找到底部并使用它:用双光子显微镜检测体内低强度值的偏移量和灵敏度。

IntraVital Pub Date : 2014-03-01 DOI:10.4161/intv.23674
Ruben M Sandoval, Exing Wang, Bruce A Molitoris
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引用次数: 17

摘要

最大化2光子参数用于获取定量活体显微镜图像,特别是当需要高灵敏度时,仍然是一个开放的研究领域。在这里,我们提出的数据正确设置的黑电平的光电倍增管放大器通过调整偏移,以允许低强度过程的准确定量。当黑色电平设置过高时,一些低强度像素值变为零,并且灵敏度发生非线性退化,从而使原本可量化的低强度值几乎无法检测到。在体外使用一系列增加的荧光白蛋白浓度偏移量的初步研究显示,在较低的白蛋白浓度下,对较高偏移量的敏感性丧失。在体内,在较高的偏移量下,敏感性也出现了类似的下降,因此正确测定白蛋白肾小球渗透系数的能力也出现了下降。当需要高灵敏度时,找到产生准确和线性数据的偏移量对于定量分析至关重要。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Finding the bottom and using it: Offsets and sensitivity in the detection of low intensity values in vivo with 2-photon microscopy.

Maximizing 2-photon parameters used in acquiring images for quantitative intravital microscopy, especially when high sensitivity is required, remains an open area of investigation. Here we present data on correctly setting the black level of the photomultiplier tube amplifier by adjusting the offset to allow for accurate quantitation of low intensity processes. When the black level is set too high some low intensity pixel values become zero and a nonlinear degradation in sensitivity occurs rendering otherwise quantifiable low intensity values virtually undetectable. Initial studies using a series of increasing offsets for a sequence of concentrations of fluorescent albumin in vitro revealed a loss of sensitivity for higher offsets at lower albumin concentrations. A similar decrease in sensitivity, and therefore the ability to correctly determine the glomerular permeability coefficient of albumin, occurred in vivo at higher offset. Finding the offset that yields accurate and linear data are essential for quantitative analysis when high sensitivity is required.

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