人类红细胞中的32P标记异常。细胞内的无机磷酸盐是否存在不止一个池？

32P-labelling anomalies in human erythrocytes. Is there more than one pool of cellular Pi?

作者信息

Kemp G J, Bevington A, Khodja D, Challa A, Russell R G

机构信息

Department of Human Metabolism and Clinical Biochemistry, University of Sheffield Medical School, U.K.

出版信息

Biochem J. 1989 Dec 15;264(3):729-36. doi: 10.1042/bj2640729.

DOI:10.1042/bj2640729

PMID:2695064

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1133646/

Abstract

Human erythrocytes were incubated in autologous plasma containing [32P]Pi, and sampled by a method which avoids washing the cells. 2. In experiments of up to 3 h duration, the specific radioactivity of cellular Pi stabilized at a value below that of extracellular Pi. This can be explained on the basis of a single cellular Pi pool exchanging with a large unlabelled pool of cellular organic phosphates. 3. However, a rapid initial phase of labelling, occurring within 30 s, was inconsistent with the situation described in point 2. A possible explanation is that about 1/4 of cellular Pi occurs in a separate, fast-labelling pool. 4. When the extracellular Pi concentration was doubled, most of the corresponding increase in the steady-state cellular Pi concentration was accounted for by the apparent fast-labelling Pi pool, which also doubled. 5. The observed initial rate of labelling of cellular organic phosphates [which probably occurs through the reaction catalysed by glyceraldehyde-3-phosphate dehydrogenase (E.C. 1.2.1.12)] was considerably lower than that predicted from the flux through the Embden-Meyerhof pathway. This implies that the enzyme is exposed to Pi whose specific radioactivity is lower than the mean specific radioactivity of cellular Pi, and fails to support earlier suggestions that this enzyme uses extracellular Pi. 6. In 3 h incubations, the rate of organic phosphate labelling was roughly constant throughout, even though the specific radioactivity of cellular Pi had risen slowly to a plateau. Viewed in conjunction with point 5, this again suggests some inhomogeneity in cellular Pi. 7. Cellular Pi and extracellular Pi only reached isotopic steady state after 2 days. At this stage some organic phosphates were probably still incompletely labelled. 8. We conclude that, whatever their physical or technical reasons, such labelling inhomogeneities and slow attainment of isotopic steady state may cause serious misinterpretation of results if ignored during 32P-labelling of intact cells.

摘要

将人类红细胞置于含有[32P]磷酸（Pi）的自体血浆中孵育，并采用避免洗涤细胞的方法进行取样。2. 在长达3小时的实验中，细胞内Pi的比放射性稳定在低于细胞外Pi的水平。这可以基于单个细胞内Pi池与大量未标记的细胞有机磷酸盐池进行交换来解释。3. 然而，在30秒内出现的快速初始标记阶段与第2点所述情况不一致。一种可能的解释是，约1/4的细胞内Pi存在于一个单独的快速标记池中。4. 当细胞外Pi浓度加倍时，稳态细胞内Pi浓度相应增加的大部分是由明显的快速标记Pi池引起的，该池也加倍了。5. 观察到的细胞有机磷酸盐的初始标记速率[可能通过甘油醛-3-磷酸脱氢酶（E.C. 1.2.1.12）催化的反应发生]远低于根据通过糖酵解途径的通量预测的速率。这意味着该酶接触到的Pi的比放射性低于细胞内Pi的平均比放射性，并且不支持早期关于该酶使用细胞外Pi的观点。6. 在3小时的孵育中，有机磷酸盐的标记速率在整个过程中大致保持恒定，尽管细胞内Pi的比放射性已缓慢上升至平稳状态。结合第5点来看，这再次表明细胞内Pi存在一些不均匀性。7. 细胞内Pi和细胞外Pi仅在2天后达到同位素稳态。在这个阶段，一些有机磷酸盐可能仍未完全标记。8. 我们得出结论，无论其物理或技术原因如何，如果在完整细胞的32P标记过程中忽略这些标记不均匀性和同位素稳态的缓慢达到，可能会导致对结果的严重误解。