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THE CALCIUM HOMEOSTASIS AND THE MEMBRANE-POTENTIAL OF CULTURED MUSCLE-CELLS FROM PATIENTS WITH MYOTONIC-DYSTROPHY
被引:33
|
作者
:
JACOBS, AEM
论文数:
0
引用数:
0
h-index:
0
机构:
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
JACOBS, AEM
BENDERS, AAGM
论文数:
0
引用数:
0
h-index:
0
机构:
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
BENDERS, AAGM
OOSTERHOF, A
论文数:
0
引用数:
0
h-index:
0
机构:
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
OOSTERHOF, A
VEERKAMP, JH
论文数:
0
引用数:
0
h-index:
0
机构:
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
VEERKAMP, JH
VANMIER, P
论文数:
0
引用数:
0
h-index:
0
机构:
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
VANMIER, P
WEVERS, RA
论文数:
0
引用数:
0
h-index:
0
机构:
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
WEVERS, RA
JOOSTEN, EMG
论文数:
0
引用数:
0
h-index:
0
机构:
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
JOOSTEN, EMG
机构
:
[1]
CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,POB 9101,6500 HB NIJMEGEN,NETHERLANDS
[2]
CATHOLIC UNIV NIJMEGEN,DEPT BIOPHYS,6500 HB NIJMEGEN,NETHERLANDS
[3]
CATHOLIC UNIV NIJMEGEN,DEPT NEUROSURG,6500 HB NIJMEGEN,NETHERLANDS
来源
:
BIOCHIMICA ET BIOPHYSICA ACTA
|
1990年
/ 1096卷
/ 01期
关键词
:
(Cultured human muscle cell);
Calcium homeostasis;
Membrane potential;
Voltage-operated calcium ion channel;
D O I
:
10.1016/0925-4439(90)90006-B
中图分类号
:
Q5 [生物化学];
Q7 [分子生物学];
学科分类号
:
071010 ;
081704 ;
摘要
:
Using the fluorescence indicator, quin2, we compared the cytoplasmic Ca2+ concentration ([Ca2+]i) of cultured myotubes obtained from control subjects and myotonic dystrophy (MyD) patients. In Ca2+-free buffer the [Ca2+]i of the cultured MyD muscle cells was not significantly different from that of the control cells. In the presence of 1 mM external Ca2+ the cultured MyD muscle cells showed a significantly higher [Ca2+]i, which was due to the influx of Ca2+ through voltage-operated nifedipine-sensitive Ca2+ channels. In the presence of external Ca2+, MyD myotubes did not respond to acetylcholine, whereas control myotubes showed a transient increase in [Ca2+]i after addition of acetylcholine. This increase was inhibited by the addition of nifedipine. The difference in Ca2+-homeostasis between cultured MyD muscle cells and control cells were not due to differences in the resting membrane potential or the inability of the MyD cells to depolarize as a response to acetylcholine. Therefore, culltured MyD muscle cells exhibit altered nifedipine-sensitive voltage-operated channels which are active under conditions in which they are normally present in the inactivie state, and which are unable to respond to depolarization cause by acetylcholine. © 1991.
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页码:14 / 19
页数:6
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