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1. Detection of Nucleocapsid Antibodies Associated with Primary SARS-CoV-2 Infection in Unvaccinated and Vaccinated Blood Donors

Author

Grebe, Eduard, Stone, Mars, Spencer, Bryan R., Akinseye, Akintunde, Wright, David J., Di Germanio, Clara, Bruhn, Roberta, Zurita, Karla G., Contestable, Paul, Green, Valerie, Lanteri, Marion C., Saa, Paula, Biggerstaff, Brad J., Coughlin, Melissa M., Kleinman, Steve, Custer, Brian, Jones, Jefferson M., and Busch, Michael P.

Subjects
Immunoassay -- Usage, Viral antibodies -- Measurement -- Health aspects, Antibodies -- Measurement -- Health aspects, Blood donors -- Health aspects
Abstract

In the United States, as in many countries, convenience sample serosurveillance studies (e.g., in blood donors) have demonstrated that most of the population has SARS-CoV-2 antibodies from vaccination, infection, or [...]

Published
2024
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4. Implementing pathogen reduction technology while discontinuing blood donor deferral criteria for sexual risk behaviors: A simulation study.

Author

Domingue, Marie‐Pier, O'Brien, Sheila F., Grégoire, Yves, Lanteri, Marion C., Stramer, Susan L., Camirand Lemyre, Félix, and Lewin, Antoine

Subjects
HEPATITIS C virus, HEPATITIS B virus, LITERATURE reviews, AT-risk behavior, HIV, BLOOD transfusion reaction
Abstract

Background: Combining pathogen reduction technology (PRT) with blood screening may alleviate concerns over the risk of transfusion‐transmitted infections (TTI) and support changes in blood donor selection to potentially increase blood availability. This study aimed to estimate the residual risk of human immunodeficiency virus (HIV), hepatitis B virus (HBV), and hepatitis C virus (HCV) transfusion‐transmission in Canada after implementing PRT, while eliminating deferrals for sexual risk behaviors. Study Design and Methods: A probabilistic approach that combined Bayesian networks with Monte Carlo simulations was used to estimate the risk of transfusing HIV‐, HBV‐, or HCV‐contaminated blood components. Different scenarios were considered to compare the current residual risk after PRT implementation, with and without donor deferral criteria for sexual risk behaviors. Donor profiles and blood component outcomes were simulated based on a literature review including the prevalence and incidence of HIV, HBV, and HCV in the Canadian blood donor population; the use of current blood screening assays; and HIV, HBV, and HCV blood donor viral loads. Results: In the universal PRT scenario (i.e., with PRT/without deferral criteria), the estimated risks of HIV, HBV, and HCV transmission were significantly lower than those in the currently observed scenario (i.e., without PRT/with deferral criteria). Conclusions: This risk model suggests that PRT for platelets and plasma (and eventually for RBCs when available) significantly reduces the residual risks of HIV, HBV and HCV transfusion‐transmission and could enable the removal of blood donor deferral criteria for sexual risk behaviors. [ABSTRACT FROM AUTHOR]

Published
2024
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5. SARS‐CoV‐2 antibody levels and long COVID occurrence in blood donors.

Author

Avelino‐Silva, Vivian I., Bruhn, Roberta, Zurita, Karla G., Deng, Xutao, Yu, Elaine A., Grebe, Eduard, Stone, Mars, Lanteri, Marion C., Spencer, Bryan R., Busch, Michael P., and Custer, Brian

Subjects
POST-acute COVID-19 syndrome, SERODIAGNOSIS, VACCINATION status, HIERARCHICAL clustering (Cluster analysis), BLOOD testing
Abstract

Background: Long COVID is a common condition lacking consensus definition; determinants remain incompletely understood. Characterizing immune profiles associated with long COVID could support the development of preventive and therapeutic strategies. Methods: We used a survey to investigate blood donors' infection/vaccination history and acute/persistent symptoms following COVID‐19. The prevalence of long COVID was evaluated using self‐report and an adapted definition from the RECOVER study. We evaluated factors associated with long COVID, focusing on anti‐spike and anti‐nucleocapsid SARS‐CoV‐2 antibodies. Lastly, we investigated long COVID clinical subphenotypes using hierarchical clustering. Results: Of 33,610 participants, 16,003 (48%) reported having had COVID‐19; 1853 (12%) had self‐reported long COVID, 685 (4%) met an adapted RECOVER definition, and 2050 (13%) met at least one definition. Higher anti‐nucleocapsid levels measured 12–24 weeks post‐infection were associated with higher risk of self‐reported and RECOVER long COVID. Higher anti‐spike IgG levels measured 12–24 weeks post‐infection were associated with lower risk of self‐reported long COVID. Higher total anti‐spike measured 24–48 weeks post‐infection was associated with lower risk of RECOVER long COVID. Cluster analysis identified four clinical subphenotypes; patterns included neurological and psychiatric for cluster 1; neurological and respiratory for cluster 2; multi‐systemic for cluster 3; and neurological for cluster 4. Discussion: Long COVID prevalence in blood donors varies depending on the adopted definition. Anti‐SARS‐CoV‐2 antibodies were time‐dependently associated with long COVID; higher anti‐nucleocapsid levels were associated with higher risk; and higher anti‐spike levels were associated with lower risk of long COVID. Different underlying pathophysiologic mechanisms may be associated with distinct clinical subphenotypes. [ABSTRACT FROM AUTHOR]

Published
2024
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7. Estimates of SARS-CoV-2 Seroprevalence and Incidence of Primary SARS-CoV-2 Infections Among Blood Donors, by COVID-19 Vaccination Status--United States, April 2021-September 2022

Author

Jones, Jefferson M., Manrique, Irene Molina, Stone, Mars S., Grebe, Eduard, Saa, Paula, Germanio, Clara D., Spencer, Bryan R., Notari, Edward, Bravo, Marjorie, Lanteri, Marion C., Green, Valerie, Briggs-Hagen, Melissa, Coughlin, Melissa M., Stramer, Susan L., Opsomer, Jean, and Busch, Michael P.

Subjects
Vaccination -- Health aspects, Medical research -- Health aspects, Medicine, Experimental -- Health aspects, Infection -- Health aspects, Blood donors -- Health aspects, Health
Abstract

Changes in testing behaviors and reporting requirements have hampered the ability to estimate the U.S. SARS-CoV-2 incidence (1). Hybrid immunity (immunity derived from both previous infection and vaccination) has been [...]

Published
2023

8. End of selection criteria based on sexual orientation: An international symposium on alternatives to donation deferral.

Author

Lewin, Antoine, Goldman, Mindy, Busch, Michael P., Davison, Katy, van de Laar, Thijs, Tiberghien, Pierre, Shinar, Eilat, O'Brien, Sheila F., Lambert, Gilles, Field, Stephen, Hervig, Tor, Tan, Darrell H. S., Custer, Brian, Drews, Steven J., Lanteri, Marion C., Klochkov, Denis, Widmer, Eleonora, Domingue, Marie‐Pier, Renaud, Christian, and Germain, Marc

Subjects
SEXUAL orientation, HIV, ANAL sex, BISEXUAL men, HIGH-income countries
Abstract

Background and Objectives: Until recently, gay, bisexual and other men who have sex with men (MSM) were deferred from donating blood for 3–12 months since the last male‐to‐male sexual contact. This MSM deferral has been discontinued by several high‐income countries (HIC) that now perform gender‐neutral donor selection. Materials and Methods: An international symposium (held on 20‐04‐2023) gathered experts from seven HICs to (1) discuss how this paradigm shift might affect the mitigation strategies for transfusion‐transmitted infections and (2) address the challenges related to gender‐neutral donor selection. Results: Most countries employed a similar approach for implementing a gender‐neutral donor selection policy: key stakeholders were consulted; the transition was bridged by time‐limited deferrals; donor compliance was monitored; and questions or remarks on anal sex and the number and/or type of sexual partners were often added. Many countries have now adopted a gender‐neutral approach in which questions on pre‐ and post‐exposure prophylaxis for human immunodeficiency virus (HIV) have been added (or retained, when already in place). Other countries used mitigation strategies, such as plasma quarantine or pathogen reduction technologies for plasma and/or platelets. Conclusion: The experience with gender‐neutral donor selection has been largely positive among the countries covered herein and seems to be acceptable to stakeholders, donors and staff. The post‐implementation surveillance data collected so far appear reassuring with regards to safety, although longer observation periods are necessary. The putative risks associated with HIV antiretrovirals should be further investigated. [ABSTRACT FROM AUTHOR]

Published
2024
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11. Blood Gene Signatures of Changas Cardiomyopathy With or Without Ventricular Dysfunction

Author

Ferreira, Ludmila Rodrigues Pinto, Ferreira, Frederico Moraes, Nakaya, Helder Imoto, Deng, Xutao, da Silva Cândido, Darlan, de Oliveira, Lea Campos, Billaud, Jean-Noel, Lanteri, Marion C., Rigaud, Vagner Oliveira-Carvalho, Seielstad, Mark, Kalil, Jorge, Fernandes, Fabio, Ribeiro, Antonio Luiz P., Sabino, Ester Cerdeira, and Cunha-Neto, Edecio

Published
2017

13. Syphilis seroprevalence and incidence in US blood donors from 2020 to 2022.

Author

Conti, Galen, Notari, Edward P, Dodd, Roger Y., Kessler, Debra, Custer, Brian, Reik, Rita, Lanteri, Marion C., Hailu, Benyam, Yang, Hong, and Stramer, Susan L.

Subjects
SYPHILIS, BLOOD donors, SEROPREVALENCE
Abstract

Background: HIV, HBV, and HCV infections for ~60% of the US blood supply are monitored by TTIMS with syphilis added in 2020. Study Design and Methods: Data were compiled from October 2020 to September 2022. Syphilis prevalence was estimated for allogeneic and directed donors who were consensus positive (CP) and the subset of those with confirmed‐active infections (AI). Prevalence and incidence were stratified by demographics for two consecutive 1‐year periods, starting October 1, 2020 and for both years combined. Incidence was estimated for repeat donors. Associations between syphilis positivity and other infections were evaluated. Results: Among 14.75 million donations, syphilis prevalence was 28.4/100,000 donations and significantly higher during the second year compared to the first year. Overall, syphilis incidence for the two‐year period was 10.8/100,000 person‐years. The adjusted odds of a CP infection were 1.18 (95% CI: 1.11, 1.26) times higher in the second year compared to the first, and for AI, 1.22 (95% CI: 1.10, 1.35) times higher in year 2. Highest rates occurred among males, first‐time, Black, and younger (ages 18–39) donors, and those in the South US Census region. Syphilis CP donors were 64 (95% CI: 46, 89) times more likely to be HIV CP, and AI donors 77 (95% CI: 52, 114) times more likely to be HIV CP than non‐CP donors, when controlling for confounders. Summary/Conclusions: Syphilis prevalence increased over the study period mirroring national trends reported by CDC and is significantly associated with HIV CP. [ABSTRACT FROM AUTHOR]

Published
2024
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14. Multiple-ancestry genome-wide association study identifies 27 loci associated with measures of hemolysis following blood storage

Author

Page, Grier P., Kanias, Tamir, Guo, Yuelong J., Lanteri, Marion C., Zhang, Xu, Mast, Alan E., Cable, Ritchard G., Spencer, Bryan R., Kiss, Joseph E., Fang, Fang, Endres-Dighe, Stacy M., Brambilla, Donald, Nouraie, Mehdi, Gordeuk, Victor R., Kleinman, Steve, Busch, Michael P., and Gladwin, Mark T.

Subjects
Hemolysis and hemolysins -- Genetic aspects, Sickle cell anemia -- Genetic aspects -- Risk factors, Genetic research, Genetic variation -- Research, Blood donors -- Genetic aspects, Hemolytic anemia -- Genetic aspects -- Risk factors, Health care industry
Abstract

Background. The evolutionary pressure of endemic malaria and other erythrocytic pathogens has shaped variation in genes encoding erythrocyte structural and functional proteins, influencing responses to hemolytic stress during transfusion and disease. Methods. We sought to identify such genetic variants in blood donors by conducting a genome-wide association study (GWAS) of 12,353 volunteer donors, including 1,406 African Americans, 1,306 Asians, and 945 Hispanics, whose stored erythrocytes were characterized by quantitative assays of in vitro osmotic, oxidative, and cold-storage hemolysis. Results. GWAS revealed 27 significant loci (P < 5 * [10.sup.-8]), many in candidate genes known to modulate erythrocyte structure, metabolism, and ion channels, including SPTA1, ALDH2, ANK1, HK1, MAPKAPK5, AQP1, PIEZO1, and SLC4A1/band 3. GWAS of oxidative hemolysis identified variants in genes encoding antioxidant enzymes, including GLRX, GPX4, G6PD, and SEC14L4 (Golgi-transport protein). Genome-wide significant loci were also tested for association with the severity of steady-state (baseline) in vivo hemolytic anemia in patients with sickle cell disease, with confirmation of identified SNPs in HBA2, G6PD, PIEZO1, AQP1, and SEC14L4. Conclusions. Many of the identified variants, such as those in G6PD, have previously been shown to impair erythrocyte recovery after transfusion, associate with anemia, or cause rare Mendelian human hemolytic diseases. Candidate SNPs in these genes, especially in polygenic combinations, may affect RBC recovery after transfusion and modulate disease severity in hemolytic diseases, such as sickle cell disease and malaria., Introduction Blood transfusion is one of the most common procedures during hospital stays, with more than 36,000 red blood cell (RBC) transfusions performed daily in the United States. Clinically, RBC [...]

Published
2021
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25. Plasma transfusion–transmission of Zika virus in mice and macaques.

Author

Van Rompay, Koen K. A., Coffey, Lark L., Yee, JoAnn L., Singapuri, Anil, Stuart, Jackson, Lanteri, Marion C., Santa Maria, Felicia, Lu, Kai, Singh, Inderdeep, Bakkour, Sonia, Stone, Mars, Williamson, Phillip C., Muench, Marcus O., Busch, Michael P., and Simmons, Graham

Subjects
ZIKA virus, MACAQUES, NUCLEIC acid amplification techniques
Abstract

Background: Zika virus (ZIKV) epidemics with infections in pregnant women are associated with severe neurological disease in newborns. Although an arbovirus, ZIKV is also blood transfusion‐transmitted (TT). Greater knowledge of the efficiency of ZIKV TT would aid decisions on testing and pathogen reduction technologies (PRT). Study Design and Methods: Plasma units from ZIKV RNA‐reactive blood donors were used to study infectivity in vitro, in mice, and in macaques. Furthermore, plasma units were subjected to PRT using amotosalen/ultraviolet light A (A/UVA) before transfusion. Results: In vitro infectivity of ZIKV RNA‐reactive plasma varied between 100 and 1000 international units (IU) of ZIKV RNA. Immunodeficient mice were more sensitive with as low as 32 IU sufficient to infect 50% of mice. 50–5500 IU of RNA led to TT in macaques using dose escalation of three different RNA‐positive, seronegative plasma units. In contrast, RNA‐reactive units collected postseroconversion were not infectious in macaques, even at a dose of 9 million IU RNA. After A/UVA PRT, transfusion of plasma containing up to 18 million IU was no longer infectious in vitro and did not result in ZIKV TT in macaques. Conclusion: Significant risks of ZIKV TT are likely confined to a relatively short viremic window before seroconversion, and that sensitive nucleic acid amplification testing likely identifies the majority of infectious plasma. PRT was demonstrated to be effective at preventing ZIKV TT. Considering that there is no approved ZIKV vaccine, these data are relevant to mitigate the risk of TT during the future ZIKV outbreaks. [ABSTRACT FROM AUTHOR]

Published
2023
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30. Tregs control the development of symptomatic West Nile virus infection in humans and mice

Author

Lanteri, Marion C., O'Brien, Katie M., Purtha, Whitney E., Cameron, Mark J., Lund, Jennifer M., Owen, Rachel E., Heitman, John W., Custer, Brian, Hirschkorn, Dale F., Tobler, Leslie H., Kiely, Nancy, Prince, Harry E., Ndhlovu, Lishomwa C., Nixon, Douglas F., Kamel, Hany T., Kelvin, David J., Busch, Michael P., Rudensky, Alexander Y., Diamond, Michael S., and Norris, Philip J.

Subjects
West Nile fever -- Risk factors -- Research, T cells -- Research -- Health aspects, Immunocompromised host -- Diseases -- Medical examination -- Research -- Risk factors, Health care industry
Abstract

West Nile virus (WNV) causes asymptomatic infection in most humans, but for undefined reasons, approximately 20% of immunocompetent individuals develop West Nile fever, a potentially debilitating febrile illness, and approximately 1% develop neuroinvasive disease syndromes. Notably, since its emergence in 1999, WNV has become the leading cause of epidemic viral encephalitis in North America. We hypothesized that [CD4.sup.+] Tregs might be differentially regulated in subjects with symptomatic compared with those with asymptomatic WNV infection. Here, we show that in 32 blood donors with acute WNV infection, Tregs expanded significantly in the 3 months after index ([RNA.sup.+]) donations in all subjects. Symptomatic donors exhibited lower Treg frequencies from 2 weeks through 1 year after index donation yet did not show differences in systemic T cell or generalized inflammatory responses. In parallel prospective experimental studies, symptomatic WNV-infected mice also developed lower Treg frequencies compared with asymptomatic mice at 2 weeks after infection. Moreover, Treg-deficient mice developed lethal WNV infection at a higher rate than controls. Together, these results suggest that higher levels of peripheral Tregs after infection protect against severe WNV disease in immunocompetent animals and humans., Introduction West Nile virus (WNV), an encephalitic positive polarity RNA virus of the Flaviviridae family, was first isolated in 1937 in the West Nile district of Uganda from the blood [...]

Published
2009
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31. Mitigating the risk of transfusion‐transmitted infections with vector‐borne agents solely by means of pathogen reduction.

Author

Stramer, Susan L., Lanteri, Marion C., Brodsky, Jaye P., Foster, Gregory A., Krysztof, David E., Groves, Jamel A., Townsend, Rebecca L., Notari, Edward, Bakkour, Sonia, Stone, Mars, Simmons, Graham, Spencer, Bryan, Tonnetti, Laura, and Busch, Michael P.

Abstract

Background: This study evaluated whether pathogen reduction technology (PRT) in plasma and platelets using amotosalen/ultraviolet A light (A/UVA) or in red blood cells using amustaline/glutathione (S‐303/GSH) may be used as the sole mitigation strategy preventing transfusion‐transmitted West Nile (WNV), dengue (DENV), Zika (ZIKV), and chikungunya (CHIKV) viral, and Babesia microti, Trypanosoma cruzi, and Plasmodium parasitic infections. Methods: Antibody (Ab) status and pathogen loads (copies/mL) were obtained for donations from US blood donors testing nucleic acid (NAT)‐positive for WNV, DENV, ZIKV, CHIKV, and B. microti. Infectivity titers derived from pathogen loads were compared to published PRT log10 reduction factors (LRF); LRFs were also reviewed for Plasmodium and T. cruzi. The potential positive impact on donor retention following removal of deferrals from required questioning and testing for WNV, Babesia, Plasmodium, and T. cruzi was estimated for American Red Cross (ARC) donors. Results: A/UVA and S‐303/GSH reduced infectivity to levels in accordance with those recognized by FDA as suitable to replace testing for all agents evaluated. If PRT replaced deferrals resulting from health history questions and/or NAT for WNV, Babesia, Plasmodium, and T. cruzi, 27,758 ARC donors could be retained allowing approximately 50,000 additional donations/year based on 1.79 donations/donor for calendar year 2019 (extrapolated to an estimated 125,000 additional donations nationally). Conclusion: Pathogen loads in donations from US blood donors demonstrated that robust PRT may provide an opportunity to replace deferrals associated with donor questioning and NAT for vector‐borne agents allowing for significant donor retention and likely increased blood availability. [ABSTRACT FROM AUTHOR]

Published
2022
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32. Robust inactivation of Plasmodium falciparum in red blood cell concentrates using amustaline and glutathione pathogen reduction.

Author

Sow, Cissé, Bouissou, Amélie, Girard, Yvette A., Singh, Gurvani B., Bounaadja, Lotfi, Payrat, Jean‐Marc, Haas, Delphine, Isola, Hervé, Lanteri, Marion C., Bringmann, Peter, and Grellier, Philippe

Abstract

Background: Plasmodium falciparum is the parasite responsible for most malaria cases globally. The risk of transfusion‐transmitted malaria (TTM) is mitigated by donor deferrals and blood screening strategies, which adversely impact blood availability. Previous studies showed robust inactivation of P. falciparum using nucleic acid‐targeting pathogen reduction technologies (PRT) for the treatment of plasma and platelet components or whole blood (WB). The efficacy of the amustaline–glutathione (GSH) PRT to inactivate P. falciparum is here evaluated in red blood cells (RBC), as well the impact of PRT on parasite loads, stages, and strains. Study Design and Methods: RBC units resuspended in AS‐1 or AS‐5 additive solutions were spiked with ring stage‐infected RBC and treated with the amustaline–GSH PRT. Parasite loads and viability were measured in samples at the time of contamination, and after treatment, using serial 10‐fold dilutions of the samples in RBC cultures maintained for up to 4 weeks. Results: P. falciparum viability assays allow for the detection of very low levels of parasite. Initial parasite titer was >5.2 log10/ml in AS‐1/5 RBC. No infectious parasites were detected in amustaline–GSH‐treated samples after 4 weeks of culture. Amustaline–GSH inactivated high parasite loads regardless of parasite stages and strains. Amustaline readily penetrates the parasite, irreversibly blocks development, and leads to parasite death and expulsion from RBC. Discussion: Amustaline–GSH PRT demonstrated robust efficacy to inactivate malaria parasites in RBC concentrates. This study completes the portfolio of studies demonstrating the efficacy of nucleic acid‐targeting PRTs to mitigate TTM risks as previously reported for platelet concentrates, plasma, and WB. [ABSTRACT FROM AUTHOR]

Published
2022
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33. Quantitative restoration of immune defense in old animals determined by naive antigen‐specific CD8 T‐cell numbers.

Author

Uhrlaub, Jennifer L., Jergović, Mladen, Bradshaw, Christine M., Sonar, Sandip, Coplen, Christopher P., Dudakov, Jarrod, Murray, Kristy O., Lanteri, Marion C., Busch, Michael P., van den Brink, Marcel R. M., and Nikolich‐Žugich, Janko

Subjects
ANIMAL defenses, T cells, CD8 antigen, WEST Nile virus, LABORATORY mice, PROTEIN microarrays
Abstract

Older humans and animals often exhibit reduced immune responses to infection and vaccination, and this often directly correlates to the numbers and frequency of naive T (Tn) cells. We found such a correlation between reduced numbers of blood CD8+ Tn cells and severe clinical outcomes of West Nile virus (WNV) in both humans naturally exposed to, and mice experimentally infected with, WNV. To examine possible causality, we sought to increase the number of CD8 Tn cells by treating C57BL/6 mice with IL‐7 complexes (IL‐7C, anti‐IL‐7 mAb bound to IL‐7), shown previously to efficiently increase peripheral T‐cell numbers by homeostatic proliferation. T cells underwent robust expansion following IL‐7C administration to old mice increasing the number of total T cells (>fourfold) and NS4b:H‐2Db‐restricted antigen‐specific CD8 T cells (twofold). This improved the numbers of NS4b‐specific CD8 T cells detected at the peak of the response against WNV, but not survival of WNV challenge. IL‐7C‐treated old animals also showed no improvement in WNV‐specific effector immunity (neutralizing antibody and in vivo T‐cell cytotoxicity). To test quantitative limits to which CD8 Tn cell restoration could improve protective immunity, we transferred graded doses of Ag‐specific precursors into old mice and showed that injection of 5400 (but not of 1800 or 600) adult naive WNV‐specific CD8 T cells significantly increased survival after WNV. These results set quantitative limits to the level of Tn reconstitution necessary to improve immune defense in older organisms and are discussed in light of targets of immune reconstitution. [ABSTRACT FROM AUTHOR]

Published
2022
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38. Sepsis from an apheresis platelet contaminated with Acinetobacter calcoaceticus/baumannii complex bacteria and Staphylococcus saprophyticus after pathogen reduction.

Author

Fridey, Joy L., Stramer, Susan L., Nambiar, Ashok, Moayeri, Morvarid, Bakkour, Sonia, Langelier, Charles, Crawford, Emily, Lu, Thea, Lanteri, Marion C., Kamm, Jack, Miller, Steve, Wagner, Stephen J., Benjamin, Richard J., and Busch, Michael P.

Subjects
ACINETOBACTER baumannii, PERIPHERALLY inserted central catheters, ACINETOBACTER, STAPHYLOCOCCUS, SEPSIS, BACTERIAL contamination, BLOOD transfusion reaction, GRAM-negative aerobic bacteria, BLOOD platelet transfusion, BACTERIAL diseases, PLATELETPHERESIS
Abstract

Background: Strategies to reduce platelet (PLT) bacterial contamination include donor screening, skin disinfection, sample diversion, bacterial culture, pathogen reduction (PR), and day-of-transfusion tests. We report bacterial sepsis following a pathogen-reduced PLT transfusion.Case Report: An adult male with relapsed acute lymphoblastic leukemia was successfully treated for central catheter-associated Staphylococcus aureus bacteremia. A peripherally inserted central catheter (PICC) was placed. Chills, rigors, and flushing developed immediately after PICC-infused pathogen-reduced PLTs, progressing to septic shock requiring intensive care management.Methods: PICC and peripheral blood (PB), transfused bag saline flushes (TBFs), environmental samples, and the pathogen-reduced untransfused co-component (CC) were cultured. Plasma metagenomic and bacterial isolate whole-genome sequencing; PLT mitochondrial DNA (mtDNA) testing of untransfused CC and TBF; CC testing for amotosalen (S-59)/S-59 photoproducts; isolate PR studies (INTERCEPT); and TBF polymerase chain reaction for recipient Y-chromosome DNA were performed.Results: PB and PICC cultures grew Acinetobacter calcoaceticus/baumannii complex (ACBC). TBF was gram-positive; mass spectrometry identified ACBC and Staphylococcus saprophyticus (SS). CC Gram stain and cultures were negative. Environmental cultures, some done after decontamination, were ACBC/SS negative. Posttransfusion patient plasma and TBF ACBC sequences were genetically identical. No Y-chromosome signal was detected in TBF. S-59 photoproducts and evidence of mtDNA amplification inhibition were found in the CC. Spiking PR studies showed >5.9-log inactivation for both isolates. Donor skin cultures for Acinetobacter were negative.Conclusion: CC sterility, PR studies, residual S-59 photoproducts, and mtDNA amplification inhibition suggest successful PR. Unidentified environmental sources and inherent or acquired bag defects may have contributed to postmanufacturing pathogen-reduced PLT contamination. [ABSTRACT FROM AUTHOR]

Published
2020
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39. Inactivation of a broad spectrum of viruses and parasites by photochemical treatment of plasma and platelets using amotosalen and ultraviolet A light.

Author

Lanteri, Marion C., Santa‐Maria, Felicia, Laughhunn, Andrew, Girard, Yvette A., Picard‐Maureau, Marcus, Payrat, Jean‐Marc, Irsch, Johannes, Stassinopoulos, Adonis, Bringmann, Peter, Santa-Maria, Felicia, Picard-Maureau, Marcus, and Payrat, Jean-Marc

Abstract

Background: The INTERCEPT Blood System pathogen reduction technology (PRT), which uses amotosalen and ultraviolet A light treatment (amotosalen/UV-PRT), inactivates pathogens in plasma and platelet components (PCs). This review summarizes data describing the inactivation efficacy of amotosalen/UVA-PRT for a broad spectrum of viruses and parasites.Methods: Twenty-five enveloped viruses, six nonenveloped viruses (NEVs), and four parasites species were evaluated for sensitivity to amotosalen/UVA-PRT. Pathogens were spiked into plasma and PC at high titers. Samples were collected before and after PRT and assessed for infectivity with cell cultures or animal models. Log reduction factors (LRFs) were defined as the difference in infectious titers before and after amotosalen/UV-PRT.Results: LRFs of ≥4.0 log were reported for 19 pathogens in plasma (range, ≥4.0 to ≥7.6), 28 pathogens in PC in platelet additive solution (PC-PAS; ≥4.1-≥7.8), and 14 pathogens in PC in 100% plasma (PC-100%; (≥4.3->8.4). Twenty-five enveloped viruses and two NEVs were sensitive to amotosalen/UV-PRT; LRF ranged from >2.9 to ≥7.6 in plasma, 2.4 or greater to greater than 6.9 in PC-PAS and >3.5 to >6.5 in PC-100%. Infectious titers for four parasites were reduced by >4.0 log in all PC and plasma (≥4.9 to >8.4).Conclusion: Amotosalen/UVA-PRT demonstrated effective infectious titer reduction for a broad spectrum of viruses and parasites. This confirms the capacity of this system to reduce the risk of viral and parasitic transfusion-transmitted infections by plasma and PCs in various geographies. [ABSTRACT FROM AUTHOR]

Published
2020
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40. Inactivation of Plasmodium falciparum in whole blood using the amustaline and glutathione pathogen reduction technology.

Author

Sow, Cissé, Laughhunn, Andrew, Girard, Yvette A., Lanteri, Marion C., Amar El Dusouqui, Soraya, Stassinopoulos, Adonis, and Grellier, Philippe

Subjects
PLASMODIUM falciparum, ERYTHROCYTES, BLOOD testing, BLOOD
Abstract

Background: Risk of transfusion-transmitted (TT) malaria is mainly associated with whole blood (WB) or red blood cell (RBC) transfusion. Risk mitigation relies mostly on donor deferral while a limited number of countries perform blood testing, both negatively impacting blood availability. This study investigated the efficacy of the pathogen reduction system using amustaline and glutathione (GSH) to inactivate Plasmodium falciparum in WB.Study Design and Methods: WB units were spiked with ring stage P. falciparum infected RBCs. Parasite loads were measured in samples at time of infection, after 24 hours at room temperature (RT), and after a 24-hour incubation at RT post-treatment with 0.2 mM amustaline and 2 mM GSH. Serial 10-fold dilutions of the samples were inoculated to RBC cultures and maintained up to 4 weeks. Parasitemia was quantified by cytometry.Results: The P. falciparum viability assay has a limit of detection of a single live parasite per sample. Input parasite titer was >5.7 log10 TCID50 per mL. A 24-hour incubation at RT paused parasite development in controls, but they retained viability and infectivity when tested in culture. In contrast, no infectious parasites were detected in the amustaline/GSH-treated sample after 4 weeks of culture.Conclusion: A robust level of P. falciparum inactivation was achieved in WB using amustaline/GSH treatment. Parasite log reduction was >5.7 log10 TCID50 per mL. Development of such a pathogen reduction system may provide an opportunity to reduce the risk of TT malaria and improve blood availability. [ABSTRACT FROM AUTHOR]

Published
2020
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41. Inactivation of yellow fever virus with amotosalen and ultraviolet A light pathogen-reduction technology.

Author

Girard, Yvette A., Santa Maria, Felicia, and Lanteri, Marion C.

Subjects
YELLOW fever, PHYTOPLASMAS, ULTRAVIOLET radiation, TECHNOLOGY, BLOOD transfusion, PHOTOSENSITIZERS, FLAVIVIRUSES, BLOOD platelets, VIRUS inactivation, IMPACT of Event Scale, PLATELETPHERESIS, PHARMACODYNAMICS
Abstract

Background: The reemergence of yellow fever virus (YFV) in Africa and Brazil, and massive vaccine campaigns triggered to contain the outbreaks, have raised concerns over blood transfusion safety and availability with increased risk of YFV transfusion-transmitted infections (TTIs) by native and vaccine-acquired YFV. Blood donor deferral for 2 to 4 weeks following live attenuated YFV vaccination, and deferral for travel to endemic/epidemic areas, may result in blood donor loss and impact platelet component (PC) stocks. This study investigated the efficacy of INTERCEPT Blood System pathogen reduction (PR) with use of amotosalen and ultraviolet A (UVA) light to inactivate high levels of YFV in PCs.Materials: Four units of apheresis platelets prepared in 35% plasma/65% platelet additive solution (PC-PAS) and 4 units of PC in 100% human plasma (PC-Plasma) were spiked with high infectious titers of YFV (YFV-17D vaccine strain). YFV-17D infectious titers were measured by plaque assay and expressed as plaque-forming units (PFU) before and after amotosalen/UVA treatment to determine log reduction.Results: The mean YFV-17D infectious titers in PC before inactivation were 5.5 ± 0.1 log PFU/mL in PC-PAS and 5.3 ± 0.1 log PFU/mL in PC-Plasma. No infectivity was detected immediately after amotosalen/UVA treatment.Conclusion: The amotosalen/UVA PR system inactivated high titers of infectious YFV-17D in PC. This PR technology could reduce the risk of YFV TTI and help secure PC supplies in areas experiencing YFV outbreaks where massive vaccination campaigns are required. [ABSTRACT FROM AUTHOR]

Published
2020
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42. Progress towards an appropriate pathogen reduction technology for whole blood in Africa.

Author

El Dusouqui, Soraya Amar, Lanteri, Marion C., Schwabe, Rudolf, Grzesiczek, Anja, North, Anne, Mufti, Nina, Sekongo, Yassongui Mamadou, Pitman, John, and Tagny, Claude Tayou

Subjects
*BLOOD, *RED Cross & Red Crescent, *NUCLEIC acids, *PATHOGENIC microorganisms, *TECHNOLOGY
Abstract

Background Interest in an effective pathogen reduction technology (PRT) for whole blood (WB) tailored to address specific needs of limited-resource settings is growing. The Swiss Red Cross Humanitarian Foundation (SRCHF) supports a clinical programme to promote PRT for WB in resource-limited settings where rates of WB use and transfusion-transmitted infections are high. Pathogen reduction technology for whole blood Cerus Corporation (INTERCEPT® Blood System) and Terumo BCT (Mirasol®) are investing in clinical trials for redblood-cell (RBC) and WB PRT. The SRCHF selected the INTERCEPT WB PRT for its clinical programme in Africa based on data related to the INTERCEPT system's pathogen reduction effectiveness and the company's goal of producing a processing kit requiring minimal electricity. Adapting the INTERCEPT RBC PRT for WB The INTERCEPT PRT for RBC and WB uses amustaline (0-2 mM) to irreversibly cross-link nucleic acids and glutathione (GSH) (20 mM for RBC and 2 mM for WB) to quench unreacted amustaline. Laboratory and clinical trial results for the RBC PRT form the basis for the WB PRT. Preliminary studies have demonstrated preservation of RBC quality in amustaline/GSH-treated WB. A Phase 1 safety trial in Côte d'Ivoire and development of a WB processing kit requiring limited electricity are described. Discussion Assessing the clinical safety of a WB PRT under local conditions is a positive step in the development of a suitable WB PRT for low-resource settings. [ABSTRACT FROM AUTHOR]

Published
2020
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43. Documentation of transfusion-transmitted arbovirus infections in endemic areas

Author

Musso, Didier, Gould, Ernest, Lanteri, Marion C., Unité de Recherche sur les Maladies Infectieuses et Tropicales Emergentes (URMITE), Institut de Recherche pour le Développement (IRD)-Aix Marseille Université (AMU)-Institut National de la Santé et de la Recherche Médicale (INSERM)-IFR48, INSB-INSB-Centre National de la Recherche Scientifique (CNRS), Emergence des Pathologies Virales (EPV), Institut National de la Santé et de la Recherche Médicale (INSERM)-Institut de Recherche pour le Développement (IRD)-Aix Marseille Université (AMU)-Assistance Publique - Hôpitaux de Marseille (APHM), Institut des sciences biologiques (INSB-CNRS)-Institut des sciences biologiques (INSB-CNRS)-Centre National de la Recherche Scientifique (CNRS), and Institut de Recherche pour le Développement (IRD)-Aix Marseille Université (AMU)-Assistance Publique - Hôpitaux de Marseille (APHM)-Institut National de la Santé et de la Recherche Médicale (INSERM)

Subjects
[SDV.MHEP.MI]Life Sciences [q-bio]/Human health and pathology/Infectious diseases, ComputingMilieux_MISCELLANEOUS
Abstract

International audience; no abstract

Published
2016

44. In vitro evaluation of pathogen inactivated platelet quality: An 8 year experience of routine use in Galicia, Spain.

Author

Castrillo Fernández, Azucena, Lanteri, Marion C., Arcas Otero, Carina, Díaz Pereira, Almudena, and Adelantado Pérez, Maria

Subjects
*ERYTHROCYTES, *BLOOD platelet activation, *PH standards, *QUALITY control, *QUALITY standards
Abstract

Abstract Background Platelet concentrates (PCs) treated by the pathogen inactivation technology (PI) using amotosalen and UVA illumination (PI-PCs) can be manufactured in additive solutions (PAS-III and PAS-IIIM) or in 100% Plasma. Quality control (QC) is an integral part of the production. We capitalized on our ongoing QC program to capture 8 years-worth of data on parameters related to the quality of 116,214 PI-PCs produced under different manufacturing methods. Materials and methods Selected in vitro parameters of metabolism, activation, and storage were analyzed for the different manufacturing periods to compare PI-PCs versus conventional PCs (C-PCs) resuspended in different PAS. Results and discussion All BC-PCs met quality standards for pH and dose and residual leucocytes. As expected, storage time correlated with increased lactate, LDH, Annexin V, CD62, sCD40 L levels and decreased glucose and pH. With PAS-IIIM, higher levels of glucose were observed toward the end of shelf life (p < 0.0001) with lower platelet activation markers Annexin V (p = 0.038) and CD62 (p = 0.0006). Following PI implementation, a low expire rate of <0.5% was observed. While a 2.3% mean increase in the production of PCs occurred from 2011 to 2015, the distribution of red blood cell concentrates dropped by 4.4%. A mean incidence of 0.14% for transfusion-related adverse reaction was observed while PI-PCs were distributed, similar to the one observed with C-PCs. Overall, PI-PCs prepared in additive solutions consistently met quality standards. Those prepared in PAS-IIIM appeared to have better retention of in vitro characteristics compared to PAS-III though all demonstrated functionality and clinical effectiveness. [ABSTRACT FROM AUTHOR]

Published
2019
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45. Intradonor reproducibility and changes in hemolytic variables during red blood cell storage: results of recall phase of the REDS-III RBC-Omics study.

Author

Lanteri, Marion C., Kanias, Tamir, Keating, Sheila, Stone, Mars, Guo, Yuelong, Page, Grier P., Brambilla, Donald J., Endres‐Dighe, Stacy M., Mast, Alan E., Bialkowski, Walter, D'Andrea, Pam, Cable, Ritchard G., Spencer, Bryan R., Triulzi, Darrell J., Murphy, Edward L., Kleinman, Steven, Gladwin, Mark T., Busch, Michael P., Endres-Dighe, Stacy M, and NHLBI Recipient Epidemiology Donor Evaluation Study (REDS)-III Program

Subjects
*ERYTHROCYTES, *BLOOD donors, *BLOOD platelets, *OXIDATIVE stress, *BLOOD collection, *ERYTHROCYTE metabolism, *DYNAMICS, *HEMOLYSIS & hemolysins, *OSMOSIS, *OXIDATION-reduction reaction, RESEARCH evaluation
Abstract

Background: Genetic determinants may underlie the susceptibility of red blood cells (RBCs) to hemolyze in vivo and during routine storage. This study characterized the reproducibility and dynamics of in vitro hemolysis variables from a subset of the 13,403 blood donors enrolled in the RBC-Omics study.Study Design and Methods: RBC-Omics donors with either low or high hemolysis results on 4°C-stored leukoreduced (LR)-RBC samples from enrollment donations stored for 39 to 42 days were recalled 2 to 12 months later to donate LR-RBCs. Samples of stored LR-RBCs from the unit and from transfer bags were evaluated for spontaneous and stress-induced hemolysis at selected storage time points. Intradonor reproducibility of hemolysis variables was evaluated in transfer bags over two donations. Hemolysis data at serial storage time points were generated on LR-RBCs from parent bags and analyzed by site, sex, race/ethnicity, and donation frequency.Results: A total of 664 donors were successfully recalled. Analysis of intradonor reproducibility revealed that osmotic and oxidative hemolysis demonstrated good and moderate reproducibility (Pearson's r = 0.85 and r = 0.53, respectively), while spontaneous hemolysis reproducibility was poor (r = 0.40). Longitudinal hemolysis in parent bags showed large increases over time in spontaneous (508.6%) and oxidative hemolysis (399.8%) and smaller increases in osmotic (9.4%) and mechanical fragility (3.4%; all p < 0.0001).Conclusion: Spontaneous hemolysis is poorly reproducible in donors over time and may depend on site processing methods, while oxidative and osmotic hemolysis were reproducible in donors and hence could reflect consistent heritable phenotypes attributable to genetic traits. Spontaneous and oxidative hemolysis increased over time of storage, whereas osmotic and mechanical hemolysis remained relatively stable. [ABSTRACT FROM AUTHOR]

Published
2019
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46. Piloting and implementation of quality assessment and quality control procedures in RBC-Omics: a large multi-center study of red blood cell hemolysis during storage.

Author

Stone, Mars, Keating, Sheila M., Kanias, Tamir, Lanteri, Marion C., Lebedeva, Mila, Sinchar, Derek, Hampton, Dylan, Jakub, Adam, Rychka, Val, Brewer, Greg, Bakkour, Sonia, Gefter, Nelly, Murcia, Karla, Page, Grier P., Endres‐Dighe, Stacy, Bialkowski, Walter, Fu, Xiaoyun, Zimring, Jim, Raife, Thomas J., and Kleinman, Steve

Subjects
HEMOLYSIS & hemolysins, ERYTHROCYTES, BLOOD collection, BLOOD donors, BLOOD testing, ADENOSINE triphosphate metabolism, ERYTHROCYTE metabolism, QUALITY control, RESEARCH funding
Abstract

Background: The major aims of the RBC-Omics study were to evaluate the genomic and metabolomic determinants of spontaneous and stress-induced hemolysis during RBC storage. This study was unique in scale and design to allow evaluation of RBC donations from a sufficient number of donors across the spectrum of race, ethnicity, sex, and donation intensity. Study procedures were carefully piloted, optimized, and controlled to enable high-quality data collection.Methods: The enrollment goal of 14,000 RBC donors across four centers, with characterization of RBC hemolysis across two testing laboratories, required rigorous piloting and optimization and establishment of a quality assurance (QA) and quality control (QC) program. Optimization of WBC elution from leukoreduction (LR) filters, development and validation of small-volume transfer bags, impact of manufacturing and sample-handling procedures on hemolysis parameters, and testing consistency across laboratories and technicians and over time were part of this quality assurance/quality control program.Results: LR filter elution procedures were optimized for obtaining DNA for analysis. Significant differences between standard and pediatric storage bags led to use of an alternative LR-RBC transfer bag. The impact of sample preparation and freezing methods on metabolomics analyses was evaluated. Proficiency testing monitored and documented testing consistency across laboratories and technicians.Conclusion: Piloting and optimization, and establishment of a robust quality assurance/quality control program documented process consistency throughout the study and was essential in executing this large-scale multicenter study. This program supports the validity of the RBC-Omics study results and a sample repository that can be used in future studies. [ABSTRACT FROM AUTHOR]

Published
2019
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47. Frequent blood donations alter susceptibility of red blood cells to storage- and stress-induced hemolysis.

Author

Kanias, Tamir, Stone, Mars, Page, Grier P., Guo, Yuelong, Endres‐Dighe, Stacy M., Lanteri, Marion C., Spencer, Bryan R., Cable, Ritchard G., Triulzi, Darrell J., Kiss, Joseph E., Murphy, Edward L., Kleinman, Steve, Gladwin, Mark T., Busch, Michael P., Mast, Alan E., Endres-Dighe, Stacy M, and NHLBI Recipient Epidemiology Donor Evaluation Study (REDS)-III Program

Subjects
DIRECTED blood donations, ERYTHROCYTES, HEMOLYSIS & hemolysins, BLOOD diseases, OXIDATIVE stress, IRON metabolism, BLOOD collection, IRON, MULTIVARIATE analysis, RESEARCH funding
Abstract

Background: Frequent whole blood donations increase the prevalence of iron depletion in blood donors, which may subsequently interfere with normal erythropoiesis. The purpose of this study was to evaluate the associations between donation frequency and red blood cell (RBC) storage stability in a racially/ethnically diverse population of blood donors.Study Design: Leukoreduced RBC concentrate-derived samples from 13,403 donors were stored for 39 to 42 days (1-6°C) and then evaluated for storage, osmotic, and oxidative hemolysis. Iron status was evaluated by plasma ferritin measurement and self-reported intake of iron supplements. Donation history in the prior 2 years was obtained for each subject.Results: Frequent blood donors enrolled in this study were likely to be white, male, and of older age (56.1 ± 5.0 years). Prior donation intensity was negatively associated with oxidative hemolysis (p < 0.0001) in multivariate analyses correcting for age, sex, and race/ethnicity. Increased plasma ferritin concentration was associated with increased RBC susceptibility to each of the three measures of hemolysis (p < 0.0001 for all), whereas self-reported iron intake was associated with reduced susceptibility to osmotic and oxidative hemolysis (p < 0.0001 for both).Conclusions: Frequent blood donations may alter the quality of blood components by modulating RBC predisposition to hemolysis. RBCs collected from frequent donors with low ferritin have altered susceptibility to hemolysis. Thus, frequent donation and associated iron loss may alter the quality of stored RBC components collected from iron-deficient donors. Further investigation is necessary to assess posttransfusion safety and efficacy in patients receiving these RBC products. [ABSTRACT FROM AUTHOR]

Published
2019
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48. Blood, sweat, and tears: Red Blood Cell-Omics study objectives, design, and recruitment activities.

Author

Endres‐Dighe, Stacy M., Guo, Yuelong, Kanias, Tamir, Lanteri, Marion, Stone, Mars, Spencer, Bryan, Cable, Ritchard G., Kiss, Joseph E., Kleinman, Steve, Gladwin, Mark T., Brambilla, Donald J., D'Andrea, Pam, Triulzi, Darrell J., Mast, Alan E., Page, Grier P., Busch, Michael P., Endres-Dighe, Stacy M, and NHLBI Recipient Epidemiology Donor Evaluation Study (REDS)-III Program

Subjects
ERYTHROCYTES, BLOOD donors, BLOOD transfusion, HEMOLYSIS & hemolysins, DIRECTED blood donations, ERYTHROCYTE metabolism, BIOCHEMISTRY, BLOOD, BLOOD collection, DYNAMICS, RESEARCH funding, GENOTYPES
Abstract

Background: The Red Blood Cell (RBC)-Omics study was initiated to build a large data set containing behavioral, genetic, and biochemical characteristics of blood donors with linkage to outcomes of the patients transfused with their donated RBCs.Study Design and Methods: The cohort was recruited from four US blood centers. Demographic and donation data were obtained from center records. A questionnaire to assess pica, restless leg syndrome, iron supplementation, hormone use, and menstrual and pregnancy history was completed at enrollment. Blood was obtained for a complete blood count, DNA, and ferritin testing. A leukocyte-reduced RBC sample was transferred to a custom storage bag for hemolysis testing at Storage Days 39 to 42. A subset was recalled to evaluate the kinetics and stability of hemolysis measures.Results: A total of 13,403 racially/ethnically diverse (12% African American, 12% Asian, 8% Hispanic, 64% white, and 5% multiracial/other) donors of both sexes were enrolled and ranged from 18 to 90 years of age; 15% were high-intensity donors (nine or more donations in the prior 24 mo without low hemoglobin deferral). Data elements are available for 97% to 99% of the cohort.Conclusions: The cohort provides demographic, behavioral, biochemical, and genetic data for a broad range of blood donor studies related to iron metabolism, adverse consequences of iron deficiency, and differential hemolysis (including oxidative and osmotic stress perturbations) during RBC storage. Linkage to recipient outcomes may permit analysis of how donor characteristics affect transfusion efficacy. Repository DNA, plasma, and RBC samples should expand the usefulness of the current data set. [ABSTRACT FROM AUTHOR]

Published
2019
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49. Heterogeneity of blood processing and storage additives in different centers impacts stored red blood cell metabolism as much as storage time: lessons from REDS-III-Omics.

Author

D'Alessandro, Angelo, Culp‐Hill, Rachel, Reisz, Julie A., Anderson, Mikayla, Fu, Xiaoyun, Nemkov, Travis, Gehrke, Sarah, Zheng, Connie, Kanias, Tamir, Guo, Yuelong, Page, Grier, Gladwin, Mark T., Kleinman, Steve, Lanteri, Marion, Stone, Mars, Busch, Michael, Zimring, James C., Culp-Hill, Rachel, and Recipient Epidemiology and Donor Evaluation Study-III (REDS-III)

Subjects
BLOOD collection, BLOOD transfusion, ERYTHROCYTES, BLOOD diseases, PHENOTYPES, METHIONINE metabolism, ERYTHROCYTE metabolism, ANALYSIS of variance, BIOCHEMISTRY, COMPARATIVE studies, GLYCOLYSIS, RESEARCH methodology, MEDICAL cooperation, MULTIVARIATE analysis, RESEARCH, RESEARCH funding, TIME, EVALUATION research, IN vitro studies
Abstract

Background: Biological and technical variability has been increasingly appreciated as a key factor impacting red blood cell (RBC) storability and, potentially, transfusion outcomes. Here, we performed metabolomics analyses to investigate the impact of factors other than storage duration on the metabolic phenotypes of stored RBC in a multicenter study.Study Design and Methods: Within the framework of the REDS-III (Recipient Epidemiology and Donor Evaluation Study-III) RBC-Omics study, 13,403 donors were enrolled from four blood centers across the United States and tested for the propensity of their RBCs to hemolyze after 42 days of storage. Extreme hemolyzers were recalled and donated a second unit of blood. Units were stored for 10, 23, and 42 days prior to sample acquisition for metabolomics analyses.Results: Unsupervised analyses of metabolomics data from 599 selected samples revealed a strong impact (14.2% of variance) of storage duration on metabolic phenotypes of RBCs. The blood center collecting and processing the units explained an additional 12.2% of the total variance, a difference primarily attributable to the storage additive (additive solution 1 vs. additive solution 3) used in the different hubs. Samples stored in mannitol-free/citrate-loaded AS-3 were characterized by elevated levels of high-energy compounds, improved glycolysis, and glutathione homeostasis. Increased methionine metabolism and activation of the transsulfuration pathway was noted in samples processed in the center using additive solution 1.Conclusion: Blood processing impacts the metabolic heterogeneity of stored RBCs from the largest multicenter metabolomics study in transfusion medicine to date. Studies are needed to understand if these metabolic differences influenced by processing/storage strategies impact the effectiveness of transfusions clinically. [ABSTRACT FROM AUTHOR]

Published
2019
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50. Distinguishing Secondary Dengue Virus Infection From Zika Virus Infection With Previous Dengue by a Combination of 3 Simple Serological Tests.

Author

Wen-Yang Tsai, Han Ha Youn, Brites, Carlos, Jih-Jin Tsai, Tyson, Jasmine, Pedroso, Celia, Drexler, Jan Felix, Stone, Mars, Simmons, Graham, Busch, Michael P., Lanteri, Marion, Stramer, Susan L., Balmaseda, Angel, Harris, Eva, and Wei-Kung Wang

Subjects
DENGUE, DIAGNOSIS of fever, IMMUNOGLOBULIN analysis, ZIKA virus infections, ALGORITHMS, DIFFERENTIAL diagnosis, ENZYME-linked immunosorbent assay, POLYMERASE chain reaction, SERODIAGNOSIS, REVERSE transcriptase polymerase chain reaction, DESCRIPTIVE statistics, DIAGNOSIS
Abstract

Background. The explosive spread of Zika virus (ZIKV) and associated microcephaly present an urgent need for sensitive and specific serodiagnostic tests, particularly for pregnant women in dengue virus (DENV)-endemic regions. Recent reports of enhanced ZIKV replication by dengue-immune sera have raised concerns about the role of previous DENV infection on the risk and severity of microcephaly and other ZIKV complications. Methods. Enzyme-linked immunosorbent assays (ELISAs) based on ZIKV and DENV nonstructural protein 1 (NS1) were established to test acute, convalescent phase, and post-convalescent phase serum/plasma samples from reverse-transcription polymerase chain reaction-confirmed cases including 20 primary ZIKV, 25 ZIKV with previous DENV, 58 secondary DENV, and 16 primary DENV1 infections. Results. ZIKV-NS1 immunoglobulin M (IgM) and immunoglobulin G (IgG) ELISAs combined can detect ZIKV infection with a sensitivity of 95% and specificity of 66.7%. The ZIKV-NS1 IgG cross-reactivity by samples from secondary DENV infection cases ranged from 66.7% to 28.1% (within 1 month to 1-2 years post-illness, respectively). Addition of DENV1-NS1 IgG ELISA can distinguish primary ZIKV infection; the ratio of absorbance of ZIKV-NS1 to DENV1-NS1 IgG ELISA can distinguish ZIKV with previous DENV and secondary DENV infections with a sensitivity of 87.5% and specificity of 81.3%. These findings were supported by analysis of sequential samples. Conclusions. An algorithm for ZIKV serodiagnosis based on 3 simple ELISAs is proposed to distinguish primary ZIKV, ZIKV with previous DENV, and secondary DENV infections; this could be applied to serodiagnosis for ZIKV, serosurveillance, and monitoring ZIKV infection during pregnancy to understand the epidemiology, pathogenesis, and complications of ZIKV in dengue-endemic regions. [ABSTRACT FROM AUTHOR]

Published
2017
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