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脱氧血红蛋白S溶解度的细胞内直接测量。

Direct intracellular measurement of deoxygenated hemoglobin S solubility.

作者信息

Fabry M E, Desrosiers L, Suzuka S M

机构信息

Department of Medicine, Division of Hematology, Albert Einstein College of Medicine, 1300 Morris Park Ave., Bronx, NY 10461, USA.

出版信息

Blood. 2001 Aug 1;98(3):883-4. doi: 10.1182/blood.v98.3.883.

Abstract

The solubility of deoxygenated hemoglobin S (HbS), which is the concentration of fully deoxygenated HbS in equilibrium with polymer (C(SAT)), is a factor that determines in vivo polymer formation. However, measurement of C(SAT) is usually performed under conditions that are far from physiological. In solution studies of HbS by Benesch et al, it was demonstrated that p50, the point at which hemoglobin is half-saturated with oxygen, is proportional to the amount of polymer formed and that it may be used to measure C(SAT). This method has been extended to measure C(SAT) in intact red cells by varying extracellular osmolarity, which, in turn, varies intracellular hemoglobin concentration. This method measures intracellular C(SAT) under physiological conditions with intact red cell contents and can be applied to human and transgenic mouse red cells. The principle is demonstrated by measuring p50 as a function of extracellular osmolarity for AA, SS, and AS red cells. (Blood. 2001;98:883-884)

摘要

脱氧血红蛋白S(HbS)的溶解度,即与聚合物处于平衡状态的完全脱氧HbS的浓度(C(SAT)),是决定体内聚合物形成的一个因素。然而,C(SAT)的测量通常是在远离生理条件的情况下进行的。在贝内施等人对HbS的溶液研究中,已证明p50(血红蛋白氧饱和度为一半时的点)与形成的聚合物量成正比,并且它可用于测量C(SAT)。通过改变细胞外渗透压(进而改变细胞内血红蛋白浓度),该方法已扩展到测量完整红细胞中的C(SAT)。此方法在生理条件下测量完整红细胞内容物中的细胞内C(SAT),并且可应用于人类和转基因小鼠红细胞。通过测量AA、SS和AS红细胞的p50作为细胞外渗透压的函数来证明该原理。(《血液》。2001年;98:883 - 884)

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