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Expression of signal transduction proteins during the differentiation of primary human erythroblasts

✍ Scribed by Viviana di Giacomo; Alessandro Matteucci; Emilia Stellacci; Angela Battistini; Angela Di Baldassarre; Silvano Capitani; Elena Alfani; Anna Rita Migliaccio; Lucio Cocco; Giovanni Migliaccio

Publisher: John Wiley and Sons
Year: 2004
Tongue: English
Weight: 232 KB
Volume: 202
Category: Article
ISSN: 0021-9541
DOI: 10.1002/jcp.20179

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✦ Synopsis

Abstract

The high number (>10^8–10^) of primary human pro‐erythroblasts (CD36^high^/CD235a^low^) obtainable in HEMA culture (Migliaccio et al., 2002) is exploited here to analyse the expression of proteins implicated in erythropoietin (EPO)‐signalling (STATs, PI‐3K, and PLCs) during the process of erythroid maturation. Human pro‐erythroblasts progressed in 4 days of culture with EPO into basophilic‐ (CD36^high^/CD235a^medium^, 24 h), polychromatic‐(CD36^high^/CD235a^high^, 48 h), and, finally, orthochromatic‐(CD36^low^/CD235a^high^, 72–96 h) erythroblasts. During this maturation, STAT‐1 was expressed up to the orthochromatic stage, expression of STAT‐5, as well as of its target proteins Bcl~xL~ and IRF~1~, remained constant up to 48 h (polychromatic‐erythroblasts) but decreased by 96 h (orthochromatic‐erythroblasts), while that of STAT‐3 decreased constantly from 24 h on and became undetectable by 96 h. Expression of PI‐3K rapidly decreased with differentiation since only 50% of original protein levels were detected by 48 h. On the other hand, among the members of PLC families investigated, PLC β~4~ was not expressed, PLC β~2~, δ~1~, and γ~2~ were expressed at constant levels throughout the maturation process, while expression of PLC β~3~ and of PLC γ~1~ decreased, as PI‐3K, by 24 h and that of PLC β~1~ was induced by 6 h and became undetectable by 24 h. In conclusion, these data depict the dynamic signalling scenario associated with the maturation of erythroid cells and provide the first indication that members of PLC families (PLC β~1~, β~3~, and γ~1~) might be involved in the control of erythroid differentiation in humans. © 2004 Wiley‐Liss, Inc.

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