M. G. Borrello scite author profile

The bcl-2 proto-oncogene, rearranged and deregulated in B-cell lymphomas bearing the t(14;lB) translocation, encodes an inner mitochondria1 membrane protein that blocks apoptotic cell death. We have developed a sensitive immunofluorescence assay for the single-and multicolor flow cytometric analysis of bcl-2 protein in relation to other markers and cell cycle, based on a fixation-permeation step of cells with paraformaldehyde and Triton XlOO and the use of a bcl-2 specific monoclonal antibody (MoAb). As an application of this method, we have examined the expression of bcl-2 in normal and neoplastic lymphoid cells.We have found that > 80% of normal Tand B-cells are bcl-2 positive; following in vitro mitogen activation, the bcl-2 reactivity decreased slightly in the former but markedly in latter cells. In both cases the bcl-2 expression was not restricted to a specific phase of the cell cycle, as evidenced by two-color analysis. On lymphoblastoid cell lines, the bcl-2 staining intensity was variable and not necessarily correlated to molecular rearrangements of the bcl-2 gene. Among fresh Bcell non-Hodgkin's lymphomas (B-NHL), most sporadic Burkitt's cases were bcl-2 negative. Of four centroblastic-centrocytic cases with rearrangements of the bcl-2 gene, only two presented elevated amounts of bcl-2 protein, indicating that the levels of bcl-2 are not diagnostic of the translocation. The flow cytometric analysis of bcl-2 protein allows study and quantification, as the single cell level and in selected cell subsets, of the expression of the bcl-2 gene and provides an important tool for assessing its role in hematopoietic cell development, proliferation, and neoplastic conversion. 0 1992 Wiley-Liss, Inc.

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trk and ret proto‐oncogene expression in human neuroblastoma specimens: High frequency of trk expression in non‐advanced stages

Borrello

Bongarzone

Plerotti

et al. 1993

Intl Journal of Cancer

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Forty-three fresh tumor specimens of human neuroblastoma belonging to different clinical stages were analyzed for the expression of 2 proto-oncogenes: trk, which encodes a tyrosine-kinase receptor for nerve growth factor (NGF) and ret, another receptor-type tyrosine kinase whose ligand is unknown. The mRNA expression of the trk gene was detected in 67.4% of cases, with increased frequency in I, II and IVs Evans' stages and in patients with favorable prognosis according to the Shimada classification. Moreover, trk expression inversely correlated with Nmyc-gene amplification. ret mRNA was found in 36.8% of cases and equally distributed in the different stages. In addition, ngfR (low-affinity NGF receptor)-gene expression was present in 9 out of 25 cases. The simultaneous presence of mRNA related to both forms of the NGF receptor, while not proving the presence of a functional receptor, indicates the existence of a sub-set of neuroblastoma cells potentially responsive to NGF.

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Rearrangements of TRK proto-oncogene in papillary thyroid carcinomas

Pierotti

Bongarzone

Borrello

et al. 1995

J Endocrinol Invest

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M. G. Borrello

Direct promoter induction of p19Arf by Pit-1 explains the dependence receptor RET/Pit-1/p53-induced apoptosis in the pituitary somatotroph cells

Induction of RET Proto-Oncogene Expression in Neuroblastoma Cells Precedes Neuronal Differentiation and Is Not Mediated by Protein Synthesis

Flow cytometric detection of the mitochondrial BCL‐2 protein in normal and neoplastic human lymphoid cells

trk and ret proto‐oncogene expression in human neuroblastoma specimens: High frequency of trk expression in non‐advanced stages

Rearrangements of TRK proto-oncogene in papillary thyroid carcinomas

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