Functional analysis of PEX13 mutation in a Zellweger syndrome spectrum patient reveals novel homooligomerization of PEX13 and its role in human peroxisome biogenesis.

[zellweger syndrome]

In humans , the concerted action of at least 13 different peroxisomal PEX proteins is needed for proper peroxisome biogenesis . Mutations in any of these PEX genes can lead to lethal neurometabolic disorders of the Zellweger syndrome spectrum (ZSS ). Previously , we identified the W 313 G mutation located within the SH 3 domain of the peroxisomal protein , PEX 13 . As this tryptophan residue is highly conserved in almost all known SH 3 proteins , we investigated the pathogenic mechanism of the W 313 G mutation and its role in PEX 13 interactions and functions in peroxisome biogenesis . Here , we report for the first time that human PEX 13 interacts with itself in peroxisomes in living cells . We demonstrate that the import of PTS 1 (peroxisomal targeting signal 1 ) proteins is specifically disrupted when homooligomerization of PEX 13 is interrupted . Live cell FRET microscopy in living cells as well as co -immunoprecipitation experiments reveal that the highly conserved W 313 residue is important for self-association of PEX 13 but is not required for interaction with PEX 14 , a well-established interaction partner at the peroxisomal membrane . Experiments with truncated constructs indicate that although the W 313 G mutation resides in the C-terminal SH 3 domain , the N-terminal half is necessary for peroxisomal localization , which in turn appears to be crucial for homooligomerization . Furthermore , rescue of homooligomerization in the W 313 G mutant cells through complementation with truncation constructs restores import of peroxisomal matrix proteins . Taken together , the thorough analyses of a ZSS patient mutation unraveled the general cell biological function of PEX 13 and its mechanism in the import of peroxisomal matrix PTS 1 proteins .