DESCRIPTION: (From the Applicant's Abstract) The goal of this project is to
obtain an understanding of the function of E. coli DbpA, a member of the large
DEAD/H family of proteins that participate in many cellular pathways involving
RNA. DEAD/H proteins couple the hydrolysis of ATP with RNA binding and are
proposed to modify RNA secondary and tertiary structure. E. Coli DbpA and its
B. subtilis homologue YxiN were chosen for detailed structural and mechanistic
studies because, unlike nearly all other DEAD/H proteins, they bind tightly and
specifically to a discrete region of 23S rRNA. The equilibrium and rate
constants for the steps in the minimal kinetic scheme of the ATPase reaction
will be determined to establish a framework for structure-function studies. The
possibility that DbpA acts as a helicase in restructuring rRNA will be
examined. RNA modification, photocrosslinking, and protein engineering
experiments will test how different domains of DbpA interact with its cognate
RNA, and whether the protein-RNA contacts change during the catalytic cycle.
Finally, a DbpA disruption strain of E. coli will be used to search for the
mechanism of action of DbpA in E. coli cells.
No Sub Projects information available for 5R01GM060268-02
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