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在表达KillerRed的斑马鱼转基因动物中进行光遗传学体内细胞操作。

Optogenetic in vivo cell manipulation in KillerRed-expressing zebrafish transgenics.

作者信息

Teh Cathleen, Chudakov Dmitry M, Poon Kar-Lai, Mamedov Ilgar Z, Sek Jun-Yan, Shidlovsky Konstantin, Lukyanov Sergey, Korzh Vladimir

机构信息

Institute of Molecular and Cell Biology, A-STAR, Singapore.

出版信息

BMC Dev Biol. 2010 Nov 2;10:110. doi: 10.1186/1471-213X-10-110.

Abstract

BACKGROUND

KillerRed (KR) is a novel photosensitizer that efficiently generates reactive oxygen species (ROS) in KR-expressing cells upon intense green or white light illumination in vitro, resulting in damage to their plasma membrane and cell death.

RESULTS

We report an in vivo modification of this technique using a fluorescent microscope and membrane-tagged KR (mem-KR)-expressing transgenic zebrafish. We generated several stable zebrafish Tol2 transposon-mediated enhancer-trap (ET) transgenic lines expressing mem-KR (SqKR series), and mapped the transposon insertion sites. As mem-KR accumulates on the cell membrane and/or Golgi, it highlights cell bodies and extensions, and reveals details of cellular morphology. The photodynamic property of KR made it possible to damage cells expressing this protein in a dose-dependent manner. As a proof-of-principle, two zebrafish transgenic lines were used to affect cell viability and function: SqKR2 expresses mem-KR in the hindbrain rhombomeres 3 and 5, and elsewhere; SqKR15 expresses mem-KR in the heart and elsewhere. Photobleaching of KR by intense light in the heart of SqKR15 embryos at lower levels caused a reduction in pumping efficiency of the heart and pericardial edema and at higher levels - in cell death in the hindbrain of SqKR2 and in the heart of SqKR15 embryos.

CONCLUSIONS

An intense illumination of tissues expressing mem-KR affects cell viability and function in living zebrafish embryos. Hence, the zebrafish transgenics expressing mem-KR in a tissue-specific manner are useful tools for studying the biological effects of ROS.

摘要

背景

KillerRed(KR)是一种新型光敏剂,在体外对表达KR的细胞进行强绿光或白光照射时,能有效产生活性氧(ROS),导致其质膜受损并引起细胞死亡。

结果

我们报道了一种利用荧光显微镜和表达膜标记KR(mem-KR)的转基因斑马鱼对该技术进行的体内改良。我们构建了几个稳定的斑马鱼Tol2转座子介导的增强子捕获(ET)转基因品系,这些品系表达mem-KR(SqKR系列),并绘制了转座子插入位点图谱。由于mem-KR积聚在细胞膜和/或高尔基体上,它突出了细胞体和细胞延伸部分,并揭示了细胞形态的细节。KR的光动力特性使得以剂量依赖的方式损伤表达该蛋白的细胞成为可能。作为原理验证,使用了两个斑马鱼转基因品系来影响细胞活力和功能:SqKR2在菱脑节3和5以及其他部位表达mem-KR;SqKR15在心脏和其他部位表达mem-KR。在较低强度下,强光对SqKR15胚胎心脏中的KR进行光漂白会导致心脏泵血效率降低和心包水肿,而在较高强度下,则会导致SqKR2胚胎菱脑和SqKR15胚胎心脏中的细胞死亡。

结论

对表达mem-KR的组织进行强光照射会影响活斑马鱼胚胎中的细胞活力和功能。因此,以组织特异性方式表达mem-KR的斑马鱼转基因是研究ROS生物学效应的有用工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/003c/2989954/60949e4ba20b/1471-213X-10-110-1.jpg

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