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Your search keyword '"Pasquale Ferranti"' showing total 7 results
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7 results on '"Pasquale Ferranti"'

1. Exposure of HL-60 human leukaemic cells to 4-hydroxynonenal promotes the formation of adduct(s) with α-enolase devoid of plasminogen binding activity.

Author

Fabrizio Gentile, Stefania Pizzimenti, Alessia Arcaro, Piergiorgio Pettazzoni, Rosalba Minelli, Daniela D'Angelo, Gianfranco Mamone, Pasquale Ferranti, Cristina Toaldo, Gianpaolo Cetrangolo, Silvestro Formisano, Mario U. Dianzani, Koji Uchida, Chiara Dianzani, and Giuseppina Barrera

Subjects
PHYSIOLOGICAL effects of chemicals, CANCER cells, LEUKEMIA, ENOLASE, PLASMINOGEN activators, LIPID metabolism, BLOOD cells, CELL adhesion, OXIDATIVE stress, IMMUNOBLOTTING
Abstract

HNE (4-hydroxynonenal), the major product of lipoperoxidation, easily reacts with proteins through adduct formation between its three main functional groups and lysyl, histidyl and cysteinyl residues of proteins. HNE is considered to be an ultimate mediator of toxic effects elicited by oxidative stress. It can be detected in several patho-physiological conditions, in which it affects cellular processes by addition to functional proteins. We demonstrated in the present study, by MS and confirmed by immunoblotting experiments, the formation of HNE–α-enolase adduct(s) in HL-60 human leukaemic cells. α-Enolase is a multifunctional protein that acts as a glycolytic enzyme, transcription factor [MBP-1 (c-myc binding protein-1)] and plasminogen receptor. HNE did not affect α-enolase enzymatic activity, expression or intracellular localization, and did not change the expression and localization of MBP-1 either. Confocal and electronic microscopy results confirmed the plasma membrane, cytosolic and nuclear localization of α-enolase in HL-60 cells and demonstrated that HNE was colocalized with α-enolase at the surface of cells early after its addition. HNE caused a dose- and time-dependent reduction of the binding of plasminogen to α-enolase. As a consequence, HNE reduced adhesion of HL-60 cells to HUVECs (human umbilical vein endothelial cells). These results could suggest a new role for HNE in the control of tumour growth and invasion. [ABSTRACT FROM AUTHOR]

Published
2009
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2. Purification and characterization of Alpha-Fetoprotein from the human hepatoblastoma HepG2 cell line in serum-free medium.

Author

Patrizia Carlini, Pasquale Ferranti, Francesca Polizio, Maria Ciriolo, and Giuseppe Rotilio

Abstract

Abstract  Alpha-fetoprotein (AFP) is a tumor-associated embryonic molecule whose precise biological function remains unclear. A complete definition of the physiological activities of this oncofetal protein has been severely limited, until now, by the lack of a purification procedure appropriate to obtain pure AFP in appreciable amount. The present report describes a purification procedure extremely rapid and simple and takes advantage of the well-known fact that AFP contains copper. We have developed a single-step purification procedure by immobilized copper-chelate affinity chromatography using the culture medium from human hepatoblastoma cell line HepG2 grown in the absence of serum. This method yields AFP at high purity and high yield. Purified AFP amino acid sequence, molecular mass, carbohydrate structure, and copper content were found to be in line with previous studies. Moreover, we found that the purified AFP has superoxide dismutase activity with efficiency similar to that of the native Cu, Zn SODs at physiological pH. This result may provide further support to the idea that AFP is a bifunctional protein, acting in cellular defence against oxidative stress both as a copper buffer and as a superoxide radical scavenger. [ABSTRACT FROM AUTHOR]

Published
2007
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