Your search keyword '"Cindy Wilkening"' showing total 3 results

1. A North American multilaboratory study of CD4 counts using flow cytometric panleukogating (PLG): A NIAID-DAIDS Immunology Quality Assessment Program Study

Author

Alan L. Landay, Thomas N. Denny, Lee Lam, Thomas J. Spira, Cindy Wilkening, Rebecca Gelman, Frank Mandy, John L. Schmitz, Raul Louzao, Michèle Bergeron, and Deborah K. Glencross

Subjects

Histology, Quality Assurance, Health Care, Coefficient of variation, Human immunodeficiency virus (HIV), medicine.disease_cause, Specimen Handling, Pathology and Forensic Medicine, Bias, Leukocytes, medicine, Humans, Cd4 t cell, Quality assessment, business.industry, Cell Biology, Flow Cytometry, Blood Cell Count, CD4 Lymphocyte Count, Cost savings, North America, Immunology, CD4 Lymphocyte, Laboratories, business, Aids pandemic, Healthcare system

Abstract

Background The global HIV/AIDS pandemic and guidelines for initiating anti-retroviral therapy (ART) and opportunistic infection prophylaxis demand affordable, reliable, and accurate CD4 testing. A simple innovative approach applicable to existing technology that has been successfully applied in resource-challenged settings, PanLeukogated CD4 (PLG), could offer solutions for cost saving and improved precision. Methods Day-old whole blood from 99 HIV+ donors was simultaneously studied in five North-American laboratories to compare the performance of their predicate methods with the dual-platform PLG method. The predicate technology included varying 4-color CD45/CD3/CD4/CD8 protocols on different flow cytometers. Each laboratory also assayed eight replicate specimens of day-old blood from 10 to 14 local donors. Bias and precision of predicate and PLG methods was studied between- and within-participating laboratories. Results Significantly (P < 0.0001) improved between-laboratory precision/coefficient of variation (CV%) was noted using the PLG method (overall median 9.3% vs. predicate median CV 13.1%). Within-laboratory precision was also significantly (P < 0.0001) better overall using PLG (median 4.6% vs. predicate median CV 6.2%) and in 3 of the 5 laboratories. PLG counts tended to be 11% smaller than predicate methods (P < 0.0001) for shipped (median of predicate—PLG = 31) and local specimens (median of predicate—PLG = 23), both overall and in 4 of 5 laboratories (median decreases of 4, 16, 20, and 21% in shipped specimens); the other laboratory had a median increase of 5%. Conclusion Laboratories using predicate CD4 methods similar to those in this study could improve their between-laboratory and their within-laboratory precision, and reduce costs, by switching to the PLG method after adequate training, if a change (usually, a decrease) in CD4 counts is acceptable to their health systems. © 2008 Clinical Cytometry Society

Published

2008

2. Analyses of quality assessment studies using CD45 for gating lymphocytes for CD3+4+%

Author

Cindy Wilkening and Rebecca Gelman

Subjects

Quality Control, CD3 Complex, T-Lymphocytes, CD4-CD8 Ratio, Biophysics, Blood Donors, Gating, Immunophenotyping, Pathology and Forensic Medicine, Endocrinology, HIV Seropositivity, Humans, Medicine, Lymphocyte Count, Quality assessment, business.industry, Reproducibility of Results, Cell Biology, Hematology, Flow Cytometry, CD4 Antigens, Immunology, Leukocyte Common Antigens, Color flow, Laboratories, business, Nuclear medicine

Abstract

BACKGROUND The purpose of this study was to assess whether laboratories which do not use CD45 for gating lymphocytes with three- (or four-) color flow cytometry (non-CD45 laboratories) for CD3+4+% and CD3+8+% do worse on quality assessment (QA) studies than laboratories which do use CD45 (CD45 laboratories). METHODS Data came from blood specimens donated by 62 donors (50 HIV-positive) assayed over 2 years (November, 1996-October, 1998) by 35 laboratories in the NIAID DAIDS Flow Cytometry QA Program. RESULTS Non-CD45 laboratories were significantly more likely to be classified as having unacceptable inter-laboratory results (far from the group median) than CD45 laboratories (5.6% vs 1.5%, P = 0.005 for CD3+4+%; 10.4% vs 5.0%, P = 0.007 for CD3+8+%). The intra-laboratory range of results on blinded replicates was significantly more likely to be deemed unacceptable (range >4%) in non-CD45 laboratories than in CD45 laboratories for CD3+8+% (14.5% vs 3.5%, P = 0.002) but not for CD3+4+% (2.6% vs 1.5%, P = 0.62). These differences in favor of CD45 gating were observed even though the non-CD45 laboratories had been doing three-color flow cytometry in the QA program significantly longer (P = 0.05) than the CD45 laboratories, and so would be expected to have fewer problems with the assay. CONCLUSIONS Laboratories which choose to use a single CD3/CD4/CD8 tube for immunophenotyping may be sacrificing both accuracy and reproducibility.Cytometry (Comm. Clin. Cytometry) 42:1–4, 2000 © 2000 Wiley-Liss, Inc.

Published

2000

3. Optimization of storage and shipment of cryopreserved peripheral blood mononuclear cells from HIV-infected and uninfected individuals for ELISPOT assays

Author

Lin Ye Song, Nancy B. Tustin, Raul Louzao, Olivier D. Defawe, Jennifer Canniff, Guido Ferrari, Ambrosia Garcia, Sudheesh Pilakka-Kanthikeel, John Hural, Cindy Wilkening, Donald K. Carter, David Shugarts, Paige E. Etter, Linda K. Lambrecht, Mark Berrong, Terry Fenton, Savita Pahwa, Tania L. Garrelts, Rebecca Gelman, and Adriana Weinberg

Subjects

Male, Enzyme-Linked Immunospot Assay, Time Factors, Cell Survival, Immunology, HIV Infections, Biology, Peripheral blood mononuclear cell, Virus, Cryopreservation, Article, Andrology, Blood cell, Antigen, medicine, Immunology and Allergy, Humans, Candida albicans, ELISPOT, hemic and immune systems, biology.organism_classification, Virology, medicine.anatomical_structure, Lentivirus, Leukocytes, Mononuclear, Female

Abstract

Functional immunologic assays using cryopreserved peripheral blood mononuclear cells (PBMC) are influenced by blood processing, storage and shipment. The objective of this study was to compare the viability, recovery and ELISPOT results of PBMC stored and shipped in liquid nitrogen (LN/LN) or stored in LN and shipped on dry ice (LN/DI) or stored at -70°C for 3 to 12 weeks and shipped on DI (70/DI 3 to 12); and to assess the effect of donor HIV infection status on the interaction between storage/shipment and the outcome measures. PBMC from 12 HIV-infected and 12 uninfected donors showed that LN/LN conferred higher viability and recovery than LN/DI or 70/DI 3, 6, 9 or 12. LN/DI PBMC had higher viability than any 70/DI PBMC. The PBMC viability and recovery linearly decreased with the duration of storage at -70°C from 3 to 12 weeks. This effect was more pronounced in samples from HIV-infected than uninfected donors. Results of ELISPOT assays using CMV pp65, CEF and Candida albicans antigens were qualitatively and quantitatively similar across LN/LN, LN/DI and 70/DI 3. However, ELISPOT values significantly decreased with the duration of storage at -70°C both in HIV-infected and uninfected donors. ELISPOT results also decreased with PBMC viability

Published

2010