Probing the Role of Highly Conserved Lysine (K279) Residue in the Editing Domain of Bacterial Prolyl-tRNA Synthetases

Mueller, Irene C.; Cao, Bach; Meitzner, Karl J.; Tschudy, Matthew J.

Probing the Role of Highly Conserved Lysine (K279) Residue in the Editing Domain of Bacterial Prolyl-tRNA Synthetases

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MuellerSpr11.pdf (1.31 MB)

Date

2011-05

Authors

Mueller, Irene C.

Cao, Bach

Meitzner, Karl J.

Tschudy, Matthew J.

Advisors

Bhattacharyya, Sudeep

Hati, Sanchita

Type

Presentation

Abstract

The Escherichia coli (Ec) prolyl-tRNA synthetase enzyme possesses three distinct domains. One of the domains, the editing domain, is critical for proofreading the charged tRNAPro, ensuring the correct amino acid has been attached to the tRNA molecule. In this editing domain, a highly conserved lysine has been found to be absolutely essential for proofreading. Through site-directed mutagenesis and enzyme kinetic studies this study attempted to probe the role of this lysine residue (K279).

Description

Color poster with text, diagrams, charts, and graphs.

Keywords

Catalytic RNA, Functional analysis, Escherichia coli, Lysine, Posters, Ligases, Microbiological synthesis

Sponsorship

University of Wisconsin--Eau Claire Office of Research and Sponsored Programs; NIH-AREA grant

URI

http://digital.library.wisc.edu/1793/55083

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Student Research Day

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Probing the Role of Highly Conserved Lysine (K279) Residue in the Editing Domain of Bacterial Prolyl-tRNA Synthetases

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