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去极化降低动脉平滑肌中肌球蛋白轻链激酶的[Ca2+]i敏感性:水母发光蛋白和fura 2对[Ca2+]i估计值的比较

Depolarization decreases the [Ca2+]i sensitivity of myosin light-chain kinase in arterial smooth muscle: comparison of aequorin and fura 2 [Ca2+]i estimates.

作者信息

Gilbert E K, Weaver B A, Rembold C M

机构信息

Department of Internal Medicine, University of Virginia Health Science Center, Charlottesville 22908.

出版信息

FASEB J. 1991 Aug;5(11):2593-9. doi: 10.1096/fasebj.5.11.1868983.

DOI:10.1096/fasebj.5.11.1868983
PMID:1868983
Abstract

Histamine stimulation of swine arterial smooth muscle is associated with a high [Ca2+]i sensitivity for increases in myosin light-chain phosphorylation. In contrast, KCl depolarization produces a relatively lower [Ca2+]i sensitivity (i.e., similar increases in [Ca2+]i induce less myosin phosphorylation). We evaluated whether 1) artifacts in the methodology for measuring [Ca2+]i or 2) true alterations in the [Ca2+]i sensitivity of myosin light-chain kinase were responsible for these apparent changes in the [Ca2+]i sensitivity of phosphorylation. The [Ca2+]i sensitivity of phosphorylation was higher with histamine stimulation regardless of whether the [Ca2+]i indicator was aequorin (which was loaded intracellularly by reversible hyperpermeabilization) or Fura 2 (which was loaded intracellularly by incubation of the tissues in Fura 2 AM). Aequorin and Fura 2 appeared to detect qualitatively similar stimulus-induced changes in [Ca2+]i with the exception that the initial response to histamine stimulation was different (histamine initially induced a large aequorin light transient and a relatively smaller increase in Fura 2 fluorescence). The [Ca2+]i sensitivity of myosin light-chain kinase extracted from KCl depolarized tissues was lower than the [Ca2+]i sensitivity of myosin light-chain kinase extracted from unstimulated or histamine stimulated tissues. These results suggest that depolarization specifically modifies myosin light-chain kinase to decrease its [Ca2+]i sensitivity. Changes in the [Ca2+]i sensitivity of myosin light-chain phosphorylation are not an artifact of the [Ca2+]i measurement technique.

摘要

组胺刺激猪动脉平滑肌时,肌球蛋白轻链磷酸化增加与高[Ca2+]i敏感性相关。相比之下,氯化钾去极化产生的[Ca2+]i敏感性相对较低(即,[Ca2+]i的类似增加诱导较少的肌球蛋白磷酸化)。我们评估了1)测量[Ca2+]i方法中的假象,或2)肌球蛋白轻链激酶的[Ca2+]i敏感性的真正改变是否是磷酸化的[Ca2+]i敏感性这些明显变化的原因。无论[Ca2+]i指示剂是水母发光蛋白(通过可逆性高通透性细胞内加载)还是Fura 2(通过将组织在Fura 2 AM中孵育细胞内加载),组胺刺激时磷酸化的[Ca2+]i敏感性都较高。除了对组胺刺激的初始反应不同(组胺最初诱导大水母发光蛋白光瞬变和Fura 2荧光相对较小的增加)外,水母发光蛋白和Fura 2似乎在定性上检测到类似的刺激诱导的[Ca2+]i变化。从氯化钾去极化组织中提取的肌球蛋白轻链激酶的[Ca2+]i敏感性低于从未刺激或组胺刺激组织中提取的肌球蛋白轻链激酶的[Ca2+]i敏感性。这些结果表明,去极化特异性地修饰肌球蛋白轻链激酶以降低其[Ca2+]i敏感性。肌球蛋白轻链磷酸化的[Ca2+]i敏感性变化不是[Ca2+]i测量技术的假象。

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