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首页> 外文期刊>American Journal of Physiology >Determinants of kinin release in isolated rat hindquarters.
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Determinants of kinin release in isolated rat hindquarters.

机译:激肽释放在离体大鼠后肢的决定因素。

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We studied the determinants of kinin release into the venous effluent of rat hindquarters perfused with Krebs bicarbonate buffer. Kinin release in preparations perfused with control media (14.6 +/- 2.5-20.7 +/- 6.7 pg/15 min) was surpassed by that in preparations perfused with media containing kininase inhibitors (243 +/- 53 to 276 +/- 78 pg/15 min). Kinin release increased when purified kininogen (from 242 +/- 43 to 3,365 +/- 725 pg/15 min) or kallikrein (from 270 +/- 49 to 30,649 +/- 8,040 pg/15 min) was added to the perfusate. Conversely, kinin release fell when the kallikrein inhibitor aprotinin (from 272 +/- 58 to 122 +/- 27 pg/15 min) or soybean trypsin inhibitor (from 273 +/- 52 to 195 +/- 25 pg/15 min) was added. Both basal and kininogen-induced kinin release were attenuated in preparations perfused with media containing cycloheximide, a protein synthesis inhibitor, but kallikrein-induced kinin release was not. These data suggest that kinin release from perfused rat hindquarters reflects the activity of both the kinin-degrading and kinin-generating pathways and that the latter is sustained by a kallikrein manufactured de novo and by preexistent kininogen(s).
机译:我们研究了灌注Krebs碳酸氢盐缓冲液的大鼠后肢静脉排泄物中激肽释放的决定因素。灌注含对照培养基的制剂(14.6 +/- 2.5-20.7 +/- 6.7 pg / 15 min)中的激肽释放超过含激肽酶抑制剂(243 +/- 53至276 +/- 78 pg的培养基)的制剂中的激肽释放/ 15分钟)。将纯化的激肽原(242 +/- 43至3,365 +/- 725 pg / 15分钟)或激肽释放酶(从270 +/- 49至30,649 +/- 8,040 pg / 15分钟)添加到灌注液中,激肽释放增加。相反,激肽释放酶抑制剂抑肽酶(从272 +/- 58到122 +/- 27 pg / 15分钟)或大豆胰蛋白酶抑制剂(从273 +/- 52到195 +/- 25 pg / 15分钟)时激肽释放下降。加入。在灌注含有蛋白质合成抑制剂环己酰亚胺的培养基的制剂中,基础和激肽原诱导的激肽释放均减弱,但激肽释放酶诱导的激肽释放未降低。这些数据表明,从灌注大鼠后肢释放的激肽反映了激肽降解和激肽生成途径的活性,并且后者由从头制造的激肽释放酶和先前存在的激肽原维持。

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