Abstract: AIMS: To establish the conditions for protein tyrosine phosphatase gamma (PTPgamma) detection in paraffin tissues using two antibodies raised against its NH(2)- (anti-P4) and COOH-termini (gammaTL1); to analyse its expression in normal tissues and to perform an initial screening of neoplastic tissues. METHODS AND RESULTS: Membranous and/or cytoplasmic PTPgamma expression was detected in the majority of epithelial cell types and in endocrine cells, with the highest expression in adrenal medulla, endocrine cells of the gastrointestinal tract and pancreatic islets. Both antibodies stained the thyroid follicular epithelium, but only anti-P4 antibody stained the colloid matrix, suggesting shedding/secretion of the PTPgamma extracellular domain. Marked loss of PTPgamma immunoreactivity was detected in subsets of ovarian (21%), breast (56%) and lung (80%) neoplasms. Conversely, cytoplasmic positivity was found in 37% of lymphomas, mainly of high-grade histotypes, while normal lymphocytes were negative. Brain tissue showed PTPgamma expression in a few neuronal and glial elements and PTPgamma was overexpressed in the majority of high-grade astrocytomas. CONCLUSIONS: We have analysed PTPgamma expression in archival paraffin-embedded tissues for the first time, demonstrating particularly high expression in endocrine cells and both down- and up-regulation in neoplasia, the latter possibly reflecting the undifferentiated state of the neoplastic cells, suggesting a complex role for this phosphatase.
Abstract: Protein Tyrosine Phosphatase gamma (PTPγ) is a receptor-like transmembrane protein belonging to
the family of classical protein tyrosine phosphatases. PTPγ is known to regulate haematopoietic
differentiation in a murine embryonic stem cells model. We have recently demonstrated that PTPγ
mRNA is expressed in monocytes, tissue-localized myeloid dendritic cells and in both myeloid and
plasmacytoid dendritic cells in peripheral blood. We now developed a PTPγ specific antibody that
recognize the protein by flow cytometry. PTPγ expression was detected in monocytes and both
myeloid and plasmacytoid dendritic cells, while PMN showed a low but consistent staining in
contrast with previous mRNA data. B cells were found to express the phosphatase while T cells
were negative. In keeping with RNA data, PTPγ was detected in monocyte-derived dendritic cells
and its expression raised upon LPS stimulation. Finally, we discovered that CD34+ haematopoietic
precursors express high PTPγ level that drops during in vitro expansion induced by IL-3 and SCF
growth factors. We therefore propose PTPγ as a new functionally regulated leukocyte marker whose
role in normal and pathological context deserve further
Abstract: Protein tyrosine phosphatase (PTPgamma) is a receptor-like molecule with a known role in murine hematopoiesis. We analyzed the regulation of PTPgamma expression in the human hematopoietic system, where it was detected in human peripheral blood monocytes and dendritic cells (DCs) of myeloid and plasmacytoid phenotypes. Its expression was maintained during in vitro monocyte differentiation to dendritic cells (moDC) and was further increased after maturation with bacterial lipopolysaccharide (LPS), CD40L, and TNFalpha. But PTPgamma was absent when monocytes from the same donor were induced to differentiate in macrophages. B and T lymphocytes did not express PTPgamma. Rather, PTPgamma mRNA was expressed in primary and secondary lymphoid tissues, and the highest expression was in the spleen. PTPgamma was detected by immunohistochemistry in subsets of myeloid-derived DCs and specialized macrophages (tingible bodies, sinus and alveolar macrophages). Classic macrophages in infective or reactive granulomatous reactions did not express PTPgamma. Increased PTPgamma expression was associated with a decreased ability to induce proliferation and interferon-gamma secretion in T cells by moDCs from patients with advanced pancreatic cancer. Taken together, these results indicate that PTPgamma is a finely regulated protein in DC and macrophage subsets in vitro and in vivo.