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Data from Characterization of Endogenous Human Promyelocytic Leukemia Isoforms

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<div>Abstract<p>Promyelocytic leukemia (<i>PML</i>) has been implicated in a variety of functions, including control of TP53 function and modulation of cellular senescence. Sumolated PML is the organizer of mature PML bodies, recruiting a variety of proteins onto these nuclear domains. The <i>PML</i> gene is predicted to encode a variety of protein isoforms. Overexpression of only one of them, PML-IV, promotes senescence in human diploid fibroblasts, whereas PML-III was proposed to specifically interact with the centrosome. We show that all PML isoform proteins are expressed in cell lines or primary cells. Unexpectedly, we found that PML-III, PML-IV, and PML-V are quantitatively minor isoforms compared with PML-I/II and could not confirm the centrosomal targeting of PML-III. Stable expression of each isoform, in a <i>pml</i>-null background, yields distinct subcellular localization patterns, suggesting that, like in other RBCC/TRIM proteins, the COOH-terminal domains of PML are involved in interactions with specific cellular components. Only the isoform-specific sequences of PML-I and PML-V are highly conserved between man and mouse. That PML-I contains all conserved exons and is more abundantly expressed than PML-IV suggests that it is a critical contributor to PML function(s). (Cancer Res 2006; 66(12): 6192-8)</p></div>
Title: Data from Characterization of Endogenous Human Promyelocytic Leukemia Isoforms
Description:
<div>Abstract<p>Promyelocytic leukemia (<i>PML</i>) has been implicated in a variety of functions, including control of TP53 function and modulation of cellular senescence.
Sumolated PML is the organizer of mature PML bodies, recruiting a variety of proteins onto these nuclear domains.
The <i>PML</i> gene is predicted to encode a variety of protein isoforms.
Overexpression of only one of them, PML-IV, promotes senescence in human diploid fibroblasts, whereas PML-III was proposed to specifically interact with the centrosome.
We show that all PML isoform proteins are expressed in cell lines or primary cells.
Unexpectedly, we found that PML-III, PML-IV, and PML-V are quantitatively minor isoforms compared with PML-I/II and could not confirm the centrosomal targeting of PML-III.
Stable expression of each isoform, in a <i>pml</i>-null background, yields distinct subcellular localization patterns, suggesting that, like in other RBCC/TRIM proteins, the COOH-terminal domains of PML are involved in interactions with specific cellular components.
Only the isoform-specific sequences of PML-I and PML-V are highly conserved between man and mouse.
That PML-I contains all conserved exons and is more abundantly expressed than PML-IV suggests that it is a critical contributor to PML function(s).
(Cancer Res 2006; 66(12): 6192-8)</p></div>.

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