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测量温度在脂多糖刺激后红细胞变形性的分布中起关键作用。

Measurement temperature plays a pivotal role in the distribution of erythrocyte deformability after LPS.

作者信息

Jagger J E, Ellis C G, Sibbald W J, Eichelbrönner O

机构信息

The A.C. Burton Vascular Biology Laboratory, London Health Sciences Centre, University of Western Ontario, London, Ontario, Canada N6A 5C1.

出版信息

Biorheology. 2001;38(5-6):439-48.

Abstract

Reductions in red blood cell membrane deformability (RBC(D)) may perturb microcirculatory blood flow and impair tissue O(2)-availability. We investigated the effect of assay temperature on the distribution of RBC(D) in endotoxin (LPS) incubated and control RBCs. Fresh blood from healthy rats was incubated with and without the presence of LPS for 6 hrs. An index of red blood cell membrane deformability, delta, was measured via the micropipette aspiration technique at 25 degrees C and 37 degrees C at 0, 2 and 6 hrs of incubation. The ATP content of RBC was measured by the luciferin-luciferase technique. At 25 degrees C, LPS caused a significant decrease in mean delta after 2 and 6 hours incubation compared to controls (-10.0%, p=0.03 and -24.0%, p=0.03, respectively) characterized by a left shift in the distribution (skewness: -1.4). However, at 37 degrees C a significant decrease in delta was only detected after 6 hrs of LPS incubation (-13.8%, p=0.01, compared to -5.1%, p=0.7 at 2 hours) and lacked the left shifted distribution (skewness: 0.2). No significant difference in ATP content of RBCs was observed between groups. We have shown that LPS incubation results in a significant decrease in RBC(D) and that room temperature measurement of physical membrane properties may exaggerate the differences between normal and perturbed RBCs.

摘要

红细胞膜变形性(RBC(D))降低可能会扰乱微循环血流并损害组织氧供应。我们研究了测定温度对内毒素(LPS)孵育的红细胞和对照红细胞中RBC(D)分布的影响。将健康大鼠的新鲜血液在有和没有LPS存在的情况下孵育6小时。通过微量移液器抽吸技术在孵育0、2和6小时时于25℃和37℃测量红细胞膜变形性指数δ。通过荧光素 - 荧光素酶技术测量红细胞的ATP含量。在25℃时,与对照组相比,LPS孵育2小时和6小时后平均δ显著降低(分别为-10.0%,p = 0.03和-24.0%,p = 0.03),其特征是分布向左偏移(偏度:-1.4)。然而,在37℃时,仅在LPS孵育6小时后才检测到δ显著降低(-13.8%,p = 0.01,相比之下2小时时为-5.1%,p = 0.7),并且没有向左偏移的分布(偏度:0.2)。各组之间红细胞的ATP含量未观察到显著差异。我们已经表明,LPS孵育会导致RBC(D)显著降低,并且在室温下测量物理膜特性可能会夸大正常红细胞和受干扰红细胞之间的差异。

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