SULFUR MUSTARD-INDUCED INCREASE IN INTRACELLULAR FREE CALCIUM LEVEL AND ARACHIDONIC-ACID RELEASE FROM CELL-MEMBRANE

被引：51

作者：

RAY, R ^{[1
]}

LEGERE, RH ^{[1
]}

MAJERUS, BJ ^{[1
]}

PETRALI, JP ^{[1
]}

机构：

[1] USA,MED RES INST CHEM DEF,COMPARAT PATHOL BRANCH,ABERDEEN PROVING GROUND,MD 21010

来源：

TOXICOLOGY AND APPLIED PHARMACOLOGY | 1995年 / 131卷 / 01期

关键词：

D O I：

10.1006/taap.1995.1045

中图分类号：

R9 [药学];

学科分类号：

1007 ;

摘要：

The mechanism of action of the alkylating agent bis-(2-chloroethyl)sulfide (sulfur mustard, SM) was studied using the in vitro mouse neuroblastoma-rat glioma hybrid NG108-15 clonal cell line model. Following 0.3 mM SM exposure, cell viability remained high (>80% of untreated control) up to 9 hr and then declined steadily to about 40% of control after 20-24 hr. During the early period of SM exposure, when there was no significant cell viability loss, the following effects were observed. The cellular glutathione level decreased 20% after 1 hr and 34% after 6 hr. Between 2 and 6 hr, there was a time-dependent increase (about 10 to 30%) in intracellular free calcium (Ca2+), which was localized to the limiting membrane of swollen endoplasmic reticula and mitochondria, to euchromatin areas of the nucleus, and to areas of the cytosol and plasma membrane. Moreover, there was also a time-dependent increase in the release of isotopically labeled arachidonic acid ([H-3]AA) from cellular membranes. Increase in [H-3]AA release was 28% at 3 hr and about 60-80% between 6 and 9 hr. This increase in [H-3]AA release was inhibited by quinacrine (20 mu M), which is a phospholipase (PLA(2)) inhibitor. At 16 hr after SM exposure, there was a large increase (about 200% of control) in [H-3]AA release, which was coincident with a 50% loss of cell viability. These results suggest a Ca2+-mediated toxic mechanism of SM via PLA(2) activation and arachidonate release. (C) 1995 Academic Press, Inc.

引用

页码：44 / 52

页数：9

共 37 条

[1] CRITICAL ROLE OF SULFHYDRYL GROUP(S) IN ATP-DEPENDENT CA-2+ SEQUESTRATION BY THE PLASMA-MEMBRANE FRACTION FROM RAT-LIVER [J].

BELLOMO, G ;

MIRABELLI, F ;

RICHELMI, P ;

ORRENIUS, S .

FEBS LETTERS, 1983, 163 (01) :136-139

[2]

BROOMFIEL CA, 1989, 1989 P MED DEF BIOSC, P433

[3]

CALABRESI P, 1990, PHARMACOL BASIS THER, P1209

[4]

COWAN FM, 1991, CELL BIOL TOXICOL, V7, P239

[5] PESTICIDE ACTION AND MEMBRANE FLUIDITY - ALLOSTERIC BEHAVIOR OF RAT ERYTHROCYTE MEMBRANE-BOUND ACETYLCHOLINESTERASE IN PRESENCE OF ORGANOPHOSPHOROUS COMPOUNDS [J].

DOMENECH, CE ;

MACHADODEDOMENECH, EE ;

BALEGNO, HF ;

MENDOZA, DD ;

FARIAS, RN .

FEBS LETTERS, 1977, 74 (02) :243-246

[6] SPIN-LABEL STUDIES OF DYNAMICS OF LIPID ALKYL CHAINS IN BIOLOGICAL-MEMBRANES - ROLE OF UNSATURATED SITES [J].

ELETR, S ;

KEITH, AD .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1972, 69 (06) :1353-&

[7] REGULATION OF ALLOSTERIC MEMBRANE-BOUND ENZYMES THROUGH CHANGES IN MEMBRANE LIPID-COMPOSITION [J].

FARIAS, RN ;

BLOJ, B ;

MORERO, RD ;

SINERIZ, F ;

TRUCCO, RE .

BIOCHIMICA ET BIOPHYSICA ACTA, 1975, 415 (02) :231-251

[8] NERVE GROWTH-FACTOR STIMULATION OF ARACHIDONIC-ACID RELEASE FROM PC12 CELLS - INDEPENDENCE FROM PHOSPHOINOSITIDE TURNOVER [J].

FINK, DW ;

GUROFF, G .

JOURNAL OF NEUROCHEMISTRY, 1990, 55 (05) :1716-1726

[9]

FRYE RA, 1983, MOL PHARMACOL, V23, P547

[10] DETERMINATION OF GLUTATHIONE AND GLUTATHIONE DISULFIDE USING GLUTATHIONE-REDUCTASE AND 2-VINYLPYRIDINE [J].

GRIFFITH, OW .

ANALYTICAL BIOCHEMISTRY, 1980, 106 (01) :207-212

← 1 2 3 4 →