Slide-to-Slide Tissue Transfer and Array Assembly From Limited Samples for Comprehensive Molecular Profiling

Stephanie E Weissinger; N Zeke Georgantas; Julia C Thierauf; Rebecca Pellerin; Emma Gardecki; Stephanie Kühlinger; Lauren L Ritterhouse; Peter Möller; Jochen K Lennerz

doi:10.1016/j.labinv.2023.100062

Slide-to-Slide Tissue Transfer and Array Assembly From Limited Samples for Comprehensive Molecular Profiling

Lab Invest. 2023 May;103(5):100062. doi: 10.1016/j.labinv.2023.100062. Epub 2023 Jan 18.

Authors

Stephanie E Weissinger¹, N Zeke Georgantas², Julia C Thierauf², Rebecca Pellerin², Emma Gardecki², Stephanie Kühlinger³, Lauren L Ritterhouse², Peter Möller⁴, Jochen K Lennerz⁵

Affiliations

¹ Institute of Pathology, Alb Fils Clinics GmbH, Göppingen, Germany; Institute of Pathology, University Hospital Ulm, Ulm, Germany.
² Center for Integrated Diagnostics, Department of Pathology, Massachusetts General Hospital/Harvard Medical School, Boston, Massachusetts.
³ Institute of Pathology, Alb Fils Clinics GmbH, Göppingen, Germany.
⁴ Institute of Pathology, University Hospital Ulm, Ulm, Germany.
⁵ Center for Integrated Diagnostics, Department of Pathology, Massachusetts General Hospital/Harvard Medical School, Boston, Massachusetts. Electronic address: JLennerz@partners.org.

Abstract

Tissue microarrays (TMA) have become an important tool in high-throughput molecular profiling of tissue samples in the translational research setting. Unfortunately, high-throughput profiling in small biopsy specimens or rare tumor samples (eg, orphan diseases or unusual tumors) is often precluded owing to limited amounts of tissue. To overcome these challenges, we devised a method that allows tissue transfer and construction of TMAs from individual 2- to 5-μm sections for subsequent molecular profiling. We named the technique slide-to-slide (STS) transfer, and it requires a series of chemical exposures (so-called xylene-methacrylate exchange) in combination with rehydrated lifting, microdissection of donor tissues into multiple small tissue fragments (methacrylate-tissue tiles), and subsequent remounting on separate recipient slides (STS array slide). We developed the STS technique by assessing the efficacy and analytical performance using the following key metrics: (a) dropout rate, (b) transfer efficacy, (c) success rates using different antigen-retrieval methods, (d) success rates of immunohistochemical stains, (e) fluorescent in situ hybridization success rates, and (f) DNA and (g) RNA extraction yields from single slides, which all functioned appropriately. The dropout rate ranged from 0.7% to 6.2%; however, we applied the same STS technique successfully to fill these dropouts ("rescue" transfer). Hematoxylin and eosin assessment of donor slides confirmed a transfer efficacy of >93%, depending on the size of the tissue (range, 76%-100%). Fluorescent in situ hybridization success rates and nucleic acid yields were comparable with those of traditional workflows. In this study, we present a quick, reliable, and cost-effective method that offers the key advantages of TMAs and other molecular techniques-even when tissue is sparse. The perspectives of this technology in biomedical sciences and clinical practice are promising, given that it allows laboratories to create more data with less tissue.

Keywords: biomarker; limitations; limited tissue; orphan disease; tissue rescue.

Publication types

Research Support, Non-U.S. Gov't
Research Support, N.I.H., Extramural

MeSH terms

DNA
Humans
In Situ Hybridization, Fluorescence
Neoplasms* / genetics
Tissue Array Analysis / methods

Substances

DNA

Grants and funding

R37 CA225655/CA/NCI NIH HHS/United States