Preethi Chandramouli scite author profile

In this paper, we present a structure of the mammalian ribosome determined at approximately 8.7 A resolution by electron cryomicroscopy and single-particle methods. A model of the ribosome was created by docking homology models of subunit rRNAs and conserved proteins into the density map. We then modeled expansion segments in the subunit rRNAs and found unclaimed density for approximately 20 proteins. In general, many conserved proteins and novel proteins interact with expansion segments to form an integrated framework that may stabilize the mature ribosome. Our structure provides a snapshot of the mammalian ribosome at the beginning of translation and lends support to current models in which large movements of the small subunit and L1 stalk occur during tRNA translocation. Finally, details are presented for intersubunit bridges that are specific to the eukaryotic ribosome. We suggest that these bridges may help reset the conformation of the ribosome to prepare for the next cycle of chain elongation.

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Architecture of the Ribosome–Channel Complex Derived from Native Membranes

Ménétret

Hegde

Heinrich

et al. 2005

Journal of Molecular Biology

125

124

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Structure and size determination of bacteriophage P2 and P4 procapsids: Function of size responsiveness mutations

Dearborn

Laurinmäki

Chandramouli

et al. 2012

Journal of Structural Biology

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Cleavage leads to expansion of bacteriophage P4 procapsids in vitro

Wang¹,

Chandramouli²,

Butcher³

et al. 2003

Virology

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Proteolytic cleavage of the structural proteins is an important part of the maturation process for most bacteriophages and other viruses. In the double-stranded DNA bacteriophages this cleavage is associated with DNA packaging, capsid expansion, and scaffold removal. To understand the role of protein cleavage in the expansion of bacteriophages P2 and P4, we have experimentally cleaved P4 procapsids produced by overexpression of the capsid and scaffolding proteins. The cleavage leads to particle expansion and scaffold removal in vitro. The resulting expanded capsid has a thin-shelled structure similar, but not identical, to that of mature virions.

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Validation of the orthogonal tilt reconstruction method with a biological test sample

Chandramouli

Hernández-López

Wang

et al. 2011

Journal of Structural Biology

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