QUANTITATION OF CYTOSOLIC [CA2+] IN WHOLE PERFUSED RAT HEARTS USING INDO-1 FLUOROMETRY .1.

被引：69

作者：

BRANDES, R

FIGUEREDO, VM

CAMACHO, SA

BAKER, AJ

WEINER, MW

机构：

[1] UNIV CALIF SAN FRANCISCO, SAN FRANCISCO GEN HOSP, CARDIOVASC RES INST, SAN FRANCISCO, CA 94110 USA

[2] UNIV CALIF SAN FRANCISCO, SAN FRANCISCO GEN HOSP, DEPT MED CARDIOL, SAN FRANCISCO, CA 94110 USA

[3] UNIV CALIF SAN FRANCISCO, SAN FRANCISCO GEN HOSP, DEPT RADIOL, SAN FRANCISCO, CA 94110 USA

[4] DEPT VET AFFAIRS MED CTR, MAGNET RESONANCE UNIT, SAN FRANCISCO, CA 94121 USA

来源：

BIOPHYSICAL JOURNAL | 1993年 / 65卷 / 05期

关键词：

D O I：

10.1016/S0006-3495(93)81274-8

中图分类号：

Q6 [生物物理学];

学科分类号：

071011 ;

摘要：

Fluorometric determination of cytosolic calcium, [Ca2+]c, using Indo-1 in intact tissue, is limited by problems in obtaining calibration parameters for Indo-1 in vivo. Therefore, the goal of this study was to calibrate Indo-1 using in vitro constants, obtained from protein-containing reference solutions designed to produce similar Indo-1 spectral properties to those in vivo. Due to wavelength-dependent tissue light absorbance, the in vitro constants had to be absorbance-corrected using a novel method. The correction factor was calculated from the relationship between the Indo-1 fluorescence intensities at the two detection wavelengths. A mixture of proteins at approximately 28 mg/ml had a similar Indo-1 isosbestic wavelength (430 nm) to that found in vivo (427 nm), and a similar fluorescence ratio maximum with saturating Ca2+ to that found in vivo (after absorbance correction). Using calibration constants from this protein mixture, calculated [Ca2+]c in a Langendorf perfused rat heart was 187 nM during diastole, and 464 nM in systole. This new calibration method circumvented the considerable experimental problems of previous methods which required measurements with the cytosol fully depleted and fully saturated with Ca2+.

引用

页码：1973 / 1982

页数：10

共 22 条

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