| ID | 57286 |
| FullText URL | |
| Author |
Nomura, Kaoru
Bioorganic Research Institute, Suntory Foundation for Life Sciences
Yamaguchi, Toshiyuki
Bioorganic Research Institute, Suntory Foundation for Life Sciences
Mori, Shoko
Bioorganic Research Institute, Suntory Foundation for Life Sciences
Fujikawa, Kohki
Bioorganic Research Institute, Suntory Foundation for Life Sciences
Nishiyama, Ken-ichi
Department of Biological Chemistry and Food Sciences, Faculty of Agriculture, Iwate University
Shimanouchi, Toshinori
Graduate School of Environmental Science, Okayama University
ORCID
Kaken ID
researchmap
Morigaki, Kenichi
Biosignal Research Center, Kobe University
Shimamoto, Keiko
Bioorganic Research Institute, Suntory Foundation for Life Sciences
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| Abstract | After a nascent chain of a membrane protein emerges from the ribosomal tunnel, the protein is integrated into the cell membrane. This process is controlled by a series of proteinaceous molecular devices, such as signal recognition particles and Sec translocons. In addition to these proteins, we discovered two endogenous components regulating membrane protein integration in the inner membrane of Escherichia coli. The integration is blocked by diacylglycerol (DAG), whereas the blocking is relieved by a glycolipid named membrane protein integrase (MPIase). Here, we investigated the influence of these integration-blocking and integration-promoting factors on the physicochemical properties of membrane lipids via solid-state NMR and fluorescence measurements. These factors did not have destructive effects on membrane morphology because the membrane maintained its lamellar structure and did not fuse in the presence of DAG and/or MPIase at their effective concentrations. We next focused on membrane flexibility. DAG did not affect the mobility of the membrane surface, whereas the sugar chain in MPIase was highly mobile and enhanced the flexibility of membrane lipid headgroups. Comparison with a synthetic MPIase analog revealed the effects of the long sugar chain on membrane properties. The acyl chain order inside the membrane was increased by DAG, whereas the increase was cancelled by the addition of MPIase. MPIase also loosened the membrane lipid packing. Focusing on the transbilayer movement, MPIase reduced the rapid flip-flop motion of DAG. On the other hand, MPIase could not compensate for the diminished lateral diffusion by DAG. These results suggest that by manipulating the membrane lipids dynamics, DAG inhibits the protein from contacting the inner membrane, whereas the flexible long sugar chain of MPIase increases the opportunity for interaction between the membrane and the protein, leading to membrane integration of the newly formed protein.
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| Published Date | 2019-07-09
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| Publication Title |
Biophysical Journal
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| Volume | volume117
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| Issue | issue1
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| Publisher | elsevier
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| Start Page | 99
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| End Page | 110
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| ISSN | 00063495
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| NCID | AA00566095
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| Content Type |
Journal Article
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| language |
English
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| OAI-PMH Set |
岡山大学
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| Copyright Holders | © 2019 Biophysical Society.
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| File Version | publisher
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| PubMed ID | |
| DOI | |
| Web of Science KeyUT | |
| Related Url | isVersionOf https://doi.org/10.1016/j.bpj.2019.05.014
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| License | http://creativecommons.org/licenses/by/4.0/
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| Citation | Nomura K, Yamaguchi T, Mori S, et al. Alteration of Membrane Physicochemical Properties by Two Factors for Membrane Protein Integration. Biophys J. 2019;117(1):99‐110. doi:10.1016/j.bpj.2019.05.014
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| Funder Name |
Japan Society for the Promotion of Science
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| 助成番号 | 18K06143
17K13262
15KT0073
17H02209
18H04433
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| Open Access (Publisher) |
OA
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| Open Archive (publisher) |
Non-OpenArchive
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