Quantitative and qualitative analysis of stability for 16 serum immunoregulators over 50 freeze–thaw cycles

Author:

Chowdhury R. N.12ORCID,Armato A.3,Culver E.4,Shteynman L.45,Kurien C.67,Cradin B.6,Margolin F.6,Nguyen T.6,Cardona C.6,Kabir N.48,Garruto R. M.14,Lum J. K.14,Wander K.1ORCID

Affiliation:

1. Department of Anthropology Binghamton University Binghamton New York USA

2. Department of Child and Family Studies University of South Florida Tampa Florida USA

3. United Health Services Wilson Memorial Hospital Johnson City New York USA

4. Department of Biological Sciences Binghamton University Binghamton New York USA

5. Renaissance School of Medicine at Stony Brook University Stony Brook New York USA

6. Department of Integrative Neuroscience Binghamton University Binghamton New York USA

7. College of Osteopathic Medicine New York Institute of Technology Long Island New York USA

8. Lake Erie College of Osteopathic Medicine Elmira New York USA

Abstract

AbstractObjectivesTo evaluate the reliability of data from the assay of bio‐archived specimens, a 50‐freeze–thaw‐cycle (FTC) degradation study of fresh sera was conducted to test the stability of 16 immunoregulators.MethodsTwenty de‐identified serum specimens were obtained from volunteers at United Health Services‐Wilson Memorial Hospital. Specimens were stored at −20°C and underwent daily 1 h thawing and subsequent freezing for each FTC over 50 consecutive days. Immunoregulator concentrations were assessed via enzyme‐linked immunosorbent assay (ELISA) in participant samples at 2 FTC (baseline), 25 FTC, and 50 FTC. Specific immunoregulators observed in the study were C‐reactive protein (CRP), interleukin (IL)‐1α, 4, 6, 8, 10, monocyte chemoattractant protein‐1 (MCP‐1, CCL2), monocyte chemoattractant protein‐2 (MCP‐2, CCL8), eotaxin‐1, thymus‐and‐activation‐regulated chemokine (TARC, CCL17), regulated on activation normal T‐cell expressed and secreted (RANTES, CCL5), growth‐regulated oncogene‐alpha (GRO‐α, CXCL1), small inducible cytokine A1 (I‐309, CCL1), interferon‐gamma (IFN‐γ), interferon‐gamma inducible protein‐10 (IP‐10, CXCL10), and tumor necrosis factor‐alpha (TNF‐α).ResultsQuantitative stability of serum immunoregulators: Serum CRP, IL‐8, IL‐10, IFN‐γ, IP‐10, and eotaxin‐1 levels appear to be statistically equivalent from baseline to 50 FTC (p ≤ .05). Retention of patterns in serum immunoregulators: patterns across FTC were retained for TARC (age) and CRP, IFN‐γ, and MCP‐2 (sex).ConclusionsWhile the effect of multiple FTC on serum immunoregulator levels may not replicate prolonged freezer storage, the results of this study provide valuable information on the robustness of immunoregulators for research using bio‐archived sera.

Funder

Binghamton University

Publisher

Wiley

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