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红细胞冷藏期间镁结合变化的进一步研究。

Further studies on alterations in magnesium binding during cold storage of erythrocytes.

作者信息

Bock J L, Yusuf Y

机构信息

Department of Pathology, New York Medical College, Valhalla.

出版信息

Biochim Biophys Acta. 1988 Jun 22;941(2):225-31. doi: 10.1016/0005-2736(88)90183-6.

Abstract

Free intracellular Mg2+ concentration ([Mg2+]i) was measured in cold-stored human erythrocytes by the method of null-point titration with ionophore A23187. [Mg2+]i was 311 +/- 41 microM (mean +/- S.D.) for cells stored 0-10 days, increasing to 458 +/- 64 microM for cells stored 22-48 days. The values for stored cells were higher than those previously determined by a 31P-NMR method (Bock et al. (1985) Blood 65, 1526-1530); however, the null-point method requires extensive washing of the cells, which we have found to increase NMR-measured [Mg2+]i. The null-point values still represent a small fraction of total cell Mg2+, and confirm that binding of Mg2+ to ligands other than ATP and 2,3-bisphosphoglycerate must increase during storage. As an initial test of whether this may imply suboptimal availability of Mg2+ for cell preservation, we used A23187 to prepare erythrocytes with altered Mg2+ content, then removed ionophore and stored the cells in plasma-free medium for up to 2 weeks. Higher Mg2+ content had a very significant positive correlation (P less than 0.0001) with higher cell ATP concentrations. Storage did not significantly affect basal or Na+-stimulated efflux of Mg2+ from Mg2+-loaded red cells.

摘要

采用离子载体A23187零位点滴定法测定了冷藏人红细胞内游离镁离子浓度([Mg2+]i)。储存0 - 10天的细胞[Mg2+]i为311±41微摩尔/升(平均值±标准差),储存22 - 48天的细胞该值增至458±64微摩尔/升。储存细胞的值高于先前用31P - NMR方法测定的值(博克等人(1985年),《血液》65卷,1526 - 1530页);然而,零位点法需要对细胞进行大量洗涤,我们发现这会增加NMR测定的[Mg2+]i。零位点值仍仅占细胞总镁的一小部分,并证实储存期间镁与ATP和2,3 - 二磷酸甘油酸以外配体的结合必定增加。作为对这是否可能意味着镁对细胞保存的可用性欠佳的初步测试,我们用A23187制备了镁含量改变的红细胞,然后去除离子载体并将细胞在无血浆培养基中储存长达2周。较高的镁含量与较高的细胞ATP浓度呈非常显著的正相关(P<0.0001)。储存对镁负载红细胞中镁的基础或钠刺激外流没有显著影响。

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