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大电导钙激活钾通道β1亚基的去糖基化改变其生物物理特性。

Deglycosylation of the beta1-subunit of the BK channel changes its biophysical properties.

作者信息

Hagen Brian M, Sanders Kenton M

机构信息

Department of Physiology and Cell Biology, University of Nevada School of Medicine, Reno, Nevada 89557-0046, USA.

出版信息

Am J Physiol Cell Physiol. 2006 Oct;291(4):C750-6. doi: 10.1152/ajpcell.00116.2006. Epub 2006 May 31.

DOI:10.1152/ajpcell.00116.2006
PMID:16738006
Abstract

Large-conductance Ca(2+)-activated potassium (BK) channels are composed of pore-forming alpha-subunits and auxiliary beta-subunits. The alpha-subunits are widely expressed in many cell types, whereas the beta-subunits are more tissue specific and influence diverse aspects of channel function. In the current study, we identified the presence of the smooth muscle-specific beta1-subunit in murine colonic tissue using Western blotting. The native beta1-subunits migrated in SDS-PAGE as two molecular mass bands. Enzymatic removal of N-linked glycosylations from the beta1-subunit resulted in a single band that migrated at a lower molecular mass than the native beta1-subunit bands, suggesting that the native beta1-subunit exists in either a core glycosylated or highly glycosylated form. We investigated the functional consequence of deglycosylating the beta1-subunit during inside-out single-channel recordings. During inside-out single-channel recordings, with N-glycosidase F in the pipette solution, the open probability (P(o)) and mean open time of BK channels increased in a time-dependent manner. Deglycosylation of BK channels did not affect the conductance but shifted the steady-state voltage of activation toward more positive potentials without affecting slope when Ca(2+) concentration was <1 microM. Treatment of myocytes lacking the beta1-subunits of the BK channel with N-glycosidase F had no effect. These data suggest that glycosylations on the beta1-subunit in smooth muscle cells can modify the biophysical properties of BK channels.

摘要

大电导钙激活钾(BK)通道由形成孔道的α亚基和辅助β亚基组成。α亚基在多种细胞类型中广泛表达,而β亚基则更具组织特异性,并影响通道功能的多个方面。在本研究中,我们通过蛋白质免疫印迹法确定了小鼠结肠组织中存在平滑肌特异性β1亚基。天然的β1亚基在SDS-PAGE中迁移为两条分子量条带。对β1亚基进行N-糖基化的酶促去除后,产生了一条迁移分子量低于天然β1亚基带的单一条带,这表明天然β1亚基以核心糖基化或高度糖基化形式存在。我们在向外膜片钳单通道记录过程中研究了β1亚基去糖基化的功能后果。在向外膜片钳单通道记录过程中,当移液管溶液中存在N-糖苷酶F时,BK通道的开放概率(P(o))和平均开放时间呈时间依赖性增加。BK通道的去糖基化不影响电导,但当Ca(2+)浓度<1 microM时,将激活的稳态电压向更正的电位移动,而不影响斜率。用N-糖苷酶F处理缺乏BK通道β1亚基的心肌细胞没有效果。这些数据表明,平滑肌细胞中β1亚基上的糖基化可以改变BK通道的生物物理特性。

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