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内皮源性舒张因子的释放受搏动性血流的频率和幅度的调节。

Release of endothelium-derived relaxing factor is modulated both by frequency and amplitude of pulsatile flow.

作者信息

Hutcheson I R, Griffith T M

机构信息

Department of Diagnostic Radiology, University of Wales College of Medicine, Heath Park, Cardiff, United Kingdom.

出版信息

Am J Physiol. 1991 Jul;261(1 Pt 2):H257-62. doi: 10.1152/ajpheart.1991.261.1.H257.

Abstract

We have dissociated the effects of frequency and amplitude of pulsatile flow on flow-induced release of endothelium-derived relaxing factor (EDRF) using cascade bioassay. Rat aortic segments were buffer perfused with a peristaltic pump at a constant mean flow rate of 9 ml/min. EDRF activity in effluent was measured by relaxation of endothelium-denuded rabbit aortic rings preconstricted by phenylephrine. Pulse frequency was varied over the range 0.1-12 Hz at a constant amplitude of 2 mmHg; pulse amplitude was varied over the range 2-16 mmHg at a constant frequency of 0.1 Hz. Relaxation of the detector vessel depended on frequency of flow through the donor; peak response occurred between 4.2 and 6 Hz and was approximately three times greater than that induced at lower or higher frequencies. In contrast, increases in pulse pressure amplitude (maximum 16 mmHg) monotonically augmented constriction of partially preconstricted detector tissue by up to 10%. Incubation of the donor vessel with NG-nitro-L-arginine methyl ester (L-NAME), an inhibitor of nitric oxide synthesis, or removal of its endothelium by rubbing, abolished both the frequency- and the amplitude-dependent effects observed in the detector tissue, indicating that these were mediated by changes in EDRF release. Increasing the amplitude of the pressure pulse also reduced mean perfusion pressure (by up to 50%), implying distension of donor vessel since mean flow rate was constant. This fall in pressure was not affected by incubation with L-NAME or removal of endothelium, indicating that it was not dependent on EDRF activity.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

我们使用级联生物测定法,分离了搏动流的频率和振幅对内皮衍生舒张因子(EDRF)流动诱导释放的影响。用蠕动泵以9毫升/分钟的恒定平均流速对大鼠主动脉段进行缓冲灌注。通过苯肾上腺素预收缩的去内皮兔主动脉环的舒张来测量流出物中的EDRF活性。在2 mmHg的恒定振幅下,脉冲频率在0.1 - 12 Hz范围内变化;在0.1 Hz的恒定频率下,脉冲振幅在2 - 16 mmHg范围内变化。检测血管的舒张取决于通过供体血管的血流频率;峰值反应出现在4.2至6 Hz之间,大约是在较低或较高频率下诱导反应的三倍。相比之下,脉冲压力振幅的增加(最大16 mmHg)单调地增强了部分预收缩检测组织的收缩,增幅高达10%。用一氧化氮合成抑制剂NG - 硝基 - L - 精氨酸甲酯(L - NAME)孵育供体血管,或通过摩擦去除其内皮,消除了在检测组织中观察到的频率和振幅依赖性效应,表明这些效应是由EDRF释放的变化介导的。增加压力脉冲的振幅也降低了平均灌注压力(高达50%),这意味着供体血管扩张,因为平均流速是恒定的。这种压力下降不受L - NAME孵育或内皮去除的影响,表明它不依赖于EDRF活性。(摘要截短于250字)

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