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通过共聚焦激光显微镜对大鼠脑内毛细血管中红细胞速度和血流以及微血管直径进行动态体内测量。

Dynamic in vivo measurement of erythrocyte velocity and flow in capillaries and of microvessel diameter in the rat brain by confocal laser microscopy.

作者信息

Seylaz J, Charbonné R, Nanri K, Von Euw D, Borredon J, Kacem K, Méric P, Pinard E

机构信息

Laboratoire de Recherches Cérébrovasculaires, CNRS UPR 646, Université Paris 7, France.

出版信息

J Cereb Blood Flow Metab. 1999 Aug;19(8):863-70. doi: 10.1097/00004647-199908000-00005.

DOI:10.1097/00004647-199908000-00005
PMID:10458593
Abstract

A new method for studying brain microcirculation is described. Both fluorescently labeled erythrocytes and plasma were visualized on-line through a closed cranial window in anesthetized rats, using laser-scanning two-dimension confocal microscopy. Video images of capillaries, arterioles, and venules were digitized off-line to measure microvessel diameter and labeled erythrocyte flow and velocity in parenchymal capillaries up to 200 microm beneath the brain surface. The method was used to analyze the rapid adaptation of microcirculation to a brief decrease in perfusion pressure. Twenty-second periods of forebrain ischemia were induced using the tour-vessel occlusion model in eight rats. EEG, arterial blood pressure, and body temperature were continuously controlled. In all conditions, labeled erythrocyte flow and velocity were both very heterogeneous in capillaries. During ischemia, capillary perfusion was close to 0, but a low blood flow persisted in arterioles and venules, while EEG was flattening. The arteriole and venule diameter did not significantly change. At the unclamping of carotid arteries, there was an instantaneous increase (by about 150%) of arteriole diameter. Capillary erythrocyte flow and velocity increased within 5 seconds, up to, respectively, 346 +/- 229% and 233 +/- 156% of their basal value. No capillary recruitment of erythrocytes was detected. All variables returned to their basal levels within less than 100 seconds after declamping. The data are discussed in terms of a possible involvement of shear stress in the reperfusion period.

摘要

本文描述了一种研究脑微循环的新方法。使用激光扫描二维共聚焦显微镜,通过麻醉大鼠的封闭颅骨视窗对荧光标记的红细胞和血浆进行在线可视化观察。毛细血管、小动脉和小静脉的视频图像离线数字化,以测量脑表面以下达200微米的实质毛细血管中的微血管直径、标记红细胞流动和速度。该方法用于分析微循环对灌注压短暂降低的快速适应性。在8只大鼠中使用游血管闭塞模型诱导20秒的前脑缺血。持续监测脑电图、动脉血压和体温。在所有情况下,标记红细胞在毛细血管中的流动和速度都非常不均匀。缺血期间,毛细血管灌注接近0,但小动脉和小静脉中仍存在低血流量,同时脑电图变平。小动脉和小静脉直径无明显变化。在松开颈动脉时,小动脉直径瞬间增加(约150%)。毛细血管红细胞流动和速度在5秒内增加,分别达到其基础值的346±229%和233±156%。未检测到红细胞的毛细血管募集。松开后不到100秒内,所有变量均恢复到基础水平。根据再灌注期剪切应力可能的参与情况对数据进行了讨论。

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