CHARACTERIZATION OF HYPOXIA-DEPENDENT PEROXIDE PRODUCTION IN CULTURES OF SACCHAROMYCES-CEREVISIAE USING FLOW-CYTOMETRY - A MODEL FOR ISCHEMIC TISSUE DESTRUCTION

被引：29

作者：

YURKOW, EJ ^{[1
]}

MCKENZIE, MA ^{[1
]}

机构：

[1] RUTGERS STATE UNIV,COLL PHARM,DEPT CHEM BIOL & PHARMACOGNOSY,PISCATAWAY,NJ 08854

来源：

CYTOMETRY | 1993年 / 14卷 / 03期

关键词：

YEAST; 2'; 7'-DICHLOROFLUORESCEIN DIACETATE; PROPIDIUM IODIDE; REPERFUSION INJURY; DUAL-PARAMETER ANALYSIS;

D O I：

10.1002/cyto.990140309

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

Peroxide production in cultures of Saccharomyces cerevisiae was measured using the H2O2-sensitive fluorescent probe 2',7'-dichlorofluorescein diacetate (DCFH-DA) and flow cytometry. Aeration of cultures of S. cerevisiae exposed to a period of hypoxia was found to induce elevated levels of peroxide that were 100-fold higher than the levels observed in cultures maintained under exclusively aerated or hypoxic conditions. Simultaneous viability analysis, using the fluorescent DNA-intercalating dye propidium iodide, indicated that the increase in peroxide generation preceded cell damage and death. Various agents were found to influence the effect of peroxides on cell viability. The addition of ethanol to hypoxic stationary cultures dramatically increased the rate of cell death without further increasing the amount of peroxide produced, while glucose inhibited peroxide production and decreased the rate of cell death. Surprisingly, elevated peroxide levels of hypoxic/reaerated cultures were maintained upon addition of KH2PPO4, although the cells remained viable for extended periods of time when compared to control and other test cultures. Similarities between our observations and those of other investigators using anoxic/reperfused organs suggest that hypoxic/reaerated yeast cultures may be a useful model system to study ischemia-dependent tissue destruction of mammals.

引用

页码：287 / 293

页数：7

共 30 条

[1]

ANDREOLI SP, 1986, J LAB CLIN MED, V108, P190

[2]

BABBS CF, 1988, ANN EMERG MED, V17, P1148

[3]

BASS DA, 1983, J IMMUNOL, V130, P1910

[4] INTRACELLULAR OXYGEN MEASUREMENTS OF MOUSE-LIVER CELLS USING QUANTITATIVE FLUORESCENCE VIDEO MICROSCOPY [J].

BENSON, DM ;

KNOPP, JA ;

LONGMUIR, IS .

BIOCHIMICA ET BIOPHYSICA ACTA, 1980, 591 (01) :187-197

[5] XANTHINE-OXIDASE AS A SOURCE OF FREE-RADICAL DAMAGE IN MYOCARDIAL ISCHEMIA [J].

CHAMBERS, DE ;

PARKS, DA ;

PATTERSON, G ;

ROY, R ;

MCCORD, JM ;

YOSHIDA, S ;

PARMLEY, LF ;

DOWNEY, JM .

JOURNAL OF MOLECULAR AND CELLULAR CARDIOLOGY, 1985, 17 (02) :145-152

[6] CONTINUOUS RECORDING OF BLOOD OXYGEN TENSIONS BY POLAROGRAPHY [J].

CLARK, LC ;

WOLF, R ;

GRANGER, D ;

TAYLOR, Z .

JOURNAL OF APPLIED PHYSIOLOGY, 1953, 6 (03) :189-193

[7]

CROME R, 1908, CARDIOVASC DRUG THER, V2, P295

[8] NEUTROPHIL ENDOTHELIAL-CELL INTERACTION - EVIDENCE FOR AND MECHANISMS OF THE SELF-PROTECTION OF BOVINE MICROVASCULAR ENDOTHELIAL-CELLS FROM HYDROGEN-PEROXIDE INDUCED OXIDATIVE STRESS [J].

DOBRINA, A ;

PATRIARCA, P .

JOURNAL OF CLINICAL INVESTIGATION, 1986, 78 (02) :462-471

[9] FERROUS-SALT-PROMOTED DAMAGE TO DEOXYRIBOSE AND BENZOATE - THE INCREASED EFFECTIVENESS OF HYDROXYL-RADICAL SCAVANGERS IN THE PRESENCE OF EDTA [J].

GUTTERIDGE, JMC .

BIOCHEMICAL JOURNAL, 1987, 243 (03) :709-714

[10]

Haugland RP, 1989, MOL PROBES HDB FLUOR

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