Concordant Proficiency in Measurement of T-Cell Immunity in Human Immunodeficiency Virus Vaccine Clinical Trials by Peripheral Blood Mononuclear Cell and Enzyme-Linked Immunospot Assays in Laboratories from Three Continents

Author:

Boaz Mark J.12345,Hayes Peter12345,Tarragona Tony12345,Seamons Laura12345,Cooper Andrew12345,Birungi Josephine12345,Kitandwe Paul12345,Semaganda Aloysius12345,Kaleebu Pontiano12345,Stevens Gwynneth12345,Anzala Omu12345,Farah Bashir12345,Ogola Simon12345,Indangasi Jackton12345,Mhlanga Patrick12345,Van Eeden Melanie12345,Thakar Madhuri12345,Pujari Ashwini12345,Mishra Shadri12345,Goonetilleke Nilu12345,Moore Stephen12345,Mahmoud Abdul12345,Sathyamoorthy Pattabiraman12345,Mahalingam Jayashri12345,Narayanan Paranji R.12345,Ramanathan Vadakkuppattu D.12345,Cox Josephine H.12345,Dally Len12345,Gill Dilbinder K.12345,Gilmour Jill12345

Affiliation:

1. International AIDS Vaccine Initiative, New York, New York

2. International AIDS Vaccine Initiative Core Laboratory, Imperial College, London, United Kingdom

3. Uganda Virus Research Institute, Entebbe, Uganda

4. Kenya Aids Vaccine Initiative, Nairobi, Kenya

5. Contract Laboratory Services, Johannesburg, South Africa

Abstract

ABSTRACT The gamma interferon (IFN-γ) enzyme-linked immunospot (ELISPOT) assay is used routinely to evaluate the potency of human immunodeficiency virus (HIV) vaccine candidates and other vaccine candidates. In order to compare candidates and pool data from multiple trial laboratories, validated standardized methods must be applied across laboratories. Proficiency panels are a key part of a comprehensive quality assurance program to monitor inter- and intralaboratory performance, as well as assay performance, over time. Seven International AIDS Vaccine Initiative-sponsored trial sites participated in the proficiency panels described in this study. At each laboratory, two operators independently processed identical sample sets consisting of frozen peripheral blood mononuclear cell (PBMC) samples from different donors by using four blind stimuli. PBMC recovery and viability after overnight resting and the IFN-γ ELISPOT assay performance were assessed. All sites demonstrated good performance in PBMC thawing and resting, with a median recovery of 78% and median viability of 95%. The laboratories were able to detect similar antigen-specific T-cell responses, ranging from 50 to >3,000 spot-forming cells per million PBMC. An approximate range of a half log in results from operators within or across sites was seen in comparisons of antigen-specific responses. Consistently low background responses were seen in all laboratories. The results of these proficiency panels demonstrate the ability of seven laboratories, located across three continents, to process PBMC samples and to rank volunteers with differential magnitudes of IFN-γ ELISPOT responses. These findings also illustrate the ability to standardize the IFN-γ ELISPOT assay across multiple laboratories when common training methods, reagents such as fetal calf serum, and standard operating procedures are adopted. These results are encouraging for laboratories that are using cell-based immunology assays to test HIV vaccines and other vaccines.

Publisher

American Society for Microbiology

Subject

Microbiology (medical),Clinical Biochemistry,Immunology,Immunology and Allergy

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