Beta adrenergic overstimulation impaired vascular contractility via actin-cytoskeleton disorganization in rabbit cerebral artery

Hyoung Kyu Kim; Won Sun Park; Mohamad Warda; So Youn Park; Eun A Ko; Min Hee Kim; Seung Hun Jeong; Hye-Jin Heo; Tae-Hoon Choi; Young-Won Hwang; Sun-Il Lee; Kyung Soo Ko; Byoung Doo Rhee; Nari Kim; Jin Han

doi:10.1371/journal.pone.0043884

Beta adrenergic overstimulation impaired vascular contractility via actin-cytoskeleton disorganization in rabbit cerebral artery

PLoS One. 2012;7(8):e43884. doi: 10.1371/journal.pone.0043884. Epub 2012 Aug 20.

Authors

Hyoung Kyu Kim¹, Won Sun Park, Mohamad Warda, So Youn Park, Eun A Ko, Min Hee Kim, Seung Hun Jeong, Hye-Jin Heo, Tae-Hoon Choi, Young-Won Hwang, Sun-Il Lee, Kyung Soo Ko, Byoung Doo Rhee, Nari Kim, Jin Han

Affiliation

¹ National Research Laboratory for Mitochondrial Signaling, Department of Physiology, College of Medicine, Cardiovascular and Metabolic Disease Center, Inje University, Busan, Korea.

Abstract

Background and purpose: Beta adrenergic overstimulation may increase the vascular damage and stroke. However, the underlying mechanisms of beta adrenergic overstimulation in cerebrovascular dysfunctions are not well known. We investigated the possible cerebrovascular dysfunction response to isoproterenol induced beta-adrenergic overstimulation (ISO) in rabbit cerebral arteries (CAs).

Methods: ISO was induced in six weeks aged male New Zealand white rabbit (0.8-1.0 kg) by 7-days isoproterenol injection (300 μg/kg/day). We investigated the alteration of protein expression in ISO treated CAs using 2DE proteomics and western blot analysis. Systemic properties of 2DE proteomics result were analyzed using bioinformatics software. ROS generation and following DNA damage were assessed to evaluate deteriorative effect of ISO on CAs. Intracellular Ca(2+) level change and vascular contractile response to vasoactive drug, angiotensin II (Ang II), were assessed to evaluate functional alteration of ISO treated CAs. Ang II-induced ROS generation was assessed to evaluated involvement of ROS generation in CA contractility.

Results: Proteomic analysis revealed remarkably decreased expression of cytoskeleton organizing proteins (e.g. actin related protein 1A and 2, α-actin, capping protein Z beta, and vimentin) and anti-oxidative stress proteins (e.g. heat shock protein 9A and stress-induced-phosphoprotein 1) in ISO-CAs. As a cause of dysregulation of actin-cytoskeleton organization, we found decreased level of RhoA and ROCK1, which are major regulators of actin-cytoskeleton organization. As functional consequences of proteomic alteration, we found the decreased transient Ca(2+) efflux and constriction response to angiotensin II and high K(+) in ISO-CAs. ISO also increased basal ROS generation and induced oxidative damage in CA; however, it decreased the Ang II-induced ROS generation rate. These results indicate that ISO disrupted actin cytoskeleton proteome network through down-regulation of RhoA/ROCK1 proteins and increased oxidative damage, which consequently led to contractile dysfunction in CA.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Actin Cytoskeleton / metabolism*
Angiotensin II / pharmacology
Animals
Cerebral Arteries / drug effects*
Cerebral Arteries / metabolism*
Isoproterenol / pharmacology*
Male
Rabbits
Reactive Oxygen Species / metabolism
rho-Associated Kinases / metabolism
rhoA GTP-Binding Protein / metabolism

Substances

Reactive Oxygen Species
Angiotensin II
rho-Associated Kinases
rhoA GTP-Binding Protein
Isoproterenol

Grants and funding

This research was supported by the Basic Science Research Program through the National Research Foundation of Korea (NRF) funded by the Ministry of Education, Science and Technology (2010-0020224 and NRF- 2009-0067574). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.