Stability of inflammation markers in human blood collected using volumetric absorptive microsampling (VAMS) under typical laboratory storage temperatures

R McMahon; C Hill; J Rudge; B Herbert; E Karsten

doi:10.1016/j.cyto.2023.156355

Stability of inflammation markers in human blood collected using volumetric absorptive microsampling (VAMS) under typical laboratory storage temperatures

Cytokine. 2023 Nov:171:156355. doi: 10.1016/j.cyto.2023.156355. Epub 2023 Sep 8.

Authors

R McMahon¹, C Hill², J Rudge³, B Herbert², E Karsten⁴

Affiliations

¹ Sangui Bio Pty Ltd, Sydney, Australia; The Kolling Institute, Sydney, Australia. Electronic address: rosalee@sanguibio.com.
² Sangui Bio Pty Ltd, Sydney, Australia; The Kolling Institute, Sydney, Australia.
³ Trajan Scientific and Medical (Neoteryx), Australia.
⁴ Sangui Bio Pty Ltd, Sydney, Australia; The Kolling Institute, Sydney, Australia; University of Sydney, Australia.

PMID: 37690424
DOI: 10.1016/j.cyto.2023.156355

Abstract

Dried blood spots (DBS) collected on filter paper such as Guthrie cards are stored for years at room temperature. The assumption is that once dried, the samples remain stable and quantifiable indefinitely since the metabolites these were initially designed to measure, are known for their extended stability. The concentration of other blood proteins such as cytokines, however, are known to vary with storage even in liquid samples stored at -80 °C for extended periods of time. We sought to determine if cytokines are stable for up to 5 months when stored as a dried blood sample using volumetric absorptive microsampling (VAMS) devices. To test this, blood was collected from 4 healthy participants, spiked with recombinant cytokines, and collected into 30 µL VAMS devices. These prepared VAMS devices were stored at room temperature, 4 °C, or -20 °C for up to 5 months and matching VAMS liquid extracts were stored at -80 °C for the same period of time. At each timepoint, the samples were extracted from the VAMS devices and the extracts were analysed by Luminex® for quantification of up to 31 cytokines. These methods were also tested in a remote clinical study over a period of up to 8 months. Cytokine analysis revealed that room temperature, the current standard for DBS and VAMS storage, performed the poorest out of all storage temperatures with significant losses in 13/21 analytes compared to 4 °C at 5 months. Storage at 4 °C or colder performed well for the majority of analytes tested, however out of those, the optimal storage temperature differed for each analyte. There were a small number of analytes that performed poorly regardless of storage conditions and for fractalkine, this was found to be caused by inefficient recovery during extraction. Cytokine concentrations from finger-prick samples were also found to be much more variable that those in venous blood samples. Our results highlight the need to understand the stability of analytes of interest before committing to longitudinal collection and storage of samples in VAMS devices. These data give confidence that storage at 4 °C or colder was beneficial for cytokine stability. Wherein 25/31 cytokines were quantifiably stable at -20 °C when stored for 3 months and 17/21 were quantifiably stable after 5 months when stored at 4 °C.

Keywords: Cytokines; Longitudinal; Proteomics; Stability; Volumetric absorptive microsampling.