Expression of Ca2+-activated K+ channels and their role in proliferation of rat cardiac fibroblasts
- Authors
- Choi, Seyong; Lee, Wooseok; Yun, Jihyun; Seo, Jeongseok; Lim, Inja
- Issue Date
- Apr-2008
- Publisher
- KOREAN JOURNAL OF PHYSIOLOGY & PHARMACOLOGY
- Keywords
- cardiac fibroblasts; Ca2+-activated K+ channels; proliferation
- Citation
- KOREAN JOURNAL OF PHYSIOLOGY & PHARMACOLOGY, v.12, no.2, pp 51 - 58
- Pages
- 8
- Journal Title
- KOREAN JOURNAL OF PHYSIOLOGY & PHARMACOLOGY
- Volume
- 12
- Number
- 2
- Start Page
- 51
- End Page
- 58
- URI
- https://scholarworks.bwise.kr/cau/handle/2019.sw.cau/23788
- DOI
- 10.4196/kjpp.2008.12.2.51
- ISSN
- 1226-4512
2093-3827
- Abstract
- Cardiac fibroblasts constitute one of the largest cell populations in the heart, and contribute to structural, biochemical, mechanical and electrical properties of the myocardium. Nonetheless, their cardiac functions, especially electrophysiological properties, have often been disregarded in studies. Ca2+-activated K+ (K-Ca) channels can control Ca2+ influx as well as a number of Ca2+-dependent physiological processes. We, therefore, attempted to identify and characterize K-Ca. channels in rat Cardiac fibroblasts. First, we showed that the cells cultured from the rat ventricle were cardiac fibroblasts by immunostaining for discoidin domain receptor 2 (DDR-2), a specific fibroblast marker. Secondly, we detected the expression of various KCa channels by reverse transcription polymerase chain reaction (RT-PCR), and found all three family members of K-Ca. channels, including large conductance K-Ca (BK-alpha 1- and -beta 1 similar to 4 subunits), intermediate conductance K-Ca (IK), and small conductance K-Ca (SK1 similar to 4 subunits) channels. Thirdly, we recorded BK, IK, and SK channels by whole cell mode patch clamp technique using their specific blockers. Finally, we performed cell proliferation assay to evaluate the effects of the channels on cell proliferation, and found that the inhibition of IK channel increased the cell proliferation. These results showed the existence of BK, IK, and SK channels in rat ventricular fibroblasts and involvement of IK channel in cell proliferation.
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