Optimizing immunostaining of archival fish samples to enhance museum collection potential

Author:

Kwan Garfield T.ORCID,Frable Benjamin W.ORCID,Thompson Andrew R.ORCID,Tresguerres MartinORCID

Abstract

AbstractImmunohistochemistry (IHC) is a powerful biochemical technique that uses antibodies to specifically label and visualize proteins of interests within biological samples. However, fluid-preserved specimens within natural history collection often use fixatives and protocols that induce high background signal (autofluorescence), which hampers IHC as it produces low signal-to-noise ratio. Here, we explored techniques to reduce autofluorescence using sodium borohydride (SBH), citrate buffer, and their combination on fish tissue preserved with paraformaldehyde, formalin, ethanol, and glutaraldehyde. We found SBH was the most effective quenching technique, and applied this pretreatment to the gill or skin of 10 different archival fishes – including specimens that had been preserved in formalin or ethanol for up to 65 and 37 years, respectively. The enzyme Na+/K+-ATPase (NKA) was successfully immunostained and imaged using confocal fluorescence microscopy, allowing for the identification and characterization of NKA-rich ionocytes essential for fish ionic and acid-base homeostasis. Altogether, our SBH-based method facilitates the use of IHC on archival samples, and unlocks the historical record on fish biological responses to environmental factors (such as climate change) using specimens from natural history collections that were preserved decades to centuries ago.HighlightsSodium borohydride pretreatment reduced aldehyde-induced autofluorescenceSuccessfully immunostained archival samples of various fixative and fixation timeLarval fish that was formalin-fixed for 63-65 years was successfully immunostained

Publisher

Cold Spring Harbor Laboratory

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