V. Baldin et al., ALTERNATIVE SPLICING OF THE HUMAN CDC25B TYROSINE PHOSPHATASE - POSSIBLE IMPLICATIONS FOR GROWTH-CONTROL, Oncogene, 14(20), 1997, pp. 2485-2495
CDC25B2, a protein tyrosine phosphatase closely related to the putativ
e CDC25B oncogene, was identified in a Burkitt lymphoma cDNA library,
CDC25B2 differs from CDC25B by a 14 residue insertion and a 41 residue
deletion, which are both located in the amino-terminal region of the
protein, upstream of the catalytic domain. Examination of the genomic
sequence revealed that CDC25B1 (formerly B) and CDC25B2 are splice var
iants of the same gene, A third variant, CDC25B3, that carries both th
e 14 and the 41 residue sequences was also identified in the same cDNA
library. All three variants were detected in a panel of human primary
culture and cell lines, although at different levels. In primary fibr
oblasts and in HeLa cells the CDC25B expression is cell cycle regulate
d, reaching a maximum in G(2)-phase. In vitro, CDC25B1 phosphatase is
slightly more active than CDC25B2 and B3. However, episomal overexpres
sion of the three CDC25B variants in fission yeast reveals that in viv
o, CDC25B2 is largely more active than either B1 or B3 (B2>B3>B1) both
to complement a thermosensitive S pombe CDC25 activity and to act as
a mitotic inducer, Alternative splicing of CDC25B may therefore contri
bute to the control of cell proliferation.