Approaching stability challenges for flow cytometry in a regulated bioanalytical environment

Anamica Muruganandham; Carolyne Dumont; Kuiyi Xing

doi:10.4155/bio-2019-0183

Approaching stability challenges for flow cytometry in a regulated bioanalytical environment

Bioanalysis. 2019 Oct;11(20):1845-1858. doi: 10.4155/bio-2019-0183. Epub 2019 Oct 22.

Authors

Anamica Muruganandham¹, Carolyne Dumont², Kuiyi Xing¹

Affiliations

¹ Celerion, Inc., 621 Rose Street, Lincoln, NE 68502, USA.
² Charles River Laboratories, 22022 Transcanadienne, Senneville, QC H9X 3R3, Canada.

PMID: 31637937
DOI: 10.4155/bio-2019-0183

Abstract

Stability of samples for flow cytometry is a critical parameter since storage period of samples is restricted to only a limited period after collection. For most studies, clinical samples have to be shipped to a testing laboratory, in contrast to preclinical samples, which can be analyzed on-site or off-site. Therefore, evaluating stability is critical to provide flexibility on testing of samples to obtain reliable data. A wide variety of factors contributes to establishing stability from sample collection through acquisition. We provided suggestions for experimental and stability parameters to be taken into consideration when designing a flow cytometry method. The case studies presented represent how certain stability issues were overcome to perform flow cytometry assays in a regulated bioanalytical environment.

Keywords: bioanalytical challenge; clinical samples; flow cytometry; preclinical samples; regulatory environment; stability.

MeSH terms

Animals
Biomarkers / metabolism
Flow Cytometry / methods*
Freezing
Lymphocytes / metabolism
Macaca fascicularis
Specimen Handling

Substances

Biomarkers