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Translation. An RNA biosensor for imaging the first round of translation from single cells to living animals.


ABSTRACT: Analysis of single molecules in living cells has provided quantitative insights into the kinetics of fundamental biological processes; however, the dynamics of messenger RNA (mRNA) translation have yet to be addressed. We have developed a fluorescence microscopy technique that reports on the first translation events of individual mRNA molecules. This allowed us to examine the spatiotemporal regulation of translation during normal growth and stress and during Drosophila oocyte development. We have shown that mRNAs are not translated in the nucleus but translate within minutes after export, that sequestration within P-bodies regulates translation, and that oskar mRNA is not translated until it reaches the posterior pole of the oocyte. This methodology provides a framework for studying initiation of protein synthesis on single mRNAs in living cells.

SUBMITTER: Halstead JM 

PROVIDER: S-EPMC4451088 | biostudies-literature | 2015 Mar

REPOSITORIES: biostudies-literature

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Translation. An RNA biosensor for imaging the first round of translation from single cells to living animals.

Halstead James M JM   Lionnet Timothée T   Wilbertz Johannes H JH   Wippich Frank F   Ephrussi Anne A   Singer Robert H RH   Chao Jeffrey A JA  

Science (New York, N.Y.) 20150301 6228


Analysis of single molecules in living cells has provided quantitative insights into the kinetics of fundamental biological processes; however, the dynamics of messenger RNA (mRNA) translation have yet to be addressed. We have developed a fluorescence microscopy technique that reports on the first translation events of individual mRNA molecules. This allowed us to examine the spatiotemporal regulation of translation during normal growth and stress and during Drosophila oocyte development. We hav  ...[more]

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