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Assembly of the human signal recognition particle (SRP): Overlap of regions required for binding of protein SRP54 and assembly control

Published online by Cambridge University Press:  11 January 2002

JIAMING YIN
Affiliation:
Department of Molecular Biology, The University of Texas Health Science Center at Tyler, Tyler, Texas 75708-3154, USA
CHING-HUI YANG
Affiliation:
Department of Molecular Biology, The University of Texas Health Science Center at Tyler, Tyler, Texas 75708-3154, USA
CHRISTIAN ZWIEB
Affiliation:
Department of Molecular Biology, The University of Texas Health Science Center at Tyler, Tyler, Texas 75708-3154, USA
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Abstract

Assembly of the human signal recognition particle (SRP) entails the incorporation of protein SRP54, mediated by a protein SRP19-induced conformational change in SRP RNA. To localize the region that controls this crucial step in the assembly of human SRP RNA, four chimeras, Ch-1 to Ch-4, composed of portions of human and Methanococcus jannashii SRP RNAs, were generated by PCR site-directed mutagenesis from a larger precursor. Protein-binding activities of the hybrid RNAs were determined using purified human SRP19 and a polypeptide (SRP54M) that corresponded to the methionine-rich domain of human SRP54. Mutant Ch-1 containing the large domain of M. jannashii SRP RNA, as well as mutant Ch-2 RNA in which helices 6 and 8 were replaced, bound SRP54M independently of SRP19. Mutant Ch-3 RNA, which contained M. jannashii helix 6, required SRP19 for binding of SRP54M, but mutant Ch-4 RNA, which possessed M. jannashii helix 8, bound SRP54M without SRP19. We concluded that the formation of a stable ternary complex did not rely on extensive conformational changes that might take place throughout the large domain of SRP, but was controlled by a smaller region encompassing certain RNA residues at positions 177 to 221. Five chimeric RNAs altered within helix 8 were used to investigate the potential role of a significant AA-to-U change and to determine the boundaries of the assembly control region. Reduced protein-binding activities of these chimeras demonstrated a considerable overlap of regions required for SRP54 binding and assembly control.

Type
REPORTS
Information
RNA , Volume 7 , Issue 10 , October 2001 , pp. 1389 - 1396
Copyright
2001 RNA Society

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