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Elimination of autofluorescence in fluorescence Correlation spectroscopy by using the AzaDiOxaTriAngulenium (ADOTA) fluorophore in combination with time correlated single photon counting (TCSPC)

机译:结合使用AzaDiOxaTriAngulenium(ADOTA)荧光团和与时间相关的单光子计数(TCSPC)消除荧光相关光谱中的自发荧光

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摘要

Fluorescence Correlation Spectroscopy (FCS) is a frequently applied technique that allows for precise and sensitive analyses of molecular diffusion and interactions. However, the potential of FCS for in vitro or ex vivo studies has not been fully realized due in part to artifacts originating from autofluorescence (fluorescence of inherent components and fixative-induced fluorescence). Here, we propose the azadioxatriangulenium (ADOTA) dye as a solution to this problem. The lifetime of the ADOTA probe, about 19.4 ns, is much longer than most components of autofluorescence. Thus, it can be easily separated by time correlated single photon counting (TCSPC) methods. Here, we demonstrate the suppression of autofluorescence in FCS by using ADOTA labeled Hyaluronan macromolecules (HAs) with Rhodamine 123 added to simulate diffusing fluorescent background components. The emission spectrum and decay rate of Rhodamine 123 overlap with the usual sources of autofluorescence, and its diffusion behavior is well known. We show that the contributions from Rhodamine 123 can be eliminated by time-gating or by fluorescence lifetime correlation spectroscopy (FLCS). While the pairing of ADOTA and time-gating is an effective strategy for the removal of autofluorescence from fluorescence imaging, the loss of photons leads to erroneous concentration values with FCS. On the other hand, FLCS eliminates autofluorescence without such errors. We then show that both time gating and FLCS may be used successfully with ADOTA-labeled HA to detect the presence of hyaluronidase, the over-expression of which has been observed in many types of cancer.
机译:荧光相关光谱法(FCS)是一种常用的技术,可以对分子扩散和相互作用进行精确而敏感的分析。但是,FCS用于体外或离体研究的潜力尚未完全实现,部分原因是由于自身荧光(固有成分的荧光和固定剂诱导的荧光)引起的伪影。在这里,我们提出了azadioxatriangulenium(ADOTA)染料作为解决此问题的方法。 ADOTA探针的寿命约为19.4 ns,比大多数自发荧光成分更长。因此,可以通过时间相关单光子计数(TCSPC)方法轻松地将其分离。在这里,我们证明了通过使用ADOTA标记的透明质酸大分子(HAs)和添加的罗丹明123以模拟扩散荧光背景成分,可以抑制FCS中的自发荧光。罗丹明123的发射光谱和衰减速率与自发荧光的常见来源重叠,并且其扩散行为是众所周知的。我们表明,可以通过时间门控或荧光寿命相关光谱法(FLCS)消除罗丹明123的贡献。虽然ADOTA和时间门控的配对是从荧光成像中去除自发荧光的有效策略,但光子的损失会导致FCS的浓度值错误。另一方面,FLCS可消除自发荧光,而不会产生此类错误。然后,我们显示时间选通和FLCS均可与ADOTA标记的HA成功地用于检测透明质酸酶的存在,透明质酸酶的过表达已在许多类型的癌症中观察到。

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