使用亲脂性钙敏感荧光染料钙绿C18对原代成骨细胞跨质膜的钙转运进行表征。

Characterization of calcium translocation across the plasma membrane of primary osteoblasts using a lipophilic calcium-sensitive fluorescent dye, calcium green C18.

作者信息

Lloyd Q P, Kuhn M A, Gay C V

机构信息

Department of Biochemistry and Molecular Biology, Pennsylvania State University, University Park 16802, USA.

出版信息

J Biol Chem. 1995 Sep 22;270(38):22445-51. doi: 10.1074/jbc.270.38.22445.

DOI:10.1074/jbc.270.38.22445

PMID:7673232

Abstract

The synthesis of Calcium Green C18, a lipophilic fluorescent calcium-sensitive dye, and its use as a monitor of Ca2+ efflux from cells is described. This indicator consists of a Calcium Green-1 molecule conjugated to a lipophilic 18-carbon alkyl chain which will intercalate into cell membranes. The Kd of the indicator for Ca2+ in aqueous solution (pH 7.2, 22 degrees C, ionic strength 0.1 M) is 0.23 +/- 0.04 microM and in the presence of liposomes is 0.062 +/- 0.007 microM. Due to its high negativity, the calcium chelating fluorophore faces the cell exterior, when loaded under a defined set of conditions. The dye was found largely on the surface of the cells when loaded at a concentration of 5 microM for 10 min at 37 degrees C. Five minutes after introduction of EGTA, 83-95% fluorescence disappeared, indicating that most of the fluorophore was on the cell surface. Photobleaching was minimal (3-13%). A confocal laser scanning microscope was used to detect and quantify fluorescence. Internalized dye was apparent in cells loaded for longer times (30-60 min) and in membrane-impaired cells, as shown by uptake of propidium iodide. Under defined confocal laser scanning microscope settings, a transient fluorescence at the periphery of approximately 30% of the cells was observed following 10(-8) M parathyroid hormone treatment, indicating the presence of outwardly directed calcium transport across the plasma membrane. Calcium efflux usually lasted 7-10 min, peaking at around 2-3 min. Changes in cell shape were also observed. Calcium efflux was shown to be sensitive to (a) 10 microM quercetin and 10 microM vanadate, partially specific inhibitors of plasma membrane Ca(2+)-ATPase, to (b) 0.1 mM trifluoperazine, an agent which renders calmodulin ineffective, and to (c) 10 mM neomycin sulfate, which blocks release of Ca2+ from intracellular stores. Thapsigargin (5 microM), an inhibitor of Ca(2+)-ATPase of the endoplasmic reticulum, prolonged fluorescence. These observations indicate that cell surface fluorescence was due to the capture of Ca2+ by Calcium Green C18 after Ca2+ had been translocated across osteoblast plasma membranes. Involvement of the plasma membrane Ca(2+)-ATPase, known to be present in osteoblasts in substantial amounts, is implicated.

摘要

描述了亲脂性荧光钙敏染料钙绿C18的合成及其作为细胞钙外流监测剂的用途。该指示剂由与亲脂性18碳烷基链缀合的钙绿-1分子组成，该烷基链可插入细胞膜。该指示剂在水溶液（pH 7.2、22℃、离子强度0.1M）中对Ca2+的解离常数（Kd）为0.23±0.04μM，在脂质体存在下为0.062±0.007μM。由于其高度负电性，在特定条件下加载时，钙螯合荧光团面向细胞外部。当在37℃以5μM的浓度加载10分钟时，发现该染料主要存在于细胞表面。引入乙二醇双四乙酸（EGTA）五分钟后，83 - 95%的荧光消失，表明大部分荧光团在细胞表面。光漂白最小（3 - 13%）。使用共聚焦激光扫描显微镜检测和定量荧光。如碘化丙啶摄取所示，在加载时间较长（30 - 60分钟）的细胞和膜受损的细胞中可明显看到内化的染料。在特定的共聚焦激光扫描显微镜设置下，用10^(-8)M甲状旁腺激素处理后，在约30%的细胞周边观察到短暂荧光，表明存在跨质膜的外向钙转运。钙外流通常持续7 - 10分钟，在约2 - 3分钟时达到峰值。还观察到细胞形状的变化。已表明钙外流对（a）10μM槲皮素和10μM钒酸盐（质膜Ca(2+)-ATP酶的部分特异性抑制剂）、（b）0.1mM三氟拉嗪（一种使钙调蛋白失活的试剂）和（c）10mM硫酸新霉素（其阻断细胞内钙库中Ca2+的释放）敏感。毒胡萝卜素（5μM）（内质网Ca(2+)-ATP酶的抑制剂）延长了荧光。这些观察结果表明，细胞表面荧光是由于Ca2+穿过成骨细胞质膜后被钙绿C18捕获Ca2+所致。这暗示了大量存在于成骨细胞中的质膜Ca(²⁺)-ATP酶的参与。