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通过微光解和共聚焦成像在单个红细胞血影中测定钙泵动力学。

Calcium pump kinetics determined in single erythrocyte ghosts by microphotolysis and confocal imaging.

作者信息

Kubitscheck U, Pratsch L, Passow H, Peters R

机构信息

Institute of Medical Physics and Biophysics, Westfälische Wilhelms University, Münster, Germany.

出版信息

Biophys J. 1995 Jul;69(1):30-41. doi: 10.1016/S0006-3495(95)79875-7.

Abstract

The activity of the plasma membrane calcium pump was measured in single cells. Human red blood cell ghosts were loaded with a fluorescent calcium indicator and either caged calcium and ATP (protocol A) or caged ATP and calcium (protocol B). In a suitably modified laser scanning microscope either calcium or ATP were released by a short UV light pulse. The time-dependent fluorescence intensity of the calcium indicator was then followed in single ghosts by repetitive confocal imaging. The fluorescence intensity was converted into calcium concentration, which in turn was used to derive the kinetic parameters of the calcium pump, the Michaelis-Menten constant Km, and the maximal transport rate vmax. Km and vmax values derived in this manner were 24 +/- 14 microM and 1.0 +/- 0.6 microM/(ghost s) for protocol A, and 4 +/- 3 microM and 1.0 +/- 0.6 microM/(ghost s) for protocol B, respectively. The difference between A and B is presumably caused by calmodulin, which is inactive in the experiments with protocol A. The possibilities to extend the new method to living nucleus-containing cells transiently transfected with mutants of the plasma membrane calcium pump are discussed.

摘要

在单细胞中测量了质膜钙泵的活性。用人红细胞血影装载荧光钙指示剂以及笼锁钙和ATP(方案A)或笼锁ATP和钙(方案B)。在经过适当改装的激光扫描显微镜中,通过短紫外光脉冲释放钙或ATP。然后通过重复共聚焦成像跟踪单个血影中钙指示剂随时间变化的荧光强度。将荧光强度转换为钙浓度,进而用于推导钙泵的动力学参数、米氏常数Km和最大转运速率vmax。以这种方式得出的方案A的Km和vmax值分别为24±14微摩尔和1.0±0.6微摩尔/(血影·秒),方案B的分别为4±3微摩尔和1.0±0.6微摩尔/(血影·秒)。A和B之间的差异可能是由钙调蛋白引起的,钙调蛋白在方案A的实验中无活性。讨论了将该新方法扩展到用质膜钙泵突变体瞬时转染的含活细胞核细胞的可能性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/977a/1236222/c0f6655bdbfd/biophysj00059-0034-a.jpg

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