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Vol. 54, Issue 6, 954-961, December 1998
Department of Pharmacology, University of Pittsburgh, School of
Medicine, Pittsburgh, Pennsylvania 15261
Bleomycin hydrolase (BH) is a highly conserved cysteine proteinase that
deamidates and inactivates the anticancer drug bleomycin. Yeast BH
self-assembles to form a homohexameric structure, which resembles a 20 S proteasome and may interact with other proteins. Therefore, we
searched for potential human BH (hBH) partners using the yeast
two-hybrid system with a HeLa cDNA library and identified the
full-length human homologue of yeast ubiquitin-conjugating enzyme 9 (UBC9). Cotransformation assays using hBH deletion mutants revealed
that the carboxyl terminus of hBH (amino acids 356-455), which
contains two of the three essential catalytic amino acids, was not
critical for protein binding in the yeast two-hybrid environment. In vitro translated human UBC9 was precipitated by
glutathione S-transferase-hBH fusion protein but not by
glutathione S-transferase. Efficient in
vitro binding occurred in the absence of the first 24 amino
acids of UBC9 and the catalytic Cys93 of UBC9. We confirmed that hBH
and UBC9 interacted in vivo by affinity copurification of proteins overexpressed in mammalian cells. Using immunocytochemical analysis, hBH was colocalized with UBC9. Coexpression of hBH and UBC9
in mammalian cells did not markedly alter the bleomycin-hydrolyzing activity of hBH or apparent small ubiquitin-related modifier 1 addition. This is the first reported heteromeric interaction with hBH,
and it suggests a role for hBH in intracellular protein processing and degradation.
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