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dc.contributor.authorFrederick, Kendra K.
dc.contributor.authorCaporini, Marc A.
dc.contributor.authorMichaelis, Vladimir K.
dc.contributor.authorAndreas, Loren
dc.contributor.authorLindquist, Susan
dc.contributor.authorDebelouchina, Galia Tzvetanova
dc.contributor.authorGriffin, Robert Guy
dc.date.accessioned2017-12-22T20:47:11Z
dc.date.available2017-12-22T20:47:11Z
dc.date.issued2017-03
dc.date.submitted2016-11
dc.identifier.issn0027-8424
dc.identifier.issn1091-6490
dc.identifier.urihttp://hdl.handle.net/1721.1/112944
dc.description.abstractThe yeast prion protein Sup35NM is a self-propagating amyloid. Despite intense study, there is no consensus on the organization of monomers within Sup35NM fibrils. Some studies point to a â-helical arrangement, whereas others suggest a parallel inregister organization. Intermolecular contacts are often determined by experiments that probe long-range heteronuclear contacts for fibrils templated from a 1:1 mixture of 13 C- and 15 N-labeled monomers. However, for Sup35NM, like many large proteins, chemical shift degeneracy limits the usefulness of this approach. Segmental and specific isotopic labeling reduce degeneracy, but experiments to measure long-range interactions are often too insensitive. To limit degeneracy and increase experimental sensitivity, we combined specific and segmental isotopic labeling schemes with dynamic nuclear polarization (DNP) NMR. Using this combination, we examined an amyloid form of Sup35NM that does not have a parallel in-register structure. The combination of a small number of specific labels with DNP NMR enables determination of architectural information about polymeric protein systems. Keyword: [PSI+] prion; solid-state NMR; amyloid; Sup35; dynamic nuclear polarizationen_US
dc.description.sponsorshipNational Institutes of Health (U.S.) (Grants GM-025874)en_US
dc.description.sponsorshipNational Institutes of Health (U.S.) (Grants EB-003151)en_US
dc.description.sponsorshipNational Institutes of Health (U.S.) (Grants EB-002804)en_US
dc.description.sponsorshipNational Institutes of Health (U.S.) (Grants EB-002026)en_US
dc.publisherProceedings of the National Academy of Sciencesen_US
dc.relation.isversionofhttp://dx.doi.org/10.1073/PNAS.1619051114en_US
dc.rightsArticle is made available in accordance with the publisher's policy and may be subject to US copyright law. Please refer to the publisher's site for terms of use.en_US
dc.sourcePNASen_US
dc.titleCombining DNP NMR with segmental and specific labeling to study a yeast prion protein strain that is not parallel in-registeren_US
dc.typeArticleen_US
dc.identifier.citationFrederick, Kendra K., et al. “Combining DNP NMR with Segmental and Specific Labeling to Study a Yeast Prion Protein Strain That Is Not Parallel in-Register.” Proceedings of the National Academy of Sciences, vol. 114, no. 14, Apr. 2017, pp. 3642–47. © 2017 National Academy of Sciencesen_US
dc.contributor.departmentMassachusetts Institute of Technology. Department of Biologyen_US
dc.contributor.departmentMassachusetts Institute of Technology. Department of Chemistryen_US
dc.contributor.departmentFrancis Bitter Magnet Laboratory (Massachusetts Institute of Technology)en_US
dc.contributor.mitauthorMichaelis, Vladimir K.
dc.contributor.mitauthorAndreas, Loren
dc.contributor.mitauthorLindquist, Susan
dc.contributor.mitauthorDebelouchina, Galia Tzvetanova
dc.contributor.mitauthorGriffin, Robert Guy
dc.relation.journalProceedings of the National Academy of Sciencesen_US
dc.eprint.versionFinal published versionen_US
dc.type.urihttp://purl.org/eprint/type/JournalArticleen_US
eprint.statushttp://purl.org/eprint/status/PeerRevieweden_US
dc.date.updated2017-12-22T17:23:06Z
dspace.orderedauthorsFrederick, Kendra K.; Michaelis, Vladimir K.; Caporini, Marc A.; Andreas, Loren B.; Debelouchina, Galia T.; Griffin, Robert G.; Lindquist, Susanen_US
dspace.embargo.termsNen_US
dc.identifier.orcidhttps://orcid.org/0000-0002-6708-7660
dc.identifier.orcidhttps://orcid.org/0000-0003-1307-882X
dc.identifier.orcidhttps://orcid.org/0000-0003-1589-832X
mit.licensePUBLISHER_POLICYen_US


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