Detection of tmRNA‐mediated trans‐translation products in Bacillus subtilis

Background: Bacterial tmRNA (10Sa RNA) is involved in a trans‐translation reaction, which contributes to the degradation of incompletely synthesized peptides and the recycling of stalled ribosomes. To investigate the physiological roles of this reaction in Bacillus subtilis, we devised a system for...

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Veröffentlicht in:Genes to cells : devoted to molecular & cellular mechanisms 2002-03, Vol.7 (3), p.343-350
Hauptverfasser: Fujihara, Ai, Tomatsu, Hisashi, Inagaki, Sachi, Tadaki, Toshimasa, Ushida, Chisato, Himeno, Hyouta, Muto, Akira
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container_end_page 350
container_issue 3
container_start_page 343
container_title Genes to cells : devoted to molecular & cellular mechanisms
container_volume 7
creator Fujihara, Ai
Tomatsu, Hisashi
Inagaki, Sachi
Tadaki, Toshimasa
Ushida, Chisato
Himeno, Hyouta
Muto, Akira
description Background: Bacterial tmRNA (10Sa RNA) is involved in a trans‐translation reaction, which contributes to the degradation of incompletely synthesized peptides and the recycling of stalled ribosomes. To investigate the physiological roles of this reaction in Bacillus subtilis, we devised a system for detecting the proteins that are subject to in vivo trans‐translation. Results: The wild‐type tmRNA gene (ssrA) in the genome was replaced by a variant ssrA encoding a tag‐peptide sequence containing six histidine residues (His‐tag) and two aspartic acids at the C‐terminus. The His‐tagged proteins that accumulated in the cells without degradation were fractionated by Ni2+‐NTA column and gel electrophoresis and were detected by Western blotting with an anti‐His‐tag antibody. The results showed that the trans‐translation occurred more frequently at a high temperature (50 °C) than at a low temperature (37 °C). Two‐dimensional (2D) gel electrophoresis of the products revealed many distinct spots, which represent specific target proteins for the trans‐translation reaction. Furthermore, the 2D gel patterns of the products from cells cultured at high and low temperatures were apparently different. Several tagged proteins were identified by the N‐terminal amino acid sequences of the products. Conclusion: Trans‐translation occurs more frequently at high temperature than at low temperature, and different proteins are tagged at different temperatures.
doi_str_mv 10.1046/j.1365-2443.2002.00523.x
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To investigate the physiological roles of this reaction in Bacillus subtilis, we devised a system for detecting the proteins that are subject to in vivo trans‐translation. Results: The wild‐type tmRNA gene (ssrA) in the genome was replaced by a variant ssrA encoding a tag‐peptide sequence containing six histidine residues (His‐tag) and two aspartic acids at the C‐terminus. The His‐tagged proteins that accumulated in the cells without degradation were fractionated by Ni2+‐NTA column and gel electrophoresis and were detected by Western blotting with an anti‐His‐tag antibody. The results showed that the trans‐translation occurred more frequently at a high temperature (50 °C) than at a low temperature (37 °C). Two‐dimensional (2D) gel electrophoresis of the products revealed many distinct spots, which represent specific target proteins for the trans‐translation reaction. Furthermore, the 2D gel patterns of the products from cells cultured at high and low temperatures were apparently different. Several tagged proteins were identified by the N‐terminal amino acid sequences of the products. 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source MEDLINE; Access via Wiley Online Library; Open Access Titles of Japan; EZB-FREE-00999 freely available EZB journals; Wiley Online Library (Open Access Collection)
subjects Bacillus subtilis - genetics
Bacterial Proteins - metabolism
Chromatography, Affinity
Mutation
Peptides - metabolism
Protein Biosynthesis
Ribosomes - metabolism
RNA, Bacterial - genetics
RNA, Bacterial - metabolism
title Detection of tmRNA‐mediated trans‐translation products in Bacillus subtilis
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