Your search keyword '"Bruce E. Torbett"' showing total 118 results

1. Sequencing and Structure Probing of Long RNAs Using MarathonRT: A Next-Generation Reverse Transcriptase

Author

Olga Potapova, Anna Marie Pyle, Brenton R. Graveley, Li-Tao Guo, Han Wan, Bruce E. Torbett, Nicholas C. Huston, Rebecca L. Adams, Christian M. Gallardo, and Sara Olson

Subjects

RNA-Seq, Computational biology, Biology, Article, Primer extension, Cell Line, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, Bacterial Proteins, Structural Biology, Humans, Nucleic acid structure, Molecular Biology, 030304 developmental biology, 0303 health sciences, Bacteria, Sequence Analysis, RNA, Computational Biology, High-Throughput Nucleotide Sequencing, RNA, RNA-Directed DNA Polymerase, Group II intron, Amplicon, Reverse transcriptase, Nucleic Acid Conformation, 030217 neurology & neurosurgery

Abstract

Reverse transcriptase (RT) enzymes are indispensable tools for interrogating diverse aspects of RNA metabolism and transcriptome composition. Due to the growing interest in sequence and structural complexity of long RNA molecules, processive RT enzymes are now required for preserving linkage and information content in mixed populations of transcripts, and the low-processivity RT enzymes that are commercially available cannot meet this need. MarathonRT is encoded within a eubacterial group II intron, and it has been shown to efficiently copy highly structured long RNA molecules in a single pass. In this work, we systematically characterize MarathonRT as a tool enzyme and optimize its performance in a variety of applications that include single-cycle reverse transcription of long RNAs, dimethyl sulfate mutational profiling (DMS-MaP), selective 2′-hydroxyl acylation analyzed by primer extension and mutational profiling (SHAPE-MaP), using ultra-long amplicons and the detection of natural RNA base modifications. By diversifying MarathonRT reaction protocols, we provide an upgraded suite of tools for cutting-edge RNA research and clinical application.

Published

2020

2. Development of Lentiviral Vectors for HIV-1 Gene Therapy with Vif-Resistant APOBEC3G

Author

Daniel Ackerman, Vinay K. Pathak, Wei-Shau Hu, Olga A. Nikolaitchik, Krista A. Delviks-Frankenberry, Maria Hamscher, Bruce E. Torbett, and Nina D. Timberlake

Subjects

0301 basic medicine, Genetic enhancement, viruses, Biology, D128K, Article, Virus, Viral vector, 03 medical and health sciences, Transduction (genetics), 0302 clinical medicine, Drug Discovery, CD34+ HSPC, Progenitor cell, APOBEC3G, lentiviral vector, hypermutation, lcsh:RM1-950, virus diseases, Cytidine deaminase, self-activating vector, gene therapy, Virology, CD4+ T cells, 3. Good health, Haematopoiesis, 030104 developmental biology, lcsh:Therapeutics. Pharmacology, 030220 oncology & carcinogenesis, HIV-1, Molecular Medicine

Abstract

Strategies to control HIV-1 replication without antiviral therapy are needed to achieve a functional cure. To exploit the innate antiviral function of restriction factor cytidine deaminase APOBEC3G (A3G), we developed self-activating lentiviral vectors that efficiently deliver HIV-1 Vif-resistant mutant A3G-D128K to target cells. To circumvent APOBEC3 expression in virus-producing cells, which diminishes virus infectivity, a vector containing two overlapping fragments of A3G-D128K was designed that maintained the gene in an inactive form in the virus-producer cells. However, during transduction of target cells, retroviral recombination between the direct repeats reconstituted an active A3G-D128K in 89%–98% of transduced cells. Lentiviral vectors that expressed A3G-D128K transduced CD34+ hematopoietic stem and progenitor cells with a high efficiency (>30%). A3G-D128K expression in T cell lines CEM, CEMSS, and PM1 potently inhibited spreading infection of several HIV-1 subtypes by C-to-U deamination leading to lethal G-to-A hypermutation and inhibition of reverse transcription. SIVmac239 and HIV-2 were not inhibited, since their Vifs degraded A3G-D128K. A3G-D128K expression in CEM cells potently suppressed HIV-1 replication for >3.5 months without detectable resistant virus, suggesting a high genetic barrier for the emergence of A3G-D128K resistance. Because of this, A3G-D128K expression in HIV-1 target cells is a potential anti-HIV gene therapy approach that could be combined with other therapies for the treatment and functional cure of HIV-1 infection., Graphical Abstract

Published

2019

3. Co-variation of viral recombination with single nucleotide variants during virus evolution revealed by CoVaMa

Author

Stephanea Sotcheff, Elizabeth Jaworski, Andrew Routh, Christian M. Gallardo, Bruce E. Torbett, and Shiyi Wang

Subjects

Genetics, Genetic complexity, chemistry.chemical_classification, Linkage disequilibrium, chemistry, Viral evolution, Nucleotide, Nanopore sequencing, Co variation, Biology, Genome, Recombination

Abstract

Adaptation of viruses to their environments occurs through the acquisition of both novel Single-Nucleotide Variants (SNV) and recombination events including insertions, deletions, and duplications. The co-occurrence of SNVs in individual viral genomes during their evolution has been well-described. However, unlike covariation of SNVs, studying the correlation between recombination events with each other or with SNVs has been hampered by their inherent genetic complexity and a lack of bioinformatic tools. Here, we expanded our previously reported CoVaMa pipeline (v0.1) to measure linkage disequilibrium between recombination events and SNVs within both short-read and long-read sequencing datasets. We demonstrate this approach using long-read nanopore sequencing data acquired from Flock House virus (FHV) serially passaged in vitro. We found SNVs that were either correlated or anti-correlated with large genomic deletions generated by nonhomologous recombination that give rise to Defective-RNAs. We also analyzed NGS data from longitudinal HIV samples derived from a patient undergoing antiretroviral therapy who proceeded to virological failure. We found correlations between insertions in the p6Gag and mutations in Gag cleavage sites. This report confirms previous findings and provides insights on novel associations between SNVs and specific recombination events within the viral genome and their role in viral evolution.

Published

2021

4. MrHAMER yields highly accurate single molecule viral sequences enabling analysis of intra-host evolution

Author

Shiyi Wang, Bruce E Torbett, David M. Smith, Andrew Routh, Susan J. Little, Christian M. Gallardo, and Daniel Jorge Montiel-Garcia

Subjects

DNA, Complementary, AcademicSubjects/SCI00010, viruses, Human immunodeficiency virus (HIV), HIV Infections, Computational biology, Genome, Viral, Biology, medicine.disease_cause, Genome, law.invention, Evolution, Molecular, chemistry.chemical_compound, Gene interaction, law, Drug Resistance, Viral, Genetics, medicine, Humans, Viral Sequencing, Polymerase chain reaction, Narese/7, Mutation, Host (biology), Reverse Transcriptase Polymerase Chain Reaction, Direct observation, RNA, HIV, Narese/22, Fusion protein, Fusion Proteins, gag-pol, Nanopore Sequencing, chemistry, Viral genomes, Methods Online, DNA

Abstract

Technical challenges remain in the sequencing of RNA viruses due to their high intra-host diversity. This bottleneck is particularly pronounced when interrogating long-range co-evolved genetic interactions given the read-length limitations of next-generation sequencing platforms. This has hampered the direct observation of these genetic interactions that code for protein-protein interfaces with relevance in both drug and vaccine development. Here we overcome these technical limitations by developing a nanopore-based long-range viral sequencing pipeline that yields accurate single molecule sequences of circulating virions from clinical samples. We demonstrate its utility in observing the evolution of individual HIV Gag-Pol genomes in response to antiviral pressure. Our pipeline, called Multi-read Hairpin Mediated Error-correction Reaction (MrHAMER), yields >1000s of viral genomes per sample at 99.9% accuracy, maintains the original proportion of sequenced virions present in a complex mixture, and allows the detection of rare viral genomes with their associated mutations present at

Published

2021

5. Interactions of HIV-1 Capsid with Host Factors and Their Implications for Developing Novel Therapeutics

Author

Shentian Zhuang and Bruce E Torbett

Subjects

0301 basic medicine, viruses, Human Immunodeficiency Virus Proteins, Human immunodeficiency virus (HIV), lcsh:QR1-502, capsid-targeting inhibitors, Host factors, HIV Infections, Review, Biology, medicine.disease_cause, Genome, lcsh:Microbiology, 03 medical and health sciences, 0302 clinical medicine, Virology, Virus Uncoating, medicine, Humans, Host Microbial Interactions, HIV-1 capsid, Virion, biochemical phenomena, metabolism, and nutrition, host factors, Chromatin, Cell biology, A-site, 030104 developmental biology, Infectious Diseases, Viral replication, Capsid, HIV-1, Capsid Proteins, high-throughput screening techniques, Nuclear transport, antiretroviral therapeutics, 030217 neurology & neurosurgery

Abstract

The Human Immunodeficiency Virus type 1 (HIV-1) virion contains a conical shell, termed capsid, encasing the viral RNA genome. After cellular entry of the virion, the capsid is released and ensures the protection and delivery of the HIV-1 genome to the host nucleus for integration. The capsid relies on many virus–host factor interactions which are regulated spatiotemporally throughout the course of infection. In this paper, we will review the current understanding of the highly dynamic HIV-1 capsid–host interplay during the early stages of viral replication, namely intracellular capsid trafficking after viral fusion, nuclear import, uncoating, and integration of the viral genome into host chromatin. Conventional anti-retroviral therapies primarily target HIV-1 enzymes. Insights of capsid structure have resulted in a first-in-class, long-acting capsid-targeting inhibitor, GS-6207 (Lenacapavir). This inhibitor binds at the interface between capsid protein subunits, a site known to bind host factors, interferes with capsid nuclear import, HIV particle assembly, and ordered assembly. Our review will highlight capsid structure, the host factors that interact with capsid, and high-throughput screening techniques, specifically genomic and proteomic approaches, that have been and can be used to identify host factors that interact with capsid. Better structural and mechanistic insights into the capsid–host factor interactions will significantly inform the understanding of HIV-1 pathogenesis and the development of capsid-centric antiretroviral therapeutics.

Published

2021

6. CD46 Null Packaging Cell Line Improves Measles Lentiviral Vector Production and Gene Delivery to Hematopoietic Stem and Progenitor Cells

Author

Olivia Garijo, Bruce E. Torbett, Elizabeth Simpson, Petra Minder, Craig X. Chen, Stosh Ozog, Els Verhoeyen, and Nina D. Timberlake

Subjects

0301 basic medicine, lcsh:QH426-470, Genetic enhancement, viruses, measles lentiviral vector, Article, Viral vector, Measles virus, 03 medical and health sciences, 0302 clinical medicine, enhanced gene delivery, stem cells, Genetics, lcsh:QH573-671, Progenitor cell, syncytia, Molecular Biology, CD46, pseudotyping, biology, lcsh:Cytology, lentiviral vector, Transfection, biology.organism_classification, vector production, 3. Good health, Cell biology, lcsh:Genetics, 030104 developmental biology, Vesicular stomatitis virus, measles glycoprotein, 030220 oncology & carcinogenesis, Pseudotyping, Molecular Medicine, Stem cell, CD46 knockout

Abstract

Lentiviral vectors (LVs) pseudotyped with the measles virus hemagglutinin (H) and fusion (F) glycoproteins have been reported to more efficiently transduce hematopoietic stem and progenitor cells (HSPCs) compared with vesicular stomatitis virus glycoprotein (VSV-G) pseudotyped LVs. However, a limit to H/F LV use is the low titer of produced vector. Here we show that measles receptor (CD46) expression on H/F transfected HEK293T vector-producing cells caused adjacent cell membrane fusion, resulting in multinucleate syncytia formation and death prior to peak vector production, leading to contaminating cell membranes that co-purified with LV. H/F LVs produced in CD46 null HEK293T cells, generated by CRISPR/Cas9-mediated knockout of CD46, produced 2-fold higher titer vector compared with LVs produced in CD46+ HEK293T cells. This resulted in approximately 2- to 3-fold higher transduction of HSPCs while significantly reducing target cell cytotoxicity caused by producer cell contaminates. Improved H/F LV entry into HSPCs and distinct entry mechanisms compared with VSV-G LV were also observed by confocal microscopy. Given that vector production is a major source of cost and variability in clinical trials of gene therapy, we propose that the use of CD46 null packaging cells may help to address these challenges., Graphical Abstract

Published

2018

7. mTOR inhibitors lower an intrinsic barrier to virus infection mediated by IFITM3

Author

Bruce E. Torbett, Stosh Ozog, Alex A. Compton, and Guoli Shi

Subjects

0301 basic medicine, fusion, viruses, virus, Endosomes, Gene delivery, Antiviral Agents, ESCRT, IFITM, Cell Line, Viral vector, 03 medical and health sciences, Interferon, Viral entry, Cell Line, Tumor, medicine, Humans, Gene silencing, endosome, PI3K/AKT/mTOR pathway, Sirolimus, Multidisciplinary, biology, Chemistry, TOR Serine-Threonine Kinases, Membrane Proteins, RNA-Binding Proteins, Cell Biology, interferon, Biological Sciences, Virus Internalization, biology.organism_classification, Sendai virus, 3. Good health, Cell biology, Protein Transport, HEK293 Cells, 030104 developmental biology, PNAS Plus, Virus Diseases, Host-Pathogen Interactions, HeLa Cells, medicine.drug

Abstract

Significance Gene delivery by virus-like particles holds enormous therapeutic potential to correct inherited genetic disorders and to prevent infectious disease. However, cells express antiviral factors that prevent virus infection and, consequently, limit the success of gene therapy. Here, we reveal the mechanism by which the drug rapamycin improves lentivirus-mediated gene delivery. Rapamycin treatment led to degradation of IFITM3, a broad and potent antiviral protein which inhibits virus entry into cells. IFITM3 is selectively cleared from endosomes, the sites where viral and cellular membranes fuse, and is sorted for disposal in lysosomes. While revealing an immunosuppressive function with clinical benefits, we caution that rapamycin use in humans may facilitate infection by pathogenic viruses like Influenza A virus., Rapamycin and its derivatives are specific inhibitors of mammalian target of rapamycin (mTOR) kinase and, as a result, are well-established immunosuppressants and antitumorigenic agents. Additionally, this class of drug promotes gene delivery by facilitating lentiviral vector entry into cells, revealing its potential to improve gene therapy efforts. However, the precise mechanism was unknown. Here, we report that mTOR inhibitor treatment results in down-regulation of the IFN-induced transmembrane (IFITM) proteins. IFITM proteins, especially IFITM3, are potent inhibitors of virus–cell fusion and are broadly active against a range of pathogenic viruses. We found that the effect of rapamycin treatment on lentiviral transduction is diminished upon IFITM silencing or knockout in primary and transformed cells, and the extent of transduction enhancement depends on basal expression of IFITM proteins, with a major contribution from IFITM3. The effect of rapamycin treatment on IFITM3 manifests at the level of protein, but not mRNA, and is selective, as many other endosome-associated transmembrane proteins are unaffected. Rapamycin-mediated degradation of IFITM3 requires endosomal trafficking, ubiquitination, endosomal sorting complex required for transport (ESCRT) machinery, and lysosomal acidification. Since IFITM proteins exhibit broad antiviral activity, we show that mTOR inhibition also promotes infection by another IFITM-sensitive virus, Influenza A virus, but not infection by Sendai virus, which is IFITM-resistant. Our results identify the molecular basis by which mTOR inhibitors enhance virus entry into cells and reveal a previously unrecognized immunosuppressive feature of these clinically important drugs. In addition, this study uncovers a functional convergence between the mTOR pathway and IFITM proteins at endolysosomal membranes.

Published

2018

8. Prostaglandin E2 Increases Lentiviral Vector Transduction Efficiency of Adult Human Hematopoietic Stem and Progenitor Cells

Author

Holly Horton, Lauryn Christiansen, Amanda Hamel, Olivia Garijo, Bruce E. Torbett, Philip D. Gregory, Garrett C. Heffner, Gretchen Lewis, Yegor Smurnyy, Dakota Campbell, Melissa Bonner, Wenliang Zhang, Gabor Istvan Veres, Seema Shaw, Francis J. Pierciey, Kendrick A. Goss, and Mitchell Finer

Subjects

0301 basic medicine, Genetic enhancement, CD34, Antigens, CD34, Transduction (genetics), Mice, Transduction, Genetic, Drug Discovery, Transgenes, Gene Transfer Techniques, Hematopoietic stem cell, transduction, gene therapy, Cell biology, Globins, Haematopoiesis, medicine.anatomical_structure, Molecular Medicine, Original Article, Genetic Vectors, Transplantation, Heterologous, Anemia, Sickle Cell, Biology, Dinoprostone, Viral vector, Cell Line, 03 medical and health sciences, vector copy number, Genetics, medicine, hemoglobinopathy, Animals, Humans, Progenitor cell, Molecular Biology, Gene Library, Pharmacology, Severe combined immunodeficiency, prostaglandin E2, lentiviral vector, Lentivirus, beta-Thalassemia, Genetic Therapy, Virus Internalization, medicine.disease, Hematopoietic Stem Cells, 030104 developmental biology, Immunology, Leukocyte Common Antigens, hematopoietic stem cell

Abstract

Gene therapy currently in development for hemoglobinopathies utilizes ex vivo lentiviral transduction of CD34+ hematopoietic stem and progenitor cells (HSPCs). A small-molecule screen identified prostaglandin E2 (PGE2) as a positive mediator of lentiviral transduction of CD34+ cells. Supplementation with PGE2 increased lentiviral vector (LVV) transduction of CD34+ cells approximately 2-fold compared to control transduction methods with no effect on cell viability. Transduction efficiency was consistently increased in primary CD34+ cells from multiple normal human donors and from patients with β-thalassemia or sickle cell disease. Notably, PGE2 increased transduction of repopulating human HSPCs in an immune-deficient (nonobese diabetic/severe combined immunodeficiency/interleukin-2 gamma receptor null [NSG]) xenotransplantation mouse model without evidence of in vivo toxicity, lineage bias, or a de novo bias of lentiviral integration sites. These data suggest that PGE2 improves lentiviral transduction and increases vector copy number, therefore resulting in increased transgene expression. As a result, PGE2 may be useful in clinical gene therapy applications using lentivirally modified HSPCs., Heffner et al. performed a small-molecule screen and identified prostaglandin E2 (PGE2) as a positive mediator of lentiviral transduction of CD34+ cells. Their data suggest that PGE2-mediated improvements in transduction efficiency may aid in clinical gene therapy applications using lentivirally modified HSPCs.

Published

2017

9. PU.1 supports TRAIL-induced cell death by inhibiting NF-kappaB-mediated cell survival and inducing DR5 expression

Author

Deborah Shan-Krauer, Thomas Kaufmann, Elena A. Federzoni, Magali Humbert, Steffen Frese, Aladin Haimovici, Thomas Brunner, Bruce E. Torbett, and Mario P. Tschan

Subjects

0301 basic medicine, Programmed cell death, Myeloid, Antineoplastic Agents, Apoptosis, HL-60 Cells, Biology, TNF-Related Apoptosis-Inducing Ligand, 03 medical and health sciences, ddc:570, Cell Line, Tumor, Proto-Oncogene Proteins, Precursor cell, hemic and lymphatic diseases, medicine, Humans, Anthracyclines, RNA, Small Interfering, Molecular Biology, Original Paper, Gene Expression Regulation, Leukemic, Cell growth, Transcription Factor RelA, Hematopoietic stem cell, Myeloid leukemia, Cell Biology, 3. Good health, Cell biology, Receptors, TNF-Related Apoptosis-Inducing Ligand, Haematopoiesis, 030104 developmental biology, medicine.anatomical_structure, Drug Resistance, Neoplasm, Trans-Activators, Tumor necrosis factor alpha, Protein Binding, Signal Transduction

Abstract

The hematopoietic Ets-domain transcription factor PU.1/SPI1 orchestrates myeloid, B- and T-cell development, and also supports hematopoietic stem cell maintenance. Although PU.1 is a renowned tumor suppressor in acute myeloid leukemia (AML), a disease characterized by an accumulation of immature blast cells, comprehensive studies analyzing the role of PU.1 during cell death responses in AML treatment are missing. Modulating PU.1 expression in AML cells, we found that PU.1 supports tumor necrosis factor-related apoptosis-inducing ligand (TRAIL)-mediated apoptosis via two mechanisms: (a) by repressing NF-κB activity via a novel direct PU.1-RelA/p65 protein-protein interaction, and (b) by directly inducing TRAIL receptor DR5 expression. Thus, expression of NF-κB-regulated antiapoptotic genes was sustained in PU.1-depleted AML cells upon TRAIL treatment and DR5 levels were decreased. Last, PU.1 deficiency significantly increased AML cell resistance to anthracycline treatment. Altogether, these results reveal a new facet of PU.1's tumor suppressor function during antileukemic therapies. published

Published

2017

10. Resveratrol trimer enhances gene delivery to hematopoietic stem cells by reducing antiviral restriction at endosomes

Author

Dale L. Boger, Gabriella Sghia-Hughes, Christopher M. Glinkerman, Elizabeth Simpson, Guoli Shi, Raymond R. Carillo, Saritha S. D'Souza, Kip Hermann, Hans-Peter Kiem, Nina D. Timberlake, Scott A. Snyder, Lauren E Schefter, Jennifer E. Adair, Kevin G. Haworth, Byoung Y. Ryu, Brian P. Sorrentino, Olivia Garijo, Bruce E. Torbett, Igor I. Slukvin, Stosh Ozog, and Alex A. Compton

Subjects

0301 basic medicine, Genetic enhancement, Immunology, Genetic Vectors, Endosomes, Gene delivery, Biology, Resveratrol, Biochemistry, 03 medical and health sciences, Transduction (genetics), chemistry.chemical_compound, Mice, 0302 clinical medicine, Transduction, Genetic, Animals, Humans, Progenitor cell, Lentivirus, Membrane Proteins, Cell Biology, Hematology, Gene Therapy, Hematopoietic Stem Cells, Cell biology, Haematopoiesis, Protein Transport, 030104 developmental biology, chemistry, 030220 oncology & carcinogenesis, Heterografts, Stem cell, Ex vivo

Abstract

Therapeutic gene delivery to hematopoietic stem cells (HSCs) holds great potential as a life-saving treatment of monogenic, oncologic, and infectious diseases. However, clinical gene therapy is severely limited by intrinsic HSC resistance to modification with lentiviral vectors (LVs), thus requiring high doses or repeat LV administration to achieve therapeutic gene correction. Here we show that temporary coapplication of the cyclic resveratrol trimer caraphenol A enhances LV gene delivery efficiency to human and nonhuman primate hematopoietic stem and progenitor cells with integrating and nonintegrating LVs. Although significant ex vivo, this effect was most dramatically observed in human lineages derived from HSCs transplanted into immunodeficient mice. We further show that caraphenol A relieves restriction of LV transduction by altering the levels of interferon-induced transmembrane (IFITM) proteins IFITM2 and IFITM3 and their association with late endosomes, thus augmenting LV core endosomal escape. Caraphenol A-mediated IFITM downregulation did not alter the LV integration pattern or bias lineage differentiation. Taken together, these findings compellingly demonstrate that the pharmacologic modification of intrinsic immune restriction factors is a promising and nontoxic approach for improving LV-mediated gene therapy.

Published

2019

11. Role of Hexokinase 2 and 3 in Energy Metabolism, Myeloid Differentiation and Cancer Development

Author

James J. Moresco, Petra Minder, Iris Mashimo, John R. Yates, Kristina Seiler, Elena A. Federzoni, Magali Humbert, Mario P. Tschan, and Bruce E. Torbett

Subjects

Myeloid, medicine.anatomical_structure, Hexokinase-2, Genetics, medicine, Energy metabolism, Cancer research, Cancer development, Biology, Molecular Biology, Biochemistry, Biotechnology

Published

2020

12. CoVaMa: Co-Variation Mapper for disequilibrium analysis of mutant loci in viral populations using next-generation sequence data

Author

Max W. Chang, Andrew Routh, Bruce E. Torbett, John E. Johnson, and Jason F. Okulicz

Subjects

Linkage disequilibrium, Disequilibrium, Population, HIV Infections, Genome, Viral, Biology, medicine.disease_cause, Genome, Article, Linkage Disequilibrium, General Biochemistry, Genetics and Molecular Biology, Virus, medicine, Humans, education, Molecular Biology, Genetics, Mutation, education.field_of_study, Sequence Analysis, RNA, HIV, High-Throughput Nucleotide Sequencing, Epistasis, Genetic, Open reading frame, RNA, Viral, Epistasis, medicine.symptom, Algorithms

Abstract

Next-Generation Sequencing (NGS) has transformed our understanding of the dynamics and diversity of virus populations for human pathogens and model systems alike. Due to the sensitivity and depth of coverage in NGS, it is possible to measure the frequency of mutations that may be present even at vanishingly low frequencies within the viral population. Here, we describe a simple bioinformatic pipeline called CoVaMa (Co-Variation Mapper) scripted in Python that detects correlated patterns of mutations in a viral sample. Our algorithm takes NGS alignment data and populates large matrices of contingency tables that correspond to every possible pairwise interaction of nucleotides in the viral genome or amino acids in the chosen open reading frame. These tables are then analysed using classical linkage disequilibrium to detect and report evidence of epistasis. We test our analysis with simulated data and then apply the approach to find epistatically linked loci in Flock House Virus genomic RNA grown under controlled cell culture conditions. We also reanalyze NGS data from a large cohort of HIV infected patients and find correlated amino acid substitution events in the protease gene that have arisen in response to anti-viral therapy. This both confirms previous findings and suggests new pairs of interactions within HIV protease. The script is publically available at http://sourceforge.net/projects/covama.

Published

2015

13. Low DICER1 expression is associated with attenuated neutrophil differentiation and autophagy of NB4 APL cells

Author

Elena A. Federzoni, Julian Wampfler, Mario P. Tschan, Bruce E. Torbett, and Martin F. Fey

Subjects

Ribonuclease III, Myeloid, Neutrophils, Immunology, CD34, Tretinoin, Biology, Cell Development, Differentiation, & Trafficking, DEAD-box RNA Helicases, Leukemia, Promyelocytic, Acute, Neutrophil differentiation, Cell Line, Tumor, hemic and lymphatic diseases, microRNA, Autophagy, medicine, Transcriptional regulation, Humans, Immunology and Allergy, RNA, Messenger, RNA Processing, Post-Transcriptional, Progenitor cell, neoplasms, Cell Differentiation, Cell Biology, MicroRNAs, medicine.anatomical_structure, Cell culture, Gene Knockdown Techniques, Cancer research

Abstract

Successful myeloid differentiation depends on the expression of a series of miRNAs. Thus, it is hardly surprising that miRNAs are globally repressed in AML, a disease mainly characterized by a block in cellular myeloid differentiation. Studies investigating the mechanisms for low miRNA expression in AML has mostly focused on altered transcriptional regulation or deletions, whereas defective miRNA processing has received less attention. In this study, we report that the expression of the key miRNA processing enzyme DICER1 is down-regulated in primary AML patient samples and healthy CD34+ progenitor cells as compared with granulocytes. In line with these findings, Dicer1 expression was induced significantly in AML cell lines upon neutrophil differentiation. The knocking down of DICER1 in AML cells significantly attenuated neutrophil differentiation, which was paralleled by decreased expression of miRNAs involved in this process. Moreover, we found that inhibiting DICER1 attenuated the activation of autophagy, a cellular recycling process that is needed for proper neutrophil differentiation of AML cells. Our results clearly indicate that DICER1 plays a novel role in neutrophil differentiation as well as in myeloid autophagy of AML cells.

Published

2015

14. Low Autophagy (ATG) Gene Expression Is Associated with an Immature AML Blast Cell Phenotype and Can Be Restored during AML Differentiation Therapy

Author

Shida Yousefi, Jing Jin, Anna M. Schläfli, Hans-Uwe Simon, Jasmin Batliner, Deborah Shan-Krauer, Mario P. Tschan, Magali Humbert, Marion Ernst, Bruce E. Torbett, Adrian Britschgi, and Elena A. Federzoni

Subjects

0301 basic medicine, Aging, Myeloid, Article Subject, ATG5, Gene Expression, 610 Medicine & health, Biology, Biochemistry, 03 medical and health sciences, Differentiation therapy, Neutrophil differentiation, hemic and lymphatic diseases, Cell Line, Tumor, Gene expression, medicine, Transcriptional regulation, Autophagy, Humans, lcsh:QH573-671, neoplasms, lcsh:Cytology, Myeloid leukemia, Cell Differentiation, Cell Biology, General Medicine, 3. Good health, Leukemia, Myeloid, Acute, 030104 developmental biology, medicine.anatomical_structure, Phenotype, Cancer research, 570 Life sciences, biology, Research Article

Abstract

Autophagy is an intracellular degradation system that ensures a dynamic recycling of a variety of building blocks required for self-renewal, homeostasis, and cell survival under stress. We used primary acute myeloid leukemia (AML) samples and human AML cell lines to investigate the regulatory mechanisms of autophagy and its role in AML differentiation. We found a significantly lower expression of key autophagy- (ATG-) related genes in primary AML as compared to healthy granulocytes, an increased autophagic activity during all-transretinoic acid- (ATRA-) induced neutrophil differentiation, and an impaired AML differentiation upon inhibition of ATG3, ATG4D, and ATG5. Supporting the notion of noncanonical autophagy, we found that ATRA-induced autophagy was Beclin1-independent compared to starvation- or arsenic trioxide- (ATO-) induced autophagy. Furthermore, we identified PU.1 as positive transcriptional regulator of ATG3, ATG4D, and ATG5. Low PU.1 expression in AML may account for low ATG gene expression in this disease. Low expression of the autophagy initiator ULK1 in AML can partially be attributed to high expression of the ULK1-targeting microRNA-106a. Our data clearly suggest that granulocytic AML differentiation relies on noncanonical autophagy pathways and that restoring autophagic activity might be beneficial in differentiation therapies.

Published

2018

15. Interactome analysis of the lymphocytic choriomeningitis virus nucleoprotein in infected cells reveals ATPase Na+/K+ transporting subunit Alpha 1 and prohibitin as host-cell factors involved in the life cycle of mammarenaviruses

Author

Yíngyún Caì, Masaharu Iwasaki, John R. Yates, Petra Minder, Jens H. Kuhn, Juan Carlos de la Torre, and Bruce E. Torbett

Subjects

0301 basic medicine, Life Cycles, Proteome, viruses, medicine.disease_cause, Biochemistry, Heat Shock Response, Mice, Cricetinae, Chlorocebus aethiops, Lymphocytic choriomeningitis virus, Small interfering RNAs, Protein Interaction Maps, Prohibitin, Biology (General), Arenaviridae, Cells, Cultured, Cellular Stress Responses, Staining, biology, Cell Staining, 3. Good health, Nucleic acids, Cell Processes, Host-Pathogen Interactions, Sodium-Potassium-Exchanging ATPase, Protein Binding, Research Article, Viral Entry, QH301-705.5, Immunology, Motor Proteins, Lymphocytic Choriomeningitis, Lymphocytic choriomeningitis, Research and Analysis Methods, Microbiology, Virus, 03 medical and health sciences, Viral life cycle, Viral entry, Molecular Motors, Virology, Prohibitins, DNA-binding proteins, medicine, Genetics, Animals, Humans, Non-coding RNA, Molecular Biology, Vero Cells, Biology and life sciences, Correction, Proteins, Cell Biology, RC581-607, biology.organism_classification, medicine.disease, Nucleoprotein, Gene regulation, Repressor Proteins, Cytoskeletal Proteins, 030104 developmental biology, Lassa virus, HEK293 Cells, Nucleoproteins, A549 Cells, Specimen Preparation and Treatment, Junin virus, RNA, Parasitology, Gene expression, Immunologic diseases. Allergy, Viral Transmission and Infection, Developmental Biology

Abstract

Several mammalian arenaviruses (mammarenaviruses) cause hemorrhagic fevers in humans and pose serious public health concerns in their endemic regions. Additionally, mounting evidence indicates that the worldwide-distributed, prototypic mammarenavirus, lymphocytic choriomeningitis virus (LCMV), is a neglected human pathogen of clinical significance. Concerns about human-pathogenic mammarenaviruses are exacerbated by of the lack of licensed vaccines, and current anti-mammarenavirus therapy is limited to off-label use of ribavirin that is only partially effective. Detailed understanding of virus/host-cell interactions may facilitate the development of novel anti-mammarenavirus strategies by targeting components of the host-cell machinery that are required for efficient virus multiplication. Here we document the generation of a recombinant LCMV encoding a nucleoprotein (NP) containing an affinity tag (rLCMV/Strep-NP) and its use to capture the NP-interactome in infected cells. Our proteomic approach combined with genetics and pharmacological validation assays identified ATPase Na+/K+ transporting subunit alpha 1 (ATP1A1) and prohibitin (PHB) as pro-viral factors. Cell-based assays revealed that ATP1A1 and PHB are involved in different steps of the virus life cycle. Accordingly, we observed a synergistic inhibitory effect on LCMV multiplication with a combination of ATP1A1 and PHB inhibitors. We show that ATP1A1 inhibitors suppress multiplication of Lassa virus and Candid#1, a live-attenuated vaccine strain of Junín virus, suggesting that the requirement of ATP1A1 in virus multiplication is conserved among genetically distantly related mammarenaviruses. Our findings suggest that clinically approved inhibitors of ATP1A1, like digoxin, could be repurposed to treat infections by mammarenaviruses pathogenic for humans., Author summary Viral hemorrhagic fever-causing mammalian viruses of the family Arenaviridae pose serious threats to humans in Africa and South America as the associated infections are highly lethal. The worldwide-distributed lymphocytic choriomeningitis virus (LCMV) is a relative of these dangerous viruses that can be worked with more safely in the laboratory. Although LCMV does not cause viral hemorrhagic fever, it can cause disease in humans. Currently, anti-arenavirus therapy options are very limited, not very effective, and associated with side effects. Development of new therapies has been hampered because knowledge on how arenaviruses interact with proteins of the host cells they infect is limited. Using a modified LCMV, we identified two host-cell proteins called ATPase Na+/K+ transporting subunit alpha 1 (ATP1A1) and prohibitin (PHB) as factors that promote arenavirus infection. Inhibitors of ATP1A1 (cardiac glycosides already used clinically for treatment of other diseases) suppressed multiplication in cell culture of Lassa virus and Junín virus, the two most significant viral hemorrhagic fever-causing mammarenaviruses. Therefore, our data suggest that these inhibitors could be used clinically to treat people infected with arenaviruses.

Published

2018

16. Inference of Epistatic Effects Leading to Entrenchment and Drug Resistance in HIV-1 Protease

Author

William F. Flynn, Bruce E. Torbett, Allan Haldane, and Ronald M. Levy

Subjects

0301 basic medicine, Models, Molecular, medicine.medical_treatment, HIV Infections, Computational biology, Drug resistance, 03 medical and health sciences, 0302 clinical medicine, HIV-1 protease, HIV Protease, Drug Resistance, Viral, Genetics, medicine, Humans, Protease inhibitor (pharmacology), Computer Simulation, Amino Acid Sequence, Molecular Biology, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Sequence (medicine), 0303 health sciences, Protease, biology, Wild type, Epistasis, Genetic, epistasis, mutational landscape, statistical inference, coevolution, HIV, drug resistance, 3. Good health, 030104 developmental biology, Mutation (genetic algorithm), Mutation, biology.protein, HIV-1, Epistasis, Fast Track, Sequence Alignment, 030217 neurology & neurosurgery

Abstract

Understanding the complex mutation patterns that give rise to drug resistant viral strains provides a foundation for developing more effective treatment strategies for HIV/AIDS. Multiple sequence alignments of drug-experienced HIV-1 protease sequences contain networks of many pair correlations which can be used to build a (Potts) Hamiltonian model of these mutation patterns. Using this Hamiltonian model we translate HIV protease sequence covariation data into quantitative predictions for the probability of observing specific mutation patterns which are in agreement with the observed sequence statistics. We find that the statistical energies of the Potts model are correlated with the fitness of individual proteins containing therapy-associated mutations as estimated by in vitro measurements of protein stability and viral infectivity. We show that the penalty for acquiring primary resistance mutations depends on the epistatic interactions with the sequence background. Primary mutations which lead to drug resistance can become highly advantageous (or entrenched) by the complex mutation patterns which arise in response to drug therapy despite being destabilizing in the wildtype background. Anticipating epistatic effects is important for the design of future protease inhibitor therapies.

Published

2017

17. Inhibition of GATE-16 attenuates ATRA-induced neutrophil differentiation of APL cells and interferes with autophagosome formation

Author

Bruce E. Torbett, Mario P. Tschan, Joy Chen, Daniel Brigger, and Martin F. Fey

Subjects

Adult, Male, Acute promyelocytic leukemia, Autophagosome, Myeloid, Adolescent, Neutrophils, Cellular differentiation, GABARAP, Biophysics, Antigens, CD34, Tretinoin, Biology, Biochemistry, Article, Cell Line, Young Adult, 03 medical and health sciences, 0302 clinical medicine, Leukemia, Promyelocytic, Acute, Neutrophil differentiation, hemic and lymphatic diseases, Autophagy, medicine, Humans, neoplasms, Molecular Biology, Adaptor Proteins, Signal Transducing, Aged, 030304 developmental biology, 0303 health sciences, Gene Expression Regulation, Leukemic, Microfilament Proteins, Myeloid leukemia, Cell Differentiation, Autophagy-Related Protein 8 Family, Cell Biology, Middle Aged, medicine.disease, Cell biology, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Female, Apoptosis Regulatory Proteins, Microtubule-Associated Proteins

Abstract

Autophagy is an intracellular bulk degradation process involved in cell survival upon stress induction, but also with a newly identified function in myeloid differentiation. The autophagy-related (ATG)8 protein family, including the GABARAP and LC3 subfamilies, is crucial for autophagosome biogenesis. In order to evaluate the significance of the GABARAPs in the pathogenesis of acute myeloid leukemia (AML), we compared their expression in primary AML patient samples, CD34(+) progenitor cells and in granulocytes from healthy donors. GABARAPL1 and GABARAPL2/GATE-16, but not GABARAP, were significantly downregulated in particular AML subtypes compared to normal granulocytes. Moreover, the expression of GABARAPL1 and GATE-16 was significantly induced during ATRA-induced neutrophil differentiation of acute promyelocytic leukemia cells (APL). Lastly, knocking down GABARAPL2/GATE-16 in APL cells attenuated neutrophil differentiation and decreased autophagic flux. In conclusion, low GABARAPL2/GATE-16 expression is associated with an immature myeloid leukemic phenotype and these proteins are necessary for neutrophil differentiation of APL cells.

Published

2013

18. The actin-binding protein CORO1A is a novel PU.1 (SPI1)- and CEBPA-regulated gene with significantly lower expression in APL and CEBPA-mutated AML patients

Author

Martin F. Fey, Magali Humbert, Gerhard Behre, Elisabeth Oppliger Leibundgut, Peter J. M. Valk, Bruce E. Torbett, Elena A. Federzoni, Mario P. Tschan, and Hematology

Subjects

Transcription, Genetic, medicine.disease_cause, 03 medical and health sciences, 0302 clinical medicine, Leukemia, Promyelocytic, Acute, Proto-Oncogene Proteins, CEBPA, Gene expression, medicine, Humans, Actin-binding protein, Gene, 030304 developmental biology, Regulation of gene expression, 0303 health sciences, Mutation, SPI1, biology, Gene Expression Regulation, Leukemic, Binding protein, Microfilament Proteins, Hematology, Leukemia, Myeloid, Acute, biology.protein, Cancer research, CCAAT-Enhancer-Binding Proteins, Trans-Activators, 030215 immunology

Published

2013

19. Activated tumor cell integrin αvβ3 cooperates with platelets to promote extravasation and metastasis from the blood stream

Author

Patrizia Marchese, Andries Zijlstra, Brunhilde H. Felding, Joseph S. Krueger, Karin Staflin, Masahiko Zuka, Mario P. Tschan, Martin R. Weber, Zaverio M. Ruggeri, James P. Quigley, Mihaela Lorger, Brian P. Eliceiri, and Bruce E. Torbett

Subjects

0301 basic medicine, Blood Platelets, Platelets, Pathology, medicine.medical_specialty, Integrin, Clinical Sciences, Mice, SCID, Biology, SCID, Neoplastic Cells, Article, Integrin activation, Collagen receptor, Metastasis, Cell Line, 03 medical and health sciences, Mice, 0302 clinical medicine, Rare Diseases, Cell Movement, Cell Line, Tumor, medicine, Circulating, Bioluminescence imaging, Animals, Humans, 2.1 Biological and endogenous factors, Neoplasm Metastasis, Aetiology, Receptor, Cancer, Integrin alphaVbeta3, Tumor, Hematology, medicine.disease, Neoplastic Cells, Circulating, Extravasation, 030104 developmental biology, Cardiovascular System & Hematology, 030220 oncology & carcinogenesis, Cancer research, biology.protein, 570 Life sciences, biology, Blood stream

Abstract

Metastasis is the main cause of death in cancer patients, and understanding mechanisms that control tumor cell dissemination may lead to improved therapy. Tumor cell adhesion receptors contribute to cancer spreading. We noted earlier that tumor cells can expressing the adhesion receptor integrin αvβ3 in distinct states of activation, and found that cells which metastasize from the blood stream express it in a constitutively high affinity form. Here, we analyzed steps of the metastatic cascade in vivo and asked, when and how the affinity state of integrin αvβ3 confers a critical advantage to cancer spreading. Following tumor cells by real time PCR, non-invasive bioluminescence imaging, intravital microscopy and histology allowed us to identify tumor cell extravasation from the blood stream as a rate-limiting step supported by high affinity αvβ3. Successful transendothelial migration depended on cooperation between tumor cells and platelets involving the high affinity tumor cell integrin and release of platelet granules. Thus, this study identifies the high affinity conformer of integrin αvβ3 and its interaction with platelets as critical for early steps during hematogenous metastasis and target for prevention of metastatic disease.

Published

2016

20. Zinc-finger Nuclease Editing of Human cxcr4 Promotes HIV-1 CD4+ T Cell Resistance and Enrichment

Author

Kenneth Kim, Colleen Fearns, Philip D. Gregory, Jinyun Yuan, Kevin Hua, Bruce E. Torbett, Karen Crain, Michael C. Holmes, and Jianbin Wang

Subjects

CD4-Positive T-Lymphocytes, Receptors, CXCR4, Biology, Peripheral blood mononuclear cell, CXCR4, Adenoviridae, Mice, Interleukin 21, Viral entry, Drug Discovery, Genetics, Animals, Humans, Cytotoxic T cell, IL-2 receptor, RNA, Small Interfering, Antigen-presenting cell, Molecular Biology, Cells, Cultured, Pharmacology, fungi, Zinc Fingers, Endonucleases, Zinc finger nuclease, Molecular biology, HIV-1, Molecular Medicine, Original Article

Abstract

HIV-1-infected individuals can harbor viral isolates that can use CCR5, as well as CXCR4, for viral entry. To genetically engineer HIV-1 resistance in CD4(+) T cells, we assessed whether transient, adenovirus delivered zinc-finger nuclease (ZFN) disruption of genomic cxcr4 or stable lentiviral expression of short hairpin RNAs (shRNAs) targeting CXCR4 mRNAs provides durable resistance to HIV-1 challenge. ZFN-modification of cxcr4 in CD4(+) T cells was found to be superior to cell integrated lentivirus-expressing CXCR4 targeting shRNAs when CD4(+) T cells were challenged with HIV-1s that utilizes CXCR4 for entry. Cxcr4 disruption in CD4(+) T cells was found to be stable, conferred resistance, and provided for continued cell enrichment during HIV-1 infection in tissue culture and, in vivo, in peripheral blood mononuclear cell transplanted NSG mice. Moreover, HIV-1-infected mice with engrafted cxcr4 ZFN-modified CD4(+) T cells demonstrated lower viral levels in contrast to mice engrafted with unmodified CD4(+) T cells. These findings provide evidence that ZFN-mediated disruption of cxcr4 provides a selective advantage to CD4(+) T cells during HIV-1 infection.

Published

2012

21. Transcriptional regulation of MIR29B by PU.1 (SPI1) and MYC during neutrophil differentiation of acute promyelocytic leukaemia cells

Author

Jasmin Batliner, Elena A. Federzoni, Bruce E. Torbett, Martin F. Fey, Andreas Tobler, Mario P. Tschan, Emanuel Buehrer, and Mathias Jenal

Subjects

0303 health sciences, SPI1, Cellular differentiation, Hematology, Biology, medicine.disease, 03 medical and health sciences, Promyelocytic leukemia protein, Leukemia, 0302 clinical medicine, Transcription (biology), Neutrophil differentiation, Cell culture, 030220 oncology & carcinogenesis, Cancer research, biology.protein, Transcriptional regulation, medicine, 030304 developmental biology

Published

2011

22. The anti-apoptotic gene BCL2A1 is a novel transcriptional target of PU.1

Author

Mathias Jenal, Jasmin Batliner, Andreas Tobler, Venkateshwar A. Reddy, Mario P. Tschan, Bruce E. Torbett, Torsten Haferlach, and Martin F. Fey

Subjects

Chromatin Immunoprecipitation, Cancer Research, Transcription, Genetic, Neutrophils, Apoptotic gene, Blotting, Western, Antigens, CD34, Antineoplastic Agents, Tretinoin, Biology, Minor Histocompatibility Antigens, 03 medical and health sciences, 0302 clinical medicine, Text mining, Proto-Oncogene Proteins, Granulocyte macrophage colony-stimulating factor receptor, Tumor Cells, Cultured, Humans, RNA, Messenger, Promoter Regions, Genetic, 030304 developmental biology, 0303 health sciences, Reverse Transcriptase Polymerase Chain Reaction, business.industry, Cell Differentiation, Hematology, Hematopoietic Stem Cells, Molecular biology, Leukemia, Myeloid, Acute, Proto-Oncogene Proteins c-bcl-2, Oncology, 030220 oncology & carcinogenesis, Trans-Activators, Cancer research, BCL2-related protein A1, business, Granulocyte colony-stimulating factor receptor, Granulocytes

Published

2010

23. A Copper(I)-Catalyzed 1,2,3-Triazole Azide−Alkyne Click Compound Is a Potent Inhibitor of a Multidrug-Resistant HIV-1 Protease Variant

Author

Michael J. Giffin, John H. Elder, Ying-Chuan Lin, H. Heaslet, Chi-Huey Wong, Bruce E. Torbett, Ashraf Brik, C. David Stout, Gabrielle Cauvi, and Duncan E. McRee

Subjects

Models, Molecular, Azides, 1,2,3-Triazole, Stereochemistry, medicine.medical_treatment, Alkenes, Crystallography, X-Ray, Virus Replication, Article, Catalysis, Cell Line, chemistry.chemical_compound, Drug Resistance, Multiple, Viral, HIV Protease, HIV-1 protease, Drug Discovery, medicine, Protease inhibitor (pharmacology), Protease, Molecular Structure, biology, virus diseases, HIV Protease Inhibitors, Triazoles, Isoenzymes, Multiple drug resistance, Biochemistry, chemistry, Enzyme inhibitor, biology.protein, Click chemistry, Molecular Medicine, Azide, Copper, Protein Binding

Abstract

Treatment with HIV-1 protease inhibitors, a component of highly active antiretroviral therapy (HAART), often results in viral resistance. Structural and biochemical characterization of a 6X protease mutant arising from in vitro selection with compound 1, a C 2-symmetric diol protease inhibitor, has been previously described. We now show that compound 2, a copper(I)-catalyzed 1,2,3-triazole derived compound previously shown to be potently effective against wild-type protease (IC 50 = 6.0 nM), has low nM activity (IC 50 = 15.7 nM) against the multidrug-resistant 6X protease mutant. Compound 2 displays similar efficacy against wild-type and 6X HIV-1 in viral replication assays. While structural studies of compound 1 bound to wild type and mutant proteases revealed a progressive change in binding mode in the mutants, the 1.3 A resolution 6X protease-compound 2 crystal structure reveals nearly identical interactions for 2 as in the wild-type protease complex with very little change in compound 2 or protease conformation.

Published

2008

24. Attenuation of EPO-dependent erythroblast formation by death-associated protein kinase-2

Author

Madhu P. Menon, Leif Oxburgh, Jing Fang, Estelle Houde, Bruce E. Torbett, Mario P. Tschan, Diya Zhang, and Don M. Wojchowski

Subjects

Anemia, Hemolytic, Erythroblasts, Red Cells, Immunology, Mice, Transgenic, Biology, Biochemistry, Mice, Reticulocyte, Erythroblast, medicine, Animals, Cell Lineage, Erythropoiesis, Phosphorylation, Kinase activity, Erythropoietin, Hemostasis, Kinase, Cell Biology, Hematology, Up-Regulation, Death-Associated Protein Kinases, Red blood cell, Haematopoiesis, medicine.anatomical_structure, Calcium-Calmodulin-Dependent Protein Kinases, Cancer research, Apoptosis Regulatory Proteins, Spleen, medicine.drug

Abstract

The adult erythron is maintained via dynamic modulation of erythroblast survival potentials. Toward identifying novel regulators of this process, murine splenic erythroblasts at 3 developmental stages were prepared, purified and profiled. Stage-to-stage modulated genes were then functionally categorized, with a focus on apoptotic factors. In parallel with BCL-X and NIX, death-associated protein kinase-2 (DAPK2) was substantially up-modulated during late erythropoiesis. Among hematopoietic lineages, DAPK2 was expressed predominantly in erythroid cells. In a Gata1-IE3.9int-DAPK2 transgenic mouse model, effects on steady-state reticulocyte and red blood cell (RBC) levels were limited. During hemolytic anemia, however, erythropoiesis was markedly deficient. Ex vivo ana-lyses revealed heightened apoptosis due to DAPK2 at a Kit−CD71highTer119− stage, together with a subsequent multifold defect in late-stage Kit−CD71highTer119+ cell formation. In UT7epo cells, siRNA knock-down of DAPK2 enhanced survival due to cytokine withdrawal, and DAPK2's phosphorylation and kinase activity also were erythropoietin (EPO)-modulated. DAPK2 therefore comprises a new candidate attenuator of stress erythropoiesis.

Published

2008

25. Modulation of drug resistance by artificial transcription factors

Author

Daniel Guthy, Pilar Blancafort, Sharon Bergquist, Bruce E. Torbett, Arndt Brachat, Dennis A Sheeter, Dirk Erdmann, Mario P. Tschan, and Carlos F. Barbas

Subjects

Zinc finger, Cancer Research, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, Kinase, Drug resistance, Biology, Pharmacology, Oncology, Drug Resistance, Neoplasm, Cell culture, Cancer cell, Cancer research, medicine, Humans, Transcription factor, Gene, Etoposide, DNA Primers, HeLa Cells, Transcription Factors, medicine.drug

Abstract

The efficiency of chemotherapeutic treatments in cancer patients is often impaired by the acquisition of drug resistance. Cancer cells develop drug resistance through dysregulation of one or more genes or cellular pathways. To isolate efficient regulators of drug resistance in tumor cells, we have adopted a genome-wide scanning approach based on the screening of large libraries of artificial transcription factors (ATFs) made of three and six randomly assembled zinc finger domains. Zinc finger libraries were linked to a VP64 activation domain and delivered into a paclitaxel-sensitive tumor cell line. Following drug treatment, several ATFs were isolated that promoted drug resistance. One of these ATFs, 3ZF-1-VP, promoted paclitaxel resistance in cell lines having mutated or inactivated p53, such as MDA-MB-435 and Kaposi's sarcoma cell lines. 3ZF-1-VP also induced strong resistance to etoposide, vincristine, and cisplatinum. Linkage of a repression domain to the selected ATF resulted in enhanced sensitivity to multiple drugs, particularly vincristine, cisplatinum, and 5-fluorouracil. Small interfering RNA–mediated inhibition of p53 revealed that 3ZF-1-VP activated both p53-dependent and p53-independent mechanisms to promote survival, whereas other ATF required intact p53. Real-time expression analysis and DNA microarrays showed that several ATFs up-regulated targets of p53, such as the cyclin-dependent kinase inhibitor p21WAF1/CIP1, and genes participating in the p14ARF-MDM2-p53 tumor suppressor pathway, such as hDMP1. Thus, ATF can be used to map genes and pathways involved in drug resistance phenotypes and have potential as novel therapeutic agents to inhibit drug resistance. [Mol Cancer Ther 2008;7(3):688–97]

Published

2008

26. The RNA binding proteins RBM38 and DND1 are repressed in AML and have a novel function in APL differentiation

Author

Bruce E. Torbett, Julian Wampfler, Martin F. Fey, Elena A. Federzoni, and Mario P. Tschan

Subjects

0301 basic medicine, Adult, Male, Cancer Research, Adolescent, Neutrophils, Cellular differentiation, Blotting, Western, RNA-binding protein, Biology, Real-Time Polymerase Chain Reaction, Small hairpin RNA, 03 medical and health sciences, Young Adult, 0302 clinical medicine, Leukemia, Promyelocytic, Acute, Neutrophil differentiation, microRNA, Humans, Aged, Messenger RNA, Gene knockdown, Gene Expression Regulation, Leukemic, RNA-Binding Proteins, Cell Differentiation, Hematology, Middle Aged, Molecular biology, Neoplasm Proteins, Leukemia, Myeloid, Acute, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Gene Knockdown Techniques, Female, Granulocyte colony-stimulating factor receptor

Abstract

The RNA binding proteins RBM binding motif protein 38 (RBM38) and DEAD END 1 (DND1) selectively stabilize mRNAs by attenuating RNAse activity or protecting them from micro(mi)RNA-mediated cleavage. Furthermore, both proteins can efficiently stabilize the mRNA of the cell cycle inhibitor p21(CIP1). Since acute myeloid leukemia (AML) differentiation requires cell cycle arrest and RBM38 as well as DND1 have antiproliferative functions, we hypothesized that decreased RBM38 and DND1 expression may contribute to the differentiation block seen in this disease. We first quantified RBM38 and DND1 mRNA expression in clinical AML patient samples and CD34(+) progenitor cells and mature granulocytes from healthy donors. We found significantly lower RBM38 and DND1 mRNA levels in AML blasts and CD34(+) progenitor cells as compared to mature neutrophils from healthy donors. Furthermore, the lowest expression of both RBM38 and DND1 mRNA correlated with t(8;21). In addition, neutrophil differentiation of CD34(+) cells in vitro with G-CSF (granulocyte colony stimulating factor) resulted in a significant increase of RBM38 and DND1 mRNA levels. Similarly, neutrophil differentiation of NB4 acute promyelocytic leukemia (APL) cells was associated with a significant induction of RBM38 and DND1 expression. To address the function of RBM38 and DND1 in neutrophil differentiation, we generated two independent NB4RBM38 as well as DND1 knockdown cell lines. Inhibition of both RBM38 and DND1 mRNA significantly attenuated NB4 differentiation and resulted in decreased p21(CIP1) mRNA expression. Our results clearly indicate that expression of the RNA binding proteins RBM38 and DND1 is repressed in primary AML patients, that neutrophil differentiation is dependent on increased expression of both proteins, and that these proteins have a critical role in regulating p21(CIP1) expression during APL differentiation.

Published

2015

27. CCR5 Disruption in Induced Pluripotent Stem Cells Using CRISPR/Cas9 Provides Selective Resistance of Immune Cells to CCR5-tropic HIV-1 Virus

Author

Walatta-Tseyon Mesquitta, Petra Minder, Mi Ae Park, HyunJun Kang, Igor I. Slukvin, and Bruce E. Torbett

Subjects

viruses, Biology, 03 medical and health sciences, 0302 clinical medicine, Genome editing, hematopoietic cells, Drug Discovery, CRISPR, Guide RNA, Induced pluripotent stem cell, CRISPR/Cas9, 030304 developmental biology, 0303 health sciences, Cas9, induced pluripotent stemcells, lcsh:RM1-950, HIV, virus diseases, Cell sorting, Virology, 3. Good health, Haematopoiesis, lcsh:Therapeutics. Pharmacology, Viral replication, 030220 oncology & carcinogenesis, Molecular Medicine, CCR5

Abstract

The chemokine (C-C motif) receptor 5 (CCR5) serves as an HIV-1 co-receptor and is essential for cell infection with CCR5-tropic viruses. Loss of functional receptor protects against HIV infection. Here, we report the successful targeting of CCR5 in GFP-marked human induced pluripotent stem cells (iPSCs) using CRISPR/Cas9 with single and dual guide RNAs (gRNAs). Following CRISPER/Cas9-mediated gene editing using a single gRNA, 12.5% of cell colonies demonstrated CCR5 editing, of which 22.2% showed biallelic editing as determined by a Surveyor nuclease assay and direct sequencing. The use of dual gRNAs significantly increased the efficacy of CCR5 editing to 27% with a biallelic gene alteration frequency of 41%. To ensure the homogeneity of gene editing within cells, we used single cell sorting to establish clonal iPSC lines. Single cell-derived iPSC lines with homozygous CCR5 mutations displayed the typical characteristics of pluripotent stem cells and differentiated efficiently into hematopoietic cells, including macrophages. Although macrophages from both wild-type and CCR5-edited iPSCs supported CXCR4-tropic virus replication, macrophages from CCR5-edited iPSCs were uniquely resistant to CCR5-tropic virus challenge. This study demonstrates the feasibility of applying iPSC technology for the study of the role of CCR5 in HIV infection in vitro, and generation of HIV-resistant cells for potential therapeutic applications.

Published

2015

28. ASGCT and JSGT Joint Position Statement on Human Genomic Editing

Author

Yasufumi Kaneda, Michel Sadelain, Theodore Friedmann, Bruce E. Torbett, Erica C. Jonlin, Nancy M. P. King, and Nelson A. Wivel

Subjects

Value (ethics), Position statement, Cognitive science, Pharmacology, Genome, Human, Zygote, Genetic Diseases, Inborn, Genetic Therapy, Genomics, Biology, Bioinformatics, United States, Human disease, Genome editing, Japan, Drug Discovery, Ethical concerns, Genetics, Commentary, Molecular Medicine, Humans, Ethics, Medical, Molecular Biology, Embryonic Stem Cells, Societies, Medical

Abstract

The American Society for Gene and Cell Therapy (ASGCT) and the Japan Society of Gene Therapy (JSGT) (collectively, “Our Societies”) recognize the great scientific advancement represented by the techniques of genome editing and their vast potential value for an improved understanding and possible treatment of human disease. These techniques provide uniquely powerful tools for generating models of human disease, for characterizing the molecular and biochemical basis for pathogenesis, and for suggesting approaches to definitive correction of genetic defects underlying much of human disease. However, our Societies also recognize that the application of genome editing under some circumstances poses very serious ethical problems for which there is no scientific or general societal consensus and that should be considered as inappropriate human genetic manipulation until and unless serious scientific and ethical concerns can be resolved.

Published

2015

29. Role of the mammalian target of rapamycin pathway in lentiviral vector transduction of hematopoietic stem cells

Author

Cathy Wang and Bruce E. Torbett

Subjects

Genetic Vectors, Gene delivery, Biology, Article, Viral vector, Transduction (genetics), Mice, Transduction, Genetic, medicine, Animals, Humans, PI3K/AKT/mTOR pathway, Regulation of gene expression, Sirolimus, TOR Serine-Threonine Kinases, Lentivirus, Hematopoietic Stem Cell Transplantation, Hematopoietic stem cell, hemic and immune systems, Hematology, Genetic Therapy, Hematopoietic Stem Cells, Molecular biology, Endocytosis, Cell biology, medicine.anatomical_structure, Gene Expression Regulation, Stem cell, Signal transduction, Signal Transduction

Abstract

Purpose of review A major goal in repopulating hematopoietic stem cell (HSC) gene therapies is achieving high-efficacy gene transfer, while maintaining robust HSC engraftment and differentiation in vivo. Recent studies have documented that rapamycin treatment of HSC during lentiviral vector transduction enhances gene transfer to human and mouse HSCs and maintains engraftment capacity. In this review, we place into context the role of mammalian target of rapamycin (mTOR) pathways in HSC quiescence and function, endocytic regulation, and lentiviral gene delivery. Recent findings Lentiviral vector transduction of human and mouse HSCs is considerably enhanced by rapamycin treatment. Furthermore, rapamycin preserves long-term engraftment of human and mouse HSCs. Investigations of cellular mechanisms that contribute to increased transduction in HSCs uncover a role for mTOR inhibition-dependent activation of endocytosis. Summary Rapamycin enhances lentiviral vector transduction of HSCs through regulation of endocytic activity via mTOR inhibition. An important attribute of rapamycin treatment during transduction is the preservation of HSC function, allowing reconstitution of long-term hematopoiesis in vivo in murine models.

Published

2015

30. Deep sequencing of protease inhibitor resistant HIV patient isolates reveals patterns of correlated mutations in Gag and protease

Author

Glenn Oliveira, William F. Flynn, Jason F. Okulicz, Jinyun Yuan, Ronald M. Levy, Max W. Chang, Bruce E. Torbett, and Zhiqiang Tan

Subjects

Proteases, medicine.medical_treatment, viruses, HIV Infections, Biology, medicine.disease_cause, gag Gene Products, Human Immunodeficiency Virus, Deep sequencing, 03 medical and health sciences, Cellular and Molecular Neuroscience, HIV Protease, Drug Resistance, Viral, Genetics, medicine, HIV Protease Inhibitor, Humans, Protease inhibitor (pharmacology), Molecular Biology, lcsh:QH301-705.5, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, 0303 health sciences, Mutation, Protease, Ecology, 030306 microbiology, Computational Biology, High-Throughput Nucleotide Sequencing, HIV Protease Inhibitors, Group-specific antigen, Virology, 3. Good health, Computational Theory and Mathematics, Capsid, lcsh:Biology (General), Modeling and Simulation, HIV-1, Research Article

Abstract

While the role of drug resistance mutations in HIV protease has been studied comprehensively, mutations in its substrate, Gag, have not been extensively cataloged. Using deep sequencing, we analyzed a unique collection of longitudinal viral samples from 93 patients who have been treated with therapies containing protease inhibitors (PIs). Due to the high sequence coverage within each sample, the frequencies of mutations at individual positions were calculated with high precision. We used this information to characterize the variability in the Gag polyprotein and its effects on PI-therapy outcomes. To examine covariation of mutations between two different sites using deep sequencing data, we developed an approach to estimate the tight bounds on the two-site bivariate probabilities in each viral sample, and the mutual information between pairs of positions based on all the bounds. Utilizing the new methodology we found that mutations in the matrix and p6 proteins contribute to continued therapy failure and have a major role in the network of strongly correlated mutations in the Gag polyprotein, as well as between Gag and protease. Although covariation is not direct evidence of structural propensities, we found the strongest correlations between residues on capsid and matrix of the same Gag protein were often due to structural proximity. This suggests that some of the strongest inter-protein Gag correlations are the result of structural proximity. Moreover, the strong covariation between residues in matrix and capsid at the N-terminus with p1 and p6 at the C-terminus is consistent with residue-residue contacts between these proteins at some point in the viral life cycle., Author Summary Understanding the structure of HIV proteins and the function of drug-resistant mutations of these proteins is critical for the development of effective HIV treatments. Selected gag mutations have been shown to provide compensatory functions for protease resistance mutations and may directly contribute to the development of drug resistance. To determine associations between protease inhibitor mutations and gag, we utilized deep sequencing of HIV gag and protease from a collection of viral isolates from patients treated with highly active retroviral protease inhibitors. Deep sequencing allows for accurate measurement of mutation frequencies at each position, allowing estimation, using a novel method we developed, of the covariation between any two residues on gag. Using this information, we characterize the variation within gag and protease and identify the most strongly correlated pairs of inter- and intra-protein residues. Our results suggest that matrix and p1/p6 mutations form the core of a network of strongly correlated gag mutations and contribute to recurrent treatment failure. Extracting gag residue covariation information from the deep sequencing of patient viral samples may provide insight into structural aspects of the Gag polyprotein as well new areas for small molecule targeting to disrupt Gag function.

Published

2015

31. T-cell protection and enrichment through lentiviral CCR5 intrabody gene delivery

Author

Christina H. Swan, Bruce E. Torbett, Bernd Bühler, Mario P. Tschan, and Carlos F. Barbas

Subjects

CD4-Positive T-Lymphocytes, Chemokine, Receptors, CCR5, T cell, Genetic enhancement, HIV Infections, Mice, SCID, Gene delivery, Antibodies, Intrabody, Cell Line, Mice, Genetics, medicine, Animals, Humans, Molecular Biology, Cells, Cultured, biology, virus diseases, Dendritic Cells, Genetic Therapy, T lymphocyte, Molecular biology, medicine.anatomical_structure, Gene Expression Regulation, Cytoprotection, HIV-1, biology.protein, Molecular Medicine, Antibody, CD8

Abstract

CCR5 is the chemokine co-receptor for R5-tropic human immunodeficiency virus type 1 (HIV-1) isolates most often associated with primary infection. We have developed an HIV-1 self-inactivating vector, CAD-R5, containing a CCR5 single-chain antibody (intrabody) gene, which when expressed in T-cell lines and primary CD4+ T cells disrupts CCR5 cell surface expression and provides protection from R5-tropic isolate exposure. Furthermore, CAD-R5 intrabody expression in primary CD4+ T cells supports significant growth and enrichment over time during HIV-1-pulsed dendritic cell-T-cell interactions. These results indicate that CCR5 intrabody-expressing CD4+ T cells are refractory against this highly efficient primary route of infection. CD34+ cells transduced with the CAD-R5 vector gave rise to CD4+ and CD8+ thymocytes in non-obese diabetic (NOD)/ severely combined-immunodeficient (SCID)-human thymus/liver (hu thy/liv) mice, suggesting that CCR5 intrabody expression can be maintained throughout differentiation without obvious cellular effects. CD4+ T cells isolated from NOD/SCID-hu thy/liv mice were resistant to R5-tropic HIV-1 challenge demonstrating the maintenance of protection. Our findings demonstrate delivery of anti-HIV-1 activity through CCR5 intrabodies in primary CD4+ T cells and CD34+ cell-derived T-cell progeny. Thus, gene delivery strategies that provide a selective survival and growth advantage for T effector cells may provide a therapeutic benefit for HIV-1-infected individuals who have failed conventional therapies.

Published

2006

32. The Class I HLA Repertoire of Pancreatic Islets Comprises the Nonclassical Class Ib Antigen HLA-G

Author

Michael T. McMaster, Jessie Zalatan, Bruce E. Torbett, Paolo Meda, Daniel R. Salomon, Laura Crisa, Vincenzo Cirulli, Camillo Ricordi, and Robyn C. Prinsen

Subjects

Transcription, Genetic, Endocrinology, Diabetes and Metabolism, Enteroendocrine cell, Human leukocyte antigen, Biology, Major histocompatibility complex, medicine.disease_cause, Polymerase Chain Reaction, Autoimmunity, Islets of Langerhans, Antigen, HLA Antigens, HLA-G, Insulin Secretion, Internal Medicine, medicine, Humans, Insulin, Cloning, Molecular, Cells, Cultured, DNA Primers, HLA-G Antigens, Base Sequence, HLA-A Antigens, Pancreatic islets, Histocompatibility Antigens Class I, Glucagon, Cell biology, medicine.anatomical_structure, HLA-B Antigens, Immunology, biology.protein, Cell Division

Abstract

Selective expression of the human class Ib HLA molecule HLA-G in immunologically protected sites and its function in the inhibition of NK and T-cell effector functions support an important role of this molecule in immunoregulation. Here, we demonstrate that HLA-G is constitutively expressed in the endocrine compartment of the human pancreas. Surface expression of this HLA determinant in endocrine cells is regulated in response to growth and inflammatory stimuli. Furthermore, we provide evidence that HLA-G expressed in this tissue may associate with a subset of insulin-containing granules and may be shuttled to the cell surface in response to secretory stimuli. Thus, HLA-G presentation by endocrine cells may be regulated in concert with their secretory activity. These results identify the expression of a major histocompatibility complex locus with putative regulatory functions in human pancreatic islets, a finding with potentially important implications for the progression of autoimmunity as well as for the establishment of transplant tolerance to this tissue.

Published

2006

33. Structural Insights into the Mechanisms of Drug Resistance in HIV-1 Protease NL4-3

Author

Ying-Chuan Lin, John H. Elder, H. Heaslet, Garrett M. Morris, Bruce E. Torbett, Victoria D Kutilek, and C. David Stout

Subjects

medicine.medical_treatment, Molecular Sequence Data, Mutant, Drug resistance, Crystallography, X-Ray, Virus, Evolution, Molecular, Drug Resistance, Multiple, Viral, HIV Protease, HIV-1 protease, Structural Biology, medicine, Humans, Point Mutation, Protease inhibitor (pharmacology), Protein Structure, Quaternary, Molecular Biology, chemistry.chemical_classification, Protease, Molecular Structure, biology, virus diseases, HIV Protease Inhibitors, Virology, NS2-3 protease, Enzyme, chemistry, Biochemistry, HIV-1, biology.protein, Dimerization, Protein Binding

Abstract

The development of resistance to anti-retroviral drugs targeted against HIV is an increasing clinical problem in the treatment of HIV-1-infected individuals. Many patients develop drug-resistant strains of the virus after treatment with inhibitor cocktails (HAART therapy), which include multiple protease inhibitors. Therefore, it is imperative that we understand the mechanisms by which the viral proteins, in particular HIV-1 protease, develop resistance. We have determined the three-dimensional structure of HIV-1 protease NL4-3 in complex with the potent protease inhibitor TL-3 at 2.0 A resolution. We have also obtained the crystal structures of three mutant forms of NL4-3 protease containing one (V82A), three (V82A, M46I, F53L) and six (V82A, M46I, F53L, V77I, L24I, L63P) point mutations in complex with TL-3. The three protease mutants arose sequentially under ex vivo selective pressure in the presence of TL-3, and exhibit fourfold, 11-fold, and 30-fold resistance to TL-3, respectively. This series of protease crystal structures offers insights into the biochemical and structural mechanisms by which the enzyme can overcome inhibition by TL-3 while recovering some of its native catalytic activity.

Published

2006

34. The role of angiopoietins in the development of endothelial cells from cord blood CD34+ progenitors

Author

Robyn C. Prinsen, Kent A. Smith, Daniel R. Salomon, Laura Crisa, Bruce E. Torbett, Patrick Hildbrand, and Vincenzo Cirulli

Subjects

DNA, Complementary, Endothelium, Angiogenesis, Blotting, Western, Immunology, Antigens, CD34, Biology, Biochemistry, Angiopoietin-2, Neovascularization, Vasculogenesis, Angiopoietin-1, medicine, Humans, Cells, Cultured, CD11b Antigen, Microscopy, Confocal, Neovascularization, Pathologic, Reverse Transcriptase Polymerase Chain Reaction, Stem Cells, Endothelial Cells, Cell Differentiation, Angiopoietins, Cell Biology, Hematology, Fetal Blood, Flow Cytometry, Up-Regulation, Cell biology, Vascular endothelial growth factor B, Endothelial stem cell, Drug Combinations, medicine.anatomical_structure, Cord blood, Proteoglycans, Collagen, Endothelium, Vascular, Laminin, medicine.symptom, Cell Division

Abstract

Circulating endothelial progenitors contribute to neovascularization at sites of injury and tumorigenesis in postnatal life. Yet, the molecular mechanisms initiating the endothelial developmental program of these precursors remain elusive. Here we provide evidence that endothelial development from progenitors circulating in human cord blood requires angiopoietins, a set of growth factors also involved in vascular branching during embryogenesis. We show that cord blood cells with the potential for endothelial development reside in a CD34+CD11b+ subset capable of autonomously producing and binding angiopoietins. Functionally, endogenous angiopoietin-1 regulates initial endothelial cell commitment, whereas angiopoietin-2 enhances expansion of the endothelial cell progeny. These findings suggest a role for angiopoietins as regulators of endothelial development from circulating progenitors and imply a function of angiopoietins at distinct developmental steps in postnatal angiogenesis.

Published

2004

35. 4. β-Deliverin: A Small Molecule for Improving Gene Transfer to Hematopoietic Stem Cells and Probing Mechanisms of Lentiviral Vector Restriction

Author

Scott A. Snyder, Saritha S. D'Souza, Nina D. Timberlake, Sergio D. Catz, Igor I. Slukvin, Bruce E. Torbett, and Stosh Ozog

Subjects

0301 basic medicine, Pharmacology, LAMP1, Endosome, Genetic enhancement, Biology, Gene delivery, Viral vector, Cell biology, 03 medical and health sciences, Haematopoiesis, Transduction (genetics), 030104 developmental biology, Drug Discovery, Immunology, Genetics, Molecular Medicine, Stem cell, Molecular Biology

Abstract

A major obstacle to the success of gene therapy for hematologic disorders is the inefficiency of lentiviral vector (LV) gene transfer to hematopoietic stem cells (HSCs). Achieving clinically relevant gene delivery levels requires prolonged ex vivo culture of HSCs with cytokines and large LV doses. Rapamycin, PGE2, and other small molecules, have been reported to increase LV transduction of HSCs, however the mechanism of action of these drugs and the basis for LV restriction in HSCs are poorly understood.Here, we report a novel small molecule, β-deliverin, which improves LV gene transfer to HSCs up to 3 fold over DMSO control in vitro. This effect is most pronounced in human adult peripheral blood-derived HSCs, but also observed in human cord-derived HSCs, and in non-human primate bone marrow-derived HSCs. Importantly, treatment with β-deliverin does not significantly affect the viability or expansion of HSCs in culture. Furthermore, for cord-derived HSCs, there was no reduction in the number or type of colony-forming cells. In vivo, β-deliverin treated HSCs engraft in the peripheral blood of NSG mice at levels comparable to control at 16 weeks post-engraftment. Despite an only modest increase in transduction efficiency in β-deliverin-treated cord-derived HSCs transduced in vitro (26% versus 20% for control), the marking frequency for control cells dropped to

Published

2016

36. Regulation of neutrophil and eosinophil secondary granule gene expression by transcription factors C/EBPε and PU.1

Author

H. Phillip Koeffler, Scott H. Kwok, Karen L. Anderson, Yuji Yamaguchi, Adrian F. Gombart, and Bruce E. Torbett

Subjects

CCAAT-Enhancer-Binding Protein-delta, Transcription, Genetic, Neutrophils, Regulatory Sequences, Nucleic Acid, Biochemistry, Mice, Gene expression, GATA1 Transcription Factor, Mice, Knockout, Oncogene Proteins, biology, Ccaat-enhancer-binding proteins, 3T3 Cells, Blood Proteins, Hematology, Eosinophil Granule Proteins, Lipocalins, DNA-Binding Proteins, medicine.anatomical_structure, Peroxidases, Gelatinases, Major basic protein, Erythroid-Specific DNA-Binding Factors, Tertiary granule, Eosinophil peroxidase, Eosinophil Peroxidase, Recombinant Fusion Proteins, Immunology, Granulocyte, Cytoplasmic Granules, Ribonucleases, Lipocalin-2, Proto-Oncogene Proteins, CCAAT-Enhancer-Binding Protein-alpha, medicine, Animals, Humans, Collagenases, RNA, Messenger, CCAAT-Enhancer-Binding Protein-beta, Neutrophil collagenase, Cell Biology, Molecular biology, Eosinophils, Lactoferrin, Gene Expression Regulation, Specific granule, CCAAT-Enhancer-Binding Proteins, Trans-Activators, biology.protein, Carrier Proteins, Acute-Phase Proteins, Transcription Factors

Abstract

In the bone marrow of C/EBP epsilon(-/-) mice, expression of neutrophil secondary and tertiary granule mRNAs is absent for lactoferrin (LF), neutrophil gelatinase (NG), murine cathelin-like protein (MCLP), and the cathelin B9; it is severely reduced for neutrophil collagenase (NC) and neutrophil gelatinase-associated lipocalin (NGAL). In addition, the expression of eosinophil granule genes, major basic protein (MBP), and eosinophil peroxidase (EPX) is absent. These mice express C/EBP alpha, C/EBP beta, and C/EBP delta in the bone marrow at levels similar to those of their wild-type counterparts, suggesting a lack of functional redundancy among the family in vivo. Stable inducible expression of C/EBP epsilon and C/EBP alpha in the murine fibroblast cell line NIH 3T3 activated expression of mRNAs for B9, MCLP, NC, and NGAL but not for LF. In transient transfections of C/EBP epsilon and C/EBP alpha, B9 was strongly induced with weaker induction of the other genes. C/EBP beta and C/EBP delta proteins weakly induced B9 expression, but C/EBP delta induced NC expression more efficiently than the other C/EBPs. The expression of MBP was inefficiently induced by C/EBP epsilon alone and weakly induced with C/EBP epsilon and GATA-1, but the addition of PU.1 resulted in a striking cooperative induction of MBP in NIH 3T3 cells. Mutation of a predicted PU.1 site in the human MBP promoter-luciferase reporter construct abrogated the response to PU.1. Gel-shift analysis demonstrated binding of PU.1 to this site. MBP and EPX mRNAs were absent in a PU.1-null myeloid cell line established from the embryonic liver of PU.1(-/-) mice. Restitution of PU.1 protein expression restored MBP and EPX protein expression. This study demonstrates that C/EBP epsilon is essential and sufficient for the expression of a particular subset of neutrophil secondary granule genes. Furthermore, it indicates the importance of PU.1 in the cooperative activation of eosinophil granule genes.

Published

2003

37. Nucleocapsid Protein: A Desirable Target for Future Therapies Against HIV-1

Author

Danny Antaki, Sébastien Lyonnais, Gilles Mirambeau, Yves Mély, Bruce E. Torbett, Lesia Kovalenko, Mattia Mori, and Maurizio Botta

Subjects

APOBEC, biology, viruses, virus diseases, Virology, Reverse transcriptase, Long terminal repeat, Nucleic acid secondary structure, chemistry.chemical_compound, Capsid, chemistry, Transfer RNA, biology.protein, Ribonuclease, DNA

Abstract

Open image in new window HIV reverse transcription and nucleocapsid. After the capsid has entered the cell, reverse transcriptase (A) creates a DNA copy (green) of the HIV RNA genome (yellow), using a cellular transfer RNA (B) as a primer. HIV nucleocapsid protein (C) acts as a chaperone to unfold the RNA secondary structure. The ribonuclease activity of RT removes the viral RNA after the DNA strand is created. Interaction of HIV Vif (D) with cellular APOBEC (E) is also shown

Published

2015

38. Combined Antiviral Therapy Using Designed Molecular Scaffolds Targeting Two Distinct Viral Functions, HIV-1 Genome Integration and Capsid Assembly

Author

Sudarat Hadpech, Pierre Boulanger, Koollawat Chupradit, Chatchai Tayapiwatana, Bruce E. Torbett, Wannisa Khamaikawin, Sawitree Nangola, Supachai Sakkhachornphop, Aftab A. Ansari, Siddappa N. Byrareddy, Nattawat Onlamoon, Somphot Saoin, Saw See Hong, Rétrovirus et Pathologie Comparée (RPC), Institut National de la Recherche Agronomique (INRA)-École pratique des hautes études (EPHE), Université Paris sciences et lettres (PSL)-Université Paris sciences et lettres (PSL)-Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Ecole Nationale Vétérinaire de Lyon (ENVL), Thailand Research Fund through the Royal Golden Jubilee Ph.D. program= [PHD/0024/2552], Cluster and Program Management Office (CPMO), National Science and Technology Development Agency (NSTDA), National Research Council of Thailand (NRCT), Health Systems Research Institute (HSRI), National Research University project under the Thailand's Office of the Commission on Higher Education, National Institutes of Health (NIH) [CFAR-P30 AI036214, GM083658, HL091219], Tayapiwatana, Chatchai, Infections Virales et Pathologie Comparée - UMR 754 (IVPC), Institut National de la Recherche Agronomique (INRA)-École pratique des hautes études (EPHE)-Université Claude Bernard Lyon 1 (UCBL), and Université de Lyon-Université de Lyon

Subjects

capside, Genetic enhancement, viruses, [SDV]Life Sciences [q-bio], anti-HIV-1 molecular scaffolds, designed ankyrin repeat proteins, designed zinc-finger proteins, HIV-1-resistant cells, Biology, Viral vector, 03 medical and health sciences, analyse de génome, 0302 clinical medicine, Complementary DNA, Drug Discovery, Vector (molecular biology), sida, Gene, 030304 developmental biology, Zinc finger, 0303 health sciences, lcsh:RM1-950, myr, virus diseases, Virology, antiviral, 3. Good health, lcsh:Therapeutics. Pharmacology, Capsid, SIV, SHIV, 030220 oncology & carcinogenesis, Molecular Medicine, Original Article

Abstract

International audience; Designed molecular scaffolds have been proposed as alternative therapeutic agents against HIV-1. The ankyrin repeat protein (Ank(GAG)1D4) and the zinc finger protein (2LTRZFP) have recently been characterized as intracellular antivirals, but these molecules, used individually, do not completely block HIV-1 replication and propagation. The capsid-binder Ank(GAG)1D4, which inhibits HIV-1 assembly, does not prevent the genome integration of newly incoming viruses. 2LTRZFP, designed to target the 2-LTR-circle junction of HIV-1 cDNA and block HIV-1 integration, would have no antiviral effect on HIV-1-infected cells. However, simultaneous expression of these two molecules should combine the advantage of preventive and curative treatments. To test this hypothesis, the genes encoding the N-myristoylated Myr(+)Ank(GAG)1D4 protein and the 2LTRZFP were introduced into human T-cells, using a third-generation lentiviral vector. SupT1 cells stably expressing 2LTRZFP alone or with Myr(+)Ank(GAG)1D4 showed a complete resistance to HIV-1 in viral challenge. Administration of the Myr(+)Ank(GAG)1D4 vector to HIV-1-preinfected SupT1 cells resulted in a significant antiviral effect. Resistance to viral infection was also observed in primary human CD4+ T-cells stably expressing Myr(+)Ank(GAG)1D4, and challenged with HIV-1, SIVmac, or SHIV. Our data suggest that our two anti-HIV-1 molecular scaffold prototypes are promising antiviral agents for anti-HIV-1 gene therapy.

Published

2015

39. A Chimeric Mouse Model of Gaucher Disease

Author

Ernest Beutler, Carol West, Hiroshi Deguchi, and Bruce E. Torbett

Subjects

Pathology, medicine.medical_specialty, medicine.medical_treatment, Spleen, Hematopoietic stem cell transplantation, Glucocerebroside, Biology, Glucosylceramides, Mice, Genetics, medicine, Animals, Molecular Biology, Genetics (clinical), Mice, Knockout, Gaucher Disease, Chimera, Hematopoietic Stem Cell Transplantation, medicine.disease, Mice, Inbred C57BL, Disease Models, Animal, Haematopoiesis, medicine.anatomical_structure, Gaucher's disease, Liver, Immunology, Knockout mouse, Glucosylceramidase, Molecular Medicine, Female, Stem cell, Glucocerebrosidase, Research Article

Abstract

BACKGROUND: There is a major need for a mouse model of Gaucher disease, but the glucocerebrosidase knockout mouse is not viable; it dies shortly before or immediately after birth, apparently because of involvement of the central nervous system and/or skin. The most common form of Gaucher disease, type I, has a phenotype that is limited to the monocyte-macrophage system. MATERIALS AND METHODS: We have created a chimeric mouse by infusing hematopoietic stem cells from fetuses that are homozygous for the glucocerebrosidase knockout into irradiated mice. RESULTS: The chimeric mice manifested a severe deficiency of glucocerebrosidase activity in peripheral blood cells and spleen indicating a lack of cell-cell correction. Levels of glucocerebroside in spleen and liver are increased, and infusing the mice with exogenous glucocerebroside/albumin particles produced a marked increase in the amount of glucocerebroside stored in liver and spleen. Morphologically identifiable Gaucher cells were not present. CONCLUSIONS: The chimeric model reflects the increased glycolipid storage in the reticuloendothelial system that is characteristic of Gaucher disease, and could be useful as a model for studying treatment of Gaucher disease.

Published

2002

40. Rapamycin relieves lentiviral vector transduction resistance in human and mouse hematopoietic stem cells

Author

David J. Rawlings, Bruce E. Torbett, Xuefeng Wang, Iram F. Khan, Blythe D. Sather, Hans-Peter Kiem, Swati Singh, Amie B. Adams, Cathy Wang, Shanshan Lang, Carol H. Miao, Gabrielle Curinga, and Jennifer E. Adair

Subjects

Genetic enhancement, Immunology, Genetic Vectors, Mice, SCID, Gene delivery, Biology, Biochemistry, Viral vector, Transduction (genetics), Mice, Mice, Inbred NOD, Inside BLOOD Commentary, Transduction, Genetic, Animals, Humans, Sirolimus, TOR Serine-Threonine Kinases, Lentivirus, Hematopoietic Stem Cell Transplantation, hemic and immune systems, Cell Biology, Hematology, Gene Therapy, Virus Internalization, Hematopoietic Stem Cells, Virology, Cell biology, Transplantation, Mice, Inbred C57BL, Haematopoiesis, Heterografts, Stem cell

Abstract

Transplantation of genetically modified hematopoietic stem cells (HSCs) is a promising therapeutic strategy for genetic diseases, HIV, and cancer. However, a barrier for clinical HSC gene therapy is the limited efficiency of gene delivery via lentiviral vectors (LVs) into HSCs. We show here that rapamycin, an allosteric inhibitor of the mammalian target of rapamycin complexes, facilitates highly efficient lentiviral transduction of mouse and human HSCs and dramatically enhances marking frequency in long-term engrafting cells in mice. Mechanistically, rapamycin enhanced postbinding endocytic events, leading to increased levels of LV cytoplasmic entry, reverse transcription, and genomic integration. Despite increasing LV copy number, rapamycin did not significantly alter LV integration site profile or chromosomal distribution in mouse HSCs. Rapamycin also enhanced in situ transduction of mouse HSCs via direct intraosseous infusion. Collectively, rapamycin strongly augments LV transduction of HSCs in vitro and in vivo and may prove useful for therapeutic gene delivery.

Published

2014

41. Safety and efficacy of a tCD25 preselective combination anti-HIV lentiviral vector in human hematopoietic stem and progenitor cells

Author

Joseph S. Anderson, Bruce E. Torbett, Sharlie L. Barclay, Alfonso Barraza, Ryan Fong, Yimin Yang, Jan A. Nolta, Gerhard Bauer, Mehrdad Abedi, and Siruo Zhang

Subjects

Genetic enhancement, Cell, Genetic Vectors, Gene Expression, HIV Infections, Biology, Viral vector, Mice, Mice, Inbred NOD, Transduction, Genetic, medicine, Animals, Humans, IL-2 receptor, Progenitor cell, Mice, Knockout, Lentivirus, Hematopoietic Stem Cell Transplantation, Interleukin-2 Receptor alpha Subunit, virus diseases, Cell Biology, Genetic Therapy, Hematopoietic Stem Cells, Transplantation, Haematopoiesis, medicine.anatomical_structure, Immunology, Molecular Medicine, Stem cell, Developmental Biology

Abstract

The successful suppression of human immunodeficiency virus (HIV) in the “Berlin Patient” has highlighted the ability of HIV-resistant hematopoietic stem cells to offer a potential functional cure for HIV-infected patients. HIV stem cell gene therapy can mimic this result by genetically modifying a patient's own cells with anti-HIV genes. Previous attempts of HIV gene therapy have been hampered by a low percentage of transplanted HIV-resistant cells which has led to minimal clinical efficacy. In our current study, we have evaluated the in vitro and in vivo safety and efficacy of a truncated/mutated form of human CD25 preselective anti-HIV lentiviral vector in human hematopoietic stem cells. This preselective vector allows us to purify vector-transduced cells prior to transplantation so an increased percentage of gene-modified cells can be delivered. Here, we demonstrate the safety of this strategy with successful engraftment and multilineage hematopoiesis of transduced cells in a humanized NOD-RAG1−/−IL-2rγ−/− knockout mouse model. Efficacy was also demonstrated with significant protection from HIV-1 infection including maintenance of human CD4+ cell levels and a decrease in HIV-1 plasma viremia. Collectively, these results establish the utility of this HIV stem cell gene therapy strategy and bring it closer to providing a functional cure for HIV-infected patients. Stem Cells 2015;33:870–879

Published

2014

42. Viral Evolution in Response to the Broad-Based Retroviral Protease Inhibitor TL-3

Author

Arthur J. Olson, Bernd Bühler, Chi-Huey Wong, John H. Elder, Garrett M. Morris, Ying-Chuan Lin, Bruce E. Torbett, and Douglas D. Richman

Subjects

Feline immunodeficiency virus, medicine.medical_treatment, Molecular Sequence Data, Immunology, Genome, Viral, Biology, Microbiology, Virus, Evolution, Molecular, Virology, Vaccines and Antiviral Agents, medicine, Animals, Humans, Protease Inhibitors, Protease inhibitor (pharmacology), Amino Acid Sequence, chemistry.chemical_classification, NS3, Protease, biology.organism_classification, Molecular biology, NS2-3 protease, Retroviridae, Enzyme, chemistry, Insect Science, Cats, MASP1

Abstract

TL-3 is a protease inhibitor developed using the feline immunodeficiency virus protease as a model. It has been shown to efficiently inhibit replication of human, simian, and feline immunodeficiency viruses and therefore has broad-based activity. We now demonstrate that TL-3 efficiently inhibits the replication of 6 of 12 isolates with confirmed resistance mutations to known protease inhibitors. To dissect the spectrum of molecular changes in protease and viral properties associated with resistance to TL-3, a panel of chronological in vitro escape variants was generated. We have virologically and biochemically characterized mutants with one (V82A), three (M46I/F53L/V82A), or six (L24I/M46I/F53L/L63P/V77I/V82A) changes in the protease and structurally modeled the protease mutant containing six changes. Virus containing six changes was found to be 17-fold more resistant to TL-3 in cell culture than was wild-type virus but maintained similar in vitro replication kinetics compared to the wild-type virus. Analyses of enzyme activity of protease variants with one, three, and six changes indicated that these enzymes, compared to wild-type protease, retained 40, 47, and 61% activity, respectively. These results suggest that deficient protease enzymatic activity is sufficient for function, and the observed protease restoration might imply a selective advantage, at least in vitro, for increased protease activity.

Published

2001

43. PU.1 inhibits GATA-1 function and erythroid differentiation by blocking GATA-1 DNA binding

Author

Kent A. Smith, Atsushi Iwama, Xiaobo Zhang, Bruce E. Torbett, Pu Zhang, Salaija Narravula, Beatrice U. Mueller, Channing Yu, Daniel G. Tenen, and Stuart H. Orkin

Subjects

Zinc finger, Erythroid-Specific DNA-Binding Factors, Cellular differentiation, GATA2, Immunology, Transfection, Plasma protein binding, Cell Biology, Hematology, Biology, Fusion protein, Molecular biology, Biochemistry, Transcription factor

Abstract

The lineage-specific transcription factors GATA-1 and PU.1 can physically interact to inhibit each other's function, but the mechanism of repression of GATA-1 function by PU.1 has not been elucidated. Both the N terminus and the C terminus of PU.1 can physically interact with the C-terminal zinc finger of GATA-1. It is demonstrated that the PU.1 N terminus, but not the C terminus, is required for inhibiting GATA-1 function. Induced overexpression of PU.1 in K562 erythroleukemia cells blocks hemin-induced erythroid differentiation. In this system, PU.1 does not affect the expression of GATA-1 messenger RNA, protein, or nuclear localization. However, GATA-1 DNA binding decreases dramatically. By means of electrophoretic mobility shift assays with purified proteins, it is demonstrated that the N-terminal 70 amino acids of PU.1 can specifically block GATA-1 DNA binding. In addition, PU.1 had a similar effect in the G1ER cell line, in which the GATA-1 null erythroid cell line G1E has been transduced with a GATA-1–estrogen receptor fusion gene, which is directly dependent on induction of the GATA-1 fusion protein to effect erythroid maturation. Consistent with in vitro binding assays, overexpression of PU.1 blocked DNA binding of the GATA-1 fusion protein as well as GATA-1–mediated erythroid differentiation of these G1ER cells. These results demonstrate a novel mechanism by which function of a lineage-specific transcription factor is inhibited by another lineage-restricted factor through direct protein–protein interactions. These findings contribute to understanding how protein–protein interactions participate in hematopoietic differentiation and leukemogenesis.

Published

2000

44. Presentation of chemokine SDF-1α by fibronectin mediates directed migration of T cells

Author

Patrick Hildbrand, Luc J. W. van der Laan, Bruce E. Torbett, Michael A. Siani, Anthony J. Pelletier, Philip E. Dawson, Daniel R. Salomon, and Darren A. Thompson

Subjects

Chemokine, Immunology, Cell Biology, Hematology, Biology, Biochemistry, Cell biology, Fibronectin, Chemokine receptor, biology.protein, CXCL9, XCL2, Stromal cell-derived factor 1, CCL25, CXCL16

Abstract

The role of chemokine–matrix interactions in integrin-dependent T-cell migration was examined to address the critical question of how chemokines provide directional information. The chemokine SDF-1α binds fibronectin (Fn) with a low nanomolar Kd(equilibrium dissociation constant). SDF-1α presented by Fn induced directed migration. Spatial concentration gradients of chemokine were not required to maintain directed migration. Fn-presented chemokine induced the polarization of cells, including the redistribution of the SDF-1α receptor, to the basal surface and leading edge of the cell. A new model for directed migration is proposed in which the co-presentation of an adhesive matrix and chemokine provides the necessary positional information independent of a soluble spatial gradient.

Published

2000

45. Infection by porcine endogenous retrovirus after islet xenotransplantation in SCID mice

Author

Chris Lockey, Daniel R. Salomon, Carolyn A. Wilson, Bradley C. Griffeth, Francine S. Frasier, Bruce E. Torbett, Zhifeng Long, Edward Otto, Luc J. W. van der Laan, David Onions, and Bernhard J. Hering

Subjects

Severe combined immunodeficiency, Multidisciplinary, Xenotransplantation, medicine.medical_treatment, Pancreatic islets, Endogenous retrovirus, Biology, medicine.disease, biology.organism_classification, Virology, Transplantation, medicine.anatomical_structure, Retrovirus, Viral replication, Immunology, medicine, Pseudotyping

Abstract

Animal donors such as pigs could provide an alternative source of organs for transplantation. However, the promise of xenotransplantation is offset by the possible public health risk of a cross-species infection. All pigs contain several copies of porcine endogenous retroviruses (PERV), and at least three variants of PERV can infect human cell lines in vitro in co-culture, infectivity and pseudotyping experiments. Thus, if xenotransplantation of pig tissues results in PERV viral replication, there is a risk of spreading and adaptation of this retrovirus to the human host. C-type retroviruses related to PERV are associated with malignancies of haematopoietic lineage cells in their natural hosts. Here we show that pig pancreatic islets produce PERV and can infect human cells in culture. After transplantation into NOD/SCID (non-obese diabetic, severe combined immunodeficiency) mice, we detect ongoing viral expression and several tissue compartments become infected. This is the first evidence that PERV is transcriptionally active and infectious cross-species in vivo after transplantation of pig tissues. These results show that a concern for PERV infection risk associated with pig islet xenotransplantation in immunosuppressed human patients may be justified.

Published

2000

46. Anti-Gag Cytolytic T Lymphocytes Specific for an Alternative Translational Reading Frame-Derived Epitope and Resistance Versus Susceptibility to Retrovirus-Induced Murine AIDS in F1 Mice

Author

Patricia A. Healy, Shawn-Marie Mayrand, William R. Green, and Bruce E. Torbett

Subjects

medicine.drug_class, Amino Acid Motifs, Congenic, Epitopes, T-Lymphocyte, Gene Products, gag, Biology, CD8-Positive T-Lymphocytes, Monoclonal antibody, Epitope, Lymphocyte Depletion, Mice, Retrovirus, Murine Acquired Immunodeficiency Syndrome, T-Lymphocyte Subsets, Virology, MHC class I, Murine leukemia virus, medicine, Animals, Genetic Predisposition to Disease, Crosses, Genetic, Mice, Inbred BALB C, Immunodominant Epitopes, biology.organism_classification, Immunity, Innate, Leukemia Virus, Murine, Mice, Inbred C57BL, CTL, Alternative Splicing, biology.protein, Disease Susceptibility, CD8, T-Lymphocytes, Cytotoxic

Abstract

Murine AIDS (MAIDS) develops in susceptible mouse strains after infection with the LP-BM5 murine leukemia virus complex that contains causative defective, and ecotropic helper, retroviruses. We previously demonstrated that the MAIDS-resistant H-2(d) strains BALB/cByJ and C57BL/KsJ generate MHC class I (K(d)) restricted virus-specific CD8(+) cytolytic T lymphocytes (CTLs) that lyse cells expressing either defective or ecotropic gag proteins. In contrast, the congenic BALB.B and closely related C57BL/6J MAIDS-susceptible H-2(b) strains were unable to serve as a source of gag-specific CTLs (Schwarz and Green, 1994), suggesting that anti-gag CTLs might provide a basis for resistance to MAIDS. Although its susceptibility to MAIDS was unknown, the (BALB/c x C57BL/6J) F(1) (CBY6F(1)) strain could also produce H-2(d)-, but not H-2(b)-, restricted, anti-gag CTLs (Schwarz and Green, 1994). Because of this correlation between anti-gag CTLs and resistance to MAIDS, it was important to provide more direct evidence in support of CTL-mediated protection and to determine both the fine specificity of CByB6F(1) anti-gag CTLs, in comparison with the resistant C57BL/Ks and BALB/c strains, and the susceptibility of this F(1) strain to LP-BM5-induced MAIDS. We report here that no symptoms of MAIDS were observed in CBY6F(1) (H-2(dxb)) mice. For F(2) mice, in contrast to the high susceptibility of H-2(b/b) mice, 77% of H-2(d/d) and 81% of H-2(b/d) F(2) mice did not exhibit MAIDS after LP-BM5 infection. These results are in contrast to other published studies that concluded that susceptibility, rather than resistance, is dominant in F(1) (resistant x susceptible or susceptible x resistant) mice. We also show that CBY6F(1) anti-gag CTLs exhibit a fine specificity shared by the MAIDS-resistant BALB/c and C57BL/Ks strains, that is, the immunodominant gag epitope, SYNTGRFPPL, encoded by an alternative open reading frame. Together with our direct demonstration here that in vivo monoclonal antibody (mAb) depletion of CD8(+) T cells converts genetically resistant mice to MAIDS susceptibility, these data on the ability to mount anti-ORF2/SYNTGRFPPL, gag-specific CTL responses strongly suggest that CTLs are a primary factor in determining MAIDS resistance. Accordingly, given the K(d)-restricted nature of the CTLs, the main genetic determinant of resistance appeared to be the codominant expression of the resistant H-2(d) haplotype. Interestingly, however, 19% of H-2(d/b) and 23% of the H-2(d/d) F(2) mice had at least one clinical aspect of MAIDS, suggesting that a non-MHC genetic determinant(s) can negatively influence T-cell protection and thus disease outcome

Published

2000

47. Functional deletion of the CCR5 receptor by intracellular immunization produces cells that are refractory to CCR5-dependent HIV-1 infection and cell fusion

Author

Carlos F. Barbas, Peter Steinberger, Bernd Bühler, Jennifer Andris-Widhopf, and Bruce E. Torbett

Subjects

Receptors, CCR5, Chemokine receptor CCR5, viruses, Genetic enhancement, HIV Infections, Receptors, Cell Surface, Transfection, medicine.disease_cause, Epitope, Cell Line, Cell Fusion, medicine, Animals, Humans, Regulation of gene expression, Multidisciplinary, biology, Antibodies, Monoclonal, Gene Products, env, virus diseases, Biological Sciences, Simian immunodeficiency virus, biology.organism_classification, Macaca mulatta, Virology, Gene Expression Regulation, COS Cells, Lentivirus, HIV-1, biology.protein, Immunization, Antibody, Plasmids

Abstract

Studies of naturally occurring polymorphisms of the CCR5 gene have shown that deletion of the functional receptor or reduced expression of the gene can have beneficial effects in preventing HIV-1 infection or delaying disease. Because these polymorphisms are found in otherwise healthy people, strategies that aim to prevent or limit expression of CCR5 should be beneficial in the treatment of HIV-1 disease. To test this approach we have developed a CCR5-specific single-chain antibody that was expressed intracellularly and retained in the endoplasmic reticulum. This CCR5-intrabody efficiently blocked surface expression of human and rhesus CCR5 and thus prevented cellular interactions with CCR5-dependent HIV-1 and simian immunodeficiency virus envelope glycoprotein. Intrabody-expressing cells were shown to be highly refractory to challenge with R5 HIV-1 viruses or infected cells. These results suggest that gene therapy approaches that deliver this intracellular antibody could be of benefit to infected individuals. Because the antibody reacts with a conserved primate epitope on CCR5 this strategy can be tested in nonhuman lentivirus models of HIV-1 disease.

Published

2000

48. Human Cord Blood Progenitors Sustain Thymic T-Cell Development and a Novel Form of Angiogenesis

Author

Mark H. Ellisman, Bruce E. Torbett, Daniel R. Salomon, Laura Crisa, Kent A. Smith, and Vincenzo Cirulli

Subjects

Immunology, Cell Biology, Hematology, Biology, Biochemistry, Endothelial stem cell, Transplantation, Haematopoiesis, Cord blood, Cancer research, Lymphopoiesis, Progenitor cell, Stem cell, Homing (hematopoietic)

Abstract

There is growing interest in using human umbilical cord blood (CB) for allogeneic bone marrow transplantation (BMT), particularly in children. Thus, CB has been identified as a rich source of hematopoietic progenitors of the erythroid, myeloid, and B-cell lineages. Whether CB blood cells engrafting in the BM space also comprise T-cell progenitors capable of trafficking to the thymus and reconstituting a functional thymopoiesis in young recipients is presently unknown. Here, we show that CB progenitors, engrafted in the BM of immunodeficient mice, sustain human thymopoiesis by generating circulating T-cell progenitors capable of homing to and developing within a human thymic graft. Surprisingly, development of CB stem cells in this in vivo model extended to elements of the endothelial cell lineage, which contributed to the revascularization of transplants and wound healing. These results demonstrate that human CB stem cell transplantation can reconstitute thymic-dependent T-cell lymphopoiesis and show a novel role of CB-derived hematopoietic stem cells in angiogenesis.

Published

1999

49. PU.1 and the Granulocyte- and Macrophage Colony-Stimulating Factor Receptors Play Distinct Roles in Late-Stage Myeloid Cell Differentiation

Author

Hugh B. Perkin, Karen L. Anderson, Carol-Gay Anderson, Kent A. Smith, Richard A. Maki, Gary Hermanson, Bruce E. Torbett, and Douglas J. Jolly

Subjects

Macrophage colony-stimulating factor, Myeloid, Growth factor, medicine.medical_treatment, Cellular differentiation, Immunology, Cell Biology, Hematology, Biology, Biochemistry, Cell biology, Haematopoiesis, medicine.anatomical_structure, Myeloid Cell Differentiation, Growth factor receptor, medicine, IRF8

Abstract

PU.1 is a hematopoietic cell–specific ets family transcription factor. Gene disruption of PU.1 results in a cell autonomous defect in hematopoietic progenitor cells that manifests as abnormal myeloid and B-lymphoid development. Of the myeloid lineages, no mature macrophages develop, and the neutrophils that develop are aberrantly and incompletely matured. One of the documented abnormalities of PU.1 null (deficient) hematopoietic cells is a failure to express receptors for granulocyte colony-stimulating factor (G-CSF), granulocyte-macrophage (GM)-CSF, and M-CSF. To elucidate the roles of the myeloid growth factor receptors in myeloid cell differentiation, and to distinguish their role from that of PU.1, we have restored expression of the G- and M-CSF receptors in PU.1-deficient cells using retroviral vectors. We have similarly expressed PU.1 in these cells. Whereas expression of growth factor receptors merely allows a PU.1-deficient cell line to survive and grow in the relevant growth factor, expression of PU.1 enables the development of F4/80+, Mac-1+/CD11b+ macrophages, expression of gp91phox and generation of superoxide, and expression of secondary granule genes for neutrophil collagenase and gelatinase. These studies reinforce the idea that availability of PU.1 is crucial for normal myeloid development and clarify some of the molecular events in developing neutrophils and macrophages that are critically dependent on PU.1.

Published

1999

50. Transduction of Human CD34+Cells That Mediate Long-Term Engraftment of NOD/SCID Mice by HIV Vectors

Author

Kent A. Smith, Hiroyuki Miyoshi, Bruce E. Torbett, Donald E. Mosier, and Inder M. Verma

Subjects

Cell Survival, medicine.medical_treatment, Genetic enhancement, Genetic Vectors, Green Fluorescent Proteins, CD34, Gene Expression, Antigens, CD34, Bone Marrow Cells, Mice, SCID, Hematopoietic stem cell transplantation, Biology, Transfection, Viral vector, Colony-Forming Units Assay, Mice, Mice, Inbred NOD, medicine, Animals, Humans, Transgenes, Promoter Regions, Genetic, Multidisciplinary, Gene Transfer Techniques, Hematopoietic Stem Cell Transplantation, HIV, Hematopoietic Stem Cells, Hematopoiesis, Leukemia Virus, Murine, Transplantation, Luminescent Proteins, Haematopoiesis, Immunology, Stem cell, Cell Division

Abstract

Efficient gene transfer into human hematopoietic stem cells (HSCs) is an important goal in the study of the hematopoietic system as well as for gene therapy of hematopoietic disorders. A lentiviral vector based on the human immunodeficiency virus (HIV) was able to transduce human CD34+cells capable of stable, long-term reconstitution of nonobese diabetic/severe combined immunodeficient (NOD/SCID) mice. High-efficiency transduction occurred in the absence of cytokine stimulation and resulted in transgene expression in multiple lineages of human hematopoietic cells for up to 22 weeks after transplantation.

Published

1999