Impact of the C-Terminal Loop of Histidine Triad Nucleotide Binding Protein1 (Hint1) on Substrate Specificity
- Creators
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Chou, Tsui-Fen
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Sham, Yuk Y.
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Wagner, Carston R.
Abstract
Although highly sequence similar, human histidine triad nucleotide binding protein (hHint1) and E. coli hinT (echinT) exhibit significant differences in their phosphoramidase substrate specificity and lysyl-adenylate hydrolytic activity. Observing that the C termini of each enzyme are highly dissimilar, we created two chimeric Hint's: one in which the C terminus of hHint1 was replaced with the C terminus of echinT (Hs/ec) and the other in which the C terminus of echinT was replaced with the C terminus of hHint1 (ec/Hs). The Hs/ec chimera exhibited nearly identical specificity constants (k_(cat)/K_m) to those found for echinT, whereas the specificity constants of the ec/Hs chimera were found to approximate those for hHint1. In particular, as observed for echinT, the Hs/ec chimera does not exhibit a preference for phosphoramidates containing d- or l- tryptophan, while the ec/Hs chimera adopts the human enzyme preference for the l configuration. In addition, the studies with each chimera revealed that differences in the ability of hHint1 and echinT to hydrolyze lysyl-AMP generated by either E. coli or human lysyl-tRNA synthetase were partially transferable by C-terminal loop exchange. Hence, our results support the critical role of the C-terminal loop of human and E. coli Hint1 on governing substrate specificity.
Additional Information
© 2007 American Chemical Society. Received 24 June 2007. Revised 1 September 2007. Published online 16 October 2007. Published in issue 1 November 2007.Attached Files
Supplemental Material - bi701244h_si_002.pdf
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Additional details
- Eprint ID
- 114041
- Resolver ID
- CaltechAUTHORS:20220323-565562000
- Created
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2022-03-24Created from EPrint's datestamp field
- Updated
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2022-03-24Created from EPrint's last_modified field