferential localization of steatosis and balloon cells in periportal zone can be a useful clue for the diagnosis of WD.

Published
2021

16. Expression of L1 Cell Adhesion Molecule (L1CAM) in extracellular vesicles in the human spinal cord during development.

Author

CAU, F., FANNI, D., MANCHIA, M., GEROSA, C., PIRAS, M., MURRU, R., PARIBELLO, P., CONGIU, T., CONI, P., PICHIRI, G., PILUDU, M., VAN EYKEN, P., GIBO, Y., LA NASA, G., ORRÙ, G., SCANO, A., COGHE, F., SABA, L., CASTAGNOLA, M., and FAA, G.

Abstract

OBJECTIVE: L1 cell adhesion molecule (L1CAM) is a glycoprotein characterized by three components: an extracellular region, a transmembrane segment, and a cytoplasmic tail. L1CAM is expressed in multiple human cells, including neurons. The neural cell adhesion molecule L1 has been implicated in a variety of neurologic processes, including neuritogenesis and cerebellar cell migration. The presence of L1CAM on the surface of nerve cells allows the adhesion of neurons among them. Furthermore, when it is bound to itself or to other proteins, L1-CAM induces signals inside the cell. The aim of this work was to study L1CAM expression in the human spinal cord during development, at different gestational ages, through immunohistochemistry. MATERIALS AND METHODS: Immunohistochemical analysis for L1CAM was performed in five human spinal cord samples, including three embryos and two fetuses of different gestational ages, ranging from 8 to 12 weeks. RESULTS: L1CAM expression was detected in all 5 spinal cords examined in this study. The adhesion molecule was found in the vast majority of cells. The highest levels of immunoreactivity for L1CAM were detected at the periphery of the developing organs, in the spinal cord zones occupied by sensory and motor fibers. In the alar and basal columns, immunoreactivity for L1CAM was characterized by a reticular pattern, being mainly expressed in axons. Strong reactivity of L1CAM was also found in extracellular vesicles. This extracellular localization might indicate the ability of L1CAM to mediate the transduction of extracellular signals that support axon outgrowth. CONCLUSIONS: The high reactivity of L1cam in the axons of developing neurons in the fetal spinal cord confirms previous studies on the ability of L1CAM to promote axon sprouting and branching in the developing nervous system. In this work, a new actor is reported to have a role in the complex field of human spinal cord development: L1CAM, whose expression is highly found in the developing neuronal and glial precursors. [ABSTRACT FROM AUTHOR]

Published
2022

17. Oct-4 is highly expressed in stem/progenitor cells and in primordial follicles of the fetal human ovary

Author

Cau, F., Fanni, D., Gerosa, C., Botta, M. C., Bardanzellu, F., Aversa, S., Sorrentino, E., Ronchi, F., Bellan, C., Faa, G., and Castagnola, M.

Subjects
ovarian stem, genetic structures, ovarian stem cells, lcsh:R, oct-4, lcsh:RJ1-570, lcsh:Medicine, lcsh:Pediatrics, progenitor cells, fetal ovary, development, immunohistochemistry, Oct-4, primordial follicles, eye diseases, Oct-4 expression, sense organs
Abstract

Oct-4 (Octamer-binding transcription factor 4) is a member of the POU (Pit-Oct-Unc) family. During development, Oct-4 is expressed in embryonic stem cells and in germ cell precursors. In this study, we investigated the expression of Oct-4 in the ovaries of human fetuses during gestation. The ovaries of 14 human fetuses and newborns, ranging in gestational age from 12 up to 38 weeks of gestation, were formalin-fixed, routinely processed and paraffin-embedded. Paraffin sections were immunostained with an anti-Oct-4 commercial antibody. Oct-4 expression was demonstrated in all the ovaries analyzed. Immunoreactivity for Oct-4 was detected in multiple stem/progenitor cells, including oogonia. Moreover, Oct-4 was expressed in oocytes, in primordial follicles. In ovarian stem/progenitor cells, Oct-4 was expressed in the nucleus, whereas in oocytes reactivity for Oct-4 was restricted to the cytoplasm. In the initial stages of gestation, the majority of Oct-4-positive precursor cells were detected in the external cortex. These preliminary data indicate Oct-4 as a major player in germ cell differentiation in the human ovary and as a useful marker for ovarian stem/progenitor cells. Given the ability of Oct-4 for the detection of ovarian stem/progenitor cells, further studies are needed in order to verify its ability to detect stem cells in adult ovaries.

Published
2021

18. Oxidative and Proteolytic Inactivation of Alpha-1 Antitrypsin in Bronchopulmonary Dysplasia Pathogenesis: A Top-Down Proteomic Bronchoalveolar Lavage Fluid Analysis

Author

Tirone, Chiara, Iavarone, Federica, Tana, Milena, Lio, Alessandra, Aurilia, Claudia, Costa, Simonetta, Castagnola, Massimo, Messana, Irene, Vento, Giovanni, Tirone C., Iavarone F. (ORCID:0000-0002-2074-5531), Tana M., Lio A., Aurilia C., Costa S., Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), Vento G. (ORCID:0000-0002-8132-5127), Tirone, Chiara, Iavarone, Federica, Tana, Milena, Lio, Alessandra, Aurilia, Claudia, Costa, Simonetta, Castagnola, Massimo, Messana, Irene, Vento, Giovanni, Tirone C., Iavarone F. (ORCID:0000-0002-2074-5531), Tana M., Lio A., Aurilia C., Costa S., Castagnola M. (ORCID:0000-0002-0959-7259), Messana I. (ORCID:0000-0002-1436-6105), and Vento G. (ORCID:0000-0002-8132-5127)

Abstract

The study investigates the role of the oxidative and proteolytic inactivation of alpha-1 antitrypsin (AAT) in the pathogenesis of bronchopulmonary dysplasia (BPD) in premature infants. Bronchoalveolar lavage fluid (BALF) samples were collected on the 3rd day of life from mechanically ventilated neonates with gestational age ≤ 30 weeks and analyzed without previous treatment (top-down proteomics) by reverse-phase high-performance liquid chromatography-electrospray ionization mass spectrometry. AAT fragments were identified by high-resolution LTQ Orbitrap XL experiments and the relative abundances determined by considering the extracted ion current (XIC) peak area. Forty preterm neonates were studied: 20 (50%) did not develop BPD (no-BPD group), 17 (42.5%) developed mild or moderate new-BPD (mild + moderate BPD group), and 3 (7.5%) developed severe new-BPD (severe BPD group). Eighteen fragments of AAT and a fragment of AAT oxidized at a methionine residue were identified: significantly higher values of AAT fragments 25–57, 375–418, 397–418, 144–171, and 397–418 with oxidized methionine were found in the severe BPD group. The significantly higher levels of several AAT fragments and of the fragment 397–418, oxidized in BALF of preterm infants developing BPD, underlie the central role of an imbalance between proteases and protease inhibitors in exacerbating lung injury and inducing most severe forms of BPD. The study has some limitations, and between them, the small sample size implies the need for further confirmation by larger studies.

Published
2021

19. C9ORF72 repeat expansion affects the proteome of primary skin fibroblasts in ALS

Author

Lualdi, M., Shafique, A., Pedrini, E., Pieroni, L., Greco, Viviana, Castagnola, M., Cucina, G., Corrado, L., Di Pierro, A., De Marchi, F., Camillo, L., Colombrita, C., D'Anca, M., Alberio, T., D'Alfonso, S., Fasano, M., Greco V. (ORCID:0000-0003-4521-0020), Lualdi, M., Shafique, A., Pedrini, E., Pieroni, L., Greco, Viviana, Castagnola, M., Cucina, G., Corrado, L., Di Pierro, A., De Marchi, F., Camillo, L., Colombrita, C., D'Anca, M., Alberio, T., D'Alfonso, S., Fasano, M., and Greco V. (ORCID:0000-0003-4521-0020)

Abstract

Amyotrophic lateral sclerosis (ALS) is a neurodegenerative disease characterized by pro-gressive degeneration of the corticospinal motor neurons, which ultimately leads to death. The repeat expansion in chromosome 9 open reading frame 72 (C9ORF72) represents the most common genetic cause of ALS and it is also involved in the pathogenesis of other neurodegenerative disorders. To offer insights into C9ORF72-mediated pathogenesis, we quantitatively analyzed the proteome of patient-derived primary skin fibroblasts from ALS patients carrying the C9ORF72 mutation compared with ALS patients who tested negative for it. Differentially expressed proteins were identified, used to generate a protein-protein interaction network and subjected to a functional enrichment analysis to unveil altered molecular pathways. ALS patients were also compared with patients affected by frontotemporal dementia carrying the C9ORF72 repeat expansion. As a result, we demonstrated that the molecular pathways mainly altered in fibroblasts (e.g., protein homeostasis) mirror the alterations observed in C9ORF72-mutated neurons. Moreover, we highlighted novel molecular pathways (nuclear and mitochondrial transports, vesicle trafficking, mitochondrial bioenergetics, glucose metabolism, ER-phagosome crosstalk and Slit/Robo signaling pathway) which might be further investigated as C9ORF72-specific pathogenetic mechanisms. Data are available via ProteomeXchange with the identifier PXD023866.

Published
2021

20. HPLC-ESI-MS top-down analysis of salivary peptides of preterm newborns evidenced high activity of some exopeptidases and convertases during late fetal development

Author

Boroumand, M., Iavarone, F., Manconi, B., Pieroni, L., Greco, V., Vento, G., Tirone, C., Desiderio, C., Fiorita, A., Faa, G., Messana, I., Cabras, T., Olianas, A., Castagnola, M., Greco V. (ORCID:0000-0003-4521-0020), Boroumand, M., Iavarone, F., Manconi, B., Pieroni, L., Greco, V., Vento, G., Tirone, C., Desiderio, C., Fiorita, A., Faa, G., Messana, I., Cabras, T., Olianas, A., Castagnola, M., and Greco V. (ORCID:0000-0003-4521-0020)

Abstract

To have information on the proteolytic activity of convertases and exo-peptidases on human salivary proteins, this study investigated the relative amounts of the truncated proteoforms in the saliva of preterm newborns and compared them with the relative amounts measured in saliva of at-term newborns, of babies (0–10 years old) and of adults. Results indicated that convertase(s), acting on acidic proline-rich proteins and histatin 3, and carboxypeptidase(s) acting on acidic proline-rich proteins, P–C peptide, histatin 6 and statherin were many folds more active in preterm newborns than in the other groups. Conversely, the aminopeptidase responsible for the removal of the N-terminal Asp residue of statherin was not active in preterm newborns, becoming active only several months after the normal term of delivery. The high activity of convertases determined in preterm newborns suggests that it is required for the molecular events connected to the fetus development, and encourages further studies devoted to the characterization of their specific substrates.

Published
2021

21. Anastomotic leaks after anterior resection for mid and low rectal cancer: survey of the Italian Society of Colorectal Surgery

Author

Asteria, C. R., Gagliardi, G., Pucciarelli, S., Romano, G., Infantino, A., La Torre, F., Tonelli, F., Martin, F., Pulica, C., Ripetti, V., Diana, G., Amicucci, G., Carlini, M., Sommariva, A., Vinciguerra, G., Poddie, D. B., Amato, A., Bassi, R., Galleano, R., Veronese, E., Mancini, S., Pescio, G., Occelli, G. L., Bracchitta, S., Castagnola, M., Pontillo, T., Cimmino, G., Prati, U., and Vincenti, R.

Published
2008
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22. Interindividual variability in L1CAM expression in the human kidney during development: are there implications for fetal programming of kidney diseases presenting in adulthood?

Author

CAU, F., GEROSA, C., MURRU, R., PICHIRI, G., CONI, P., PIRAS, M., SCANO, A., ORRÙ, G., LA NASA, G., COGHE, F., CASTAGNOLA, M., VAN EYKEN, P., SABA, L., FANNI, D., and FAA, G.

Abstract

OBJECTIVE: L1 cell adhesion molecule (L1CAM) is a member of the immunoglobulin superfamily of cell adhesion molecules. The present study investigated the expression of L1CAM during the development in the fetal human kidney at different gestational ages, to reach a better knowledge on the role of L1CAM in renal morphogenesis. MATERIALS AND METHODS: The immunohistochemical analysis for L1CAM was performed in 24 fetal kidneys of different gestational ages, ranging from 10 to 38 weeks. L1CAM expression was observed in all 24 kidneys examined. RESULTS: Immunoreactivity for L1CAM was restricted to the collecting tubules, of the developing fetal kidneys. Moreover, L1CAM was detected in the ureteric bud tips, near the subcapsular metanephric mesenchymal stem/progenitor cells. L1CAM was also expressed in the collecting tubules undergoing fusion with the distal tubules of the developing nephrons. L1CAM was mainly expressed along the cell membrane. In fetal kidneys in which the renal pelvis was observed, epithelial cells of the renal pelvis showed strong membranous reactivity for L1CAM. CONCLUSIONS: Our study shows that L1CAM is expressed in all stages of human kidney nephrogenesis, being restricted to the renal structures derived from the ureteric bud. The expression of L1CAM in the cells of the ureteric bud tips suggests a major role for this adhesion molecule in the induction of metanephric mesenchymal cells to undergo mesenchymal-to-epithelial transition and differentiation into new nephrons. The interindividual variability in L1CAM expression observed in this study might be related to different levels of nephrogenesis, suggesting L1CAM involvement in the fetal programming of adult kidney diseases. [ABSTRACT FROM AUTHOR]

Published
2022

23. Proteomic identification of altered protein O-GlcNAcylation in a triple transgenic mouse model of Alzheimer's disease

Author

Tramutola, A., Sharma, N., Barone, E., Lanzillotta, C., Castellani, A., Iavarone, F., Vincenzoni, F., Castagnola, M., Butterfield, D. A., Gaetani, S., Cassano, T., Perluigi, M., Di Domenico, F., Iavarone F. (ORCID:0000-0002-2074-5531), Castagnola M. (ORCID:0000-0002-0959-7259), Tramutola, A., Sharma, N., Barone, E., Lanzillotta, C., Castellani, A., Iavarone, F., Vincenzoni, F., Castagnola, M., Butterfield, D. A., Gaetani, S., Cassano, T., Perluigi, M., Di Domenico, F., Iavarone F. (ORCID:0000-0002-2074-5531), and Castagnola M. (ORCID:0000-0002-0959-7259)

Abstract

PET scan analysis demonstrated the early reduction of cerebral glucose metabolism in Alzheimer disease (AD) patients that can make neurons vulnerable to damage via the alteration of the hexosamine biosynthetic pathway (HBP). Defective HBP leads to flawed protein O-GlcNAcylation coupled, by a mutual inverse relationship, with increased protein phosphorylation on Ser/Thr residues. Altered O-GlcNAcylation of Tau and APP have been reported in AD and is closely related with pathology onset and progression. In addition, type 2 diabetes patients show an altered O-GlcNAcylation/phosphorylation that might represent a link between metabolic defects and AD progression. Our study aimed to decipher the specific protein targets of altered O-GlcNAcylation in brain of 12-month-old 3×Tg-AD mice compared with age-matched non-Tg mice. Hence, we analysed the global O-GlcNAc levels, the levels and activity of OGT and OGA, the enzymes controlling its cycling and protein specific O-GlcNAc levels using a bi-dimensional electrophoresis (2DE) approach. Our data demonstrate the alteration of OGT and OGA activation coupled with the decrease of total O-GlcNAcylation levels. Data from proteomics analysis led to the identification of several proteins with reduced O-GlcNAcylation levels, which belong to key pathways involved in the progression of AD such as neuronal structure, protein degradation and glucose metabolism. In parallel, we analysed the O-GlcNAcylation/phosphorylation ratio of IRS1 and AKT, whose alterations may contribute to insulin resistance and reduced glucose uptake. Our findings may contribute to better understand the role of altered protein O-GlcNAcylation profile in AD, by possibly identifying novel mechanisms of disease progression related to glucose hypometabolism.

Published
2018

24. Exploring the HeLa Dark Mitochondrial Proteome

Author

Marini, F, Carregari, Vc, Greco, Viviana, Ronci, M, Iavarone, Federica, Persichilli, Silvia, Castagnola, Massimo, Urbani, Andrea, Pieroni, L, Greco V (ORCID:0000-0003-4521-0020), Iavarone F (ORCID:0000-0002-2074-5531), Persichilli S (ORCID:0000-0002-7955-8810), Castagnola M (ORCID:0000-0002-0959-7259), Urbani A (ORCID:0000-0001-9168-3174), Marini, F, Carregari, Vc, Greco, Viviana, Ronci, M, Iavarone, Federica, Persichilli, Silvia, Castagnola, Massimo, Urbani, Andrea, Pieroni, L, Greco V (ORCID:0000-0003-4521-0020), Iavarone F (ORCID:0000-0002-2074-5531), Persichilli S (ORCID:0000-0002-7955-8810), Castagnola M (ORCID:0000-0002-0959-7259), and Urbani A (ORCID:0000-0001-9168-3174)

Abstract

In the framework of the Human Proteome Project initiative, we aim to improve mapping and characterization of mitochondrial proteome. In this work we implemented an experimental workflow, combining classical biochemical enrichments and mass spectrometry, to pursue a much deeper definition of mitochondrial proteome and possibly mine mitochondrial uncharacterized dark proteins. We fractionated in two compartments mitochondria enriched from HeLa cells in order to annotate 4230 proteins in both fraction by means of a multiple-enzyme digestion (trypsin, chymotrypsin and Glu-C) followed by mass spectrometry analysis using a combination of Data Dependent Acquisition (DDA) and Data Independent Acquisition (DIA). We detected 22 mitochondrial dark proteins not annotated for their function and we provide their relative abundance inside the mitochondrial organelle. Considering this work as a pilot study we expect that the same approach, in different biological system, could represent an advancement in the characterization of the human mitochondrial proteome providing uncharted ground to explore the mitonuclear phenotypic relationships. All spectra have been deposited to ProteomeXchange with PXD014201 and PXD014200 identifier.

Published
2020

28. Acyl-CoA binding protein (ACBP) is highly expressed in the developing human kidney.

Author

PIRAS, M., GEROSA, C., FANNI, D., CAU, F., CONI, P., MURRU, R., DENOTTI, G., ORRÙ, G., SCANO, A., LEDDA, F., VAN EYKEN, P., COGHE, F., FAA, G., and CASTAGNOLA, M.

Abstract

OBJECTIVE: Acyl-CoA-binding protein (ACBP), also known as diazepam binding inhibitor (DBI), is a small phylogenetically conserved protein. This ancestral peptide is multifunctional, performing intracellular activities as ACBP protein or extracellular roles as DBI. Several studies showed its endless facets, including a relevant activity as appetite stimulator and as anabolic factor. High levels of ACBP have been described in erythrocytes, liver, kidney, and gut cells. The aim of this study was to analyze, at immunohistochemical level, the expression of ACBP in fetal human tissues during development, focusing on the developing kidney. MATERIALS AND METHODS: Immunohistochemistry for ACBP was performed on 30 human fetal kidneys, from 15 fetuses of gestational age ranging from 13 to 19 weeks. At autopsy, all kidney samples were 10% formalin-fixed, routinely processed and paraffin-embedded. Five micron-thick paraffin sections were stained with Hematoxylin and Eosin and PAS stain for a morphological examination. RESULTS: ACBP was detected in all 30 kidneys analyzed in this study. No significant changes in ACBP expression were observed at different gestational ages. Immunostaining for ACBP was restricted to the epithelium covering the renal pelvis, the papillae, the collecting tubules, and the proximal and distal tubules. On the other hand, medullary regions and in the metanephric mesenchymal stem/progenitor cells did not show any reactivity for ACBP. CONCLUSIONS: According to our findings, ACBP should be considered as a new player in the complex field of human nephrogenesis, given that it was detected in all fetal kidneys immunostained. Its preferential localization in the renal structures derived from the Wolf duct, such as pelvis epithelium and collecting ducts, suggests a major role for ACBP in the induction of the metanephric mesenchymal cells toward the differentiation into glomerular structures. ACBP expression in proximal and distal tubules, two structures originating from the metanephric mesenchyme, indicates a further role of this protein in nephron development. In conclusion, ACBP should be added to the multiple molecules involved in human nephrogenesis. [ABSTRACT FROM AUTHOR]

Published
2022

29. Strong ACE-2 expression in the choroidal vessels: do high choroid plexuses serve as a gateway for SARS-CoV-2 infection on the human brain?

Author

PIRAS, M., CAU, F., MANCHIA, M., PARIBELLO, P., SABA, L., SURI, J. S., FAA, G., PICHIRI, G., CERRONE, G., SCANO, A., ORRÙ, G., LA NASA, G., COGHE, F., CASTAGNOLA, M., FANNI, D., and GEROSA, C.

Abstract

OBJECTIVE: Previous studies have confirmed the key mechanism by which SARS-CoV-2 enters human cells. It is well established that ACE2 is the receptor that can mark the beginning of the infection. In light of this, the organs that express higher levels of ACE2 are generally considered at higher risk, while those with lower levels should be somehow more protected. This - if related to the scarcity of ace2-expressing cells in the brain - seems to contrast with the presence of a variety of neurological symptoms that follow infection with ace2. The aim of this work was to analyze ACE2 expression in the human brain, focusing on the choroid plexuses. PATIENTS AND METHODS: Twenty brain samples were obtained at autopsy from ten human fetuses and from ten adult subjects. All samples were selected to contain the choroid plexus. Specimens were fixed in 10% formalin, routinely processed and paraffin embedded. 5-micron sections were stained with Hematoxylin and Eosin (H&E) and immunostained with a commercial anti-human ACE2 rabbit monoclonal antibody at 1:100 dilution. RESULTS: We analyzed 20 samples by immunohistochemistry, and we noted that, as far as fetal samples are concerned, a strong reactivity for ACE2 was detected in the myxoid stroma of the choroid plexuses and in the endothelial cells in fetuses. The complete absence of the ACE2 marker was detected in epithelial cells, neurons and glial cells of the cerebral cortex, both in fetuses and in adults. Whereas a strong but selective reactivity for ACE2 was also detected in adult choroid plexuses, mainly localized in the endothelial cells of the choroid capillaries. CONCLUSIONS: Our study shows a strong expression of ACE in the fetal and adult brain choroid plexuses. This new histopathological finding may clarify the susceptibility of the human brain to SARS-COV-2 infection. Our data indicate the choroid plexus as the entry gate of virus for in the human brain; therefore, the entrance of SARS-CoV-2 into the cerebrospinal fluid through the choroid plexuses might represent the mechanism utilized by this coronavirus to cause direct injury to brain cells. [ABSTRACT FROM AUTHOR]

Published
2022

31. Determination of Biophysical Parameters of Polypeptide Retro - Inverso Isomers and Their Analogues by Capillary electrophoresis

Author

Hearn, M.T.W., Keah, H.H., Boysen, R.I., Messana, I., Misiti, F., Rossetti, D.V., Giardina, B., and Castagnola, M.

Subjects
Polypeptides -- Research, Electrophoresis -- Usage, Chemistry
Abstract

The relationship between the electrophoretic mobility, (mu)(sub obs), Stokes radius, r(sub s), ionization state, and solution conformation of the all L-(alpha)-polypeptide, 1, the corresponding retro-all D-(alpha)-polypeptide, 2, and several truncated analogues, 3-5, has been investigated under low pH buffer conditions by high-performance capillary zonal electrophoresis (HPCZE) with coated capillaries. The results confirm that, under these conditions, all L-(alpha)-polypeptide, 1, and its retro-inverso isomer, 2, exhibit nonidentical electrophoretic mobilities and thus different Stokes radii. At higher pH values, i.e., pH 5.0, the electrophoretic behavior of this retro-inverso isomer pair, however, converges. These results indicate that variations in the dipole characteristics of the polypeptide main chain and subtle differences introduced by the spatial constraints of the L-(alpha)-Pro > d-(alpha)-Pro residue replacement lead to differences in the Stokes radii and electrophoretic mobilities of these polypeptides. Since the observed electrophoretic mobilities, (mu)(sub obs), reflect the mean of the mobilities of each charge species participating according to their Stokes radius or their intrinsic charge and mole fraction abundances, the results confirm that polypeptide retro-inverso isomers with unmodified amino and carboxy termini are resolvable. This outcome was achieved despite their notional topographical and conformational similarities as assessed from high-field proton nuclear magnetic resonance ((super 1)H NMR) spectroscopy and circular dichroism (CD) spectroscopy.

Published
2000

33. Thymosin β4 and β10 are highly expressed at the deep infiltrative margins of colorectal cancer - A mass spectrometry analysis.

Author

OLIANAS, A., SERRAO, S., PIRAS, V., MANCONI, B., CONTINI, C., IAVARONE, F., PICHIRI, G., CONI, P., ZORCOLO, L., ORRÙ, G., MESSANA, I., FAA, G., CASTAGNOLA, M., FANNI, D., and CABRAS, T.

Abstract

OBJECTIVE: Colorectal cancer (CRC) is a complicated tumor, involving several oncogenic signaling pathways, and with a molecular mechanism not fully understood yet. The implication of thymosin β4 (Tβ4) with tumor in-surgence and in migration of CRC cells was evidenced in the past with different methodologies, while Tβ10 connection with CRC has been sporadically investigated. This study focused on the implication of both types of thymosin in CRC progression and invasion by analyzing the changes in their levels according to different zones of the tumor, and to Dukes stage and budding index. PATIENTS AND METHODS: Tβ4 and Tβ10 were analyzed in deep and superficial tumor samples, and normal mucosa from 18 patients. Concentrations of Tpβ and Tβ10 have been measured by high-pressure liquid chromatography (HPLC) coupled to electrospray-ion trap mass spectrometry (ESI-IT-MS). Ms data were compared by f-test and ANOVA statistical analysis. Identification of thymosin and their proteo-forms has been performed by HPLC-high reso-lution-ESI-IT-MSMS. RESULTS: Both Tβ4 and Tβ10, exhibited intra-tumoral quantitative differences, being up-regulated in the deep part of the CRC. They exhibited, moreover, strong association with the Dukes stage and the budding grade, being more concentrated in patients at Dukes stage B and with budding index "2". CONCLUSIONS: The results obtained in the present investigation encouraged the hypothesis that the two thymosin are involved in colorectal cancer progression, and in promoting cancer invasion. Thus, they are good candidates to be diagnostic/prognostic biomarkers and therapy targets. [ABSTRACT FROM AUTHOR]

Published
2021

36. Restoration of aberrant mTOR signaling by intranasal rapamycin reduces oxidative damage: Focus on HNE-modified proteins in a mouse model of down syndrome

Author

Di Domenico, F., Tramutola, A., Barone, E., Lanzillotta, C., Defever, O., Arena, A., Zuliani, Ivana, Foppoli, C., Iavarone, Federica, Vincenzoni, F., Castagnola, Massimo, Butterfield, D. A., Perluigi, M., Zuliani I., Iavarone F. (ORCID:0000-0002-2074-5531), Castagnola M. (ORCID:0000-0002-0959-7259), Di Domenico, F., Tramutola, A., Barone, E., Lanzillotta, C., Defever, O., Arena, A., Zuliani, Ivana, Foppoli, C., Iavarone, Federica, Vincenzoni, F., Castagnola, Massimo, Butterfield, D. A., Perluigi, M., Zuliani I., Iavarone F. (ORCID:0000-0002-2074-5531), and Castagnola M. (ORCID:0000-0002-0959-7259)

Abstract

Increasing evidences support the notion that the impairment of intracellular degradative machinery is responsible for the accumulation of oxidized/misfolded proteins that ultimately results in the deposition of protein aggregates. These events are key pathological aspects of “protein misfolding diseases”, including Alzheimer disease (AD). Interestingly, Down syndrome (DS) neuropathology shares many features with AD, such as the deposition of both amyloid plaques and neurofibrillary tangles. Studies from our group and others demonstrated, in DS brain, the dysfunction of both proteasome and autophagy degradative systems, coupled with increased oxidative damage. Further, we observed the aberrant increase of mTOR signaling and of its down-stream pathways in both DS brain and in Ts65Dn mice. Based on these findings, we support the ability of intranasal rapamycin treatment (InRapa) to restore mTOR pathway but also to restrain oxidative stress resulting in the decreased accumulation of lipoxidized proteins. By proteomics approach, we were able to identify specific proteins that showed decreased levels of HNE-modification after InRapa treatment compared with vehicle group. Among MS-identified proteins, we found that reduced oxidation of arginase-1 (ARG-1) and protein phosphatase 2A (PP2A) might play a key role in reducing brain damage associated with synaptic transmission failure and tau hyperphosphorylation. InRapa treatment, by reducing ARG-1 protein-bound HNE levels, rescues its enzyme activity and conceivably contribute to the recovery of arginase-regulated functions. Further, it was shown that PP2A inhibition induces tau hyperphosphorylation and spatial memory deficits. Our data suggest that InRapa was able to rescue PP2A activity as suggested by reduced p-tau levels. In summary, considering that mTOR pathway is a central hub of multiple intracellular signaling, we propose that InRapa treatment is able to lower the lipoxidation-mediated damage to proteins, thus represe

Published
2019

37. Quantitative Analysis of the Seminal Plasma Proteome in Secondary Hypogonadism

Author

Grande, G, Vincenzoni, F, Mancini, F, Barrachina, F, Giampietro, A, Castagnola, M, Urbani, Andrea, Oliva, R, Milardi, D, Pontecorvi, Alfredo, Urbani, A (ORCID:0000-0001-9168-3174), Pontecorvi, A (ORCID:0000-0003-0570-6865), Grande, G, Vincenzoni, F, Mancini, F, Barrachina, F, Giampietro, A, Castagnola, M, Urbani, Andrea, Oliva, R, Milardi, D, Pontecorvi, Alfredo, Urbani, A (ORCID:0000-0001-9168-3174), and Pontecorvi, A (ORCID:0000-0003-0570-6865)

Abstract

In the grey zone of testosterone levels between 8 and 12 nmol/L, the usefulness of therapy is controversial; as such, markers of tissue action of androgens may be helpful in adjusting clinical decisions. To better understand the effect of the hypothalamic-pituitary-testicular axis on male accessory secretion, we performed a proteomic quantitative analysis of seminal plasma in patients with secondary hypogonadism, before and after testosterone replacement therapy (TRT). Ten male patients with postsurgical hypogonadotrophic hypogonadism were enrolled in this study, and five of these patients were evaluated after testosterone treatment. Ten men with proven fertility were selected as a control group. An aliquot of seminal plasma from each individual was subjected to an in-solution digestion protocol and analyzed using an Ultimate 3000 RSLC-nano HPLC apparatus coupled to a LTQ Orbitrap Elite mass spectrometer. The label-free quantitative analysis was performed via Precursor Ions Area Detector Node. Eleven proteins were identified as decreased in hypogonadic patients versus controls, which are primarily included in hydrolase activity and protein binding activity. The comparison of the proteome before and after TRT comes about within the discovery of six increased proteins. This is the primary application of quantitative proteomics pointed to uncover a cluster of proteins reflecting an impairment not only of spermatogenesis but of the epididymal and prostate epithelial cell secretory function in male hypogonadism. The identified proteins might represent putative clinical markers valuable within the follow-up of patients with distinctive grades of male hypogonadism.

Published
2019

38. Exploring the brain tissue proteome of TgCRND8 Alzheimer's Disease model mice under B vitamin deficient diet induced hyperhomocysteinemia by LC-MS top-down platform

Author

Delfino, Daniela, Rossetti, Dv, Martelli, C, Inserra, Ilaria, Vincenzoni, F, Castagnola, Massimo, Urbani, Andrea, Scarpa, S, Fuso, Paola, Cavallaro, Ra, Desiderio, Claudia, Delfino, D, Inserra, I, Castagnola, M (ORCID:0000-0002-0959-7259), Urbani, A (ORCID:0000-0001-9168-3174), Fuso, A, Desiderio, C, Delfino, Daniela, Rossetti, Dv, Martelli, C, Inserra, Ilaria, Vincenzoni, F, Castagnola, Massimo, Urbani, Andrea, Scarpa, S, Fuso, Paola, Cavallaro, Ra, Desiderio, Claudia, Delfino, D, Inserra, I, Castagnola, M (ORCID:0000-0002-0959-7259), Urbani, A (ORCID:0000-0001-9168-3174), Fuso, A, and Desiderio, C

Abstract

The multifactorial nature of Late Onset Alzheimer's Disease (LOAD), the AD form of major relevance on epidemiological and social aspects, has driven the original investigation by LC-MS and top-down proteomics approach of the protein repertoire of the brain tissue of TgCRND8 model mice fed with a diet deficient in B vitamins. The analysis of the acid-soluble fraction of brain tissue homogenates identified a list of proteins and peptides, proteoforms and PTMs. In order to disclose possible modulations, their relative quantification in wild type and AD model mice under both B vitamin deficient and control diets was performed. The levels of metallothionein III, guanine nucleotide-binding protein G(I)/G(S)/G(0) subunit gamma-2 and brain acid soluble protein 1 showed statistically significant alterations depending on genotype, diet or both effects, respectively. Particularly, metallothionein III exhibited increased levels in TgCRND8 mice under B vitamin deficient diet with respect to wild type mice under both diets. Brain acid soluble protein 1 showed the opposite, revealing decreased levels in all diet groups of AD model mice with respect to wild type mice in control diet. Lower levels of brain acid soluble protein 1 were also observed in wild type mice under deficiency of B vitamins. These results, besides contributing to increase the knowledge of AD at molecular level, give new suggestions for deeply investigating metallothionein III and brain acid soluble protein 1 in AD.

Published
2019

39. Investigating the Protein Signature of Adamantinomatous Craniopharyngioma Pediatric Brain Tumor Tissue: Towards the Comprehension of Its Aggressive Behavior

Author

Martelli, C, Serra, Teresa, Inserra, Ilaria, Rossetti, Dv, Iavarone, Federica, Vincenzoni, F, Castagnola, Massimo, Urbani, Andrea, Tamburrini, Gianpiero, Caldarelli, Massimo, Massimi, Luca, Desiderio, C, Serra, R, Inserra, I, Iavarone, F (ORCID:0000-0002-2074-5531), Castagnola, M (ORCID:0000-0002-0959-7259), Urbani, A (ORCID:0000-0001-9168-3174), Tamburrini, G (ORCID:0000-0002-7139-5711), Caldarelli, M (ORCID:0000-0002-2111-3800), Massimi, L, Martelli, C, Serra, Teresa, Inserra, Ilaria, Rossetti, Dv, Iavarone, Federica, Vincenzoni, F, Castagnola, Massimo, Urbani, Andrea, Tamburrini, Gianpiero, Caldarelli, Massimo, Massimi, Luca, Desiderio, C, Serra, R, Inserra, I, Iavarone, F (ORCID:0000-0002-2074-5531), Castagnola, M (ORCID:0000-0002-0959-7259), Urbani, A (ORCID:0000-0001-9168-3174), Tamburrini, G (ORCID:0000-0002-7139-5711), Caldarelli, M (ORCID:0000-0002-2111-3800), and Massimi, L

Abstract

Although histologically benign, adamantinomatous craniopharyngioma (AC) pediatric brain tumor is a locally aggressive disease that frequently determines symptoms and hormonal dysfunctions related to the mass effect on the surrounding structures. Another typical feature of this benign neoplasm is the presence of voluminous liquid cysts frequently associated with the solid component. Even if studies have been devoted to the proteomic characterization of the tumor intracystic fluid, poor explorations have been performed on its solid part, principally investigated by transcriptomics technologies. In the present study, seven specimens of AC whole tumor tissue have been analyzed by LC-MS for a preliminary assessment of the proteomic profile by a top-down/bottom-up integrated approach. Thymosin beta 4, ubiquitin, calmodulin, S100 proteins, prothymosin alpha isoform 2, alpha-defensins 1-4, and fragments largely belonging to vimentin, hemoglobin, and glial fibrillary acidic protein characterized the intact proteome. The identification of alpha-defensins, formerly characterized in AC intracystic fluid, reinforces the hypothesis of a role for inflammation in tumor pathogenesis. A total number of 1798 unique elements were identified by a bottom-up approach with a special focus on the 433 proteins commonly characterized in the 85.7% of the samples analyzed. Their gene ontology classification evidenced the involvement of the adherence system, intermediate filaments, and actin cytoskeleton in tumor pathogenesis and of elements part of the Wnt, FGF, and EGFR signaling pathways. In addition, proteins involved in calcium modulation, innate immunity, inflammation, CCKR and integrin signaling, and gonadotropin-releasing hormone receptor pathways were also outlined. Further than confirming proteomic data previously obtained on AC intracystic fluid, these results offer a preliminary overview of the AC whole tissue protein phenotype, adding new hints towards the comprehension of this stil

Published
2019

40. Proteomic evaluation of GCF in the development of pregnancy related periodontal disease: A pilot clinical study

Author

Dassatti, Leonardo, Manicone, Paolo Francesco, Iavarone, Federica, Stefanelli, N., Nicoletti, F., Lazzareschi, Ilaria, Luciano, Rita Paola Maria, Castagnola, Massimo, D'Addona, Antonio, Dassatti, Leonardo (ORCID:0000-0003-4794-3439), Manicone P. F. (ORCID:0000-0003-0283-2903), Iavarone F. (ORCID:0000-0002-2074-5531), Lazzareschi I. (ORCID:0000-0001-7221-2983), Luciano R. P. M. (ORCID:0000-0003-4358-0757), Castagnola M. (ORCID:0000-0002-0959-7259), D'Addona A. (ORCID:0000-0002-0876-7594), Dassatti, Leonardo, Manicone, Paolo Francesco, Iavarone, Federica, Stefanelli, N., Nicoletti, F., Lazzareschi, Ilaria, Luciano, Rita Paola Maria, Castagnola, Massimo, D'Addona, Antonio, Dassatti, Leonardo (ORCID:0000-0003-4794-3439), Manicone P. F. (ORCID:0000-0003-0283-2903), Iavarone F. (ORCID:0000-0002-2074-5531), Lazzareschi I. (ORCID:0000-0001-7221-2983), Luciano R. P. M. (ORCID:0000-0003-4358-0757), Castagnola M. (ORCID:0000-0002-0959-7259), and D'Addona A. (ORCID:0000-0002-0876-7594)

Abstract

OBJECTIVE: This pilot study analyzed the possible changes of periodontal disease status in female patients during the period following pregnancy. Both clinical and laboratory data were collected and analyzed. PATIENTS AND METHODS: A non-randomized controlled clinical trial was conducted by the Periodontal Department of the Dental Clinic in collaboration with the Pediatrics Department, at Fondazione Policlinico Universitario A. Gemelli, Rome, Italy. Ten female patients, who completed the pregnancy without complications, were enrolled in this research protocol forming the experimental group. During the first post-partum days, gingival crevicular fluid (GCF) samples were collected and analyzed with high-performance liquid chromatography associated with high-resolution mass spectrometry (HPLC ESI MS); periodontal parameters as pocket depth (PD), full mouth plaque score (FMPS) and full mouth bleeding score (FMBS) were recorded, and a professional oral hygiene session was performed. The same protocol was applied after three months with the same patients forming the recall group. A control group was created in order to compare the results with GCF samples from 10 not pregnant fertile women. RESULTS: Student's t-test has been used to evaluate the statistical significance of the collected data. Mean levels of PD decreased from 3.75 mm ± 1.2 mm after pregnancy to 2.88 mm ± 0.85 mm at three months post-partum (p<0.01). Mean value of FMPS and FMBS decreased from 21.8% ± 1.35% and 34.27% ± 1.5% after pregnancy to 13% ± 2.81% and 17.55% ± 2.84% at three months post-partum, respectively (p<0.05). The concentration of each analyzed peptide has changed in relation to the general improvement of the periodontal status at three months post-partum. CONCLUSIONS: Pregnancy may be associated with an increased risk of periodontal disease. Both clinical and laboratory data have demonstrated that a professional oral hygiene session can affect the course of pregnancy inducing periodontal

Published
2019

41. Fetal programming of atherosclerosis: may the barker hypothesis explain the susceptibility of a subset of patients to develop stroke or cardiac infarct?

Author

GEROSA, C., FAA, G., FANNI, D., CERRONE, G., SURI, J. S., BARCELLONA, D., CONI, P., CONGIU, T., LAI, M. L., PIRAS, M., CAU, F., COGHE, F., BALESTRIERI, A., CAU, R., ORRU', G., SCANO, A., VAN EYKEN, P., LA NASA, G., CAMPAGNA, M., and CASTAGNOLA, M.

Abstract

The risk stratification of young adults between subjects who will develop a mild form of atherosclerosis and subjects who will undergo a severe disease remains inaccurate. In the eighties of the previous century, David JP Barker has demonstrated the relationship between fetal conditions and occurrence of pathologies in adulthood. In this paper, the multiple evidence that might explain the increased susceptibility to severe forms of atherosclerosis, including stroke and cardiac infarct, in subjects who underwent intrauterine growth restriction (IUGR) will be analyzed. Specifically, we will review those inter-connected data indicating an association between a low weight at birth and an adult phenotype which might favor a severe outcome of atherosclerosis. Young and adult subjects born too small (IUGR) or too early (pre-terms) might represent a subgroup of "at risk subjects", more susceptible toward severe forms of atherosclerosis. Given that low birth weight (LBW) may be considered a surrogate of IUGR, this phenotypic feature could be considered among those indispensable clinical data collected in every patient presenting with atherosclerosis, irrespectively of age. According to the hypothesis that structural arterial changes might represent the link between LBW and susceptibility to atherosclerosis later in life, we suggest that the prevention of atherosclerosis should begin at birth. Regenerative and physiological substances such as thymosin Beta-4 could be challenged for a new "arterial regenerative medicine" in the perinatal period. The goal of this new approach should be the reinforcement of the structure of the arterial wall, allowing LBW newborns to avoid the most severe complications of atherosclerosis later in life: a dream that our research could contribute to bringing to life. [ABSTRACT FROM AUTHOR]

Published
2021

44. Thymosin beta-4 prenatal administration improves fetal development and halts side effects due to preterm delivery.

Author

FAA, G., PIRAS, M., MANCUSO, L., CONI, P., PICHIRI, G., ORRÙ, G., FANNI, D., GEROSA, C., CAO, G., TAIBI, R., PAVONE, P., and CASTAGNOLA, M.

Abstract

OBJECTIVE: Thymosin beta 4 (TB4) is the most abundant member of the beta-thymosin family in humans. The main physiological role of TB4 is the regulation of actin polymerization. TB4 is also involved in angiogenesis, cell survival, cell migration and fetal development. The aim of this study was to evaluate the activity of TB4 as a fetal growth promoter when administered during pregnancy. MATERIALS AND METHODS: Our protocols have been carried out in full conformity with the rules and guidelines expected for this kind of trial. 10 pregnant mice received the same injection regimen. Only 6 of these 10 are part of this experiment because they were pregnant. At 10:00 a.m. on day E14 and E17 of gestation mice were weighed and treated with an intraperitoneal injection of TB4 (Regene RX, Rockville, MD, USA; 6 mg/kg in PBS). RESULTS: The mothers treated with TB4 for two days precisely E14 and E17, showed a higher cranio-caudal length when compared to control newborns. At histology, maternal TB4 treatment was associated with more advanced development of lungs, heart, kidney, cerebral cortex and notochord. CONCLUSIONS: Our study shows that TB4 administration during gestation may act as a powerful fetal growth promoter, by accelerating the development of newborn organs and tissues. [ABSTRACT FROM AUTHOR]

Published
2021

47. Proteomics in pediatric cystic craniopharyngioma

Author

Massimi L., Martelli C., Caldarelli M., Castagnola M., and Desiderio C.

Subjects
interferon-?, brain tumors, proteomic analysis, craniopharyngioma, thymosins, defensins
Abstract

Adamantinomatous craniopharyngioma (ACP) is still often burdened by a poor prognosis in children as far as the risk of recurrence and the quality of life are concerned. Therefore, many efforts are now dedicated to investigate the molecular characteristics of this tumor aiming at finding new therapeutic options. ACP is prevalently a cystic lesion so that an increasing number of researches are focused on the analysis of its cystic content. In the present article, the main results of the current proteomic analysis (PA) on the ACP fluid are summarized. Both "bottom-up" and "top-down" approaches have been utilized. In the bottom-up approach, proteins and peptides are enzymatically or chemically digested prior to liquid chromatography and mass spectrometry analyses. The bottom-up approach pointed out several proteins of the inflammation (namely, ?2-HS-glycoprotein, ?1-antichymotrypsin and apolipoproteins) as possibly involved in the genesis and growth of the cystic component of ACP. The top-down strategy analyzes proteins and peptides in the intact state, making it particularly suitable for the identification of peptides and low molecular weight proteins and for the characterization of their possible isoforms and post-translational modifications. The top-down approach disclosed the presence of the thymosin ? family. Thymosin ?4, in particular, which is involved in the cytoskeleton organization and migration of several tumors, could play a role in the progression of ACP. Finally, PA was utilized to investigate alterations in cyst fluid character after treatment with interferon-?. The analyzed samples showed a progressive reduction of the levels of ?-defensins (proteins involved in the inflammatory-mediated response) after the intracystic injection of interferon-?, thus reinforcing the hypothesis that inflammation contributes to ACP cyst pathogenesis. Additional studies on the solid component of ACP are still necessary to further validate the previous results and to identify possible markers for targeted therapy.

Published
2017

48. Biomarkers e proteomica salivari: Prospettive future cliniche e diagnostiche

Author

Castagnola, Massimo, Scarano, Emanuele, Passali, Giulio Cesare, Messana, Irene, Cabras, Tiziana, Iavarone, Federica, Di Cintio, Giovanni, Fiorita, Antonella, De Corso, Eugenio, Paludetti, Gaetano, Castagnola, M. (ORCID:0000-0002-0959-7259), Scarano, E. (ORCID:0000-0003-2570-1121), Passali, Giulio Cesare (ORCID:0000-0002-8176-0962), Messana, I. (ORCID:0000-0002-1436-6105), Cabras, T., Iavarone, F. (ORCID:0000-0002-2074-5531), Di Cintio, G., Fiorita, A., De Corso, E., Paludetti, G. (ORCID:0000-0003-2480-1243), Castagnola, Massimo, Scarano, Emanuele, Passali, Giulio Cesare, Messana, Irene, Cabras, Tiziana, Iavarone, Federica, Di Cintio, Giovanni, Fiorita, Antonella, De Corso, Eugenio, Paludetti, Gaetano, Castagnola, M. (ORCID:0000-0002-0959-7259), Scarano, E. (ORCID:0000-0003-2570-1121), Passali, Giulio Cesare (ORCID:0000-0002-8176-0962), Messana, I. (ORCID:0000-0002-1436-6105), Cabras, T., Iavarone, F. (ORCID:0000-0002-2074-5531), Di Cintio, G., Fiorita, A., De Corso, E., and Paludetti, G. (ORCID:0000-0003-2480-1243)

Abstract

Saliva testing is a non-invasive and inexpensive test that can serve as a source of information useful for diagnosis of disease. As we enter the era of genomic technologies and –omic research, collection of saliva has increased. Recent proteomic platforms have analysed the human salivary proteome and characterised about 3000 differentially expressed proteins and peptides: in saliva, more than 90% of proteins in weight are derived from the secretion of three couples of “major” glands; all the other components are derived from minor glands, gingival crevicular fluid, mucosal exudates and oral microflora. The most common aim of proteomic analysis is to discriminate between physiological and pathological conditions. A proteomic protocol to analyze the whole saliva proteome is not currently available. It is possible distinguish two type of proteomic platforms: top-down proteomics investigates intact naturally-occurring structure of a protein under examination; bottom-up proteomics analyses peptide fragments after pre-digestion (typically with trypsin). Because of this heterogeneity, many different biomarkers may be proposed for the same pathology. The salivary proteome has been characterised in several diseases: oral squamous cell carcinoma and oral leukoplakia, chronic graft-versus-host disease Sjögren’s syndrome and other autoimmune disorders such as SAPHO, schizophrenia and bipolar disorder, and genetic diseases like Down’s Syndrome and Wilson disease. The results of research reported herein suggest that in the near future human saliva will be a relevant diagnostic fluid for clinical diagnosis and prognosis.

Published
2017

50. The intriguing heterogeneity of human salivary proline-rich proteins: Short title: Salivary proline-rich protein species

Author

Manconi B, Castagnola M, Cabras T, Olianas A, Alberto Vitali, Desiderio C, Mt, Sanna, and Messana I

Subjects
N-/O-glycosylated proline-rich proteins, N-pyroglutaminylation, Proteolysis, Basic proline-rich proteins, Humans, Carboxypeptidases, Phosphorylation, Peptides, Settore BIO/10 - BIOCHIMICA, Protein Processing, Post-Translational, Acidic proline-rich proteins, Salivary Proline-Rich Proteins
Abstract

The most heterogeneous family of human salivary proteins is represented by proline-rich proteins (PRPs) divided in acidic, basic, and basic glycosylated (aPRPs, bPRPs, gPRPs). They are encoded by six genes, clustered on chromosome 12p13.2: PRH1-2 encode aPRPs, PRB1-4 encode bPRPs and gPRPs. Each gene exists in different allelic forms: two for PRH2, three for PRH1, PRB2, and PRB4, four for PRB1, and PRB3. During granule maturation, PRP proproteins undergo proteolysis by the action of convertases and carboxypeptidases. Differently from bPRPs, proteolysis of aPRPs is not complete, and, besides fragments, entire protein species are also secreted. Maturation process generates ten aPRPs (PRP-1, PRP-2, PIF-s, Db-s, Pa, PRP-3, PRP-4, PIF-f, Db-f, P-C), and at least 18 bPRPs (II-2, P-E, IB-6, Ps-1, Ps-2, IB-1, P-J, IB-8a, P-F, P-H, P-D, II-1, protein glycosylated A, CD-IIg, and Gl1-4). In addition, single nucleotide and length polymorphisms, and differentially spliced transcripts originate several natural variants. Phosphorylation, N-pyroglutaminylation, dimerization, and N-/O-glycosylation also occur during maturation, enlarging the number of protein species, further increased by proteolytic events governed by carboxy- and endo-peptidases during and after secretion, and giving rise to a huge number of small peptides. The PRP functional role is still poorly understood. Significance: The high polymorphism of PRPs gives an important contribution to the high heterogeneity and inter-individual variability of the human salivary proteome. The products of six genes clustered on chromosome 12p13.2 comprise a mixture of entire, truncated, phosphorylated, glycosylated and dimerized protein/peptide species, sharing large part of their sequences, and possibly involved in different biological activities. Whatever the role of PRP species is, it should be crucial, given that PRPs are the most conserved oral salivary proteins among mammals.

Published
2016
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