Your search keyword '"Rausch JW"' showing total 59 results

1. Interaction of p55 reverse transcriptase from the Saccharomyces cerevisiae retrotransposon Ty3 with conformationally distinct nucleic acid duplexes.

Author

Rausch, JW, Grice, MK, Henrietta, M, Nymark-McMahon, Miller, JT, and Le Grice, SF

Subjects

Saccharomyces cerevisiae, RNA-Directed DNA Polymerase, Fungal Proteins, DNA, Fungal, Retroelements, RNA, Fungal, Base Sequence, Nucleic Acid Conformation, Molecular Sequence Data, DNA, Fungal, RNA, Biological Sciences, Medical and Health Sciences, Chemical Sciences, Biochemistry & Molecular Biology

Abstract

The 55-kDa reverse transcriptase (RT) domain of the Ty3 POL3 open reading frame was purified and evaluated on conformationally distinct nucleic acid duplexes. Purified enzyme migrated as a monomer by size exclusion chromatography. Enzymatic footprinting indicate Ty3 RT protects template nucleotides +7 through -21 and primer nucleotides -1 through -24. Contrary to previous data with retroviral enzymes, a 4-base pair region of the template-primer duplex remained nuclease accessible. The C-terminal portion of Ty3 RT encodes a functional RNase H domain, although the hydrolysis profile suggests an increased spatial separation between the catalytic centers. Despite conservation of catalytically important residues in the RNase H domain, Fe(2+) fails to replace Mg(2+) in the RNase H catalytic center for localized generation of hydroxyl radicals, again suggesting this domain may be structurally distinct from its retroviral counterparts. RNase H specificity was investigated using a model system challenging the enzyme to select the polypurine tract primer from within an RNA/DNA hybrid, extend this into (+) DNA, and excise the primer from nascent DNA. Purified RT catalyzed each of these three steps but was almost inactive on a non-polypurine tract RNA primer. Our studies provide the first detailed characterization of the enzymatic activities of a retrotransposon reverse transcriptase.

Published

2000

2. Reverse Transcriptase-Associated Ribonuclease H Activity as a Target for Antiviral Chemotherapy

Author

Rausch, JW, primary and Grice, SFJ Le, additional

Published

1997

3. HIV Expression in Infected T Cell Clones.

Author

Rausch JW, Parvez S, Pathak S, Capoferri AA, and Kearney MF

Subjects

Humans, CD4-Positive T-Lymphocytes, T-Lymphocytes, Cytotoxic, Cell Division, Clone Cells, HIV Seropositivity, HIV-1

Abstract

The principal barrier to an HIV-1 cure is the persistence of infected cells harboring replication-competent proviruses despite antiretroviral therapy (ART). HIV-1 transcriptional suppression, referred to as viral latency, is foremost among persistence determinants, as it allows infected cells to evade the cytopathic effects of virion production and killing by cytotoxic T lymphocytes (CTL) and other immune factors. HIV-1 persistence is also governed by cellular proliferation, an innate and essential capacity of CD4+ T cells that both sustains cell populations over time and enables a robust directed response to immunological threats. However, when HIV-1 infects CD4+ T cells, this capacity for proliferation can enable surreptitious HIV-1 propagation without the deleterious effects of viral gene expression in latently infected cells. Over time on ART, the HIV-1 reservoir is shaped by both persistence determinants, with selective forces most often favoring clonally expanded infected cell populations harboring transcriptionally quiescent proviruses. Moreover, if HIV latency is incomplete or sporadically reversed in clonal infected cell populations that are replenished faster than they are depleted, such populations could both persist indefinitely and contribute to low-level persistent viremia during ART and viremic rebound if treatment is withdrawn. In this review, select genetic, epigenetic, cellular, and immunological determinants of viral transcriptional suppression and clonal expansion of HIV-1 reservoir T cells, interdependencies among these determinants, and implications for HIV-1 persistence will be presented and discussed.

Published

2024

4. Deep Sequencing Analysis of Individual HIV-1 Proviruses Reveals Frequent Asymmetric Long Terminal Repeats.

Author

Joseph KW, Halvas EK, Brandt LD, Patro SC, Rausch JW, Chopra A, Mallal S, Kearney MF, Coffin JM, and Mellors JW

Subjects

HIV Infections virology, High-Throughput Nucleotide Sequencing, Humans, Leukocytes, Mononuclear virology, HIV-1 genetics, HIV-1 metabolism, Proviruses genetics, Proviruses metabolism, Terminal Repeat Sequences genetics

Abstract

Effective strategies to eliminate human immunodeficiency virus type 1 (HIV-1) reservoirs are likely to require more thorough characterizations of proviruses that persist on antiretroviral therapy (ART). The rarity of infected CD4 + T-cells and related technical challenges have limited the characterization of integrated proviruses. Current approaches using next-generation sequencing can be inefficient and limited sequencing depth can make it difficult to link proviral sequences to their respective integration sites. Here, we report on an efficient method by which HIV-1 proviruses and their sites of integration are amplified and sequenced. Across five HIV-1-positive individuals on clinically effective ART, a median of 41.2% ( n  = 88 of 209) of amplifications yielded near-full-length proviruses and their 5'-host-virus junctions containing a median of 430 bp (range, 18 to 1,363 bp) of flanking host sequence. Unexpectedly, 29.5% ( n  = 26 of 88) of the sequenced proviruses had structural asymmetries between the 5' and 3' long terminal repeats (LTRs), commonly in the form of major 3' deletions. Sequence-intact proviruses were detected in 3 of 5 donors, and infected CD4 + T-cell clones were detected in 4 of 5 donors. The accuracy of the method was validated by amplifying and sequencing full-length proviruses and flanking host sequences directly from peripheral blood mononuclear cell DNA. The individual proviral sequencing assay (IPSA) described here can provide an accurate, in-depth, and longitudinal characterization of HIV-1 proviruses that persist on ART, which is important for targeting proviruses for elimination and assessing the impact of interventions designed to eradicate HIV-1. IMPORTANCE The integration of human immunodeficiency virus type 1 (HIV-1) into chromosomal DNA establishes the long-term persistence of HIV-1 as proviruses despite effective antiretroviral therapy (ART). Characterizing proviruses is difficult because of their rarity in individuals on long-term suppressive ART, their highly polymorphic sequences and genetic structures, and the need for efficient amplification and sequencing of the provirus and its integration site. Here, we describe a novel, integrated, two-step method (individual proviral sequencing assay [IPSA]) that amplifies the host-virus junction and the full-length provirus except for the last 69 bp of the 3' long terminal repeat (LTR). Using this method, we identified the integration sites of proviruses, including those that are sequence intact and replication competent or defective. Importantly, this new method identified previously unreported asymmetries between LTRs that have implications for how proviruses are detected and quantified. The IPSA method reported is unaffected by LTR asymmetries, permitting a more accurate and comprehensive characterization of the proviral landscape.

Published

2022

5. A Pre-Vaccination Baseline of SARS-CoV-2 Genetic Surveillance and Diversity in the United States.

Author

Capoferri AA, Shao W, Spindler J, Coffin JM, Rausch JW, and Kearney MF

Subjects

COVID-19 epidemiology, COVID-19 prevention & control, COVID-19 Vaccines immunology, Evolution, Molecular, Genetic Variation, Humans, Mutation, Phylogeny, SARS-CoV-2 classification, SARS-CoV-2 immunology, Spike Glycoprotein, Coronavirus genetics, Spike Glycoprotein, Coronavirus immunology, United States epidemiology, COVID-19 virology, SARS-CoV-2 genetics

Abstract

COVID-19 vaccines were first administered on 15 December 2020, marking an important transition point for the spread of SARS-CoV-2 in the United States (U.S.). Prior to this point in time, the virus spread to an almost completely immunologically naïve population, whereas subsequently, vaccine-induced immune pressure and prior infections might be expected to influence viral evolution. Accordingly, we conducted a study to characterize the spread of SARS-CoV-2 in the U.S. pre-vaccination, investigate the depth and uniformity of genetic surveillance during this period, and measure and otherwise characterize changing viral genetic diversity, including by comparison with more recently emergent variants of concern (VOCs). In 2020, SARS-CoV-2 spread across the U.S. in three phases distinguishable by peaks in the numbers of infections and shifting geographical distributions. Virus was genetically sampled during this period at an overall rate of ~1.2%, though there was a substantial mismatch between case rates and genetic sampling nationwide. Viral genetic diversity tripled over this period but remained low in comparison to other widespread RNA virus pathogens, and although 54 amino acid changes were detected at frequencies exceeding 5%, linkage among them was not observed. Based on our collective observations, our analysis supports a targeted strategy for worldwide genetic surveillance as perhaps the most sensitive and efficient means of detecting new VOCs.

Published

2022

6. 2020 SARS-CoV-2 diversification in the United States: Establishing a pre-vaccination baseline.

Author

Capoferri AA, Shao W, Spindler J, Coffin JM, Rausch JW, and Kearney MF

Abstract

In 2020, SARS-CoV-2 spread across the United States (U.S.) in three phases distinguished by peaks in the numbers of infections and shifting geographical distribution. We investigated the viral genetic diversity in each phase using sequences publicly available prior to December 15 th , 2020, when vaccination was initiated in the U.S. In Phase 1 (winter/spring), sequences were already dominated by the D614G Spike mutation and by Phase 3 (fall), genetic diversity of the viral population had tripled and at least 54 new amino acid changes had emerged at frequencies above 5%, several of which were within known antibody epitopes. These findings highlight the need to track the evolution of SARS-CoV-2 variants in the U.S. to ensure continued efficacy of vaccines and antiviral treatments., One Sentence Summary: SARS-CoV-2 genetic diversity in the U.S. increased 3-fold in 2020 and 54 emergent nonsynonymous mutations were detected.

Published

2021

7. CpG Methylation Profiles of HIV-1 Pro-Viral DNA in Individuals on ART.

Author

Boltz VF, Ceriani C, Rausch JW, Shao W, Bale MJ, Keele BF, Hoh R, Milush JM, Deeks SG, Maldarelli F, Kearney MF, and Coffin JM

Subjects

Antiretroviral Therapy, Highly Active, Gene Expression Regulation, Viral, Genome, Viral, Genomics methods, HIV Infections drug therapy, HIV Long Terminal Repeat genetics, Humans, Virus Latency genetics, CpG Islands, DNA Methylation, DNA, Viral, HIV Infections genetics, HIV Infections virology, HIV-1 genetics, Proviruses genetics

Abstract

The latent HIV-1 reservoir is comprised of stably integrated and intact proviruses with limited to no viral transcription. It has been proposed that latent infection may be maintained by methylation of pro-viral DNA. Here, for the first time, we investigate the cytosine methylation of a replication competent provirus (AMBI-1) found in a T cell clone in a donor on antiretroviral therapy (ART). Methylation profiles of the AMBI-1 provirus were compared to other proviruses in the same donor and in samples from three other individuals on ART, including proviruses isolated from lymph node mononuclear cells (LNMCs) and peripheral blood mononuclear cells (PBMCs). We also evaluated the apparent methylation of cytosines outside of CpG (i.e., CpH) motifs. We found no evidence for methylation in AMBI-1 or any other provirus tested within the 5' LTR promoter. In contrast, CpG methylation was observed in the env-tat-rev overlapping reading frame. In addition, we found evidence for differential provirus methylation in cells isolated from LNMCs vs. PBMCs in some individuals, possibly from the expansion of infected cell clones. Finally, we determined that apparent low-level methylation of CpH cytosines is consistent with occasional bisulfite reaction failures. In conclusion, our data do not support the proposition that latent HIV infection is associated with methylation of the HIV 5' LTR promoter.

Published

2021

8. Characterizing and circumventing sequence restrictions for synthesis of circular RNA in vitro.

Author

Rausch JW, Heinz WF, Payea MJ, Sherpa C, Gorospe M, and Le Grice SFJ

Subjects

Base Sequence, Exons, Humans, Introns, Mutagenesis, Mutation, Nucleic Acid Conformation, RNA, Circular chemistry, RNA, Circular chemical synthesis

Abstract

Just as eukaryotic circular RNA (circRNA) is a product of intracellular backsplicing, custom circRNA can be synthesized in vitro using a transcription template in which transposed halves of a split group I intron flank the sequence of the RNA to be circularized. Such permuted intron-exon (PIE) constructs have been used to produce circRNA versions of ribozymes, mimics of viral RNA motifs, a streptavidin aptamer, and protein expression vectors for genetic engineering and vaccine development. One limitation of this approach is the obligatory incorporation of small RNA segments (E1 and E2) into nascent circRNA at the site of end-joining. This restriction may preclude synthesis of small circRNA therapeutics and RNA nanoparticles that are sensitive to extraneous sequence, as well as larger circRNA mimics whose sequences must precisely match those of the native species on which they are modelled. In this work, we used serial mutagenesis and in vitro selection to determine how varying E1 and E2 sequences in a thymidylate synthase (td) group I intron PIE transcription template construct affects circRNA synthesis yield. Based on our collective findings, we present guidelines for the design of custom-tailored PIE transcription templates from which synthetic circRNAs of almost any sequence may be efficiently synthesized., (Published by Oxford University Press on behalf of Nucleic Acids Research 2021.)

Published

2021

9. HIV-1 viremia not suppressible by antiretroviral therapy can originate from large T cell clones producing infectious virus.

Author

Halvas EK, Joseph KW, Brandt LD, Guo S, Sobolewski MD, Jacobs JL, Tumiotto C, Bui JK, Cyktor JC, Keele BF, Morse GD, Bale MJ, Shao W, Kearney MF, Coffin JM, Rausch JW, Wu X, Hughes SH, and Mellors JW

Subjects

Anti-Retroviral Agents, Female, HIV-1 genetics, Humans, Introns immunology, Male, RNA, Viral genetics, HIV Infections genetics, HIV Infections immunology, HIV-1 immunology, RNA, Viral immunology, T-Lymphocytes immunology, T-Lymphocytes virology, Viremia genetics, Viremia immunology, Virus Integration

Abstract

BACKGROUNDHIV-1 viremia that is not suppressed by combination antiretroviral therapy (ART) is generally attributed to incomplete medication adherence and/or drug resistance. We evaluated individuals referred by clinicians for nonsuppressible viremia (plasma HIV-1 RNA above 40 copies/mL) despite reported adherence to ART and the absence of drug resistance to the current ART regimen.METHODSSamples were collected from at least 2 time points from 8 donors who had nonsuppressible viremia for more than 6 months. Single templates of HIV-1 RNA obtained from plasma and viral outgrowth of cultured cells and from proviral DNA were amplified by PCR and sequenced for evidence of clones of cells that produced infectious viruses. Clones were confirmed by host-proviral integration site analysis.RESULTSHIV-1 genomic RNA with identical sequences were identified in plasma samples from all 8 donors. The identical viral RNA sequences did not change over time and did not evolve resistance to the ART regimen. In 4 of the donors, viral RNA sequences obtained from plasma matched those sequences from viral outgrowth cultures, indicating that the viruses were replication competent. Integration sites for infectious proviruses from those 4 donors were mapped to the introns of the MATR3, ZNF268, ZNF721/ABCA11P, and ABCA11P genes. The sizes of the clones were estimated to be from 50 million to 350 million cells.CONCLUSIONThese findings show that clones of HIV-1-infected cells producing virus can cause failure of ART to suppress viremia. The mechanisms involved in clonal expansion and persistence need to be defined to effectively target viremia and the HIV-1 reservoir.FUNDINGNational Cancer Institute, NIH; Howard Hughes Medical Research Fellows Program, Howard Hughes Medical Institute; Bill and Melinda Gates Foundation; Office of AIDS Research; American Cancer Society; National Cancer Institute through a Leidos subcontract; National Institute for Allergy and Infectious Diseases, NIH, to the I4C Martin Delaney Collaboratory; University of Rochester Center for AIDS Research and University of Rochester HIV/AIDS Clinical Trials Unit.

Published

2020

10. Low genetic diversity may be an Achilles heel of SARS-CoV-2.

Author

Rausch JW, Capoferri AA, Katusiime MG, Patro SC, and Kearney MF

Subjects

Betacoronavirus, COVID-19, COVID-19 Vaccines, Genetic Variation, Humans, SARS-CoV-2, Viral Vaccines, Coronavirus Infections prevention & control, Pandemics, Pneumonia, Viral, Severe Acute Respiratory Syndrome

Abstract

Competing Interests: The authors declare no competing interest.

Published

2020

11. HIV Genetic Diversity - Superpower of a Formidable Virus.

Author

Sherpa C, Rausch JW, and Le Grice SFJ

Subjects

Antibodies, Viral therapeutic use, Dependovirus genetics, HIV Infections epidemiology, HIV Infections virology, HIV-1 isolation & purification, Humans, Anti-HIV Agents therapeutic use, Genetic Variation genetics, HIV Infections drug therapy, HIV-1 drug effects, HIV-1 genetics

Published

2020

12. Characterizing the Latent HIV-1 Reservoir in Patients with Viremia Suppressed on cART: Progress, Challenges, and Opportunities.

Author

Rausch JW and Le Grice SFJ

Subjects

HIV-1 drug effects, Humans, Viral Load drug effects, Viremia drug therapy, Virus Activation drug effects, Virus Replication drug effects, Acquired Immunodeficiency Syndrome drug therapy, Anti-HIV Agents therapeutic use, CD4-Positive T-Lymphocytes virology, Proviruses genetics, Viral Load genetics, Virus Latency genetics

Abstract

Modern combination antiretroviral therapy (cART) can bring HIV-1 in blood plasma to level undetectable by standard tests, prevent the onset of acquired immune deficiency syndrome (AIDS), and allow a near-normal life expectancy for HIV-infected individuals. Unfortunately, cART is not curative, as within a few weeks of treatment cessation, HIV viremia in most patients rebounds to pre-cART levels. The primary source of this rebound, and the principal barrier to a cure, is the highly stable reservoir of latent yet replication-competent HIV-1 proviruses integrated into the genomic DNA of resting memory CD4+ T cells. In this review, prevailing models for how the latent reservoir is established and maintained, residual viremia and viremic rebound upon withdrawal of cART, and the types and characteristics of cells harboring latent HIV-1 will be discussed. Selected technologies currently being used to advance our understanding of HIV latency will also be presented, as will a perspective on which areas of advancement are most essential for producing the next generation of HIV-1 therapeutics., (Copyright© Bentham Science Publishers; For any queries, please email at epub@benthamscience.net.)

Published

2020

13. Combined HIV-1 sequence and integration site analysis informs viral dynamics and allows reconstruction of replicating viral ancestors.

Author

Patro SC, Brandt LD, Bale MJ, Halvas EK, Joseph KW, Shao W, Wu X, Guo S, Murrell B, Wiegand A, Spindler J, Raley C, Hautman C, Sobolewski M, Fennessey CM, Hu WS, Luke B, Hasson JM, Niyongabo A, Capoferri AA, Keele BF, Milush J, Hoh R, Deeks SG, Maldarelli F, Hughes SH, Coffin JM, Rausch JW, Mellors JW, and Kearney MF

Subjects

Anti-Retroviral Agents therapeutic use, Base Sequence, Cell Line, DNA, Viral genetics, Drug Resistance, Viral, HIV Infections virology, Humans, Leukocytes, Mononuclear virology, Lymph Nodes virology, Mutation, Proviruses genetics, Virus Integration physiology, HIV-1 genetics, Virus Integration genetics, Virus Replication genetics

Abstract

Understanding HIV-1 persistence despite antiretroviral therapy (ART) is of paramount importance. Both single-genome sequencing (SGS) and integration site analysis (ISA) provide useful information regarding the structure of persistent HIV DNA populations; however, until recently, there was no way to link integration sites to their cognate proviral sequences. Here, we used multiple-displacement amplification (MDA) of cellular DNA diluted to a proviral endpoint to obtain full-length proviral sequences and their corresponding sites of integration. We applied this method to lymph node and peripheral blood mononuclear cells from 5 ART-treated donors to determine whether groups of identical subgenomic sequences in the 2 compartments are the result of clonal expansion of infected cells or a viral genetic bottleneck. We found that identical proviral sequences can result from both cellular expansion and viral genetic bottlenecks occurring prior to ART initiation and following ART failure. We identified an expanded T cell clone carrying an intact provirus that matched a variant previously detected by viral outgrowth assays and expanded clones with wild-type and drug-resistant defective proviruses. We also found 2 clones from 1 donor that carried identical proviruses except for nonoverlapping deletions, from which we could infer the sequence of the intact parental virus. Thus, MDA-SGS can be used for "viral reconstruction" to better understand intrapatient HIV-1 evolution and to determine the clonality and structure of proviruses within expanded clones, including those with drug-resistant mutations. Importantly, we demonstrate that identical sequences observed by standard SGS are not always sufficient to establish proviral clonality., Competing Interests: Competing interest statement: J.W.M. is a consultant to Gilead Sciences, Merck Research Laboratories, Janssen Pharmaceuticals, and AccelevirDx, and a share option holder of Co-Crystal, Inc. B.F.K. and J.A.H. are co-authors on an October 2015 article. The remaining authors have no potential conflicts.

Published

2019

14. Using SHAPE-MaP to probe small molecule-RNA interactions.

Author

Martin S, Blankenship C, Rausch JW, and Sztuba-Solinska J

Subjects

Acylation drug effects, Humans, Ligands, RNA drug effects, RNA ultrastructure, Small Molecule Libraries pharmacology, Nucleic Acid Conformation drug effects, RNA chemistry, Sequence Analysis, RNA methods, Small Molecule Libraries chemistry

Abstract

RNA is a regulator and catalyst of many cellular processes. Efforts to therapeutically harness RNA began with the discovery of myriad coding and non-coding RNAs and their versatile modes of action. However, due to its dynamic structure and the polar and repetitive nature of its surface, RNA presents a challenging target for drug design. For an RNA to be druggable, it must contain a motif that assumes a nearly fixed and unique conformation that a small molecule can recognize and bind consistently and with high affinity. Hence, reliable methods for determining the secondary and tertiary structures of RNA, and even the features and occupancy of potential drug binding sites are of utmost importance for the effective design of RNA-based therapeutics. Selective 2'-hydroxyl acylation analyzed by primer extension and mutational profiling (SHAPE-MaP) has emerged as such a method, by which RNA secondary structure can be probed at single-nucleotide resolution, under a variety of conditions, and in the presence of RNA-specific small-molecule ligands. In this review, we describe an in-depth protocol for using SHAPE-MaP to characterize RNA-small molecule interactions in cell culture (in cellulo). This method can be applied to transcripts of any size or abundance, and to determine the sites and affinities of small molecule binding, making it an essential and versatile tool for drug discovery., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2019

15. Interplay of primary sequence, position and secondary RNA structure determines alternative splicing of LMNA in a pre-mature aging syndrome.

Author

Shilo A, Tosto FA, Rausch JW, Le Grice SFJ, and Misteli T

Subjects

DNA Mutational Analysis, Exons, Fibroblasts metabolism, HEK293 Cells, Humans, Lamin Type A metabolism, Mutation, Nuclear Proteins metabolism, Nucleic Acid Conformation, Point Mutation, Progeria genetics, Protein Structure, Secondary, RNA Splice Sites, RNA Splicing, RNA, Small Nuclear, Syndrome, Alternative Splicing, Lamin Type A genetics, RNA chemistry

Abstract

Aberrant splicing in exon 11 of the LMNA gene causes the premature aging disorder Hutchinson-Gilford Progeria Syndrome. A de novo C1824T mutation activates an internal alternative 5' splice site, resulting in formation of the disease-causing progerin protein. The underlying mechanism for this 5' splice site selection is unknown. Here, we have applied a combination of targeted mutational analysis in a cell-based system and structural mapping by SHAPE-MaP to comprehensively probe the contributions of primary sequence, secondary RNA structure and linear splice site position in determining in vivo mechanisms of splice site choice in LMNA. While splice site choice is in part defined by sequence complementarity to U1 snRNA, we identify RNA secondary structural elements near the alternative 5' splice sites and show that splice site choice is significantly influenced by the structural context of the available splice sites. Furthermore, relative positioning of the competing sites within the primary sequence of the pre-mRNA is a predictor of 5' splice site usage, with the distal position favored over the proximal, regardless of sequence composition. Together, these results demonstrate that 5' splice site selection in LMNA is determined by an intricate interplay among RNA sequence, secondary structure and splice site position., (Published by Oxford University Press on behalf of Nucleic Acids Research 2019.)

Published

2019

16. APOL1 risk allele RNA contributes to renal toxicity by activating protein kinase R.

Author

Okamoto K, Rausch JW, Wakashin H, Fu Y, Chung JY, Dummer PD, Shin MK, Chandra P, Suzuki K, Shrivastav S, Rosenberg AZ, Hewitt SM, Ray PE, Noiri E, Le Grice SFJ, Hoek M, Han Z, Winkler CA, and Kopp JB

Abstract

APOL1 risk alleles associate with chronic kidney disease in African Americans, but the mechanisms remain to be fully understood. We show that APOL1 risk alleles activate protein kinase R (PKR) in cultured cells and transgenic mice. This effect is preserved when a premature stop codon is introduced to APOL1 risk alleles, suggesting that APOL1 RNA but not protein is required for the effect. Podocyte expression of APOL1 risk allele RNA, but not protein, in transgenic mice induces glomerular injury and proteinuria. Structural analysis of the APOL1 RNA shows that the risk variants possess secondary structure serving as a scaffold for tandem PKR binding and activation. These findings provide a mechanism by which APOL1 variants damage podocytes and suggest novel therapeutic strategies., Competing Interests: The authors declare no competing interests.

Published

2018

17. Structural characterization of maternally expressed gene 3 RNA reveals conserved motifs and potential sites of interaction with polycomb repressive complex 2.

Author

Sherpa C, Rausch JW, and Le Grice SF

Subjects

Chromatin chemistry, Chromatin genetics, DNA chemistry, DNA genetics, Gene Expression Regulation, Neoplastic genetics, Gene Regulatory Networks genetics, Genome, Human genetics, Humans, RNA, Long Noncoding chemistry, Epigenesis, Genetic, Neoplasms genetics, Nucleic Acid Conformation, RNA, Long Noncoding genetics

Abstract

Long non-coding RNAs (lncRNAs) have emerged as key players in gene regulation. However, our incomplete understanding of the structure of lncRNAs has hindered molecular characterization of their function. Maternally expressed gene 3 (Meg3) lncRNA is a tumor suppressor that is downregulated in various types of cancer. Mechanistic studies have reported a role for Meg3 in epigenetic regulation by interacting with chromatin-modifying complexes such as the polycomb repressive complex 2 (PRC2), guiding them to genomic sites via DNA-RNA triplex formation. Resolving the structure of Meg3 RNA and characterizing its interactions with cellular binding partners will deepen our understanding of tumorigenesis and provide a framework for RNA-based anti-cancer therapies. Herein, we characterize the architectural landscape of Meg3 RNA and its interactions with PRC2 from a functional standpoint.

Published

2018

18. Probing the Structures of Viral RNA Regulatory Elements with SHAPE and Related Methodologies.

Author

Rausch JW, Sztuba-Solinska J, and Le Grice SFJ

Abstract

Viral RNAs were selected by evolution to possess maximum functionality in a minimal sequence. Depending on the classification of the virus and the type of RNA in question, viral RNAs must alternately be replicated, spliced, transcribed, transported from the nucleus into the cytoplasm, translated and/or packaged into nascent virions, and in most cases, provide the sequence and structural determinants to facilitate these processes. One consequence of this compact multifunctionality is that viral RNA structures can be exquisitely complex, often involving intermolecular interactions with RNA or protein, intramolecular interactions between sequence segments separated by several thousands of nucleotides, or specialized motifs such as pseudoknots or kissing loops. The fluidity of viral RNA structure can also present a challenge when attempting to characterize it, as genomic RNAs especially are likely to sample numerous conformations at various stages of the virus life cycle. Here we review advances in chemoenzymatic structure probing that have made it possible to address such challenges with respect to cis -acting elements, full-length viral genomes and long non-coding RNAs that play a major role in regulating viral gene expression.

Published

2018

19. Kaposi's sarcoma-associated herpesvirus polyadenylated nuclear RNA: a structural scaffold for nuclear, cytoplasmic and viral proteins.

Author

Sztuba-Solinska J, Rausch JW, Smith R, Miller JT, Whitby D, and Le Grice SFJ

Subjects

Binding Sites, Cell Nucleus metabolism, Cell Nucleus virology, Cytoplasm metabolism, Cytoplasm virology, Herpesvirus 8, Human metabolism, Humans, Inverted Repeat Sequences, Nuclear Proteins metabolism, Nucleic Acid Conformation, Open Reading Frames, Polymorphism, Single Nucleotide, Protein Binding, RNA, Messenger genetics, RNA, Nuclear genetics, RNA, Viral genetics, Tumor Cells, Cultured, Viral Proteins genetics, Viral Proteins metabolism, Virus Replication, Herpesvirus 8, Human genetics, RNA, Messenger metabolism, RNA, Nuclear metabolism, RNA, Viral metabolism

Abstract

Kaposi's sarcoma-associated herpes virus (KSHV) polyadenylated nuclear (PAN) RNA facilitates lytic infection, modulating the cellular immune response by interacting with viral and cellular proteins and DNA. Although a number nucleoprotein interactions involving PAN have been implicated, our understanding of binding partners and PAN RNA binding motifs remains incomplete. Herein, we used SHAPE-mutational profiling (SHAPE-MaP) to probe PAN in its nuclear, cytoplasmic or viral environments or following cell/virion lysis and removal of proteins. We thus characterized and put into context discrete RNA structural elements, including the cis-acting Mta responsive element and expression and nuclear retention element (1,2). By comparing mutational profiles in different biological contexts, we identified sites on PAN either protected from chemical modification by protein binding or characterized by a loss of structure. While some protein binding sites were selectively localized, others were occupied in all three biological contexts. Individual binding sites of select KSHV gene products on PAN RNA were also identified in in vitro experiments. This work constitutes the most extensive structural characterization of a viral lncRNA and interactions with its protein partners in discrete biological contexts, providing a broad framework for understanding the roles of PAN RNA in KSHV infection., (Published by Oxford University Press on behalf of Nucleic Acids Research 2017.)

Published

2017

20. Reverse Transcription in the Saccharomyces cerevisiae Long-Terminal Repeat Retrotransposon Ty3.

Author

Rausch JW, Miller JT, and Le Grice SF

Subjects

RNA-Directed DNA Polymerase chemistry, RNA-Directed DNA Polymerase genetics, Saccharomyces cerevisiae Proteins chemistry, Saccharomyces cerevisiae Proteins genetics, RNA-Directed DNA Polymerase metabolism, Retroelements, Reverse Transcription, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins metabolism, Terminal Repeat Sequences

Abstract

Converting the single-stranded retroviral RNA into integration-competent double-stranded DNA is achieved through a multi-step process mediated by the virus-coded reverse transcriptase (RT). With the exception that it is restricted to an intracellular life cycle, replication of the Saccharomyces cerevisiae long terminal repeat (LTR)-retrotransposon Ty3 genome is guided by equivalent events that, while generally similar, show many unique and subtle differences relative to the retroviral counterparts. Until only recently, our knowledge of RT structure and function was guided by a vast body of literature on the human immunodeficiency virus (HIV) enzyme. Although the recently-solved structure of Ty3 RT in the presence of an RNA/DNA hybrid adds little in terms of novelty to the mechanistic basis underlying DNA polymerase and ribonuclease H activity, it highlights quite remarkable topological differences between retroviral and LTR-retrotransposon RTs. The theme of overall similarity but distinct differences extends to the priming mechanisms used by Ty3 RT to initiate (-) and (+) strand DNA synthesis. The unique structural organization of the retrotransposon enzyme and interaction with its nucleic acid substrates, with emphasis on polypurine tract (PPT)-primed initiation of (+) strand synthesis, is the subject of this review.

Published

2017

21. Novel Biochemical Tools for Probing HIV RNA Structure.

Author

Rausch JW, Sztuba-Solinska J, Lusvarghi S, and Le Grice SF

Subjects

Binding Sites, Electrophoresis, Capillary methods, HIV metabolism, HIV Infections virology, Humans, Models, Molecular, Native Polyacrylamide Gel Electrophoresis methods, Nucleic Acid Conformation, Peptides metabolism, RNA Folding, RNA Probes analysis, RNA Probes isolation & purification, RNA Probes metabolism, RNA, Viral analysis, RNA, Viral isolation & purification, RNA, Viral metabolism, Reverse Transcription, HIV chemistry, RNA Probes chemistry, RNA, Viral chemistry

Abstract

Functional analysis of viral RNA requires knowledge of secondary structure arrangements and tertiary base interactions. Thus, high-throughput and comprehensive methods for assessing RNA structure are highly desirable. Selective 2'-hydroxyl acylation analyzed by primer extension (SHAPE) has proven highly useful for modeling the secondary structures of HIV and other retroviral RNAs in recent years. This technology is not without its limitations however, as SHAPE data can be severely compromised when the RNA under study is structurally heterogeneous. In addition, the method reveals little information regarding the three-dimensional (3D) organization of an RNA. This chapter outlines four detailed SHAPE-related methodologies that circumvent these limitations. "Ensemble" and "in-gel" variations of SHAPE permit structural analysis of individual conformers within structurally heterogeneous mixtures of RNA, while probing strategies that utilize "through-space" cleavage reagents such as methidiumpropyl-EDTA (MPE) and peptides appended with an ATCUN (amino terminal copper/nickel binding motif) can provide insight into 3D organization. Combinational application of these techniques provides a formidable arsenal for exploring the structures of HIV RNAs and associated nucleoprotein complexes.

Published

2016

22. HIV Rev Assembly on the Rev Response Element (RRE): A Structural Perspective.

Author

Rausch JW and Le Grice SF

Subjects

Crystallography, X-Ray, HIV-1 chemistry, HIV-1 genetics, HIV-1 ultrastructure, Humans, Microscopy, Electron, Protein Binding, Protein Conformation, Scattering, Small Angle, rev Gene Products, Human Immunodeficiency Virus chemistry, rev Gene Products, Human Immunodeficiency Virus genetics, Genes, env, HIV-1 physiology, RNA, Viral metabolism, Virus Assembly, rev Gene Products, Human Immunodeficiency Virus metabolism

Abstract

HIV-1 Rev is an ~13 kD accessory protein expressed during the early stage of virus replication. After translation, Rev enters the nucleus and binds the Rev response element (RRE), a ~350 nucleotide, highly structured element embedded in the env gene in unspliced and singly spliced viral RNA transcripts. Rev-RNA assemblies subsequently recruit Crm1 and other cellular proteins to form larger complexes that are exported from the nucleus. Once in the cytoplasm, the complexes dissociate and unspliced and singly-spliced viral RNAs are packaged into nascent virions or translated into viral structural proteins and enzymes, respectively. Rev binding to the RRE is a complex process, as multiple copies of the protein assemble on the RNA in a coordinated fashion via a series of Rev-Rev and Rev-RNA interactions. Our understanding of the nature of these interactions has been greatly advanced by recent studies using X-ray crystallography, small angle X-ray scattering (SAXS) and single particle electron microscopy as well as biochemical and genetic methodologies. These advances are discussed in detail in this review, along with perspectives on development of antiviral therapies targeting the HIV-1 RRE.

Published

2015

23. The HIV-1 Rev response element (RRE) adopts alternative conformations that promote different rates of virus replication.

Author

Sherpa C, Rausch JW, Le Grice SF, Hammarskjold ML, and Rekosh D

Subjects

Fusion Proteins, gag-pol metabolism, Genes, env, HIV-1 physiology, Mutation, Nucleic Acid Conformation, RNA, Viral metabolism, HIV-1 genetics, RNA, Viral chemistry, Regulatory Sequences, Ribonucleic Acid, Virus Replication genetics, rev Gene Products, Human Immunodeficiency Virus metabolism

Abstract

The HIV Rev protein forms a complex with a 351 nucleotide sequence present in unspliced and incompletely spliced human immunodeficiency virus (HIV) mRNAs, the Rev response element (RRE), to recruit the cellular nuclear export receptor Crm1 and Ran-GTP. This complex facilitates nucleo-cytoplasmic export of these mRNAs. The precise secondary structure of the HIV-1 RRE has been controversial, since studies have reported alternative structures comprising either four or five stem-loops. The published structures differ only in regions that lie outside of the primary Rev binding site. Using in-gel SHAPE, we have now determined that the wt NL4-3 RRE exists as a mixture of both structures. To assess functional differences between these RRE 'conformers', we created conformationally locked mutants by site-directed mutagenesis. Using subgenomic reporters, as well as HIV replication assays, we demonstrate that the five stem-loop form of the RRE promotes greater functional Rev/RRE activity compared to the four stem-loop counterpart., (© The Author(s) 2015. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2015

24. SiRNA-induced mutation in HIV-1 polypurine tract region and its influence on viral fitness.

Author

Rausch JW, Tian M, Li Y, Angelova L, Bagaya BS, Krebs KC, Qian F, Zhu C, Arts EJ, Le Grice SF, and Gao Y

Subjects

3' Flanking Region, Base Sequence, Cell Line, DNA Primers genetics, DNA Primers metabolism, HIV-1 enzymology, HIV-1 genetics, Humans, Mutation, RNA Interference, RNA, Small Interfering genetics, RNA, Small Interfering metabolism, RNA, Viral antagonists & inhibitors, RNA, Viral genetics, RNA, Viral metabolism, Ribonuclease H metabolism, Sequence Alignment, Virus Replication, HIV-1 physiology

Abstract

Converting single-stranded viral RNA into double stranded DNA for integration is an essential step in HIV-1 replication. Initial polymerization of minus-strand DNA is primed from a host derived tRNA, whereas subsequent plus-strand synthesis requires viral primers derived from the 3' and central polypurine tracts (3' and cPPTs). The 5' and 3' termini of these conserved RNA sequence elements are precisely cleaved by RT-associated RNase H to generate specific primers that are used to initiate plus-strand DNA synthesis. In this study, siRNA wad used to produce a replicative HIV-1 variant contained G(-1)A and T(-16)A substitutions within/adjacent to the 3'PPT sequence. Introducing either or both mutations into the 3'PPT region or only the G(-1)A substitution in the cPPT region of NL4-3 produced infectious virus with decreased fitness relative to the wild-type virus. In contrast, introducing the T(-16)A or both mutations into the cPPT rendered the virus(es) incapable of replication, most likely due to the F185L integrase mutation produced by this nucleotide substitution. Finally, the effects of G(-1)A and T(-16)A mutations on cleavage of the 3'PPT were examined using an in vitro RNase H cleavage assay. Substrate containing both mutations was mis-cleaved to a greater extent than either wild-type substrate or substrate containing the T(-16)A mutation alone, which is consistent with the observed effects of the equivalent nucleotide substitutions on the replication fitness of NL4-3 virus. In conclusion, siRNA targeting of the HIV-1 3'PPT region can substantially suppress virus replication, and this selective pressure can be used to generate infectious virus containing mutations within or near the HIV-1 PPT. Moreover, in-depth analysis of the resistance mutations demonstrates that although virus containing a G(-1)A mutation within the 3'PPT is capable of replication, this nucleotide substitution shifts the 3'-terminal cleavage site in the 3'PPT by one nucleotide (nt) and significantly reduces viral fitness.

Published

2015

25. An unusual topological structure of the HIV-1 Rev response element.

Author

Fang X, Wang J, O'Carroll IP, Mitchell M, Zuo X, Wang Y, Yu P, Liu Y, Rausch JW, Dyba MA, Kjems J, Schwieters CD, Seifert S, Winans RE, Watts NR, Stahl SJ, Wingfield PT, Byrd RA, Le Grice SF, Rein A, and Wang YX

Subjects

Base Sequence, Binding Sites, Cell Nucleus metabolism, HEK293 Cells, HIV-1 genetics, Humans, Molecular Sequence Data, Nuclear Pore metabolism, Nucleic Acid Conformation, RNA Folding, RNA, Messenger genetics, RNA, Messenger metabolism, RNA, Viral genetics, RNA, Viral metabolism, Scattering, Small Angle, X-Ray Diffraction, rev Gene Products, Human Immunodeficiency Virus genetics, rev Gene Products, Human Immunodeficiency Virus metabolism, Active Transport, Cell Nucleus, HIV-1 chemistry, RNA, Messenger chemistry, RNA, Viral chemistry, rev Gene Products, Human Immunodeficiency Virus chemistry

Abstract

Nuclear export of unspliced and singly spliced viral mRNA is a critical step in the HIV life cycle. The structural basis by which the virus selects its own mRNA among more abundant host cellular RNAs for export has been a mystery for more than 25 years. Here, we describe an unusual topological structure that the virus uses to recognize its own mRNA. The viral Rev response element (RRE) adopts an "A"-like structure in which the two legs constitute two tracks of binding sites for the viral Rev protein and position the two primary known Rev-binding sites ~55 Å apart, matching the distance between the two RNA-binding motifs in the Rev dimer. Both the legs of the "A" and the separation between them are required for optimal RRE function. This structure accounts for the specificity of Rev for the RRE and thus the specific recognition of the viral RNA., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013

26. Exploiting drug-resistant enzymes as tools to identify thienopyrimidinone inhibitors of human immunodeficiency virus reverse transcriptase-associated ribonuclease H.

Author

Masaoka T, Chung S, Caboni P, Rausch JW, Wilson JA, Taskent-Sezgin H, Beutler JA, Tocco G, and Le Grice SF

Subjects

Antiviral Agents chemistry, Antiviral Agents pharmacology, Drug Resistance, Viral genetics, Enzyme Inhibitors chemistry, Enzyme Stability drug effects, HIV Reverse Transcriptase chemistry, HIV Reverse Transcriptase genetics, HIV-1 drug effects, HIV-1 enzymology, HIV-1 genetics, Humans, Models, Molecular, Molecular Structure, Mutation, Protein Binding, Protein Structure, Tertiary, Pyrimidinones chemistry, Reverse Transcriptase Inhibitors chemistry, Reverse Transcriptase Inhibitors pharmacology, Ribonuclease H, Human Immunodeficiency Virus chemistry, Ribonuclease H, Human Immunodeficiency Virus genetics, Temperature, Drug Resistance, Viral drug effects, Enzyme Inhibitors pharmacology, HIV Reverse Transcriptase antagonists & inhibitors, Pyrimidinones pharmacology, Ribonuclease H, Human Immunodeficiency Virus antagonists & inhibitors

Abstract

The thienopyrimidinone 5,6-dimethyl-2-(4-nitrophenyl)thieno[2,3-d]pyrimidin-4(3H)-one (DNTP) occupies the interface between the p66 ribonuclease H (RNase H) domain and p51 thumb of human immunodeficiency virus reverse transcriptase (HIV RT), thereby inducing a conformational change incompatible with catalysis. Here, we combined biochemical characterization of 39 DNTP derivatives with antiviral testing of selected compounds. In addition to wild-type HIV-1 RT, derivatives were evaluated with rationally designed, p66/p51 heterodimers exhibiting high-level DNTP sensitivity or resistance. This strategy identified 3',4'-dihydroxyphenyl (catechol) substituted thienopyrimidinones with submicromolar in vitro activity against both wild type HIV-1 RT and drug-resistant variants. Thermal shift analysis indicates that, in contrast to active site RNase H inhibitors, these thienopyrimidinones destabilize the enzyme, in some instances reducing the Tm by 5 °C. Importantly, catechol-containing thienopyrimidinones also inhibit HIV-1 replication in cells. Our data strengthen the case for allosteric inhibition of HIV RNase H activity, providing a platform for designing improved antagonists for use in combination antiviral therapy.

Published

2013

27. The HIV-2 Rev-response element: determining secondary structure and defining folding intermediates.

Author

Lusvarghi S, Sztuba-Solinska J, Purzycka KJ, Pauly GT, Rausch JW, and Grice SF

Subjects

5' Untranslated Regions, Base Sequence, Edetic Acid analogs & derivatives, Edetic Acid chemistry, Models, Molecular, Molecular Sequence Data, Nucleic Acid Conformation, RNA Folding, HIV-2 genetics, RNA, Viral chemistry, rev Gene Products, Human Immunodeficiency Virus metabolism

Abstract

Interaction between the viral protein Rev and the RNA motifs known as Rev response elements (RREs) is required for transport of unspliced and partially spliced human immunodeficiency virus (HIV)-1 and HIV-2 RNAs from the nucleus to the cytoplasm during the later stages of virus replication. A more detailed understanding of these nucleoprotein complexes and the host factors with which they interact should accelerate the development of new antiviral drugs targeting cis-acting RNA regulatory signals. In this communication, the secondary structures of the HIV-2 RRE and two RNA folding precursors have been identified using the SHAPE (selective 2'-hydroxyl acylation analyzed by primer extension) chemical probing methodology together with a novel mathematical approach for determining the secondary structures of RNA conformers present in a mixture. A complementary chemical probing technique was also used to support these secondary structure models, to confirm that the RRE2 RNA undergoes a folding transition and to obtain information about the relative positioning of RRE2 substructures in three dimensions. Our analysis collectively suggests that the HIV-2 RRE undergoes two conformational transitions before assuming the energetically most favorable conformer. The 3D models for the HIV-2 RRE and folding intermediates are also presented, wherein the Rev-binding stem-loops (IIB and I) are located coaxially in the former, which is in agreement with previous models for HIV-1 Rev-RRE binding.

Published

2013

28. RNA secondary structure prediction using high-throughput SHAPE.

Author

Lusvarghi S, Sztuba-Solinska J, Purzycka KJ, Rausch JW, and Le Grice SF

Subjects

Acylation, Electrophoresis, Capillary methods, Fluorescent Dyes chemistry, High-Throughput Screening Assays methods, Nucleic Acid Conformation, Nucleic Acid Probes chemistry, RNA chemistry

Abstract

Understanding the function of RNA involved in biological processes requires a thorough knowledge of RNA structure. Toward this end, the methodology dubbed "high-throughput selective 2' hydroxyl acylation analyzed by primer extension", or SHAPE, allows prediction of RNA secondary structure with single nucleotide resolution. This approach utilizes chemical probing agents that preferentially acylate single stranded or flexible regions of RNA in aqueous solution. Sites of chemical modification are detected by reverse transcription of the modified RNA, and the products of this reaction are fractionated by automated capillary electrophoresis (CE). Since reverse transcriptase pauses at those RNA nucleotides modified by the SHAPE reagents, the resulting cDNA library indirectly maps those ribonucleotides that are single stranded in the context of the folded RNA. Using ShapeFinder software, the electropherograms produced by automated CE are processed and converted into nucleotide reactivity tables that are themselves converted into pseudo-energy constraints used in the RNAStructure (v5.3) prediction algorithm. The two-dimensional RNA structures obtained by combining SHAPE probing with in silico RNA secondary structure prediction have been found to be far more accurate than structures obtained using either method alone.

Published

2013

29. Structural complexity of Dengue virus untranslated regions: cis-acting RNA motifs and pseudoknot interactions modulating functionality of the viral genome.

Author

Sztuba-Solinska J, Teramoto T, Rausch JW, Shapiro BA, Padmanabhan R, and Le Grice SF

Subjects

Models, Molecular, Mutation, Nucleic Acid Conformation, Nucleotide Motifs, Oligonucleotides, Antisense chemistry, Dengue Virus genetics, Genome, Viral, RNA, Viral chemistry, Untranslated Regions

Abstract

The Dengue virus (DENV) genome contains multiple cis-acting elements required for translation and replication. Previous studies indicated that a 719-nt subgenomic minigenome (DENV-MINI) is an efficient template for translation and (-) strand RNA synthesis in vitro. We performed a detailed structural analysis of DENV-MINI RNA, combining chemical acylation techniques, Pb(2+) ion-induced hydrolysis and site-directed mutagenesis. Our results highlight protein-independent 5'-3' terminal interactions involving hybridization between recognized cis-acting motifs. Probing analyses identified tandem dumbbell structures (DBs) within the 3' terminus spaced by single-stranded regions, internal loops and hairpins with embedded GNRA-like motifs. Analysis of conserved motifs and top loops (TLs) of these dumbbells, and their proposed interactions with downstream pseudoknot (PK) regions, predicted an H-type pseudoknot involving TL1 of the 5' DB and the complementary region, PK2. As disrupting the TL1/PK2 interaction, via 'flipping' mutations of PK2, previously attenuated DENV replication, this pseudoknot may participate in regulation of RNA synthesis. Computer modeling implied that this motif might function as autonomous structural/regulatory element. In addition, our studies targeting elements of the 3' DB and its complementary region PK1 indicated that communication between 5'-3' terminal regions strongly depends on structure and sequence composition of the 5' cyclization region.

Published

2013

30. Structural analysis of monomeric retroviral reverse transcriptase in complex with an RNA/DNA hybrid.

Author

Nowak E, Potrzebowski W, Konarev PV, Rausch JW, Bona MK, Svergun DI, Bujnicki JM, Le Grice SF, and Nowotny M

Subjects

Amino Acid Sequence, DNA metabolism, HIV Reverse Transcriptase genetics, HIV Reverse Transcriptase metabolism, Models, Molecular, Molecular Sequence Data, Mutagenesis, Site-Directed, Protein Binding, RNA metabolism, Xenotropic murine leukemia virus-related virus enzymology, DNA chemistry, HIV Reverse Transcriptase chemistry, RNA chemistry

Abstract

A key step in proliferation of retroviruses is the conversion of their RNA genome to double-stranded DNA, a process catalysed by multifunctional reverse transcriptases (RTs). Dimeric and monomeric RTs have been described, the latter exemplified by the enzyme of Moloney murine leukaemia virus. However, structural information is lacking that describes the substrate binding mechanism for a monomeric RT. We report here the first crystal structure of a complex between an RNA/DNA hybrid substrate and polymerase-connection fragment of the single-subunit RT from xenotropic murine leukaemia virus-related virus, a close relative of Moloney murine leukaemia virus. A comparison with p66/p51 human immunodeficiency virus-1 RT shows that substrate binding around the polymerase active site is conserved but differs in the thumb and connection subdomains. Small-angle X-ray scattering was used to model full-length xenotropic murine leukaemia virus-related virus RT, demonstrating that its mobile RNase H domain becomes ordered in the presence of a substrate-a key difference between monomeric and dimeric RTs.

Published

2013

31. Synthesis, activity, and structural analysis of novel α-hydroxytropolone inhibitors of human immunodeficiency virus reverse transcriptase-associated ribonuclease H.

Author

Chung S, Himmel DM, Jiang JK, Wojtak K, Bauman JD, Rausch JW, Wilson JA, Beutler JA, Thomas CJ, Arnold E, and Le Grice SF

Subjects

Anti-HIV Agents pharmacology, Benzocycloheptenes chemistry, Catalytic Domain, Cations, Divalent, Cell Line, Coordination Complexes chemistry, Crystallography, X-Ray, DNA-Directed DNA Polymerase chemistry, HIV Reverse Transcriptase chemistry, HIV-1 physiology, Humans, Manganese chemistry, Models, Molecular, Molecular Structure, Mutation, Nitriles chemistry, Protein Conformation, Pyrimidines chemistry, Ribonuclease H, Human Immunodeficiency Virus chemistry, Ribonuclease H, Human Immunodeficiency Virus genetics, Rilpivirine, Structure-Activity Relationship, Tropolone pharmacology, Virus Replication, Anti-HIV Agents chemical synthesis, HIV Reverse Transcriptase antagonists & inhibitors, HIV-1 drug effects, Ribonuclease H, Human Immunodeficiency Virus antagonists & inhibitors, Tropolone analogs & derivatives, Tropolone chemical synthesis

Abstract

The α-hydroxytroplone, manicol (5,7-dihydroxy-2-isopropenyl-9-methyl-1,2,3,4-tetrahydro-benzocyclohepten-6-one), potently and specifically inhibits ribonuclease H (RNase H) activity of human immunodeficiency virus reverse transcriptase (HIV RT) in vitro. However, manicol was ineffective in reducing virus replication in culture. Ongoing efforts to improve the potency and specificity over the lead compound led us to synthesize 14 manicol derivatives that retain the divalent metal-chelating α-hydroxytropolone pharmacophore. These efforts were augmented by a high resolution structure of p66/p51 HIV-1 RT containing the nonnucleoside reverse transcriptase inhibitor (NNRTI), TMC278 and manicol in the DNA polymerase and RNase H active sites, respectively. We demonstrate here that several modified α-hydroxytropolones exhibit antiviral activity at noncytotoxic concentrations. Inclusion of RNase H active site mutants indicated that manicol analogues can occupy an additional site in or around the DNA polymerase catalytic center. Collectively, our studies will promote future structure-based design of improved α-hydroxytropolones to complement the NRTI and NNRTI currently in clinical use.

Published

2011

32. Structure-activity analysis of vinylogous urea inhibitors of human immunodeficiency virus-encoded ribonuclease H.

Author

Chung S, Wendeler M, Rausch JW, Beilhartz G, Gotte M, O'Keefe BR, Bermingham A, Beutler JA, Liu S, Zhuang X, and Le Grice SF

Subjects

Catalytic Domain, Humans, Models, Molecular, Molecular Structure, Temperature, Thermodynamics, Anti-HIV Agents chemistry, Anti-HIV Agents pharmacology, Enzyme Inhibitors chemistry, Enzyme Inhibitors pharmacology, Ribonuclease H, Human Immunodeficiency Virus antagonists & inhibitors, Ribonuclease H, Human Immunodeficiency Virus chemistry

Abstract

Vinylogous ureas 2-amino-5,6,7,8-tetrahydro-4H-cyclohepta[b]thiophene-3-carboxamide and N-[3-(aminocarbonyl)-4,5-dimethyl-2-thienyl]-2-furancarboxamide (compounds 1 and 2, respectively) were recently identified to be modestly potent inhibitors of the RNase H activity of HIV-1 and HIV-2 reverse transcriptase (RT). Both compounds shared a 3-CONH(2)-substituted thiophene ring but were otherwise structurally unrelated, which prevented a precise definition of the pharmacophore. We have therefore examined a larger series of vinylogous ureas carrying amide, amine, and cycloalkane modifications of the thiophene ring of compound 1. While cycloheptane- and cyclohexane-substituted derivatives retained potency, cyclopentane and cyclooctane substitutions eliminated activity. In the presence of a cycloheptane ring, modifying the 2-NH(2) or 3-CONH(2) functions decreased the potency. With respect to compound 2, vinylogous ureas whose dimethylthiophene ring contained modifications of the 2-NH(2) and 3-CONH(2) functions were investigated. 2-NH(2)-modified analogs displayed potency equivalent to or enhanced over that of compound 2, the most active of which, compound 16, reflected intramolecular cyclization of the 2-NH(2) and 3-CONH(2) groups. Molecular modeling was used to define an inhibitor binding site in the p51 thumb subdomain, suggesting that an interaction with the catalytically conserved His539 of the p66 RNase H domain could underlie inhibition of RNase H activity. Collectively, our data indicate that multiple functional groups of vinylogous ureas contribute to their potencies as RNase H inhibitors. Finally, single-molecule spectroscopy indicates that vinylogous ureas have the property of altering the reverse transcriptase orientation on a model RNA-DNA hybrid mimicking initiation plus-strand DNA synthesis.

Published

2010

33. Reverse transcriptase in motion: conformational dynamics of enzyme-substrate interactions.

Author

Götte M, Rausch JW, Marchand B, Sarafianos S, and Le Grice SF

Subjects

DNA, Viral metabolism, Humans, Molecular Conformation, HIV Reverse Transcriptase chemistry

Abstract

Human immunodeficiency virus type 1 reverse transcriptase (HIV-1 RT) catalyzes synthesis of integration-competent, double-stranded DNA from the single-stranded viral RNA genome, combining both polymerizing and hydrolytic functions to synthesize approximately 20,000 phosphodiester bonds. Despite a wealth of biochemical studies, the manner whereby the enzyme adopts different orientations to coordinate its DNA polymerase and ribonuclease (RNase) H activities has remained elusive. Likewise, the lower processivity of HIV-1 RT raises the issue of polymerization site targeting, should the enzyme re-engage its nucleic acid substrate several hundred nucleotides from the primer terminus. Although X-ray crystallography has clearly contributed to our understanding of RT-containing nucleoprotein complexes, it provides a static picture, revealing few details regarding motion of the enzyme on the substrate. Recent development of site-specific footprinting and the application of single molecule spectroscopy have allowed us to follow individual steps in the reverse transcription process with significantly greater precision. Progress in these areas and the implications for investigational and established inhibitors that interfere with RT motion on nucleic acid is reviewed here., (Published by Elsevier B.V.)

Published

2010

34. HIV-1 transmission by dendritic cell-specific ICAM-3-grabbing nonintegrin (DC-SIGN) is regulated by determinants in the carbohydrate recognition domain that are absent in liver/lymph node-SIGN (L-SIGN).

Author

Chung NP, Breun SK, Bashirova A, Baumann JG, Martin TD, Karamchandani JM, Rausch JW, Le Grice SF, Wu L, Carrington M, and Kewalramani VN

Subjects

Alleles, Animals, B-Lymphocytes metabolism, Cell Adhesion Molecules genetics, Cell Line, Gene Expression Regulation, Humans, Lectins metabolism, Lectins, C-Type genetics, Mice, Models, Molecular, Protein Structure, Tertiary, Receptors, Cell Surface genetics, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Carbohydrate Metabolism, Cell Adhesion Molecules chemistry, Cell Adhesion Molecules metabolism, HIV Infections metabolism, HIV Infections transmission, HIV-1, Lectins, C-Type chemistry, Lectins, C-Type metabolism, Receptors, Cell Surface chemistry, Receptors, Cell Surface metabolism

Abstract

In this study, we identify determinants in dendritic cell-specific ICAM-3-grabbing nonintegrin (DC-SIGN) necessary for human immunodeficiency virus, type 1 (HIV-1), transmission. Although human B cell lines expressing DC-SIGN efficiently capture and transmit HIV-1 to susceptible target cells, cells expressing the related molecule liver/lymph node-specific ICAM-3-grabbing nonintegrin (L-SIGN) do not. To understand the differences between DC-SIGN and L-SIGN that affect HIV-1 interactions, we developed Raji B cell lines expressing different DC-SIGN/L-SIGN chimeras. Testing of the chimeras demonstrated that replacement of the DC-SIGN carbohydrate-recognition domain (CRD) with that of L-SIGN was sufficient to impair virus binding and prevent transmission. Conversely, the ability to bind and transmit HIV-1 was conferred to L-SIGN chimeras containing the DC-SIGN CRD. We identified Trp-258 in the DC-SIGN CRD to be essential for HIV-1 transmission. Although introduction of a K270W mutation at the same position in L-SIGN was insufficient for HIV-1 binding, an L-SIGN mutant molecule with K270W and a C-terminal DC-SIGN CRD subdomain transmitted HIV-1. These data suggest that DC-SIGN structural elements distinct from the oligosaccharide-binding site are required for HIV-1 glycoprotein selectivity.

Published

2010

35. Dissecting APOBEC3G substrate specificity by nucleoside analog interference.

Author

Rausch JW, Chelico L, Goodman MF, and Le Grice SF

Subjects

APOBEC-3G Deaminase, Amino Acid Motifs physiology, Animals, Apolipoproteins B biosynthesis, Apolipoproteins B genetics, Cell Line, Cytidine Deaminase antagonists & inhibitors, Cytidine Deaminase genetics, Cytidine Deaminase metabolism, DNA, Single-Stranded genetics, DNA, Single-Stranded metabolism, HIV Infections genetics, HIV-1, Humans, RNA Editing physiology, RNA, Messenger chemistry, RNA, Messenger genetics, RNA, Messenger metabolism, Spodoptera, Substrate Specificity physiology, Zinc chemistry, Zinc metabolism, vif Gene Products, Human Immunodeficiency Virus chemistry, vif Gene Products, Human Immunodeficiency Virus genetics, vif Gene Products, Human Immunodeficiency Virus metabolism, Cytidine Deaminase chemistry, DNA, Single-Stranded chemistry, HIV Infections enzymology, Nucleosides chemistry

Abstract

The apolipoprotein B mRNA-editing enzyme, catalytic polypeptide-like (APOBEC) cytidine deaminase genes encode a set of enzymes including APOBEC1 (A1), APOBEC2 (A2), APOBEC4 (A4), and APOBEC3A-H (A3A-H). Although each possesses one or more zinc binding motifs conserved among enzymes catalyzing C-->U conversion, the functions and substrate specificities of these gene products vary considerably. For example, although two closely related enzymes, A3F and A3G, both restrict HIV-1 infection in strains deficient in virus infectivity factor (vif), A3F selectively deaminates cytosine within 5'-TTCA-3' motifs in single stranded DNA, whereas A3G targets 5'-CCCA-3' sequences. In the present study we have used nucleoside analog interference mapping to probe A3G-DNA interactions throughout the enzyme-substrate complex as well as to determine which DNA structural features determine substrate specificity. Our results indicate that multiple components of nucleosides within the consensus sequence are important for substrate recognition by A3G (with base moieties being most critical), whereas deamination interference by analog substitution outside this region is minimal. Furthermore, exocyclic groups in pyrimidines 1-2 nucleotides 5' of the target cytosine were shown to dictate substrate recognition by A3G, with chemical composition at ring positions 3 and 4 found to be more important than at ring position 5. Taken together, these results provide insights into how the enzyme selects A3G hotspot motifs for deamination as well as which approaches might be best suited for forming a stable, catalytically competent cross-linked A3G-DNA complex for future structural studies.

Published

2009

36. Slide into action: dynamic shuttling of HIV reverse transcriptase on nucleic acid substrates.

Author

Liu S, Abbondanzieri EA, Rausch JW, Le Grice SF, and Zhuang X

Subjects

Binding Sites, Carbocyanines, DNA Primers metabolism, DNA, Viral biosynthesis, Fluorescence Resonance Energy Transfer, Fluorescent Dyes, HIV Reverse Transcriptase chemistry, Kinetics, Models, Molecular, Nevirapine metabolism, Nevirapine pharmacology, Nucleic Acid Hybridization, Nucleotides metabolism, Protein Binding, Protein Conformation, Protein Structure, Tertiary, Reverse Transcriptase Inhibitors metabolism, Reverse Transcriptase Inhibitors pharmacology, Reverse Transcription, Ribonuclease H chemistry, Ribonuclease H metabolism, DNA, Viral metabolism, HIV Reverse Transcriptase metabolism, HIV-1 enzymology, RNA, Viral metabolism

Abstract

The reverse transcriptase (RT) of human immunodeficiency virus (HIV) catalyzes a series of reactions to convert single-stranded viral RNA into double-stranded DNA for host cell integration. This process requires a variety of enzymatic activities, including DNA polymerization, RNA cleavage, strand transfer, and strand displacement synthesis. We used single-molecule fluorescence resonance energy transfer to probe the interactions between RT and nucleic acid substrates in real time. RT was observed to slide on nucleic acid duplexes, rapidly shuttling between opposite termini of the duplex. Upon reaching the DNA 3' terminus, RT can spontaneously flip into a polymerization orientation. Sliding kinetics were regulated by cognate nucleotides and anti-HIV drugs, which stabilized and destabilized the polymerization mode, respectively. These long-range translocation activities facilitate multiple stages of the reverse transcription pathway, including normal DNA polymerization and strand displacement synthesis.

Published

2008

37. Dynamic binding orientations direct activity of HIV reverse transcriptase.

Author

Abbondanzieri EA, Bokinsky G, Rausch JW, Zhang JX, Le Grice SF, and Zhuang X

Subjects

Binding Sites, Catalysis, DNA Primers genetics, DNA Primers metabolism, Fluorescence Resonance Energy Transfer, HIV genetics, Hydrolysis, Ligands, RNA genetics, Substrate Specificity, Templates, Genetic, DNA biosynthesis, DNA Replication, HIV enzymology, HIV Reverse Transcriptase chemistry, HIV Reverse Transcriptase metabolism, RNA metabolism, Reverse Transcription

Abstract

The reverse transcriptase of human immunodeficiency virus (HIV) catalyses a series of reactions to convert the single-stranded RNA genome of HIV into double-stranded DNA for host-cell integration. This task requires the reverse transcriptase to discriminate a variety of nucleic-acid substrates such that active sites of the enzyme are correctly positioned to support one of three catalytic functions: RNA-directed DNA synthesis, DNA-directed DNA synthesis and DNA-directed RNA hydrolysis. However, the mechanism by which substrates regulate reverse transcriptase activities remains unclear. Here we report distinct orientational dynamics of reverse transcriptase observed on different substrates with a single-molecule assay. The enzyme adopted opposite binding orientations on duplexes containing DNA or RNA primers, directing its DNA synthesis or RNA hydrolysis activity, respectively. On duplexes containing the unique polypurine RNA primers for plus-strand DNA synthesis, the enzyme can rapidly switch between the two orientations. The switching kinetics were regulated by cognate nucleotides and non-nucleoside reverse transcriptase inhibitors, a major class of anti-HIV drugs. These results indicate that the activities of reverse transcriptase are determined by its binding orientation on substrates.

Published

2008

38. Structural probing of the HIV-1 polypurine tract RNA:DNA hybrid using classic nucleic acid ligands.

Author

Turner KB, Brinson RG, Yi-Brunozzi HY, Rausch JW, Miller JT, Le Grice SF, Marino JP, and Fabris D

Subjects

Aminoglycosides chemistry, Binding Sites, Framycetin chemistry, Ligands, Mass Spectrometry, Nuclear Magnetic Resonance, Biomolecular, Nucleic Acid Probes, Purines chemistry, Thermodynamics, DNA, Viral chemistry, HIV-1 genetics, RNA, Viral chemistry

Abstract

The interactions of archetypical nucleic acid ligands with the HIV-1 polypurine tract (PPT) RNA:DNA hybrid, as well as analogous DNA:DNA, RNA:RNA and swapped hybrid substrates, were used to probe structural features of the PPT that contribute to its specific recognition and processing by reverse transcriptase (RT). Results from intercalative and groove-binding ligands indicate that the wild-type PPT hybrid does not contain any strikingly unique groove geometries and/or stacking arrangements that might contribute to the specificity of its interaction with RT. In contrast, neomycin bound preferentially and selectively to the PPT near the 5'(rA)(4):(dT)(4) tract and the 3' PPT-U3 junction. Nuclear magnetic resonance data from a complex between HIV-1 RT and the PPT indicate RT contacts within the same regions highlighted on the PPT by neomycin. These observations, together with the fact that the sites are correctly spaced to allow interaction with residues in the ribonuclease H (RNase H) active site and thumb subdomain of the p66 RT subunit, suggest that despite the long cleft employed by RT to make contact with nucleic acids substrates, these sites provide discrete binding units working in concert to determine not only specific PPT recognition, but also its orientation on the hybrid structure.

Published

2008

39. Purine analog substitution of the HIV-1 polypurine tract primer defines regions controlling initiation of plus-strand DNA synthesis.

Author

Rausch JW and Le Grice SF

Subjects

Adenine chemistry, Base Sequence, Guanine chemistry, Models, Genetic, Mutation, RNA metabolism, RNA, Viral metabolism, Ribonuclease H metabolism, Uracil chemistry, DNA Replication, DNA, Viral biosynthesis, HIV-1 genetics, Purine Nucleosides chemistry, RNA chemistry, RNA, Viral chemistry, Regulatory Sequences, Ribonucleic Acid

Abstract

Despite extensive study, the mechanism by which retroviral reverse transciptases (RTs) specifically utilize polypurine tract (PPT) RNA for initiation of plus-strand DNA synthesis remains unclear. Three sequence motifs within or adjacent to the purine-rich elements are highly conserved, namely, a rU:dA tract region immediately 5' to the PPT, an rA:dT-rich sequence constituting the upstream portion of the PPT and a downstream rG:dC tract. Using an in vitro HIV-1 model system, we determined that the former two elements define the 5' terminus of the (+)-strand primer, whereas the rG:dC tract serves as the primary determinant of initiation specificity. Subsequent analysis demonstrated that G-->A or A-->G substitution at PPT positions -2, -4 and +1 (relative to the scissile phosphate) substantially reduces (+)-strand priming. We explored this observation further using PPT substrates substituted with a variety of nucleoside analogs [inosine (I), purine riboside (PR), 2-aminopurine (2-AP), 2,6-diaminopurine (2,6-DAP), isoguanine (iG)], or one of the naturally occurring bases at these positions. Our results demonstrate that for PPT positions -2 or +1, substituting position 2 of the purine was an important determinant of cleavage specificity. In addition, cleavage specificity was greatly affected by substituting -4G with an analog containing a 6-NH2 moiety.

Published

2007

40. Exploiting structurally diverse nucleoside analogs as probes of reverse transcription complexes.

Author

Rausch JW and Le Grice SF

Subjects

DNA, Viral biosynthesis, DNA, Viral chemistry, HIV-1 genetics, Hydrogen Bonding, RNA, Viral chemistry, HIV Reverse Transcriptase chemistry, Nucleosides chemistry, Reverse Transcription

Abstract

Crystal structures of HIV-1 reverse transcriptase (RT) in complex with either duplex DNA or an RNA/DNA hybrid have provided significant insights into the manner in which this highly versatile enzyme accommodates the conformationally-distinct nucleic acid substrates encountered during the reverse transcription cycle. Biochemical data likewise suggest that unique structural features of the nucleic acid substrates contribute towards recognition by their cognate RT. While site-directed mutagenesis of catalytically- and structurally-critical protein motifs is relatively facile, understanding how nucleic acid structure contributes to its recognition presents a greater challenge. The relative ease with which large DNA and RNA fragments can now be chemically synthesized, in conjunction with the increased availability of ribo- and deoxyribonucleoside analogs, allows nucleic acid structure to be examined with respect to the role of hydrogen bonding, nucleobase stacking, sugar ring geometry and charge of the phosphodiester backbone. This review summarizes our use of nucleoside analogs to understand how the structure of cis-acting regulatory signals mediates their recognition by structurally diverse retroviral and retrotransposon enzymes.

Published

2007

41. 'Binding, bending and bonding': polypurine tract-primed initiation of plus-strand DNA synthesis in human immunodeficiency virus.

Author

Rausch JW and Le Grice SF

Subjects

DNA, Viral chemistry, DNA, Viral metabolism, HIV Reverse Transcriptase genetics, HIV Reverse Transcriptase metabolism, Purines chemistry, Ribonuclease H metabolism, Sequence Homology, Nucleic Acid, DNA, Viral biosynthesis, HIV-1 genetics, HIV-1 metabolism, Purines metabolism

Abstract

During the course of reverse transcription, human immunodeficiency virus type 1 reverse transcriptase (HIV-1 RT) initiates plus-strand DNA synthesis from two highly conserved, purine-rich RNA segments of the viral genome referred to as the 3' and central polypurine tracts (3' and cPPTs). Processing of these elements occurs in several sequential steps including (1) minus-strand DNA synthesis over the PPT(s), (2) ribonuclease H (RNase H) mediated cleavage at the PPT 3' terminus, (3) plus-strand DNA synthesis from the nascent RNA primer(s), and (4) primer removal. Completing each of these steps precisely and specifically is essential, as failure to do so can result in reduced virus replication and/or impaired integration of viral DNA into the host cell genome. In this review, plus-strand primer processing in HIV-1 is discussed from biochemical, structural, and historical perspectives. A comparative analysis of PPT-processing in different LTR-containing retroelements is also presented., (Copyright 2004 Elsevier B.V.)

Published

2004

42. Using pyrrolo-deoxycytosine to probe RNA/DNA hybrids containing the human immunodeficiency virus type-1 3' polypurine tract.

Author

Dash C, Rausch JW, and Le Grice SF

Subjects

Adenine chemistry, Base Pairing, Base Sequence, Cytosine analogs & derivatives, DNA, Viral biosynthesis, Fluorescent Dyes chemistry, Guanine chemistry, HIV Reverse Transcriptase metabolism, HIV-1 enzymology, Hydrogen Bonding, Mutation, Nucleic Acid Heteroduplexes chemistry, Nucleic Acid Heteroduplexes metabolism, Ribonuclease H genetics, Ribonuclease H metabolism, Templates, Genetic, Cytosine chemistry, DNA, Viral chemistry, HIV-1 genetics, Nucleic Acid Probes chemistry, Purines chemistry, RNA, Viral chemistry

Abstract

Recent structural analyses indicate that localized regions of abnormal base pairing exist within RNA/DNA hybrids containing the HIV-1 polypurine tract (PPT) and that these distortions may play a role in PPT function. To examine this directly, we have introduced pyrrolo-deoxycytosine (pdC), a fluorescent, environmentally sensitive analog of deoxycytosine (dC), into the DNA strand of PPT-containing hybrids. Steady-state fluorescence analysis of these hybrids reveals that the DNA base 11 nt from the PPT-U3 junction is unpaired even in the absence of reverse transcriptase (RT). Unstable base pairing is also observed within the (rG:dC)6 tract in the downstream portion of the duplex, suggesting that HIV-1 RT may recognize multiple pre-existing distortions during PPT selection. HIV-1 RT hydrolyzes pdC-containing hybrids primarily at the PPT-U3 junction, indicating that the analog does not induce a gross structural deformation of the duplex. However, aberrant cleavage is frequently observed 3 bp from the site of pdC substitution, most likely reflecting a specific interaction between the analog and amino acid residues within the RNase H primer grip. pdC substitution within the template strand of a DNA duplex does not appear to significantly affect RT-catalyzed DNA synthesis. Implications of these findings on the use of pdC to examine nucleic acid structure are discussed.

Published

2004

43. Hydrolysis of RNA/DNA hybrids containing nonpolar pyrimidine isosteres defines regions essential for HIV type 1 polypurine tract selection.

Author

Rausch JW, Qu J, Yi-Brunozzi HY, Kool ET, and Le Grice SF

Subjects

Base Sequence, DNA Primers, HIV Reverse Transcriptase metabolism, HIV-1 enzymology, Hydrolysis, Nucleic Acid Hybridization, DNA metabolism, HIV-1 metabolism, Purines metabolism, Pyrimidines metabolism, RNA metabolism

Abstract

Both x-ray crystallography and chemical footprinting indicate that bases of the HIV type 1 (HIV-1) polypurine tract (PPT)-containing RNA/DNA hybrid deviate from standard Watson-Crick base pairing. However, the contribution of these structural anomalies to the accuracy of plus-strand primer selection by HIV-1 reverse transcriptase is not immediately clear. To address this issue, DNA templates harboring single and pairwise non-hydrogen-bonding isosteres of cytosine (2-fluoro-4-methylbenzene deoxyribonucleoside) and thymine (2,4-difluoro-5-methylbenzene deoxyribonucleoside) were synthesized and hybridized to PPT-containing RNA primers as a means of locally removing hydrogen bonding and destabilizing paired structure. Cleavage of these hybrids was examined with p66/p51 HIV-1 reverse transcriptase and a mutant carrying an alteration in the p66 RNase H primer shown to specifically impair PPT processing. Analog insertion within the PPT (rG):(dC) and central (rA):(dT) tracts repositioned the RNase H domain such that the RNA/DNA hybrid was cleaved 3-4 bp from the site of insertion, a distance corresponding closely to the spatial separation between the catalytic center and RNase H primer grip. However, PPT processing was significantly impaired when the junction between these tracts was substituted. Substitutions within the upstream (rA):(dT) tract, where maximum distortion had previously been observed, destroyed PPT processing. Collectively, our scanning mutagenesis approach implicates multiple regions of the PPT in the accuracy with which it is excised from (+) U3 RNA and DNA, and also provides evidence for close cooperation between the RNase H primer grip and catalytic center in achieving this cleavage.

Published

2003

44. Mutations in the ribonuclease H active site of HIV-RT reveal a role for this site in stabilizing enzyme-primer-template binding.

Author

Cristofaro JV, Rausch JW, Le Grice SF, and DeStefano JJ

Subjects

Binding Sites genetics, Cations, Divalent chemistry, DNA Primers chemical synthesis, Enzyme Stability genetics, Histidine genetics, Hydrolysis, Magnesium Chloride chemistry, Osmolar Concentration, Protein Binding genetics, RNA chemical synthesis, RNA Processing, Post-Transcriptional genetics, RNA, Viral chemical synthesis, Recombinant Fusion Proteins chemistry, Substrate Specificity genetics, Templates, Genetic, DNA Primers chemistry, HIV Reverse Transcriptase chemistry, HIV Reverse Transcriptase genetics, Mutagenesis, Site-Directed, RNA chemistry, RNA, Viral chemistry, Ribonuclease H chemistry, Ribonuclease H genetics

Abstract

The RNase H activity of HIV-RT is coordinated by a catalytic triad (E478, D443, D498) of acidic residues that bind divalent cations. We examined the effect of RNase H deficient E(478)-->Q and D(549)-->N mutations that do not alter polymerase activity on binding of enzyme to various nucleic acid substrates. Binding of the mutant and wild-type enzymes to various nucleic acid substrates was examined by determining dissociation rate constants (k(off)) by titrating both Mg(2+) and salt concentrations. In agreement with the unaltered polymerase activity of the mutant, the k(off) values for the wild-type and mutant enzymes were essentially identical using DNA-DNA templates in the presence of 6 mM Mg(2+). However, with lower concentrations of Mg(2+) and in the absence of Mg(2+), although both enzymes dissociated more rapidly, the mutant enzymes dissociated several-fold more slowly than the wild type. This was also observed on RNA-DNA templates. These results indicate that alterations in residues essential for Mg(2+) binding have a pronounced positive effect on enzyme-template stability and that the negative residues in the RNase H region of the enzyme have a negative influence on binding in the absence of Mg(2+). In this regard RT is similar to other nucleic acid cleaving enzymes that show enhanced binding upon mutation of active site residues.

Published

2002

45. Altering the RNase H primer grip of human immunodeficiency virus reverse transcriptase modifies cleavage specificity.

Author

Rausch JW, Lener D, Miller JT, Julias JG, Hughes SH, and Le Grice SF

Subjects

Amino Acid Sequence, Catalytic Domain, DNA Primers chemistry, DNA Primers metabolism, DNA Replication, Deoxyribonuclease I, HIV-1 genetics, Humans, Kinetics, Polymerase Chain Reaction, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Transcription, Genetic, HIV Reverse Transcriptase chemistry, HIV Reverse Transcriptase metabolism, HIV-1 enzymology, Ribonuclease H chemistry

Abstract

Recent crystallographic data suggest that conserved residues in the connection subdomain and C-terminal ribonuclease H (RNase H) domain of human immunodeficiency virus type 1 reverse transcriptase (HIV-1 RT) contact the nascent DNA primer and modulate the trajectory of the template relative to the RNase H catalytic center. Within the RNase H domain, these residues include Thr473, Glu475, Lys476, Tyr501, and Ile505, while His539 and Asn474 interact with the scissile phosphate of the RNA template. Amino acid substitutions at several of these positions were evaluated in the context of hydrolysis of nonspecific RNA-DNA hybrids and substrates mimicking specific RNase H-mediated events. With the exception of mutant I505G, which exhibited a dimerization defect, substituting alanine at positions 473-476 and 501 had minimal consequences for DNA synthesis on duplex and hybrid DNA and RNA substrates. In contrast, the efficiency with which most mutants catalyzed polymerization-independent RNase H cleavage was sharply reduced. This deficiency was more pronounced when mutant enzymes were challenged to process the (+) strand polypurine tract (PPT) primer from either (+) RNA or a PPT/(+) DNA RNA/DNA chimera. Reduced polymerization-independent RNase H activity also significantly influenced the rate of DNA strand transfer, suggesting the donor template must be reduced in size below 13 nt before this event proceeds.

Published

2002

46. HIV-1 reverse transcriptase interaction with model RNA-DNA duplexes.

Author

Gorshkova II, Rausch JW, Le Grice SF, and Crouch RJ

Subjects

Algorithms, Base Sequence, Binding, Competitive, Biotinylation, DNA genetics, DNA Primers genetics, DNA Primers metabolism, HIV Reverse Transcriptase genetics, Kinetics, Ligands, Mutation genetics, Nucleic Acid Heteroduplexes genetics, Oligonucleotide Array Sequence Analysis, Protein Binding, RNA genetics, Substrate Specificity, Surface Plasmon Resonance, Templates, Genetic, Thermodynamics, DNA metabolism, HIV Reverse Transcriptase metabolism, HIV-1 enzymology, Nucleic Acid Heteroduplexes metabolism, RNA metabolism

Abstract

HIV-1 reverse transcriptase (HIV-1 RT) is a multifunctional enzyme responsible for converting viral RNA into preintegrative DNA during the early stages of viral infection. DNA polymerase and RNase H activities are required, and several conformationally distinct primer-templates must be accommodated by the enzyme during the process. Parameters of interaction between model substrates (ligands) and HIV-1 RT (wild type p66/p51 and the RNase H-deficient mutant p66(E478Q)/p51) (analytes) were estimated by surface plasmon resonance at 25 degrees C, pH 8.0. Binding of RT to the ligands is specific and can be analyzed using a conventional 1:1 binding algorithm. RNA-DNA hybrids with 5'-template overhangs of 6 and 12 nucleotides bind to RT approximately one order of magnitude stronger than the corresponding 36-mer with blunt ends due to slower dissociation. Immobilization of the latter through either the 5'-end of RNA or DNA strand does not change the equilibrium constant (K(D)) for wild-type RT but the values of kinetic constants of association and dissociation differ significantly. For the p66(E478Q)/p51 enzyme, orientation effects are notable even altering the K(D) value. Binding of the p66(E478Q)/p51 to any RNA-DNA hybrids is slightly stronger compared with wild type. Data can be interpreted in terms of the mechanism of reverse transcription., (Copyright 2001 Academic Press.)

Published

2001

47. Evaluation of retroviral ribonuclease H activity.

Author

Miller JT, Rausch JW, and Le Grice SF

Subjects

HIV Reverse Transcriptase isolation & purification, Humans, HIV Reverse Transcriptase metabolism, HIV-1 enzymology

Published

2001

48. Probing contacts between the ribonuclease H domain of HIV-1 reverse transcriptase and nucleic acid by site-specific photocross-linking.

Author

Rausch JW, Sathyanarayana BK, Bona MK, and Le Grice SF

Subjects

Azides metabolism, Cross-Linking Reagents metabolism, Crystallography, X-Ray, Cysteine genetics, DNA biosynthesis, DNA chemistry, DNA Primers, HIV Reverse Transcriptase genetics, Humans, Models, Molecular, Mutation, Nucleic Acid Conformation, Nucleoproteins chemistry, Protein Structure, Secondary, RNA chemistry, Ribonuclease H genetics, HIV Reverse Transcriptase chemistry, HIV-1 enzymology, Ribonuclease H chemistry

Abstract

Cys(38) and Cys(280) of p66/p51 human immunodeficiency virus type 1 reverse transcriptase (HIV-1 RT) can be converted to Ser without affecting enzyme function. We have exploited this feature to construct and purify "monocysteine" RT derivatives for site-specific modification with the photoactivable cross-linking agent, p-azidophenacyl bromide. Acylation of a unique cysteine residue introduced at the extreme C terminus of the p66 subunit (C(561)) with an azidophenacyl group allowed us to probe contacts between residues C-terminal to alpha-helix E' of the RNase H domain and structurally divergent nucleic acid duplexes. In a binary complex of RT and template-primer, we demonstrate efficient cross-linking to primer nucleotides -21 to -24/-25, and template nucleotides -18 to -21. Cross-linking specificity was confirmed by an analogous evaluation following limited primer extension, where the profile is displaced by the register of DNA synthesis. Finally, contact with a DNA primer hybridized to an isogenic RNA or DNA template indicates subtle alterations in cross-linking specificity, suggesting differences in nucleic acid geometry between duplex DNA and RNA/DNA hybrids at the RNase H domain. These data exemplify how site-specific acylation of HIV-1 RT can be used to provide high resolution structural data to complement crystallographic studies.

Published

2000

49. Metal-ion stoichiometry of the HIV-1 RT ribonuclease H domain: evidence for two mutually exclusive sites leads to new mechanistic insights on metal-mediated hydrolysis in nucleic acid biochemistry.

Author

Cowan JA, Ohyama T, Howard K, Rausch JW, Cowan SM, and Le Grice SF

Subjects

Calorimetry, Crystallography, X-Ray, HIV Reverse Transcriptase chemistry, HIV Reverse Transcriptase genetics, Hydrolysis, Models, Molecular, Protein Binding, Protein Conformation, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Thermodynamics, HIV Reverse Transcriptase metabolism, Manganese metabolism, Nucleic Acids metabolism, Ribonuclease H metabolism

Abstract

Crystallographic studies of the Mn(2+)-doped RNase H domain of human immunodeficiency virus type 1 reverse transcriptase (HIV-1 RT) have revealed two bound Mn2+ separated by approximately 4A and surrounded by a cluster of four conserved carboxylates. Escherichia coli RNase H is structurally similar to the RNase H domain of HIV-1 RT, but requires one divalent metal cation for its activity, implying either that the HIV-1 RT RNase H domain contrasts in its ability to bind two divalent metal ions, or that the crystallographic data reflect specific use of Mn2+ and/ or the doping technique employed. Metal binding stoichiometry has been determined for Mn2+ and the biologically more relevant Mg2+ cation by solution calorimetric studies of native and recombinant p66/p51 HIV-1 RT. Three Mn2+ ions bind to HIV-1 RT apo-enzyme: one at the DNA polymerase and two at the RNase H catalytic center, the latter being consistent with crystallographic results. However, only one Mg2+ ion is bound in the RNase H catalytic center. Several mechanistic implications arise from these results, including the possibility of mutually exclusive Mg2+ binding sites that might be occupied according to the specific reaction being catalyzed by the multifunctional RNase H domain. The occurrence of distinct binding stoichiometries for Mg2+ and Mn2+ to multifunctional enzymes has previously been reported.

Published

2000

50. Characterization of (+) strand initiation and termination sequences located at the center of the equine infectious anemia virus genome.

Author

Stetor SR, Rausch JW, Guo MJ, Burnham JP, Boone LR, Waring MJ, and Le Grice SF

Subjects

Animals, Cells, Cultured, DNA, Viral biosynthesis, Genome, Viral, Horses, DNA, Viral genetics, Infectious Anemia Virus, Equine genetics, Virus Replication

Abstract

Permeabilized preparations of equine infectious anemia virus (EIAV) are shown here to support efficient and accurate synthesis of full-length double-stranded proviral DNA. When (-) and (+) strand products were analyzed by Southern blotting, a discontinuity, mapping approximately to the center of the EIAV genome, could be demonstrated for the (+) strand, predicting a second site for initiation of DNA synthesis and a specific mechanism of (+) strand termination. Precise localization of this (+) strand origin within the integrase (IN) coding region was achieved through its in vitro selection and extension into, and excision from, nascent DNA by purified recombinant p66/p51 EIAV reverse transcriptase (RT), suggesting that the EIAV genome harbors a central polypurine tract (cPPT). In addition, a model system was developed for evaluating whether sequences immediately downstream of the cPPT would terminate (+) strand synthesis in the context of strand displacement. Such a sequence was indeed discovered which functions in a manner analogous to that of the central termination sequence (CTS) of HIV, where A-tract-induced minor groove compression has been suggested to induce localized distortion of the nucleic acid duplex and termination of (+) strand synthesis. This interpretation is reinforced by experiments indicating that read-through of the CTS can be efficiently promoted by substituting 2,6-diaminopurine for adenine, thereby relieving minor groove compression. The nucleotide substitution can also shift the site of termination in strand displacement (+) strand synthesis. Collectively, our data support proposals that lentiviruses may have evolved specialized mechanisms for initiating and terminating (+) strand DNA synthesis at the center of their genomes.

Published

1999