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将对数通道数转换为相对线性荧光强度。

Conversion of logarithmic channel numbers into relative linear fluorescence intensity.

作者信息

Schmid I, Schmid P, Giorgi J V

机构信息

Department of Microbiology, UCLA School of Medicine 90024.

出版信息

Cytometry. 1988 Nov;9(6):533-8. doi: 10.1002/cyto.990090605.

Abstract

We describe a simple, reproducible, and generally applicable method to assess the performance of log amplifiers by using a fluorescent sample that provides multiple peaks of different intensities. The channel differences between multiple peaks are used to evaluate the logarithmic behavior of the fluorescence signal amplifier on the flow cytometer. A calibration curve can be created to correct the channel numbers for deviations from true logarithmic behavior and then convert data into relative linear intensities. By using these linear fluorescent intensities, we compared the capacity of different antisera against HIV-1 (human immunodeficiency virus type 1) peptides to inhibit the binding of HIV-1 to CEM, a CD4-positive T-cell line. A wide range of applications for this calibration procedure can be envisioned and the method is valuable for monitoring instrument performance over time.

摘要

我们描述了一种简单、可重复且普遍适用的方法,通过使用提供多个不同强度峰值的荧光样本评估对数放大器的性能。多个峰值之间的通道差异用于评估流式细胞仪上荧光信号放大器的对数行为。可以创建校准曲线,以校正通道数与真实对数行为的偏差,然后将数据转换为相对线性强度。通过使用这些线性荧光强度,我们比较了不同抗HIV-1(人类免疫缺陷病毒1型)肽的抗血清抑制HIV-1与CD4阳性T细胞系CEM结合的能力。可以设想这种校准程序有广泛的应用,并且该方法对于长期监测仪器性能很有价值。

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