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一种测量成年果蝇心肌钙处理的方法。

A method to measure myocardial calcium handling in adult Drosophila.

机构信息

Institute of Molecular Medicine, Peking University, Beijing, China.

出版信息

Circ Res. 2011 May 27;108(11):1306-15. doi: 10.1161/CIRCRESAHA.110.238105. Epub 2011 Apr 14.

Abstract

RATIONALE

Normal cardiac physiology requires highly regulated cytosolic Ca(2+) concentrations and abnormalities in Ca(2+) handling are associated with heart failure. The majority of approaches to identifying the components that regulate intracellular Ca(2+) dynamics rely on cells in culture, mouse models, and human samples. However, a genetically robust system for unbiased screens of mutations that affect Ca(2+) handling remains a challenge.

OBJECTIVE

We sought to develop a new method to measure myocardial Ca(2+) cycling in adult Drosophila and determine whether cardiomyopathic fly hearts recapitulate aspects of diseased mammalian myocardium.

METHODS AND RESULTS

Using engineered transgenic Drosophila that have cardiac-specific expression of Ca(2+)-sensing fluorescent protein, GCaMP2, we developed methods to measure parameters associated with myocardial Ca(2+) handling. The following key observations were identified: (1) Control w(1118) Drosophila hearts have readily measureable Ca(2+)-dependent fluorescent signals that are dependent on L-type Ca(2+) channels and SR Ca(2+) stores and originate from rostral and caudal pacemakers. (2) A fly mutant, held-up(2) (hdp(2)), that has a point mutation in troponin I and has a dilated cardiomyopathic phenotype demonstrates abnormalities in myocardial Ca(2+) handling that include increases in the duration of the 50% rise in intensity to peak intensity, the half-time of fluorescence decline from peak, the full duration at half-maximal intensity, and decreases in the linear slope of decay from 80% to 20% intensity decay. (3) Hearts from hdp(2) mutants had reductions in caffeine-induced Ca(2+) increases and reductions in ryanodine receptor (RyR) without changes in L-type Ca(2+) channel transcripts in comparison with w(1118).

CONCLUSIONS

Our results show that the cardiac-specific expression of GCaMP2 provides a means of characterizing propagating Ca(2+) transients in adult fly hearts. Moreover, the adult fruit fly heart recapitulates several aspects of Ca(2+) regulation observed in mammalian myocardium. A mutation in Drosophila that causes an enlarged cardiac chamber and impaired contractile function is associated with abnormalities in the cytosolic Ca(2+) transient as well as changes in transcript levels of proteins associated with Ca(2+) handling. This new methodology has the potential to permit an examination of evolutionarily conserved myocardial Ca(2+)-handing mechanisms by applying the vast resources available in the fly genomics community to conduct genetic screens to identify new genes involved in generated Ca(2+) transients and arrhythmias.

摘要

背景

正常的心脏生理学需要高度调节的细胞质 Ca(2+)浓度,而 Ca(2+)处理的异常与心力衰竭有关。大多数识别调节细胞内 Ca(2+)动力学的成分的方法都依赖于培养细胞、小鼠模型和人类样本。然而,一种用于鉴定影响 Ca(2+)处理的突变的遗传稳健的无偏筛选方法仍然是一个挑战。

目的

我们试图开发一种新的方法来测量成年果蝇的心肌 Ca(2+)循环,并确定心肌病变的果蝇心脏是否再现了患病哺乳动物心肌的某些方面。

方法和结果

使用具有心脏特异性表达 Ca(2+)敏感荧光蛋白 GCaMP2 的工程转基因果蝇,我们开发了测量与心肌 Ca(2+)处理相关的参数的方法。确定了以下关键观察结果:(1)对照 w(1118)果蝇心脏具有可测量的 Ca(2+)-依赖性荧光信号,该信号依赖于 L 型 Ca(2+)通道和 SR Ca(2+)储存库,源自头侧和尾侧起搏器。(2)一种果蝇突变体,held-up(2)(hdp(2)),其肌钙蛋白 I 中的一个点突变并具有扩张型心肌病表型,表现出心肌 Ca(2+)处理异常,包括强度增加 50%达到峰值强度的持续时间增加、荧光下降的半衰期从峰值、半强度持续时间和从 80%到 20%强度衰减的线性斜率降低。(3)与 w(1118)相比,hdp(2)突变体的心脏中的咖啡因诱导的 Ca(2+)增加减少,Ryanodine 受体(RyR)减少,而 L 型 Ca(2+)通道转录本没有变化。

结论

我们的结果表明,GCaMP2 的心脏特异性表达为表征成年果蝇心脏中的传播 Ca(2+)瞬变提供了一种手段。此外,成年果蝇心脏再现了哺乳动物心肌中观察到的几个 Ca(2+)调节方面。导致心脏腔室增大和收缩功能受损的果蝇突变与细胞质 Ca(2+)瞬变异常以及与 Ca(2+)处理相关的蛋白转录本水平变化有关。这种新方法有可能通过应用果蝇基因组学社区中可用的大量资源来进行遗传筛选,以鉴定参与产生 Ca(2+)瞬变和心律失常的新基因,从而检查进化保守的心肌 Ca(2+)处理机制。

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