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自动发光基因编码比率型指示剂,用于单细胞水平的实时 Ca2+成像。

Auto-luminescent genetically-encoded ratiometric indicator for real-time Ca2+ imaging at the single cell level.

机构信息

Research Institute for Electronic Science, Hokkaido University, Kita-20, Nishi-10 Kita-ku, Sapporo, Hokkaido, Japan.

出版信息

PLoS One. 2010 Apr 1;5(4):e9935. doi: 10.1371/journal.pone.0009935.

Abstract

BACKGROUND

Efficient bioluminescence resonance energy transfer (BRET) from a bioluminescent protein to a fluorescent protein with high fluorescent quantum yield has been utilized to enhance luminescence intensity, allowing single-cell imaging in near real time without external light illumination.

METHODOLOGY/PRINCIPAL FINDINGS: We applied BRET to develop an autoluminescent Ca(2+) indicator, BRAC, which is composed of Ca(2+)-binding protein, calmodulin, and its target peptide, M13, sandwiched between a yellow fluorescent protein variant, Venus, and an enhanced Renilla luciferase, RLuc8. Adjusting the relative dipole orientation of the luminescent protein's chromophores improved the dynamic range of BRET signal change in BRAC up to 60%, which is the largest dynamic range among BRET-based indicators reported so far. Using BRAC, we demonstrated successful visualization of Ca(2+) dynamics at the single-cell level with temporal resolution at 1 Hz. Moreover, BRAC signals were acquired by ratiometric imaging capable of canceling out Ca(2+)-independent signal drifts due to change in cell shape, focus shift, etc.

CONCLUSIONS/SIGNIFICANCE: The brightness and large dynamic range of BRAC should facilitate high-sensitive Ca(2+) imaging not only in single live cells but also in small living subjects.

摘要

背景

高效的生物发光共振能量转移(BRET)可将生物发光蛋白中的能量转移到具有高荧光量子产率的荧光蛋白上,从而增强发光强度,实现在近实时条件下无需外部光照即可对单细胞进行成像。

方法/主要发现:我们应用 BRET 开发了一种自发光 Ca2+指示剂 BRAC,它由 Ca2+结合蛋白钙调蛋白及其靶肽 M13 夹在黄色荧光蛋白变体 Venus 和增强型海肾荧光素酶 RLuc8 之间组成。调整发光蛋白发色团的相对偶极取向可将 BRAC 中 BRET 信号变化的动态范围提高至 60%,这是迄今为止报道的基于 BRET 的指示剂中最大的动态范围。使用 BRAC,我们成功地以 1 Hz 的时间分辨率在单细胞水平上可视化 Ca2+动力学。此外,BRAC 信号可以通过比率成像获得,这种成像方式能够消除由于细胞形状变化、焦点偏移等引起的 Ca2+非依赖性信号漂移。

结论/意义:BRAC 的亮度和大动态范围应有助于实现高灵敏度的 Ca2+成像,不仅可以在单个活细胞中进行,也可以在小型活体中进行。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/29d2/2848576/391cdc428396/pone.0009935.g001.jpg

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