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Evaluating and improving the photostability of fluorescent proteins

机译:评估和改善荧光蛋白的光稳定性

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摘要

Fluorescent proteins are the most common and versatile class of genetically encoded optical probes. While structure-guided rational design and directed evolution approaches have largely overcome early problems such as oligomerization, poor folding at physiological temperatures, and availability of wavelengths suitable for multi-color imaging, nearly all fluorescent proteins have yet to be fully optimized. We have developed novel methods for evaluating the current generation of fluorescent proteins and improving their remaining suboptimal properties. Little is yet known about the mechanisms responsible for photobleaching of fluorescent proteins, and inadequate photostability is a chief complaint among end users. In order to compare the performance of fluorescent proteins across the visual spectrum, we have standardized a method used to measure photostability in live cells under both widefield and confocal laser illumination. This method has allowed us to evaluate a large number of commonly used fluorescent proteins, and has uncovered surprisingly complex and unpredictable behaviors in many of these proteins. We have also developed novel methods for selecting explicitly for high photostability during the directed evolution process, leading to the development of highly improved monomeric orange and red fluorescent proteins. These proteins, most notably our photostable derivative of TagRFP, have remarkably high photostability and have proven useful as fusion tags for long-term imaging. Our methods should be applicable to any of the large number of fluorescent proteins still in need of improved photostability.
机译:荧光蛋白是遗传编码光学探针中最常见和用途最广泛的一类。尽管结构指导的合理设计和定向进化方法已在很大程度上克服了早期问题,例如低聚,在生理温度下折叠不佳以及适用于多色成像的波长的可用性,但几乎所有荧光蛋白都尚未完全优化。我们已经开发出新颖的方法来评估当前一代的荧光蛋白并改善其剩余的次优特性。引起荧光蛋白光漂白的机理还知之甚少,光稳定性不足是最终用户的主要抱怨。为了在整个光谱范围内比较荧光蛋白的性能,我们已经标准化了一种用于在宽视野和共聚焦激光照射下测量活细胞光稳定性的方法。这种方法使我们能够评估大量常用的荧光蛋白,并且在许多这些蛋白中发现了令人惊讶的复杂且不可预测的行为。我们还开发了新颖的方法,可在定向进化过程中明确选择高光稳定性,从而开发出高度改进的橙色和红色荧光单体单体。这些蛋白质,尤其是我们TagRFP的光稳定衍生物,具有极高的光稳定性,并已证明可用作长期成像的融合标签。我们的方法应适用于仍然需要提高光稳定性的大量荧光蛋白中的任何一种。

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