A Simple and Cost-Effective Method for Measuring Hemolysis in Biobank Serum Specimens

Randi E Gislefoss; Urszula Berge; Marianne Lauritzen; Hilde Langseth; Marcin W Wojewodzic

doi:10.1089/bio.2021.0037

A Simple and Cost-Effective Method for Measuring Hemolysis in Biobank Serum Specimens

Biopreserv Biobank. 2021 Dec;19(6):525-530. doi: 10.1089/bio.2021.0037. Epub 2021 Oct 5.

Authors

Randi E Gislefoss¹, Urszula Berge¹, Marianne Lauritzen¹, Hilde Langseth^{1

2}, Marcin W Wojewodzic^{1

3

4}

Affiliations

¹ Department of Research, Cancer Registry of Norway, Oslo, Norway.
² Department of Epidemiology and Biostatistics, Imperial College, London, United Kingdom.
³ Environmental Genomics, School of Biosciences, University of Birmingham, Birmingham, United Kingdom.
⁴ Department of Environmental Health, Norwegian Institute of Public Health, Oslo, Norway.

PMID: 34613836
DOI: 10.1089/bio.2021.0037

Abstract

Background: During sampling and processing, blood samples can be affected by hemolysis. Information is lacking regarding hemolysis for biobank samples. There is a need for a method that can easily measure hemoglobin as an indicator of hemolysis in stored samples before they are included in research projects. In this study we present a simple method for estimating hemolysis and investigate the effect of centrifugation speeds and temperatures on sample turbidity that commonly interferes with measurements. Methods: Using a variation of the Beer-Lambert law, we quantified the hemoglobin concentration in 75 long-term stored samples at a wavelength of 414 nm with a NanoDrop™ 8000 spectrophotometer. Owing to interference from turbidity, the samples underwent different treatments post-thawing: centrifugation at 10,000 and 20,000 g at two different temperatures (4°C and 19°C) for 15 minutes. In addition, freshly collected serum samples (n = 20) underwent a single freeze-thaw cycle, with hemoglobin measured prefreeze, post-thaw, and postcentrifugation. Kruskal-Wallis rank sum test groups and pairwise Wilcoxon rank test were used for statistical analysis. Results: A strong effect of centrifugation on the turbidity was shown for the long-term stored samples, however, this effect was independent of the temperature or centrifugation speeds. Centrifugation at 20,000 g for 15 minutes at 19°C reduced the turbidity up to 50%. A single freeze-thaw cycle in the fresh samples increased the optical density at 414 nm slightly, indicating a false increase of hemoglobin concentration. The following centrifugation reduced the concentration to less than the initial sample measurements, suggesting the presence of interference immediately after sampling. Conclusion: We describe here a simple and cost-effective NanoDrop-based method for measuring hemolysis levels intended for use in biobank facilities. We found that centrifugation, but not temperature, is a crucial step to reduce interference from turbidity.

Keywords: biobank; hemolysis; serum; spectrophotometric method; turbidity.

MeSH terms

Biological Specimen Banks*
Centrifugation
Cost-Benefit Analysis
Freezing
Hemolysis*
Humans