Methods to measure calcitonin receptor activity, up-regulated in cell stress, apoptosis and autophagy [version 1; peer review: 2 approved]

Peter Wookey; Pragya Gupta; Lucas Bittencourt; Shane Cheung; David Hare; Sebastian Furness

doi:10.12688/f1000research.72845.1

F1000Research (Oct 2021)

Methods to measure calcitonin receptor activity, up-regulated in cell stress, apoptosis and autophagy [version 1; peer review: 2 approved]

Peter Wookey,
Pragya Gupta,
Lucas Bittencourt,
Shane Cheung,
David Hare,
Sebastian Furness

Affiliations

Peter Wookey: Medicine, University of Melbourne, Heidelberg, Victoria, 3084, Australia
Pragya Gupta: Medicine, University of Melbourne, Heidelberg, Victoria, 3084, Australia
Lucas Bittencourt: Medicine, University of Melbourne, Heidelberg, Victoria, 3084, Australia
Shane Cheung: BOMP, University of Melbourne, Parkville, Victoria, 3052, Australia
David Hare: Medicine, University of Melbourne, Heidelberg, Victoria, 3084, Australia
Sebastian Furness: School of Biomedical Sciences, Faculty of Medicine, The University of Queensland, St Lucia, Queensland, 4067, Australia

DOI: https://doi.org/10.12688/f1000research.72845.1
Journal volume & issue: Vol. 10

Abstract

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The expression of the calcitonin receptor (CT Receptor) is widespread throughout the life cycle of mammals and in many diseases, and in these contexts the functions of the common isoforms is largely unknown. The relatively recent development of anti-CT Receptor antibodies that bind separate epitopes on the CTa Receptor and CTb Receptor isoforms has advanced our knowledge and understanding of these events. CT Receptor at the protein level is upregulated in programmed cell death including apoptosis (as described in a previous publication) and autophagy, which is discussed in our upcoming, unpublished review. Incomplete data sets are cited in this review on the upregulation of CACLR (encoding CT Receptor) mRNA, in particular the insert-positive isoform (CTb Receptor), in response to cell stress. Cell stress is induced by growth in depleted foetal bovine serum (dFBS) or without FBS, both of which induce degrees of starvation and autophagy, or dFBS plus staurosporine, which induces apoptosis. Details of the methods deployed to generate these data are described here including measurement of the upregulation of CTb Receptor mRNA with qPCR and nanopore long range sequencing. An anti-CT Receptor antibody also known as CalRexinTM, which binds an epitope in the N-terminal domain, was conjugated to either fluorophore 568, which is accumulated into apoptotic cells as previously reported, or pHrodo Red, a pH dependent fluorescent dye, which is accumulated into autophagic and apoptotic cells. These conjugates are under development to image programmed cell death. The methods for conjugation and high content imaging on the Operetta platform are described. The high fluorescence intensity at low pH of CalRexin:pHrodo Red in both autophagic and apoptotic cells suggests localisation in autophago-lysosomes and lysosomes respectively. Overall, these observations and the methods that underpin them have contributed to our understanding of the widespread expression of CT Receptor isoforms.

Published in F1000Research

ISSN: 2046-1402 (Online)
Publisher: F1000 Research Ltd
Country of publisher: United Kingdom
LCC subjects: Medicine; Science
Website: https://f1000research.com

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