Comparison of skin biopsy sample processing and storage methods on high dimensional immune gene expression using the Nanostring nCounter system

Jelena Vider; Andrew Croaker; Amanda J. Cox; Emma Raymond; Rebecca Rogers; Stuart Adamson; Michael Doyle; Blake O’Brien; Allan W. Cripps; Nicholas P. West

doi:10.1186/s13000-020-00974-4

Diagnostic Pathology (May 2020)

Comparison of skin biopsy sample processing and storage methods on high dimensional immune gene expression using the Nanostring nCounter system

Jelena Vider,
Andrew Croaker,
Amanda J. Cox,
Emma Raymond,
Rebecca Rogers,
Stuart Adamson,
Michael Doyle,
Blake O’Brien,
Allan W. Cripps,
Nicholas P. West

Affiliations

Jelena Vider: School of Medical Science and Menzies Health Institute QLD, Griffith University
Andrew Croaker: School of Health and Human Sciences, Southern Cross University
Amanda J. Cox: School of Medical Science and Menzies Health Institute QLD, Griffith University
Emma Raymond: Wesley Medical Research
Rebecca Rogers: Wesley Medical Research
Stuart Adamson: Mid-West Aero Medical
Michael Doyle: Wesley Medical Research
Blake O’Brien: Sullivan &Nicolaides Pathology
Allan W. Cripps: Systems Biology and Data Science, Menzies Health Institute QLD, Griffith University
Nicholas P. West: School of Medical Science and Menzies Health Institute QLD, Griffith University

DOI: https://doi.org/10.1186/s13000-020-00974-4
Journal volume & issue: Vol. 15, no. 1
pp. 1 – 7

Abstract

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Abstract Background Digital multiplex gene expression profiling is overcoming the limitations of many tissue-processing and RNA extraction techniques for the reproducible and quantitative molecular classification of disease. We assessed the effect of different skin biopsy collection/storage conditions on mRNA quality and quantity and the NanoString nCounter™ System’s ability to reproducibly quantify the expression of 730 immune genes from skin biopsies. Methods Healthy human skin punch biopsies (n = 6) obtained from skin sections from four patients undergoing routine abdominoplasty were subject to one of several collection/storage protocols, including: i) snap freezing in liquid nitrogen and transportation on dry ice; ii) RNAlater (ThermoFisher) for 24 h at room temperature then stored at − 80 °C; iii) formalin fixation with further processing for FFPE blocks; iv) DNA/RNA shield (Zymo) stored and shipped at room temperature; v) placed in TRIzol then stored at − 80 °C; vi) saline without RNAse for 24 h at room temperature then stored at − 80 °C. RNA yield and integrity was assessed following extraction via NanoDrop, QuantiFluor with RNA specific dye and a Bioanalyser (LabChip24, PerkinElmer). Immune gene expression was analysed using the NanoString Pancancer Immune Profiling Panel containing 730 genes. Results Except for saline, all protocols yielded total RNA in quantities/qualities that could be analysed by NanoString nCounter technology, although the quality of the extracted RNA varied widely. Mean RNA integrity was highest from samples that were placed in RNALater (RQS 8.2 ± 1.15), with integrity lowest from the saline stored sample (RQS 10,000 similar across extraction protocols. Conclusions A variety of processing methods can be used for digital immune gene expression profiling in mRNA extracted from skin that are comparable to snap frozen skin specimens, providing skin cancer clinicians greater opportunity to supply skin specimens to tissue banks. NanoString nCounter technology can determine gene expression in skin biopsy specimens with a high degree of sensitivity despite lower RNA yields and processing methods that may generate poorer quality RNA. The increased sensitivity of digital gene expression profiling continues to expand molecular pathology profiling of disease.

Published in Diagnostic Pathology

ISSN: 1746-1596 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine: Pathology
Website: https://diagnosticpathology.biomedcentral.com/

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