来自营养不良(mdx)小鼠和正常小鼠骨骼肌的肌管中的钙离子(Ca2+)水平。
Ca2+ levels in myotubes grown from the skeletal muscle of dystrophic (mdx) and normal mice.
作者信息
Bakker A J, Head S I, Williams D A, Stephenson D G
机构信息
Department of Zoology, La Trobe University, Bundoora, Victoria, Australia.
出版信息
J Physiol. 1993 Jan;460:1-13. doi: 10.1113/jphysiol.1993.sp019455.
Abstract
- Myotubes were grown in culture from normal (C57BL/ScSn) and mdx mice and the cytosolic [Ca2+] was monitored through development (5-21 days in culture) using fura-2 loaded via ionophoresis. Simultaneous measurements of the membrane potential and cytosolic [Ca2+] were made in normal and mdx myotubes before, during and after stimulation by action potentials elicited following anode break excitation. All experiments were undertaken at 22 degrees C. All data are expressed as means +/- S.E.M. 2. A new method was developed which enabled accurate determination of the fluorescence characteristics of fura-2 in murine skeletal muscle fibres. In the under in vitro conditions by 14.60 +/- 0.05, 9.40 +/- 0.15 and 6.90 +/- 0.43% respectively. 3. The resting cytosolic [Ca2+] in the mdx myotubes was consistently higher than in the normal myotubes throughout the developmental period measured. Overall, the resting cytosolic [Ca2+] in mdx myotubes (134 +/- 9 nM, n = 22) was twofold higher than in normal myotubes (66 +/- 6 nM, n = 26). After stimulation (one to three action potentials) the cytosolic [Ca2+] of both mdx and normal myotubes remained elevated. The mdx myotubes (236 +/- 55 nM, n = 5) again had approximately double the cytosolic [Ca2+] of normal myotubes (109 +/- 19 nM, n = 9). 4. The time course and amplitude of the Ca2+ responses measured in the mdx and normal myotubes after action potential stimulation were variable. Two categories of Ca2+ response were observed in mdx and normal myotubes, the first consisted of a small, slow rise in [Ca2+] that remained elevated and the second consisted of a rapid (time to peak 7.4 +/- 1.5 ms) (n = 8) rise in [Ca2+] with amplitudes in the range 61-773 nM and a [Ca2+] decay rate constant of 4.35 +/- 1.57 s-1 (n = 8) (range 0.96-15 s-1). 5. In conclusion, the elevated cytosolic [Ca2+] reported here through development of cultured mdx myotubes suggests that this genetic disorder results in a defect which compromises the ability of the myotubes to strictly regulate cytosolic [Ca2+]. The results are consistent with the presence of functionally abnormal Ca2+ channels recently reported in mdx myotubes.
摘要
- 从正常(C57BL/ScSn)小鼠和mdx小鼠的肌肉组织中培养出肌管,并使用通过离子载体加载的fura-2监测其在发育过程中(培养5 - 21天)的胞质[Ca2+]。在阳极断路激发引发动作电位刺激之前、期间和之后,对正常和mdx肌管的膜电位和胞质[Ca2+]进行同步测量。所有实验均在22摄氏度下进行。所有数据均表示为平均值±标准误。2. 开发了一种新方法,能够准确测定fura-2在小鼠骨骼肌纤维中的荧光特性。在体外条件下,分别为14.60±0.05、9.40±0.15和6.90±0.43%。3. 在整个测量的发育期间,mdx肌管中的静息胞质[Ca2+]始终高于正常肌管。总体而言,mdx肌管中的静息胞质[Ca2+](134±9 nM,n = 22)比正常肌管(66±6 nM,n = 26)高两倍。刺激后(一到三个动作电位),mdx和正常肌管的胞质[Ca2+]均保持升高。mdx肌管(236±55 nM,n = 5)的胞质[Ca2+]再次约为正常肌管(109±19 nM,n = 9)的两倍。4. 在动作电位刺激后,mdx和正常肌管中测量的Ca2+反应的时间进程和幅度是可变的。在mdx和正常肌管中观察到两类Ca2+反应,第一类由[Ca2+]的小而缓慢上升组成,且保持升高,第二类由[Ca2+]的快速(峰值时间7.4±1.5毫秒)(n = 8)上升组成,幅度在61 - 773 nM范围内,[Ca2+]衰减速率常数为4.35±1.57 s-1(n = 8)(范围0.96 - 15 s-1)。5. 总之,通过培养mdx肌管的发育过程所报告的胞质[Ca2+]升高表明,这种遗传性疾病导致了一种缺陷,损害了肌管严格调节胞质[Ca2+]的能力。这些结果与最近报道的mdx肌管中功能异常的Ca2+通道的存在一致。
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