Acute, pro‐contractile effects of prorenin on rat mesenteric arteries

Author:

Rognant Salomé1ORCID,Baldwin Samuel N.1ORCID,Pritchard Harry A. T.23ORCID,Greenstein Adam23ORCID,Calloe Kirstine4ORCID,Aalkjaer Christian5ORCID,Jepps Thomas A.1ORCID

Affiliation:

1. Department of Biomedical Sciences University of Copenhagen Copenhagen N Denmark

2. Division of Cardiovascular Sciences, Faculty of Biology, Medicine and Health Manchester University Teaching Hospitals NHS Foundation Trust, University of Manchester Manchester UK

3. Geoffrey Jefferson Brain Research Centre, The Manchester Academic Health Science Centre, Northern Care Alliance NHS Foundation Trust University of Manchester Manchester UK

4. Section for Pathobiological Sciences, Department of Veterinary and Animal Sciences University of Copenhagen Frederiksberg C Denmark

5. Department of Biomedicine Aarhus University Aarhus C Denmark

Abstract

AbstractProrenin and the prorenin receptor ((P)RR) are important, yet controversial, members of the renin–angiotensin–aldosterone system. The ((P)RR) is expressed throughout the body, including the vasculature, however, the direct effect of prorenin on arterial contractility is yet to be determined. Within rat mesenteric arteries, immunostaining and proximity ligation assays were used to determine the interacting partners of (P)RR in freshly isolated vascular smooth muscle cells (VSMCs). Wire myography examined the functional effect of prorenin. Simultaneous changes in [Ca2+]i and force were recorded in arteries loaded with Fura‐2AM. Spontaneously transient outward currents were recorded via perforated whole‐cell patch‐clamp configuration in freshly isolated VSMCs. We found that the (P)RR is located within a distance of less than 40 nm from the V‐ATPase, caveolin‐1, ryanodine receptors, and large conductance Ca2+‐activated K+ channels (BKCa) in VSMCs. [Ca2+]i imaging and isometric tension recordings indicate that 1 nM prorenin enhanced α1‐adrenoreceptor‐mediated contraction, associated with an increased number of Ca2+ waves, independent of voltage‐gated Ca2+ channels activation. Incubation of VSMCs with 1 nM prorenin decreased the amplitude and frequency of spontaneously transient outward currents and attenuated BKCa‐mediated relaxation. Inhibition of the V‐ATPase with 100 nM bafilomycin prevented prorenin‐mediated inhibition of BKCa‐derived relaxation. Renin (1 nM) had no effect on BKCa‐mediated relaxation. In conclusion, prorenin enhances arterial contractility by inhibition of BKCa and increasing intracellular Ca2+ release. It is likely that this effect is mediated through a local shift in pH upon activation of the (P)RR and stimulation of the V‐ATPase.

Funder

Carlsbergfondet

Lundbeckfonden

Publisher

Wiley

Subject

Genetics,Molecular Biology,Biochemistry,Biotechnology

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