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首页> 外文期刊>Scientific reports. >A Novel Ultra-Stable, Monomeric Green Fluorescent Protein For Direct Volumetric Imaging of Whole Organs Using CLARITY
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A Novel Ultra-Stable, Monomeric Green Fluorescent Protein For Direct Volumetric Imaging of Whole Organs Using CLARITY

机译:一种新型超稳定的单体绿色荧光蛋白,用于使用清晰度直接成像整体器官

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摘要

Recent advances in thick tissue clearing are enabling high resolution, volumetric fluorescence imaging of complex cellular networks. Fluorescent proteins (FPs) such as GFP, however, can be inactivated by the denaturing chemicals used to remove lipids in some tissue clearing methods. Here, we solved the crystal structure of a recently engineered ultra-stable GFP (usGFP) and propose that the two stabilising mutations, Q69L and N164Y, act to improve hydrophobic packing in the core of the protein and facilitate hydrogen bonding networks at the surface, respectively. usGFP was found to dimerise strongly, which is not desirable for some applications. A point mutation at the dimer interface, F223D, generated monomeric usGFP (muGFP). Neurons in whole mouse brains were virally transduced with either EGFP or muGFP and subjected to Clear Lipid-exchanged Acrylamide-hybridized Rigid Imaging/Immunostaining/In situ hybridization-compatible Tissue-hYdrogel (CLARITY) clearing. muGFP fluorescence was retained after CLARITY whereas EGFP fluorescence was highly attenuated, thus demonstrating muGFP is a novel FP suitable for applications where high fluorescence stability and minimal self-association are required.
机译:厚组织清除的最近进展是使复数的高分辨率,复合蜂窝网络的体积荧光成像。然而,例如GFP如GFP的荧光蛋白(FPS)可以通过用于除去一些组织清除方法中的脂质的变性化学物质来灭活。在这里,我们解决了最近工程的超稳定GFP(USGFP)的晶体结构,并提出了两个稳定突变,Q69L和N164Y,以改善蛋白质核心的疏水包装,并促进表面氢键网络,分别。 USGFP被发现强烈二次,这对于某些应用来说是不可取的。二聚体界面的点突变,F223D,生成的单体USGFP(MUGFP)。整个小鼠大脑中的神经元与EGFP或MuGFP进行病变转导,并进行清晰的脂质交换的丙烯酰胺杂交的刚性成像/免疫染色/原位杂交相容的组织 - 水凝胶(透明度)清除。在透明度之后保留MuGFP荧光,而EGFP荧光高度衰减,因此证明Mugfp是适用于需要高荧光稳定性和最小自关联的应用的新型FP。

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