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1. Predominance of antibody-resistant SARS-CoV-2 variants in vaccine breakthrough cases from the San Francisco Bay Area, California

Author

Servellita, Venice, Morris, Mary Kate, Sotomayor-Gonzalez, Alicia, Gliwa, Amelia S., Torres, Erika, Brazer, Noah, Zhou, Alicia, Hernandez, Katherine T., Sankaran, Madeline, Wang, Baolin, Wong, Daniel, Wang, Candace, Zhang, Yueyuan, Reyes, Kevin R., Glasner, Dustin, Deng, Xianding, Streithorst, Jessica, Miller, Steve, Frias, Edwin, Rodgers, Mary, Cloherty, Gavin, Hackett, Jr., John, Hanson, Carl, Wadford, Debra, Philip, Susan, Topper, Scott, Sachdev, Darpun, and Chiu, Charles Y.

Published
2022
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3. Metagenomic sequencing with spiked primer enrichment for viral diagnostics and genomic surveillance

Author

Deng, Xianding, Achari, Asmeeta, Federman, Scot, Yu, Guixia, Somasekar, Sneha, Bártolo, Inês, Yagi, Shigeo, Mbala-Kingebeni, Placide, Kapetshi, Jimmy, Ahuka-Mundeke, Steve, Muyembe-Tamfum, Jean-Jacques, Ahmed, Asim A., Ganesh, Vijay, Tamhankar, Manasi, Patterson, Jean L., Ndembi, Nicaise, Mbanya, Dora, Kaptue, Lazare, McArthur, Carole, Muñoz-Medina, José E., Gonzalez-Bonilla, Cesar R., López, Susana, Arias, Carlos F., Arevalo, Shaun, Miller, Steve, Stone, Mars, Busch, Michael, Hsieh, Kristina, Messenger, Sharon, Wadford, Debra A., Rodgers, Mary, Cloherty, Gavin, Faria, Nuno R., Thézé, Julien, Pybus, Oliver G., Neto, Zoraima, Morais, Joana, Taveira, Nuno, R. Hackett, Jr., John, and Chiu, Charles Y.

Published
2020
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6. Author Correction: Metagenomic sequencing with spiked primer enrichment for viral diagnostics and genomic surveillance

Author

Deng, Xianding, Achari, Asmeeta, Federman, Scot, Yu, Guixia, Somasekar, Sneha, Bártolo, Inês, Yagi, Shigeo, Mbala-Kingebeni, Placide, Kapetshi, Jimmy, Ahuka-Mundeke, Steve, Muyembe-Tamfum, Jean-Jacques, Ahmed, Asim A., Ganesh, Vijay, Tamhankar, Manasi, Patterson, Jean L., Ndembi, Nicaise, Mbanya, Dora, Kaptue, Lazare, McArthur, Carole, Muñoz-Medina, José E., Gonzalez-Bonilla, Cesar R., López, Susana, Arias, Carlos F., Arevalo, Shaun, Miller, Steve, Stone, Mars, Busch, Michael, Hsieh, Kristina, Messenger, Sharon, Wadford, Debra A., Rodgers, Mary, Cloherty, Gavin, Faria, Nuno R., Thézé, Julien, Pybus, Oliver G., Neto, Zoraima, Morais, Joana, Taveira, Nuno, Hackett, Jr., John R., and Chiu, Charles Y.

Published
2020
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9. Chronic Human Pegivirus 2 without Hepatitis C Virus Co-infection.

Author

Coller, Kelly E., Bruce, Veronica, Cassidy, Michael, Gersch, Jeffrey, Frankel, Matthew B., Vallari, Ana, Cloherty, Gavin, Hackett Jr., John, Evans, Jennifer L., Page, Kimberly, Dawson, George J., and Hackett, John Jr

Subjects
HEPATITIS C virus, MIXED infections
Abstract

Most human pegivirus 2 (HPgV-2) infections are associated with past or current hepatitis C virus (HCV) infection. HPgV-2 is thought to be a bloodborne virus: higher prevalence of active infection has been found in populations with a history of parenteral exposure to viruses. We evaluated longitudinally collected blood samples obtained from injection drug users (IDUs) for active and resolved HPgV-2 infections using a combination of HPgV-2-specific molecular and serologic tests. We found evidence of HPgV-2 infection in 11.2% (22/197) of past or current HCV-infected IDUs, compared with 1.9% (4/205) of an HCV-negative IDU population. Testing of available longitudinal blood samples from HPgV-2-positive participants identified 5 with chronic infection (>6 months viremia in >3 timepoints); 2 were identified among the HCV-positive IDUs and 3 among the HCV-negative IDUs. Our findings indicate that HPgV-2 can establish chronic infection and replicate in the absence of HCV. [ABSTRACT FROM AUTHOR]

Published
2020
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10. Serologic Prevalence of Ebola Virus in Equatorial Africa.

Author

Steffen, Imke, Kai Lu, Yamamoto, Lauren K., Hoff, Nicole A., Mulembakani, Prime, Wemakoy, Emile O., Muyembe-Tamfum, Jean-Jacques, Ndembi, Nicaise, Brennan, Catherine A., Hackett Jr., John, Stramer, Susan L., Switzer, William M., Saragosti, Sentob, Mbensa, Guy O., Laperche, Syria, Rimoin, Anne W., Simmons, Graham, Lu, Kai, and Hackett, John Jr

Subjects
EBOLA virus, EBOLA virus disease, DISEASE prevalence, RISK exposure, SEROPREVALENCE
Abstract

We conducted a serologic survey of 2,430 serum samples collected during 1997-2012 for various studies to determine the prevalence of the hemorrhagic fever virus Ebola virus (EBOV) in equatorial Africa. We screened serum samples for neutralizing antibodies by using a pseudotype microneutralization assay and a newly developed luciferase immunoprecipitation system assay. Specimens seroreactive for EBOV were confirmed by using an ELISA. Our results suggest a serologic prevalence of 2%-3.5% in the Republic of the Congo and the Democratic Republic of the Congo, which have reported outbreaks of infection with EBOV. In addition we detected a seroprevalence of 1.3% in southern Cameroon, which indicated a low risk for exposure in this region. [ABSTRACT FROM AUTHOR]

Published
2019
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12. Xenotropic murine leukemia virus-related virus does not pose a risk to blood recipient safety

Author

Dodd, Roger Y., primary, Hackett Jr, John, additional, Linnen, Jeffrey M., additional, Dorsey, Kerri, additional, Wu, Yanyun, additional, Zou, Shimian, additional, Qiu, Xiaoxing, additional, Swanson, Priscilla, additional, Schochetman, Gerald, additional, Gao, Kui, additional, Carrick, James M., additional, Krysztof, David E., additional, and Stramer, Susan L., additional

Published
2011
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14. HIV-1 Strains Identified in Brazilian Blood Donors: Significant Prevalence of B/F1 Recombinants

Author

Brennan, Catherine A., primary, Brites, Carlos, additional, Bodelle, Pierre, additional, Golden, Alan, additional, Hackett, Jr., John, additional, Holzmayer, Vera, additional, Swanson, Priscilla, additional, Vallari, Ana, additional, Yamaguchi, Julie, additional, Devare, Sushil, additional, Pedroso, Celia, additional, Ramos, André, additional, and Badaro, Roberto, additional

Published
2007
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15. Failure to Identify HIV-infected Individuals in a Clinical Trial Using a Single HIV Rapid Test for Screening.

Author

Piwowar-Manning, Estelle, Fogel, Jessica M., Laeyendecker, Oliver, Shauna Wolf, Cummings, Vanessa, Marzinke, Mark A., Clarke, William, Breaud, Autumn, Wendel, Sarah, Lei Wang, Swanson, Priscilla, Hackett Jr., John, Mannheimer, Sharon, del Rio, Carlos, Kuo, Irene, Harawa, Nina T., Koblin, Beryl A., Moore, Richard, Blankson, Joel N., and Eshleman, Susan H.

Abstract

Background: In the HIV Prevention Trials Network (HPTN) 061 study, 8 (2.3%) of 348 HIV-infected participants identified as HIV uninfected at study enrollment using a single HIV rapid test for screening were found to be HIV infected after additional testing. Objectives: To evaluate the performance of different HIV assays for detection of HIV infection in HPTN 061 participants with missed infection and individuals with viral suppression. Methods: Plasma samples from 8 HPTN 061 participants, 17 elite controllers, and 101 individuals on antiretroviral treatment (ART) were tested for HIV with 3 rapid tests, 2 laboratory-based immunoassays, and a Western blot assay. The HPTN 061 samples were also tested with 2 HIV RNA assays and an antiretroviral drug assay. Results: Of the 8 HPTN 061 participants with missed infection, 1 was an elite controller, 1 was taking ART, 2 were missed because of testing or clerical errors, 1 had recent HIV infection (Identified using a multi-assay algorithm), and 3 had acute HIV infection. Two (1.7%) of 118 individuals with viral suppression (both taking ART) had at least 1 false-negative test. Conclusions: In clinical trials, HIV infections can be missed for a variety of reasons. Using more than one assay to screen for HIV infection may reduce the number of missed infections. [ABSTRACT FROM AUTHOR]

Published
2014
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16. Performance of Rapid Point-of-Care and Laboratory Tests for Acute and Established HIV Infection in San Francisco.

Author

Pilcher, Christopher D., Louie, Brian, Facente, Shelley, Keating, Sheila, Hackett Jr, John, Vallari, Ana, Hall, Chris, Dowling, Teri, Busch, Michael P., Klausner, Jeffrey D., Hecht, Frederick M., Liska, Sally, and Pandori, Mark W.

Subjects
DIAGNOSIS of HIV infections, POINT-of-care testing, CLINICAL pathology, HIV antibodies, GENETIC algorithms, IMMUNE complexes
Abstract

Background: Current laboratory and point-of-care tests for HIV detect different analytes and use different sample types. Some have fast turnaround times (<1 hour). We investigated how HIV test choice could impact case finding by testing programs. Methods: We analyzed 21,234 consecutive HIV tests with venous blood obtained by San Francisco HIV testing programs from 2003 to 2008. For a subset, oral fluid (n = 6446) or fingerstick blood (n = 8127) samples were also obtained for rapid testing. In all cases, HIV status was determined using an HIV antibody-plus-RNA test algorithm. We assessed how the screening antibody tests performed individually versus the gold standard of the full algorithm. We then evaluated the potential ability of other tests (including new tests) to detect more cases, by re-testing all specimens that had negative/discrepant antibody results on initial screening. Findings: The antibody-RNA algorithm identified 58 acute and 703 established HIV infection cases. 1st-generation (Vironostika) and 3rd-generation (Genetic Systems) immunoassays had 92 and 96 percent sensitivity, respectively. The Oraquick rapid test had clinical sensitivity of only 86 percent on oral fluid samples, but 92 percent on finger-stick blood. Newer 4th-generation, antigen-antibody combo rapid immunoassay (ARCHITECT) detected HIV in 87 percent of all the acute cases that had been missed by one of the previous screening assays. A point-of-care 4th generation antigen-antibody combo rapid test (Determine) detected about 54 percent of such acute cases. Conclusions: Our study suggests that some rapid antibody blood tests will give similar case detection to laboratory antibody tests, but that oral fluid testing greatly reduces ability to detect HIV. New 4th-generation combo tests can detect the majority of acute infections detectable by HIV RNA but with rapid results. Using these tests as a primary screening assay in high-risk HIV testing programs could reduce or eliminate the need for HIV RNA testing. [ABSTRACT FROM AUTHOR]

Published
2013
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17. Estimation of HIV Incidence in a Large, Community-Based, Randomized Clinical Trial: NIMH Project Accept (HIV Prevention Trials Network 043).

Author

Laeyendecker, Oliver, Piwowar-Manning, Estelle, Fiamma, Agnes, Kulich, Michal, Donnell, Deborah, Bassuk, Deb, Mullis, Caroline E., Chin, Craig, Swanson, Priscilla, Hackett Jr, John, Clarke, William, Marzinke, Mark, Szekeres, Greg, Gray, Glenda, Richter, Linda, Alexandre, Michel W., Chariyalertsak, Suwat, Chingono, Alfred, Celentano, David D., and Morin, Stephen F.

Subjects
HIV prevention, DISEASE incidence, CLINICAL trials, VIRAL disease diagnosis, APPLIED mathematics, COMMUNICABLE diseases
Abstract

Background: National Institute of Mental Health Project Accept (HIV Prevention Trials Network [HPTN] 043) is a large, Phase III, community-randomized, HIV prevention trial conducted in 48 matched communities in Africa and Thailand. The study intervention included enhanced community-based voluntary counseling and testing. The primary endpoint was HIV incidence, assessed in a single, cross-sectional, post-intervention survey of >50,000 participants. Methods: HIV rapid tests were performed in-country. HIV status was confirmed at a central laboratory in the United States. HIV incidence was estimated using a multi-assay algorithm (MAA) that included the BED capture immunoassay, an avidity assay, CD4 cell count, and HIV viral load. Results: Data from Thailand was not used in the endpoint analysis because HIV prevalence was low. Overall, 7,361 HIV infections were identified (4 acute, 3 early, and 7,354 established infections). Samples from established infections were analyzed using the MAA; 467 MAA positive samples were identified; 29 of those samples were excluded because they contained antiretroviral drugs. HIV prevalence was 16.5% (range at study sites: 5.93% to 30.8%). HIV incidence was 1.60% (range at study sites: 0.78% to 3.90%). Conclusions: In this community-randomized trial, a MAA was used to estimate HIV incidence in a single, cross-sectional post-intervention survey. Results from this analysis were subsequently used to compare HIV incidence in the control and intervention communities. Trial Registration: ClinicalTrials.gov NCT00203749 [ABSTRACT FROM AUTHOR]

Published
2013
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19. Prevalence of Xenotropic Murine Leukemia Virus-Related Virus Infection in Different Risk Populations in Spain.

Author

Arredondo, Mliguel, Hackett, Jr., John, de Bethencourt, Fermín R., Treviño, Ana, Escudero, Domingo, Collado, Antonio, Xiaoxing Qiu, Swanson, Priscilla, Sorianoi, Vincent, and de Mendoza, Carmen

Abstract

Human infection with the xenotropic murine leukemia virus-related virus (XMRV) has been associated controversially with prostate cancer and chronic fatigue syndrome. Information is lacking about the mechanisms of transmission and potential risk groups for XMRV infection. Plasma and peripheral blood mononuclear cells (PBMCs) from individuals with retroviral infections, chronic viral hepatitis, autoimmune diseases, prostate cancer, chronic fatigue syndrome, and blood donors were tested for XMRV markers. Antibodies to XMRV proteins pl5E and gp70 were examined using research assays. DNA extracted from PBMCs was tested for the presence of XMRV gag and env sequences. A total of 1103 specimens belonging to individuals with chronic fatigue syndrome and/or fibromyalgia (437), prostate cancer (69), HIV-1 (149), HTLV-1/2 (31), chronic hepatitis Β (81), chronic hepatitis C (72), autoimmune diseases (18), and blood donors (246) were examined. Overall, three samples (0.3%) were pl5E seroreactive (two HTLV-1 and one HCV patient). Another 15 (1.4%) were gp70 seroreactive (six chronic fatigue syndrome-fibromyalgia, four blood donors, two HIV-l, one prostate cancer, one HBV, and one HCV). Four specimens were initially positive for XMRV gag sequences, but none could be confirmed by repeated testing. In summary, no evidence of XMRV infection was found in populations with retroviral and viral hepatitis infections in Spain. Likewise, XMRV was not recognized in patients with autoimmune diseases, chronic fatigue syndrome-fibromyalgia, prostate cancer, or healthy blood donors. [ABSTRACT FROM AUTHOR]

Published
2012
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20. In-Depth Investigation of Archival and Prospectively Collected Samples Reveals No Evidence for XMRV Infection in Prostate Cancer.

Author

Lee, Deanna, Das Gupta, Jaydip, Gaughan, Christina, Steffen, Imke, Ning Tang, Ka-Cheung Luk, Xiaoxing Qiu, Urisman, Anatoly, Fischer, Nicole, Molinaro, Ross, Broz, Miranda, Schochetman, Gerald, Klein, Eric A., Ganem, Don, Derisi, Joseph L., Simmons, Graham, Hackett Jr., John, Silverman, Robert H., Chiu, Charles Y., and Tachedjian, Gilda

Subjects
PROSTATE cancer, VIRUSES, CANCER patients, CHRONIC fatigue syndrome, CELL lines
Abstract

XMRV, or xenotropic murine leukemia virus (MLV)-related virus, is a novel gammaretrovirus originally identified in studies that analyzed tissue from prostate cancer patients in 2006 and blood from patients with chronic fatigue syndrome (CFS) in 2009. However, a large number of subsequent studies failed to confirm a link between XMRV infection and CFS or prostate cancer. On the contrary, recent evidence indicates that XMRV is a contaminant originating from the recombination of two mouse endogenous retroviruses during passaging of a prostate tumor xenograft (CWR22) in mice, generating laboratory-derived cell lines that are XMRV-infected. To confirm or refute an association between XMRV and prostate cancer, we analyzed prostate cancer tissues and plasma from a prospectively collected cohort of 39 patients as well as archival RNA and prostate tissue from the original 2006 study. Despite comprehensive microarray, PCR, FISH, and serological testing, XMRV was not detected in any of the newly collected samples or in archival tissue, although archival RNA remained XMRV-positive. Notably, archival VP62 prostate tissue, from which the prototype XMRV strain was derived, tested negative for XMRV on reanalysis. Analysis of viral genomic and human mitochondrial sequences revealed that all previously characterized XMRV strains are identical and that the archival RNA had been contaminated by an XMRV-infected laboratory cell line. These findings reveal no association between XMRV and prostate cancer, and underscore the conclusion that XMRV is not a naturally acquired human infection. [ABSTRACT FROM AUTHOR]

Published
2012
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21. Absence of XMRV and Closely Related Viruses in Primary Prostate Cancer Tissues Used to Derive the XMRV-Infected Cell Line 22Rv1.

Author

Gupta, Jaydip Das, Luk, Ka-Cheung, Tang, Ning, Gaughan, Christina, Klein, Eric A., Kandel, Eugene S., Hackett, Jr., John, and Silverman, Robert H.

Subjects
CELL lines, PROSTATE cancer, CANCER cells, MOUSE leukemia viruses, XENOGRAFTS, FLUORESCENCE in situ hybridization
Abstract

The 22Rv1 cell line is widely used for prostate cancer research and other studies throughout the world. These cells were established from a human prostate tumor, CWR22, that was serially passaged in nude mice and selected for androgen independence. The 22Rv1 cells are known to produce high titers of xenotropic murine leukemia virus-related virus (XMRV). Recent studies suggested that XMRV was inadvertently created in the 1990's when two murine leukemia virus (MLV) genomes (pre-XMRV1 and pre-XMRV-2) recombined during passaging of the CWR22 tumor in mice. The conclusion that XMRV originated from mice and not the patient was based partly on the failure to detect XMRV in early CWR22 xenografts. While that deduction is certainly justified, we examined the possibility that a closely related virus could have been present in primary tumor tissue. Here we report that we have located the original prostate tumor tissue excised from patient CWR22 and have assayed the corresponding DNA by PCR and the tissue sections by fluorescence in situ hybridization for the presence of XMRV or a similar virus. The primary tumor tissues lacked mouse DNA as determined by PCR for intracisternal A type particle DNA, thus avoiding one of the limitations of studying xenografts. We show that neither XMRV nor a closely related virus was present in primary prostate tissue of patient CWR22. Our findings confirm and reinforce the conclusion that XMRV is a recombinant laboratory-generated mouse virus that is highly adapted for human prostate cancer cells. [ABSTRACT FROM AUTHOR]

Published
2012
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22. Failure to Detect XMRV-Specific Antibodies in the Plasma of CFS Patients Using Highly Sensitive Chemiluminescence Immunoassays.

Author

Oakes, Brendan, Xiaoxing Qiu, Levine, Susan, Hackett, Jr., John, and Huber, Brigitte T.

Subjects
MOUSE leukemia viruses, CHRONIC fatigue syndrome, CHEMILUMINESCENCE immunoassay, VIRAL antibodies, BLOOD testing, POLYMERASE chain reaction, PATIENTS
Abstract

In 2009, Lombardi et al. reported their startling finding that the gammaretrovirus xenotropic murine leukemia virus-related retrovirus (XMRV) is present in 67% of blood samples of patients suffering from chronic fatigue syndrome (CFS), as opposed to only 3.7% of samples from healthy individuals. However, we and others could not confirm these results, using a nested PCR assay. An alternative to this highly sensitive, but contamination-prone, technique is to measure the serological response to XMRV. Thus, we tested the plasma samples from our cohorts of CFS patients and healthy controls for the presence of XMRV-specific antibodies. Using two novel chemiluminescence immunoassays (CMIAs), we show that none of our samples have any XMRV-reactive antibodies. Taken together with our previous findings, we conclude that XMRV is not present in any human individual tested by us, regardless of CFS or healthy control. [ABSTRACT FROM AUTHOR]

Published
2011
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23. A Metagenomic Analysis of Pandemic Influenza A (2009 H1N1) Infection in Patients from North America.

Author

Greninger, Alexander L., Chen, Eunice C., Sittler, Taylor, Scheinerman, Alex, Roubinian, Nareg, Guixia Yu, Kim, Edward, Pillai, Dylan R., Guyard, Cyril, Mazzulli, Tony, Isa, Pavel, Arias, Carlos F., Hackett Jr., John, Schochetman, Gerald, Miller, Steve, Tang, Patrick, and Chiu, Charles Y.

Subjects
PANDEMICS, H1N1 influenza, PATHOGENIC microorganisms, PUBLIC health, COMMUNICABLE disease diagnosis, EPIDEMIOLOGY, RESPIRATORY infections, PATHOLOGY, GENE expression
Abstract

Although metagenomics has been previously employed for pathogen discovery, its cost and complexity have prevented its use as a practical front-line diagnostic for unknown infectious diseases. Here we demonstrate the utility of two metagenomics-based strategies, a pan-viral microarray (Virochip) and deep sequencing, for the identification and characterization of 2009 pandemic H1N1 influenza A virus. Using nasopharyngeal swabs collected during the earliest stages of the pandemic in Mexico, Canada, and the United States (n = 17), the Virochip was able to detect a novel virus most closely related to swine influenza viruses without a priori information. Deep sequencing yielded reads corresponding to 2009 H1N1 influenza in each sample (percentage of aligned sequences corresponding to 2009 H1N1 ranging from 0.0011% to 10.9%), with up to 97% coverage of the influenza genome in one sample. Detection of 2009 H1N1 by deep sequencing was possible even at titers near the limits of detection for specific RT-PCR, and the percentage of sequence reads was linearly correlated with virus titer. Deep sequencing also provided insights into the upper respiratory microbiota and host gene expression in response to 2009 H1N1 infection. An unbiased analysis combining sequence data from all 17 outbreak samples revealed that 90% of the 2009 H1N1 genome could be assembled de novo without the use of any reference sequence, including assembly of several near full-length genomic segments. These results indicate that a streamlined metagenomics detection strategy can potentially replace the multiple conventional diagnostic tests required to investigate an outbreak of a novel pathogen, and provide a blueprint for comprehensive diagnosis of unexplained acute illnesses or outbreaks in clinical and public health settings. [ABSTRACT FROM AUTHOR]

Published
2010
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24. Characterization of antibodies elicited by XMRV infection and development of immunoassays useful for epidemiologic studies.

Author

Xiaoxing Qiu, Swanson, Priscilla, Ka-Cheung Luk, Tu, Bailin, Villinger, Francois, Gupta, Jaydip Das, Silverman, Robert H., Klein, Eric A., Devare, Sushil, Schochetman, Gerald, and Hackett, Jr., John

Subjects
IMMUNOGLOBULINS, IMMUNOASSAY, MOUSE leukemia viruses, PROSTATE cancer, CHRONIC fatigue syndrome
Abstract

Background: Xenotropic Murine Leukemia Virus-related Virus (XMRV) is a human gammaretrovirus recently identified in prostate cancer tissue and in lymphocytes of patients with chronic fatigue syndrome. To establish the etiologic role of XMRV infection in human disease requires large scale epidemiologic studies. Development of assays to detect XMRV-specific antibodies would greatly facilitate such studies. However, the nature and kinetics of the antibody response to XMRV infection have yet to be determined. Results: Three rhesus macaques were infected with XMRV to determine the dynamics of the antibody responses elicited by infection with XMRV. All macaques developed antibodies to XMRV during the second week of infection, and the predominant responses were to the envelope protein gp70, transmembrane protein p15E, and capsid protein p30. In general, antibody responses to gp70 and p15E appeared early with higher titers than to p30, especially in the early period of seroconversion. Antibodies to gp70, p15E and p30 persisted to 158 days and were substantially boosted by re-infection, thus, were identified as useful serologic markers. Three high-throughput prototype assays were developed using recombinant proteins to detect antibodies to these viral proteins. Both gp70 and p15E prototype assays demonstrated 100% sensitivity by detecting all Western blot (WB) positive serial bleeds from the XMRV-infected macaques and good specificity (99.5-99.9%) with blood donors. Seroconversion sensitivity and specificity of the p30 prototype assay were 92% and 99.4% respectively. Conclusions: This study provides the first demonstration of seroconversion patterns elicited by XMRV infection. The nature and kinetics of antibody responses to XMRV in primates were fully characterized. Moreover, key serologic markers useful for detection of XMRV infection were identified. Three prototype immunoassays were developed to detect XMRV-specific antibodies. These assays demonstrated good sensitivity and specificity; thus, they will facilitate large scale epidemiologic studies of XMRV infection in humans. [ABSTRACT FROM AUTHOR]

Published
2010
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26. The Prevalence of Diverse HIV-1 Strains Was Stable in Cameroonian Blood Donors From 1996 to 2004.

Author

Brennan, Catherine A., Bodelle, Pierre, Coffey, Ruthie, Devare, Sushil G., Golden, Alan, Hackett, Jr., John, Harris, Barbara, Holzmayer, Vera, Luk, Ka-Cheung, Schochetman, Gerald, Swanson, Priscilla, Yamaguchi, Julie, Vallari, Ana, Ndembi, Nicaise, Ngansop, Charlotte, Makamche, Florence, Mbanya, Dora, Gürtler, Lutz G., Zekeng, Leopold, and Kaptué, Lazare

Published
2008
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27. Xenotropic murine leukemia virus-related virus does not pose a risk to blood recipient safety.

Author

Dodd, Roger Y., Hackett Jr, John, Linnen, Jeffrey M., Dorsey, Kerri, Wu, Yanyun, Zou, Shimian, Qiu, Xiaoxing, Swanson, Priscilla, Schochetman, Gerald, Gao, Kui, Carrick, James M., Krysztof, David E., and Stramer, Susan L.

Subjects
*MOUSE leukemia viruses, *CHRONIC fatigue syndrome, *BLOOD donors, *BLOOD transfusion, *IMMUNOGLOBULINS, *RNA
Abstract

BACKGROUND: When xenotropic murine leukemia virus-related virus (XMRV) was first reported in association with chronic fatigue syndrome, it was suggested that it might offer a risk to blood safety. Thus, the prevalence of the virus among blood donors and, if present, its transmissibility by transfusion need to be defined. STUDY DESIGN AND METHODS: Two populations of routine blood donor samples (1435 and 13,399) were obtained for prevalence evaluations; samples from a linked donor-recipient repository were also evaluated. Samples were tested for the presence of antibodies to XMRV-related recombinant antigens and/or for XMRV RNA, using validated, high-throughput systems. RESULTS: The presence of antibodies to XMRV could not be confirmed among a total of 17,249 blood donors or recipients (0%; 95% confidence interval [CI], 0%-0.017%); 1763 tested samples were nonreactive for XMRV RNA (0%; 95% CI, 0%-0.17%). Evidence of infection was absent from 109 recipients and 830 evaluable blood samples tested after transfusion of a total of 3741 blood components. CONCLUSIONS: XMRV and related murine leukemia virus (MLV) markers are not present among a large population of blood donors and evidence of transfusion transmission could not be detected. Thus, these viruses do not currently pose a threat to blood recipient safety and further actions relating to XMRV and MLV are not justified. [ABSTRACT FROM AUTHOR]

Published
2012
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28. Seroprevalence of xenotropic murine leukemia virus-related virus in normal and retrovirus-infected blood donors.

Author

Qiu, Xiaoxing, Swanson, Priscilla, Tang, Ning, Leckie, Gregor W., Devare, Sushil G., Schochetman, Gerald, and Hackett Jr, John

Subjects
MOUSE leukemia viruses, CHRONIC fatigue syndrome, BLOOD donors, HIV, REVERSE transcriptase polymerase chain reaction, IMMUNOGLOBULINS
Abstract

BACKGROUND: Xenotropic murine leukemia virus-related virus (XMRV) has been reported in patients with prostate cancer and chronic fatigue syndrome. Although results have been conflicting, the potential of XMRV as an infectious human retrovirus has raised concerns about transfusion safety. To address this issue, normal and retrovirus-infected blood donors were screened for evidence of XMRV infection. STUDY DESIGN AND METHODS: Plasma from 1000 US, 100 human immunodeficiency virus Type 1-infected Cameroonian, and 642 human T-lymphotropic virus Type I (HTLV-I)-infected or uninfected Japanese blood donors as well as 311 sexually transmitted disease diagnostic specimens were screened for antibodies to XMRV gp70 and p15E using chemiluminescent immunoassays (CMIAs). CMIA-reactive samples were evaluated by p30 CMIA, Western blot, and real-time reverse transcriptase polymerase chain reaction. RESULTS: XMRV seroreactivity was low (0%-0.6%) with the exception of the HTLV-I-infected donors (4.9%). Antibody was detected against only a single XMRV protein (p15E or gp70); none of the seroreactive samples had detectable XMRV pol or env sequences. The elevated seroreactivity in HTLV-I-infected donors was due to an increased p15E seroreactive rate (4.1%). Inspection of XMRV and HTLV sequences revealed a high level of conservation within the immunodominant region (IDR) of the transmembrane protein. In some cases, HTLV IDR peptide competitively reduced the XMRV p15E signal. CONCLUSIONS: Based on the low prevalence of seroreactivity, detection of antibody to only a single XMRV protein and the absence of XMRV sequences, this study finds no compelling evidence of XMRV in normal or retrovirus-infected blood donors. The increased p15E seroreactivity observed in HTLV infection is likely due to cross-reactive antibodies. [ABSTRACT FROM AUTHOR]

Published
2012
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29. Prevalence of XMRV in blood donors, HTLV and HIV cohorts.

Author

Xiaoxing Qiu, Swanson, Priscilla, Ning Tang, Leckie, Gregor W., Devare, Sushil, Schochetman, Gerald, and Hackett, Jr., John

Subjects
MOUSE leukemia viruses, HTLV, BLOOD donors
Abstract

An abstract of the research paper titled,"Prevalence of Xenotropic murine leukemia virus-related virus (XMRV) in blood donors, HTLV and HIV cohorts,"is presented.

Published
2011
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30. A prototype RT-PCR assay for detection of XMRV in multiple human sample types.

Author

Ning Tang, Frank, Andrea, Kowal, Robert, Leckie, Gregor, Hackett, Jr., John, Simmons, Graham, Busch, Michael, and Abravaya, Klara

Subjects
MOUSE leukemia viruses, CANCER cells
Abstract

An abstract of the research paper titled,"A prototype RT-PCR assay for detection of Xenotropic murine leukemia virus-related virus (XMRV) in multiple human sample types,"is presented.

Published
2011
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31. XMRV replicates preferentially in mucosal sites in vivo: Relevance to XMRV transmission?

Author

Villinger, Francois, Das Gupta, Jaydip, Onlamoon, Nattawat, Molinaro, Ross, Suppiah, Suganthi, Sharma, Prachi, Rogers, Kenneth, Gaughan, Christina, Klein, Eric, Xiaoxing Qiu, Schochetman, Gerald, Hackett, Jr., John, and Silverman, Robert H.

Subjects
RETROVIRUSES, RETROVIRUS diseases
Abstract

An abstract of the research paper titled,"Xenotropic murine leukemia virus-related virus (XMRV) replicates preferentially in mucosal cites in vivo: Relevance to XMRV transmission?", is presented.

Published
2011
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32. The Perils of Pathogen Discovery: Origin of a Novel Parvovirus-Like Hybrid Genome Traced to Nucleic Acid Extraction Spin Columns.

Author

Naccache, Samia N., Greninger, Alexander L., Lee, Deanna, Coffey, Lark L., Tung Phan, Rein-Weston, Annie, Aronsohn, Andrew, Hackett Jr., John, Delwart, Eric L., and Chiua, Charles Y.

Subjects
*DNA viruses, *PARVOVIRUSES, *NUCLEOTIDE sequence, *PATHOGENIC microorganisms, *NUCLEIC acid isolation methods, *COLUMNS, *HEPATITIS, *CHINESE people, *AMINO acids, *DISEASES
Abstract

Next-generation sequencing was used for discovery and de novo assembly of a novel, highly divergent DNA virus at the interface between the Parvoviridae and Circoviridae. The virus, provisionally named parvovirus-like hybrid virus (PHV), is nearly identical by sequence to another DNA virus, NIH-CQV, previously detected in Chinese patients with seronegative (non-A-E) hepatitis. Although we initially detected PHV in a wide range of clinical samples, with all strains sharing~99% nucleotide and amino acid identity with each other and with NIH-CQV, the exact origin of the virus was eventually traced to contaminated silica-binding spin columns used for nucleic acid extraction. Definitive confirmation of the origin of PHV, and presumably NIH-CQV, was obtained by in-depth analyses of water eluted through contaminated spin columns. Analysis of environmental metagenome libraries detected PHV sequences in coastal marine waters of North America, suggesting that a potential association between PHV and diatoms (algae) that generate the silica matrix used in the spin columns may have resulted in inadvertent viral contamination during manufacture. The confirmation of PHV/NIH-CQV as laboratory reagent contaminants and not bona fide infectious agents of humans underscores the rigorous approach needed to establish the validity of new viral genomes discovered by nextgeneration sequencing. [ABSTRACT FROM AUTHOR]

Published
2013
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33. ARCHITECT® HIV Ag/Ab Combo assay: Correlation of HIV-1 p24 antigen sensitivity and RNA viral load using genetically diverse virus isolates

Author

Brennan, Catherine A., Yamaguchi, Julie, Vallari, Ana, Swanson, Priscilla, and Hackett Jr, John R.

Subjects
*DIAGNOSIS of HIV infections, *HIV, *HIV antibodies, *RNA, *BIOLOGICAL assay, *CELL culture, *VIRUS isolation
Abstract

Abstract: Background: HIV antigen/antibody (Ag/Ab) combination assays represent a significant advancement in assays used for diagnosing HIV infection based on their ability to detect acute and chronic infections. During acute HIV infection (AHI), detection depends on assay sensitivity for p24 Ag. Objective: To directly compare the Ag sensitivity of the ARCHITECT® HIV Ag/Ab Combo assay to RNA viral load using cell culture supernatants of virus isolates. HIV-1 isolates allow correlation in the total absence of an antibody response to infection and across genetically diverse HIV-1 group M strains. Methods: Thirty-five HIV-1 isolates comprising subtypes A–D, F and G, CRF01_AE, CRF02_AG, and unique recombinant forms were evaluated. Cell-free culture supernatant for each isolate was diluted to four levels and tested in the HIV Combo assay to determine a signal to cutoff ratio and the RealTime® HIV-1 assay to quantify RNA. The RNA copies/mL at the HIV Combo assay cutoff was determined. Results: The median RNA copies/mL at the HIV Combo assay cutoff was 57,900 for individual virus isolates (range 26,440–102,400). A single plot of all the data gave a value of 58,500RNA copies/mL. An analysis of data published for acute HIV infection in human subjects gave a similar result; HIV Combo detected 97% of AHIs with RNA copies/mL>30,700. Conclusions: Based on analysis of virus isolates, the ARCHITECT HIV Combo assay can detect p24 Ag when RNA is above approximately 58,000copies/mL. The correlation of viral load and Ag sensitivity was consistent across genetically diverse HIV-1 group M strains. [Copyright &y& Elsevier]

Published
2013
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34. Failure to Confirm XMRV/MLVs in the Blood of Patients with Chronic Fatigue Syndrome: A Multi-Laboratory Study.

Author

Simmons, Graham, Glynn, Simone A., Komaroff, Anthony L., Mikovits, Judy A., Tobler, Leslie H., Hackett Jr., John, Ning Tang, Switzer, William M., Heneine, Walid, Hewlett, Indira K., Jiangqin Zhao, Shyh-Ching Lo, Alter, Harvey J., Linnen, Jeffrey M., Kui Gao, Coffin, John M., Kearney, Mary F., Ruscetti, Francis W., Pfost, Max A., and Bethel, James

Subjects
*SECONDARY analysis, *BLOOD testing, *CHRONIC fatigue syndrome, *MOUSE leukemia viruses, *RESEARCH methodology, *BLIND experiment, *PATIENTS
Abstract

Murine leukemia viruses (MLVs), including xenotropic-MLV-related virus (XMRV), have been controversially linked to chronic fatigue syndrome (CFS). To explore this issue in greater depth, we compiled coded replicate samples of blood from 15 subjects previously reported to be XMRV/MLV-positive (14 with CFS) and from 15 healthy donors previously determined to be negative for the viruses. These samples were distributed in a blinded fashion to nine laboratories, which performed assays designed to detect XMRV/MLV nucleic acid, virus replication, and antibody. Only two laboratories reported evidence of XMRV/MLVs; however, replicate sample results showed disagreement, and reactivity was similar among CFS subjects and negative controls. These results indicate that current assays do not reproducibly detect XMRV/NILV in blood samples and that blood donor screening is not warranted. [ABSTRACT FROM AUTHOR]

Published
2011
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35. No Evidence of Murine-Like Gammaretroviruses in CFS Patients Previously Identified as XMRV-Infected.

Author

Knox, Konstance, Carrigan, Donald, Simmons, Graham, Teque, Fernando, Yanchen Zhou, Hackett Jr., John, Xiaoxing Qiu, Ka-Cheung Luk, Schochetman, Gerald, Knox, Allyn, Kogelnik, Andreas M., and Levy, Jay A.

Subjects
*CHRONIC fatigue syndrome, *ETIOLOGY of diseases, *RETROVIRUS diseases, *MOUSE leukemia viruses, *DIAGNOSTIC use of polymerase chain reaction, *REVERSE transcriptase polymerase chain reaction, *VIRAL antibodies, *NUCLEIC acids
Abstract

Members of the gammaretroviruses--such as murine leukemia viruses (MLVs), most notably XMRV [xenotropic murine leukemia virus (X-MLV)-related virus--have been reported to be present in the blood of patients with chronic fatigue syndrome (CFS). We evaluated blood samples from 61 patients with CFS from a single clinical practice, 43 of whom had previously been identified as XMRV-positive. Our analysis included polymerase chain reaction and reverse transcription polymerase chain reaction procedures for detection of viral nucleic acids and assays for detection of infectious virus and virus-specific antibodies. We found no evidence of XMRV or other MLVs in these blood samples. In addition, we found that these gammaretroviruses were strongly (X-MLV) or partially (XMRV) susceptible to inactivation by sera from CFS patients and healthy controls, which suggested that establishment of a successful MLV infection in humans would be unlikely. Consistent with previous reports, we detected MLV sequences in commercial laboratory reagents. Our results indicate that previous evidence (inking XMRV and MLVs to CFS is likely attributable to laboratory contamination. [ABSTRACT FROM AUTHOR]

Published
2011
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