The Evolution of Erythrocytes Becoming Red in Respect to Fluorescence

Laura Hertz,Petra Weissgerber,Sandra Ruppenthal,Polina Petkova-Kirova,Christian Wagner,Greta Simionato,Ulrich Boehm,Lars Kaestner,Stephan Quint,Asena Abay,Matthias W Laschke,Alexander Kihm

doi:10.3389/fphys.2019.00753

Laura Hertz, Petra Weissgerber + Show 10 more

Open Access

https://doi.org/10.3389/fphys.2019.00753

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Abstract

Very young red blood cells, namely reticulocytes, can be quite easily recognized and labeled by cluster of differentiation antibodies (CD71, transferrin receptor) or by staining remnant RNA with thiazol orange. In contrast, age specific erythrocyte labeling is more difficult in later periods of their life time. While erythrocytes contain band 4.1 protein, a molecular clock, so far it has not been possible to read this clock on individual cells. One concept to track erythrocytes during their life time is to mark them when they are young, either directly in vivo or ex vivo followed by a transfusion. Several methods like biotinylation, use of isotopes or fluorescent labeling have proved to be useful experimental approaches but also have several inherent disadvantages. Genetic engineering of mice provides additional options to express fluorescent proteins in erythrocytes. To allow co-staining with popular green fluorescent dyes like Fluo-4 or other fluorescein-based dyes, we bred a mouse line expressing a tandem red fluorescent protein (tdRFP). Within this Brief Research Report, we provide the initial characterisation of this mouse line and show application examples ranging from transfusion experiments and intravital microscopy to multicolour flow cytometry and confocal imaging. We provide a versatile new tool for erythrocyte research and discuss a range of experimental opportunities to study membrane processes and other aspects of erythrocyte development and aging with help of these animals.

Highlights

We face many scenarios in erythrocyte research where we need to label erythrocytes
Fluorescence intensity in erythrocytes is sufficient for a range of applications in erythrocyte research such as 3D-shape analysis (Figure 1Db and Supplementary Video 1), transfusion experiments (Figures 2A,Ba), intravital microscopy (Figure 2B and Supplementary Video 2) and fluorescence multiplexing (Figures 2Aa,C)
All authors listed have made a substantial, direct and intellectual contribution to the work, and approved it for publication

Summary

INTRODUCTION

We face many scenarios in erythrocyte research where we need to label erythrocytes This might be in the context of determining a particular cell shape (Quint et al, 2017), transfusion experiments (Dholakia et al, 2015) or following cell age (Wang et al, 2013). There are numerous strategies available to label erythrocytes based on small molecular dyes (Haugland, 2002), antibodies (Pepe, 1968) or fluorescent proteins (Jung, 2011). The latter one has particular advantages such as high biocompatibility due to cell internal translation, permanent expression and specific subcellular localization (Kaestner et al, 2014). We set out to genetically label erythrocytes with red fluorescence in mice

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