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通过对豚鼠心肌细胞中笼锁钙进行双光子激发光解所揭示的基本钙释放事件。

Fundamental calcium release events revealed by two-photon excitation photolysis of caged calcium in Guinea-pig cardiac myocytes.

作者信息

Lipp P, Niggli E

机构信息

Department of Physiology, University of Bern, Buhlplatz 5, 3012 Bern, Switzerland.

出版信息

J Physiol. 1998 May 1;508 ( Pt 3)(Pt 3):801-9. doi: 10.1111/j.1469-7793.1998.801bp.x.

Abstract
  1. In cardiac muscle, 'Ca2+ sparks' have been proposed to underlie Ca2+-induced Ca2+ release (CICR), and to result from openings of clusters of Ca2+ channels (ryanodine receptors; RyRs) located in the sarcoplasmic reticulum membrane. 2. To investigate the elementary nature of these Ca2+ signals directly, a diffraction-limited point source of Ca2+ was created in single cardiac myocytes by two-photon excitation photolysis of caged Ca2+. Simultaneously, concentration profiles of released Ca2+ were imaged at high temporal and spatial resolution with a laser-scanning confocal microscope. 3. This approach enabled us to generate and detect photolytic Ca2+ signals that closely resembled the Ca2+ sparks occurring naturally, not only in amplitude and size, but also in their ability to trigger additional Ca2+ sparks or Ca2+ waves. 4. Surprisingly, at low photolytic power minuscule events with estimated Ca2+ release fluxes 20-40 times smaller than those calculated for a typical Ca2+ spark were directly resolved. These events appeared to arise from the opening of a more limited number of RyRs (possibly one) or from RyRs exhibiting a different gating mode and may correspond to the elusive 'Ca2+ quark'. 5. The Ca2+ quark represents the fundamental Ca2+ release event of excitable cells implementing hierarchical Ca2+ signalling systems with Ca2+ release events of various but distinct amplitude levels (i.e. Ca2+ quarks, Ca2+ sparks and full cellular Ca2+ transients). 6. A graded recruitment of nanoscopic Ca2+ release domains (i.e. Ca2+ quarks) exhibiting variable degrees of spatial coherence and coupling may then build up intermediate Ca2+ signalling events (i.e. Ca2+ sparks). This mechanism suggests the existence of Ca2+ sparks caused by gating of a variable fraction of RyRs from within an individual cluster. Additional mobilization of a variable number of these Ca2+ sparks enables cardiac cells to show graded cellular Ca2+ transients. Similar recruitment processes may underlie regulation of Ca2+ signalling on the cellular level in general.
摘要
  1. 在心肌中,“Ca2+ 火花”被认为是 Ca2+ 诱导的 Ca2+ 释放(CICR)的基础,并且是由位于肌浆网膜上的 Ca2+ 通道簇(兰尼碱受体;RyRs)开放所导致的。2. 为了直接研究这些 Ca2+ 信号的基本性质,通过对笼锁 Ca2+ 进行双光子激发光解,在单个心肌细胞中创建了一个衍射极限的 Ca2+ 点源。同时,使用激光扫描共聚焦显微镜以高时间和空间分辨率对释放的 Ca2+ 的浓度分布进行成像。3. 这种方法使我们能够生成并检测到光解 Ca2+ 信号,这些信号不仅在幅度和大小上,而且在触发额外 Ca2+ 火花或 Ca2+ 波的能力上,都与自然发生的 Ca2+ 火花非常相似。4. 令人惊讶的是,在低光解功率下,直接分辨出了估计 Ca2+ 释放通量比典型 Ca2+ 火花计算值小 20 - 40 倍的微小事件。这些事件似乎源于数量更有限的 RyRs(可能是一个)的开放,或者源于表现出不同门控模式的 RyRs,并且可能对应于难以捉摸的“Ca2+ 夸克”。5. Ca2+ 夸克代表了可兴奋细胞实现具有不同但独特幅度水平(即 Ca2+ 夸克、Ca2+ 火花和完整细胞 Ca2+ 瞬变)的分级 Ca2+ 信号系统的基本 Ca2+ 释放事件。6. 然后,对具有不同程度空间相干性和耦合的纳米级 Ca2+ 释放域(即 Ca2+ 夸克)进行分级募集,可能会形成中间 Ca2+ 信号事件(即 Ca2+ 火花)。这种机制表明存在由单个簇内可变比例的 RyRs 门控引起的 Ca2+ 火花。可变数量的这些 Ca2+ 火花的额外动员使心肌细胞能够表现出分级的细胞 Ca2+ 瞬变。类似的募集过程可能总体上是细胞水平上 Ca2+ 信号调节的基础。

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To quark or to spark, that is the question.是夸克还是火花,这是个问题。
J Physiol. 1997 Jul 1;502 ( Pt 1)(Pt 1):1. doi: 10.1111/j.1469-7793.1997.001bl.x.
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J Physiol. 1997 Mar 1;499 ( Pt 2)(Pt 2):307-14. doi: 10.1113/jphysiol.1997.sp021928.
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A hierarchical concept of cellular and subcellular Ca(2+)-signalling.细胞及亚细胞钙信号的分级概念。
Prog Biophys Mol Biol. 1996;65(3):265-96. doi: 10.1016/s0079-6107(96)00014-4.

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