用可见光光谱光学相干断层扫描定量测定全血血红蛋白浓度(会议报告)

C. Veenstra, S. Kruitwagen, Dafne Groener, Wilma Petersen, W. Steenbergen, Nienke Bosschaart
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引用次数: 0

摘要

血液中血红蛋白浓度(tHb)的降低(贫血)与器官供氧受损有关,这可能导致器官损伤和心力衰竭。目前,tHb分析需要侵入性方法(例如手指戳),这既耗时又会给患者带来不适。利用光谱学,可以通过量化血液中的光吸收来估计tHb。然而,目前用于tHb定量的非侵入性光学技术的准确性受到皮肤背景衰减和总光学探测体积中未知的血容量分数的限制。光谱光学相干断层扫描(sOCT)允许在有限的测量体积内对光学衰减进行定量测量,有可能实现对单个血管内血红蛋白浓度的非侵入性估计。尽管多项研究表明,sOCT能够定量局部氧饱和度,但尚未有关于生理相关浓度的tHb定量的报道。利用自制的可见光sOCT系统,我们量化了可见光波长范围(450-600nm)的光衰减。零延迟采集和焦点跟踪的实现优化了系统灵敏度,并确保测量的衰减仅受样品本身衰减的影响。我们在健康志愿者的人全血(tHb在12-18 g/dL)上验证了我们的方法。通过PBS稀释或血浆去除,红细胞压积变化到覆盖整个病理生理范围(tHb在9-21 g/dL)。我们的系统在整个病理生理范围内定量全血中tHb,准确度为10%。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Quantificiation of hemoglobin concentrations in whole blood by visible-light spectroscopic optical coherence tomography (Conference Presentation)
A decreased hemoglobin concentration (tHb) in blood (anemia) is associated with impaired oxygen delivery to organs, which can result in organ damage and heart failure. Currently, tHb analysis requires invasive methods (e.g. a fingerstick), which are time consuming and cause discomfort to the patient. Using optical spectroscopy, the tHb can be estimated by quantifying light absorption in blood. However, the accuracy of current noninvasive optical techniques for tHb quantification is limited by the background attenuation of skin and the unknown blood volume fraction in the total optical probing volume. Spectroscopic optical coherence tomography (sOCT) allows for quantitative measurements of the optical attenuation in a confined measurement volume, potentially enabling non-invasive estimation of the hemoglobin concentration within individual blood vessels. Although multiple studies have shown that sOCT is capable of quantifying localized oxygen saturation, quantification of the tHb has not yet been reported for physiologically relevant concentrations. With a home-built visible-light sOCT system we quantified optical attenuation in the visible wavelength range (450–600nm). Implementation of both zero-delay acquisition and focus tracking optimized system sensitivity and ensured that the measured attenuation is only affected by the attenuation of the sample itself. We validated our method ex-vivo on human whole blood from healthy volunteers (tHb within 12-18 g/dL). The hematocrit was varied to cover the entire pathophysiological range (tHb within 9-21 g/dL) by either dilution with PBS, or plasma removal. Our system quantified the tHb in whole blood throughout the entire pathophysiological range with an accuracy of 10%.
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