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大鼠尾动脉和鸡砂囊肌丝中肌球蛋白的非钙依赖性磷酸化

Ca2+-independent phosphorylation of myosin in rat caudal artery and chicken gizzard myofilaments.

作者信息

Weber L P, Van Lierop J E, Walsh M P

机构信息

Smooth Muscle Research Group and Department of Biochemistry and Molecular Biology, Faculty of Medicine, University of Calgary, 3330 Hospital Drive N.W., Calgary, Alberta, Canada T2N 4N1.

出版信息

J Physiol. 1999 May 1;516 ( Pt 3)(Pt 3):805-24. doi: 10.1111/j.1469-7793.1999.0805u.x.

DOI:10.1111/j.1469-7793.1999.0805u.x
PMID:10200427
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2269290/
Abstract
  1. Smooth muscle contraction is activated primarily by the Ca2+-calmodulin (CaM)-dependent phosphorylation of the 20 kDa light chains (LC20) of myosin. Activation can also occur in some instances without a change in intracellular free [Ca2+] or indeed in a Ca2+-independent manner. These signalling pathways often involve inhibition of myosin light chain phosphatase and unmasking of basal kinase activity leading to LC20 phosphorylation and contraction. 2. We have used demembranated rat caudal arterial smooth muscle strips and isolated chicken gizzard myofilaments in conjunction with the phosphatase inhibitor microcystin-LR to investigate the mechanism of Ca2+-independent phosphorylation of LC20 and contraction. 3. Treatment of Triton X-100-demembranated rat caudal arterial smooth muscle strips with microcystin at pCa 9 triggered a concentration-dependent contraction that was slower than that induced by pCa 4.5 or 6 but reached comparable steady-state levels of tension. 4. This Ca2+-independent, microcystin-induced contraction correlated with phosphorylation of LC20 at serine-19 and threonine-18. 5. Whereas Ca2+-dependent LC20 phosphorylation and contraction were inhibited by a synthetic peptide (AV25) based on the autoinhibitory domain of myosin light chain kinase (MLCK), Ca2+-independent, microcystin-induced LC20 phosphorylation and contraction were resistant to AV25. 6. Ca2+-independent LC20 kinase activity was also detected in chicken gizzard smooth muscle myofilaments and catalysed phosphorylation of endogenous myosin LC20 at serine-19 and/or threonine-18. This is in contrast to MLCK which phosphorylates threonine-18 only after prior phosphorylation of serine-19. 7. Gizzard Ca2+-independent LC20 kinase could be separated from MLCK by differential extraction from myofilaments and by CaM affinity chromatography. Its activity was resistant to AV25. 8. We conclude that inhibition of smooth muscle myosin light chain phosphatase (MLCP) unmasks the activity of a Ca2+-independent LC20 kinase associated with the myofilaments and distinct from MLCK. This kinase, therefore, probably plays a role in Ca2+ sensitization and Ca2+-independent contraction of smooth muscle in response to stimuli that act via Ca2+-independent pathways, leading to inhibition of MLCP.
摘要
  1. 平滑肌收缩主要由肌球蛋白20kDa轻链(LC20)的Ca2 + -钙调蛋白(CaM)依赖性磷酸化激活。在某些情况下,激活也可能在细胞内游离[Ca2 +]没有变化的情况下发生,或者实际上以不依赖Ca2 +的方式发生。这些信号通路通常涉及肌球蛋白轻链磷酸酶的抑制和基础激酶活性的暴露,导致LC20磷酸化和收缩。2. 我们使用去膜大鼠尾动脉平滑肌条和分离的鸡砂囊肌丝,结合磷酸酶抑制剂微囊藻毒素-LR,来研究LC20不依赖Ca2 +的磷酸化和收缩机制。3. 在pCa 9时用微囊藻毒素处理经Triton X-100去膜的大鼠尾动脉平滑肌条,引发了浓度依赖性收缩,该收缩比pCa 4.5或6诱导的收缩慢,但达到了相当的稳态张力水平。4. 这种不依赖Ca2 +、微囊藻毒素诱导的收缩与LC20在丝氨酸-19和苏氨酸-18处的磷酸化相关。5. 基于肌球蛋白轻链激酶(MLCK)的自身抑制结构域的合成肽(AV25)抑制了依赖Ca2 +的LC20磷酸化和收缩,而不依赖Ca2 +、微囊藻毒素诱导的LC20磷酸化和收缩对AV25具有抗性。6. 在鸡砂囊平滑肌肌丝中也检测到了不依赖Ca2 +的LC20激酶活性,并且催化了内源性肌球蛋白LC20在丝氨酸-19和/或苏氨酸-18处的磷酸化。这与MLCK不同,MLCK仅在丝氨酸-19预先磷酸化后才磷酸化苏氨酸-18。7. 通过从肌丝中进行差异提取和通过CaM亲和色谱法,可以将砂囊不依赖Ca2 +的LC20激酶与MLCK分离。其活性对AV25具有抗性。8. 我们得出结论,平滑肌肌球蛋白轻链磷酸酶(MLCP)的抑制暴露了一种与肌丝相关且不同于MLCK的不依赖Ca2 +的LC20激酶的活性。因此,这种激酶可能在平滑肌对通过不依赖Ca2 +的途径起作用的刺激的Ca2 +致敏和不依赖Ca2 +的收缩中起作用,导致MLCP的抑制。

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