Your search keyword '"Bernadette Alford"' showing total 10 results

1. Inactivation of protozoan parasites in red blood cells using INACTINE PEN110 chemistry

Author

Boris Zavizion, David J. Bzik, Bernadette Alford, John Wehrley Chapman, Andrei Purmal, Thomas N. Mather, Milena De Melo Jorge, Mercio Pereira, Diana Serebryanik, and Nathan J. Miller

Subjects

Infectivity, biology, Immunology, Hematology, Parasitemia, medicine.disease, biology.organism_classification, Virology, Blood cell, Red blood cell, medicine.anatomical_structure, parasitic diseases, Babesia, medicine, Immunology and Allergy, Parasite hosting, Protozoa, Trypanosoma cruzi

Abstract

BACKGROUND: The transmission of parasites, including Babesia, plasmodia, and Trypanosoma cruzi, via transfusions is an important public health concern. INACTINE technology is a pathogen-reduction process that utilizes PEN110, an electrophilic agent that inac-tivates a wide range of pathogens by disrupting nucleic acid replication. The present study investigated the effect of PEN110 treatment on the viability of protozoa in RBCs. STUDY DESIGN AND METHODS:B. microti-parasitized RBCs from infected hamsters were treated with PEN110 and inoculated to naive animals. Parasitemia was detected by blood smears and PCR. Human RBCs infected with P. falciparum were treated with PEN110 and incubated with fresh RBCs. P. falciparum multiplication was detected by blood smears. Human RBCs spiked with T. cruzi and treated with PEN110 were analyzed for the presence of live parasites using in-vitro infectivity assay or by inoculating susceptible mice. RESULTS: Treatment of RBCs infected with B. microti or P. falciparum with 0.01 to 0.1 percent (vol/vol) PEN110 resulted in parasite inactivation to below the limit of detection during 24 hours. T. cruzi inoculated into human RBCs was inactivated below the limit of detection by 0.1 percent PEN110 after 3 hours. CONCLUSION: The study demonstrates that treatment of blood with PEN110 is highly effective in eradicating transfusion-transmitted protozoan parasites.

Published

2004

2. Development of a sensitive PCR inhibition method to demonstrate HBV nucleic acid inactivation

Author

Shahika Aytay, John Chapman, Asa Ohagen, Michael P. Busch, Aris Lazo, and Bernadette Alford

Subjects

Hepatitis B virus, Infectivity, DNA damage, Immunology, Hematology, Biology, medicine.disease_cause, Virology, Molecular biology, In vitro, Virus, law.invention, In vivo, law, medicine, Nucleic acid, Immunology and Allergy, Polymerase chain reaction

Abstract

BACKGROUND: The evaluation of pathogen reduction technologies with relevant viruses currently contaminating the blood supply is limited by the availability of high-titer virus inocula and sensitive in vitro or in vivo infectivity assays. Because HBV infectivity can only be assessed by in vivo studies with chimpanzees, a sensitive PCR inhibition assay was developed to measure PEN110 inactivation of HBV. STUDY DESIGN AND METHODS: PCR amplification of 1.1 kb of HBV genome was optimized to determine DNA damage introduced by treatment with PEN110 in RBCs. Inactivation of duck HBV (DHBV) in RBCs, with measurement of the in vitro infectivity, was performed to validate the PCR assay. RESULTS: The PCR was highly specific and sensitive for amplification of the HBV genome and used to demonstrate a reduction of at least 7.2 and 8.1 log geq per mL within the first 18 hours of PEN110 treatment. PEN110 inactivation of DHBV was also achieved within the first 18 hours with a reduction factor of at least 5.0 log tissue culture infectious dose 50 percent per mL, suggesting that PCR inhibition is an alternative to infectivity assays. CONCLUSION: This study establishes PCR inhibition as a reasonable approach to assess the efficiency of PEN110 inactivation of human pathogens with human plasma donations that have been found to contain high titers of relevant agents during different stages of infection.

Published

2004

3. Inactivation of mycoplasma species in blood by INACTINE PEN110 process

Author

Andrei Purmal, John Wehrley Chapman, Bernadette Alford, and Boris Zavizion

Subjects

Inoculation, Immunology, Mycoplasma species, Mycoplasmataceae, Hematology, Mycoplasma, Biology, biology.organism_classification, medicine.disease_cause, Virology, Microbiology, medicine, Mollicutes, Immunology and Allergy, Incubation, Bacteria, Whole blood

Abstract

BACKGROUND: Mycoplasmas have been associated with multiple acute and chronic diseases. Mycoplasma genome is found in the blood of 10 to 15 percent of subjectively healthy individuals. If blood borne and viable in donated blood, mycoplasmas could potentially be transfusion transmissible. The INACTINE PEN110 technology is a pathogen reduction process that is in Phase 3 clinical studies. The present study investigated the ability of this process to eradicate mycoplasmas in human blood. STUDY DESIGN AND METHODS: Identical whole blood or RBC units inoculated with Mycoplasma arthritidis or M. pneumoniae were incubated with PEN110 (inactivating agent) for 24 hours at 23°C. Sham controls were treated with buffer under the same conditions. 4°C controls were put on storage immediately after the spike. RESULTS: No viable microorganisms were detected in PEN110-treated units after 24 hours of incubation. Sham controls showed no changes to mycoplasma titers during the incubation. In 4°C controls, minor decrease of mycoplasma titers was observed during the storage. CONCLUSION: The INACTINE process inactivates more than 107 mycoplasma CFU per mL in whole blood and RBCs. This study is the first demonstration of susceptibility of mycoplasmas to pathogen reduction. The data provide further support for the ability of INACTINE technology to address microbial safety issues that are not well characterized.

Published

2004

4. West Nile virus in blood: stability, distribution, and susceptibility to PEN110 inactivation

Author

Jodie Tassello, Robert B. Tesh, John Wehrley Chapman, Thomas N. Mather, Tsutomu Takeda, Diana Serebryanik, Asa Ohagen, Ed Kramer, Aris Lazo, Bernadette Alford, and Fred Brown

Subjects

Infectivity, biology, viruses, Immunology, virus diseases, Hematology, biology.organism_classification, Virology, Peripheral blood mononuclear cell, Virus, Titer, Flavivirus, Immunology and Allergy, Viral disease, Viral load, Whole blood

Abstract

BACKGROUND The outbreak of West Nile virus (WNV) is the most recent reminder that the blood supply continues to be vulnerable to emerging and reemerging pathogens. A potentially prospective approach to reducing the risk of transfusion-transmitted infections of a known or newly emerging microbe is implementation of a broad-spectrum pathogen reduction technology. The purpose of this study was to evaluate the susceptibility of WNV to PEN110 inactivation in RBCs and to characterize the WNV interaction with blood, including the stability of WNV in RBCs stored at 1 to 6 degrees C, its distribution and infectivity, and its ability to infect WBCs. STUDY DESIGN AND METHODS Inactivation was performed with three WNV isolates spiked into WBC-reduced RBCs. The stability of the virus was evaluated by spiking two viral loads into RBCs followed by storing at 1 to 6 degrees C for up to 42 days. The distribution of the virus in plasma, RBCs, and PBMCs was evaluated with whole blood from infected hamsters. Finally, in vitro propagation of WNV was evaluated with the THP-1 cell line and primary monocytes. RESULTS The kinetics of PEN110 inactivation of WNV isolates RI-44, NJ-176, and 99-3494031 were fast and complete within 24 hours with reduction factors of 5 to 7 log plaque-forming units per mL. WNV remained infectious for up to 42 days at 1 to 6 degrees C. The WNV titers in whole blood, plasma, RBCs, and PBMC fractions were equally distributed and ranged from 2 to 3 log tissue culture infectious dose 50 percent per mL. Productive infection of stimulated monocytes and THP-1 cells was also demonstrated. CONCLUSIONS These studies demonstrated that PEN110 efficiently inactivated WNV in RBCs and whole blood from infected hamsters to the limit of detection. WNV survived in RBCs stored at 1 to 6 degrees C with a gradual loss of titer but infectivity could still be observed for up to 42 days. In addition, it was observed that WNV was equally distributed in all blood fractions including PBMCs and it was possible to establish productive infection of a human monocytic cell line and stimulated human monocytes.

Published

2003

5. Pharmacology and Biological Efficacy of a Recombinant, Humanized, Single-Chain Antibody C5 Complement Inhibitor in Patients Undergoing Coronary Artery Bypass Graft Surgery With Cardiopulmonary Bypass

Author

Gary S. Kopf, Philip Kraker, Roberta Hines, Louis A. Matis, Richard K. Shaw, Gregory L. Stahl, Bernadette Alford, Sary F. Aranki, Lan Li, Ruth O'Hara, Charles D. Collard, Michael L. Dewar, Henry M. Rinder, Scott A. Rollins, Brian G. Smith, Jane C. K. Fitch, John A. Elefteriades, Stanton K. Shernan, and Christine S. Rinder

Subjects

medicine.medical_specialty, Blood Loss, Surgical, Coronary Disease, Myocardial Reperfusion Injury, Inflammation, Complement Membrane Attack Complex, Pharmacology, Antibodies, Monoclonal, Humanized, law.invention, Proinflammatory cytokine, Complement inhibitor, Postoperative Complications, law, Physiology (medical), Pexelizumab, Cardiopulmonary bypass, medicine, Humans, Prospective Studies, Coronary Artery Bypass, Complement Activation, Creatine Kinase, Complement component 5, Psychological Tests, Cardiopulmonary Bypass, biology, business.industry, Antibodies, Monoclonal, Complement C5, Middle Aged, Complement system, Surgery, Isoenzymes, Integrin alpha M, biology.protein, medicine.symptom, Cognition Disorders, Cardiology and Cardiovascular Medicine, business, Single-Chain Antibodies, medicine.drug

Abstract

Background —Cardiopulmonary bypass (CPB) induces a systemic inflammatory response that causes substantial clinical morbidity. Activation of complement during CPB contributes significantly to this inflammatory process. We examined the capability of a novel therapeutic complement inhibitor to prevent pathological complement activation and tissue injury in patients undergoing CPB. Methods and Results —A humanized, recombinant, single-chain antibody specific for human C5, h5G1.1-scFv, was intravenously administered in 1 of 4 doses ranging from 0.2 to 2.0 mg/kg before CPB. h5G1.1-scFv was found to be safe and well tolerated. Pharmacokinetic analysis revealed a sustained half-life from 7.0 to 14.5 hours. Pharmacodynamic analysis demonstrated significant dose-dependent inhibition of complement hemolytic activity for up to 14 hours at 2 mg/kg. The generation of proinflammatory complement byproducts (sC5b-9) was effectively inhibited in a dose-dependent fashion. Leukocyte activation, as measured by surface expression of CD11b, was reduced ( P P =0.05) in patients who received 2 mg/kg. Sequential Mini-Mental State Examinations (MMSE) demonstrated an 80% reduction in new cognitive deficits ( P P Conclusions —A single-chain antibody specific for human C5 is a safe and effective inhibitor of pathological complement activation in patients undergoing CPB. In addition to significantly reducing sC5b-9 formation and leukocyte CD11b expression, C5 inhibition significantly attenuates postoperative myocardial injury, cognitive deficits, and blood loss. These data suggest that C5 inhibition may represent a novel therapeutic strategy for preventing complement-mediated inflammation and tissue injury.

Published

1999

6. Inactivation of protozoan parasites in red blood cells using INACTINE PEN110 chemistry

Author

Boris, Zavizion, Mercio, Pereira, Milena, de Melo Jorge, Diana, Serebryanik, Thomas N, Mather, John, Chapman, Nathan J, Miller, Bernadette, Alford, David J, Bzik, and Andrei, Purmal

Subjects

Erythrocytes, Trypanosoma cruzi, Plasmodium falciparum, Polyamines, Animals, Humans, Babesia microti

Abstract

The transmission of parasites, including Babesia, plasmodia, and Trypanosoma cruzi, via transfusions is an important public health concern. INACTINE technology is a pathogen-reduction process that utilizes PEN110, an electrophilic agent that inac-tivates a wide range of pathogens by disrupting nucleic acid replication. The present study investigated the effect of PEN110 treatment on the viability of protozoa in RBCs.B. microti-parasitized RBCs from infected hamsters were treated with PEN110 and inoculated to naïve animals. Parasitemia was detected by blood smears and PCR. Human RBCs infected with P. falciparum were treated with PEN110 and incubated with fresh RBCs. P. falciparum multiplication was detected by blood smears. Human RBCs spiked with T. cruzi and treated with PEN110 were analyzed for the presence of live parasites using in-vitro infectivity assay or by inoculating susceptible mice.Treatment of RBCs infected with B. microti or P. falciparum with 0.01 to 0.1 percent (vol/vol) PEN110 resulted in parasite inactivation to below the limit of detection during 24 hours. T. cruzi inoculated into human RBCs was inactivated below the limit of detection by 0.1 percent PEN110 after 3 hours.The study demonstrates that treatment of blood with PEN110 is highly effective in eradicating transfusion-transmitted protozoan parasites.

Published

2004

7. Development of a sensitive PCR inhibition method to demonstrate HBV nucleic acid inactivation

Author

Shahika, Aytay, Asa, Ohagen, Michael R, Busch, Bernadette, Alford, John R, Chapman, and Aris, Lazo

Subjects

Hepatitis B virus, Infection Control, Erythrocytes, Pan troglodytes, DNA, Viral, Polyamines, Animals, Virus Inactivation, Blood Donors, Hepatitis B, Polymerase Chain Reaction, Sensitivity and Specificity

Abstract

The evaluation of pathogen reduction technologies with relevant viruses currently contaminating the blood supply is limited by the availability of high-titer virus inocula and sensitive in vitro or in vivo infectivity assays. Because HBV infectivity can only be assessed by in vivo studies with chimpanzees, a sensitive PCR inhibition assay was developed to measure PEN110 inactivation of HBV.PCR amplification of 1.1 kb of HBV genome was optimized to determine DNA damage introduced by treatment with PEN110 in RBCs. Inactivation of duck HBV (DHBV) in RBCs, with measurement of the in vitro infectivity, was performed to validate the PCR assay.The PCR was highly specific and sensitive for amplification of the HBV genome and used to demonstrate a reduction of at least 7.2 and 8.1 log geq per mL within the first 18 hours of PEN110 treatment. PEN110 inactivation of DHBV was also achieved within the first 18 hours with a reduction factor of at least 5.0 log tissue culture infectious dose 50 percent per mL, suggesting that PCR inhibition is an alternative to infectivity assays.This study establishes PCR inhibition as a reasonable approach to assess the efficiency of PEN110 inactivation of human pathogens with human plasma donations that have been found to contain high titers of relevant agents during different stages of infection.

Published

2004

8. Inactivation of mycoplasma species in blood by INACTINE PEN110 process

Author

Boris, Zavizion, Andrei, Purmal, John, Chapman, and Bernadette, Alford

Subjects

Cryopreservation, Erythrocytes, Blood Preservation, Leukocytes, Polyamines, Blood Banks, Humans, Mycoplasma Infections, In Vitro Techniques, Mycoplasma arthritidis

Abstract

Mycoplasmas have been associated with multiple acute and chronic diseases. Mycoplasma genome is found in the blood of 10 to 15 percent of subjectively healthy individuals. If blood borne and viable in donated blood, mycoplasmas could potentially be transfusion transmissible. The INACTINE PEN110 technology is a pathogen reduction process that is in Phase 3 clinical studies. The present study investigated the ability of this process to eradicate mycoplasmas in human blood.Identical whole blood or RBC units inoculated with Mycoplasma arthritidis or M. pneumoniae were incubated with PEN110 (inactivating agent) for 24 hours at 23 degrees C. Sham controls were treated with buffer under the same conditions. 4 degrees C controls were put on storage immediately after the spike.No viable microorganisms were detected in PEN110-treated units after 24 hours of incubation. Sham controls showed no changes to mycoplasma titers during the incubation. In 4 degrees C controls, minor decrease of mycoplasma titers was observed during the storage.The INACTINE process inactivates more than 107 mycoplasma CFU per mL in whole blood and RBCs. This study is the first demonstration of susceptibility of mycoplasmas to pathogen reduction. The data provide further support for the ability of INACTINE technology to address microbial safety issues that are not well characterized.

Published

2004

9. West Nile virus in blood: stability, distribution, and susceptibility to PEN110 inactivation

Author

Thomas, Mather, Tsutomu, Takeda, Jodie, Tassello, Asa, Ohagen, Diana, Serebryanik, Ed, Kramer, Fred, Brown, Robert, Tesh, Bernadette, Alford, John, Chapman, and Aris, Lazo

Subjects

Erythrocytes, Dose-Response Relationship, Drug, Virus Replication, Antiviral Agents, Kinetics, Blood, Blood Preservation, Cricetinae, Chlorocebus aethiops, Polyamines, Animals, Blood Banks, Humans, Virus Inactivation, Leukapheresis, Vero Cells, West Nile virus, West Nile Fever

Abstract

The outbreak of West Nile virus (WNV) is the most recent reminder that the blood supply continues to be vulnerable to emerging and reemerging pathogens. A potentially prospective approach to reducing the risk of transfusion-transmitted infections of a known or newly emerging microbe is implementation of a broad-spectrum pathogen reduction technology. The purpose of this study was to evaluate the susceptibility of WNV to PEN110 inactivation in RBCs and to characterize the WNV interaction with blood, including the stability of WNV in RBCs stored at 1 to 6 degrees C, its distribution and infectivity, and its ability to infect WBCs.Inactivation was performed with three WNV isolates spiked into WBC-reduced RBCs. The stability of the virus was evaluated by spiking two viral loads into RBCs followed by storing at 1 to 6 degrees C for up to 42 days. The distribution of the virus in plasma, RBCs, and PBMCs was evaluated with whole blood from infected hamsters. Finally, in vitro propagation of WNV was evaluated with the THP-1 cell line and primary monocytes.The kinetics of PEN110 inactivation of WNV isolates RI-44, NJ-176, and 99-3494031 were fast and complete within 24 hours with reduction factors of 5 to 7 log plaque-forming units per mL. WNV remained infectious for up to 42 days at 1 to 6 degrees C. The WNV titers in whole blood, plasma, RBCs, and PBMC fractions were equally distributed and ranged from 2 to 3 log tissue culture infectious dose 50 percent per mL. Productive infection of stimulated monocytes and THP-1 cells was also demonstrated.These studies demonstrated that PEN110 efficiently inactivated WNV in RBCs and whole blood from infected hamsters to the limit of detection. WNV survived in RBCs stored at 1 to 6 degrees C with a gradual loss of titer but infectivity could still be observed for up to 42 days. In addition, it was observed that WNV was equally distributed in all blood fractions including PBMCs and it was possible to establish productive infection of a human monocytic cell line and stimulated human monocytes.

Published

2003

10. A63 SAFETY, PHARMACOKINETICS, AND IMMUNOGENICITY OF INTRAVENOUS ADMINISTRATION OF H5G1.1-SCFV IN HUMANS

Author

Jane C. K. Fitch, John A. Elefteriades, Bernadette Alford, Roberta Hines, and Scott A. Rollins

Subjects

Anesthesiology and Pain Medicine, Pharmacokinetics, business.industry, Immunogenicity, H5G1.1-scFv, Medicine, Pharmacology, business, Administration (government)

Published

1997