慢速骨骼肌钙蛋白I在磷蛋白敲除小鼠心脏中的表达改变了肾上腺素能刺激的松弛作用

B. Wolska, Grace M. Arteaga, J. Peña, G. Nowak, Ronald M. Phillips, Shalini Sahai, Pieter P. de Tombe, Anne F. Martin, Evangelia G. Kranias, R. J. Solaro
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引用次数: 59

摘要

-肾上腺素能刺激心脏导致与心肌肌钙蛋白I (cTnI)和磷蛋白(PLB)磷酸化相关的松弛率增强。我们研究了通过与PLB敲除(PLBKO)小鼠杂交产生的表达慢速骨骼肌钙蛋白I (ssTnI)的小鼠的新品系。这种杂交产生了PLB/cTnI、PLB/ssTnI、PLBKO/cTnI和PLBKO/ssTnI小鼠。异丙肾上腺素(ISO)灌注显著提高了PLB/cTnI组、PLBKO/cTnI组和PLBKO/ssTnI组小鼠fura-2比值的峰值幅度。然而,在ISO存在的情况下,PLB/cTnI、PLBKO/cTnI和PLBKO/ssTnI小鼠心脏分离细胞中fura-2比值的峰值幅度没有差异。在PLB/cTnI小鼠细胞中,&bgr;-肾上腺素能刺激时,缩短程度增加,松弛时间明显缩短。在PLBKO/cTnI细胞中,ISO刺激导致缩短程度增加,而松弛时间没有变化。然而,用ISO刺激PLBKO/ssTnI小鼠分离的细胞不仅显著增加了细胞缩短的程度,而且增加了松弛的时间。我们还测定了在存在和不存在ISO的情况下,从所有四组动物分离的乳头肌松弛动力学。灌注ISO仅增加PLB/cTnI、PLB/ssTnI和PLBKO/cTnI肌肉的松弛率。在ISO刺激下,PLBKO/ssTnI肌肉的松弛时间不变。我们的数据直接表明,PLB和cTnI的磷酸化有助于在-肾上腺素能刺激期间增加松弛率。
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Expression of Slow Skeletal Troponin I in Hearts of Phospholamban Knockout Mice Alters the Relaxant Effect of &bgr;-Adrenergic Stimulation
&bgr;-Adrenergic stimulation of the heart results in an enhanced relaxation rate in association with phosphorylation of both cardiac troponin I (cTnI) and phospholamban (PLB). We studied new lines of mice generated by crossbreeding mice that express slow skeletal troponin I (ssTnI) with PLB knockout (PLBKO) mice. This crossbreeding resulted in the generation of PLB/cTnI, PLB/ssTnI, PLBKO/cTnI, and PLBKO/ssTnI mice. Perfusion with isoproterenol (ISO) significantly increased the peak amplitude of fura-2 ratio in PLB/cTnI, PLBKO/cTnI, and PLBKO/ssTnI groups of mice. However, in the presence of ISO, there were no differences in the peak amplitude of fura-2 ratio among cells isolated from hearts of PLB/cTnI, PLBKO/cTnI, and PLBKO/ssTnI mice. In cells from PLB/cTnI mice, the extent of shortening was increased and the time of relaxation was significantly decreased during &bgr;-adrenergic stimulation. In PLBKO/cTnI cells, stimulation with ISO resulted in an increased extent of shortening and no change in time of relaxation. However, stimulation with ISO in cells isolated from PLBKO/ssTnI mice not only significantly increased the extent of cell shortening but also increased the time of relaxation. We also determined the kinetics of relaxation of papillary muscles isolated from all four groups of animals in the presence and absence of ISO. Perfusion with ISO increased the rate of relaxation only in PLB/cTnI, PLB/ssTnI, and PLBKO/cTnI muscles. During ISO stimulation, the time of relaxation was unchanged in PLBKO/ssTnI muscles. Our data directly demonstrate that phosphorylation of both PLB and cTnI contributes to increased rate of relaxation during &bgr;-adrenergic stimulation.
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