Ne regulation. It has been suggested that some SCAN domains act as specific cellular localization sequences. For example, the SCAN POR 8 domain of Zfp42 is reported to be essential for targeting the protein to promyelocytic leukemia nuclear bodies in the cell nucleus [45].Figure 7. The dimer interface of PEG3-SCAN (III). A pronounced hydrophobic patch occurs at each end of the assembly to stabilize the dimer. The conserved Tyr94 extends across the dimer interface, contributes to hydrophobic interations and donates a hydrogen bond to the carbonyl of Pro60. doi:10.1371/journal.pone.0069538.gSCAN Domain of PEGFigure 8. The dimer interface of PEG3-SCAN (IV). A group of conserved, aliphatic and aromatic residues form a hydrophobic core to stabilize the dimer. doi:10.1371/journal.pone.0069538.gHowever, since localization studies using different constructs of PEG3 have indicted that the SCAN domain was not required for nuclear localization [12] then such a general function is unlikely. It is not known whether SCAN domains interact with any other protein motifs in addition to self-association with other SCAN members. The function of PEG3 in regulation of TNF and Wnt signal transduction pathways has been implied by an ability to bind TRAF2, the E3 ubiquitin ligase Siah1 and b-catenin [10?2]. A yeast two-hybrid screen showed residues outside the SCAN domain (residues 268?02) to be required for interaction with fulllength TRAF2 as well as a Siah2 fragment missing the RING (really interesting gene) domain (residues 106?26) [10]. The same study reported the interaction of a mouse PEG3 with Siah proteins by immunoprecipitation, while the later experiments using deletion generated constructs of human PEG3 revealed that the N-terminus including the SCAN domain (residues 1?68) were required for binding the full-length Siah1. Many proteins that interact with Siah1 contain the consensus Siah1 binding motif Valx-Pro [46,47]. This amino acid sequence is also present within the SCAN domain of PEG3, Val58-Gly59-Pro60, on a short segment of extended structure leading to a2 (Fig. 7). We sought to investigate whether the human PEG3-SCAN domain (residues 40?30) interacted with human Siah1. A construct of Siah1 without the RING domain (residues 90?82) was cloned, expressed and purified separately and combined with PEG3SCAN in 94-09-7 one-to-one stoichiometry. The sample was analyzed on a size exclusion column, but there was no evidence of complex formation (data not shown). An NMR study revealed no differences in chemical shifts in the two-dimensional 1H?5N HSQC (heteronuclear single quantum coherence spectroscopy)spectra of 15N-labeled Siah1 upon addition of unlabeled PEG3SCAN (data not shown) indicative of a lack of interactions between the polypeptides. The lack of an association suggests that residues outside the SCAN domain might be required for interaction with Siah1 but there is no other obvious Siah1 binding motif. The PEG3-SCAN structure reveals that the Val58-Gly59-Pro60 motif is an extended conformation immediately prior to a2. The proline is buried and involved in inter-subunit interactions, and the valine side chain tucked down towards the side of a2, away from the surface of the protein. We speculate that if this is indeed a recognition site for Siah1 then conformational changes might be required to allow for complex formation. The conditions under which we investigated the potential interaction may not have been correct to allow such changes or alternatively the.Ne regulation. It has been suggested that some SCAN domains act as specific cellular localization sequences. For example, the SCAN domain of Zfp42 is reported to be essential for targeting the protein to promyelocytic leukemia nuclear bodies in the cell nucleus [45].Figure 7. The dimer interface of PEG3-SCAN (III). A pronounced hydrophobic patch occurs at each end of the assembly to stabilize the dimer. The conserved Tyr94 extends across the dimer interface, contributes to hydrophobic interations and donates a hydrogen bond to the carbonyl of Pro60. doi:10.1371/journal.pone.0069538.gSCAN Domain of PEGFigure 8. The dimer interface of PEG3-SCAN (IV). A group of conserved, aliphatic and aromatic residues form a hydrophobic core to stabilize the dimer. doi:10.1371/journal.pone.0069538.gHowever, since localization studies using different constructs of PEG3 have indicted that the SCAN domain was not required for nuclear localization [12] then such a general function is unlikely. It is not known whether SCAN domains interact with any other protein motifs in addition to self-association with other SCAN members. The function of PEG3 in regulation of TNF and Wnt signal transduction pathways has been implied by an ability to bind TRAF2, the E3 ubiquitin ligase Siah1 and b-catenin [10?2]. A yeast two-hybrid screen showed residues outside the SCAN domain (residues 268?02) to be required for interaction with fulllength TRAF2 as well as a Siah2 fragment missing the RING (really interesting gene) domain (residues 106?26) [10]. The same study reported the interaction of a mouse PEG3 with Siah proteins by immunoprecipitation, while the later experiments using deletion generated constructs of human PEG3 revealed that the N-terminus including the SCAN domain (residues 1?68) were required for binding the full-length Siah1. Many proteins that interact with Siah1 contain the consensus Siah1 binding motif Valx-Pro [46,47]. This amino acid sequence is also present within the SCAN domain of PEG3, Val58-Gly59-Pro60, on a short segment of extended structure leading to a2 (Fig. 7). We sought to investigate whether the human PEG3-SCAN domain (residues 40?30) interacted with human Siah1. A construct of Siah1 without the RING domain (residues 90?82) was cloned, expressed and purified separately and combined with PEG3SCAN in one-to-one stoichiometry. The sample was analyzed on a size exclusion column, but there was no evidence of complex formation (data not shown). An NMR study revealed no differences in chemical shifts in the two-dimensional 1H?5N HSQC (heteronuclear single quantum coherence spectroscopy)spectra of 15N-labeled Siah1 upon addition of unlabeled PEG3SCAN (data not shown) indicative of a lack of interactions between the polypeptides. The lack of an association suggests that residues outside the SCAN domain might be required for interaction with Siah1 but there is no other obvious Siah1 binding motif. The PEG3-SCAN structure reveals that the Val58-Gly59-Pro60 motif is an extended conformation immediately prior to a2. The proline is buried and involved in inter-subunit interactions, and the valine side chain tucked down towards the side of a2, away from the surface of the protein. We speculate that if this is indeed a recognition site for Siah1 then conformational changes might be required to allow for complex formation. The conditions under which we investigated the potential interaction may not have been correct to allow such changes or alternatively the.
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