Your search keyword '"Heather M. Frank"' showing total 2 results

1. Identification of the initial nucleocapsid recognition element in the HIV-1 RNA packaging signal

Author

Aaron Kidane, Emily Cannistraci, Heather M. Frank, Hana Flores, Alice Telesnitsky, Christina Quasney, Pengfei Ding, Verna Van, Alexis Waller, Sapna Basappa, Nansen Kuo, Ugonna Mbaekwe, Michael F. Summers, Canessa Swanson, Siarhei Kharytonchyk, Mitali Sarkar, and Ridhi Chaudhary

Subjects

Base pair, packaging, nucleocapsid, HIV Infections, Genome, Viral, Regulatory Sequences, Ribonucleic Acid, Biochemistry, Hiv 1 rna, Virus, Commentaries, Humans, Binding site, genome, Binding Sites, Multidisciplinary, Base Sequence, Chemistry, Virus Assembly, Virion, RNA, Nucleocapsid Proteins, Biological Sciences, Affinities, Helix, Biophysics, HIV-1, Nucleic Acid Conformation, RNA, Viral, Function (biology), Protein Binding

Abstract

Significance Understanding the molecular determinants of retroviral genome packaging is important for drug discovery and development of vectors for gene delivery. We show that the HIV-1 leader, which contains the RNA elements necessary for genome packaging, binds approximately two dozen copies of the cognate NC protein with affinities ranging from ∼40 nM to 1.4 µM. Binding to the four highest-affinity “initial” binding sites occurs with endothermic energetics attributed to NC-induced localized RNA melting. Mutations that stabilize these sites inhibit NC binding in vitro and RNA packaging in transfected cells. A small-molecule inhibitor of RNA packaging binds specifically to the initial NC binding sites and stabilizes the RNA structure. Our findings identify a potential RNA Achilles’ heel for HIV therapeutic development., Selective packaging of the HIV-1 genome during virus assembly is mediated by interactions between the dimeric 5ʹ-leader of the unspliced viral RNA and the nucleocapsid (NC) domains of a small number of assembling viral Gag polyproteins. Here, we show that the dimeric 5′-leader contains more than two dozen NC binding sites with affinities ranging from 40 nM to 1.4 μM, and that all high-affinity sites (Kd ≲ 400 nM) reside within a ∼150-nt region of the leader sufficient to promote RNA packaging (core encapsidation signal, ΨCES). The four initial binding sites with highest affinity reside near two symmetrically equivalent three-way junction structures. Unlike the other high-affinity sites, which bind NC with exothermic energetics, binding to these sites occurs endothermically due to concomitant unwinding of a weakly base-paired [UUUU]:[GGAG] helical element. Mutations that stabilize base pairing within this element eliminate NC binding to this site and severely impair RNA packaging into virus-like particles. NMR studies reveal that a recently discovered small-molecule inhibitor of HIV-1 RNA packaging that appears to function by stabilizing the structure of the leader binds directly to the [UUUU]:[GGAG] helix. Our findings suggest a sequential NC binding mechanism for Gag-genome assembly and identify a potential RNA Achilles’ heel to which HIV therapeutics may be targeted.

Published

2020

2. NMR detection of intermolecular interaction sites in the dimeric 5′-leader of the HIV-1 genome

Author

Justin Santos, Michael F. Summers, Sarah C. Keane, Xiao Heng, Sayo McCowin, Carly A. Sciandra, Heather M. Frank, and Verna Van

Subjects

0301 basic medicine, chemistry.chemical_classification, Multidisciplinary, Pseudodiploid, 030102 biochemistry & molecular biology, Polyadenylation, Base pair, Dimer, Intermolecular force, RNA, Biology, 03 medical and health sciences, Crystallography, chemistry.chemical_compound, 030104 developmental biology, chemistry, Duplex (building), Nucleotide

Abstract

HIV type-1 (HIV-1) contains a pseudodiploid RNA genome that is selected for packaging and maintained in virions as a noncovalently linked dimer. Genome dimerization is mediated by conserved elements within the 5′-leader of the RNA, including a palindromic dimer initiation signal (DIS) that has been proposed to form kissing hairpin and/or extended duplex intermolecular contacts. Here, we have applied a 2H-edited NMR approach to directly probe for intermolecular interactions in the full-length, dimeric HIV-1 5′-leader (688 nucleotides; 230 kDa). The interface is extensive and includes DIS:DIS base pairing in an extended duplex state as well as intermolecular pairing between elements of the upstream Unique-5′ (U5) sequence and those near the gag start site (AUG). Other pseudopalindromic regions of the leader, including the transcription activation (TAR), polyadenylation (PolyA), and primer binding (PBS) elements, do not participate in intermolecular base pairing. Using a 2H-edited one-dimensional NMR approach, we also show that the extended interface structure forms on a time scale similar to that of overall RNA dimerization. Our studies indicate that a kissing dimer-mediated structure, if formed, exists only transiently and readily converts to the extended interface structure, even in the absence of the HIV-1 nucleocapsid protein or other RNA chaperones.

Published

2016