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用fura-2盐显微注射大鼠心脏小梁的荧光特性。

Fluorescent properties of rat cardiac trabeculae microinjected with fura-2 salt.

作者信息

Backx P H, Ter Keurs H E

机构信息

Department of Medicine and Medical Physiology, University of Calgary, Alberta, Canada.

出版信息

Am J Physiol. 1993 Apr;264(4 Pt 2):H1098-110. doi: 10.1152/ajpheart.1993.264.4.H1098.

Abstract

We have measured force, sarcomere length, and Ca2+ during twitches in rat cardiac trabeculae. To avoid the difficulties associated with fura-2/acetoxymethyl ester (AM), fura-2 salt was iontophoretically microinjected into the preparation using a single impalement site; this is possible because fura-2 diffuses through the gap junctions between cells. By use of this method, the estimated peak of the [Ca2+] transient during a twitch was not statistically different at different sarcomere lengths: 875 +/- 92 nM at a sarcomere length of 2.15 microns vs. 905 +/- 67 nM at a sarcomere length of 1.65 microns (means +/- SD, n = 10). When trabeculae were loaded using fura-2/AM, the estimated peak of the [Ca2+] transient at a sarcomere length of 2.15 microns was 540 +/- 180 nM (means +/- SD, n = 5). The time course of the Ca2+ transients at different sarcomere lengths is qualitatively similar, but small systematic differences were observed during the relaxation period. On the other hand, the duration of twitch force increases dramatically as the muscle length is increased. As a result, when the trabeculae were held at short muscle lengths, the temporal relationship between force and the Ca2+ transient resembled the relationship between cell shortening and the Ca2+ transient measured in isolated myocytes. At longer lengths the temporal relationship between force and the Ca2+ transient more closely resembles that obtained in papillary muscles using aequorin.

摘要

我们在大鼠心脏小梁的单收缩过程中测量了力、肌节长度和钙离子浓度。为避免与fura-2/乙酰氧甲酯(AM)相关的困难,使用单个刺入位点将fura-2盐通过离子电渗法微量注射到标本中;这是可行的,因为fura-2可通过细胞间的缝隙连接扩散。通过使用这种方法,在不同肌节长度下单收缩期间[Ca2+]瞬变的估计峰值在统计学上无差异:肌节长度为2.15微米时为875±92 nM,而肌节长度为1.65微米时为905±67 nM(均值±标准差,n = 10)。当小梁用fura-2/AM加载时,肌节长度为2.15微米时[Ca2+]瞬变的估计峰值为540±180 nM(均值±标准差,n = 5)。不同肌节长度下Ca2+瞬变的时间进程在定性上相似,但在舒张期观察到了小的系统性差异。另一方面,随着肌肉长度增加,单收缩力的持续时间显著增加。因此,当小梁保持在短肌肉长度时,力与Ca2+瞬变之间的时间关系类似于在分离的心肌细胞中测量的细胞缩短与Ca2+瞬变之间的关系。在更长的长度下,力与Ca2+瞬变之间的时间关系更类似于使用水母发光蛋白在乳头肌中获得的关系。

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