Your search keyword '"Laurie R. Gray"' showing total 22 results

1. HIV-1 Rev interacts with HERV-K RcREs present in the human genome and promotes export of unspliced HERV-K proviral RNA

Author

Laurie R. Gray, Rachel E. Jackson, Patrick E. H. Jackson, Stefan Bekiranov, David Rekosh, and Marie-Louise Hammarskjöld

Subjects

HIV-1, HERV-K, HIV RRE, HIV Rev, HERV-K RcRE, RNA export, Immunologic diseases. Allergy, RC581-607

Abstract

Abstract Background The HERV-K (HML-2) viruses are the youngest of the human endogenous retroviruses. They are present as several almost complete proviral copies and numerous fragments in the human genome. Many HERV-K proviruses express a regulatory protein Rec, which binds to an element present in HERV-K mRNAs called the RcRE. This interaction is necessary for the nucleo-cytoplasmic export and expression of HERV-K mRNAs that retain introns and plays a role analogous to that of Rev and the RRE in HIV replication. There are over 900 HERV-K RcREs distributed throughout the human genome. Thus, it was of interest to determine if Rev could functionally interact with selected RcRE elements that map either to HERV-K proviruses or human gene regions. This interaction would have the potential to alter the expression of both HERV-K mRNAs and cellular mRNAs during HIV-1 infection. Results In this study we employed a combination of RNAseq, bioinformatics and cell-based functional assays. Potential RcREs were identified through a number of bioinformatic approaches. They were then tested for their ability to promote export and translation of a reporter mRNA with a retained intron in conjunction with Rev or Rec. Some of the selected elements functioned well with either Rev, Rec or both, whereas some showed little or no function. Rev function on individual RcREs varied and was also dependent on the Rev sequence. We also performed RNAseq on total and cytoplasmic RNA isolated from SupT1 cells expressing HIV Rev, with or without Tat, or HERV-K Rec. Proviral mRNA from three HERV-K loci (4p16.1b, 22q11.23 and most significantly 3q12.3) accumulated in the cytoplasm in the presence of Rev or Tat and Rev, but not Rec. Consistent with this, the 3′ RcRE from 3q12.3 functioned well with HIV-Rev in our reporter assay. In contrast, this RcRE showed little or no function with Rec. Conclusions The HIV Rev protein can functionally interact with many RcREs present in the human genome, depending on the RcRE sequence, as well as the Rev sequence. This leads to export of some of the HERV-K proviral mRNAs and also has the potential to change the expression of non-viral genes.

Published

2019

2. Characterization of APOBEC3 variation in a population of HIV-1 infected individuals in northern South Africa

Author

Nontokozo D. Matume, Denis M. Tebit, Laurie R. Gray, Stephen D. Turner, David Rekosh, Pascal O. Bessong, and Marie-Louise Hammarskjöld

Subjects

APOBEC3, Single nucleotide polymorphism, South Africa, Internal medicine, RC31-1245, Genetics, QH426-470

Abstract

Abstract Background The apolipoprotein B mRNA-editing enzyme, catalytic polypeptide-like 3 (APOBEC3) genes A3D, A3F, A3G and A3H have all been implicated in the restriction of human immunodeficiency virus type 1 (HIV-1) replication. Polymorphisms in these genes are likely to impact viral replication and fitness, contributing to viral diversity. Currently, only a few studies indicate that polymorphisms in the A3 genes may be correlated with infection risk and disease progression. Methods To characterize polymorphisms in the coding regions of these APOBEC3 genes in an HIV-1 infected population from the Limpopo Province of South Africa, APOBEC3 gene fragments were amplified from genomic DNA of 192 HIV-1 infected subjects and sequenced on an Illumina MiSeq platform. SNPs were confirmed and compared to SNPs in other populations reported in the 1000 Genome Phase III and HapMap databases, as well as in the ExAC exome database. Hardy-Weinberg Equilibrium was calculated and haplotypes were inferred using the LDlink 3.0 web tool. Linkage Disequilibrium (LD) for these SNPS were calculated in the total 1000 genome and AFR populations using the same tool. Results Known variants compared to the GRCh37 consensus genome sequence were detected at relatively high frequencies (> 5%) in all of the APOBEC3 genes. A3H showed the most variation, with several of the variants present in both alleles in almost all of the patients. Several minor allele variants (

Published

2019

3. Arbovirus Prevalence in Mosquitoes, Kenya

Author

A. Desiree LaBeaud, Laura J. Sutherland, Samuel Muiruri, Eric M. Muchiri, Laurie R. Gray, Peter A. Zimmerman, Amy G. Hise, and Charles H. King

Subjects

Arboviruses, zoonoses, viruses, Rift Valley fever virus, West Nile virus, vectors, Medicine, Infectious and parasitic diseases, RC109-216

Abstract

Few studies have investigated the many mosquito species that harbor arboviruses in Kenya. During the 2006–2007 Rift Valley fever outbreak in North Eastern Province, Kenya, exophilic mosquitoes were collected from homesteads within 2 affected areas: Gumarey (rural) and Sogan-Godud (urban). Mosquitoes (n = 920) were pooled by trap location and tested for Rift Valley fever virus and West Nile virus. The most common mosquitoes trapped belonged to the genus Culex (75%). Of 105 mosquito pools tested, 22% were positive for Rift Valley fever virus, 18% were positive for West Nile virus, and 3% were positive for both. Estimated mosquito minimum infection rates did not differ between locations. Our data demonstrate the local abundance of mosquitoes that could propagate arboviral infections in Kenya and the high prevalence of vector arbovirus positivity during a Rift Valley fever outbreak.

Published

2011

4. Ly49R activation receptor drives self-MHC–educated NK cell immunity against cytomegalovirus infection

Author

John M. Cronk, Patryk Puchalski, Alyssa L. Gillespie, Marie-Louise Hammarskjold, Michael G. Brown, Hairong Wei, William T. Nash, Awndre Gamache, Laurie R. Gray, and Wenhao Xu

Subjects

Multidisciplinary, biology, Effector, Hepatitis C virus, Biological Sciences, medicine.disease_cause, Major histocompatibility complex, Virus, Immunity, MHC class I, Immunology, medicine, biology.protein, IL-2 receptor, Receptor

Abstract

Natural killer (NK) cells mediate vital control of cancer and viral infection. They rely on MHC class I (MHC I)-specific self-receptors to identify and lyse diseased cells without harming self-MHC I-bearing host cells. NK cells bearing inhibitory self-receptors for host MHC I also undergo education, referred to as licensing, which causes them to become more responsive to stimulation via activation receptor signaling. Previous work has shown that licensed NK cells selectively expand during virus infections and they are associated with improved clinical response in human patients experiencing certain chronic virus infections, including HIV and hepatitis C virus. However, the importance of inhibitory self-receptors in NK-mediated virus immunity is debated as they also limit signals in NK cells emanating from virus-specific activation receptors. Using a mouse model of MHC I-dependent (H-2D k ) virus immunity, we discovered that NK cells depend on the Ly49G2 inhibitory self-receptor to mediate virus control, which coincided with host survival during murine cytomegalovirus infection. This antiviral effect further requires active signaling in NK cells via the Ly49R activation receptor that also binds H-2D k . In tandem, these functionally discordant Ly49 self-receptors increase NK cell proliferation and effector activity during infection, resulting in selective up-regulation of CD25 and KLRG1 in virus-specific Ly49R + Ly49G2 + NK cells. Our findings establish that paired self-receptors act as major determinants of NK cell-mediated virus sensing and immunity.

Published

2019

5. Human endogenous retrovirus-K mRNA expression and genomic alignment data in hepatoblastoma

Author

Stefan Bekiranov, David F. Grabski, Aakrosh Ratan, Sara K. Rasmussen, Marie-Louise Hammarskjold, David Rekosh, and Laurie R. Gray

Subjects

Hepatoblastoma, Mrna expression, viruses, Computational biology, Biology, lcsh:Computer applications to medicine. Medical informatics, Germline, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, Biochemistry, Genetics and Molecular Biology, Gene expression, medicine, Human endogenous retrovirus K, lcsh:Science (General), 030304 developmental biology, 0303 health sciences, Multidisciplinary, medicine.disease, Genomic alignment, GenBank, lcsh:R858-859.7, Human genome, Transcriptome analysis, Human endogenous retrovirus-K, 030217 neurology & neurosurgery, lcsh:Q1-390

Abstract

Human Endogenous Retroviruses are a class of genomic elements that are the result of ancient retroviral infection of the human germline. Many are biologically active elements that have been implicated in multiple diseases including cancer. The most recent class to invade the human genome is the HERV-K(HML-2) (HERV-K) family. Approximately 90 HERV-K proviruses and many smaller elements have been identified to date in the human genome. Additional proviruses are continually being discovered with the rapid advancement of deep-sequencing and long-read sequencing technologies. HERV-K proviruses are poorly annotated in human transcriptome databases making their analysis in RNA-seq data difficult. To enable analysis, we compiled the sequences of 91 HERV-K proviruses identified in NCBI GenBank (ID JN675007-JN675097) and created a proviral alignment tool for visualizing RNA-seq reads aligned across individual proviruses. This allowed us to analyse publicly available RNA-seq data from 10 hepatoblastoma samples and 3 normal liver controls (GEO Accession ID: GSE89775). This data report includes the raw FASTA sequence files of the HERV-K proviruses from NCBI, a differential gene expression list between hepatoblastoma samples, and genomic alignment figures from 5 HERV-K proviruses identified as differentially expressed in the companion research article “Upregulation of Human Endogenous Retrovirus-K (HML-2) mRNAs in hepatoblastoma: Identification of potential new immunotherapeutic targets and biomarkers [1]. The data provided here are available for other research groups interested in evaluating individual HERV-K proviral expression using RNA-seq data. Furthermore, the data analysis is highly flexible and will accommodate the addition of other HERV-K proviruses.

Published

2020

6. Upregulation of Human Endogenous Retrovirus-K (HML-2) mRNAs in hepatoblastoma: Identification of potential new immunotherapeutic targets and biomarkers

Author

Marie-Louise Hammarskjold, Sara K. Rasmussen, David Rekosh, Stefan Bekiranov, Aakrosh Ratan, Laurie R. Gray, and David F. Grabski

Subjects

0303 health sciences, Messenger RNA, Hepatoblastoma, cDNA library, viruses, Biology, Provirus, medicine.disease, digestive system diseases, 3. Good health, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, 030220 oncology & carcinogenesis, Cancer research, medicine, Biomarker (medicine), Human genome, Human endogenous retrovirus K, 030304 developmental biology

Abstract

PurposeHepatoblastoma is the most common liver malignancy in children. In order to advance therapy against hepatoblastoma, novel immunologic targets and biomarkers are needed. Our purpose in this investigation is to examine hepatoblastoma transcriptomes for the expression of a class of genomic elements known as Human Endogenous Retrovirus (HERVs). HERVs are abundant in the human genome and are biologically active elements that have been associated with multiple malignancies and proposed as immunologic targets in a subset of tumors. A sub-family of HERVs, HERV-K (HML-2), have been shown to be tightly regulated in fetal development, making investigation of these elements in pediatric tumors paramount.MethodsWe first created a HERVK-FASTA file utilizing 91 previously described HML-2 proviruses. We then concatenated the file onto the GRCh38.95 cDNA library from Ensembl. We used this computational tool to evaluate existing RNA-seq data from 10 hepatoblastoma tumors and 3 normal liver controls (GEO accession ID: GSE89775). Quantification and differential proviral expression analysis between hepatoblastoma and normal liver controls was performed using the pseudo-alignment program Salmon and DESeq2, respectively.ResultsHERV-K mRNA was expressed in hepatoblastoma from multiple proviral loci. All HERV-K proviral loci were expressed at higher levels in hepatoblastoma compared to normal liver controls. Five HERV-K proviruses (1q21.3, 3q27.2, 7q22.2, 12q24.33 and 17p13.1) were significantly differentially expressed (p-adjusted value < 0.05, |log2 fold change| > 1.5) across conditions. The provirus at 17p13.1 had an approximately 300-fold increased expression in hepatoblastoma as compared to normal liver. This was in part due to the near absence of HERV-K mRNA at the 17p13.1 locus in fully differentiated liver samples.ConclusionsOur investigation demonstrates that HERV-K is expressed from multiple loci in hepatoblastoma and that the expression is increased from several proviruses as compared to normal liver controls. Our results suggest that HERV-K mRNA expression may find use as a biomarker in hepatoblastoma, given the large differential expression profiles in hepatoblastoma, with very low mRNA levels in liver control samples.

Published

2020

7. Upregulation of human endogenous retrovirus-K (HML-2) mRNAs in hepatoblastoma: Identification of potential new immunotherapeutic targets and biomarkers

Author

Sara K. Rasmussen, Laurie R. Gray, Stefan Bekiranov, David Rekosh, David F. Grabski, Marie-Louise Hammarskjold, and Aakrosh Ratan

Subjects

Hepatoblastoma, viruses, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, 030225 pediatrics, medicine, Humans, Human endogenous retrovirus K, RNA, Messenger, Child, Messenger RNA, cDNA library, business.industry, Endogenous Retroviruses, Liver Neoplasms, General Medicine, Provirus, medicine.disease, digestive system diseases, Up-Regulation, 030220 oncology & carcinogenesis, embryonic structures, Pediatrics, Perinatology and Child Health, Cancer research, Biomarker (medicine), Surgery, Human genome, Immunotherapy, business, Biomarkers

Abstract

Purpose Hepatoblastoma is the most common liver malignancy in children. In order to advance therapy against hepatoblastoma, novel immunologic targets and biomarkers are needed. Our purpose in this investigation is to examine hepatoblastoma transcriptomes for the expression of a class of genomic elements known as Human Endogenous Retrovirus (HERVs). HERVs are abundant in the human genome and are biologically active elements that have been associated with multiple malignancies and proposed as immunologic targets in a subset of tumors. A sub-family of HERVs, HERV-K(HML-2) (HERV-K), have been shown to be tightly regulated in fetal development, making investigation of these elements in pediatric tumors paramount. Methods We first created a HERVK-FASTA file utilizing 91 previously described HML-2 proviruses. We then concatenated the file onto the GRCh38.95 cDNA library from Ensembl. We used this reference database to evaluate existing RNA-seq data from 10 hepatoblastoma tumors and 3 normal liver controls (GEO accession ID: GSE8977575 ). Quantification and differential proviral expression analysis between hepatoblastoma and normal liver controls was performed using the pseudo-alignment program Salmon and DESeq2, respectively. Results HERV-K mRNA was expressed in hepatoblastoma from multiple proviral loci. All expressed HERV-K proviral loci were upregulated in hepatoblastoma compared to normal liver controls. Five HERV-K proviruses (1q21.3, 3q27.2, 7q22.2, 12q24.33 and 17p13.1) were significantly differentially expressed (p-adjusted value 1.5) across conditions. The provirus at 17p13.1 had an approximately 300-fold increased expression in hepatoblastoma as compared to normal liver. This was in part due to the near absence of HERV-K mRNA at the 17p13.1 locus in fully differentiated liver samples. Conclusions Our investigation demonstrates that HERV-K is expressed from multiple loci in hepatoblastoma and that the expression is increased for several proviruses compared to normal liver controls. Our results suggest that HERV-K mRNA expression may be useful as a biomarker in hepatoblastoma, given the large differential expression profiles in hepatoblastoma, with very low mRNA levels in liver control samples.

Published

2020

8. Next generation sequencing reveals a high frequency of CXCR4 utilizing viruses in HIV-1 chronically infected drug experienced individuals in South Africa

Author

Pascal O. Bessong, Denis M. Tebit, Marie-Louise Hammarskjold, Laurie R. Gray, Nontokozo D. Matume, and David Rekosh

Subjects

Adult, Male, 0301 basic medicine, Receptors, CXCR4, Adolescent, Genotype, Genotyping Techniques, viruses, Virus Attachment, Salvage therapy, HIV Infections, Viral quasispecies, Biology, V3 loop, Article, Maraviroc, South Africa, Young Adult, 03 medical and health sciences, chemistry.chemical_compound, Receptors, HIV, 0302 clinical medicine, Proviruses, Virology, Humans, 030212 general & internal medicine, Child, Genotyping, Tropism, Aged, High-Throughput Nucleotide Sequencing, Middle Aged, Viral Tropism, 030104 developmental biology, Infectious Diseases, Anti-Retroviral Agents, chemistry, Child, Preschool, HIV-1, Leukocytes, Mononuclear, Tissue tropism, Female

Abstract

Background Entry inhibitors, such as Maraviroc, bind to CCR5 inhibiting entry of CCR5 utilizing viruses (R5 viruses). In the course of HIV infection, CXCR4 utilizing viruses (X4 viruses) may emerge and outgrow R5 viruses, and potentially limit the effectiveness of Maraviroc. The use of Maraviroc is reserved for salvage therapy in South Africa. Objective In this study, we examined the frequency of R5 and X4 viruses, using next generation sequencing, in patients under treatment to draw inferences on the utility of Maraviroc in a South African population. Study design Proviral DNA was isolated from peripheral blood mononuclear cells (PBMC) of 72 chronically HIV infected patients on antiretroviral treatment. HIV V3 loop gene was amplified and sequenced on an Illumina MiniSeq platform. Viral subtypes were determined by the jumping profile Hidden Markov Model (jpHMM) and REGA genotyping tools. De Novo consensus sequences were derived for the majority and minority populations for each patient using Geneious® software version 8.1.5. HIV-1 tropism was inferred using PSSMsinsi, Geno2pheno and Phenoseq-C web-based tools. Results Quality V3 loop sequences were obtained from 72 patients, with 5 years (range: 0–16) median duration on treatment. Subtypes A1, B and C viruses were identified at frequencies of 4% (3/72), 4% (3/72) and 92% (66/72) respectively. Fifty four percent (39/72) of patients exclusively harboured R5 viral quasispecies; and 21% (15/72) exclusively harbored X4 viral quasispecies. Twenty five percent of patients (18/72) harbored dual/mixture of R5X4 quasispecies. Of these 18 patients, about 28% (5/18) harbored the R5+X4, a mixture with a majority R5 and minority X4 viruses, while about 72% (13/18) harbored the R5X4+ mixture with a majority X4 and minority R5 viruses. The proportion of all patients who harbored X4 viruses either exclusively or dual/mixture was 46% (33/72). Thirty-five percent (23/66) of the patients who were of HIV-1 subtype C harboured X4 viruses (χ2 = 3.58; p = .058), and 57% of these (13/23) harbored X4 viruses exclusively. CD4+ cell count less than 350 cell/μl was associated with the presence of X4 viruses (χ2 = 4.99; p = .008). Conclusion The effectiveness of Maraviroc as a component in salvage therapy may be compromised for a significant number of chronically infected patients harboring CXCR4 utilizing viruses.

Published

2018

9. Evolution of the HIV-1 Rev Response Element during Natural Infection Reveals Nucleotide Changes That Correlate with Altered Structure and Increased Activity over Time

Author

Laurie R. Gray, Chringma Sherpa, Kathryn Anastos, David Rekosh, Stuart F.J. Le Grice, Marie-Louise Hammarskjold, and Patrick E. H. Jackson

Subjects

viruses, Immunology, Response element, HIV Infections, Biology, Response Elements, Virus Replication, medicine.disease_cause, Genes, env, Microbiology, Pathogenesis, 03 medical and health sciences, Virology, HIV Seropositivity, medicine, Humans, Nucleotide, RNA, Messenger, Nucleic acid structure, 030304 developmental biology, Sequence (medicine), Genetics, chemistry.chemical_classification, 0303 health sciences, Mutation, Nucleotides, 030302 biochemistry & molecular biology, RNA, rev Gene Products, Human Immunodeficiency Virus, Gene Products, rev, Genetic Diversity and Evolution, chemistry, Insect Science, HIV-1, Nucleic Acid Conformation, RNA, Viral, Function (biology), Protein Binding

Abstract

The HIV-1 Rev response element (RRE) is a cis-acting RNA element characterized by multiple stem-loops. Binding and multimerization of the HIV Rev protein on the RRE promote the nucleocytoplasmic export of incompletely spliced mRNAs, an essential step in HIV replication. Most of our understanding of the Rev-RRE regulatory axis comes from studies of lab-adapted HIV clones. However, in human infection, HIV evolves rapidly, and mechanistic studies of naturally occurring Rev and RRE sequences are essential to understanding this system. We previously described the functional activity of two RREs found in circulating viruses in a patient followed during the course of HIV infection. The early RRE was less functionally active than the late RRE, despite differing in sequence by only 4 nucleotides. In this study, we describe the sequence, function, and structural evolution of circulating RREs in this patient using plasma samples collected over 6 years of untreated infection. RRE sequence diversity varied over the course of infection, with evidence of selection pressure that led to sequence convergence as disease progressed being found. An increase in RRE functional activity was observed over time, and a key mutation was identified that correlates with a major conformational change in the RRE and increased functional activity. Additional mutations were found that may have contributed to increased activity as a result of greater Shannon entropy in RRE stem-loop II, which is key to primary Rev binding. IMPORTANCE HIV-1 replication requires interaction of the viral Rev protein with a cis-acting regulatory RNA, the Rev response element (RRE), whose sequence changes over time during infection within a single host. In this study, we show that the RRE is subject to selection pressure and that RREs from later time points in infection tend to have higher functional activity. Differences in RRE functional activity are attributable to specific changes in RNA structure. Our results suggest that RRE evolution during infection may be important for HIV pathogenesis and that efforts to develop therapies acting on this viral pathway should take this into account.

Published

2019

10. Evolution of the HIV-1 RRE during natural infection reveals nucleotide changes that correlate with altered structure and increased activity over time

Author

Laurie R. Gray, Kathryn Anastos, Patrick E. H. Jackson, Chringma Sherpa, David Rekosh, Marie-Louise Hammarskjold, and Stuart F.J. Le Grice

Subjects

Genetics, chemistry.chemical_classification, 0303 health sciences, Mutation, viruses, 030302 biochemistry & molecular biology, Response element, RNA, Biology, medicine.disease_cause, 3. Good health, Pathogenesis, 03 medical and health sciences, chemistry, medicine, Nucleotide, Nucleic acid structure, Function (biology), 030304 developmental biology, Sequence (medicine)

Abstract

AbstractThe HIV-1 Rev Response Element (RRE) is acis-acting RNA element characterized by multiple stem-loops. Binding and multimerization of the HIV Rev protein on the RRE promotes nucleocytoplasmic export of incompletely spliced mRNAs, an essential step in HIV replication. Most of our understanding of the Rev-RRE regulatory axis comes from studies of lab-adapted HIV clones. However, in human infection, HIV evolves rapidly and mechanistic studies of naturally occurring Rev and RRE sequences are essential to understanding this system. We previously described the functional activity of two RREs found in circulating viruses in a patient followed during the course of HIV infection. The “early” RRE was less functionally active than the “late” RRE despite differing in sequence by only four nucleotides. In this study, we describe the sequence, function, and structural evolution of circulating RREs in this patient using plasma samples collected over six years of untreated infection. RRE sequence diversity varied over the course of infection with evidence of selection pressure that led to sequence convergence as disease progressed. An increase in RRE functional activity was observed over time, and a key mutation was identified that correlates with a major conformational change in the RRE and increased functional activity. Additional mutations were found that may have contributed to increased activity as a result of greater Shannon entropy in RRE stem-loop II, which is key to primary Rev binding.ImportanceHIV-1 replication requires interaction of the viral Rev protein with acis-acting regulatory RNA, the Rev Response Element (RRE), whose sequence changes over time during infection within a single host. In this study, we show that the RRE is subject to selection pressure and that RREs from later time points in infection tend to have higher functional activity. Differences in RRE functional activity are attributable to specific changes in RNA structure. Our results suggest that RRE evolution during infection may be important for HIV pathogenesis and that efforts to develop therapies acting on this viral pathway should take this into account.

Published

2018

11. Effect of intercalator and Lewis acid-base branched peptide complex formation: boosting affinity towards HIV-1 RRE RNA

Author

David Rekosh, Laurie R. Gray, Jessica E. Wynn, Marie-Louise Hammarskjold, Wenyu Zhang, Denis M. Tebit, and Webster L. Santos

Subjects

0301 basic medicine, Pharmacology, chemistry.chemical_classification, inorganic chemicals, Stereochemistry, High-throughput screening, viruses, Organic Chemistry, Pharmaceutical Science, RNA, Peptide, Biochemistry, Article, Dissociation constant, 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, Capsid, chemistry, Drug Discovery, Acridine, Molecular Medicine, Lewis acids and bases, Boronic acid

Abstract

High throughput screening of a 4096 compound library of boronic acid and acridine containing branched peptides revealed compounds that have dissociation constants in the low nanomolar regime for HIV-1 RRE IIB RNA. We demonstrate that branched peptide boronic acids A5, A6, and A7 inhibit the production of p24, an HIV-1 capsid protein, in a dose-dependent manner.

Published

2016

12. Characterization and in vitro activity of a branched peptide boronic acid that interacts with HIV-1 RRE RNA

Author

David Rekosh, Marie-Louise Hammarskjold, Jessica E. Wynn, Denis M. Tebit, Wenyu Zhang, Webster L. Santos, and Laurie R. Gray

Subjects

0301 basic medicine, Anti-HIV Agents, viruses, Clinical Biochemistry, HIV Core Protein p24, Pharmaceutical Science, Peptide, Integrase Inhibitors, Quinolones, Response Elements, Virus Replication, Biochemistry, Article, 03 medical and health sciences, chemistry.chemical_compound, Structure-Activity Relationship, Peptide Library, Raltegravir Potassium, Drug Discovery, Structure–activity relationship, Humans, Binding site, Peptide library, Molecular Biology, chemistry.chemical_classification, Organic Chemistry, RNA, Boronic Acids, Footprinting, 030104 developmental biology, chemistry, Lamivudine, Transfer RNA, HIV-1, Molecular Medicine, Nucleic Acid Conformation, RNA, Viral, Peptides, Zidovudine, Boronic acid, HeLa Cells

Abstract

A branched peptide containing multiple boronic acids was found to bind RRE IIB selectively and inhibit HIV-1 p24 capsid production in a dose-dependent manner. Structure–activity relationship studies revealed that branching in the peptide is crucial for the low micromolar binding towards RRE IIB, and the peptide demonstrates selectivity towards RRE IIB in the presence of tRNA. Footprinting studies suggest a binding site on the upper stem and internal loop regions of the RNA, which induces enzymatic cleavage of the internal loops of RRE IIB upon binding.

Published

2016

13. Arbovirus Prevalence in Mosquitoes, Kenya

Author

Laurie R. Gray, Peter A. Zimmerman, Eric M. Muchiri, Amy G. Hise, Samuel Muiruri, Charles H. King, Laura J. Sutherland, and A. Desiree LaBeaud

Subjects

Rift Valley fever virus, Veterinary medicine, Rift Valley Fever, Epidemiology, viruses, lcsh:Medicine, medicine.disease_cause, Polymerase Chain Reaction, 0302 clinical medicine, vectors, Rift Valley fever, 0303 health sciences, High prevalence, Reverse Transcriptase Polymerase Chain Reaction, virus diseases, 3. Good health, Culex, Infectious Diseases, RNA, Viral, West Nile virus, Microbiology (medical), 030231 tropical medicine, RT-PCR, Biology, Arbovirus, lcsh:Infectious and parasitic diseases, 03 medical and health sciences, parasitic diseases, medicine, Animals, Humans, lcsh:RC109-216, mosquitoes, 030304 developmental biology, Research, fungi, lcsh:R, Outbreak, medicine.disease, biology.organism_classification, Kenya, Insect Vectors, zoonoses, Culicidae, Vector (epidemiology), West Nile Fever, Arboviruses

Abstract

Few studies have investigated the many mosquito species that harbor arboviruses in Kenya. During the 2006–2007 Rift Valley fever outbreak in North Eastern Province, Kenya, exophilic mosquitoes were collected from homesteads within 2 affected areas: Gumarey (rural) and Sogan-Godud (urban). Mosquitoes (n = 920) were pooled by trap location and tested for Rift Valley fever virus and West Nile virus. The most common mosquitoes trapped belonged to the genus Culex (75%). Of 105 mosquito pools tested, 22% were positive for Rift Valley fever virus, 18% were positive for West Nile virus, and 3% were positive for both. Estimated mosquito minimum infection rates did not differ between locations. Our data demonstrate the local abundance of mosquitoes that could propagate arboviral infections in Kenya and the high prevalence of vector arbovirus positivity during a Rift Valley fever outbreak.

Published

2011

14. Molecular-Based Assay for Simultaneous Detection of Four Plasmodium spp. and Wuchereria bancrofti Infections

Author

Melinda J. Blood-Zikursh, Edward K. Thomsen, Zachary A. Kloos, Moses Baisor, Nandao Tarongka, Manasseh Baea, Daniel J. Tisch, Peter A. Zimmerman, Kaye Baea, Will Kastens, Rajeev K. Mehlotra, Laurie R. Gray, Lisa J. Reimer, Cara N. Henry-Halldin, and James W. Kazura

Subjects

Plasmodium, Biology, medicine.disease_cause, Polymerase Chain Reaction, Sensitivity and Specificity, Filariasis, law.invention, Apicomplexa, law, Virology, parasitic diseases, Multiplex polymerase chain reaction, medicine, Animals, Humans, Parasite hosting, Wuchereria bancrofti, Multiplex, Polymerase chain reaction, Lymphatic filariasis, Genome, Articles, DNA, Helminth, DNA, Protozoan, medicine.disease, biology.organism_classification, Malaria, Infectious Diseases, Parasitology

Abstract

Four major malaria-causing Plasmodium spp. and lymphatic filariasis-causing Wuchereria bancrofti are co-endemic in many tropical and sub-tropical regions. Among molecular diagnostic assays, multiplex polymerase chain reaction (PCR)–based assays for the simultaneous detection of DNAs from these parasite species are currently available only for P. falciparum and W. bancrofti or P. vivax and W. bancrofti. Using a post-PCR oligonucleotide ligation detection reaction–fluorescent microsphere assay (LDR-FMA), we developed a multiplex assay that has the capability to simultaneously detect all four Plasmodium spp. and W. bancrofti infections in blood samples. Compared with microfilarial positivity in the blood, the LDR-FMA assay is highly concordant (91%), sensitive (86%), and specific (94%), and has high reproducibility for Plasmodium spp. (85–93%) and W. bancrofti (90%) diagnoses. The development of this assay for the simultaneous diagnosis of multiple parasitic infections enables efficient screening of large numbers of human blood and mosquito samples from co-endemic areas.

Published

2010

15. Plasmodium vivax clinical malaria is commonly observed in Duffy-negative Malagasy people

Author

Brian T. Grimberg, Vincent Thonier, Peter A. Zimmerman, Olivier Domarle, Jean François Carod, Laurie R. Gray, Julien Picot, Didier Menard, Christopher L. King, Arsène Ratsimbasoa, Céline Barnadas, Yves Colin, Odile Mercereau-Puijalon, Cara N. Henry-Halldin, Olivier F. Bertrand, Christiane Bouchier, Institut Pasteur de Madagascar, Réseau International des Instituts Pasteur (RIIP), Immunologie moléculaire des parasites, Institut Pasteur [Paris] (IP)-Centre National de la Recherche Scientifique (CNRS), Center for Global Health and Diseases, School of Medicine-Case Western Reserve University [Cleveland], Génomique (Plate-Forme) - Genomics Platform, Institut Pasteur [Paris] (IP), Ministère de la Santé, du Planning Familial et de la Protection Sociale, Protéines de la membrane érythrocytaire et homologues non-érythroides, Université des Antilles et de la Guyane (UAG)-Institut National de la Transfusion Sanguine [Paris] (INTS)-Université Paris Diderot - Paris 7 (UPD7)-Université de La Réunion (UR)-Institut National de la Santé et de la Recherche Médicale (INSERM), Veterans Affairs Research Service, Institut Pasteur [Paris]-Centre National de la Recherche Scientifique (CNRS), and Institut Pasteur [Paris]

Subjects

Male, Erythrocytes, Plasmodium vivax, MESH: Base Sequence, MESH: Madagascar, 0302 clinical medicine, [SDV.MHEP.MI]Life Sciences [q-bio]/Human health and pathology/Infectious diseases, MESH: Child, Epidemiology, Parasite hosting, Child, MESH: Genetic Association Studies, 0303 health sciences, MESH: Asian Continental Ancestry Group, Multidisciplinary, biology, MESH: Erythrocytes, Biological Sciences, MESH: Plasmodium vivax, 3. Good health, Child, Preschool, Female, medicine.symptom, MESH: DNA Primers, medicine.medical_specialty, Adolescent, Molecular Sequence Data, 030231 tropical medicine, Black People, MESH: Host-Parasite Interactions, Asymptomatic, Host-Parasite Interactions, 03 medical and health sciences, Asian People, Antigen, parasitic diseases, Madagascar, Malaria, Vivax, Gametocyte, medicine, Humans, Genotyping, Genetic Association Studies, DNA Primers, 030304 developmental biology, MESH: Adolescent, MESH: Humans, MESH: Molecular Sequence Data, Base Sequence, MESH: Child, Preschool, MESH: Malaria, Vivax, biology.organism_classification, medicine.disease, Virology, MESH: Male, MESH: Duffy Blood-Group System, Immunology, MESH: African Continental Ancestry Group, Duffy Blood-Group System, MESH: Female, Malaria

Abstract

Malaria therapy, experimental, and epidemiological studies have shown that erythrocyte Duffy blood group-negative people, largely of African ancestry, are resistant to erythrocyte Plasmodium vivax infection. These findings established a paradigm that the Duffy antigen is required for P. vivax erythrocyte invasion. P. vivax is endemic in Madagascar, where admixture of Duffy-negative and Duffy-positive populations of diverse ethnic backgrounds has occurred over 2 millennia. There, we investigated susceptibility to P. vivax blood-stage infection and disease in association with Duffy blood group polymorphism. Duffy blood group genotyping identified 72% Duffy-negative individuals ( FY*B ES /*B ES ) in community surveys conducted at eight sentinel sites. Flow cytometry and adsorption–elution results confirmed the absence of Duffy antigen expression on Duffy-negative erythrocytes. P. vivax PCR positivity was observed in 8.8% (42/476) of asymptomatic Duffy-negative people. Clinical vivax malaria was identified in Duffy-negative subjects with nine P. vivax monoinfections and eight mixed Plasmodium species infections that included P. vivax (4.9 and 4.4% of 183 participants, respectively). Microscopy examination of blood smears confirmed blood-stage development of P. vivax , including gametocytes. Genotyping of polymorphic surface and microsatellite markers suggested that multiple P. vivax strains were infecting Duffy-negative people. In Madagascar, P. vivax has broken through its dependence on the Duffy antigen for establishing human blood-stage infection and disease. Further studies are necessary to identify the parasite and host molecules that enable this Duffy-independent P. vivax invasion of human erythrocytes.

Published

2010

16. Hyper-excretion of Human Immunodeficiency Virus Type 1 RNA in Saliva

Author

Diane C. Shugars, Lauren L. Patton, Stephanie A. Freel, Laurie R. Gray, Susan A. Fiscus, Joseph J. Eron, and R. T. Vollmer

Subjects

Adult, Male, 0301 basic medicine, Saliva, Anti-HIV Agents, Cell, HIV Infections, Biology, Statistics, Nonparametric, Excretion, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Blood plasma, medicine, Humans, General Dentistry, Chi-Square Distribution, Case-control study, RNA, 030206 dentistry, Viral Load, Gingivitis, Cross-Sectional Studies, 030104 developmental biology, medicine.anatomical_structure, chemistry, Case-Control Studies, DNA, Viral, Immunology, HIV-1, Female, Viral load, DNA

Abstract

Anatomical compartments (e.g., the reproductive tract) are reservoirs of human immunodeficiency virus type-1 (HIV-1) and potential sites of residual infection in patients receiving anti-retroviral therapy (ART). Viral hyper-excretion relative to blood is a hallmark of reservoirs. To determine whether hyper-excretion can occur in the oral cavity, we compared viral loads in blood plasma and saliva of 67 adults. Salivary viral hyper-excretion was defined as a four-fold or higher viral load in saliva than in plasma. HIV-1 RNA was detected in 79% of plasma samples, in 44% of unfiltered saliva samples, in 16% of filtered saliva samples, and in 59% of saliva-derived cell pellets. Compared with non-hyper-excretors (n = 62), hyper-excretors (n = 5) had elevated levels of viral RNA in unfiltered saliva and saliva-derived cells, HIV-associated periodontal disease, gingival inflammation, and no combination ART. Morphological characterization of cell pellets identified lymphocytes as a likely HIV-1 source. These collective findings are consistent with an oral HIV-1 reservoir in selected individuals.

Published

2001

17. Limited nucleotide changes in the Rev response element (RRE) during HIV-1 infection alter overall Rev-RRE activity and Rev multimerization

Author

Marie-Louise Hammarskjold, Emily A. Sloan, Kathryn Anastos, Joseph B. Margolick, Laurie R. Gray, Frank Maldarelli, David Rekosh, Mary F. Kearney, and Eric S. Daar

Subjects

Adult, Male, Period (gene), viruses, Immunology, Response element, HIV Infections, Biology, Virus Replication, Microbiology, Genome, Genes, env, Plasma, Virology, Cluster Analysis, Humans, Nucleotide, Nuclear export signal, Phylogeny, chemistry.chemical_classification, Genetics, Functional analysis, Phylogenetic tree, rev Gene Products, Human Immunodeficiency Virus, Sequence Analysis, DNA, Middle Aged, Genome Replication and Regulation of Viral Gene Expression, chemistry, Viral replication, Insect Science, Mutation, HIV-1, RNA, Viral, Female

Abstract

HIV-1 Rev and the Rev response element (RRE) enable a critical step in the viral replication cycle by facilitating the nuclear export of intron-containing mRNAs, yet their activities have rarely been analyzed in natural infections. This study characterized their genetic and functional variation in a small cohort of HIV-infected individuals. Multiple Rev and RRE sequences were obtained using single-genome sequencing (SGS) of plasma samples collected within 6 months after seroconversion and at a later time. This allowed the identification of cognate sequences that were linked in vivo in the same viral genome and acted together as a functional unit. Phylogenetic analyses of these sequences indicated that 4/5 infections were founded by a single transmission event. Rev and RRE variants from each time point were subjected to functional analysis as both cognate pairs and as individual components. While a range of Rev-RRE activities were seen, the activity of cognate pairs from a single time point clustered to a discrete level, which was termed the set point. In 3/5 patients, this set point changed significantly over the time period studied. In all patients, RRE activity was more sensitive to sequence variation than Rev activity and acted as the primary driver of the cognate set point. Selected patient RREs were also shown to have differences in Rev multimerization using gel shift binding assays. Thus, rather than acting as a simple on-off switch or maintaining a constant level of activity throughout infection, the Rev-RRE system can fluctuate, presumably to control replication.

Published

2013

18. A new high-throughput method for simultaneous detection of drug resistance associated mutations in Plasmodium vivax dhfr, dhps and mdr1 genes

Author

Peter J. Thomas, Laurie R. Gray, David Kent, Jonah Iga, Peter A. Zimmerman, Ivo Mueller, Peter Siba, Lincoln Timinao, and Céline Barnadas

Subjects

lcsh:Arctic medicine. Tropical medicine, lcsh:RC955-962, 030231 tropical medicine, Plasmodium vivax, Population, Drug Resistance, Protozoan Proteins, Single-nucleotide polymorphism, DHPS, Drug resistance, Biology, Polymorphism, Single Nucleotide, lcsh:Infectious and parasitic diseases, 03 medical and health sciences, Papua New Guinea, 0302 clinical medicine, Parasitic Sensitivity Tests, Genotype, parasitic diseases, Malaria, Vivax, Humans, lcsh:RC109-216, education, Genotyping, Genetics, 0303 health sciences, education.field_of_study, Dihydropteroate Synthase, 030306 microbiology, Haplotype, Methodology, Infant, DNA, Protozoan, biology.organism_classification, Virology, 3. Good health, High-Throughput Screening Assays, Tetrahydrofolate Dehydrogenase, Infectious Diseases, Child, Preschool, Mutation, Parasitology, Multidrug Resistance-Associated Proteins

Abstract

Background Reports of severe cases and increasing levels of drug resistance highlight the importance of improved Plasmodium vivax case management. Whereas monitoring P. vivax resistance to anti-malarial drug by in vivo and in vitro tests remain challenging, molecular markers of resistance represent a valuable tool for high-scale analysis and surveillance studies. A new high-throughput assay for detecting the most relevant markers related to P. vivax drug resistance was developed and assessed on Papua New Guinea (PNG) patient isolates. Methods Pvdhfr, pvdhps and pvmdr1 fragments were amplified by multiplex nested PCR. Then, PCR products were processed through an LDR-FMA (ligase detection reaction - fluorescent microsphere assay). 23 SNPs, including pvdhfr 57-58-61 and 173, pvdhps 382-383, 553, 647 and pvmdr1 976, were simultaneously screened in 366 PNG P. vivax samples. Results Genotyping was successful in 95.4% of the samples for at least one gene. The coexistence of multiple distinct haplotypes in the parasite population necessitated the introduction of a computer-assisted approach to data analysis. Whereas 73.1% of patients were infected with at least one wild-type genotype at codons 57, 58 and 61 of pvdhfr, a triple mutant genotype was detected in 65.6% of the patients, often associated with the 117T mutation. Only one patient carried the 173L mutation. The mutant 647P pvdhps genotype allele was approaching genetic fixation (99.3%), whereas 35.1% of patients were infected with parasites carrying the pvmdr1 976F mutant allele. Conclusions The LDR-FMA described here allows a discriminant genotyping of resistance alleles in the pvdhfr, pvdhps, and pvmdr1 genes and can be used in large-scale surveillance studies.

Published

2011

19. Salivary secretory leukocyte protease inhibitor and oral candidiasis in human immunodeficiency virus type 1-infected persons

Author

Gary D. Slade, Amit Chattopadhyay, Diane C. Shugars, Daniel J. Caplan, Hsaio Chuan Tien, Laurie R. Gray, and Lauren L. Patton

Subjects

Adult, Male, Saliva, Adolescent, medicine.medical_treatment, Immunology, Proteinase Inhibitory Proteins, Secretory, HIV Infections, Biology, Microbiology, Oropharyngeal Candidiasis, Candidiasis, Oral, Candida albicans, medicine, Humans, Secretory Leukocyte Peptidase Inhibitor, Mycosis, AIDS-Related Opportunistic Infections, Proteins, Immunosuppression, medicine.disease, biology.organism_classification, Corpus albicans, CD4 Lymphocyte Count, Infectious Diseases, Cross-Sectional Studies, Oral microbiology, Parasitology, Female, Fungal and Parasitic Infections, SLPI

Abstract

Oropharyngeal candidiasis, typically caused by Candida albicans , is the most common oral disease associated with human immunodeficiency virus type 1 (HIV-1) infection. Secretory leukocyte protease inhibitor (SLPI), a 12-kDa antiprotease, suppresses the growth of C. albicans in vitro. To determine whether the mucosal protein plays a role in protecting oral tissues against fungal infection, we conducted a cross-sectional study investigating the oral and systemic health and salivary SLPI levels in 91 dentate HIV-1-infected adults receiving medical care in the southeastern United States. Participants with a self-reported history of clinical oropharyngeal candidiasis during the previous 2 years constituted the test group ( n = 52), while the comparison group ( n = 39) had no oropharyngeal candidiasis during that period. Data collected from medical records, oral examination, and SLPI enzyme-linked immunosorbent assay quantitation of whole saliva were analyzed by t test, analysis of variance, linear regression, and unconditional logistic regression. The test group had a significantly higher mean salivary SLPI level than the comparison group (1.9 μg/ml versus 1.1 μg/ml, P < 0.05). Linear regression modeling identified CD4 cell count and history of oropharyngeal candidiasis as key predictors of salivary SLPI and revealed a significant interaction ( P < 0.05) between immunosuppression (CD4 cell count below 200 cells/μl) and positive history of oropharyngeal candidiasis in predicting salivary SLPI level. By logistic regression modeling, a salivary SLPI level exceeding 2.1 μg/ml, low CD4 count, antiretroviral monotherapy, and smoking were key predictors of oropharyngeal candidiasis. These data support a key role for SLPI in the oral mucosal defense against C. albicans . The antimicrobial mucosal protein may serve as an indicator of previous oropharyngeal candidiasis infection among immunosuppressed persons.

Published

2004

20. Construction, non-denaturing affinity purification, and characterization of baculovirally expressed human secretory leukocyte protease inhibitor

Author

Laurie R. Gray, Diane C. Shugars, and Audrey Alexander

Subjects

Proteases, Protein Denaturation, Proteinase Inhibitory Proteins, Secretory, Gene Expression, Spodoptera, Chromatography, Affinity, FLAG-tag, Affinity chromatography, Protein purification, Animals, Humans, Protease Inhibitors, Secretory Leukocyte Peptidase Inhibitor, Serine protease, Tandem affinity purification, biology, Proteins, Molecular biology, Enteropeptidase, Biochemistry, Protein Biosynthesis, biology.protein, Baculoviridae, Biotechnology, SLPI, Myc-tag

Abstract

Secretory leukocyte protease inhibitor (SLPI) is a 11.7 kDa mucosal protein with potent anti-microbial, anti-inflammatory, and wound healing activities. Previous efforts to express and purify the non-glycosylated cationic protein as a recombinant protein in bacteria required extensive denaturation and renaturation to refold the disulfide-rich protein into its biologically active form. To overcome this limitation, we have expressed human SLPI as a polyhistidine-tagged protein (bvHisSLPI) using a recombinant baculovirus expression system. Studies were conducted to determine the timing of maximal protein production following baculovirus infection of Sf21 cells. The 16.4 kDa-tagged protein was then overexpressed in Sf21 cells following a 48-h infection with bvHisSLPI-encoding baculovirus, purified by nickel-chelating affinity chromatography under non-denaturing conditions, and analyzed by Coomassie-stained SDS–polyacrylamide gel electrophoresis (SDS–PAGE) and Western blot. Purified bvHisSLPI was further characterized by enterokinase digestion to remove the polyhistidine tag from its N-terminus. In serine protease inhibition assays, purified bvHisSLPI blocked substrate cleavage by two serine proteases, chymotrypsin and cathepsin G, comparable to bacterially expressed SLPI. The baculovirus expression and affinity purification strategy described here will facilitate further studies of the structural and biological properties of this important multifunctional protein.

Published

2002

21. Differential Patterns of Infection and Disease with P. falciparum and P. vivax in Young Papua New Guinean Children

Author

Peter Siba, Leanne J. Robinson, Stuart Dobbie, Peter A. Zimmerman, Inoni Betuela, Sonja Schöpflin, Ivo Mueller, Annemarie Laumaea, Benson Kiniboro, Louis Schofield, Enmoore Lin, Laurie R. Gray, Danielle I. Stanisic, Melinda J. Blood-Zikursh, and Ingrid Felger

Subjects

Endemic Diseases, Plasmodium vivax, Prevalence, lcsh:Medicine, Public Health and Epidemiology/Infectious Diseases, Polymerase Chain Reaction, Cohort Studies, 0302 clinical medicine, Epidemiology, Malaria, Falciparum, lcsh:Science, 0303 health sciences, education.field_of_study, Multidisciplinary, Geography, biology, Incidence, Incidence (epidemiology), Age Factors, Public Health and Epidemiology/Global Health, 3. Good health, Child, Preschool, Cohort, Seasons, Research Article, Infectious Diseases/Epidemiology and Control of Infectious Diseases, medicine.medical_specialty, Plasmodium falciparum, 030231 tropical medicine, Population, Papua New Guinea, 03 medical and health sciences, Internal medicine, parasitic diseases, Malaria, Vivax, medicine, Humans, Insecticide-Treated Bednets, education, 030304 developmental biology, lcsh:R, Infectious Diseases/Protozoal Infections, Infant, biology.organism_classification, medicine.disease, Cross-Sectional Studies, Multivariate Analysis, Immunology, Leukocytes, Mononuclear, lcsh:Q, Public Health and Epidemiology/Epidemiology, Malaria, Follow-Up Studies

Abstract

BACKGROUND: Where P. vivax and P. falciparum occur in the same population the peak burden of P. vivax infection and illness is often concentrated in younger age groups. Experiences from malaria therapy patients indicate that immunity is acquired faster to P. vivax than to P. falciparum challenge. There is however little prospective data on the comparative risk of infection and disease from both species in young children living in co endemic areas. METHODOLOGY/PRINCIPAL FINDINGS: A cohort of 264 Papua New Guinean children aged 1 3 years (at enrolment) were actively followed up for Plasmodium infection and febrile illness for 16 months. Infection status was determined by light microscopy and PCR every 8 weeks and at each febrile episode. A generalised estimating equation (GEE) approach was used to analyse both prevalence of infection and incidence of clinical episodes. A more pronounced rise in prevalence of P. falciparum compared to P. vivax infection was evident with increasing age. Although the overall incidence of clinical episodes was comparable (P. falciparum: 2.56 P. vivax 2.46 episodes / child / yr) P. falciparum and P. vivax infectious episodes showed strong but opposing age trends: P. falciparum incidence increased until the age of 30 months with little change thereafter but incidence of P. vivax decreased significantly with age throughout the entire age range. For P. falciparum both prevalence and incidence of P. falciparum showed marked seasonality whereas only P. vivax incidence but not prevalence decreased in the dry season. CONCLUSIONS/SIGNIFICANCE: Under high perennial exposure children in PNG begin acquiring significant clinical immunity characterized by an increasing ability to control parasite densities below the pyrogenic threshold to P. vivax but not to P. falciparum in the 2(nd) and 3(rd) year of life. The ability to relapse from long lasting liver stages restricts the seasonal variation in prevalence of P. vivax infections.

Published

2010

22. Human endogenous retrovirus-K mRNA expression and genomic alignment data in hepatoblastoma

Author

David F Grabski, Aakrosh Ratan, Laurie R Gray, Stefan Bekiranov, David Rekosh, Marie-Louise Hammarskjold, and Sara K Rasmussen

Subjects

Human endogenous retrovirus-K, Hepatoblastoma, Transcriptome analysis, Genomic alignment, Computer applications to medicine. Medical informatics, R858-859.7, Science (General), Q1-390

Abstract

Human Endogenous Retroviruses are a class of genomic elements that are the result of ancient retroviral infection of the human germline. Many are biologically active elements that have been implicated in multiple diseases including cancer. The most recent class to invade the human genome is the HERV-K(HML-2) (HERV-K) family. Approximately 90 HERV-K proviruses and many smaller elements have been identified to date in the human genome. Additional proviruses are continually being discovered with the rapid advancement of deep-sequencing and long-read sequencing technologies. HERV-K proviruses are poorly annotated in human transcriptome databases making their analysis in RNA-seq data difficult. To enable analysis, we compiled the sequences of 91 HERV-K proviruses identified in NCBI GenBank (ID JN675007-JN675097) and created a proviral alignment tool for visualizing RNA-seq reads aligned across individual proviruses. This allowed us to analyse publicly available RNA-seq data from 10 hepatoblastoma samples and 3 normal liver controls (GEO Accession ID: GSE89775). This data report includes the raw FASTA sequence files of the HERV-K proviruses from NCBI, a differential gene expression list between hepatoblastoma samples, and genomic alignment figures from 5 HERV-K proviruses identified as differentially expressed in the companion research article “Upregulation of Human Endogenous Retrovirus-K (HML-2) mRNAs in hepatoblastoma: Identification of potential new immunotherapeutic targets and biomarkers [1]. The data provided here are available for other research groups interested in evaluating individual HERV-K proviral expression using RNA-seq data. Furthermore, the data analysis is highly flexible and will accommodate the addition of other HERV-K proviruses.

Published

2020