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The effects of exogenous calcium buffers on the systolic calcium transient in rat ventricular myocytes.

机译:外源钙缓冲剂对大鼠心室肌细胞收缩钙瞬变的影响。

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摘要

The aim of this work was to characterize the effects that two commonly used "caged" calcium buffers (NP-EGTA and nitr-5) have on the amplitude and time course of decay of the calcium transient. We made quantitative measurements of both free and total calcium using the measured buffering properties of the cell. Intracellular calcium concentration ([Ca(2+)](i)) was measured with fluo-3 in rat ventricular myocytes. Incorporation of the buffer NP-EGTA decreased both the amplitude and rate of decay of the caffeine response. The slowing could be quantitatively accounted for by the measured increased buffering. These effects were removed by photolysis of NP-EGTA. Similar results were obtained with nitr-5 except that the effects were not completely removed by photolysis. This was shown to be due to the persistence of a component of the increased buffering after photolysis. Both buffers decreased the amplitude of the systolic calcium transient. However, although nitr-5 produced a simple slowing of the decay, NP-EGTA resulted in an initial rapid phase of decay. This rapid phase of decay is attributed to calcium binding to NP-EGTA. This work represents the first quantitative analysis of the effects that extra buffering by a fast and a slow calcium chelator may have on the calcium transient.
机译:这项工作的目的是表征两种常用的“笼式”钙缓冲液(NP-EGTA和nitro-5)对钙瞬变衰减幅度和时间过程的影响。我们使用细胞的缓冲特性对游离钙和总钙进行了定量测量。用fluo-3测定大鼠心室肌细胞中的细胞内钙浓度([Ca(2 +)](i))。缓冲液NP-EGTA的加入降低了咖啡因反应的幅度和衰减率。减慢可以通过所测量的增加的缓冲来定量地解释。通过NP-EGTA的光解作用消除了这些影响。使用硝化氮5可获得类似的结果,除了通过光解不能完全消除影响。已证明这是由于光解后持久的增加缓冲成分的缘故。两种缓冲液均降低了收缩期钙瞬变的幅度。然而,尽管硝5产生了简单的衰减减慢,但是NP-EGTA导致了衰减的初始快速阶段。衰变的快速阶段归因于钙与NP-EGTA的结合。这项工作代表了对快速和慢速钙螯合剂额外缓冲可能对钙瞬变产生的影响的首次定量分析。

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